WO2009078977A2 - Compositions and methods to concurrently treat or prevent multiple diseases with cupredoxins - Google Patents

Compositions and methods to concurrently treat or prevent multiple diseases with cupredoxins Download PDF

Info

Publication number
WO2009078977A2
WO2009078977A2 PCT/US2008/013721 US2008013721W WO2009078977A2 WO 2009078977 A2 WO2009078977 A2 WO 2009078977A2 US 2008013721 W US2008013721 W US 2008013721W WO 2009078977 A2 WO2009078977 A2 WO 2009078977A2
Authority
WO
WIPO (PCT)
Prior art keywords
ala
giy
asp
vai
cancer
Prior art date
Application number
PCT/US2008/013721
Other languages
French (fr)
Other versions
WO2009078977A9 (en
WO2009078977A3 (en
Inventor
Tapas Das Gupta
Ananda Chakrabarty
Original Assignee
Cdg Therapeutics Inc
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Cdg Therapeutics Inc filed Critical Cdg Therapeutics Inc
Publication of WO2009078977A2 publication Critical patent/WO2009078977A2/en
Publication of WO2009078977A3 publication Critical patent/WO2009078977A3/en
Publication of WO2009078977A9 publication Critical patent/WO2009078977A9/en

Links

Classifications

    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/795Porphyrin- or corrin-ring-containing peptides
    • C07K14/80Cytochromes
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/195Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • YGENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
    • Y02TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
    • Y02ATECHNOLOGIES FOR ADAPTATION TO CLIMATE CHANGE
    • Y02A50/00TECHNOLOGIES FOR ADAPTATION TO CLIMATE CHANGE in human health protection, e.g. against extreme weather
    • Y02A50/30Against vector-borne diseases, e.g. mosquito-borne, fly-borne, tick-borne or waterborne diseases whose impact is exacerbated by climate change

Definitions

  • the present invention relates to compositions comprising variants, derivatives and structural equivalents of cupredoxins that concurrently treat and/or prevent two or more conditions in a patient.
  • HIV infection Human immunodeficiency virus (HIV) infection, which results in AIDS, is a relatively new infection in the human population, and has quickly risen to the foremost health problem in the world.
  • HIV/ AIDS is now the leading cause of death in sub-Saharan Africa, and is the fourth biggest killer worldwide.
  • the Centers for Disease Control (CDC) estimates that nearly 800,000 people are living with AIDS in the US, and 40,000 new cases diagnosed each year. While better treatment methods are now known to prolong the life of patients with HIV infection, there is still no cure.
  • Modern anti-HIV drugs target several different stages of the HIV life cycle, and several of the enzymes that HIV requires to replicate and survive.
  • nucleoside reverse transcriptase inhibitors such as AZT, ddl, ddC, d4T, 3TC, and abacavir
  • nucleotide reverse transcriptase inhibitors such as tenofovir
  • non-nucleoside reverse transcriptase inhibitors such as nevirapine, efavirenz and delavirdine
  • protease inhibitors such as saquinavir, ritonavir, indinavir, nelfinavir, amprinavir, lopinavir and atazanavir
  • fusion inhibitors such as enfuvirtide.
  • none of these antiviral drugs is effective to prevent the progression of chronic infection or treat acute AIDS.
  • the high mutation rate of the HIV virus and associated emergence of HIV strains resistant to drugs may be one large factor that results in the inability to effectively treat HIV infection.
  • MSPl Merozoite Surface Protein 1
  • the merozoite MSPl protein undergoes proteolytic cleavage, producing a C-terminal cleavage product MSP 1-42, which subsequently undergoes a second cleavage, producing an 11 kDa peptide MSP1-19, which remains attached to the parasite surface as it enters the erythrocyte.
  • the formation of the cleavage product MSP 1-19 is very important for successful invasion by the parasite since inhibition of its proteolytic formation or its neutralization by monoclonal antibodies prevents entry of the parasite to the erythrocytes (Blackman et al., J. Exptl., Med.
  • MSPl-19 peptide is one of the most important malaria vaccine candidates available. MSPl-19-specific antibodies from malaria-resistant human sera react with the antigen and include a major erythrocyte-invasion inhibitory component (Holder & Riley, Parasitol. Today, 12: 173-174 (1996); O'Donnell et al, J. Expt. Med. 193: 1403-1412 (2001)). Serum from donors in malaria-endemic regions usually demonstrates strong antibody reactivity towards Pf MSP1-19. (Nwuba et al, Infect. Immun. 70: 5328-5331 (2002))
  • the monoclonal antibody (mAb) Gl 7.12 was raised against recombinant Pf MSPl-19 and recognizes its epitope on the parasite surface, demonstrating that this region of the antigen is accessible on the native MSPl polypeptide complex (Pizarro et al, J. MoI. Biol. 328:1091-1103 (2003)). Interestingly, erythrocyte invasion experiments in vitro showed that infection is not inhibited in the presence of G 17.12, even at 200 ⁇ g/ml concentration and Gl 7.12 does not inhibit in vitro secondary processing of MSPl. Id.
  • Cerebral malaria a rare but fatal infection restricted to P. falciparum invasion of brain capillaries because of the sequestration of parasitized erythrocytes, is often untreatable because most drugs cannot cross the blood-brain barrier to reach the brain capillaries.
  • Adhesion of P. falciparum - infected erythrocytes to brain capillaries is mediated by the interaction of parasite ligands Pf Emp-1 family of proteins expressed on the surface of infected erythrocytes with ICAM-I and CD36 expressed on the surface of capillary endothelium cells in cerebral vessels.
  • chloroquine that targets the heme detoxification pathway
  • Chloroquine antagonizes heme polymerization mediated by parasite-induced HRPs (histidine-rich proteins), as heme monomers are highly toxic for malaria parasites.
  • HRPs histidine-rich proteins
  • the polymerization of heme allows detoxification, which is reversed by chloroquine.
  • Another drug, artemisinin is effective against chloroquine-resistant P. falciparum in cerebral malaria. Artemisinin forms adducts with globin-bound heme in hemoglobin, which binds HRPs to prevent heme polymerization.
  • a cancer is a malignant tumor of potentially unlimited growth. It is primarily the pathogenic replication (a loss of normal regulatory control) of various types of cells found in the human body. Initial treatment of the disease is often surgery, radiation treatment or the combination of these treatments, but locally recurrent and metastatic disease is frequent. Chemotherapeutic treatments for some cancers are available but these seldom induce long term regression. Hence, they are often not curative. Commonly, tumors and their metastases become refractory to chemotherapy, in an event known as the development of multidrug resistance. In many cases, tumors are inherently resistant to some classes of chemotherapeutic agents. In addition, such treatments threaten noncancerous cells, are stressful to the human body, and produce many side effects.
  • Angiogenesis is the formation of new blood vessels from preexisting endothelial vasculature. Folkman, et al., J. Exp. Med. 133:275-288, (1971). Most tumors require angiogenesis to sustain growth beyond a critical volume of 1 -2 mm, when the supply of nutrients and metabolites becomes insufficient due to the limits of diffusional exchange. Folkman, J. Nat. Cancer Inst. 82:4-6 (1990). Tumors deprived of angiogenesis remain dormant indefinitely, only to rapidly grow when a blood supply is acquired. Brem et al, Cancer Res.36:2807-2812 (1976). The degree of angiogenesis often increases with tumor progression. Dome et al., J. Pathol.
  • angiogenesis is an integral process in the growth and spread of tumors, it is an important focus of cancer therapy.
  • Anti-angiogenesis therapy is effective not only for solid tumors, but also hematopoietic tumors, leukemia and myeloma, Bellamy et al., Cancer Res. 59:728-733 (1999); Rajkumar et al, Leukemia.
  • Endothelial cells are thought to be better targets for therapy than tumor cells because they have a longer generation time and more genetic stability that tumor cells. Endothelial cells are therefore less likely to "escape" therapy by developing drug resistance to the therapy administered. Boehn-Vaiswanathan, Curr. Opin. Oncol. 12:89-94 ( 2000). Other conditions suffered by mammals are also related to inappropriate angiogenesis. Wet macular degeneration occurs when blood capillaries inappropriately grow into the retina. Inappropriate angiogenesis has also been implicated as a fundamental characteristic of diabetic retinopathy, psoriasis and rheumatoid arthritis, among other diseases. Bussolino et al, Trends Biochem. Sci. 22:251-256 (1997); Folkman, Nat. Med. 1 : 27-31 (1995).
  • Numerous diseases may occur concurrently in a patient, or one disease may cause or increase the probability of causing another disease in a patient.
  • an HIV infected patient is associated with an increased risk of acquiring large cell lymphoma or Kaposi's sarcoma.
  • the Merck Manual of Diagnosis and Therapy, (Beers et al., 18 th edition, Merck Research Laboratories, 2006).
  • a female patient that acquires human papilloma- virus has an increased risk of acquiring cervical carcinoma. Id.
  • Environmental factors may include a patient's lifestyle, eating habits and/or geographic location.
  • co-infections with HIV and malaria are very common in many areas of the world, and in particular sub-Saharan Africa
  • Genetic predisposition may also play a factor in a patient acquiring two diseases concurrently. For example, it is known that when a person carries a particular cystic fibrosis transmembrane regulator (CFTR) mutation, that person has a higher risk for cystic fibrosis and pancreatic cancer. Weiss et al, Gut; 54: 1456-1460 (2005).
  • CTR cystic fibrosis transmembrane regulator
  • the present invention relates to compositions comprising peptides that may be cupredoxin or cytochrome or variants, derivatives, truncations and structural equivalents of cupredoxin or cytochrome that treat and/or prevent two or more conditions in a mammalian cell.
  • the present invention further relates to compositions that may comprise cupredoxin or cytochrome, and/or variants, derivatives, truncations, or structural equivalents of cupredoxin or cytochrome, that retain the ability to concurrently treat and/or prevent two or more conditions such as cancer, inappropriate angiogenesis, HIV and malaria in a patient.
  • compositions may be isolated peptides or pharmaceutical compositions, among others.
  • the cupredoxin may be azurin, pseudoazurin, plastocyanin, rusticyanin, Laz, auracyanin, stellacyanin and cucumber basic protein, and specifically may be azurin.
  • the cupredoxin may be from an organism such as Pseudomonas aeruginosa, Alcaligenes faecalis, Ulva pertussis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp.
  • Neisseria meningitidis Neisseria gonorrhea
  • Pseudomonas fluorescens Bordetella pertussis
  • Pseudomonas syringae Pseudomonas chloror aphis
  • Xylella fastidiosa Vibrio parahaemolyticus, and specifically may be Pseudomonas aeruginosa.
  • the isolated peptide may inhibit parasitemia by malaria in P. falciparum-infected human red blood cells.
  • the isolated peptide may be fused to a H.8 region of Laz.
  • the isolated peptide may be a structural equivalent of monoclonal antibody Gl 7.12.
  • the isolated peptide may be a cytochrome selected from one or more of the group consisting of cytochrome c, cytochrome f and cytochrome C 55 ⁇ .
  • the isolated peptide of cytochrome c may be from an organism selected from the group consisting of human and Pseudomonas aeruginosa.
  • the isolated peptide of cytochrome f may be from cyanobacteria.
  • the isolated peptide may be part of SEQ ID NOS: 1, 5-12, 18 and 23, a mutant of SEQ ID NOS: 1, 5-12, 18 and 23, or have at least 90% amino acid sequence identity to SEQ ID NOS: 1, 5-12, 18 and 23.
  • the isolated peptide may be a truncation of a peptide selected from one or more of the group consisting of SEQ ID NOS: 1, 5-12, 18 and 23. In another embodiment, the isolated peptide may be a truncation of a cupredoxin.
  • the isolated peptide may be any suitable length, including from 10 to 100 residues, 18 to 100 residues, or 18 to 28 residues.
  • the isolated peptide may comprise or consist of a sequence and/or the equivalent residues of a cupredoxin as a region selected from the group consisting of Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30),
  • Pseudomonas aeruginosa azurin residues 36-88 SEQ ID NO: 50
  • Pseudomonas aeruginosa azurin residues 36-128 SEQ ID NO: 31
  • Pseudomonas aeruginosa azurin residues 88-113 SEQ ID NO: 49
  • Pseudomonas aeruginosa azurin residues 36-89 SEQ ID NO: 32
  • Pseudomonas aeruginosa azurin residues 96-113 SEQ ID NO: 48
  • Vibrio parahaemolyticus azurin residues 52-78 SEQ ID NO: 27
  • Pseudomonas syringae azurin residues 51-77 SEQ ID NO: 25
  • Bordetella bronchiseptica azurin residues 51-77 SEQ ID NO: 28
  • the isolated peptide may also be a truncation of any of those sequences or a truncation of a larger sequence that comprises those sequences.
  • the isolated peptide may comprise equivalent residues of a region of the isolated peptide, wherein the peptide comprises the sequence and/or the equivalent residues of a cupredoxin as a region selected from the group consisting of Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID
  • the isolated peptide may also be a truncation of any of those sequences or a truncation of a larger sequence that comprises those sequences.
  • the compositions may comprise one or at least two cupredoxins, cytochromes or peptides in a pharmaceutical composition.
  • the pharmaceutical compositions may comprise the isolated peptides of the present invention.
  • the cupredoxin in a pharmaceutical composition may be from an organism such as Pseudomonas aeruginosa, Alcaligenes faecalis, Ulva pertussis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp., Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas fluorescens, Bordetella pertussis, Pseudomonas syringae, Pseudomonas chlororaphis, Xylella fastidiosa and Vibrio parahaemolyticus, and specifically may be Pseudomonas aeruginosa.
  • an organism such as Pseudomonas aeruginosa, Alcaligenes faecalis, Ulva pertussis, Achromobacter xylosoxidan, Bordetell
  • the cupredoxin in a pharmaceutical composition may be selected from one or more of the group consisting of SEQ ID NOS: 1, 5- 12, 18, 23, 25, 27-33 and 48-50. In another embodiment of the present invention, the cupredoxin in a pharmaceutical composition may comprise SEQ ID NO: 30.
  • the composition may be administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papilloma virus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomegalovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles
  • IC interstitial
  • the composition may comprise a therapeutic agent for the concurrent prevention and/or treatment of cancer selected from the group consisting of melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors, and prostate cancer.
  • the compositions may be administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
  • the compositions may comprise a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
  • compositions may comprise a therapeutic agent for the treatment of malaria, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
  • compositions may comprise a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
  • compositions may comprise a therapeutic agent for the treatment of HIV, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
  • compositions may comprise a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
  • compositions may comprise a therapeutic agent for the treatment of cancer, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
  • compositions may comprise a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or malaria.
  • the compositions may comprise a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or malaria.
  • the compositions may comprise another drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
  • the pharmaceutical composition may be administered by intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection or oral.
  • the pharmaceutical composition may be co-administered with at least one other drug.
  • the pharmaceutical composition may be co-administered with one other drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
  • the pharmaceutical composition may be administered at about the same time with another drug.
  • the other drug may be an antimalarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
  • the methods may include administering to a patient the composition comprising one or at least two cupredoxins, cytochromes or peptides in a pharmaceutical composition.
  • the patient is human.
  • the methods may include administering the compositions to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papilloma virus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, me
  • IC interstitial
  • the methods may include administering the compositions to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of malaria, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of HIV, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of cancer, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
  • the methods may utilize a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or malaria.
  • the methods may utilize a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or malaria.
  • the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop cancer than the general population.
  • the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop HIV than the general population.
  • the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop malaria than the general population.
  • the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop inappropriate angiogenesis than the general population.
  • the methods may utilize compositions wherein the composition is administered to a patient that has a higher risk than the general population of acquiring one or more of the group consisting of HIV, cancer, angiogenesis and malaria.
  • the methods may utilize compositions wherein the composition is administered to a patient that has at least one high risk feature.
  • the methods may utilize a pharmaceutical composition administered by intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection or oral, and specifically may be administered by intravenous injection.
  • the methods may utilize a pharmaceutical composition co-administered with at least one other drug.
  • the other drug may be an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
  • the methods may utilize a pharmaceutical composition administered at about the same time with at least one other drug.
  • the methods may utilize a pharmaceutical composition administered at about the same time with at least one other drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
  • the composition may be a kit comprising the pharmaceutical composition of the invention.
  • the kit may be designed for intravenous administration.
  • the composition be an isolated peptide that can bind a protein selected from the group consisting of CD4, gpl20, ICAM3, DC-SIGN, PFMSP 1-19 and PFMSP 1-42.
  • SEQ ID NO: 1 Amino acid sequence of azurin from Pseudomonas aeruginosa(A ⁇ a GIu Cys Ser VaI Asp He GIn GIy Asn Asp GIn Met GIn Phe Asn Thr Asn Ala He Thr VaI Asp Lys Ser Cys Lys GIn Phe Thr VaI Asn Leu Ser His Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu He GIy Ser GIy GIu Lys Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr Phe Pro GIy His
  • SEQ ID NO: 3 Amino acid sequence of rusticyanin from Thiob ⁇ cillus ferrooxid ⁇ ns (GIy Thr Leu Asp Thr Thr Trp Lys GIu Ala Thr Leu Pro GIn VaI Lys Ala Met Leu GIu Lys Asp Thr GIy Lys VaI Ser GIy Asp Thr VaI Thr Tyr Ser GIy Lys Thr VaI His VaI VaI Ala Ala Ala VaI Leu Pro GIy Phe Pro Phe Pro Ser Phe GIu VaI His Asp Lys Lys Asn Pro Thr Leu GIu He Pro Ala GIy Ala Thr VaI Asp VaI Thr Phe He Asn Thr Asn Lys GIy Phe GIy His Ser Phe Asp He Thr Lys Lys GIy Pro Pro Tyr Ala VaI Met Pro VaI He Asp Pro He VaI Ala GIy Thr GIy Phe Ser Pro VaI Pro Lys Asp GIy Ly
  • SEQ ID NO: 8 Amino acid sequence of azurin from Methylomonas sp. J (Ala Ser Cys GIu Thr Thr VaI Thr Ser GIy Asp Thr Met Thr Tyr Ser Thr Arg Ser He Ser VaI Pro Ala Ser Cys Ala GIu Phe Thr VaI Asn Phe GIu His Lys GIy His Met Pro Lys Thr GIy Met GIy His Asn Trp VaI Leu Ala Lys Ser Ala Asp VaI GIy Asp VaI Ala Lys GIu GIy Ala His Ala GIy Ala Asp Asn Asn Phe VaI Thr Pro GIy Asp Lys Arg VaI He Ala Phe Thr Pro He He He GIy GIy GIy GIu Lys Thr Ser VaI Lys Phe Lys VaI Ser Ala Leu Ser Lys Asp GIu Ala Tyr Thr Tyr Phe Cys Ser Tyr Pro GIy His P
  • SEQ ID NO: 9 Amino acid sequence of azurin from Neisseria meningitides Z2491 (Cys Ser GIn GIu Pro Ala Ala Pro Ala Ala GIu Ala Thr Pro Ala Ala GIu Ala Pro Ala Ser GIu Ala Pro Ala Ala GIu Ala Ala Pro Ala Asp Ala Ala GIu Ala Pro Ala Ala GIy Asn Cys Ala Ala Thr VaI GIu Ser Asn Asp Asn Met GIn Phe Asn Thr Lys Asp He GIn VaI Ser Lys Ala Cys Lys GIu Phe Thr He Thr Leu Lys His Thr GIy Thr GIn Pro Lys Thr Ser Met GIy His Asn He VaI He GIy Lys Thr GIu Asp Met Asp GIy He Phe Lys Asp GIy VaI GIy Ala Ala Asp Tyr VaI Lys Pro Asp Asp Ala
  • SEQ ID NO: 10 Amino acid sequence of azurin from Pseudomonas fluorescen (Ala GIu Cys Lys Thr Thr He Asp Ser Thr Asp GIn Met Ser Phe Asn Thr Lys Ala He GIu He Asp Lys Ala Cys Lys Thr Phe Thr VaI GIu Leu Thr His Ser GIy Ser Leu Pro Lys Asn VaI Met GIy His Asn Leu VaI He Ser Lys GIn Ala Asp Met GIn Pro He Ala Thr Asp GIy Leu Ser Ala GIy He Asp Lys Asn Tyr Leu Lys GIu GIy Asp Thr Arg VaI He Ala His Thr Lys VaI He GIy Ala GIy GIu Lys Asp Ser Leu Thr He Asp VaI Ser GIy Ala GIy GIu Lys Asp Ser Leu Thr He Asp VaI Ser Lys Leu Asn Ala Ala
  • SEQ ID NO: 13 Amino acid sequence of stellacyanin from Cucumis sativus (Met GIn Ser Thr VaI His He VaI GIy Asp Asn Thr GIy Trp Ser VaI Pro Ser Ser Pro Asn Phe Tyr Ser GIn Trp Ala Ala GIy Lys Thr Phe Arg VaI GIy Asp Ser Leu GIn Phe Asn Phe Pro Ala Asn Ala His Asn VaI His GIu Met GIu Thr Lys GIn Ser Phe Asp Ala Cys Asn Phe VaI Asn Ser Asp Asn Asp VaI GIu Arg Thr Ser Pro VaI He GIu Arg Leu Asp GIu Leu GIy Met His Tyr Phe VaI Cys Thr VaI GIy Thr His Cys Ser Asn GIy GIn Lys Leu Ser He Asn VaI VaI Ala Ala Asn Ala Thr VaI Ser Met Pro Pro Pro Pro Ser Ser Ser Pro Pro Ser VaI Met Pro Pro
  • SEQ ID NO: 14 Amino acid sequence of auracyanin A from Chloroflexus aurantiacus (Met Lys He Thr Leu Arg Met Met VaI Leu Ala VaI Leu Thr Ala Met Ala Met VaI Leu Ala Ala Cys GIy GIy GIy GIy Ser Ser GIy GIy Ser Thr GIy GIy GIy Ser GIy Ser GIy Pro VaI Thr He GIu He GIy Ser Lys GIy GIu GIu Leu Ala Phe Asp Lys Thr GIu Leu Thr VaI Ser Ala GIy GIn Thr VaI Thr He Arg Phe Lys Asn Asn Ser Ala VaI GIn GIn His Asn Trp He Leu VaI Lys GIy GIy GIu Ala GIu Ala Ala Asn He Ala Asn Ala GIy Leu Ser Ala GIy Pro Ala Ala Ala Asn Tyr Leu Pro Ala
  • SEQ ID NO: 15 Amino acid sequence of auracyanin B from Chloroflexus aurantiacus (Ala Ala Asn Ala Pro GIy GIy Ser Asn VaI VaI Asn GIu Thr Pro Ala GIn Thr VaI GIu VaI Arg Ala Ala Pro Asp Ala Leu Ala Phe Ala GIn Thr Ser Leu Ser Leu Pro Ala Asn Thr VaI VaI Arg Leu Asp Phe VaI Asn GIn Asn Asn Leu GIy VaI GIn His Asn Trp VaI Leu VaI Asn GIy GIy Asp Asp VaI Ala Ala Ala VaI Asn Thr Ala Ala GIn Asn Asn Ala Asp Ala Leu Phe VaI Pro Pro Pro Asp Thr Pro Asn Ala Leu Ala Trp Thr Ala Met Leu Asn Ala GIy GIu Ser GIy Ser VaI Thr Phe Arg Thr Pro Ala Pro GI
  • SEQ ID NO: 16 Amino acid sequence of cucumber basic protein from Cucumis sativus (Ala VaI Tyr VaI VaI GIy GIy Ser GIy GIy Tip Thr Phe Asn Thr GIu Ser Tip Pro Lys GIy Lys Arg Phe Arg Ala GIy Asp He Leu Leu Phe Asn Tyr Asn Pro Ser Met His Asn VaI VaI VaI Asn GIn GIy GIy Phe Ser Thr Cys Asn Thr Pro Ala GIy Ala Lys VaI Tyr Thr Ser GIy Arg Asp GIn He Lys Leu Pro Lys GIy GIn Ser Tyr Phe He Cys Asn Phe Pro GIy His Cys GIn Ser GIy Met Lys He Ala VaI Asn Ala Leu).
  • SEQ ID NO: 19 Amino acid sequence of cytochrome c from Homo sapiens (GIy Asp VaI GIu Lys GIy Lys Lys He Phe He Met Lys Cys Ser GIn Cys His Thr VaI GIu Lys GIy GIy Lys His Lys Thr GIy Pro Asn Leu His GIy Leu Phe GIy Arg Lys Thr GIy GIn Ala Pro GIy Tyr Ser Tyr Thr Ala Ala Asn Lys Asn Lys GIy He He Trp GIy GIu Asp Thr Leu Met GIu Tyr Leu GIu Asn Pro Lys Lys Tyr He Pro GIy Thr Lys Met He Phe VaI GIy He Lys Lys Lys GIu GIu Arg Ala Asp Leu He Ala Tyr Leu Lys Lys Ala Thr Asn GIu). SEQ ID NO: 20. Amino acid sequence of cytochrome f from cyanobacteri
  • Phormidium laminosum (Met Asn Phe Lys VaI Cys Ser Phe Pro Ser Arg Arg GIn Ser He Ala Ala Phe VaI Arg VaI Leu Met VaI He Leu Leu Thr Leu GIy Ala Leu VaI Ser Ser Asp VaI Leu Leu Pro GIn Pro Ala Ala Ala Tyr Pro Phe Tip Ala GIn GIn Asn Tyr Ala Asn Pro Arg GIu Ala Thr GIy Arg He VaI Cys Ala Asn Cys His Leu Ala Ala Lys Pro Ala GIu He GIu VaI Pro GIn Ala VaI Leu Pro Asp Ser VaI Phe Lys Ala VaI VaI Lys He Pro Tyr Asp His Ser VaI GIn GIn VaI GIn Ala Asp GIy Ser Lys GIy Pro Leu Asn VaI GIy Ala VaI Leu Met Leu Pro GIu GIy Phe Thr He Ala Pro GIu Asp Arg He Pro
  • SEQ ID NO: 21 Amino acid sequence of cytochrome C 551 from Pseudomonas aeruginosa (GIu Asp Pro GIu VaI Leu Phe Lys Asn Lys GIy Cys VaI Ala Cys His Ala He Asp Thr Lys Met VaI GIy Pro Ala Tyr Lys Asp VaI Ala Ala Lys Phe Ala GIy GIn Ala GIy Ala GIu Ala GIu Leu Ala GIn Arg He Lys Asn GIy Ser GIn GIy VaI Trp GIy Pro He Pro Met Pro Pro Pro Asn Ala VaI Ser Asp Asp Asp GIu Ala GIn Thr Leu Ala Lys Trp VaI Leu Ser GIn Lys).
  • SEQ ID NO: 22 Amino acid sequence of the H.8 region of Laz from Neisseria gonorrhoeae F62 (Cys Ser GIn GIu Pro Ala Ala Pro Ala Ala GIu Ala Thr Pro Ala GIy GIu Ala Pro Ala Ser GIu Ala Pro Ala Ala GIu Ala Ala Pro Ala Asp Ala Ala GIu Ala Pro Ala Ala).
  • SEQ ID NO: 23 is the amino acid sequence of the azurin from Bordetella pertussis (Ala GIu Cys Ser VaI Asp He Ala GIy Thr Asp GIn Met GIn Phe Asp Lys Lys Ala He GIu VaI Ser Lys Ser Cys Lys GIn Phe Thx VaI Asn Leu Lys His Thr GIy Lys Leu Pro Arg Asn VaI Met GIy His Asn Trp VaI Leu Thr Lys Thr Ala Asp Met GIn Ala VaI GIu Lys Asp GIy He Ala Ala GIy Leu Asp Asn GIn Tyr Leu Lys Ala GIy Asp Thr Arg VaI Leu Ala His Thr Lys VaI Leu GIy GIy GIy GIu Ser Asp Ser VaI Thr Phe Asp VaI Ala Lys Leu Ala Ala GIy Asp Asp Tyr Thr Phe Phe Cys Ser Phe Pro
  • SEQ ID NO: 24 Amino acid sequence of amino acids 57- 89 of auracyanin B of Chloro ⁇ exus aurantiacus (His Asn Trp VaI Leu VaI Asn GIy GIy Asp Asp VaI Ala Ala Ala VaI Asn Thr Ala Ala GIn Asn Asn Ala Asp Ala Leu Phe VaI Pro Pro Pro Asp).
  • SEQ ID NO: 25 Amino acid sequence of amino acids 51-77 of P 'seudomonas syringae azurin (Ser Lys Lys Ala Asp Ala Ser Ala He Thr Thr Asp GIy Met Ser VaI GIy He Asp Lys Asp Tyr VaI Lys Pro Asp Asp).
  • SEQ ID NO: 26 Amino acid sequence of amino acids 89-115 of Neisseria meningitides Laz (He GIy Lys Thr GIu Asp Met Asp GIy He Phe Lys Asp GIy VaI GIy Ala Ala Asp Thr Asp Tyr VaI Lys Pro Asp Asp).
  • SEQ ID NO: 27 Amino acid sequence of amino acids 52-78 of Vibrio parahaemolyticus azurin (Ala Asp Thr Ala Asn He GIn Ala VaI GIy Thr Asp GIy Met Ser Ala GIy Ala Asp Asn Ser Tyr VaI Lys Pro Asp Asp).
  • SEQ HD NO: 28 Amino acid sequence of amino acids 51-77 of Bordetella bronchiseptica azurin (Thr Lys Thr Ala Asp Met GIn Ala VaI GIu Lys Asp GIy He Ala Ala GIy Leu Asp Asn GIn Tyr Leu Lys Ala GIy Asp).
  • SEQ ID NO: 29 is the amino acid sequence of the 50-77 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 30 is the amino acid sequence of the 50-67 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy).
  • SEQ ID NO: 31 is the amino acid sequence of the 36-128 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu He GIy Ser GIy GIu Lys Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr Phe Pro GIy His Ser Ala Leu Met Lys GIy Thr Leu Thr Leu Lys).
  • SEQ ID NO: 32 is the amino acid sequence of the 36-89 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu He GIy Ser).
  • SEQ ID NO: 33 is the amino acid sequence of the 36-77 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 34 is the forward primer to PCR amplify the Laz-encoding gene (laz) of
  • Neisseria gonorrhoeae ccggaattcc ggcagggatg ttgtaaatat ccg.
  • SEQ ID NO: 35 is the reverse primer to PCR amplify the Laz-encoding gene (laz) of Neisseria gonorrhoeae (ggggtaccgc cgtggcaggc atacagcatt tcaatcgg).
  • SEQ ID NO: 36 is the forward primer to PCR amplify a 3.1 kb fragment of pUC18- laz (ggcagcaggg gcttcggcag catctgc).
  • SEQ ID NO: 37 is the reverse primer to PCR amplify a 3.1 kb fragment of pucl8-laz (ctgcaggtcg actctagagg atcccg).
  • SEQ ID NO: 38 is the forward primer to PCR amplify a 0.4 kb fragment of pUC19- paz (gccgagtgct cggtggacat ccagg).
  • SEQ ID NO: 39 is the reverse primer to PCR amplify a 0.4 kb fragment of pUCl 9- paz (tactcgagtc acttcagggt cagggtg).
  • SEQ ID NO: 40 is the forward primer for pGST-azu 36-128 (ggcaacctgc cgaagaacgt catgggc).
  • SEQ ID NO: 41 is the reverse primer for pGST-azu 36-128 (cggaattcgc atcacttcag ggtcaggg).
  • SEQ ID NO: 42 is the forward primer for pGST-azu 36-89 (ccaagctgat cggctcgtga gagaaggact cggtgacc).
  • SEQ ID NO: 43 is the reverse primer for pGST-azu 36-89 (ggtcaccgag tccttctctc acgagccgat cagcttgg).
  • SEQ ID NO: 44 is the forward primer for pGST-azu 88-113 (cggggatccc cggctcgggc gagaaggac).
  • SEQ ID NO: 45 is the reverse primer for pGST-azu 88-113 (cgggaattct ccacttcagg gtcagggtg).
  • SEQ ID NO: 46 is an oligonucleotide for site directed mutagenesis for the preparation of pGST-azu 88-113 (gttcttctgc acctagccgg gccactccg).
  • SEQ ID NO: 47 is an oligonucleotide for site directed mutagenesis for the preparation of pGST-azu 88-1 13 (cggagtggcc cggctaggtg cagaagaac).
  • SEQ ID NO: 48 is the amino acid sequence of the 96-113 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr).
  • SEQ ID NO: 49 is the amino acid sequence of the 88-113 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (GIy Ser GIy GIu Lys Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr).
  • SEQ ID NO: 50 is the amino acid sequence of the 36-88 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu Ue GIy).
  • SEQ ID NO: 51 is the amino acid sequence of a variant of the azurin truncation p28 (Leu Ser Thr Ala Ala Asp Met GIn Ala VaI VaI Thr Asp Thr Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 52 is the amino acid sequence of a variant of the azurin truncation p28 (Leu Ser Thr Ala Ala Asp Leu GIn GIy VaI VaI Thr Asp GIy Leu Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 53 is the amino acid sequence of a variant of the azurin truncation p28 (Leu Ser Thr Ala Ala Asp VaI GIn GIy VaI VaI Thr Asp GIy VaI Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 54 is the amino acid sequence of a modified cupredoxin derived peptide
  • SEQ ID NO: 55 is the amino acid sequence of a modified cupredoxin derived peptide (Acetylation- Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp-amidation).
  • SEQ ID NO: 56 is the amino acid sequence of a hexapeptide (VaI Ser Pro Pro Ala Arg).
  • SEQ ID NO: 57 is the amino acid sequence of a hexapeptide (Tyr Thr Pro Pro Ala Leu).
  • SEQ ID NO: 58 is the amino acid sequence of a hexapeptide (Phe Ser Phe Phe Ala
  • SEQ ID NO: 59 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Thr Pro GIy Cys).
  • SEQ ID NO: 60 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Cys GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 61 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Cys Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 62 is the amino acid sequence of a modified cupredoxin-derived peptide
  • SEQ ID NO: 63 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Thr Met GIn Cys VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 64 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Thr Met GIn GIy Cys VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 65 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asn Thr GIn GIy Cys VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 66 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asn Thr GIn GIy VaI Cys Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 67 is the amino acid sequence of a modified cupredoxin-derived peptide
  • SEQ ID NO: 68 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Thr Ala VaI VaI Cys Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 69 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn Thr VaI VaI Cys Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 70 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn Thr VaI VaI Thr Cys GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 71 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn Ala Thr VaI Thr Cys GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 72 is the amino acid sequence of a modified cupredoxin-derived peptide
  • SEQ ID NO: 73 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI Thr Ala Asp Cys Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 74 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI Thr Ala Asp GIy Cys Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 75 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asn GIy Cys Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 76 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Ala Thr Met GIy Ser GIy Leu Cys Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 77 is the amino acid sequence of a modified cupredoxin-derived peptide
  • SEQ ID NO: 78 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 79 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Trp GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 80 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Trp Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 81 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 82 is the amino acid sequence of a modified cupredoxin-derived peptide
  • SEQ ID NO: 83 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met GIn GIy VaI VaI Trp Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 84 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met GIn GIy VaI VaI Thr Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 85 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Trp GIy VaI VaI Trp Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 86 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Trp GIy VaI VaI Thr Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 87 is the amino acid sequence of a modified cupredoxin-derived peptide
  • SEQ ID NO: 88 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met Trp GIy VaI VaI Trp Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • SEQ ID NO: 89 is the amino acid sequence of a modified cupredoxin-derived peptide (X 1 Ser X 2 Ala Ala Asp X 3 X 4 X 5 VaI VaI X 6 Asp X 7 X 8 Ala Ser GIy Leu Asp Lys Asp Tyr Leu Ly s Pro Asp X 9 ).
  • SEQ ID NO: 90 is the amino acid sequence of a modified cupredoxin-derived peptide (Xi Asp Pro Lys Leu Tyr Asp Lys Asp Leu GIy Ser Ala X 2 X 3 Asp X 4 VaI VaI X 5 X 6 X 7 Asp Ala Ala X 8 Ser X 9 ).
  • SEQ ID NO: 91 is the amino acid sequence of pi 8b, the 60-77 amino acid fragment of wt-azurin from Pseudomonas aeruginosa (VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp)
  • SEQ ID NO: 92 is the amino acid sequence of the 10 C-terminal amino acids of p28
  • SEQ ID NO: 93 is the amino acid sequence of the 12 C-terminal amino acids of p28 (Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
  • Figure 1 depicts confocal microscopy images of malignant and normal cells incubated with p28 labeled with Alexafluor ® 568 and the cells are then stained with DAPI. The indicated cell lines were incubated in the absence (negative control) or presence (p28) of 20 ⁇ M Alexafluor ® 568 labeled p28 for 2h at 37°C. The images are indicative of amount of cellular entry observed.
  • Figure IA depicts the Alexafluor 568 fluorescence and control fluorescence of human melanoma, pancreatic, breast (BCA-I), breast (MCF-7), glioblastoma, astrocytoma, lung and prostrate cancer cells.
  • Figure IB depicts the Alexafluor ® 568 fluorescence and control fluorescence of human normal fibroblast, pancreas and breast cells.
  • Figure 1C depicts the Alexafluor ® 568 fluorescence and control fluorescence of human umbilical vein endothelial cells (HUVEC).
  • HUVEC umbilical vein endothelial cells
  • Figure 2 depicts the capillary tube formation by HUVEC cells plated on Matrigel ® in the presence or absence of p28. Culture media contained 20ng/ml VEGF.
  • Figure 2A shows images of HUVEC cells incubated for 4h at 37°C with 0.1 O ⁇ M, 0.30 ⁇ M, 0.92 ⁇ M, 2.77 ⁇ M, 8.33 ⁇ M, 25 ⁇ M and 75 ⁇ M of p28, and then stained with calcein AM and visualized using fluorescence microscopy.
  • the graph shows the average number of tubes formed in peptide treated and control (untreated) cells.
  • Figure 3 depicts the results of the scratch wound HUVEC migration assay.
  • Figures 3A-C show the fixed cells that were stained for F-actin and nuclei.
  • Figure 3 A HUVEC cells at 90% confluence were scratched using a 1 ml plastic pipette tip.
  • Figure 3B the HUVEC cells were scratched and then incubated in the culture media containing 20ng/ml VEGF for 24h at 37°C in the absence of p28.
  • Figure 3 C the HUVEC cells were scratched and then incubated for 24h at 37°C in the presence of 25 ⁇ M p28.
  • the insets of Figures 3A-C show the cell density in the area away from the scored area.
  • a bar graph indicates the average # of cells in 20 different fields (20X) of the scratched area in control and p28 treated wells ( Figures 3B and C). Data represent mean ⁇ SEM. * indicates the differences are statistically significant.
  • Figure 4 depicts the images of the localization of cell structural proteins with and without p28 treatment.
  • HUVEC cells were plated on Matrigel ® -coated cover slips, incubated in the culture media containing 20ng/ml VEGF in the presence or absence of p28 peptide (25 ⁇ M) for 4 and 24h, fixed, and processed for staining of CD31 /PECAM-I, paxillin, Fak (focal adhesion kinase), vinculin, WASP (Wiskott Aldrich Syndrome protein) and ⁇ - catenin.
  • FIG. 4 A is CD31/PECAM-1; Figure 4B is paxillin; Figure 4C is Fak; Figure 4D is WASP; Figure 4E is vinculin; and Figure 4F is ⁇ -catenin.
  • Figure 4 A is CD31/PECAM-1; Figure 4B is paxillin; Figure 4C is Fak; Figure 4D is WASP; Figure 4E is vinculin; and Figure 4F is ⁇ -catenin.
  • Figure 5 depicts Mel-2 cells which were treated with increasing concentrations of p28 for 24, 48, and 72 hours. The number of cells in treated and control wells were counted using a Coulter counter. Data represent percentage of cell growth inhibition when compared to control cultures at the time point.
  • Figure 6 Depicts the results when Mel-2 cells were injected subcutaneously in the left flank (about 1 million cells/animal). Animals received p28 at the indicated dose at the time of injection.
  • Figure 6A shows the incidence of tumor occurrence after initiation of treatment with a graph indicating % of tumor free animals at days post treatment with Mel-2 cells.
  • Figure 6B shows the rumor size after initiation of treatment with a graph indicating the average volume of the tumors (cm 3 ) at days post treatment with Mel-2 cells.
  • Figure 7 depicts surface plasmon resonance binding titrations depicting the interactions of Azurin, H.8-azurin (H.8-Az), Laz, and GST-azurin (GST- Azu) constructs with MSPl -19 and MSP 1-42.
  • A Binding curves demonstrating the interactions of azurin and its analogues with MSPl -19 immobilized on carboxymethyldextran coated gold sensor chips (MSPl -19-CM5). Concentration dependent binding of the azurin proteins to MSPl -19 was determined via injection of various concentrations (0.05-300 nM) over the sensor surface and the extent of binding was evaluated as a function of the equilibrium resonance response value measured in resonance units (RU).
  • the MSPl -19 binding Kd values are: 32.2 ⁇ 2.4 nM (azurin), 26.2 ⁇ 2.4 nM (Laz), 11.8 ⁇ 0.3 nM (H.8-Az), and those for MSPl -42 binding are: 54.3 ⁇ 7.6 nM (azurin), 45.6 ⁇ 2.4 nM (Laz) and 14.3 ⁇ 1.7 nM (H.8-Az).
  • C Binding titrations for the interactions of GST-Azu fusion proteins over the MSP1-19-CM5 sensors surface demonstrate the recognition of GST-Azu 36-128 and GST-Azu 36-89 with MSP1-19. No binding was seen with GST or GST-Azu 88-113.
  • Figure 8 depicts inhibition of P. falciparum parasitemia (parasite growth within the RBC) by different concentrations, as shown, of Azurin, H.8-azurin (H.8-Az) and Laz.
  • Azurin H.8-azurin
  • Laz Laz.
  • normal red blood cells were infected with schizonts in absence or in presence of the proteins at different concentrations, incubated overnight and the number of intracellular parasites was scored by thin blood smear and Giemsa staining.
  • Figure 9 depicts surface plasmon resonance binding curves for the binding of ICAMs (ICAM-I, ICAM-2, ICAM-3 and NCAM, inset) with immobilized azurin. Due to large nonspecific binding to the bare Au-CM5 chip, CM5 was added as an eluent to the running buffer (1 mg/ml CM5 to HBS-EP buffer). The selective recognition of azurin with ICAM-3, but not with ICAM-I or ICAM-2, is notable and the binding strength was 19.5 ⁇ 5.4 nM. The Kd for NCAM binding with azurin, as shown in the inset, was 20 ⁇ 5.0 nM. Figure 10.
  • Figure 10 depicts the inhibition of HIV-I viral growth by azurin, H.8- azurin (H.8-Az) and Laz. These three proteins were incubated at different concentrations with PBMC followed by addition of the three subtypes of HIV-I. After 2 h incubation, the virus was removed but the proteins added back as described in Example 18. Suppression of virus growth was determined by ELISA assays of p24.
  • Figure 11 depicts surface plasmon resonance binding curves depicting the binding patterns of cupredoxins with CD4 and HIV-I gpl20.
  • A SPR titration curves showing novel and specific binding of azurin, and GST-Azu 36-128 (shown as an inset) with immobilized CD4 on carboxymethyldextran coated gold sensor chips (CD4-CM5).
  • CD4-CM5 carboxymethyldextran coated gold sensor chips
  • HIV-I gpl20, HIV-I gag, and HIV-I nef served as the positive and negative controls respectively.
  • the CD4 binding K d values are: 36.9 ⁇ 2.0 nM (azurin), 0.34 ⁇ 0.04 nM (GST-Azu 36-128), and 48.1 ⁇ 3.1 nM (HIV-I gpl20).
  • Az-CM5 The binding titrations when immobilized azurin (Az-CM5) is in contact with HIV proteins. Due to large nonspecific binding to the bare Au-CM5 chip, CM5 was added as an eluent to the running buffer (1 mg/ml CM5 to HBS-EP buffer). Curve fits gave Kd's of 25.1 ⁇ 3.1 nM (CD4), and 8.9 ⁇ 0.8 nM (HIV-I gpl20).
  • C SPR curves for the binding of ICAMs (ICAM- 1, ICAM-2, ICAM-3 and NCAM, inset) with immobilized azurin were determined under similar conditions as for experiments in part (B).
  • D SPR binding competition studies with CD4 immobilized on CM5 sensor chips.
  • Azurin + HIV-I gpl20 solutions were added at different azurin concentrations (0-4500 nM, [HIV-I gpl20] is 242 nM) to the sensor surface and the data were plotted as a ratio of resonances, % total response [R eq (azurin+HIV-1 gpl20)/(R eq /(HIV-l gpl20))].
  • GST- Azu 36-128 was titrated with HIV-I gpl20 to immobilized CD4 and analyzed in a similar manner. Competition data suggests 1 :1 stoichiometry of binding between azurin and GST- Azu 36-128 with immobilized CD4.
  • Figure 12 depicts surface plasmon resonance binding titrations depicting the interactions of azurin, and GST- Azurin fusions with DC-SIGN.
  • A Concentration dependent binding of azurin, ICAM-3, and GST- Azu 36-89 with DC-SIGN were determined via injection of various concentrations of the proteins (0 - 100 nM) over a DC-SIGN modified CM5 sensor surface and the extent of binding was evaluated as a function of the equilibrium resonance response value measured in resonance units (RU).
  • B The binding titration curve of GST- Azu 88-113 with DC-SIGN using the same sensor chip and protocol as described for azurin in part A.
  • Figure 13 depicts the effects of cupredoxin peptides on cancer cell viability.
  • Fig. 13 A effect of azurin (Azu 96-113) and plastocyanin (PIc 70-84) synthetic peptides on cell viability of Astrocytoma CCF-STTGl and Glioblastoma LN-229 cancer cell lines.
  • Fig. 13B effect of different concentrations of plastocyanin (PIc 70-84) synthetic peptide on Melanoma UISO-Mel-2 cell viability. Cancer cells (2 x 10 4 cells per well in 96- well plates) were treated with the synthetic peptides at different concentrations for 24 h at 37°C.
  • cytotoxic activity of Azu 96-113 synthetic peptide towards Glioblastoma LN-229 cells were determined by MTT assay. Cancer (2 x 10 4 cells per well in 96-well plates) were treated with various concentrations of Azu 96-113 (10, 25, 50, 75, 100 ⁇ M) for 24 h at 37°C. Percent cytotoxicity is expressed as percentage of cell death as compared to that of untreated control (0% cytotoxicity).
  • Figure 14 Effect of GST- Azu 36-128 and GST- Azu 88-113 on cell viability of MCF-7 cells.
  • GST- Azu peptides were added at increasing concentrations (1.25, 6.25 and 12.5 ⁇ M) into 96 well plates containing 8 x 10 3 cancer cells per well, incubated at 37°C for 48 h and subsequently analyzed using MTT assay.
  • GST and GST-Azu 36-89 at the same concentrations and untreated cells were run in parallel with GST-Azu 36-128 and GST-Azu 88-113 as controls.
  • FIGS 15 A-C Depict photographs showing penetration of azurin derived peptides, pi 8 and p28, into cancer cell lines of diverse histogenesis and their normal counterparts.
  • A Photos showing penetration of Alexafluor 568 labeled p28 or pi 8 after 2hrs at 37°C. The cationic Arg 8 was used as a control.
  • B Graphs depicting flow cytometric analysis of the penetration of Alexafluor 568 labeled p28 or pl8 into the same cell lines after 2hrs at 37°C.
  • C Graphs depicting fold increase over fluorescence from normal cells. Similar observations of p28 or pi 8 entry into 4 melanoma cell lines show a several fold increase over fluorescence from normal cells.
  • Figures 16 A and B Depict photographs showing entry of azu 60-77 (pl8b) and azu 66-77 (pl2) into cancer and normal cells. Cells were incubated with alexafluor 568 labeled p 18b (A) or pi 2 (B) at 37°C for 2 hrs and images recorded by confocal microscopy.
  • Figures 17 A and B Graphs depicting cellular membrane toxicity of azurin and its peptides.
  • FIGS 19 A-D (A) Depicts photographs showing confocal analysis of 28, pl8 (20 ⁇ M) and Arg 8 (10 ⁇ M) entry into UISO-Mel-2 cells after 1 hr at 37°C in the presence/absence of heparin sulfate (lOO ⁇ g/ml). (B) Graphs showing flow cytometric analysis of p28 or pl8 entry in the presence of inhibitors. Cell fluorescence intensity in the absence of inhibitor (control) was considered as 100%. (C) Graphs depicting FRCS analysis of p28 and pi 8 entry into fibroblasts in presence of inhibitors. (D) Depicts photographs showing colocalization of pi 8 and p28 with caveolin I (Panel 1 ).
  • UISO-Mel-2 cells were incubated with Alexafluor 568 labeled pi 8 or p28 (20 ⁇ M) or media for 2hrs at 37°C. Cells were fixed and processed for anti-caveolin 1 immunostaining. Confocal analysis of entry of Alexafluor 568 labeled pi 8 or p28 (20 ⁇ M) into UISO-Mel-2 cells after 2hrs at 37 0 C followed by antigolgin 97 antibodies (Panel 2 ). Colocalization of Alexafluor 568 labeled azurin, p28 and pi 8 (red) with mitotracker (green) (Panel 3 ) and Lysotracker (green) (Panel 4) dyes in
  • UISO-Mel-2 cells Cells were incubated at 37°C with 20 ⁇ M azurin, p28, pi 8 or media only. After 90 min incubation, mitotracker/lysotracker probes were added and cells incubated for 30min. Cells were counterstained with DAPI (blue). Colocalization of azurin, p28 or pi 8 appears as a yellow florescence.
  • Figures 20 A and B Graphs depicting UISO-Mel-2 cells that were incubated with increasing concentrations of azurin, p28, or pl8 at 37°C for 72hrs. MTT (A); Direct cell count (B). Cell viability (MTT) or cell number in control wells were considered as 100%. Data represent mean ⁇ SEM.
  • FIG. 21 (A) through (C). Graphs and charts depicting peptide binding and entry into cells.
  • A UISO-Mel-2 or fibroblast cells (3x10 5 cells) were suspended in MEME media without phenol red. Reactions were started by adding Alexafluor 568-conjugated p28 at 10, 50, 100, 150, 250, 300 and 400 ⁇ M for 30, 60, 90 and 120 sec on ice. Cells were analyzed by flow cytometry.
  • the K m and V max were calculated by plotting peptide concentration ( ⁇ M) vs velocity (MFI/sec).
  • FIG. C also depicts photographs of mouse organs, including the heart, lung, liver, kidney, spleen, and brain, taken 46 hours after injection of pl8.
  • (A) Depicts side and back photographs of mice with tumors taken 12 hours after injection with pi 8, p28, and arg-8 at 60 ⁇ molar concentration.
  • (B) Depicts photographs of mouse organs, including mouse brains, taken 12 hours after injection with pi 8, p28, and arg-8.
  • FIG. 25 (A) and (B).
  • (A) Depicts side and back photographs of mice with melanoma MEL-6 tumors taken 40 hours after injections of 600 ⁇ M concentrations of pi 8 and arg-8 into tail veins. Animals treated with pi 8 received 0.5 million cells, and animals treated with arg-8 received 1 million cells.
  • (B) Depicts photographs of mouse organs taken 40 hours after injections of 600 ⁇ M concentrations of pi 8 and arg-8.
  • FIG. 26 (A) and (B).
  • A Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 16 hours after injections of 60 ⁇ M concentrations of p28, pi 8, and arg-8.
  • B Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 24 hours after injections of 60 ⁇ M concentrations of p28, pl8, and arg-8.
  • Figure 27 Depicts photographs of mouse organs taken 48 hours after injection of 60 ⁇ M concentrations of p28 and pi 8 dye peptide complex into mice with melanoma MEL-23.
  • Figure 28 Depicts photographs of mouse organs taken 24 hours after injection of 60 ⁇ M concentrations of p28 into mice with MEL-23 tumors and organs.
  • Figure 29 Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 16 hours after injections of 60 ⁇ M concentrations of p28 and arg-8.
  • Figure 30 Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 16 hours after injections of 60 ⁇ M concentrations of pi 8.
  • Figure 31 Depicts side photographs of mice with tumors taken 10 and 24 hours after high dose treatment with 240 ⁇ M concentrations of pi 8, p28, and arg-8.
  • Figure 32 Depicts side and back photographs of mice with MCF-7 tumors and organs taken 28 hours after high dose treatment with 240 ⁇ M concentrations of pi 8, p28, and arg-8. Also depicts photographs of mouse organs with MCF-7 taken 28 hours after high dose treatment with 240 ⁇ M concentrations of pi 8, p28, and arg-8.
  • Figure 33 Depicts side and back photographs of mice with tumors taken 50 hours after high dose treatment with 240 ⁇ M concentrations of pi 8, p28, and arg-8.
  • Figure 34 Depicts photographs of mouse organs taken 24 hours after injection of 120 ⁇ M concentrations of pi 8, p28, and arg-8 into the tail veins of mice with HCT-116 tumors and organs.
  • FIG 35 (A) and (B).
  • A Depicts photographs of mouse organs taken 24 hours after injection of 120 ⁇ M concentrations of pi 8, p28, and arg-8 into the tail veins of mice with HCT-116 tumors and organs.
  • B Depicts side photographs of mice with HCT-116 tumors taken 21 hours after injection of 120 ⁇ M concentrations of pi 8, p28, and arg-8 into their tail veins.
  • Figure 36 (A) and (B).
  • A Depicts side and back photographs of mice with HCT- 116 24 hours after injection with 120 ⁇ M concentrations of p28, 47 days after injection of 1 million cells into tail veins.
  • B Depicts photographs of mouse organs taken from mice with HCT-116 4 hours after injection with 120 ⁇ M concentrations of p28, 47 days after injection of 1 million cells into tail veins.
  • Figure 37 Depicts photographs of organs from MEL-6 mice taken 24 hours after treatment with 120 ⁇ M concentrations of pi 8, p28, and arg-8.
  • FIG 38 (A) and (B).
  • A Depicts side and back photographs of MEL-6 mice taken 22 hours after injection of 120 ⁇ M concentrations of pi 8, p28, and arg-8, and 60 60 ⁇ M concentration of arg-8.
  • B Depicts photographs of MEL-6 mouse organs after treatment with 120 ⁇ M concentrations of pi 8, p28, and arg-8, and 60 ⁇ M concentration of arg-8.
  • Figure 39 (A) and (B).
  • Figure 40 Depicts side and back photographs of HT- 1080 mice during Doxorubicin vs. p28 study taken 16 hours after treatment with 60 and 120 ⁇ M concentrations of pi 8, p28, and arg-8.
  • Figure 41 (A) and (B).
  • A Depicts photographs of organs from HT-1080 mice taken 22 hours after treatment with 60 and 120 ⁇ M concentrations of p28 and arg-8.
  • B Depicts side-by-side photographs of brains from HT-1080 mice taken 22 hours after treatment with 60 and 120 ⁇ M concentrations of p28 and arg-8.
  • Figure 42 (A) and (B).
  • A Depicts photographs of organs from HT-1080 mice taken 22 hours after treatment with 60 and 120 ⁇ M concentrations of pi 8 and arg-8.
  • B Depicts side-by-side photographs of brains from HT-1080 mice taken 22 hours after treatment with 60 and 120 ⁇ M concentrations of pl8 and arg-8.
  • FIG 43 (A) through (E). Depicts photographs of HT-1080 mice with lung metastases treated via their tail veins with (A) 3mg/kg Doxorubicin IP, 3 treatments; (B) 5mg/kg IP p28 daily; (C) PBS control, PBS IP daily; (D) 10 mg/kg IP p28 daily; (E) 20 mg/kg IP daily.
  • Figure 44 (A) and (B).
  • A Depicts photographs of organs from HT-1080 mice in an animal study, whereby 1x10 6 cells are injected into tail veins (43 days) and all treated mice have lung metastases, taken 24 and 26 hours after 60 ⁇ M concentrations of p28 injected into tail veins. Animal 6982 was dead when photographed.
  • B Depicts side and back photographs of HT-1080 mice in an animal study, whereby 1x10 6 cells are injected into tail veins (43 days), taken 22 hours after 60 ⁇ M concentrations of p28 injected into tail veins. Animal 6982 was dead when photographed.
  • Figure 45 Depicts side and back photographs of HT-1080 mice in an animal study, whereby 1x10 6 cells are injected into tail veins (43 days), taken 26 hours after 60 ⁇ M concentrations of p28 injected into tail veins.
  • Figure 46 (A) and (B). Depicts photographs of (A) organs from mice and (B) back views of mice in BaIb-C peptide study taken 12 hours after treatment with 60 and 120 ⁇ M concentrations of pi 8, p28, and arg-8.
  • FIG 47 (A) and (B). Depicts photographs of (A) organs from mice and (B) side views of mice in BaIb-C peptide study taken 24 hours after treatment with 60 and 120 ⁇ M concentrations of pi 8, p28, and arg-8.
  • Figure 48 Depicts side and back photographs of MEL-6 mice (0.5 million cells injected via tail vein) 16 hours after injection into tail veins of 60 ⁇ M concentrations of pi 8 and arg-8.
  • Figure 49, (A) through (D). Depicts photographs of mouse organs, and specifically mouse brains, after treatment with pi 8 and p28.
  • Figure 50 Depicts photographs of organs from MEL-6 mice taken 24 hours after treatment with p28, pi 8, and arg-8.
  • FIG 51 (A) through (C).
  • A Depicts side and back photographs of MEL-6 mice 3 hours after injection with 60 ⁇ M concentrations of pi 8, p28, and arg-8.
  • B Depicts side and back photographs of MEL-6 mice, and photographs of organs from MEL-6 mice, taken 22 hours after injection with 60 ⁇ M concentrations of pi 8, p28, and arg-8.
  • C Depicts photographs of organs from MEL-6 mice 24 hours after injection with 60 ⁇ M concentrations of pl8, p28, and arg-8.
  • Figure 52 (A) and (B). Depict uptake of pi 8 and p28 into (A) mouse brains and (B) mouse organs).
  • Figure 53 Depicts side and back photographs of MEL-6 mice in study whereby 0.5 million cells injected LV. into tail vein (44 days post), taken 120 hours after injection into tail vein of 24 ⁇ M concentrations of pi 8 and arg-8.
  • Figure 54 Depicts photographs of organs from MEL-6 mice taken 168 hours after tratment with pi 8.
  • Figure 55 Depicts side and back photographs of MEL-6 mice taken after injection of arg-8 and pi 8, 72 hrs, day 41 post injection.
  • Figure 56 Depicts back photographs of mice taken after injection of arg-8 and pi 8.
  • Figure 57 Depicts side and front photographs of mice taken 3, 24, and 48 hours after injection of arg-8 and pi 8.
  • the term “cell” includes either the singular or the plural of the term, unless specifically described as a “single cell.”
  • polypeptide polypeptide
  • peptide protein
  • the terms “polypeptide,” “peptide,” and “protein” are used interchangeably to refer to a polymer of amino acid residues. The terms apply to amino acid polymers in which one or more amino acid residue is an artificial chemical analogue of a corresponding naturally occurring amino acid. The terms also apply to naturally occurring amino acid polymers.
  • the terms “polypeptide,” “peptide,” and “protein” are also inclusive of modifications including, but not limited to, glycosylation, lipid attachment, sulfation, gamma- carboxylation of glutamic acid residues, hydroxylation and ADP-ribosylation.
  • polypeptides are not always entirely linear.
  • polypeptides may be branched as a result of ubiquitination and they may be circular (with or without branching), generally as a result of post-translation events, including natural processing event and events brought about by human manipulation which do not occur naturally.
  • Circular, branched and branched circular polypeptides may be synthesized by non-translation natural process and by entirely synthetic methods as well.
  • the term "pharmacologic activity” means the effect of a drug or other chemical on a biological system.
  • the effect of chemical may be beneficial (therapeutic) or harmful (toxic).
  • the pure chemicals or mixtures may be of natural origin (plant, animal, or mineral) or may be synthetic compounds.
  • premalignant means precancerous, or before abnormal cells divide without control.
  • the term “lesion” means an area of abnormal tissue.
  • pathological condition includes anatomic and physiological deviations from the normal that constitute an impairment of the normal state of the living animal or one of its parts, that interrupts or modifies the performance of the bodily functions, and is a response to various factors (as malnutrition, industrial hazards, or climate), to specific infective agents (as worms, parasitic protozoa, bacteria, or viruses), to inherent defects of the organism (as genetic anomalies), or to combinations of these factors.
  • condition includes anatomic and physiological deviations from the normal that constitute an impairment of the normal state of the living animal or one of its parts, that interrupts or modifies the performance of the bodily functions.
  • a “condition” may be, but is not limited to an ailment, disease, infection or illness.
  • the term "suffering from” includes presently exhibiting the symptoms of a pathological condition, having a pathological condition even without observable symptoms, in recovery from a pathological condition, or recovered from a pathological condition.
  • chemoprevention is the use of drugs, vitamins, or other agents to try to reduce the risk of, or delay the development or recurrence of, cancer.
  • treatment includes preventing, lowering, stopping, or reversing the progression or severity of the condition or symptoms associated with a condition being treated.
  • treatment includes medical, therapeutic, and/or prophylactic administration, as appropriate. Treatment may also include preventing or lessening the development of a condition, such as cancer.
  • inhibite cell growth means the slowing or ceasing of cell division and/or cell expansion. This term also includes the inhibition of cell development or increases in cell death.
  • the term "inhibit the growth of HIV infection” means any means by which HIV infection is decreased, or prevented from increasing in the human body. These means can include, but are not limited to, inhibition of replication of the HIV genome, inhibition of synthesis and/or assembly of the HIV coat proteins, and inhibition of HIV entry into uninfected cells. This definition includes any the method of action of any of the currently known HIV therapies.
  • anti-malarial activity includes any activity that decreases the infectivity, the reproduction, or inhibits the progress of the lifecycle of a malaria parasite.
  • Anti-malarial activity includes inhibition of the growth of malaria infection by all of the means of observed with current anti-malarial drugs.
  • anti-malarial drug refers to drugs with anti-malarial activity that may be used to decrease the infectivity, the reproduction, or inhibit the progress of the lifecycle of a malaria parasite.
  • anti-HIV drug refers to drugs with anti-HIV activity HIV by which HIV infection in mammals is decreased, or prevented from increasing in the human body, by any means including, but are not limited to, inhibition of replication of the HIV genome, inhibition of synthesis and/or assembly of the HIV coat proteins, and inhibition of HIV entry into uninfected cells.
  • the term "inhibit angiogenesis” refers to the slowing, ceasing or reverse of the formation of blood vessels in a particular cells, tissues, or location of the body.
  • the inhibition of angiogenesis may be due to direct or indirect effects on endothelial cells.
  • the inhibition may also be at any stage of the angiogenesis process.
  • the inhibition may be due to preventing a tumor from producing Vascular Endothelial Growth Factor (VEGF), direct inhibition of endothelial cell proliferation and/or migration, acting as an antagonist of angiogenesis growth factors, inhibition of endothelial-specific integrin/survival signaling, or chelation of copper.
  • VEGF Vascular Endothelial Growth Factor
  • the inhibition of angiogenesis may be by any means by which the formation of blood vessels is slowed, ceased or reversed, including any means currently used by any anti-angiogenesis drug under development or on the market.
  • Inappropriate angiogenesis refers to any occurrence of angiogenesis that is undesirable.
  • Inappropriate angiogenesis may be angiogenesis that is associated with a condition in a mammal.
  • the inappropriate angiogenesis may be either the cause or the symptom of such a condition.
  • Inappropriate angiogenesis in a broader sense may be any angiogenesis that is unwanted, even though it may be within the realm of normal mammalian physiology.
  • a “therapeutically effective amount” is an amount effective to prevent or slow the development of, or to partially or totally alleviate the existing symptoms in a particular condition for which the subject is being treated. Determination of a therapeutically effective amount is well within the capability of those skilled in the art.
  • substantially pure when used to modify a protein or other cellular product of the invention, refers to, for example, a protein isolated from the growth medium or cellular contents, in a form substantially free of, or unadulterated by, other proteins and/or other compounds.
  • substantially pure refers to a factor in an amount of at least about 75%, by dry weight, of isolated fraction, or at least "75% substantially pure.” More specifically, the term “substantially pure” refers to a compound of at least about 85%, by dry weight, of isolated fraction, or at least "85% substantially pure.” Most specifically, the term “substantially pure” refers to a compound of at least about 95%, by dry weight, of isolated fraction, or at least "95% substantially pure.”
  • the term “substantially pure” may also be used to modify a synthetically-made protein or compound of the invention, where, for example, the synthetic protein is isolated from the reagents and byproducts of the synthesis reaction(s).
  • pharmaceutical grade when referring to a peptide or compound of the invention, is a peptide or compound that is isolated substantially or essentially from components which normally accompany the material as it is found in its natural state, including synthesis reagents and by-products, and substantially or essentially isolated from components that would impair its use as a pharmaceutical.
  • a “pharmaceutical grade” peptide may be isolated from any carcinogen.
  • “pharmaceutical grade” may be modified by the intended method of administration, such as "intravenous pharmaceutical grade,” in order to specify a peptide or compound that is substantially or essentially isolated from any substance that would render the composition unsuitable for intravenous administration to a patient.
  • an "intravenous pharmaceutical grade” peptide may be isolated from detergents, such as SDS, and antibacterial agents, such as azide.
  • the terms "isolated,” “purified” or “biologically pure” refer to material which is substantially or essentially free from components which normally accompany the material as it is found in its native state.
  • isolated peptides in accordance with the invention preferably do not contain materials normally associated with the peptides in their in situ environment.
  • An "isolated" region of a polypeptide refers to a region that does not include the whole sequence of the polypeptide from which the region was derived.
  • nucleic acid, protein, or respective fragment thereof has been substantially removed from its in vivo environment so that it may be manipulated by the skilled artisan, such as but not limited to, nucleotide sequencing, restriction digestion, site-directed mutagenesis, and subcloning into expression vectors for a nucleic acid fragment as well as obtaining the protein or protein fragment in substantially pure quantities.
  • substantially pure when used to modify the term a polypeptide or other compound, as used herein, refers to a polypeptide or compound, for example, a polypeptide isolated from the growth medium, in a form substantially free of, or unadulterated by, active inhibitory agents.
  • substantially pure refers to a compound in an amount of at least about 75%, by dry weight, of isolated fraction, or "75% substantially pure.” More specifically, the term “substantially pure” refers to a compound of at least about 85%, by dry weight, active compound, or “85% substantially pure.” Most specifically, the term “substantially pure” refers to a compound of at least about 95%, by dry weight, active compound, or "95% substantially pure.”
  • the substantially pure cupredoxin or cytochrome or a variant or derivative thereof can be used in combination with one or more other substantially pure compounds, or another isolated cupredoxin or cytochrome.
  • variant refers to amino acid sequence variants which may have amino acids replaced, deleted, or inserted as compared to the wild-type polypeptide. Variants may be truncations of the wild-type peptide. A “deletion” is the removal of one or more amino acids from within the polypeptide, while a “truncation” is the removal of one or more amino acids from one or both ends of the polypeptide.
  • a variant peptide may be made by manipulation of genes encoding the polypeptide.
  • a variant may be made by altering the basic composition or characteristics of the polypeptide, but not at least some of its pharmacologic activities.
  • a "variant" of azurin can be a mutated azurin that retains its ability to inhibit the development of premalignant mammalian cells.
  • a variant peptide is synthesized with non- natural amino acids, such as ⁇ -(3,5-dinitrobenzoyl)-Lys residues. Ghadiri & Fernholz, J. Am. Chem. Soc, 112:9633-9635 (1990).
  • a "variant" of azurin can be a mutated azurin that retains its ability to inhibit the growth of HIV infection in mammalian cells.
  • a "variant" of azurin can be a mutated azurin that retains its ability to inhibit parasitemia in malaria-infected human red blood cells.
  • the variant has not more than 20 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 15 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 10 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 6 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof.
  • the variant has not more than 5 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 3 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof.
  • amino acid means an amino acid moiety that comprises any naturally-occurring or non-naturally occurring or synthetic amino acid residue, i.e., any moiety comprising at least one carboxyl and at least one amino residue directly linked by one, two three or more carbon atoms, typically one ( ⁇ ) carbon atom.
  • a “derivative” of azurin refers to a peptide that is derived from the subject peptide.
  • a derivation includes chemical modifications of the peptide such that the peptide still retains some of its fundamental activities.
  • a "derivative" of azurin can, for example, be a chemically modified azurin that retains its ability to inhibit angiogenesis in mammalian cells.
  • Chemical modifications of interest include, but are not limited to, amidation, acetylation, sulfation, polyethylene glycol (PEG) modification, phosphorylation or glycosylation of the peptide.
  • a derivative peptide may be a fusion of a polypeptide or fragment thereof to a chemical compound, such as but not limited to, another peptide, drug molecule or other therapeutic or pharmaceutical agent or a detectable probe.
  • percent (%) amino acid sequence identity is defined as the percentage of amino acid residues in a polypeptide that are identical with amino acid residues in a candidate sequence when the two sequences are aligned. To determine % amino acid identity, sequences are aligned and if necessary, gaps are introduced to achieve the maximum % sequence identity; conservative substitutions are not considered as part of the sequence identity. Amino acid sequence alignment procedures to determine percent identity are well known to those of skill in the art. Often publicly available computer software such as BLAST, BLAST2, ALIGN2 or Megalign (DNASTAR) software is used to align peptide sequences. In a specific embodiment, Blastp (available from the National Center for Biotechnology Information, Bethesda MD) is used using the default parameters of long complexity filter, expect 10, word size 3, existence 11 and extension 1.
  • % amino acid sequence identity of a given amino acid sequence A to, with, or against a given amino acid sequence B can be calculated as:
  • X is the number of amino acid residues scored as identical matches by the sequence alignment program's or algorithm's alignment of A and B and Y is the total number of amino acid residues in B.
  • the % amino acid sequence identity of A to B will not equal the % amino acid sequence identity of B to A.
  • the shorter sequence will be the "B" sequence.
  • the truncated peptide will be the "B" sequence.
  • the present invention provides compositions comprising cupredoxin or cytochrome, and variants, derivatives, truncations, and structural equivalents of cupredoxin or cytochrome, and methods to treat and/or prevent two or more conditions in mammalian cells.
  • the invention also provides methods to administer to a patient to treat and/or prevent two or more diseases in a patient, comprising administering to the patient with one peptide or at least two peptides that are a cupredoxin, cytochrome and variants, derivatives, truncations, and structural equivalents of cupredoxin or cytochrome.
  • the invention provides compositions comprising Pseudomonas aeruginosa azurin, variants, derivatives, truncations, and structural equivalents of azurin, and their use to concurrently treat and/or prevent two or more conditions in a patient. More specifically, the present invention provides compositions for the concurrent treatment and/or prevention of conditions such as cancer, inappropriate angiogenesis, HIV and malaria, and patients at a higher risk of acquiring these conditions than the general population.
  • Members of the cupredoxin family, specifically azurin from Pseudomonas aeruginosa are promising compounds for therapeutic and preventative treatment of numerous diseases or conditions.
  • azurin is known to inhibit angiogenesis in human umbilical vascular endothelium cells (HUVECs).
  • Azurin from P. aeruginosa is also known for its ability to inhibit the growth of HIV- 1 infection in peripheral blood mononuclear cells and to inhibit parasitemia of malaria- infected mammalian red blood cells .
  • Azurin from P. aeruginosa is also known to interfere with the ephrin signaling system in various mammalian cells and tissues.
  • Azurin from P. aeruginosa preferentially enters J774 murine reticulum cell sarcoma cells, forms a complex with and stabilizes the tumor suppressor protein p53, enhances the intracellular concentration of p53, and induces apoptosis.
  • Rusticyanin from Thiobacillus ferrooxidans can also enter macrophages and induce apoptosis. Yamada et ah, Cell Cycle 3:1182-1187 (2004); Yamada et ah, Cell. Micro. 7:1418-1431 (2005). Plastocyanin from Phormidium laminosum and pseudoazurin form Achromobacter cycloclastes also are cytotoxic towards macrophages. U.S. Pat. Pub. No. 20060040269, published Feb. 23, 2006.
  • CPPs cationic cell penetrating peptides
  • Caveolae are a 50- to 100-nm omega-shaped subset of lipid raft invaginations of the plasma membrane defined by the presence of caveolin specific proteins (caveolin- 1, -2, or -3) that function as regulators of signal transduction.
  • Azurin, p28, and pi 8 all bind to cancer cells with high affinity and high capacity relative to many other potential anti-cancer peptides. It is believed that after binding, this protein/receptor complex localizes in caveolae and is internalized, eventually moving (via caveosomes) to the golgi, ER, and nucleus. In addition to caveolar-mediated entry, kinetic analysis also demonstrates that p28 and pi 8 penetrate the plasma membrane via a non- clathrin caveolae mediated process.
  • a clathrin- and caveolin-independent pathway can exist as a constitutive internalization mechanism, such as for the interleukin 2 receptor and for certain glycosyl-phosphatidylinositol (GPI)-anchored proteins.
  • GPI glycosyl-phosphatidylinositol
  • pi 8 and p28 are also able to penetrate the blood-brain barrier and enter mammalian brains, as demonstrated by, for example, Figures 24A, 24B, 25B, 27, 28, 32, 34, 35A, 36B, 37, 38B, 39A-B, 41 A-C, 42A-C, 44A, 46A, 47 A, 49 A-D, 50, 5 IB, 52A-B, and 54.
  • these peptides may be used to treat conditions in mammalian brains and brain cells.
  • synthesized p28 not only enters into a variety of malignant cell lines (melanoma (Mel-2), MCF-7, pancreatic, astrocytoma, glioblastoma, among others), but also non-cancerous human umbilical vein endothelial cells (HUVEC). See Example 1. p28 enters into these cells in a temperature dependent manner, but does not enter normal cells (fibroblast, normal mammary epithelium). As HUVEC cells are known to instigate angiogenesis in human embryos, the entry of p28 into HUVEC cells prompted an examination of the effect of p28 on angiogenesis.
  • malignant cell lines melanoma (Mel-2), MCF-7, pancreatic, astrocytoma, glioblastoma, among others
  • HUVEC human umbilical vein endothelial cells
  • HUVEC cells (20,000 cells) were plated on Matrigel ® coated wells and incubated in media containing 0-75 ⁇ M of p28. Cultures were examined under light microscopy at 4h and 24h post-treatment.
  • the p28 peptide inhibited capillary tube formation of the HUVEC in a dose dependent manner, suggesting that p28 inhibits the capillary tube formation step of angiogenesis. See Example 2.
  • p28 inhibited the migration of HUVEC cells on Matrigel ® in a scratch wound migration assay, indicating that p28 also inhibits the migration step of angiogenesis. See Example 3.
  • HUVEC cells on Matrigel ® p28 inhibits two critical steps in angiogenesis, capillary tube formation and cell migration.
  • azurin, and peptides derived from azurin, such as p28 have chemopreventative properties. It is now known that azurin, and p28, prevent the formation of premalignant preneoplastic lesions in mouse mammary gland organ culture. In a mouse mammary gland organ culture model, azurin at 50 ⁇ g/ml was found to inhibit the formation of alveolar lesions by 67%. Likewise, p28 at 25 ⁇ g/ml was found to inhibit the formation of alveolar lesions by 67%.
  • azurin at 50 ⁇ g/ml was found to inhibit the formation of ductal lesions by 79%, and p28 at 25 ⁇ g/ml inhibited the formation of ductal lesions by 71%.
  • Confocal microscopy and FAC showed that azurin and p28 entered normal murine mammary epithelial cells (MM3MG) and mammary cancer cells (4Tl). It is therefore now known that azurin and variants of azurin may be used to inhibit the formation of premalignant preneoplastic lesions, and thus the development of cancer, and specifically breast cancer, in mammalian patients.
  • cupredoxins and cytochromes will inhibit in vitro parasitemia in human red blood cells by the malaria parasite Plasmodium falciparum.
  • the cupredoxins azurin and Laz inhibit parasitemia in P. falciparum by about 50% and about 75% respectively.
  • rusticyanin and cytochromes c and f inhibited parasitemia by 20-30 %.
  • azurin has a discernable structural homology to the Fab fragment of Gl 7.12 mouse monoclonal antibody when complexed to the PfMSP 1-19 fragment of the MSP 1 surface protein of P. falciparum . While not limiting the mode of inhibition to any one means, it is thought that azurin may inhibit parasitemia of P. falciparum by interaction with the MSPl protein on the parasite's surface.
  • cytochrome C 551 aeruginosa cytochrome C 551
  • human cytochrome c and Phormidium laminosum cytochrome f will inhibit parasitemia in malaria- infected human red blood cells.
  • the cytochrome is cytochrome C 551 from P. aeruginosa, human cytochrome c or cytochrome f.
  • the cytochrome comprises an amino acid sequence that is SEQ ID NO: 19-21.
  • azurin can induce about a 90% suppression of growth of HIV-I in peripheral blood mononuclear cell (PBMC) cultures.
  • PBMC peripheral blood mononuclear cell
  • Azurin is now known to inhibit the growth of three strains of HIV-I, BaI (the most predominant clade B circulating in the US and Western Europe), a clade B African isolate RW/92/008/RE1, and a clade C Indian isolate IN/2167 D 15.
  • a cupredoxin-like protein from Neisseria, Laz is now also known to inhibit the growth of these three HIV-I strains, as well as a fusion of the H.8 region of the Laz protein with P. aeruginosa azurin.
  • M44KM64E mutant of azurin and cytochrome c551 from P. aeruginosa can inhibit HIV infection in HIV-infected human blood lymphocytes. See, Example 16.
  • cupredoxin may be, but is not limited to, azurin, pseudoazurin, plastocyanin, auracyanin, Laz, rusticyanin, stellacyanin or cucumber basic protein. In a more specific embodiment, the cupredoxin may be azurin.
  • the cupredoxin or azurin may be derived from Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp. , Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas fluorescens, Pseudomonas chlor or aphis, Bordetella pertussis, Pseudomonas syringae, Xylella fastidiosa and Vibrio parahaemolyticus.
  • the azurin is from P. aeruginosa.
  • the cupredoxin comprises an amino acid sequence that is SEQ ID NOs: 1, 5-12, 18 and 23.
  • Several cupredoxins are known to have pharmacokinetic activities similar to those of azurin from Pseudomonas aeruginosa.
  • rusticyanin from Thiobacillus ferrooxidans can also enter macrophages and induce apoptosis. Yamada et al, Cell Cycle 3:1182-1187 (2004); Yamada et ah, Cell. Micro. 7:1418—1431 (2005).
  • cupredoxins from P hormidium laminosum and pseudoazurin form Achromobacter cycloclastes also are cytotoxic towards macrophages.
  • variants and derivatives may include, but are not limited to, truncations of a cupredoxin, conservative substitutions of amino acids and proteins modifications such as PEGylation, all-hydrocarbon stabling of ⁇ -helices, and other methods and techniques disclosed herein.
  • the cytochrome is from a pathogenic bacterium.
  • the cytochrome inhibits parasitism in malaria-infected red blood cells, and more specifically, human red blood cells.
  • the cytochrome inhibits viral infection such as HIV.
  • the cytochrome inhibits cell cycle progression in a mammalian cancer cell, and more specifically in a J774 cell.
  • compositions of the Invention provides for peptides that are cupredoxins and/or cytochromes, and/or variants, derivatives or structural equivalents of cupredoxin or cytochrome.
  • the peptide is isolated.
  • the peptide is substantially pure or pharmaceutical grade.
  • the peptide is in a composition that comprises, or consists essentially of, the peptide.
  • the peptide is non-antigenic and does not raise an immune response in a mammal, and more specifically a human.
  • the peptide is less than a full-length cupredoxin or cytochrome, and retains some of the pharmacologic activities of the cupredoxin or cytochrome.
  • the peptide may retain the ability to concurrently treat and/or prevent two or more conditions in a mammalian cell or a patient.
  • the peptide retains the ability to inhibit the growth of viral or bacterial infection.
  • the peptide retains the ability to inhibit specifically HIV-I infection in peripheral blood mononuclear cells, or parasitemia in malaria- infected red blood cells, or P.
  • the invention also provides compositions comprising at least one peptide that is a cupredoxin, or variant, derivative, truncation, or structural equivalent of a cupredoxin.
  • the invention also provides compositions comprising at least one peptide that is a cytochrome, or variant, derivative, truncation, or structural equivalent of a cytochrome. In other embodiments, the composition consists essentially of the peptide.
  • the cupredoxin is selected from the group consisting of azurin, pseudoazurin, plastocyanin, rusticyanin, Laz, auracyanin, stellacyanin and cucumber basic protein. In some embodiments, the cupredoxin is from an organism selected from the group consisting of Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp.
  • the cupredoxin is from Pseudomonas aeruginosa.
  • the cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof is fused to a H.8 region of Laz from Neisseria meningitides or Neisseria gonorrhea.
  • a H.8 region of Laz from Neisseria meningitides or Neisseria gonorrhea is fused to a H.8 region of Laz from Neisseria meningitides or Neisseria gonorrhea.
  • a H.8 region is SEQ ID NO: 22, or a variant, derivative, truncation, or structural equivalent thereof.
  • the variant or derivative of cupredoxin has a significant structural homology to the Fab fragment of G 17.12 mouse monoclonal antibody.
  • An example of how this structural similarity can be determined can be found in Example 11.
  • significant structural homology between a cupredoxin and the Fab fragment of Gl 7.12 mouse monoclonal antibody can be determined by using the VAST algorithm (Gibrat et al, id.; Madej et al, id.).
  • the VAST p-value from a structural comparison of a cupredoxin to the Fab fragment of Gl 7.12 mouse monoclonal antibody can be less than about 10 "4 , less than about 10 "5 , less than about 10 "6 , or less than about 10 "7 .
  • the VAST score from a structural comparison of a cupredoxin to the Fab fragment of G 17.12 mouse monoclonal antibody can be greater than about 9, greater than about 10, greater than about 11 or greater than about 12.
  • the variant, derivative, truncation, or structural equivalent thereof has some of the functional characteristics of the P. aeruginosa azurin, P. aeruginosa cytochrome C 551 , human cytochrome c or cyanobacterial cytochrome f.
  • the peptide of the invention inhibits parasitemia by malaria in malaria-infected red blood cells, and more specifically parasitemia by P. falciparum in P. falciparum-infected human red blood cells.
  • the invention also provides for the variants, derivatives and structural equivalents of cupredoxin and cytochrome C 551 that retain the ability to inhibit parasitemia in malaria-infected red blood cells, and more specifically parasitemia by P.
  • the inhibition of parasitemia by P. falciparum in P. falciparum-infected human red blood cells may be determined by the method described in Example 14.
  • the invention provides for amino acid sequence variants of a cupredoxin or cytochrome which have amino acids replaced, deleted, or inserted as compared to the wild- type polypeptide. Variants of the invention may be truncations of the wild-type polypeptide.
  • the composition comprises a peptide that consists of a region of a cupredoxin or cytochrome that is less than the full length wild-type polypeptide.
  • the composition comprises a peptide that consists of more than about 10 residues, more than about 15 residues or more than about 20 residues of a truncated cupredoxin or cytochrome. In some embodiments, the composition comprises a peptide that consists of not more than about 100 residues, not more than about 50 residues, not more than about 40 residues or not more than about 30 residues of a truncated cupredoxin or cytochrome. In some embodiments, the composition comprises a peptide to which a cupredoxin or cytochrome, and more specifically to SEQ ID NOS. :1, 5-12, 18 and 23, and has at least about 90% amino acid sequence identity, at least about 95% amino acid sequence identity or at least about 99% amino acid sequence identity or is a mutant of SEQ ID NOS.: 1, 5-12, 18 and 23.
  • the variant of cupredoxin comprises Pseudomonas aeruginosa azurin residues 50-77 (p28, SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (pi 8, SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio par ahaem
  • the variant of cupredoxin consists of Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio par ahaemolyticus
  • cupredoxin variants can be designed that have a similar pharmacological activity to Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48),
  • the subject cupredoxin amino acid sequence will be aligned to the Pseudomonas aeruginosa azurin sequence using BLAST, BLAST2, ALIGN2 or Megalign (DNASTAR), the relevant residues located on the P. aeruginosa azurin amino acid sequence, and the equivalent residues found on the subject cupredoxin sequence, and the equivalent peptide thus designed.
  • the variants also include peptides made with synthetic amino acids not naturally occurring.
  • non-naturally occurring amino acids may be integrated into the variant peptide to extend or optimize the half-life of the composition in the bloodstream.
  • Such variants include, but are not limited to, D,L-peptides (diastereomer), (Futaki et al., J. Biol. Chem. 276(8):5836-40 (2001); Papo et al, Cancer Res. 64(16):5779-86 (2004); Miller et al, Biochem. Pharmacol. 36(l):169-76, (1987); peptides containing unusual amino acids (Lee et al., J. Pept. Res.
  • the invention also provides compositions comprising one peptide or at least two peptides that are a cupredoxin, cytochrome, or variant, derivative, truncation, or structural equivalent of a cupredoxin or cytochrome in a pharmaceutical composition.
  • the cupredoxin is in a pharmaceutical composition and is from an organism selected from the group consisting of Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidans ssp.
  • the cupredoxin is from Pseudomonas aeruginosa.
  • the cupredoxin or cytochrome is selected from the group consisting of SEQ ID NOS: 1, 5-12, 18, 23, 25, 27-33 and 48-50 in a pharmaceutical composition.
  • the cupredoxin may comprise SEQ ID NO: 30.
  • the peptide of the invention is a derivative of a cupredoxin or cytochrome.
  • the derivatives of cupredoxin or cytochrome are chemical modifications of the peptide such that the peptide still retains some of its fundamental activities.
  • a "derivative" of azurin can be a chemically modified azurin that retains its ability to treat and/or prevent more than one condition in a mammalian cell.
  • Chemical modifications of interest include, but are not limited to, amidation, acetylation, sulfation, polyethylene glycol (PEG) modification, phosphorylation, glycosylation of the peptide, and other modifications disclosed herein.
  • a derivative peptide maybe a fusion of a cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof to a chemical compound, such as but not limited to, another peptide, drug molecule or other therapeutic or pharmaceutical agent or a detectable probe.
  • a chemical compound such as but not limited to, another peptide, drug molecule or other therapeutic or pharmaceutical agent or a detectable probe.
  • Derivatives of interest include chemical modifications by which the half-life in the bloodstream of the peptides and compositions of the invention can be extended or optimized, such as by several methods well known to those in the art, including but not limited to, circularized peptides (Monk et al. , BioDrugs 19(4):261-78, (2005); DeFreest et al., J. Pept. Res.
  • the peptide of the composition of invention may be more than one of a variant, derivative and structural equivalent of a cupredoxin or cytochrome.
  • the peptide may be a truncation of azurin that has been PEGylated, thus making it both a variant and a derivative.
  • the peptides of the invention are synthesized with ⁇ , ⁇ -disubstituted non-natural amino acids containing olefin-bearing tethers, followed by an all-hydrocarbon "staple" by ruthenium catalyzed olefin metathesis. (Scharmeister et ai, J. Am. Chem. Soc.
  • peptides that are structural equivalents of azurin may be fused to other peptides, thus making a peptide that is both a structural equivalent and a derivative.
  • peptides that are structural equivalents of azurin may be fused to other peptides, thus making a peptide that is both a structural equivalent and a derivative.
  • the cupredoxin may be varied using methods that include, but are not limited to, those which decrease the hydrolysis of the peptide, decrease the deamidation of the peptide, decrease the oxidation, decrease the immunogenicity and/or increase the structural stability of the peptide. It is contemplated that two or more of the modifications described herein may be combined in one modified cupredoxin derived peptide, as well as combinations of one or more modifications described herein with other modification to improve pharmacokinetic properties that are well know to those in the art. Many methods to design such variants and derivatives are well known in the art, and some are discussed below and herein.
  • cupredoxins cytochromes, and variants, derivatives, truncations, and structural equivalents thereof, particularly cupredoxin-derived peptides such as truncations of azurin
  • One approach to improving the pharmacokinetic properties of cupredoxins, cytochromes, and variants, derivatives, truncations, and structural equivalents thereof, particularly cupredoxin-derived peptides such as truncations of azurin is to create variants and derivatives of the cupredoxin derived peptides that are less susceptible to biotransformation. Biotransformation may decrease the pharmacologic activity of the peptide as well as increase the rate at which it is eliminated from the patient's body.
  • One way of achieving this is to determine the amino acids and/or amino acid sequences that are most likely to be biotransformed and to replace these amino acids with ones that are not susceptible to that particular transformative process.
  • the cupredoxin derived peptides may include unnatural amino acids or modified amino acids.
  • the introduction of certain unnatural amino acids enhances the pharmcaokinetic properties of the cupredoxin derived peptide. Such introduction may be site-specific and may be done to avoid certain biochemical modifications in vivo.
  • Exemplary unnatural amino acids include b-amino acids (e.g., b3 and b2), homo-amino acids, cyclic amino acids, aromatic amino acids, Pro and Pyr derivatives, 3- substituted Alanine derivatives, Glycine derivatives, Ring-substituted Phe and Tyr Derivatives, Linear Core Amino Acids and Diamino Acids.
  • Such unnatural amino acids may be incorporated into peptides by site directed modification, ribosomal translation, or by chemical synthesis of the peptide. Each of these methods may be applied in synthesizing cupredoxin derived peptides.
  • modified cupredoxin derived peptides may be synthesized by the use of wild-type Aminoacyl-tRNA synthetases (AARSs) with unnatural amino acids building for the production of unnatural cupredoxin variants.
  • AARSs Aminoacyl-tRNA synthetases
  • the specificity of the ribosomal translation apparatus limits the diversity of unnatural amino acids that may be incorporated into peptides using ribosomal translation. Over ninety unnatural building blocks that are AARS substates have been uncovered including side chain and backbone analogs.
  • optically active ⁇ -amino acids may include the use of optically active ⁇ -amino acids.
  • optically active ⁇ -amino acids and their derivatives is being expanded for their use in pharmaceuticals, agrochemicals and as chiral ligands.
  • chiral glycine and alanine equivalents plan an important role.
  • At least one stereoselective strategy for constructing ⁇ -amino acids has been proposed, allowing for enantiopure ⁇ -amino acids in predetermined stereochemistry.
  • Hydrolysis is generally a problem in peptides containing aspartate.
  • Aspartate is susceptible to dehydration to form a cyclic imide intermediate, causing the aspartate to be converted to the potentially inactive iso-aspartate analog, and ultimately cleaving the peptide chain.
  • Aspartic acid— proline in the peptide sequence, the acid catalyzed formation of cyclic imide intermediate can result to cleavage of the peptide chain.
  • aspartic acid— glycine in the peptide sequence, the cyclic intermediate can be hydrolyzed either into the original aspartate form (harmless) or into the iso-aspartate analog.
  • sequences with serine can also be dehydrated to form a cyclic imide intermediate that can cleave the peptide chain. Cleavage of the peptide may result in reduced plasma half-life as well as reduced specific pharmacologic activity of the peptide.
  • substituting other amino acids for asparagine and/or serine in the sequence of the cupredoxin derived peptide may result in a peptide with improved pharmacokinetic properties such as a longer plasma half-life and increased specific activity of a pharmacologic activity of the peptide.
  • at one or more asparagine residues of the cupredoxin derived peptide may be replaced with another amino acid residue, and specifically a glutamic acid residue.
  • one or more serine residues of the cupredoxin derived peptide may be replaced with another amino acid residue, and specifically a threonine residue.
  • cupredoxin derived peptide one or more asparagine residues and one or more serine residues are substituted. In some embodiments, conservative substitutions are made. In other embodiments, non-conservative substitutions are made. Deamidation of amino acid residues is a particular problem in biotransformation.
  • This base-catalyzed reaction frequently occurs in sequences containing asparagine— glycine or glutamine— glycine and follows a mechanism analogous to the aspartic acid— glycine sequence above.
  • the de-amidation of the asparagine— glycine sequence forms a cyclic imide intermediate that is subsequently hydrolyzed to form the aspartate or iso-asparate analog of asparagine.
  • the cyclic imide intermediate can lead to racemization into D- aspartic acid or D-iso-aspartic acid analogs of asparagine, all of which can potentially lead to inactive forms of the peptide.
  • cupredoxin peptides may be prevented by replacing a glycine, asparagine and/or glutamine of the asparagine— glycine or glutamine — glycine sequences of the cupredoxin with another amino acid and may result in a peptide with improved pharmacokinetic properties, such as a longer plasma half-life and increased specific activity of a pharmacologic activity of the peptide.
  • the one or more glycine residues of the cupredoxin derived peptide are replaced by another amino acid residue.
  • one or more glycine residues of the cupredoxin derived peptide are replaced with a threonine or an alanine residue. In some embodiments, the one or more asparagine or glutamine residues of the cupredoxin derived peptide are replaced by another amino acid residue. In specific embodiments, one or more asparagine or glutamine residues of the cupredoxin derived peptide are replaced with an alanine residue. In other specific embodiments, the glycine at residues 58 and/or 63 of P.
  • aeruginosa azurin (SEQ ID NO: 1), or equivalent glycines of other cupredoxins, are replaced with an alanine or a threonine.
  • the methionine at residue 59 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent methionine residue of another cupredoxin derived peptide is replaced by an alanine residue.
  • the glycine at residue 63 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent glycine residue of another cupredoxin derived peptide, is replaced by a threonine residue.
  • the modified cupredoxin derived peptide of the invention comprises the following sequence, wherein the underlined amino acids are substituted into the wildtype Pseudomonas aeruginosa p28 sequence
  • LSTAADMQAVVTDTMASGLDKDYLKPDD (SEQ ID NO: 51).
  • Reversible and irreversible oxidation of amino acids are other biotransformative processes that may also pose a problem that may reduce the pharmacologic activity, and/or plasma half-life of cupredoxin derived peptides.
  • the cysteine and methionine residues are the predominant residues that undergo reversible oxidation. Oxidation of cysteine is accelerated at higher pH, where the thiol is more easily deprotonated and readily forms intra- chain or inter-chain disulfide bonds.
  • DTT dithiothreitol
  • TCEP tris(2-carboxyethylphosphine) hydrochloride
  • oxidation in the cupredoxin derived peptides may be prevented by replacing methionine and/or cysteine residues with other residues.
  • one or more methionine and/or cysteine residues of the cupredoxin derived peptide are replaced by another amino acid residue.
  • the methionine residue is replaced with a leucine or valine residue.
  • one or more of the methionines at residues 56 and 64 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent methionine residues in other cupredoxin derived peptides are replaced with leucine or valine.
  • conservative substitutions are made.
  • cupredoxin peptides of the invention comprise one of the following sequences, wherein the underlined amino acid is substituted into the wildtype Pseudomonas aeruginosa p28 sequence:
  • LSTAADLQGVVTDGLASGLDKDYLKPDD SEQ ID NO: 52
  • LSTAADVQGVVTDGVASGLDKDYLKPDD SEQ ID NO: 53.
  • Another biotransformative process that may affect the pharmacologic activity, plasma half-life and/or immunogenicity of the cupredoxin derived peptides is diketopiperazine and pyroglutamic acid formation. Diketopiperazine formation usually occurs when glycine is in the third position from the N-terminus, and more especially if proline or glycine is in position 1 or 2.
  • the reaction involves nucleophilic attack of the N-terminal nitrogen on the amide carbonyl between the second and third amino acid, which leads to the cleavage of the first two amino acids in the form of a diketopiperazine.
  • pyroglutamic acid formation may be almost inevitable if glutamine is in the N-terminus.
  • This is an analogous reaction where the N-terminal nitrogen attacks the side chain carbonyl carbon of glutamine to form a deaminated pyroglutamayl peptide analog. This conversion also occurs in peptide containing asparagine in the N-terminus, but to a much lesser extent.
  • diketopiperazine and pyroglutamic acid formation may be decreased in cupredoxin derived peptides by replacing glycine in position 1 , 2, or 3 from the N-terminus, proline in position 3 from the N-terminus, or asparagine at the N-terminus of the peptide with another amino acid residue.
  • a glycine in positions 1, 2, or 3 from the N-terminus of the cupredoxin derived peptide is replaced with another amino acid residue.
  • the glycine residue is replaced by a threonine or alanine residue.
  • a proline at position 3 from the N-terminus of the cupredoxin derived peptide is replaced with another amino acid residue.
  • the proline is replaced by an alanine residue.
  • an asparagine at the N-terminus is replaced with another amino acid residue.
  • the asparagine residue is replaced by a glutamine residue.
  • conservative substitutions are made.
  • non-conservative substitutions are made.
  • racemization Another biotransformative process that may affect the pharmacologic activity, plasma half-life and/or immunigenicity of the cupredoxin derived peptide is racemization. This term is loosely used to refer to the overall loss of chiral integrity of the amino acid or peptide.
  • Racemization involves the base-catalyzed conversion of one enantiomer (usually the L-form) of an amino acid into a 1 : 1 mixture of L- and D-enantiomers.
  • One way to improve stability of the peptide in general is by making a retro-inverso (D-isomer) peptide.
  • the double inversion of peptide structure often leaves the surface topology of the side-chain intact and has been used extensively to stabilize biologically active peptides.
  • Snyder et al PLoS Biol. 2:0186-0193 (2004).
  • a D-amino acid substituted Tat is internalized into cells as well as the L- amino acid peptide. Futaki et al, J. Biol. Chem.
  • the modified cupredoxin derived peptide is a retro-inverso (D-isomer) version of the cupredoxin derived peptide. In a specific embodiment, the modified cupredoxin derived peptide is
  • DDPKLYDKDLGSAMGDTVVGQMDAATSL SEQ ID NO: 54.
  • Other methods to protect a cupredoxin derived peptide from biotransformative degradation are N-acetylation and C-amidation. These derivatives may protect the peptide from degradation and may make the cupredoxin derived peptide more closely mimic the charge state of the alpha amino and carboxyl groups in the native protein. Peptides with the N-acetylation and/or C-amidation can be provided by commercial suppliers.
  • the N-terminus of the cupredoxin derived peptide may be acetylated.
  • the C-terminus of the cupredoxin derived peptides may be amidated.
  • the modified cupredoxin derived peptide is
  • Acetylation-LSTAADMQGVVTDGMASGLDKDYLKPDD-amidation SEQ ID NO: 55.
  • Cyclization is an additional manner of biotransformation that may be beneficial to therapeutic peptides including the cupredoxins as described herein. Cyclization may stabilize therapeutic peptides, allowing them to be stored longer, be administered at lower doses and be administered less frequently. Cyclization has been shown to protect peptides against peptidase and protease degradation. Cyclization can be done chemically or enzymatically. Enzymatic cyclization is generally less problematic than chemical cyclization, as chemical cyclization can lack in regio- and stereospecificity, can lead to multimerization in lieu of cyclization and can require complicated multistep processes. Indeed, it has been shown that thioether cyclization is more protective and stable than a disulfide bond against proteolytic enzymes.
  • Lantibiotics are produced by and inhibit the growth • of gram-positive bacteria.
  • dehydroalanine and dehydrobutyrine are created by enzyme mediated dehydration of serine and threonine residues. Cysteines are then enzymatically coupled to the dehydrated serine and threonine residues to form thioether cyclizations.
  • lantibiotics show such couplings via thioether bonds between residues that are up to 19 residues apart.
  • Thioether ring formation depends upon the leader peptide.
  • the location of the cyclization depends upon the cyclase mediated regio- and stereospecific ring closure and the positions of the dehydratable serine and threonine residues.
  • the best characterized of the lantibiotics is nisin — a pentacyclic peptide antiobiotic produced by Lactococcus lactis.
  • Nisin is composed of four methyllanthionines, one lanthionine, two dehydroalanines, one dehydrobutyrine, and twenty-six unmodified amino acids.
  • Nisin's five thioether cross-links are formed by the addition of cysteine residues to dehydroalanine and dehydrobutyrine residues that originate from serine and threonine.
  • Nisin contains thioether-containing amino acids that are posttranslationally introduced by a membrane-associated enzyme complex. This enzyme complex includes: transporter NisT, serine and threonine dehydratase NisB, and cyclase NisC.
  • NisB dehydrates serine and threonine residues, converting them into dehydroalanine and dehydrobutyrine, respectively.
  • NisC catalyzed enantioselective coupling of cysteines to the formed dehydoresidues.
  • NisT facilitates the export of the modified prenisin.
  • NisP cleaves the nisin leader peptide from prenisin.
  • the cyclase NisC has been well characterized. Li et al, "Structure and Mechanism of the Lantibiotic Cylclase Involved in Nisin Biosynthesis" 311 Science, 1464-67 (2006) (hereby incorporated by reference in its entirety).
  • hexapeptides VSPPAR (SEQ ID NO: 56), YTPPAL (SEQ ID NO: 57) and FSFFAF (SEQ ID NO: 58).
  • the hexapeptides suggest that the presence of a proline at position 3 or 4 or having phenylalanine flanking both sides may prohbit dehydration.
  • the rings are typically formed by coupling a dehydrated residue to a C-terminally located cysteine. However, rings may be formed by coupling a dehydrate residue to a N-terminally located cysteine.
  • nisin dehydrating and transport enzymes are not specific to nisin and may, in fact, be used to modify non-nisin peptides (and non-lantibiotic peptides).
  • NisB has been shown to dehydrate serine and threonine residues in peptides such as human peptide hormones when such peptides are N-terminally fused to the lantibiotic leader peptide.
  • similar ring formation characteristics apply; namely, the extent of dehydration can be controlled by the amino acid context of the flanking region of the dehydratable serine and threonine residues.
  • hydrophobic flanking residues e.g., alanine and valine
  • hydrophobic flanking residues e.g., alanine and valine
  • the presence of an N-terminal aspartate and C-terminally flanked arginine prevented dehydration. It also shown that the presence of proline residues and phenylalanine residues is disfavorable for dehydration.
  • hydrophilic flanking residues prevented dehydration of the serine and threonine residues. Hydrophobic flanking favors dehydration; hydrophilic flanking disfavors dehydration.
  • the average hydrophobicity of the flanking residues of serines and threonine is positive ⁇ .40 on the N- terminal side and .13 on the C-terminal side. Also, the average hydrophobicity of the residues flanking serines and threonines that are not dehydrated is negative — .36 on the N- terminal side and -1.03 on the C-terminal side. Deydration is not restricted by the presence of a series of flanking threonine residues and is not restricted by the distance bteween the nisin leader peptide and the residue to be dehydrated.
  • NisC has been shown to catalyze the regiospecif ⁇ c formation of thioether rings in peptides unrelated to naturally occuring lantibiotics. Generally, such peptides must be fused to the nisin leader peptide. In some cases, thioether rings may form spontaneously, for example where a dehydroalanine is spaced by two amino acids from a cysteine. Unlike spontaneous cyclization, NisC catalyzed cyclization is stereospecific for dehydrated pre- nisin. Consequently, the methyllanthionines and lanthionine in nisin are in the DL configuration. It is thought that cyclization in nonlantibiotic peptides will also be stereospecific
  • cupredoxins and cytochromes and derivatives, variants, truncations, or structural equivalents thereof, such as truncated azurin may be modified by introducing thioether bridges into the structure.
  • the azurin truncation p28 (SEQ ID NO: 29), for example, may be modified using this method.
  • Structure 2 Result of 70 ns simulation.
  • amino acid sequence of p28 is SEQ ID NO: 29
  • LSTAADMQGVVIDGMASGLDKDYLKPDD The amino acid sequence known as pi 8 is SEQ ID NO: 30 (LSTAADMQGVVTDGMASG).
  • Thioether bridges can be formed between Ser/Thr on the N-side to Cys on the C-side.
  • the serine/threonine is dehydrated and subsequently coupled to the cysteine.
  • Threonines are preferred since they are more easily dehydrated than serines.
  • hydrophobic flanking residues (at least one) to the threonine are preferred since they enhance the extent of dehydration. Negatively charged amino acids, glutamate and aspartate, that are flanking residues have a strong negative effect on dehydration.
  • hydrophilic flanking residues especially glycin
  • glycin do not favor dehydration.
  • Cys there is a slight preference for charged hydrophilic residues, especially glutamate/aspartate.
  • the bulkiness of the amino acids that participate in the ring matters.
  • the truncated azurin sequence is LSTAADMQGVVTDGMASGLDKDYLTPGC (SEQ ID NO: 59).
  • a thioether bridge is formed between positions 25 and 28 of p28, and will be fully protected against carboxyetidases. Positions 2, 3 and 25 will be dehydrated, but neither the import sequence, nor the sequence thought to be relevant for interaction with p53, is altered by thioether ring introduction. As such, peptide activity should not be altered.
  • the threonine is between two hydrophobic amino acids and hence is expected to be fully dehydrated by dehydratase, NisB, according to specific guidelines. See Rink et al., Biochemistry 2005. The same guidelines also predict cyclization involving positions 25 and 28 by cyclase NisC, especially because of the aspartate located before the cysteine.
  • the truncated azurin sequence is LSTAADCQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 60) and the thioether bridge is formed between positions 3 and 7.
  • the ring between position 3 and 7 mimics ring A of nisin and makes use of the existing threonine at position 2.
  • the aspartate at position 6 will favor cyclization.
  • the truncated azurin sequence is LSTAACMQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 61), and the threonine in position 2 is utilized to form a thioether bridge.
  • two or more of the thioether rings in the truncated azurins described in the paragraphs above are combined into one peptide.
  • many truncated azurin sequences can be created and screened for threonine rings by analyzing the peptides with a ring of one lanthionine and two to three additional amino acids under the sulfur bridge. This might involve one or combinations of the sequences below: LSTACDMQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 62) LSTAATMQCVVTDGMASGLDKDYLKPDD (SEQ ID NO: 63) LSTAATMQGCVTDGMASGLDKDYLKPDD (SEQ ID NO: 64) LSTAANTQGCVTDGMASGLDKDYLKPDD (SEQ ID NO: 65) LSTAANTQGVCTDGMASGLDKDYLKPDD (SEQ ID NO: 66) LSTAADMTAVCTDGMASGLDKDYLKPDD (SEQ ID NO: 67) LSTAADMTAVVCDGMASGLDKDYLKPDD (SEQ ID NO: 68) LSTAADMQTVVCDG
  • a practical approach would be to genetically make a large number of such sequences and select a group for purification on the basis of extent of modification and level of production.
  • a thioether bridge is formed between a threonine at position 12 in p28 (SEQ ID NO: 29) and the c-terminus of the peptide.
  • the distance between the Ca of position 13 and the aspartate at position 28 might be 17.52 angstroms, larger than 1.5 nanometers, implying significant alteration of the structure of the peptide.
  • Structure 3 Measurement of thioether bridge positions based on distances between Ca atoms in a simulated structure.
  • LSTAADMQGVVTATMGSGLCKDYLKPDD (SEQ ID NO: 76), with a thioether bridge from position 14 to position 2 at a distance of 4.38 angstroms.
  • the mutation of aspartate at position 13 to alanine favors dehydration of threonine at position 14.
  • Mutation of alanine at position 16 to glycine completely prevents dehydration of serine at position 17 and enhances cyclization.
  • LSTAADMQGVVTDLTASGLCKDYLKPDD (SEQ ID NO: 77), with the thioether bridge from position 15 to position 20 at a distance of 5.83 angstroms.
  • mutation of glycine at position 14 to leucine favors dehydration of threonine at position 15.
  • the stability of the tertiary structure of the cupredoxin, cytochrome, or variant, derivative, truncation, or structural equivalent thereof will affect most aspects of the pharmacokinetics, including the pharmacologic activity, plasma half-life, and/or immunogenicity among others. See Kanovsky et al, Cancer Chemother. Pharmacol. 52:202- 208 (2003); Kanovsky et al, PNAS 23:12438-12443 (2001). Peptide helices often fall apart into random coils, becoming more susceptible to protease attack and may not penetrate cell membrane well. Schafffle et al, J. Am. Chem. Soc. 122:5891-5892 (2000).
  • one way to stabilize the overall structure of a peptide such as a cupredoxin is to stabilize the ⁇ -helix structure of the peptide.
  • the intra-molecular hydrogen bonding associated with helix formation reduces the exposure of the polar amide backbone, thereby reducing the barrier to membrane penetration in a transport peptide, and thus increasing related pharmacologic activities and increasing the resistance of the peptide to protease cleavage.
  • Pseudomonas aeruginosa azurin (SEQ ID NO: 1) has ⁇ -helices at residues 53-56, 58-64 and 68-70.
  • One method to stabilize an ⁇ -helix is to replace in the ⁇ -helix helix breaking amino acid residues such as glycine, proline, serine and aspartic acid, or helix neutral amino acid residues such as alanine, threonine, valine, glutamine, asparagine, cysteine, histidine, lysine or arginine, with helix forming residues, such as leucine, isoleucine, phenylalanine, glutamic acid, tyrosine, tryptophan and methionine or helix favoring amino acid residue substitutions, for example ⁇ -amino-isobutyric acid (Aib). See Miranda et al, J. Med.
  • cupredoxin derived peptides may be stabilized by replacing one or more glycine, proline, serine and/or aspartic acid residues with other amino acids.
  • the glycine, proline, serine, aspartic acid, alanine, threonine, valine, glutamine, asparagine, cysteine, histidine, lysine and/or arginine residues are replaced by leucine, isoleucine, phenylalanine, glutamic acid, tyrosine, tryptophan, Aib and/or methionine residues. See Lee et al, Cancer Cell Intl. 11:21 (2005).
  • one or more serine or glutamine residues in the ⁇ -helices of a cupredoxin derived peptide may be substituted.
  • the serine and/or glutamine residues in residues 53-56, 58-64 and 68-70 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides may be replaced.
  • the glutamine residue at amino acid residue 57 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide may be replaced, more specifically replaced with tryptophan.
  • aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan.
  • the threonine residue at amino acid residue 61 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide may be replaced, more specifically replaced with tryptophan.
  • the glycine residue at amino acid residue 63 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan.
  • one or more threonine, glutamine or glycine residues at amino acid residues 52, 57, 61 or 63 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide may be replaced, more specifically replaced with tryptophan.
  • the cupredoxin peptide comprises one of the following sequences wherein the underlined amino acid is substituted into the wildtype Pseudomonas aeruginosa p28 sequence:
  • LSTAADMWGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 79); LSTAADMQGVVWDGMASGLDKD YLKPDD (SEQ ID NO: 80);
  • LSWAADMQGVVTDWMASGLDKDYLKPDD (SEQ ID NO: 84); LSTAADMWGVVWDGMASGLDKDYLKPDD (SEQ ID NO: 85);
  • equivalent amino acids in other cupredoxin derived peptides are substituted with tryptophan.
  • Another method to stabilize an ⁇ -helix tertiary structure involves using unnatural amino acid residues capable of ⁇ -stacking.
  • unnatural amino acid residues capable of ⁇ -stacking.
  • pairs of ⁇ -(3,5-dinitrobenzoyl)-Lys residues were substituted into the ⁇ -helix region of a peptide at different spacings.
  • the overall results showed that the ⁇ ,(/ ' +4) spacing was the most effective stabilizing arrangement.
  • the cupredoxin derived peptide may be modified so that the lysine residues are substituted by ⁇ -(3,5-dinitrobenzoyl)-Lys residues.
  • the lysine residues may be substituted by ⁇ -(3,5- dinitrobenzoyl)-Lys in a /,(/+4) spacing.
  • Another method to stabilize an ⁇ -helix tertiary structure uses the electrostatic interactions between side-chains in the ⁇ -helix.
  • the cupredoxin derived peptides may comprise macrocyclic cw-[Ru- (NH 3 ) 4 L 2 ] 3+ complexes where L 2 is the side chains of two histidines.
  • one or more histidine-cysteine or histidine-histidine residue pairs may be substituted an i,(i+4) arrangement into the ⁇ -helices of the cupredoxin derived peptide.
  • one or more histidine-cysteine or histidine-histidine residue pairs may be substituted an i,(i+4) arrangement in residues 53-56, 58-64 and 68-70 of P.
  • cupredoxin derived peptide may further comprise Cu, Zn, Cd and/or Ru ions.
  • Another method to stabilize an ⁇ -helix tertiary structure involves disulfide bond formation between side-chains of the ⁇ -helix. It is also possible to stabilize helical structures by means of formal covalent bonds between residues separated in the peptide sequence. The commonly employed natural method is to use disulfide bonds. Pierret et al., Intl. J. Pept. Prot. Res., 46:471-479 (1995).
  • one or more cysteine residue pairs are substituted into the ⁇ -helices of the cupredoxin derived peptide.
  • one or more cysteine residue pairs are substituted at residues 53-56, 58-64 and 68-70 of P.
  • aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides.
  • Another method to stabilize an ⁇ -helical tertiary structure involves the use of side chain lactam bridges.
  • a lactam is a cyclic amide which can form from the cyclisation of amino acids.
  • Side chain to side chain bridges have been successfully used as constraints in a variety of peptides and peptide analogues, such as amphipathic or model ⁇ -helical peptides, oxytocin antagonists, melanoptropin analogues, glucagon, and SDF-I peptide analogues.
  • the Glucagon-like Peptide- 1 gradually assumes a helical conformation under certain helix-favoring conditions and can be stabilized using lactam bridging.
  • lactam bridges may be varied in size, effecting stability and binding affinity. Id. Such modifications improved the stability of the compounds in plasma. Id.
  • lactam bridges can be used to induce and stabilize turn or helical conformations.
  • cupredoxin or variant analogues are prepared with lactam bridging between nearby amino acids (such as i to i+4 glutamic acid-lysine constraints).
  • the cupredoxin derived peptide may comprise such modifications to enhance ⁇ -helix content.
  • Another method to stabilize an ⁇ -helix tertiary structure is the all-carbon cross-link method.
  • the all-hydrocarbon cross-link method is proven to increase the stabilization of helical structure, protease resistant and cell-permeability. Walensky et al, Science, 305, 1466-1470 (2004). ⁇ , ⁇ - disubstituted non-natural amino acids containing olefin-bearing tethers are incorporated into peptides. Ruthenium catalyzed olefin metathesis generates an all-hydrocarbon "staple" to cross-link the helix. Schafmeister et al, J. Am. Chem.
  • Non-natural amino acids containing olefin-bearing tethers may be synthesized according to methodology provided in Schafmeister et al (id.) and Williams and Im (J. Am. Chem. Soc, 113:9276-9286 (1991)).
  • the cupredoxin derived peptides are stabilized by all-hydrocarbon staples.
  • one or more pairs of ⁇ , ⁇ - disubstituted non-natural amino acids containing olefin-bearing tethers corresponding to the native amino acids are substituted into the ⁇ - helices of the cupredoxin derived peptide.
  • one or more pairs of ⁇ , ⁇ - disubstituted non-natural amino acids containing olefin-bearing tethers corresponded to the native amino acids are substituted into residues 53-56, 58-64 and 68-70 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides.
  • the modified cupredoxin derived peptide may comprise X I SX 2 AADX 3 X 4 X 5 VVX 6 DX 7 X 8 ASGLDKDYLKPDX 9 (SEQ ID NO: 89), where Xi is L or acetylated-L, X 2 is T or W, X 3 is M, L or V, X 4 is Q or W, X 5 is G or A, X 6 is T or W, X 7 is G, T or W, X 8 is M, L or V, and Xg is D or amidated-D.
  • the modified cupredoxin derived peptide may consist of
  • X I SX 2 AADX 3 X 4 X 5 VVX 6 DX 7 X 8 ASGLDKDYLKPDX 9 (SEQ ID NO: 89), where X, is L or acetylated-L, X 2 is T or W, X 3 is M, L or V, X 4 is Q or W, X 5 is G or A, X 6 is T or W, X 7 is G, T or W, X 8 is M, L or V, and X 9 is D or amidated-D.
  • the modified cupredoxin derived peptide may comprise
  • X 1 DPKLYDKDLGSAX 2 X 3 DX 4 VVX 5 X 6 X 7 DAAX 8 SX 9 (SEQ ID NO: 90), where Xi is D or acetylated-D, X 2 is M, L or V, X 3 is G, T or W, X 4 is T or W, X 5 is G or A, X 6 is Q or W, X 7 is M, L or V, X 8 is T or W, and X 9 is L or amidated-L.
  • the modified cupredoxin derived peptide may consist of X I DPKLYDKDLGSAX 2 X 3 DX 4 VVX 5 X 6 X 7 DAAX 8 SX 9 (SEQ ID NO: 90), where Xj is D or acetylated-D, X 2 is M, L or V, X 3 is G, T or W, X 4 is T or W, X 5 is G or A, X 6 is Q or W, X 7 is M, L or V, X 8 is T or W, and X 9 is L or amidated-L. Specific peptides of interest are listed in Table 3.
  • PEG attachment has improved the pharmacokinetic properties of many therapeutic proteins, including interleukins (Kaufman et al, J. Biol. Chem. 263:15064 (1988); Tsutsumi et al, J. Controlled Release 33:447 (1995)), interferons (Kita et al, Drug Des. Delivery 6:157 (1990)), catalase (Abuchowski et al, J. Biol. Chem.
  • PEG for use as a vehicle or base in foods, cosmetics and pharmaceuticals, including injectable, topical, rectal and nasal formulations.
  • PEG shows little toxicity, and is eliminated from the body intact by either the kidneys (for PEGs ⁇ 30 kDa) or in the feces (for PEGs > 20 kDa).
  • PEG is highly soluble in water.
  • PEGylation of cupredoxins, cytochromes, and/or variants, derivatives, truncations, and structural equivalents thereof, particularly cupredoxin-derived peptides such as truncations of azurin may be used to increase the lifetime of the peptide in the bloodstream of the patient by reducing renal ultrafiltration, and thus reduce elimination of the drug from the body.
  • Charge masking may affect renal permeation.
  • Charge masking may be a consequence of the paramchemical modification of protein ionizable functional group, namely amines or carboxyls.
  • the most common procedures for producing protein-PEG derivatives involves the conversion of protein amino groups into amides with the consequent loss of positive charges, and this can alter protein ultrafiltration. Since anionic macromolecules have been found to be cleared by renal ultrafiltration more slowly than neutral or positive ones, it could be expected that PEG conjugation to amino groups prolongs the permanence of the PEGylated peptide in the bloodstream.
  • Molecular size and globular ultrafiltration may also affect renal ultrafiltration of therapeutic peptides.
  • the molecular weight cut off for kidney elimination of native globular proteins is considered to be about 70 kDa, which is close to the molecular weight of serum albumin.
  • proteins with molecular weight exceeding 70 kDa are mainly eliminated from the body by pathways other than renal ultrafiltration, such as liver uptake, proteolytic digestion and clearance by the immune system. Therefore, increasing the size of a therapeutic peptide by PEGylation may decrease renal ultrafiltration of that peptide form the bloodstream of the patient.
  • PEGylation of a peptide may decrease the immunogenicity of that peptide, as well as protect the peptide from proteolytic enzymes, phagocytic cells, and other factors that require direct contact with the therapeutic peptide.
  • the umbrella-like structure of branched PEG in particular has been found to give better protection than linear PEG towards approaching proteolytic enzymes, antibodies, phagocytic cells, etc. Caliceti and Veronese, Adv. Drug. Deliv. Rev. 55:1261-12778 (2003).
  • the cupredoxin derived peptides are modified to have one or more PEG molecules covalently bonded to a cysteine molecule.
  • the covalent bonding does not necessarily need to be a covalent bond directly from the PEG molecule to the cupredoxin derived peptide, but may be covalently bonded to one or more linker molecules which in turn are covalently bonded to each other and/or the cupredoxin derived peptide.
  • the cupredoxin derived peptide have site-specific PEGylation.
  • the PEG molecule(s) may be covalently bonded to the cysteine residues 3, 26 and/or 112 of P.
  • aeruginosa azurin SEQ ID NO: 1
  • one or more cysteine residues may be substituted into the cupredoxin derived peptide and is PEGylated.
  • the method to PEGylate the cupredoxin derived peptide may be NHS, reductive animation, malimid or epoxid, among others.
  • the cupredoxin derived peptides may be PEGylated on one or more lysine, cysteine, histidine, arginine, aspartic acid, glutamic acid, serine, threonine, or tyrosine, or the N-terminal amino group or the C-terminal carboxylic acid.
  • the cupredoxin derived peptides may be PEGylated on one or more lysines or N-terminal amino groups. In other embodiments, one or more lysine, cysteine, histidine, arginine, aspartic acid, glutamic acid, serine, threonine, or tyrosine residue are substituted into the cupredoxin derived peptides and are PEGylated. In other embodiments, the cupredoxin derived peptides may be PEGylated on one or more amino groups. In other embodiments, the cupredoxin derived peptides may be PEGylated in a random, non-site specific manner.
  • the cupredoxin derived peptides may have an average molecular weight of PEG-based polymers of about 200 daltons to about 100,000 daltons, about 2,000 daltons to about 20,000 daltons, or about 2,000 daltons to about 5,000 daltons.
  • the cupredoxin derived peptides may be comprised of one or more PEG molecules that is branched, specifically a branched PEG molecule that is about 50 kDa.
  • the cupredoxin derived peptides may comprise one or more linear PEG molecules, specifically a linear PEG molecule that is about 5 kDa.
  • the chemopreventive agent is a peptide that is a cupredoxin, or variant, truncation, structural equivalent, or derivative thereof that is a conjugate of Pep42, a cyclic 13-mer oligopeptide that specifically binds to glucose-regulated protein 78 (GRP78) and is internalized into cancer cells.
  • GRP78 glucose-regulated protein 78
  • cupredoxin or variant, structural equivalent, or derivative of cupredoxin may be conjugated with Pep42 pursuant to the synthesis methods disclosed in Yoneda et al, "A cell-penetrating peptidic GRP78 ligand for tumor cell-specific prodrug therapy," Bioorganic & Medicinal Chemistry Letters 18: 1632-1636 (2008), the disclosure of which is incorporated in its entirety herein.
  • the peptide is a structural equivalent of a cupredoxin or cytochrome. Examples of studies that determine significant structural homology between cupredoxins and cytochromes and other proteins include Toth et al. ⁇ Developmental Cell 1 :82-92 (2001)).
  • VAST p value from a structural comparison of a cupredoxin or cytochrome to the structural equivalent is less than about 10 "3 , less than about 10 "5 , or less than about 10 "7 .
  • significant structural homology between a cupredoxin or cytochrome and its structural equivalents are determined by using the DALI algorithm (Holm & Sander, J. MoI. Biol.
  • the DALI Z score for a pairwise structural comparison is at least about 3.5, at least about 7.0, or at least about 10.0.
  • the cupredoxin, or variant, derivative, truncation, or structural equivalent thereof has some of the pharmacologic activities of the P. aeruginosa azurin, and p28.
  • the cupredoxins and variants, derivatives and structural equivalents of cupredoxins that may inhibit prevent the development of premalignant lesions in mammalian cells, tissues or animals, and specifically but not limited to, mammary gland cells.
  • cupredoxins and variants, derivatives and structural equivalents of cupredoxins may have the ability to inhibit the development of mammalian premalignant lesions, and specifically but not limited to, melanoma, breast, pancreas, glioblastoma, astrocytoma, lung, colorectal, neck and head, bladder, prostate, skin and cervical cancer cells.
  • Inhibition of the development of cancer cells is any decrease, or lessening of the rate of increase, of the development of premalignant lesions that is statistically significant as compared to control treatments.
  • the cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof has some of the functional characteristics of the P. aeruginosa azurin or cytochrome.
  • the cupredoxin or cytochrome inhibits the growth of viral or bacterial infection, and specifically HIV infection in mammalian cells, more specifically in peripheral blood mononuclear cells infected with HIV.
  • the invention also provides for the variants, derivatives and structural equivalents of cupredoxin and cytochrome C 551 that retain the ability to inhibit the growth of viral or bacterial infection, and specifically HIV infection in mammalian cells.
  • the growth of HIV-I infection in the cells may be determined by measuring the change in the production of HIV-I p24 antigen in the cell culture supernatant by a commercial p24 enzyme immunoassay (PerkinElmer Life Sciences, Inc., Wellesley, Mass.)- Inhibition of a growth of infection is any decrease or lessening of the rate of increase of that infection that is statistically signification as compared to control treatments.
  • the peptide of the invention may also induce apoptosis in a mammalian cancer cell, more specifically a J774 cell.
  • the ability of a cupredoxin or other polypeptide to induce apoptosis may be observed by mitosensor Apo Alert confocal microscopy using a MITOSENSORTM APOLERTTM Mitochondrial Membrane Sensor kit (Clontech Laboratories, Inc., Palo Alto, California, U.S.A.), by measuring caspase-8, caspase-9 and caspase-3 activity using the method described in Zou et al. (J. Biol. Chem.
  • the peptide of the invention may also induce cellular growth arrest in a mammalian cancer cell, more specifically a J774 cell.
  • Cellular growth arrest can be determined by measuring the extent of inhibition of cell cycle progression, such as by the method found in Yamada et al. (PNAS 101 :4770-4775 (2004)).
  • the cupredoxin or cytochrome C 551 , or variant, derivative, truncation, or structural equivalent thereof inhibits cell cycle progression in a mammalian cancer cell, more specifically a J774 cell.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural thereof is administered to a patient for the concurrent treatment and/or prevention of two or more conditions such as interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papilloma virus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, he ⁇ es simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepati
  • IC intersti
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural thereof is administered to a patient for the concurrent treatment and/or prevention of two or more conditions selected from the group consisting of cancer, HIV, malaria and inappropriate angiogenesis.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be in a composition as a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from HIV, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, cancer or inappropriate angiogenesis.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be in a composition as a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from malaria, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as malaria, cancer or inappropriate angiogenesis.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be in a composition as a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from HIV, malaria or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, malaria or inappropriate angiogenesis.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be in a composition as a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from HIV, cancer or malaria or has a higher risk than the general population of acquiring a condition such as HIV, cancer or malaria.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be in a composition with, may be coadministered, or may be administered at about the same time as another drug.
  • Such drugs may include, but are not limited to an anti-malarial drug, an anti-HIV drug, an anti-cancer drug, or an anti-angiogenesis drug.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be in a composition that is administered by a mode of intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection and oral.
  • cupredoxins small blue copper proteins
  • electron transfer proteins (10-20 kDa) that participate in bacterial electron transfer chains or are of unknown function.
  • the copper ion is solely bound by the protein matrix.
  • a special distorted trigonal planar arrangement to two histidine and one cystine ligands around the copper gives rise to very peculiar electronic properties of the metal site and an intense blue color.
  • a number of cupredoxins have been crystallographically characterized at medium to high resolution.
  • cupredoxins in general have a low sequence homology but high structural homology.
  • Gough & Clothia Structure 12:917-925 (2004); De Rienzo et al, Protein Science 9:1439-1454 (2000).
  • amino acid sequence of azurin is 31% identical to that of auracyanin B, 16.3% to that of rusticyanin, 20.3 % to that of plastocyanin, and 17.3% to that of pseudoazurin. See Table 1.
  • the structural similarity of these proteins is more pronounced.
  • VAST p value for the comparison of the structure of azurin to auracyanin B is 10 "74 , azurin to rusticyanin is 10 "5 , azurin to plastocyanin is 10 "5 6 , and azurin to psuedoazurin is 10 "4 -1 .
  • cupredoxins possess an eight-stranded Greek key beta-barrel or beta-sandwich fold and have a highly conserved site architecture.
  • a prominent hydrophobic patch due to the presence of many long chain aliphatic residues such as methionines and leucines, is present around the copper site in azurins, amicyanins, cyanobacterial plastocyanins, cucumber basic protein and to a lesser extent, pseudoazurin and eukaryotic plastocyanins.
  • Hydrophobic patches are also found to a lesser extent in stellacyanin and rusticyanin copper sites, but have different features.
  • Table 1 Sequence and structure alignment of azurin (IJZG) from P. aeruginosa to other proteins using VAST algorithm.
  • VAST p value is a measure of the significance of the comparison, expressed as a probability. For example, if the p value is 0.001, then the odds are 1000 to 1 against seeing a match of this quality by pure chance.
  • the p value from VAST is adjusted for the effects of multiple comparisons using the assumption that there are 500 independent and unrelated types of domains in the MMDB database. The p value shown thus corresponds to the p value for the pairwise comparison of each domain pair, divided by 500.
  • VAST structure-similarity score The VAST structure-similarity score. This number is related to the number of secondary structure elements superimposed and the quality of that superposition. Higher VAST scores correlate with higher similarity.
  • RMSD The root mean square superposition residual in Angstroms. This number is calculated after optimal superposition of two structures, as the square root of the mean square distances between equivalent C-alpha atoms. Note that the RMSD value scales with the extent of the structural alignments and that this size must be taken into consideration when using RMSD as a descriptor of overall structural similarity. 5 C. elegcms major sperm protein proved to be an ephrin antagonist in oocyte maturation (Kuwabara, 2003 "The multifaceted C. elegans major sperm protein: an ephrin signaling antagonist in oocyte maturation" Genes and Development, 17:155-161.
  • the azurins are copper containing proteins of 128 amino acid residues which belong to the family of cupredoxins involved in electron transfer in plants and certain bacteria.
  • the azurins include those from P. aeruginosa (PA) (SEQ ID NO: 1), A. xylosoxidans, and A. denitrificans (SEQ ID NO: 6).
  • PA P. aeruginosa
  • SEQ ID NO: 6 A. xylosoxidans
  • SEQ ID NO: 6 A. denitrificans
  • the amino acid sequence identity between the azurins varies between 60-90%, these proteins showed a strong structural homology. All azurins have a characteristic ⁇ -sandwich with Greek key motif and the single copper atom is always placed at the same region of the protein.
  • azurins possess an essentially neutral hydrophobic patch surrounding the copper site. Id.
  • the plastocyanins are soluble proteins of cyanobacteria, algae and plants that contain one molecule of copper per molecule and are blue in their oxidized form. They occur in the chloroplast, where they function as electron carriers. Since the determination of the structure of poplar plastocyanin in 1978, the structure of algal (Scenedesmus, Enteromorpha,
  • Chlamydomonas and plant (French bean) plastocyanins has been determined either by crystallographic or NMR methods, and the poplar structure has been refined to 1.33 A resolution.
  • SEQ ID NO: 2 shows the amino acid sequence of plastocyanin from Phormidium laminosum, a thermophilic cyanobacterium. Despite the sequence divergence among plastocyanins of algae and vascular plants (e.g., 62% sequence identity between the Chlamydomonas and poplar proteins), the three-dimensional structures are conserved (e.g., 0.76 A rms deviation in the C alpha positions between the Chlamydomonas and Poplar proteins).
  • Structural features include a distorted tetrahedral copper binding site at one end of an eight-stranded antiparallel beta-barrel, a pronounced negative patch, and a flat hydrophobic surface.
  • the copper site is optimized for its electron transfer function, and the negative and hydrophobic patches are proposed to be involved in recognition of physiological reaction partners.
  • Chemical modification, cross-linking, and site-directed mutagenesis experiments have confirmed the importance of the negative and hydrophobic patches in binding interactions with cytochrome f , and validated the model of two functionally significant electron transfer paths involving plastocyanin.
  • One putative electron transfer path is relatively short (approximately 4 A) and involves the solvent- exposed copper ligand His-87 in the hydrophobic patch, while the other is more lengthy (approximately 12-15 A) and involves the nearly conserved residue Tyr-83 in the negative patch, Redinbo et ah, J. Bioenerg. Biomembr. 26:49-66 (1994).
  • Rusticyanins are blue-copper containing single-chain polypeptides obtained from a
  • Thiobacillus (now called Acidithiobacillus).
  • the X-ray crystal structure of the oxidized form of the extremely stable and highly oxidizing cupredoxin rusticyanin from Thiobacillus ferrooxidans (SEQ ID NO: 3) has been determined by multi wavelength anomalous diffraction and refined to 1.9A resolution.
  • the rusticyanins are composed of a core beta- sandwich fold composed of a six- and a seven-stranded b-sheet.
  • the copper ion is coordinated by a cluster of four conserved residues (His 85, Cysl38, Hisl43, Met 148) arranged in a distorted tetrahedron. Walter, R.L. et al., J. MoI. Biol., vol. 263, pp- 730-51 (1996).
  • the pseudoazurins are a family of blue-copper containing single-chain polypeptide.
  • the amino acid sequence of pseudoazurin obtained from Achromobacter cycloclastes is shown in SEQ ID NO: 4.
  • the X-ray structure analysis of pseudoazurin shows that it has a similar structure to the azurins although there is low sequence homology between these proteins.
  • azurins In the mid-peptide region azurins contain an extended loop, shortened in the pseudoazurins, which forms a flap containing a short ⁇ -helix.
  • the only major differences at the copper atom site are the conformation of the MET side-chain and the Met-S copper bond length, which is significantly shorter in pseudoazurin than in azurin.
  • the proteins identifiable as phytocyanins include, but are not limited to, cucumber basic protein, stellacyanin, mavicyanin, umecyanin, a cucumber peeling cupredoxin, a putative blue copper protein in pea pods, and a blue copper protein from Arabidopsis thaliana.
  • cucumber basic protein and the pea-pod protein the axial methionine ligand normally found at blue copper sites is replaced by glutamine.
  • Auracyanin Three small blue copper proteins designated auracyanin A, auracyanin B-I, and auracyanin B-2 have been isolated from the thermophilic green gliding photosynthetic bacterium Chloroflexus aurantiacus. The two B forms are glycoproteins and have almost identical properties to each other, but are distinct from the A form.
  • the sodium dodecyl sulfate-polyacrylamide gel electrophoresis demonstrates apparent monomer molecular masses as 14 (A), 18 (B-2), and 22 (B-I) kDa.
  • auracyanin A The amino acid sequence of auracyanin A has been determined and showed auracyanin A to be a polypeptide of 139 residues. (Van Dreissche et ah, Protein Science 8:947-957 (1999).) His58, Cysl23, Hisl28, and Metl32 are spaced in a way to be expected if they are the evolutionary conserved metal ligands as in the known small copper proteins plastocyanin and azurin. Secondary structure prediction also indicates that auracyanin has a general beta-barrel structure similar to that of azurin from Pseudomonas aeruginosa and plastocyanin from poplar leaves. However, auracyanin appears to have sequence characteristics of both small copper protein sequence classes.
  • the overall similarity with a consensus sequence of azurin is roughly the same as that with a consensus sequence of plastocyanin, namely 30.5%.
  • the N-terminal sequence region 1-18 of auracyanin is remarkably rich in glycine and hydroxy amino acids. Id. See exemplary amino acid sequence SEQ ID NO: 14 for chain A of auracyanin from Chloroflexus aurantiacus (NCBI Protein Data Bank Accession No. AAMl 2874).
  • the auracyanin B molecule has a standard cupredoxin fold.
  • the crystal structure of auracyanin B from Chloroflexus aurantiacus has been studied. (Bond et ah, J. MoI. Biol. 306:47-67 (2001).) With the exception of an additional N-terminal strand, the molecule is very similar to that of the bacterial cupredoxin, azurin.
  • one of the Cu ligands lies on strand 4 of the polypeptide, and the other three lie along a large loop between strands 7 and 8.
  • the Cu site geometry is discussed with reference to the amino acid spacing between the latter three ligands.
  • the crystallographically characterized Cu-binding domain of auracyanin B is probably tethered to the periplasmic side of the cytoplasmic membrane by an N-terminal tail that exhibits significant sequence identity with known tethers in several other membrane-associated electron-transfer proteins.
  • the amino acid sequences of the B forms are presented in McManus et al. (J Biol Chem. 267:6531-6540 (1992).). See exemplary amino acid sequence SEQ ID NO: 15 for chain B of auracyanin from Chloroflexus aurantiacus (NCBI Protein Data Bank Accession No. IQHQA).
  • Stellacyanins are a subclass of phytocyanins, a ubiquitous family of plant cupredoxins.
  • An exemplary sequence of a stellacyanin is included herein as SEQ ID NO: 13.
  • the crystal structure of umecyanin, a stellacyanin from horseradish root (Koch et al, J. Am. Chem. Soc. 127:158-166 (2005)) and cucumber stellacyanin (Hart el al., Protein Science
  • the protein has an overall fold similar to the other phytocyanins.
  • the ephrin B2 protein ectodomain tertiary structure bears a significant similarity to stellacyanin. (Toth et al, Developmental Cell 1 :83-92 (2001).)
  • An exemplary amino acid sequence of a stellacyanin is found in the National Center for Biotechnology Information Protein Data Bank as Accession No . 1 JER, SEQ ID NO : 13.
  • An exemplary amino acid sequence from a cucumber basic protein is included herein as SEQ ID NO: 16.
  • the crystal structure of the cucumber basic protein (CBP), a type 1 blue copper protein, has been refined at 1.8 A resolution.
  • the molecule resembles other blue copper proteins in having a Greek key beta-barrel structure, except that the barrel is open on one side and is better described as a "beta-sandwich” or "beta-taco”.
  • the ephrinB2 protein ectodomain tertiary structure bears a high similarity (rms deviation 1.5A for the 50 ⁇ carbons) to the cucumber basic protein.
  • a disulphide link, (Cys52)-S-S-(Cys85) appears to play an important role in stabilizing the molecular structure.
  • the polypeptide fold is typical of a sub-family of blue copper proteins (phytocyanins) as well as a non-metalloprotein, ragweed allergen Ra3, with which CBP has a high degree of sequence identity.
  • the proteins currently identifiable as phytocyanins are CBP, stellacyanin, mavicyanin, umecyanin, a cucumber peeling cupredoxin, a putative blue copper protein in pea pods, and a blue copper protein from Arabidopsis thaliana.
  • CBP CBP
  • stellacyanin mavicyanin
  • umecyanin a cucumber peeling cupredoxin
  • a putative blue copper protein in pea pods a putative blue copper protein in pea pods
  • a blue copper protein from Arabidopsis thaliana In all except CBP and the pea-pod protein, the axial methionine ligand normally found at blue copper sites is replaced by glutamine.
  • An exemplary sequence for cucumber basic protein is found in NCBI Protein Data Bank Accession No. 2CBP, SEQ ID NO: 16.
  • Cytochrome C 551 from P. aeruginosa is a monomeric redox protein of 82 amino-acid residues (SEQ ID NO: 21), involved in dissimilative denitrification as the physiological electron donor of nitrite reductase.
  • the functional properties of Pa-C551 have been extensively investigated. The reactions with non-physiological small inorganic redox reactants and with other macromolecules, like blue copper proteins, eukaryotic cytochrome c and the physiological partner nitrite reductase have provided a test for protein-protein electron transfer.
  • Pa-C551 which is a member of bacterial class I cytochromes, shows a single low-spin heme with His-Met ligation and the typical polypeptide fold which however leaves the edges of pyrrole rings II and III of the heme exposed (Cutruzzola et al, J. Morgan. Chem. 88:353-61 (2002)).
  • the lack of a 20-residue omega loop, present in the mammalian class I cytochromes, causes further exposure of the heme edge at the level of propionate 13.
  • the distribution of charged residues on the surface of Pa-C551 is very anisotropic: one side is richer in acidic residues whereas the other displays a ring of positive side chains, mainly lysines, located at the border of a hydrophobic patch which surrounds the heme crevice.
  • This patch comprises residues Glyll, VaI 13, Alal4, Met22, Val23, Pro58, Ile59, Pro60, Pro62, Pro63 and Ala65.
  • the anisotropic charge distribution leads to a large dipolar moment which is important for electron transfer complex formation.
  • the charge distribution described above for Pa-C551 has been reported for other electron transfer proteins and their electron acceptors.
  • the cytochrome c-type domain has a fold consisting of a series of alpha helices and reverse turns that serve to envelop the covalently bound haem within a hydrophobic pocket.
  • This domain can be found in monodomain cytochrome c proteins, such as cytochrome c6, cytochrome C 552 , cytochrome c 459 and mitochondrial cytochrome c.
  • the cytochrome c-type domain occurs in a number of other proteins, such as in cytochrome cdl -nitrite reductase as the N-terminal haem c domain, in quinoprotein alcohol dehydrogenase as the C-terminal domain, in Quinohemoprotein amine dehydrogenase A chain as domains 1 and 2, and in the cytochrome bcj complex as the cytochrome be t domain.
  • Structural analysis with VAST algorithm cytochrome C 551 from Pseudomonas aeruginosa as a query
  • showed significant structural neighbors P values between 10 "1 to 10 "4 5 ) only for cytochromes.
  • the invention provides methods to administer to a patient the compositions comprising cupredoxin or cytochrome, and variants, derivatives and structural equivalents of cupredoxin or cytochrome.
  • the invention provides methods to administer to a patient a composition comprising at least one peptide, or at least two peptides that are a cupredoxin, cytochrome and variants, derivatives and structural equivalents of cupredoxin or cytochrome. More specifically, the invention provides methods to administer to a human a composition comprising at least one peptide that is a cupredoxin, cytochrome and variants, derivatives and structural equivalents of cupredoxin or cytochrome.
  • the invention provides methods to administer to a patient compositions comprising cupredoxin or cytochrome and variants, derivatives and structural equivalents of cupredoxin or cytochrome, and their use to concurrently treat and/or prevent two or more conditions in a patient.
  • the methods may utilize pharmaceutical compositions for the administration to a patient.
  • the invention provides methods for the concurrent prevention and/or treatment of two or more conditions such as interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papillomavirus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus,
  • IC
  • Cupredoxin family specifically azurin from Pseudomonas aeruginosa, are promising compounds for therapeutic and preventative treatment of numerous conditions. Such conditions may include, but are not limited to HIV, malaria, cancer and inappropriate angiogenesis.
  • two redox proteins elaborated by P. aeruginosa the cupredoxin azurin and cytochrome Cs S1 (Cyt Cs 51 ), both enter J774 cells and show significant cytotoxic activity towards the human cancer cells as compared to normal cells.
  • Zaborina et ah Microbiology 146: 2521-2530 (2000).
  • Azurin can also enter human melanoma UISO-Mel-2 or human breast cancer MCF-7 cells. Yamada et al, PNAS
  • azurin from P. aeruginosa preferentially enters J774 murine reticulum cell sarcoma cells, forms a complex with and stabilizes the tumor suppressor protein p53, enhances the intracellular concentration of p53, and induces apoptosis .
  • Azurin also caused a significant increase of apoptosis in human osteosarcoma cells as compared to noncancerous cells.
  • the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, wherein the patient has at least one "high risk feature.”
  • "High risk features” may be factors of the patient that increase the risk of a patient developing one or more conditions or where the patient has a higher risk than the general population.
  • the increased risk may be due to numerous variables or factors such as, but not limited to, environmental and behavioral factors, increased risk caused from other conditions, and genetic predisposition.
  • an HIV infected patient is associated with an increased risk of acquiring large cell lymphoma or Kaposi's sarcoma.
  • the Merck Manual of Diagnosis and Therapy (Beers et al., 18 edition, Merck Research Laboratories, 2006).
  • a female patient that acquires human papillomavirus has an increased risk of acquiring cervical carcinoma. Id.
  • Environmental factors may include, but are not limited to, a patient's lifestyle, eating habits and/or geographic location.
  • a patient's lifestyle For example, co-infections with HIV and malaria are very common in many areas of the world, and in particular sub-Saharan Africa
  • Behavioral factors may include actions by the patient that predispose a patient to many conditions.
  • the risk of acquiring cancer and heart disease may be increased due to factors such as, but not limited to, smoking, diet, alcohol consumption, hormone replacement therapy and higher body mass index.
  • Genetic predisposition may play a factor in a patient acquiring numerous conditions. For example, it is known that when a person carries a particular cystic fibrosis transmembrane regulator (CFTK) mutation, that person has a higher risk for cystic fibrosis and pancreatic cancer.
  • CFTK cystic fibrosis transmembrane regulator
  • genetic factors that predispose a patient to various forms of cancer include, but are not limited to, a family history of cancer, gene carrier status of BRCAl and BRCA2, prior history of breast neoplasia, familial adenomatous polyposis (FAP), hereditary nonpolyposis colorectal cancer (HNPCC), red or blond hair and fair-skinned phenotype, xeroderma pigmentosum, and ethnicity.
  • FAP familial adenomatous polyposis
  • HNPCC hereditary nonpolyposis colorectal cancer
  • red or blond hair and fair-skinned phenotype xeroderma pigmentosum
  • ethnicity a genetic factors that predispose a patient to various forms of cancer
  • Patients with high risk features, such as higher risk to develop cancer than the general population may be patients with premalignant lesions, and patients that have been cured of their initial cancer or definitively treated for their premalignant lesions. See generally Ts
  • patients at a higher risk of developing cancer may be determined by the use of various risk models that have been developed for certain kinds of cancer.
  • patients predisposed to breast cancer may be determined using the Gail risk model, or the Claus model, among others. See Gail et al, J Natl Cancer Inst 81 :1879-1886 (1989); Cuzick, Breast 12:405-411 (2003); Huang et al, Am J Epidemiol 151 :703-714 (2000).
  • the methods may utilize compositions to be administered to a patient for the concurrent treatment and/or prevention of two or more conditions where the patient has a higher risk than the general population of acquiring a condition.
  • Such conditions may include, but are not limited to, cancer, HIV, malaria or inappropriate angiogenesis.
  • the methods may comprise a composition including a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from HIV, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, cancer or inappropriate angiogenesis.
  • the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from malaria, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as malaria, cancer or inappropriate angiogenesis.
  • the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from HIV, malaria or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, malaria or inappropriate angiogenesis.
  • the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from HIV, cancer or malaria or has a higher risk than the general population of acquiring a condition such as HIV, cancer or malaria.
  • compositions comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be administered to the patient by many routes and in many regimens that will be well known to those in the art.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof is administered intravenously, intramuscularly, subcutaneously, topically, orally, or by inhalation.
  • the methods may utilize compositions that additionally comprise another drug.
  • the additional drug may be an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
  • the methods may comprise co-administering to a patient one unit dose of a composition comprising a cupredoxin, cytochrome or a variant, derivative, truncation, or structural equivalent of cupredoxin or cytochrome and one unit dose of a composition comprising another drug, in either order, administered at about the same time, or within about a given time following the administration of the other, for example, about one minute to about 60 minutes following the administration of the other drug, or about 1 hour to about 12 hours following the administration of the other drug.
  • the other drug may be, but is not limited to an anti-malarial drug, an anti-HIV drug, an anti- cancer drug, and an anti-angiogenesis drug.
  • Anti-malarial drugs of interest include, but are not limited to, proguanil, chlorproguanil, trimethoprim, chloroquine, mefloquine, lumefantrine, atovaquone, pyrimethamine-sulfadoxine, pyrimethamine-dapsone, halofantrine, quinine, quinidine, amodiaquine, amopyroquine, sulphonamides, artemisinin, arteflene, artemether, artesunate, primaquine, pyronaridine, proguanil, chloroquine, mefloquine, pyrimethamine-sulfadoxine, pyrimethamine-dapsone, halofantrine, quinine, proguanil, chloroquine, mefloquine, 1,16- hexadecamethylenebis(N-methylpyrrolidinium)dibromide, and combinations thereof.
  • Anti-HIV drugs include, but are not limited to, reverse transcriptase inhibitors: AZT (zidovudine [Retrovir]), ddC (zalcitabine [Hivid], dideoxyinosine), d4T (stavudine [Zerit]), and 3TC (lamivudine [Epivir]), nonnucleoside reverse transcriptase inhibitors (NNRTIS): delavirdine (Rescriptor) and nevirapine (Viramune), protease inhibitors: ritonavir (Norvir), a lopinavir and ritonavir combination (Kaletra), saquinavir (Invirase), indinavir sulphate (Crixivan), amprenavir (Agenerase), and nelfinavir (Viracept).
  • AZT zidovudine [Retrovir]
  • ddC zalcitabine [Hivid]
  • Anti-cancer and/or anti-angiogenesis drugs of interest include, but are not limited to, tamoxifen, aromatase inhibitors such as letrozole and anastrozole (Arimidex j, retinoids such as N-[4-hydroxyphenyl] retinamide (4-HPR, fenretinide), nonsteriodal anti-inflammatory agents (NSAIDs) such as aspirin and sulindac, celecoxib (COX-2 inhibitor), defluoromethylornithing (DFMO), ursodeoxycholic acid, 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors, EKI-785 (EGFR inhibitor), bevacizumab (antibody to VEGF-receptor), cetuximab (antibody to EGFR), retinol such as vitamin A, beta-carotene, 13-cis retinoic acid, isotretinoin and retinyl palmitate, ⁇ -tocopherol
  • compositions Comprising Cupredoxin, Or Variant, Derivative, Truncation, Or Structural Equivalent Thereof
  • compositions comprising cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalents thereof, can be manufactured in any conventional manner, e.g., by conventional mixing, dissolving, granulating, dragee-making, emulsifying, encapsulating, entrapping, or lyophilizing processes.
  • the substantially pure or pharmaceutical grade cupredoxin, cytochrome or variants, derivatives and structural equivalents thereof can be readily combined with a pharmaceutically acceptable carrier well- known in the art.
  • Such carriers enable the preparation to be formulated as a tablet, pill, dragee, capsule, liquid, gel, syrup, slurry, suspension, and the like.
  • Suitable carriers or excipients can also include, for example, fillers and cellulose preparations.
  • Other excipients can include, for example, flavoring agents, coloring agents, detackif ⁇ ers, thickeners, and other acceptable additives, adjuvants, or binders.
  • the pharmaceutical preparation is substantially free of preservatives. In other embodiments, the pharmaceutical preparation may contain at least one preservative. General methodology on pharmaceutical dosage forms is found in Ansel et ah, Pharmaceutical Dosage Forms and Drug Delivery Systems (Lippencott Williams & Wilkins, Baltimore MD (1999)).
  • composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof used in the invention may be administered in a variety of ways, including by injection (e.g., intradermal, subcutaneous, intramuscular, intraperitoneal and the like), by inhalation, by topical administration, by suppository, by using a transdermal patch or by mouth.
  • injection e.g., intradermal, subcutaneous, intramuscular, intraperitoneal and the like
  • topical administration e.g., by topical administration, by suppository, by using a transdermal patch or by mouth.
  • General information on drug delivery systems can be found in Ansel et al, id..
  • the composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be formulated and used directly as injectables, for subcutaneous and intravenous injection, among others.
  • the injectable formulation in particular, can advantageously be used to prevent and/or treat patients with more than one condition.
  • the composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can also be taken orally after mixing with protective agents such as polypropylene glycols or similar coating agents.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be formulated in aqueous solutions, specifically in physiologically compatible buffers such as Hanks solution, Ringer's solution, or physiological saline buffer.
  • the solution may contain formulatory agents such as suspending, stabilizing and/or dispersing agents.
  • the cupredoxin or variant, derivative, truncation, or structural equivalent thereof may be in powder form for constitution with a suitable vehicle, e.g. , sterile pyrogen-free water, before use.
  • the pharmaceutical composition does not comprise an adjuvant or any other substance added to enhance the immune response stimulated by the peptide.
  • the pharmaceutical composition comprises a substance that inhibits an immune response to the peptide.
  • the intravenous fluids for use administering the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be composed of crystalloids or colloids.
  • Crystalloids as used herein are aqueous solutions of mineral salts or other water-soluble molecules.
  • Colloids as used herein contain larger insoluble molecules, such as gelatin.
  • Intravenous fluids may be sterile.
  • Crystalloid fluids that may be used for intravenous administration include but are not limited to, normal saline (a solution of sodium chloride at 0.9% concentration), Ringer's lactate or Ringer's solution, and a solution of 5% dextrose in water sometimes called D5W, as described in Table 2.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be delivered in the form of an aerosol spray from pressurized packs or a nebulizer with the use of a suitable propellant, e.g., dichlorodifluoromethane, trichlorofluoromethane, carbon dioxide or other suitable gas.
  • a suitable propellant e.g., dichlorodifluoromethane, trichlorofluoromethane, carbon dioxide or other suitable gas.
  • the dosage unit may be determined by providing a valve to deliver a metered amount.
  • Capsules and cartridges of, e.g., gelatin, for use in an inhaler or insufflator may be formulated containing a powder mix of the proteins and a suitable powder base such as lactose or starch.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be formulated as solutions, gels, ointments, creams, jellies, suspensions, and the like, as are well known in the art.
  • administration is by means of a transdermal patch.
  • cupredoxin, cytochrome or variants and derivatives thereof compositions may also be formulated in compositions containing conventional suppository bases.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be readily formulated by combining the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof with pharmaceutically acceptable carriers well known in the art.
  • a solid carrier such as mannitol, lactose, magnesium stearate, and the like may be employed; such carriers enable the cupredoxin and variants, derivatives or structural equivalent thereof to be formulated as tablets, pills, dragees, capsules, liquids, gels, syrups, slurries, suspensions and the like, for oral ingestion by a subject to be treated.
  • suitable excipients include fillers such as sugars, cellulose preparation, granulating agents, and binding agents.
  • sustained-release formulations that include a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof allow for the release of cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof over extended periods of time, such that without the sustained release formulation, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof would be cleared from a subject's system, and/or degraded by, for example, proteases and simple hydrolysis before eliciting or enhancing a therapeutic effect.
  • compositions of the invention can be extended or optimized by several methods well known to those in the art, including but not limited to, circularized peptides (Monk et al, BioDrugs 19(4):261-78, (2005); DeFreest et al., J. Pept. Res. 63(5):409-19 (2004)), D,L-peptides (diastereomer), (Futaki et al, J. Biol. Chem. Feb 23;276(8):5836-40 (2001); Papo et al, Cancer Res. 64(16):5779-86 (2004); Miller et al, Biochem. Pharmacol.
  • the pharmaceutical composition includes carriers and excipients (including but not limited to buffers, carbohydrates, mannitol, proteins, polypeptides or amino acids such as glycine, antioxidants, bacteriostats, chelating agents, suspending agents, thickening agents and/or preservatives), water, oils, saline solutions, aqueous dextrose and glycerol solutions, other pharmaceutically acceptable auxiliary substances as required to approximate physiological conditions, such as buffering agents, tonicity adjusting agents, wetting agents and the like.
  • suitable carrier known to those of ordinary skill in the art may be employed to administer the compositions of this invention, the type of carrier will vary depending on the mode of administration.
  • Biodegradable microspheres may also be employed as carriers for the pharmaceutical compositions of this invention. Suitable biodegradable microspheres are disclosed, for example, in U.S. Patent Nos. 4,897,268; 5,075,109; 5,928,647; 5,811,128; 5,820,883; 5,853,763; 5,814,344 and 5,942,252.
  • the pharmaceutical compositions may be sterilized by conventional, well-known sterilization techniques, or may be sterile filtered.
  • the resulting aqueous solutions may be packaged for use as is, or lyophilized, the lyophilized preparation being combined with a sterile solution prior to administration.
  • cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be administered formulated as pharmaceutical compositions and administered by any suitable route, for example, by oral, buccal, inhalation, sublingual, rectal, vaginal, transurethral, nasal, topical, percutaneous, i.e., transdermal or parenteral (including intravenous, intramuscular, subcutaneous and intracoronary) or vitreous administration.
  • the pharmaceutical formulations thereof can be administered in any amount effective to achieve its intended purpose. More specifically, the composition is administered in a therapeutically effective amount. In specific embodiments, the therapeutically effective amount is generally from about 0.01-20 mg/day/kg of body weight.
  • the compounds comprising cupredoxin or variant, derivative, truncation, or structural equivalent thereof are useful for the prevention and/or treatment of more than one condition, alone or in combination with other active agents.
  • the appropriate dosage will, of course, vary depending upon, for example, the compound of cupredoxin or variant, derivative, truncation, or structural equivalent thereof employed, the host, the mode of administration and the nature and severity of the potential cancer. However, in general, satisfactory results in humans are indicated to be obtained at daily dosages from about 0.01-20 mg/kg of body weight.
  • An indicated daily dosage in humans is in the range from about 0.7 mg to about 1400 mg of a compound of cupredoxin or variant, derivative, truncation, or structural equivalent thereof conveniently administered, for example, in daily doses, weekly doses, monthly doses, and/or continuous dosing.
  • Daily doses can be in discrete dosages from 1 to 12 times per day.
  • doses can be administered every other day, every third day, every fourth day, every fifth day, every sixth day, every week, and similarly in day increments up to 31 days or over.
  • dosing can be continuous using patches, i.v. administration and the like.
  • the exact formulation, route of administration, and dosage is determined by the attending physician in view of the patient's condition. Dosage amount and interval can be adjusted individually to provide plasma levels of the active cupredoxin or variant, derivative, truncation, or structural equivalent thereof which are sufficient to maintain therapeutic effect.
  • the desired cupredoxin or variant, derivative, truncation, or structural equivalent thereof is administered in an admixture with a pharmaceutical carrier selected with regard to the intended route of administration and standard pharmaceutical practice.
  • the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof is delivered as DNA such that the polypeptide is generated in situ.
  • the DNA is "naked," as described, for example, in Ulmer et al., (Science 259:1745-1749 (1993)) and reviewed by Cohen (Science 259:1691-1692 (1993)).
  • the uptake of naked DNA may be increased by coating the DNA onto a carrier, e.g., biodegradable beads, which are then efficiently transported into the cells.
  • the DNA may be present within any of a variety of delivery systems known to those of ordinary skill in the art, including nucleic acid expression systems, bacterial and viral expression systems. Techniques for incorporating DNA into such expression systems are well known to those of ordinary skill in the art. See, e.g. , WO90/11092, WO93/24640, WO 93/17706, and U.S. Pat. No. 5,736,524.
  • Vectors used to shuttle genetic material from organism to organism, can be divided into two general classes: Cloning vectors are replicating plasmid or phage with regions that are essential for propagation in an appropriate host cell and into which foreign DNA can be inserted; the foreign DNA is replicated and propagated as if it were a component of the vector.
  • An expression vector (such as a plasmid, yeast, or animal virus genome) is used to introduce foreign genetic material into a host cell or tissue in order to transcribe and translate the foreign DNA, such as the DNA of a cupredoxia
  • the introduced DNA is operably-linked to elements such as promoters that signal to the host cell to highly transcribe the inserted DNA.
  • Some promoters are exceptionally useful, such as inducible promoters that control gene transcription in response to specific factors. Operably-linking a cupredoxin and variants and derivatives thereof polynucleotide to an inducible promoter can control the expression of the cupredoxin and variants and derivatives thereof in response to specific factors.
  • Examples of classic inducible promoters include those that are responsive to ⁇ -interferon, heat shock, heavy metal ions, and steroids such as glucocorticoids (Kaufman, Methods Enzymol. 185:487-511 (1990)) and tetracycline.
  • desirable inducible promoters include those that are not endogenous to the cells in which the construct is being introduced, but, are responsive in those cells when the induction agent is exogenously supplied.
  • useful expression vectors are often plasmids.
  • other forms of expression vectors such as viral vectors (e.g., replication defective retroviruses, adenoviruses and adeno-associated viruses) are contemplated
  • Vector choice is dictated by the organism or cells being used and the desired fate of the vector.
  • vectors comprise signal sequences, origins of replication, marker genes, polylinker sites, enhancer elements, promoters, and transcription termination sequences. The exact formulation, route of administration, and dosage is determined by the attending physician in view of the patient's condition.
  • Dosage amount and interval can be adjusted individually to provide plasma levels of the active cupredoxin and/or cytochrome and variants and derivatives thereof which are sufficient to treat the patient and/or maintain therapeutic effect.
  • the desired cupredoxin and/or cytochrome and variants and derivatives thereof can be administered in an admixture with a pharmaceutical carrier selected with regard to the intended route of administration and standard pharmaceutical practice.
  • compositions used in accordance with the present invention can be formulated in a conventional manner using one or more physiologically acceptable carriers comprising excipients and auxiliaries that facilitate processing of the cupredoxin and/or cytochrome and variants and derivatives thereof, active agents, for inhibiting or stimulating the secretion of cupredoxin and/or cytochrome and variants and derivatives thereof, or a mixture thereof into preparations which can be used therapeutically.
  • Kits Comprising Cupredoxin, And/Or Cytochrome, Or Variant, Derivative, Truncation, Or Structural Equivalent Thereof
  • the invention provides regimens or kits comprising one or more of the following in a package or container: (1) a pharmacologically active composition comprising at least one cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof; (2) an additional chemopreventive drug, (3) apparatus to administer the biologically active composition to the patient, such as a syringe, nebulizer etc..
  • kits When a kit is supplied, the different components of the composition may be packaged in separate containers, if appropriate, and admixed immediately before use. Such packaging of the components separately may permit long-term storage without losing the active components' functions.
  • the reagents included in the kits can be supplied in containers of any sort such that the life of the different components are preserved and are not adsorbed or altered by the materials of the container.
  • sealed glass ampoules may contain lyophilized cupredoxin and variants, derivatives and structural equivalents thereof, or buffers that have been packaged under a neutral, non-reacting gas, such as nitrogea
  • Ampoules may consist of any suitable material, such as glass, organic polymers, such as polycarbonate, polystyrene, etc., ceramic, metal or any other material typically employed to hold similar reagents.
  • suitable containers include simple bottles that may be fabricated from similar substances as ampoules, and envelopes, that may comprise foil-lined interiors, such as aluminum or an alloy.
  • Other containers include test tubes, vials, flasks, bottles, syringes, or the like.
  • Containers may have a sterile access port, such as a bottle having a stopper that can be pierced by a hypodermic injection needle.
  • Other containers may have two compartments that are separated by a readily removable membrane that upon removal permits the components to be mixed.
  • Removable membranes may be glass, plastic, rubber, etc.
  • Kits may also be supplied with instructional materials. Instructions may be printed on paper or other substrate, and/or may be supplied as an electronic-readable medium, such as a floppy disc, CD-ROM, DVD-ROM, Zip disc, videotape, audiotape, flash memory device etc. Detailed instructions may not be physically associated with the kit; instead, a user may be directed to an internet web site specified by the manufacturer or distributor of the kit, or supplied as electronic mail.
  • Cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalents thereof may be chemically modified or genetically altered to produce variants and derivatives as explained above. Such variants and derivatives may be synthesized by standard techniques.
  • allelic variants of cupredoxin changes can be introduced by mutation into cupredoxin coding sequence that incur alterations in the amino acid sequences of the encoded cupredoxin that do not significantly alter the ability of cupredoxin to inhibit the development of premalignant lesions.
  • non-essential amino acid residue is a residue that can be altered from the wild-type sequences of the cupredoxin without altering pharmacologic activity, whereas an "essential" amino acid residue is required for such pharmacologic activity.
  • amino acid residues that are conserved among the cupredoxins are predicted to be particularly non-amenable to alteration, and thus "essential.”
  • amino acids for which conservative substitutions that do not change the pharmacologic activity of the polypeptide can be made are well known in the art. Useful conservative substitutions are shown in Table 3, "Preferred substitutions.” Conservative substitutions whereby an amino acid of one class is replaced with another amino acid of the same type fall within the scope of the invention so long as the substitution does not materially alter the pharmacologic activity of the compound.
  • Non-conservative substitutions that affect (1) the structure of the polypeptide backbone, such as a ⁇ -sheet or ⁇ -helical conformation, (2) the charge, (3) hydrophobicity, or (4) the bulk of the side chain of the target site can modify the pharmacologic activity.
  • Residues are divided into groups based on common side-chain properties as denoted in Table 4.
  • Non-conservative substitutions entail exchanging a member of one of these classes for another class. Substitutions may be introduced into conservative substitution sites or more specifically into non-conserved sites.
  • the variant polypeptides can be made using methods known in the art such as oligonucleotide-mediated (site-directed) mutagenesis, alanine scanning, and PCR mutagenesis.
  • Site-directed mutagenesis Carter, Biochem J. 237:1-7 (1986); Zoller and Smith, Methods Enzymol. 154:329-350 (1987)
  • cassette mutagenesis restriction selection mutagenesis
  • restriction selection mutagenesis Wells et al, Gene 34:315-323 (1985)
  • other known techniques can be performed on the cloned DNA to produce the cupredoxin variant DNA.
  • cupredoxins and cytochrome can also be used to create variant cupredoxin and cytochrome to be used in the methods of the invention.
  • the C 112D and M44KM64E mutants of azurin are known to have cytotoxic and growth arresting activity that is different from the native azurin, and such altered activity can be useful in the treatment and/or prevention methods of the present invention.
  • Example 1 Entry of p28 into human umbilical vein endothelial cells.
  • p28 was labeled with 20 ⁇ M Alexafluor ® 568 (Molecular Probes, Eugene, OR). Indicated cell lines were cultured on cell culture coated cover slips overnight at 37°C. Pre- warmed media containing labeled peptide was added at indicated concentrations. After incubation with the labeled peptide, the cover slips were washed 3X with PBS and fixed in formalin for 5 minutes. Cover slips were then mounted in media containing 1.5 ⁇ g ml "1 DAPI for nuclear staining (VECTASHIELD ® , Vector Laboratories, Burlingame, CA).
  • p28 effectively entered malignant cell lines originating from melanoma, breast, pancreas, glioblastoma, astrocytoma, and lung (Fig. IA).
  • p28 was also efficiently entered HUVEC cells (Fig. 1C). No significant entry was observed in other "normal" cell lines originating from skin fibroblasts, breast and pancreas Fig. IB). Therefore, in addition to specifically entering mammalian cancer cells, p28 also specifically enters HUVEC cells.
  • the P. aeruginosa azurin 50-77 peptide has activity that inhibits capillary tube formation in endothelial cells, one step in angiogenesis.
  • the P. aeruginosa azurin 50-77 peptide can therefore be used to control angiogenesis and hence be utilized as a cancer treatment, and treatment of other conditions related to inappropriate angiogenesis.
  • Example 2 Effects of p28 on HUVEC capillary tube formation on Matrigel .
  • Matrigel ® Matrix (Becton Dickinson Biosciences, San Jose CA) is a solubulized basement membrane preparation extracted from EHS mouse sarcoma, a tumor rich in ECM proteins. Its major component is laminin, followed by collagen IV, heparan sulfate proteoglycans, and entactin 1. At room temperature, Matrigel Matrix polymerizes to produce biologically active matrix material resembling the mammalian cellular basement membrane. Cells behave as they do in vivo when they are cultured on Matrigel ® Matrix. It provides a physiologically relevant environment for studies of cell morphology, biochemical function, migration or invasion, and gene expression.
  • Matrigel ® Matrix serves as a substrate for in vitro endothelial cell invasion and tube formation assays.
  • the effects of p28 on the capillary tube formation of HUVEC cells were investigated using Matrigel ® .
  • HUVEC cells were plated (15,000 cells/well) on Matrigel ® coated 8 well chamber slides with 20ng/ml VEGF and in the presence or absence of peptide.
  • p28 concentrations of O ⁇ M (control), O.lO ⁇ M, 0.30 ⁇ M, 0.92 ⁇ M, 2.77 ⁇ M, 8.33 ⁇ M, 25 ⁇ M and 75 ⁇ M were used.
  • Cells were stained 4h and 24h post-treatment with calcein AM, and capillary tube formation was examined using a fluorescence microscope (Fig. 2A).
  • HUVEC motility was investigated with the scratch wound migration assay.
  • HUVEC cells were plated in 60mm tissue culture dishes and allowed to reach 90% confluence. After removing the media, cell layers were wounded using a 1 ml sterile plastic pipette tip. Plates were rinsed with culture media. Media with 20ng/ml VEGF alone or media with 20ng/ml VEGF and containing p28 peptide was then added to the plates. One dish was scratched as above and fixed immediately in order to mark exact wound area.
  • Figure 3 A After 24h, cultures were fixed and stained for F-actin and nuclei using Phalloidin and Hoechst stain. Scratched areas were examined using a florescence microscope and photographed. The number of cells that migrated into the scratched area was counted in the control (Fig. 3B) and peptide treated dishes (Fig. 3C).
  • HUVEC cells plated on Matrigel ® coated cover slips were incubated with 20ng/ml VEGF in the presence or absence of 25 ⁇ M p28 peptide for 4h or 24h. After incubation, cells were rinsed in PBS, fixed in buffered formalin and permeablized in 0.2% triton in PBS. Cells were incubated with indicated antibodies for 90min, and if necessary incubated with a specific secondary antibody, and then mounted in DAPI containing mounting media. Analysis was performed with a confocal microscope (model LC510, Carl Zeiss).
  • Proteins examined are as follows: CD-31 (protein present at intercellular junctions that is necessary for cell to cell attachment), Fak (focal adhesion kinase), Paxillin, Vinculin (critical adhesion assembly proteins), WASP (Wiskott Aldrich Syndrome protein, required for nucleation and elongation of F-actin fibers), ⁇ -catenin (required for cell survival, regulation of cell surface proteins).
  • CD31/PECAM1 detected cells, pronounced CD31/PECAM localization was found at cell/cell junctions in p28 treated cells as compared to control (Fig. 4A).
  • the paxillin detected cell the paxillin was mainly localized on cell surface of the control cells, however it was more often found on F-actin fibers in the p28 treated cells (Fig. 4B).
  • Fak detected cells Fak was mainly on localized cell surface of the control cells, while it was more often found on F-actin fibers of the p28 treated cells (Fig. 4C).
  • WASP detected cells at 4h WASP localization was mostly nuclear in control cells, while WASP was localized on the nucleus and at the cell surface in p28 treated cells (Fig.
  • ⁇ -catenin localization was mostly on the cell membrane and in the nucleus in the control cells, while ⁇ -catenin was localized on the cell membrane and perinuclear area in p28 treated cells. Therefore, the presence of p28 prevented the structural changes normally found in HUVECs undergoing angiogenesis.
  • Example 5 In vitro growth inhibition of human melanoma cells by p28.
  • p28 The ability of p28 to inhibit the growth of human melanoma Mel-2 cells in vitro was determined.
  • Mel-2 cells were plated in 24 well culture plates at 10,000-12,000 cells/well and allowed to attach to the plate overnight. Cells were then incubated at 37 0 C in media alone (MEM-E with 10% FBS) or media containing p28 peptide.
  • p28 was added at 5 ⁇ M, 50 ⁇ M, and 100 ⁇ M. The number of cells in each well was counted at Oh, 24h, 48h and 72h. The number of cells in each well was counted using a Coulter counter at the indicated time.
  • Example 6 In vivo anti-tumor activity of p28 peptides.
  • Example 7 Efficacy of the synthetic peptides derived from azurin and plastocyanin.
  • MCF-7 breast cancer cells were incubated in 16-well plates with 5 and 50 ug/ml of the 18-mer azurin peptide for 0, 24, 48 and 72 hours, after which the number of MCF-7 cells were counted in a coulter counter.
  • the peptide was seen at 50 ug/ml to inhibit MCF-7 cell growth by 50% in 48 to 72 hours, as compared to cells without the synthetic peptide treatment.
  • the extent of cell growth inhibition was about 25% at 5 ug/ml of the 18-mer synthetic peptide as compared to untreated control. This experiment shows that the synthetic peptide d does in fact inhibit the cancer cell progression promoted by the B-2 ephrin.
  • Example 8 In vitro measurement of effect of cupredoxins on the growth of Mel-2 and MCF-7 cells.
  • the growth of cells treated with cupredoxins was measured using a 16-well plate.
  • Mel-2 or MCF-7 cells (5 x 10 5 cells per well) were allowed to adhere to multiwell (16-well, in this instance) plates for 24 hours. After adherence, the growth medium was siphoned off.
  • PBS phosphate-buffered saline
  • various cupredoxins/cytochromes at concentrations of 0.1 to 10 ⁇ M in PBS were then added to the wells containing fresh growth media and the growth of the cancer cells was followed for 24, 48 and 72 hours. After the incubation period, trypan blue was added to the culture and the number of dead floating cells was counted. Both live and dead floating cells were counted to determine the IC50 at various cupredoxin doses.
  • the IC50 is the concentration of protein that inhibits the cell culture growth by 50%. At 500,000 cells per well at 24 hours of growth, enough cells were present for reproducible counts. In the cupredoxin-minus control cell cultures, as the cells grew, they had less space to adhere to the bottom of the well, began to die and became floating cells. In the cupredoxin-treated cell cultures, both the Mel-2 and MCF-7 cell line growth was inhibited leading to very few floating cells.
  • Example 9 In Vitro Inhibition of P. falciparum Parasitemia by Cupredoxin and Cytochrome.
  • cupredoxins bacterial wt azurin, M44KM64E azurin, rusticyanin and cyanobacterial plastocyanin, as well as the cytochromes Pseudomonas aeruginosa cytochrome C 551 , human cytochrome c and Phormidium laminosum cytochrome f were tested in a normal red blood cell (RBC) assay at 200 ⁇ g/ml concentrations at 30 hours post inoculation.
  • RBC red blood cell
  • Hct RBCs 200 ⁇ l of 10% Hct RBCs were added to each of 24 wells (final 2% Hct at ImI) in addition to 30 ⁇ l complete RPMI containing recombinant cupredoxin or cytochrome proteins at 666 ⁇ M for a final concentration of 200 ⁇ M.
  • the control showed 9.5% parasitemia (standard error 1.3%), wt azurin 6.9% (s.e. 1.4%), M44KM64E azurin 9.1% (s.e. 1.0%), rusticyanin 7.2% (s.e. 0.7%), cytochrome C 551 7.5% (s.e. 1.5%), human cytochrome c 8.4% (s.e. 0.4%), plastocyanin 8.1% (s.e. 1.3%) and cytochrome f 6.6% (s.e. 1.0%), suggesting that cupredoxins such as wt azurin and rusticyanin and cytochromes such as cytochrome for cytochrome C 551 demonstrated 20 to 30% inhibition of parasitemia.
  • Example 10 Inhibition In Vitro of P. falciparum Intracellular Replication by Rusticyanin.
  • red blood cells were loaded to an intracellular recombinant protein concentration of 200 ⁇ g/ml using a hypotonic ghost preparation. Cells where then washed, resuspended and infected with schizont-stage parasites (P. falciparum) as described in Example 9. The red blood cell ghosts were incubated for 19 hours and 40 hours and giemsa smears were made.
  • Wt azurin, M44KM64E mutant azurin, plastocyanin, cytochrome C 551 , human cytochrome c and cynobacterial cytochrome f proteins showed parasitemia varying from 4.2 to 5.4% .
  • Example 11 Structural Homology between Azurin and Fab Fragment of G17.12 Monoclonal Antibody Complexed with Pf MSP1-19.
  • cupredoxins show structural similarity to the variable domains of the immunoglobulin superfamily members.
  • the DALI algorithm Holm & Park, Bioinformatics 16:566-567 (2000)
  • Azurin exhibits structural similarity to the Fab fragment of G 17.12 monoclonal antibody in complexation with Pf MSP 1 - 19 fragment of the MSP 1 merozoite surface protein of P. falciparum.
  • Azurin also demonstrates structural similarity to CD4 (Table 5), the primary host cell surface receptor for HIV-I. (Maddon et al., Cell 47:333-348 (1986)). Azurin also exhibits a structural similarity to ICAM-I (Table 6), which is involved in cerebral malaria and implicated as a receptor on the endothelial cells in the micro vasculture of the brain and other tissues for sequestering P. f ale iparum-m ' t ected erythrocytes. (Smith et al, Proc. Natl. Acad. Sci.
  • ICAM-I is also found in HIV- 1 particles during their passage through the host cells and is known to enhance HIV-I infectivity by enhancing cytosolic delivery of the viral materials.
  • ICAM-I is known also to be subverted as receptors for major groups of rhino viruses and coxsackie viruses. (Bella & Rossmann, J. Struct. Biol. 128:69-74 (1999))
  • cupredoxins including azurin demonstrate structural similarities in having two anti-parallel ⁇ sheets packed face to face and linked by a disulfide bridge to the variable domains of the immunoglobulin superfamily members as well as extracellular domains of the intercellular adhesion molecules (ICAM) and their ligands.
  • IAM intercellular adhesion molecules
  • CDH CD4 (D1D2 Fragment)
  • the laz gene from Neisseria gonorrhoeae was cloned based on its known sequence (SEQ ID NO: 22).
  • the P. aeruginosa azurin gene (SEQ ID NO: 1), termed paz, and the sequence of the H.8 epitope of laz from TV. gonorrhoeae (SEQ ID NO: 23), were used to clone in frame the H.8 epitope gene in the 5'-end of paz to produce H.S-paz or in the 3'-end of paz to generate paz-H.8.
  • Table 7 Cancer cells, bacterial strains and genetic constructs
  • the forward and reverse primers used were 5'-CCGGAATTCCGGCAGGGATGTTGTAAATATCCG-S' (SEQ ID NO: 34) and 5'-GGGGTACCGCCGTGGCAGGCATACAGCATTTCAATCGG-S' (SEQ ID NO: 35) where the additionally introduced restriction sites of EcoRI and Kpnl sites are underlined respectively.
  • the plasmids expressing fusion H.8 of N. gonorrhoeae Laz and azurin of P. aeruginosa were constructed by PCR with pUC19-/? ⁇ z and pUCl S-laz as templates.
  • a 3.1 kb fragment was amplified with pUC18-/ ⁇ z as a template and primers, 5'-(phosphorylated)GGCAGCAGGGGCTTCGGCAGCATCTGC-3' (SEQ ID NO: 36) and 5'-CTGCAGGTCGACTCTAGAGGATCCCG-S' (SEQ ID NO: 37) where a Sail site is underlined.
  • a PCR amplified a 0.4 kb fragment was obtained from p ⁇ JC ⁇ 9-paz as a template and primers, 5'-(phosphorylated)GCCGAGTGCTCGGTGGACATCCAGG-3' (SEQ ID NO: 38) and 5'-TACTCGAGTC ACTTC AGGGTC AGGGTG-3' (SEQ ID NO: 39) where a Xhol site is underlined.
  • a Sail digested PCR fragment from pUC 1 S-laz and Xhol digested PCR fragment from pUC19-/? ⁇ z were cloned to yield an expression plasmid pUC18-H.8-p ⁇ z (Table 7).
  • E. coli JM 109 was used as a host strain for expression of azurin and its derivative genes.
  • Recombinant E. coli strains were cultivated in 2 X YT medium containing 100 ⁇ g/ml ampicillin, 0.1 mM IPTG and 0.5 mM CuSO 4 for 16 h at 37°C to produce the azurin proteins.
  • E. coli strains harboring these plasmids were grown in presence of IPTG, cells lysed and the proteins purified as described for azurin (Yamada, et al., Proc. Natl. Acad. Sci.
  • Plasmid Construction for Fusion GST Proteins Plasmids expressing fusion glutathione S-transferase (GST)-truncated wt-azurin (azu) derivatives were constructed by a polymerase chain reaction using proofreading DNA polymerase. For pGST- azu 36-128, an amplified PCR fragment was introduced into the BamHl and EcoRl sites of the commercial GST expression vector pGEX-5X (Amersham Biosciences, Piscataway, NJ).
  • the fragment was amplified with pUC19-azu as a template and primers, 5'-CGGGATCC CCG GCA ACC TGC CGA AGA ACG TCA TGG GC-3'(SEQ ID NO: 40) and 5'- CGGAATTC GCA TCA CTT CAG GGT CAG GG-3' (SEQ ID NO: 41), where the additionally introduced BamHl and EcoRI sites are underlined respectively.
  • Carboxyl- terminus truncation of azu gene was cumulatively performed by introducing a stop codon using QuickChange site-direct mutagenesis kit (Stratagene, La Jolla, CA).
  • pGST-azu 36-89 For pGST-azu 36-89, a stop codon were introduced into Gly90.
  • the plasmid carrying pGST-azu 36-128 was used as template DNA.
  • Three sets of oligonucleotides for site-direct mutagenesis are shown as follows. For pGST-azu 36-89: 5'-CCA AGC TGA TCG GCT CGT GAG AGA AGG ACT CGG TGA CC-3' (SEQ ID NO: 42), and 5'-GGT CAC CGA GTC CTT CTC TCA CGA GCC GAT CAG CTT GG-3 (SEQ ID NO: 43).
  • pGST-azu 88-113 carboxyl terminus truncation of azu gene was cumulatively performed by introducing stop codon using QuickChange site directed mutagenesis kit (Stratagene, La Jolla, CA).
  • QuickChange site directed mutagenesis kit (Stratagene, La Jolla, CA).
  • pGST-azu 88-113 a stop codon was introduced into Phel 14.
  • the plasmid carrying pGST-azu 88-128 was used as the template.
  • an amplified PCR fragment was introduced into the BamHl and EcoRl sites of the commercial GST expression vector pGEX-5X (Amersham Biosciences).
  • the fragment was amplified with pUC19-azu as the template and primers, 5'-CGGGGATCC CCG GCT CGG GCG AGA AGG AC-3' (SEQ ID NO: 44) and 5'-CGGGAATTC TCC ACT TCA GGG TCA GGG TG- 3' (SEQ ID NO: 45) where the additionally introduced BamHl and EcoRl sites are underlined respectively.
  • oligonucleotides for site directed mutagenesis are shown as follows for the preparation of pGST-azu 88-113: 5'-GTT CTT CTG CAC CTA GCC GGG CCA CTC CG- 3' (SEQ ID NO: 46) and 5'-CGG ' AGT GGC CCG GCT AGG TGC AGA AGA AC-3' (SEQ ID NO: 47).
  • pGST-azu 88-113 was used to transform E. coli XL-I Blue strains. Plasmid extraction was performed using a commercial kit (Qiagen, Venlo, The Netherlands) and PCR sequencing were performed to assess plasmid insertion and transfection.
  • E. coli BL21 (DE3) was used as a host strain for expression of the gst and its fusions derivatives.
  • E. coli strain XLl -Blue transformed with pGST-azu plasmids was grown in LB media with ampicillin for three hours at 37°C upon which IPTG induction (0.4 mM) was performed an subsequent incubation for 2-4 h at 37°C to maximize the expression levels.
  • Cells were isolated by centrifugation, resuspended in 25 mL of IX PBS buffer. Subsequent cell lysis involved two sequential treatments of the cell suspension via sonication (20 min on ice) and heat-cold shock in acetone-dry ice bath (using the appropriate protease inhibitors).
  • H.8-azurin where the H.8 epitope of Laz has been fused in the N-terminal part of P. aeruginosa azurin in frame (as described in Example 12) were tested.
  • Binding studies were performed by injecting protein eluents (50 ⁇ l) over the protein-CM5 surface at flow rates of 30 ⁇ l/min with a 120 sec time delay at the end of the injections.
  • Protein eluents included GST-azurin fusion proteins (GST, GST- Azu 36- 128, GST-Azu 36-89, and GST-Azu 88-113, as described in Example 12).
  • Sensor chip surfaces were regenerated between protein injections using 100 mM NaOH (10 ⁇ l injection pulse). All binding studies were run in parallel against a negative flow channel with bare Au- CM5 sensor surface to correct for nonspecific binding to the chips.
  • both H.8-azurin and Laz demonstrated a higher affinity of binding with the merozoite surface protein MSPl cleavage products, with characteristic Kd values of 32.2 nM between azurin and MSP1-19 and 54.3 nM between azurin and MSP1-42.
  • the Kd values between H.8-azurin and MSP1-19 and MSP1-42 were 11.8 nM and 14.3 nM while such values between Laz and MSPl -19 and MSP1-42 ranged from 26.2 nM and 45.6 nM respectively.
  • PfMSPl -19 or PfMSP 1-42 moieties the ability of glutathione S-transferase (GST) and a fusion derivative H.8-GST where the H.8 epitope was fused in the N-terminal of GST (see Example 12), to bind MSPl-19 or MSP 1-42 was tested.
  • GST glutathione S-transferase
  • H.8-GST fusion derivative H.8-GST where the H.8 epitope was fused in the N-terminal of GST
  • Glutathione S transferase and some of the fusion proteins where parts of azurin were fused to GST (Yamada et al. , Cell. Microbiol. 7: 1418-1431 (2005), and Example 4) were tested for their ability to bind to MSP.1-19.
  • Example 14 Inhibition of Plasmodium falciparum Parasitemia by Azurin, H.8- Azurin and Laz.
  • the extent of parasitemia was determined using schizont stage parasites and normal red blood cells (RBC).
  • Normal red blood cells (RBCs) were washed twice in serum-free medium and resuspended to 10% hematocrit in complete RPMI. 200 ⁇ l of 10% hematocrit RBCs were added to each of 24 wells in addition to 300 ⁇ l complete RPMI without or with azurin, H.8-azurin or Laz at various concentrations.
  • Schizont stage P. falciparum parasites were prepared by centrifuging a late-stage culture through a Percoll cushion at 3200 rpm for 10 min. For infection, 4x10 6 parasites per well in 500 ⁇ l volume were added at time zero. The plate was incubated overnight (about 16 h) and then scored by thin blood smear and Giemsa stain at that time.
  • azurin does not enter normal cells such as macrophages, mast cells, etc, and the effect of azurin, H.8-azurin or Laz is at the entry level rather than the intracellular replication of the parasite.
  • the data in Fig. 8 demonstrate the potential antimalarial action of azurin, H.8-azurin and Laz through interference in the invasion of the RBC by the parasites.
  • Example 16 In Vivo Inhibition Of HIV Infection Of Lymphocytes By Azurin Mutant And Cytochrome C 551 .
  • the M44KM64E mutant of azurin was mixed with cytochrome C 551 on a 1 :1 basis (1 ⁇ M azurin : 1 ⁇ M cytochrome C 551 ).
  • HIV-infected human blood lymphocytes were incubated with the mixed azurin/cytochrome C 55 1 proteins at concentrations of 0, 500 to 1000 ⁇ g/ml protein for 7 days.
  • the HIV p24 levels were then measured in the infected lymphocytes. p24 levels are known to be colinear with HIV virus levels in infected blood. Measuring the change in p24 concentrations in blood will indicate the change of HIV virus titer in the blood.
  • Controls with non-infected human blood lymphocytes were also run in a parallel manner. After the 7 day incubation, the HIV p24 levels in the infected lymphocytes were reduced by 25% to 90% as compared to the control infected lymphocytes with 0 ⁇ g/ml azurin and cytochrome C 551 - In the non-infected control cells, after 7 days of incubation with the protein mixture, neither cell death nor cytotoxicity was found.
  • Example 17 Effect of Azurin, H.8-Azurin and Laz on HIV-I Entry and Viral Growth.
  • PBMCs peripheral blood mononuclear cells
  • Example 18 Effect of Azurin, H.8-Azurin and Laz on HIV-I Entry and Viral Growth.
  • Plasmid construction and expression of Azurin, H.8-Azurin and Laz were performed as in Example 12.
  • PBMC Peripheral blood mononuclear cells
  • PBMC Peripheral blood mononuclear cells
  • the plate was spun at 800 rpm for 5 min to collect the cells.
  • the supernatant was taken off and media with protein (at concentrations of 0.3, 0.6, 1.2, 6.0 and 30 ⁇ M) was added (100 ⁇ l).
  • the cells were then incubated for 1 h.
  • AZT 25 ⁇ M was used as a control.
  • the proteins were left on cells and 100 ⁇ l of virus (BaI, 2167, or RW/92/008/RE1) was added and incubated for 2 h. The plate was spun again at 800 rpm for 5 minutes and protein and virus was removed. Protein and media were added back for a total volume of 100 ⁇ l and incubated for 5 days. At the end of the 5 day period, the culture supernatant was tested for HIV/p24 by ELISA.
  • the Neisserial protein Laz which also harbors the H.8 epitope in the N-terminal part of the Neisserial azurin homolog (Gotschlich & Seiff FEMS Microbiol. Lett. 43:253-255 (1987); Kawula et al, MoI. Microbiol. 1 :179-185 (1987)), had similar inhibitory activity for the three subtypes, particularly for the African and the Indian subtypes (Fig. 10), demonstrating a role of the H.8 epitope in promoting enhanced anti-HIV-1 activity by azurin.
  • No effect on host cell (PBMC) death by MTT assay (Yamada et al., Proc. Natl. Acad. Sci. USA 99:14098-14103 (2002); Punj et al., Oncogene 23:2367-2378 (2004)) was discernible for all concentrations of these three proteins, suggesting that inhibition of HIV-I growth was not due to death of the host cells.
  • Example 19 Azurin Binding with gpl20 and CD4 as Studied by Surface Plasmon Resonance.
  • Surface Plasmon Resonance experiments were conducted to determine the extent of azurin binding not only to CD4 but also to HIV-I surface proteins such as gpl20 or gp41 known to be involved in HIV-I entry and other proteins such as Nef or Gag that are involved in intracellular virus multiplication.
  • Protein immobilizations on CM5 chips were conducted according to the amine coupling procedure. Due to differences in protein crosslinking efficiencies, proteins were immobilized under various conditions after NHS/EDC preactivation of the CM5 surface: 50 ⁇ l injections of azurin (510 ⁇ M), or 35 ⁇ l injections of CD4 (25 ⁇ M, 2x), or HIV-I gpl20 (10 ⁇ M). Subsequent treatment of CM5 surface with ethanolamine (IM, pH 8.8) removed uncrosslinked proteins prior to binding studies. Binding studies were performed by injecting protein eluents (50 ⁇ l) over the protein-CM5 surface at flow rates of 30 ⁇ l/min with a 120 sec time delay at the end of the injections.
  • IM ethanolamine
  • Protein eluents included CD4 (Protein Sciences Corp., Meriden, CT), HIV-I gpl20 (Immunodiagnostics Inc., Woburn, MA), HIV-I gp41 (Bioclone Inc., San Diego, CA), HIV-I gag and HIV- 1 -nef (Chemicon International, Temecula, CA) and GST-azurin fusion proteins (GST, GST- Azu 36-128, GST- Azu 36-89, and GST- Azu 88- 113, expressed in inventor's laboratory). Sensor chip surfaces were regenerated between protein injections using 100 raM NaOH (10 ⁇ l injection pulse).
  • gpl20 showed somewhat stronger binding to azurin than CD4 (Fig. HB), clearly demonstrating that azurin binds both to gpl20 and CD4 with a high affinity.
  • gp41 also involved in HIV-I entry into the host cell, did not show any binding to azurin (Fig. 1 IB). Similar lack of binding was demonstrated for Gag and Nef.
  • Example 20 Azurin Binding with ICAMs and CD5 as Studied by Surface Plasmon Resonance.
  • NCAM Fig. 11C, inset
  • Example 21 Azurin Competition with gpl20 for CD4 as Studied by Surface Plasmon Resonance. Due to the higher affinity of binding of azurin to CD4, as compared to gpl20 (Fig.
  • Example 22 Azurin and ICAM-3 Binding with DC-SIGN as Studied by Surface Plasmon Resonance.
  • DC-SIGN DC-specific intercellular adhesion molecule 3-grabbing nonintegrin
  • DC-SIGN/R a related protein that influences the binding of another very important HIV-I binding protein present on the surface of dendritic cells (DC) known as DC-SIGN (DC-specific intercellular adhesion molecule 3-grabbing nonintegrin) and a related protein called DC-SIGN/R.
  • DC-SIGN is expressed abundantly on DC while DC-SIGN/R is expressed primarily on sinusoidal and endothelial cells.
  • DC-SIGN plays a major role in HIV-I immunopathogenesis by allowing DC, which are professional antigen presenting cells, to capture and present pathogens including HIV-I to resting T cells through their interactions with ICAM-3 on the T cell surface.
  • DC-SIGN has also been shown to bind avidly to HIV-I envelope protein gpl20, thereby capturing HIV-I and transporting it to CD4 + T cells, where HIV-I can replicate freely.
  • DC-SIGN a critical molecule on DC surface responsible for transmitting HIV-I from the mucosal cells to the lymphoid T cells, may well find a strong competitor in azurin or Laz that can also avidly bind gpl20, CD4 and ICAM-3.
  • Example 23 Azurin/Laz Acts in the Entry Stage of HIV-I Infection.
  • CD4+RO+ cells are enriched by magnetic separation and FACS sorting, and assayed to determine infectivity with respect to naive and uninfected cell co-culture experiments. This analysis of CD4+RO+ memory cells shows the presence of infective HIV.
  • the patients are injected with a pharmaceutical preparation of purified P. aeruginosa azurin. Two such patients serve as treated controls.
  • the sterile pharmaceutical preparation is in the form of 0.5 ml single-dose ampoules of sterile P. aeruginosa azurin in a pharmaceutical preparation designed for intravenous administration, as will be well known to those in the art.
  • the pharmaceutical preparation is stored at 4° C. and protected from light before administration.
  • P. aeruginosa azurin is prepared at five different concentrations: 10 ⁇ g, 30 ⁇ g, 100 ⁇ g, 300 ⁇ g and 800 ⁇ g azurin/cytochrome c 55 i (1 :1 on molecule basis) per 0.5 ml dose.
  • the pharmaceutical preparation is given intravenously to twenty two patients for each 10 doses. Patients receive primary treatment at day 0 and subsequent doses identical doses for a period of 3 months until CD4+ cells, including memory cells, are at low levels
  • Complete blood count and serum chemistry profiles are rechecked two days after each dose.
  • the presence of the malaria parasite are determined by light microscopic examination (ME) of the stained blood smears, or the ICT Malaria P.f./P.v. test kits ( Binax, Inc., Portland, ME) .
  • the patients are also followed at frequent intervals and monitored for CD34 cell level, reestablishment of CD4+ cells and quantitation of CD4+RO+ cells. Additionally, the patients' plasma is assayed for viral load by cell co-culture experiments. On reducing virus load in active and memory CD4+ T cells to low or non- detectable concentrations, the patients are weaned from azurin.
  • the patients are weaned from antibiotic and antifungal therapy. Following this, the patients are followed at 6 month intervals and assayed for viral content.
  • the results demonstrate the effectiveness of azurin therapy for patients with HIV infection.
  • the results demonstrate the effectiveness of the therapy.
  • Human cancer and non-cancer (immortalized and non- immortalized) cell lines were obtained from ATCC [lung cancer (A549 and NCI-H23 adenocarcinoma), normal lung (CCD- 13 Lu), prostate cancers (DU 145 and LN-CAP), normal prostate (CRLl 1611), breast cancer (MCF-7), normal breast (MCF-IOA), colon cancer
  • HCTl 16 normal colon
  • CCD33Co normal colon
  • fibrosarcoma HTl 080
  • SK-OV3 adenocarcinoma ovarian cancer
  • UISO-Mel-2 All cells except UISO-Mel-2 were cultured in MEM-E (Invitrogen, Carlsbad, CA) supplemented with 10% heat- inactivated fetal bovine serum (Atlanta Biological Inc., Lawrenceville, GA), 100 units/ml penicillin and lOO ⁇ g/ml streptomycin at 37C in 5% CO2 or air.
  • Proliferation assays/Cell growth Melanoma cells were seeded (four replicates) in flat bottom 24 well plates (Becton Dickinson, Franklin Lakes, NJ) at a density of 12x103 cells/well. After 24 hrs media was changed and fresh p 18, p28 , azurin or a similar volume of media without peptide (eight replicates) added daily for 72 hr. Cells were then counted in a Beckman Coulter (Z 1 coulter particle counter). Values represent the mean ⁇ SD of 4 replicates.
  • MITT Assay Melanoma cells were seeded at a density of 2000 cells/well in flat- bottomed 96 well plates (Becton Dickinson, Franklin Lakes, NJ) and allowed to attach for 24 hrs. Freshly prepared peptide (10 ⁇ l) or culture medium was then added to each well. After 24 hrs, medium was changed and pi 8, p28 or azurin added daily. After 72 hr incubation, lO ⁇ l of MTT reagent (Trevigen, Gaithersburg, MD) was added to each well, the samples incubated for 3hr, RT/sig 100 ⁇ l of detergent added to each well, and the samples incubated for an additional 3hr at 37°C.
  • MTT reagent Tevigen, Gaithersburg, MD
  • a protein i.e., azurin
  • MRS membranephilic residue score
  • MAS membranephilic area score
  • K mpha coefficient of membranephilic asymmetry
  • Peptide/Protein labeling Peptides were dissolved in ImI PBS mixed with Alexafluor 568 dye (Molecular Probes, Eugene, OR) at a 1 :2 protein:dye ratio, lOO ⁇ l sodium bicarbonate added, and the mixture incubated overnight at 4°C with continuous stirring. Labeled peptide was separated from free dye by dialyzing against cold-PBS using Slide- A- Lyzerg Dialysis Cassettes 1000 MWCO for pl2 and 2000 MWCO for others (Pierce Biotechnology, Rockford, IL).
  • Alexafluor 568 dye Molecular Probes, Eugene, OR
  • Cell penetrationfconfocal analysis Cells were seeded on glass coverslips and allowed to attach overnight at 37°C under 5% CO 2 . Cells were rinsed with fresh media and incubated at 37 0 C for 2 hrs in pre-warmed media containing Alexafluor 568 labeled azurin peptides (20 ⁇ M) or Arg8 (5 ⁇ M), or media alone. Following incubation, coverslips were rinsed 3x with PBS, cells fixed in 2.5% formalin for 5 min, and washed 2x in PBS, once in d.i. H 2 O, and coverslips mounted in media containing 1.5 ⁇ g/ml DAPI for nuclear counter staining (VECTASHIELD® Vector Laboratories, Burlingame CA). Cellular uptake and distribution were photographed under an inverted confocal laser scanning microscope ('Model LC510, Carl Zeiss Inc., Gottingen, Germany).
  • Peptide co-localization with lysosomes or mitochondria was determined by incubating cells growing on a glass coverslip for 2 hrs at 37° with Alexafluor 568 labeled azurin or peptides. Mitrotracker (MitroTracker® Green FM Invitrogen Corporation, Carlsbad, CA) or lysotracker (LysoTracker® Green DND-26 Invitrogen Corporation, Carlsbad, CA) was added (final concentraion 1 ⁇ M) for the last 30 mins of incubation. Cells were rinsed 3x with PBS, fixed in 2.5 % formalin for 5 mins, washed 2x with PBS and incubated in 0.1% Triton-XlOO in PBS for 15 min.
  • UISO-Mel-2 cells on coverslips were preincubated in MEM-E containing 100 ⁇ g/ml heparin sulfate (Sigma-Aldrich, St. Louis, MO) for 30 min and pi 8, p28 or Arg 8 added to bring the final concentration to 20 ⁇ M. After lhr, coverslips were washed, fixed, and analyzed as described above.
  • Cell penetration by FFACS Cells (1.0 x 10 6 /500 ⁇ l PBS) were incubated for 2 hrs at 37°C with Alexafluor 568 labeled pi 8 or p28 (20 ⁇ M), Argg (5 ⁇ M), or media alone, washed 3x in PBS, fixed in 2.5% formalin for 5 min, washed twice in PBS, resuspended in 200 ⁇ l PBS, and passed through a screen to obtain a single cell suspension. Samples were analyzed with a MoFIo Cell Sorter (Dako, Glostrup, Denmark) ⁇ eX 568 nm and ⁇ em 603 nm and the fold increase of the mean fluorescence intensity over background levels calculated.
  • Results represent mean fluorescence of three separate experiments. Entry inhibitors: UISO-Mel-2 cells (3xlO 5 per 300 ⁇ l), maintained in phenol red-, serum-free MEM-E at 37 0 C, were pretreated with inhibitors, including: Chloropromazine (inhibitor of clathrin-mediatied endocytosis, 10 ⁇ g/ml, 60 min); Amiloride (macropinocytosis inhibitor, 50 ⁇ M, 30 min); Nystatin (50 ⁇ g/ml, 30 min); Methyl- ⁇ -cyclodextrin (M ⁇ CD, 5mM, 60 min); Filipin (inhibitor of caveolae-mediated endocytosis, 3 ⁇ g/ml, 60 min); Taxol (microtubule stabilizer, 20 ⁇ M, 30 min); Staurosporine (cell cycle inhibitor, 250 nM, 10 min); Sodium azide (metabolic inhibitor, 1 mM, 60 min); Oauabain (ATP
  • Hemolysis assay Human whole blood samples (2-3ml) were centrifuged for 10 min at 1000xg, and the pellets washed once with PBS and once with HKR buffer pH7.4 ( 18). Cell pellets were then resuspended in HKR buffer to 4% erythrocytes, 50 ⁇ l transferred to a 1.5ml tube with 950 ⁇ l of peptides, azurin (5, 50 and lOO ⁇ M) or 0.1% Triton X-100 in HRK buffer to completely disrupt the RBC membrane. MAP and Mastoparan7 (Bachem California, Inc., Torrance, CA) were used as positive controls. After 30 min incubation at 37 0 C with rotation, tubes were centrifuged for 2 min at 1000xg, 300 ⁇ l of supernatants transferred to a 96-well plate and absorbance recorded at 540 nm.
  • UISO-Mel-2 cells (5x 10 5 cells) in 1.5 ml tubes were suspended in MEME media without phenol red. Reactions were started by adding either Alexa fluor 568- conjugated p 18 at 0, 10, 20, 50, 100, 150 and 200 ⁇ M for 5, 10, 15 and 20 sec ., or Alexafluor 568-conjugated p28 at 1, 10, 25, 50, 100, 150 and 200 ⁇ M for 30 , 60, 90 and 120 sec on ice. After incubation, 1 ml of cold-PBS was added to the 250 ⁇ l reaction in mixture. Cells were centrifuged twice at 600xg for 2 min at 4°C. At least 10,000 fixed cells were analyzed by flow cytometry in each reaction and their background and relative fluorescence calculated.
  • Radioactivity in cells incubated with I 125 azurin alone was considered total binding; radioactivity in the presence of unlabeled azurin, pi 8, or p28 was considered nonspecific binding. Specific binding was determined by subtracting nonspecific binding from total binding and Scatchard plots generated.
  • Example 26 Domain of p28 responsible for preferential entry into cancer cells
  • pi 8 The predicted Robson structure (data not shown) of pi 8 suggests that the C-terminal amino acids form a partial ⁇ -sheet. This and the shorter length of pi 8, which lacks the hydrophilic C-terminal 10 amino acids (aa 68-77, SEQ ID NO: 92) of p28, suggests that pi 8, as a putative PTD for azurin, may have a more rapid entry into cancer and normal cells via a non-endocytotic over an endocytotic or membrane receptor mediated process.
  • MAPAS data (MRS 3.74, MAS 87.1, K mpha 2.37) predict that aa's 69, 70, 75, 76, 85 of azurin provide the best opportunity for membrane contact, suggesting the C-terminal region of p28, not present on pi 8 (aa 50-67) is most likely to contact specific residues on the cell membrane, irrespective of a cell's status.
  • pi 8b has a short ⁇ -helix and partial ⁇ -sheet, and is extremely hydrophilic which together may negate preferential entry
  • pi 2 (theoretical p/ 4.33) lacks a secondary ⁇ -helical structure, but is also hydrophilic suggesting overall hydrophilicity may be a major contributor to the decrease in selectivity of cell penetration.
  • Example 27 Cell penetration is not a result of membrane disruption
  • Example 28 - pl8/p28 penetration is energy dependent and saturable
  • the kinetics of p28 and pi 8 entry into UISO-Mel-2 cells relative to human fibroblasts was calculated after incubation, when cells were fixed and mean fluorescence intensity (MFI) determined.
  • the Km and Vmax of each peptide were calculated by plotting peptide concentration ( ⁇ M) vs velocity (MFI/sec) or by Scatchard analysis.
  • Example 30 - pl8/p28 penetration involves Caveolae and the Golgi Complex Peptides called cell-penetrating peptides (CPPs) or cell-delivery vectors (CDVs), such as penetratin, transportan, Tat (amino acids 47-57 or 48-60), and the model amphipathic peptide MAP, are short, amphipathic and cationic peptides and peptide derivatives, usually containing multiple lysine and arginine residues. Fischer, P. M., Med Res Rev, 27: 755-795 (2007).
  • CPPs cell-penetrating peptides
  • CDVs cell-delivery vectors
  • cationic CPPs such as pTat and Arg 8 enter cells by initially binding to anionic, sulfated proteoglycans prior to endocytosis.
  • Chlorpromazine (CPZ), a specific inhibitor of clathrin mediated endocytosis, also had no effect on penetration, nor did the macropinocytosis inhibitor amiloride.
  • Figure 15 B Stabilization of microtubules with taxol had no effect on penetration , but disruption of actin filaments and macropinocytosis with Cytochalasin D produced a small (-20%), reproducible inhibition of the penetration of pi 8 and p28.
  • the lack of effect of amiloride suggests that the inhibitory activity of Cytochalasin D is probably through its effect on actin filaments. Inhibition of the cell cycle with staurosporine did not block penetration, suggesting that penetration was not cell cycle specific.
  • wortmannin an inhibitor of early endosome formation, monensin, which inhibits late endosome/lysosome, and brefeldin A (BFA), a disruptor of the Golgi apparatus.
  • Wortmannin did not block the intracellular accumulation of either pi 8 or p28 suggesting that, unlike cholera toxin, a caveolae to early endosome pathway is not involved in the intracellular trafficking of pi 8 and p28.
  • the lack of early endosome involvement in the intracellular trafficking of pi 8 and p28 also suggests that clathrin mediated endocytosis is not involved in internalization of these peptides.
  • Example 31 Functional Analysis of p28 and pl8 Azurin inhibits the growth of several human cancer cell lines in vitro and in vivo.
  • Figures 20 A and B illustrate the effect of pi 8 and p28 relative to azurin and dacarbazine (DTIC) on UISO-Mel-2 cells as determined by MTT and cell count.
  • azurin decreased (p ⁇ 0.05) cell survival at 100 and 200 ⁇ M -15% ( Figure 20 A).
  • p28 had inhibited cell survival 14 and 22% (p 0.05) at 100 and 200 ⁇ M, respectively.
  • pi 8 had no effect, while dacarbazine (DTIC) produced a significant dose-related decrease on UISO-Mel-2 survival.

Landscapes

  • Chemical & Material Sciences (AREA)
  • Organic Chemistry (AREA)
  • Health & Medical Sciences (AREA)
  • General Health & Medical Sciences (AREA)
  • Biochemistry (AREA)
  • Biophysics (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Genetics & Genomics (AREA)
  • Medicinal Chemistry (AREA)
  • Molecular Biology (AREA)
  • Proteomics, Peptides & Aminoacids (AREA)
  • Gastroenterology & Hepatology (AREA)
  • Medicines That Contain Protein Lipid Enzymes And Other Medicines (AREA)

Abstract

The present invention relates to compositions and methods to administer compositions comprising cupredoxin and/or cytochrome and/or variants, derivatives, truncations and structural equivalents of cupredoxin and cytochrome to treat and/or prevent two or more conditions in a mammalian cell. The invention also relates to compositions and methods to administer compositions comprising cupredoxin and/or cytochrome and/or variants, derivatives, truncations and structural equivalents of cupredoxin and cytochrome to concurrently treat and/or prevent two or more conditions in a patient such as HIV, cancer, malaria and inappropriate angiogenesis.

Description

COMPOSITIONS AND METHODS TO CONCURRENTLY TREAT OR PREVENT MULTIPLE DISEASES WITH CUPREDOXINS
CROSS REFERENCE TO RELATED APPLICATIONS
This application claims priority under 35 U.S. C. §§ 119 and 120 to U.S. Provisional Patent Application Serial No. 61/013,709, filed on December 14, 2007, and is a continuation in part of U.S. Patent Application Serial No. 11/943,034, filed on November 20, 2007, which is a divisional of U.S. Application Serial No. 11/436,591, filed on May 19, 2006, which issued as U.S. Patent No. 7,301,010, and is also a continuation in part of U.S. Application Serial No. 11/861,536, filed on September 26, 2007, which is a divisional of U.S. Patent Application Serial No. 11/436,590, filed on May 19, 2006, which issued as U.S. Patent No. 7,338,766, and is also a continuation in part of U.S. Application Serial No. 11/488,693, filed on July 19, 2006, and is also a continuation in part of U.S. Application Serial No. 12/013,122, filed on January 11 , 2008, which is a continuation in part of U.S. Application Serial No.
11/436,592, filed on May 19, 2006, which issued as U.S. Patent No. 7,381,701. Each of these documents is hereby incorporated by reference in its entirety herein.
FIELD OF THE INVENTION The present invention relates to compositions comprising variants, derivatives and structural equivalents of cupredoxins that concurrently treat and/or prevent two or more conditions in a patient.
BACKGROUND OF THE INVENTION
Human immunodeficiency virus (HIV) infection, which results in AIDS, is a relatively new infection in the human population, and has quickly risen to the foremost health problem in the world. HI V/ AIDS is now the leading cause of death in sub-Saharan Africa, and is the fourth biggest killer worldwide. At the end of 2001, it was estimated that 40 million people were living with HIV infection world wide. The Centers for Disease Control (CDC) estimates that nearly 800,000 people are living with AIDS in the US, and 40,000 new cases diagnosed each year. While better treatment methods are now known to prolong the life of patients with HIV infection, there is still no cure. Modern anti-HIV drugs target several different stages of the HIV life cycle, and several of the enzymes that HIV requires to replicate and survive. Some of the commonly used anti-HIV drugs include nucleoside reverse transcriptase inhibitors such as AZT, ddl, ddC, d4T, 3TC, and abacavir; nucleotide reverse transcriptase inhibitors such as tenofovir; non-nucleoside reverse transcriptase inhibitors such as nevirapine, efavirenz and delavirdine; protease inhibitors such as saquinavir, ritonavir, indinavir, nelfinavir, amprinavir, lopinavir and atazanavir; and fusion inhibitors such as enfuvirtide. However, in some HIV infected patients, none of these antiviral drugs, alone or in combination, is effective to prevent the progression of chronic infection or treat acute AIDS. The high mutation rate of the HIV virus and associated emergence of HIV strains resistant to drugs may be one large factor that results in the inability to effectively treat HIV infection.
About one quarter of the world's population is exposed to the risk of malaria and more than a million people die of malaria each year. Of the four species of malarial parasites that infect humans, the two major species are Plasmodium falciparum and P. vivax.
The P. falciparum blood stage merozoites bind to and parasitize the erythrocytes using a variety of surface proteins (Cowman et al., FEBS Lett. 476:84-88 (2000); Baum et al, J. Biol. Chem. 281:5197-5208 (2006)), a major antigenic member of which is called Merozoite Surface Protein 1 (MSPl), a 195 kDa protein. MSPl is present in all the erythrocyte-invasive species of Plasmodium, anchored to the merozoite surface by a glycosyl-phosphatidylinositol linkage. During early stages of the erythrocyte invasion process, soon after release from infected erythrocytes, the merozoite MSPl protein undergoes proteolytic cleavage, producing a C-terminal cleavage product MSP 1-42, which subsequently undergoes a second cleavage, producing an 11 kDa peptide MSP1-19, which remains attached to the parasite surface as it enters the erythrocyte. The formation of the cleavage product MSP 1-19 is very important for successful invasion by the parasite since inhibition of its proteolytic formation or its neutralization by monoclonal antibodies prevents entry of the parasite to the erythrocytes (Blackman et al., J. Exptl., Med. 180:389-393 (1994)). The MSPl-19 peptide is one of the most important malaria vaccine candidates available. MSPl-19-specific antibodies from malaria-resistant human sera react with the antigen and include a major erythrocyte-invasion inhibitory component (Holder & Riley, Parasitol. Today, 12: 173-174 (1996); O'Donnell et al, J. Expt. Med. 193: 1403-1412 (2001)). Serum from donors in malaria-endemic regions usually demonstrates strong antibody reactivity towards Pf MSP1-19. (Nwuba et al, Infect. Immun. 70: 5328-5331 (2002))
The monoclonal antibody (mAb) Gl 7.12 was raised against recombinant Pf MSPl-19 and recognizes its epitope on the parasite surface, demonstrating that this region of the antigen is accessible on the native MSPl polypeptide complex (Pizarro et al, J. MoI. Biol. 328:1091-1103 (2003)). Interestingly, erythrocyte invasion experiments in vitro showed that infection is not inhibited in the presence of G 17.12, even at 200 μg/ml concentration and Gl 7.12 does not inhibit in vitro secondary processing of MSPl. Id. The presence of antibodies that block the binding of invasion - inhibitory antibodies, thereby facilitating parasite survival, has also been demonstrated (Guevara Patino et al, J. Expt. Med. 186: 1689- 1699(1997)), and may be responsible for the failure of G 17.12 mAb to inhibit erythrocyte invasion by M. falciparum.
Cerebral malaria, a rare but fatal infection restricted to P. falciparum invasion of brain capillaries because of the sequestration of parasitized erythrocytes, is often untreatable because most drugs cannot cross the blood-brain barrier to reach the brain capillaries. Adhesion of P. falciparum - infected erythrocytes to brain capillaries is mediated by the interaction of parasite ligands Pf Emp-1 family of proteins expressed on the surface of infected erythrocytes with ICAM-I and CD36 expressed on the surface of capillary endothelium cells in cerebral vessels. (Smith et al., Proc. Natl. Acad. Sci. USA 97:1766- 1771 (2000); Franke-Fayard et al., Proc. Natl. Acad. Sci. USA 102, 11468-11473 (2005).
Although a few drugs, such as chloroquine that targets the heme detoxification pathway, are used to treat malaria, there are increasing incidence of parasite resistance to drugs and mosquito vector resistance to insecticides. Chloroquine antagonizes heme polymerization mediated by parasite-induced HRPs (histidine-rich proteins), as heme monomers are highly toxic for malaria parasites. The polymerization of heme allows detoxification, which is reversed by chloroquine. Another drug, artemisinin, is effective against chloroquine-resistant P. falciparum in cerebral malaria. Artemisinin forms adducts with globin-bound heme in hemoglobin, which binds HRPs to prevent heme polymerization.
A cancer is a malignant tumor of potentially unlimited growth. It is primarily the pathogenic replication (a loss of normal regulatory control) of various types of cells found in the human body. Initial treatment of the disease is often surgery, radiation treatment or the combination of these treatments, but locally recurrent and metastatic disease is frequent. Chemotherapeutic treatments for some cancers are available but these seldom induce long term regression. Hence, they are often not curative. Commonly, tumors and their metastases become refractory to chemotherapy, in an event known as the development of multidrug resistance. In many cases, tumors are inherently resistant to some classes of chemotherapeutic agents. In addition, such treatments threaten noncancerous cells, are stressful to the human body, and produce many side effects.
Angiogenesis is the formation of new blood vessels from preexisting endothelial vasculature. Folkman, et al., J. Exp. Med. 133:275-288, (1971). Most tumors require angiogenesis to sustain growth beyond a critical volume of 1 -2 mm, when the supply of nutrients and metabolites becomes insufficient due to the limits of diffusional exchange. Folkman, J. Nat. Cancer Inst. 82:4-6 (1990). Tumors deprived of angiogenesis remain dormant indefinitely, only to rapidly grow when a blood supply is acquired. Brem et al, Cancer Res.36:2807-2812 (1976). The degree of angiogenesis often increases with tumor progression. Dome et al., J. Pathol. 197:355-362 (2002). Further, invasion and metastatic spread of tumors are also thought to be angiogenesis-dependant events. Folkman, Ann Surg. 175:409-416 (1972). The newly formed blood vessels provide a route for cancer cells to enter the circulatory system and spread to distant parts of the body. Fidler and Ellis, Cell 79:185-188 (1994). Because angiogenesis is an integral process in the growth and spread of tumors, it is an important focus of cancer therapy. Anti-angiogenesis therapy is effective not only for solid tumors, but also hematopoietic tumors, leukemia and myeloma, Bellamy et al., Cancer Res. 59:728-733 (1999); Rajkumar et al, Leukemia. 13:469-472 (1999). Endothelial cells are thought to be better targets for therapy than tumor cells because they have a longer generation time and more genetic stability that tumor cells. Endothelial cells are therefore less likely to "escape" therapy by developing drug resistance to the therapy administered. Boehn-Vaiswanathan, Curr. Opin. Oncol. 12:89-94 ( 2000). Other conditions suffered by mammals are also related to inappropriate angiogenesis. Wet macular degeneration occurs when blood capillaries inappropriately grow into the retina. Inappropriate angiogenesis has also been implicated as a fundamental characteristic of diabetic retinopathy, psoriasis and rheumatoid arthritis, among other diseases. Bussolino et al, Trends Biochem. Sci. 22:251-256 (1997); Folkman, Nat. Med. 1 : 27-31 (1995).
Numerous diseases, such as those discussed above, may occur concurrently in a patient, or one disease may cause or increase the probability of causing another disease in a patient. For example, an HIV infected patient is associated with an increased risk of acquiring large cell lymphoma or Kaposi's sarcoma. The Merck Manual of Diagnosis and Therapy, (Beers et al., 18th edition, Merck Research Laboratories, 2006). For another example, a female patient that acquires human papilloma- virus has an increased risk of acquiring cervical carcinoma. Id.
Numerous diseases also have a high probability to infect a patient concurrently due to environmental factors. Environmental factors may include a patient's lifestyle, eating habits and/or geographic location. For example, co-infections with HIV and malaria are very common in many areas of the world, and in particular sub-Saharan Africa
Genetic predisposition may also play a factor in a patient acquiring two diseases concurrently. For example, it is known that when a person carries a particular cystic fibrosis transmembrane regulator (CFTR) mutation, that person has a higher risk for cystic fibrosis and pancreatic cancer. Weiss et al, Gut; 54: 1456-1460 (2005).
Because so many factors can cause or increase the probability of a patient acquiring two or more diseases or conditions, it would be practical to have one compound or a group of related compounds that could inhibit, or treat and/or prevent two or more diseases or conditions concurrently.
SUMMARY OF THE INVENTION
The present invention relates to compositions comprising peptides that may be cupredoxin or cytochrome or variants, derivatives, truncations and structural equivalents of cupredoxin or cytochrome that treat and/or prevent two or more conditions in a mammalian cell.
The present invention further relates to compositions that may comprise cupredoxin or cytochrome, and/or variants, derivatives, truncations, or structural equivalents of cupredoxin or cytochrome, that retain the ability to concurrently treat and/or prevent two or more conditions such as cancer, inappropriate angiogenesis, HIV and malaria in a patient. These compositions may be isolated peptides or pharmaceutical compositions, among others.
In one embodiment of the present invention, the cupredoxin may be azurin, pseudoazurin, plastocyanin, rusticyanin, Laz, auracyanin, stellacyanin and cucumber basic protein, and specifically may be azurin. The cupredoxin may be from an organism such as Pseudomonas aeruginosa, Alcaligenes faecalis, Ulva pertussis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp. , Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas fluorescens, Bordetella pertussis, Pseudomonas syringae, Pseudomonas chloror aphis, Xylella fastidiosa and Vibrio parahaemolyticus, and specifically may be Pseudomonas aeruginosa.
In another embodiment of the present invention, the isolated peptide may inhibit parasitemia by malaria in P. falciparum-infected human red blood cells.
In another embodiment, the isolated peptide may be fused to a H.8 region of Laz.
In another embodiment of the present invention, the isolated peptide may be a structural equivalent of monoclonal antibody Gl 7.12.
In another embodiment of the present invention, the isolated peptide may be a cytochrome selected from one or more of the group consisting of cytochrome c, cytochrome f and cytochrome C55 \.
In another embodiment of the present invention, the isolated peptide of cytochrome c may be from an organism selected from the group consisting of human and Pseudomonas aeruginosa. In another embodiment of the present invention, the isolated peptide of cytochrome f may be from cyanobacteria. In another embodiment, the isolated peptide may be part of SEQ ID NOS: 1, 5-12, 18 and 23, a mutant of SEQ ID NOS: 1, 5-12, 18 and 23, or have at least 90% amino acid sequence identity to SEQ ID NOS: 1, 5-12, 18 and 23. In another embodiment, the isolated peptide may be a truncation of a peptide selected from one or more of the group consisting of SEQ ID NOS: 1, 5-12, 18 and 23. In another embodiment, the isolated peptide may be a truncation of a cupredoxin. The isolated peptide may be any suitable length, including from 10 to 100 residues, 18 to 100 residues, or 18 to 28 residues. The isolated peptide may comprise or consist of a sequence and/or the equivalent residues of a cupredoxin as a region selected from the group consisting of Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30),
Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio parahaemolyticus azurin residues 52-78 (SEQ ID NO: 27), Pseudomonas syringae azurin residues 51-77 (SEQ ID NO: 25), Bordetella bronchiseptica azurin residues 51-77 (SEQ ID NO: 28), and Pseudomonas aeruginosa azurin residues 36-77 (SEQ ID NO: 33). The isolated peptide may also be a truncation of any of those sequences or a truncation of a larger sequence that comprises those sequences. The isolated peptide may comprise equivalent residues of a region of the isolated peptide, wherein the peptide comprises the sequence and/or the equivalent residues of a cupredoxin as a region selected from the group consisting of Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio parahaemolyticus azurin residues 52-78 (SEQ ID NO: 27), Pseudomonas syringae azurin residues 51-77 (SEQ ID NO: 25), Bordetella bronchiseptica azurin residues 51-77 (SEQ ID NO: 28), and Pseudomonas aeruginosa azurin residues 36-77 (SEQ ID NO: 33). The isolated peptide may also be a truncation of any of those sequences or a truncation of a larger sequence that comprises those sequences. In another embodiment of the present invention, the compositions may comprise one or at least two cupredoxins, cytochromes or peptides in a pharmaceutical composition. In some the embodiments, the pharmaceutical compositions may comprise the isolated peptides of the present invention. In another embodiment, the cupredoxin in a pharmaceutical composition may be from an organism such as Pseudomonas aeruginosa, Alcaligenes faecalis, Ulva pertussis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp., Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas fluorescens, Bordetella pertussis, Pseudomonas syringae, Pseudomonas chlororaphis, Xylella fastidiosa and Vibrio parahaemolyticus, and specifically may be Pseudomonas aeruginosa.
In another embodiment of the present invention, the cupredoxin in a pharmaceutical composition may be selected from one or more of the group consisting of SEQ ID NOS: 1, 5- 12, 18, 23, 25, 27-33 and 48-50. In another embodiment of the present invention, the cupredoxin in a pharmaceutical composition may comprise SEQ ID NO: 30. In another embodiment of the present invention, the composition may be administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papilloma virus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomegalovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus, arena virus, Dhori virus, poliovirus, rubella virus, dengue virus; SIV, Mycobacterium tuberculosis and cancer.
In another embodiment of the present invention, the composition may comprise a therapeutic agent for the concurrent prevention and/or treatment of cancer selected from the group consisting of melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors, and prostate cancer. In another embodiment of the present invention, the compositions may be administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of HIV, malaria, cancer and inappropriate angiogenesis. In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of malaria, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis. In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of HIV, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of cancer, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or malaria.
In another embodiment of the present invention, the compositions may comprise a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or malaria. In another embodiment of the present invention, the compositions may comprise another drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
In another embodiment of the present invention, the pharmaceutical composition may be administered by intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection or oral.
In another embodiment of the present invention, the pharmaceutical composition may be co-administered with at least one other drug. In another embodiment, the pharmaceutical composition may be co-administered with one other drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug. In another embodiment of the present invention, the pharmaceutical composition may be administered at about the same time with another drug. The other drug may be an antimalarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
In another embodiment of the present invention, the methods may include administering to a patient the composition comprising one or at least two cupredoxins, cytochromes or peptides in a pharmaceutical composition. In another embodiment, the patient is human.
In another embodiment of the present invention, the methods may include administering the compositions to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papilloma virus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus, arena virus, Dhori virus, poliovirus, rubella virus, dengue virus; SIV, Mycobacterium tuberculosis and cancer. The cancer may be selected from the group consisting of melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors, and prostate cancer.
In another embodiment of the present invention, the methods may include administering the compositions to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis. In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of malaria, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or inappropriate angiogenesis.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of HIV, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of malaria, cancer or inappropriate angiogenesis.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of cancer, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, malaria or inappropriate angiogenesis.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from one or more of the group consisting of HIV, cancer or malaria.
In another embodiment of the present invention, the methods may utilize a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, cancer or malaria.
In another embodiment of the present invention, the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop cancer than the general population.
In another embodiment of the present invention, the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop HIV than the general population.
In another embodiment of the present invention, the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop malaria than the general population.
In another embodiment of the present invention, the methods may utilize compositions wherein the composition is administered to a patient at a higher risk to develop inappropriate angiogenesis than the general population. In another embodiment of the present invention, the methods may utilize compositions wherein the composition is administered to a patient that has a higher risk than the general population of acquiring one or more of the group consisting of HIV, cancer, angiogenesis and malaria.
In another embodiment of the present invention, the methods may utilize compositions wherein the composition is administered to a patient that has at least one high risk feature.
In another embodiment of the present invention, the methods may utilize a pharmaceutical composition administered by intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection or oral, and specifically may be administered by intravenous injection.
In another embodiment of the present invention, the methods may utilize a pharmaceutical composition co-administered with at least one other drug. In another embodiment, the other drug may be an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug. In another embodiment of the present invention, the methods may utilize a pharmaceutical composition administered at about the same time with at least one other drug. In another embodiment, the methods may utilize a pharmaceutical composition administered at about the same time with at least one other drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
In another embodiment of the present invention, the composition may be a kit comprising the pharmaceutical composition of the invention. In another embodiment of the present invention, the kit may be designed for intravenous administration.
In another embodiment of the present invention, the composition be an isolated peptide that can bind a protein selected from the group consisting of CD4, gpl20, ICAM3, DC-SIGN, PFMSP 1-19 and PFMSP 1-42.
These and other aspects, advantages, and features of the invention will become apparent from the following figures and detailed description of the specific embodiments.
DESCRIPTION OF THE SEQUENCES
SEQ ID NO: 1. Amino acid sequence of azurin from Pseudomonas aeruginosa(A\a GIu Cys Ser VaI Asp He GIn GIy Asn Asp GIn Met GIn Phe Asn Thr Asn Ala He Thr VaI Asp Lys Ser Cys Lys GIn Phe Thr VaI Asn Leu Ser His Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu He GIy Ser GIy GIu Lys Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr Phe Pro GIy His Ser Ala Leu Met Lys GIy Thr Leu Thr Leu Lys). SEQ ID NO: 2. Amino acid sequence of plastocyanin from Phormidium lαminosum
(GIu Thr Phe Thr VaI Lys Met GIy Ala Asp Ser GIy Leu Leu GIn Phe GIu Pro Ala Asn VaI Thr VaI His Pro GIy Asp Thr VaI Lys Trp VaI Asn Asn Lys Leu Pro Pro His Asn He Leu Phe Asp Asp Lys GIn VaI Pro GIy Ala Ser Lys GIu Leu Ala Asp Lys Leu Ser His Ser GIn Leu Met Phe Ser Pro GIy GIu Ser Tyr GIu He Thr Phe Ser Ser Asp Phe Pro Ala GIy Thr Tyr Thr Tyr Tyr Cys Ala Pro His Arg GIy Ala GIy Met VaI GIy Lys He Thr VaI GIu GIy).
SEQ ID NO: 3. Amino acid sequence of rusticyanin from Thiobαcillus ferrooxidαns (GIy Thr Leu Asp Thr Thr Trp Lys GIu Ala Thr Leu Pro GIn VaI Lys Ala Met Leu GIu Lys Asp Thr GIy Lys VaI Ser GIy Asp Thr VaI Thr Tyr Ser GIy Lys Thr VaI His VaI VaI Ala Ala Ala VaI Leu Pro GIy Phe Pro Phe Pro Ser Phe GIu VaI His Asp Lys Lys Asn Pro Thr Leu GIu He Pro Ala GIy Ala Thr VaI Asp VaI Thr Phe He Asn Thr Asn Lys GIy Phe GIy His Ser Phe Asp He Thr Lys Lys GIy Pro Pro Tyr Ala VaI Met Pro VaI He Asp Pro He VaI Ala GIy Thr GIy Phe Ser Pro VaI Pro Lys Asp GIy Lys Phe GIy Tyr Thr Asp Phe Thr Trp His Pro Thr AIa GIy Thr Tyr Tyr Tyr VaI Cys GIn He Pro GIy His Ala Ala Thr GIy Met Phe GIy Lys He VaI VaI Lys).
SEQ ID NO: 4. Amino acid sequence of pseudoazurin from Achromobacter cycloclastes (Ala Asp Phe GIu VaI His Met Leu Asn Lys GIy Lys Asp GIy Ala Met VaI Phe GIu Pro Ala Ser Leu Lys VaI Ala Pro GIy Asp Thr VaI Thr Phe He Pro Thr Asp Lys GIy His Asn VaI GIu Thr He Lys GIy Met He Pro Asp GIy Ala GIu Ala Phe Lys Ser Lys He Asn GIu Asn Tyr Lys VaI Thr Phe Thr Ala Pro GIy VaI Tyr GIy VaI Lys Cys Thr Pro His Tyr GIy Met GIy Met VaI GIy VaI VaI GIn VaI GIy Asp Ala Pro Ala Asn Leu GIu Ala VaI Lys GIy Ala Lys Asn Pro Lys Lys Ala GIn GIu Arg Leu Asp Ala Ala Leu Ala Ala Leu GIy Asn). SEQ ID NO: 5. Amino acid sequence of azurin from Alcaligenes faecalis (Ala Cys
Asp VaI Ser He GIu GIy Asn Asp Ser Met GIn Phe Asn Thr Lys Ser He VaI VaI Asp Lys Thr Cys Lys GIu Phe Thr He Asn Leu Lys His Thr GIy Lys Leu Pro Lys Ala Ala Met GIy His Asn VaI VaI VaI Ser Lys Lys Ser Asp GIu Ser Ala VaI Ala Thr Asp GIy Met Lys Ala GIy Leu Asn Asn Asp Tyr VaI Lys Ala GIy Asp GIu Arg VaI He Ala His Thr Ser VaI He GIy GIy GIy GIu Thr Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu Asp Tyr Ala Phe Phe Cys Ser Phe Pro GIy His Trp Ser He Met Lys GIy Thr He GIu Leu GIy Ser).
SEQ ID NO: 6. Amino acid sequence of azurin from Achromobacter xylosoxidans ssp. denitrificans I (Ala GIn Cys GIu Ala Thr He GIu Ser Asn Asp Ala Met GIn Tyr Asn Leu Lys GIu Met VaI VaI Asp Lys Ser Cys Lys GIn Phe Thr VaI His Leu Lys His VaI GIy Lys Met Ala Lys VaI Ala Met GIy His Asn Trp VaI Leu Thr Lys GIu Ala Asp Lys GIn GIy VaI Ala Thr Asp GIy Met Asn Ala GIy Leu Ala GIn Asp Tyr VaI Lys Ala GIy Asp Thr Arg VaI He Ala His Thr Lys VaI He GIy GIy GIy GIu Ser Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Thr Pro GIy GIu Ala Tyr Ala Tyr Phe Cys Ser Phe Pro GIy His Trp Ala Met Met Lys GIy Thr Leu Lys Leu Ser Asn). SEQ ID NO: 7. Amino acid sequence of azurin from Bordetella bronchiseptica (Ala
GIu Cys Ser VaI Asp He Ala GIy Thr Asp GIn Met GIn Phe Asp Lys Lys Ala He GIu VaI Ser Lys Ser Cys Lys GIn Phe Thr VaI Asn Leu Lys His Thr GIy Lys Leu Pro Arg Asn VaI Met GIy His Asn Trp VaI Leu Thr Lys Thr Ala Asp Met GIn Ala VaI GIu Lys Asp GIy He Ala Ala GIy Leu Asp Asn GIn Tyr Leu Lys Ala GIy Asp Thr Arg VaI Leu Ala His Thr Lys VaI Leu GIy GIy GIy GIu Ser Asp Ser VaI Thr Phe Asp VaI Ala Lys Leu Ala Ala GIy Asp Asp Tyr Thr Phe Phe Cys Ser Phe Pro GIy His GIy Ala Leu Met Lys GIy Thr Leu Lys Leu VaI Asp). SEQ ID NO: 8. Amino acid sequence of azurin from Methylomonas sp. J (Ala Ser Cys GIu Thr Thr VaI Thr Ser GIy Asp Thr Met Thr Tyr Ser Thr Arg Ser He Ser VaI Pro Ala Ser Cys Ala GIu Phe Thr VaI Asn Phe GIu His Lys GIy His Met Pro Lys Thr GIy Met GIy His Asn Trp VaI Leu Ala Lys Ser Ala Asp VaI GIy Asp VaI Ala Lys GIu GIy Ala His Ala GIy Ala Asp Asn Asn Phe VaI Thr Pro GIy Asp Lys Arg VaI He Ala Phe Thr Pro He He GIy GIy GIy GIu Lys Thr Ser VaI Lys Phe Lys VaI Ser Ala Leu Ser Lys Asp GIu Ala Tyr Thr Tyr Phe Cys Ser Tyr Pro GIy His Phe Ser Met Met Arg GIy Thr Leu Lys Leu GIu GIu).
SEQ ID NO: 9. Amino acid sequence of azurin from Neisseria meningitides Z2491 (Cys Ser GIn GIu Pro Ala Ala Pro Ala Ala GIu Ala Thr Pro Ala Ala GIu Ala Pro Ala Ser GIu Ala Pro Ala Ala GIu Ala Ala Pro Ala Asp Ala Ala GIu Ala Pro Ala Ala GIy Asn Cys Ala Ala Thr VaI GIu Ser Asn Asp Asn Met GIn Phe Asn Thr Lys Asp He GIn VaI Ser Lys Ala Cys Lys GIu Phe Thr He Thr Leu Lys His Thr GIy Thr GIn Pro Lys Thr Ser Met GIy His Asn He VaI He GIy Lys Thr GIu Asp Met Asp GIy He Phe Lys Asp GIy VaI GIy Ala Ala Asp Thr Asp Tyr VaI Lys Pro Asp Asp Ala Arg VaI VaI Ala His Thr Lys Leu He GIy GIy GIy GIu GIu Ser Ser Leu Thr Leu Asp Pro Ala Lys Leu Ala Asp GIy GIu Tyr Lys Phe Ala Cys Thr Phe Pro GIy His GIy Ala Leu Met Asn GIy Lys VaI Thr Leu VaI Asp).
SEQ ID NO: 10. Amino acid sequence of azurin from Pseudomonas fluorescen (Ala GIu Cys Lys Thr Thr He Asp Ser Thr Asp GIn Met Ser Phe Asn Thr Lys Ala He GIu He Asp Lys Ala Cys Lys Thr Phe Thr VaI GIu Leu Thr His Ser GIy Ser Leu Pro Lys Asn VaI Met GIy His Asn Leu VaI He Ser Lys GIn Ala Asp Met GIn Pro He Ala Thr Asp GIy Leu Ser Ala GIy He Asp Lys Asn Tyr Leu Lys GIu GIy Asp Thr Arg VaI He Ala His Thr Lys VaI He GIy Ala GIy GIu Lys Asp Ser Leu Thr He Asp VaI Ser Lys Leu Asn Ala Ala GIu Lys Tyr GIy Phe Phe Cys Ser Phe Pro GIy His He Ser Met Met Lys GIy Thr VaI Thr Leu Lys).
SEQ ID NO: 11. Amino acid sequence of azurin from Pseudomonas syringae (Met Ala Ser GIy GIn Leu Leu Ala Ala GIu Cys Ser Ala Thr VaI Asp Ser Thr Asp GIn Met Met Tyr Asp Thr Lys Ala He GIn He Asp Lys Ser Cys Lys GIu Phe Thr Leu Asn Leu Thr His Ser GIy Ser Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Lys Lys Ala Asp Ala Ser Ala He Thr Thr Asp GIy Met Ser VaI GIy He Asp Lys Asp Tyr VaI Lys Pro Asp Asp Thr Arg VaI He Ala His Thr Lys He He GIy Ala GIy GIu Asn Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Asp Pro Ala GIu Asp Tyr GIn Phe Phe Cys Thr Phe Pro GIy His He Ser Met Met Lys GIy Ala VaI Thr Leu Lys). SEQ ID NO: 12. Amino acid sequence of azurin from Xylella fastidiosa 9a5c (Lys Thr Cys Ala VaI Thr He Ser Ala Asn Asp GIn Met Lys Phe Asp GIn Asn Thr Ue Lys He Ala Ala GIu Cys Thr His VaI Asn Leu Thr Leu Thr His Thr GIy Lys Lys Ser Ala Arg VaI Met GIy His Asn Trp VaI Leu Thr Lys Thr Thr Asp Met GIn Ala VaI Ala Leu Ala GIy Leu His Ala Thr Leu Ala Asp Asn Tyr VaI Pro Lys Ala Asp Pro Arg VaI He Ala His Thr Ala He He GIy GIy GIy GIu Arg Thr Ser He Thr Phe Pro Thr Asn Thr Leu Ser Lys Asn VaI Ser Tyr Thr Phe Phe Cys Ser Phe Pro GIy His Trp Ala Leu Met Lys GIy Thr Leu Asn Phe GIy GIy).
SEQ ID NO: 13 Amino acid sequence of stellacyanin from Cucumis sativus (Met GIn Ser Thr VaI His He VaI GIy Asp Asn Thr GIy Trp Ser VaI Pro Ser Ser Pro Asn Phe Tyr Ser GIn Trp Ala Ala GIy Lys Thr Phe Arg VaI GIy Asp Ser Leu GIn Phe Asn Phe Pro Ala Asn Ala His Asn VaI His GIu Met GIu Thr Lys GIn Ser Phe Asp Ala Cys Asn Phe VaI Asn Ser Asp Asn Asp VaI GIu Arg Thr Ser Pro VaI He GIu Arg Leu Asp GIu Leu GIy Met His Tyr Phe VaI Cys Thr VaI GIy Thr His Cys Ser Asn GIy GIn Lys Leu Ser He Asn VaI VaI Ala Ala Asn Ala Thr VaI Ser Met Pro Pro Pro Ser Ser Ser Pro Pro Ser Ser VaI Met Pro Pro Pro VaI Met Pro Pro Pro Ser Pro Ser).
SEQ ID NO: 14. Amino acid sequence of auracyanin A from Chloroflexus aurantiacus (Met Lys He Thr Leu Arg Met Met VaI Leu Ala VaI Leu Thr Ala Met Ala Met VaI Leu Ala Ala Cys GIy GIy GIy GIy Ser Ser GIy GIy Ser Thr GIy GIy GIy Ser GIy Ser GIy Pro VaI Thr He GIu He GIy Ser Lys GIy GIu GIu Leu Ala Phe Asp Lys Thr GIu Leu Thr VaI Ser Ala GIy GIn Thr VaI Thr He Arg Phe Lys Asn Asn Ser Ala VaI GIn GIn His Asn Trp He Leu VaI Lys GIy GIy GIu Ala GIu Ala Ala Asn He Ala Asn Ala GIy Leu Ser Ala GIy Pro Ala Ala Asn Tyr Leu Pro Ala Asp Lys Ser Asn He He Ala GIu Ser Pro Leu Ala Asn GIy Asn GIu Thr VaI GIu VaI Thr Phe Thr Ala Pro Ala Ala GIy Thr Tyr Leu Tyr He Cys Thr VaI Pro GIy His Tyr Pro Leu Met GIn GIy Lys Leu VaI VaI Asn). SEQ ID NO: 15. Amino acid sequence of auracyanin B from Chloroflexus aurantiacus (Ala Ala Asn Ala Pro GIy GIy Ser Asn VaI VaI Asn GIu Thr Pro Ala GIn Thr VaI GIu VaI Arg Ala Ala Pro Asp Ala Leu Ala Phe Ala GIn Thr Ser Leu Ser Leu Pro Ala Asn Thr VaI VaI Arg Leu Asp Phe VaI Asn GIn Asn Asn Leu GIy VaI GIn His Asn Trp VaI Leu VaI Asn GIy GIy Asp Asp VaI Ala Ala Ala VaI Asn Thr Ala Ala GIn Asn Asn Ala Asp Ala Leu Phe VaI Pro Pro Pro Asp Thr Pro Asn Ala Leu Ala Trp Thr Ala Met Leu Asn Ala GIy GIu Ser GIy Ser VaI Thr Phe Arg Thr Pro Ala Pro GIy Thr Tyr Leu Tyr He Cys Thr Phe Pro GIy His Tyr Leu Ala GIy Met Lys GIy Thr Leu Thr VaI Thr Pro). SEQ ID NO: 16. Amino acid sequence of cucumber basic protein from Cucumis sativus (Ala VaI Tyr VaI VaI GIy GIy Ser GIy GIy Tip Thr Phe Asn Thr GIu Ser Tip Pro Lys GIy Lys Arg Phe Arg Ala GIy Asp He Leu Leu Phe Asn Tyr Asn Pro Ser Met His Asn VaI VaI VaI VaI Asn GIn GIy GIy Phe Ser Thr Cys Asn Thr Pro Ala GIy Ala Lys VaI Tyr Thr Ser GIy Arg Asp GIn He Lys Leu Pro Lys GIy GIn Ser Tyr Phe He Cys Asn Phe Pro GIy His Cys GIn Ser GIy Met Lys He Ala VaI Asn Ala Leu).
SEQ ID NO: 17. Amino acid sequence of Laz from Neisseria gonorrhoeae F62 (Cys Ser GIn GIu Pro Ala Ala Pro Ala Ala GIu Ala Thr Pro Ala GIy GIu Ala Pro Ala Ser GIu Ala Pro Ala Ala GIu Ala Ala Pro Ala Asp Ala Ala GIu Ala Pro Ala Ala GIy Asn Cys Ala Ala Thr VaI GIu Ser Asn Asp Asn Met GIn Phe Asn Thr Lys Asp He GIn VaI Ser Lys Ala Cys Lys GIu Phe Thr He Thr Leu Lys His Thr GIy Thr GIn Pro Lys Ala Ser Met GIy His Asn Leu VaI He Ala Lys Ala GIu Asp Met Asp GIy VaI Phe Lys Asp GIy VaI GIy Ala Ala Asp Thr Asp Tyr VaI Lys Pro Asp Asp Ala Arg VaI VaI Ala His Thr Lys Leu He GIy GIy GIy GIu GIu Ser Ser Leu Thr Leu Asp Pro Ala Lys Leu Ala Asp GIy Asp Tyr Lys Phe Ala Cys Thr Phe Pro GIy His GIy Ala Leu Met Asn GIy Lys VaI Thr Leu VaI Asp).
SEQ ID NO: 18. Amino acid sequence of the azurin from Vibrio par ahaemolyticus (Met Ser Leu Arg He Leu Ala Ala Thr Leu Ala Leu Ala GIy Leu Ser Phe GIy Ala GIn Ala Ser Ala GIu Cys GIu VaI Ser He Asp Ala Asn Asp Met Met GIn Phe Ser Thr Lys Thr Leu Ser VaI Pro Ala Thr Cys Lys GIu VaI Thr Leu Thr Leu Asn His Thr GIy Lys Met Pro Ala GIn Ser Met GIy His Asn VaI VaI He Ala Asp Thr Ala Asn He GIn Ala VaI GIy Thr Asp GIy Met Ser Ala GIy Ala Asp Asn Ser Tyr VaI Lys Pro Asp Asp GIu Arg VaI Tyr Ala His Thr Lys VaI VaI GIy GIy GIy GIu Ser Thr Ser He Thr Phe Ser Thr GIu Lys Met Thr Ala GIy GIy Asp Tyr Ser Phe Phe Cys Ser Phe Pro GIy His Trp Ala He Met GIn GIy Lys Phe GIu Phe Lys).
SEQ ID NO: 19. Amino acid sequence of cytochrome c from Homo sapiens (GIy Asp VaI GIu Lys GIy Lys Lys He Phe He Met Lys Cys Ser GIn Cys His Thr VaI GIu Lys GIy GIy Lys His Lys Thr GIy Pro Asn Leu His GIy Leu Phe GIy Arg Lys Thr GIy GIn Ala Pro GIy Tyr Ser Tyr Thr Ala Ala Asn Lys Asn Lys GIy He He Trp GIy GIu Asp Thr Leu Met GIu Tyr Leu GIu Asn Pro Lys Lys Tyr He Pro GIy Thr Lys Met He Phe VaI GIy He Lys Lys Lys GIu GIu Arg Ala Asp Leu He Ala Tyr Leu Lys Lys Ala Thr Asn GIu). SEQ ID NO: 20. Amino acid sequence of cytochrome f from cyanobacteria
Phormidium laminosum (Met Asn Phe Lys VaI Cys Ser Phe Pro Ser Arg Arg GIn Ser He Ala Ala Phe VaI Arg VaI Leu Met VaI He Leu Leu Thr Leu GIy Ala Leu VaI Ser Ser Asp VaI Leu Leu Pro GIn Pro Ala Ala Ala Tyr Pro Phe Tip Ala GIn GIn Asn Tyr Ala Asn Pro Arg GIu Ala Thr GIy Arg He VaI Cys Ala Asn Cys His Leu Ala Ala Lys Pro Ala GIu He GIu VaI Pro GIn Ala VaI Leu Pro Asp Ser VaI Phe Lys Ala VaI VaI Lys He Pro Tyr Asp His Ser VaI GIn GIn VaI GIn Ala Asp GIy Ser Lys GIy Pro Leu Asn VaI GIy Ala VaI Leu Met Leu Pro GIu GIy Phe Thr He Ala Pro GIu Asp Arg He Pro GIu GIu Met Lys GIu GIu VaI GIy Pro Ser Tyr Leu Phe GIn Pro Tyr Ala Asp Asp Lys GIn Asn He VaI Leu VaI GIy Pro Leu Pro GIy Asp GIn Tyr GIu GIu He VaI Phe Pro VaI Leu Ser Pro Asn Pro Ala Thr Asn Lys Ser VaI Ala Phe GIy Lys Tyr Ser He His Leu GIy Ala Asn Arg GIy Arg GIy GIn He Tyr Pro Thr GIy GIu Lys Ser Asn Asn Ala VaI Tyr Asn Ala Ser Ala Ala GIy VaI He Thr Ala He Ala Lys Ala Asp Asp GIy Ser Ala GIu VaI Lys He Arg Thr GIu Asp GIy Thr Thr He VaI Asp Lys He Pro Ala GIy Pro GIu Leu He VaI Ser GIu GIy GIu GIu VaI Ala Ala GIy Ala Ala Leu Thr Asn Asn Pro Asn VaI GIy GIy Phe GIy GIn Lys Asp Thr GIu He VaI Leu GIn Ser Pro Asn Arg VaI Lys GIy Arg He Ala Phe Leu Ala Ala He Thr Leu Thr GIn He Leu Leu VaI Leu Lys Lys Lys GIn VaI GIu Arg VaI GIn Ala GIy Arg Asp Asp Leu Leu Lys Ala Ala Phe He Ala GIy). SEQ ID NO: 21. Amino acid sequence of cytochrome C551 from Pseudomonas aeruginosa (GIu Asp Pro GIu VaI Leu Phe Lys Asn Lys GIy Cys VaI Ala Cys His Ala He Asp Thr Lys Met VaI GIy Pro Ala Tyr Lys Asp VaI Ala Ala Lys Phe Ala GIy GIn Ala GIy Ala GIu Ala GIu Leu Ala GIn Arg He Lys Asn GIy Ser GIn GIy VaI Trp GIy Pro He Pro Met Pro Pro Asn Ala VaI Ser Asp Asp GIu Ala GIn Thr Leu Ala Lys Trp VaI Leu Ser GIn Lys). SEQ ID NO: 22. Amino acid sequence of the H.8 region of Laz from Neisseria gonorrhoeae F62 (Cys Ser GIn GIu Pro Ala Ala Pro Ala Ala GIu Ala Thr Pro Ala GIy GIu Ala Pro Ala Ser GIu Ala Pro Ala Ala GIu Ala Ala Pro Ala Asp Ala Ala GIu Ala Pro Ala Ala).
SEQ ID NO: 23 is the amino acid sequence of the azurin from Bordetella pertussis (Ala GIu Cys Ser VaI Asp He Ala GIy Thr Asp GIn Met GIn Phe Asp Lys Lys Ala He GIu VaI Ser Lys Ser Cys Lys GIn Phe Thx VaI Asn Leu Lys His Thr GIy Lys Leu Pro Arg Asn VaI Met GIy His Asn Trp VaI Leu Thr Lys Thr Ala Asp Met GIn Ala VaI GIu Lys Asp GIy He Ala Ala GIy Leu Asp Asn GIn Tyr Leu Lys Ala GIy Asp Thr Arg VaI Leu Ala His Thr Lys VaI Leu GIy GIy GIy GIu Ser Asp Ser VaI Thr Phe Asp VaI Ala Lys Leu Ala Ala GIy Asp Asp Tyr Thr Phe Phe Cys Ser Phe Pro GIy His GIy Ala Leu Met Lys GIy Thr Leu Lys Leu VaI Asp). SEQ ID NO: 24. Amino acid sequence of amino acids 57- 89 of auracyanin B of Chloroβexus aurantiacus (His Asn Trp VaI Leu VaI Asn GIy GIy Asp Asp VaI Ala Ala Ala VaI Asn Thr Ala Ala GIn Asn Asn Ala Asp Ala Leu Phe VaI Pro Pro Pro Asp).
SEQ ID NO: 25. Amino acid sequence of amino acids 51-77 of P 'seudomonas syringae azurin (Ser Lys Lys Ala Asp Ala Ser Ala He Thr Thr Asp GIy Met Ser VaI GIy He Asp Lys Asp Tyr VaI Lys Pro Asp Asp).
SEQ ID NO: 26. Amino acid sequence of amino acids 89-115 of Neisseria meningitides Laz (He GIy Lys Thr GIu Asp Met Asp GIy He Phe Lys Asp GIy VaI GIy Ala Ala Asp Thr Asp Tyr VaI Lys Pro Asp Asp). SEQ ID NO: 27. Amino acid sequence of amino acids 52-78 of Vibrio parahaemolyticus azurin (Ala Asp Thr Ala Asn He GIn Ala VaI GIy Thr Asp GIy Met Ser Ala GIy Ala Asp Asn Ser Tyr VaI Lys Pro Asp Asp).
SEQ HD NO: 28. Amino acid sequence of amino acids 51-77 of Bordetella bronchiseptica azurin (Thr Lys Thr Ala Asp Met GIn Ala VaI GIu Lys Asp GIy He Ala Ala GIy Leu Asp Asn GIn Tyr Leu Lys Ala GIy Asp).
SEQ ID NO: 29 is the amino acid sequence of the 50-77 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 30 is the amino acid sequence of the 50-67 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy).
SEQ ID NO: 31 is the amino acid sequence of the 36-128 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu He GIy Ser GIy GIu Lys Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr Phe Pro GIy His Ser Ala Leu Met Lys GIy Thr Leu Thr Leu Lys).
SEQ ID NO: 32 is the amino acid sequence of the 36-89 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu He GIy Ser). SEQ ID NO: 33 is the amino acid sequence of the 36-77 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 34 is the forward primer to PCR amplify the Laz-encoding gene (laz) of
Neisseria gonorrhoeae (ccggaattcc ggcagggatg ttgtaaatat ccg).
SEQ ID NO: 35 is the reverse primer to PCR amplify the Laz-encoding gene (laz) of Neisseria gonorrhoeae (ggggtaccgc cgtggcaggc atacagcatt tcaatcgg).
SEQ ID NO: 36 is the forward primer to PCR amplify a 3.1 kb fragment of pUC18- laz (ggcagcaggg gcttcggcag catctgc).
SEQ ID NO: 37 is the reverse primer to PCR amplify a 3.1 kb fragment of pucl8-laz (ctgcaggtcg actctagagg atcccg).
SEQ ID NO: 38 is the forward primer to PCR amplify a 0.4 kb fragment of pUC19- paz (gccgagtgct cggtggacat ccagg). SEQ ID NO: 39 is the reverse primer to PCR amplify a 0.4 kb fragment of pUCl 9- paz (tactcgagtc acttcagggt cagggtg).
SEQ ID NO: 40 is the forward primer for pGST-azu 36-128 (ggcaacctgc cgaagaacgt catgggc).
SEQ ID NO: 41 is the reverse primer for pGST-azu 36-128 (cggaattcgc atcacttcag ggtcaggg).
SEQ ID NO: 42 is the forward primer for pGST-azu 36-89 (ccaagctgat cggctcgtga gagaaggact cggtgacc).
SEQ ID NO: 43 is the reverse primer for pGST-azu 36-89 (ggtcaccgag tccttctctc acgagccgat cagcttgg). SEQ ID NO: 44 is the forward primer for pGST-azu 88-113 (cggggatccc cggctcgggc gagaaggac).
SEQ ID NO: 45 is the reverse primer for pGST-azu 88-113 (cgggaattct ccacttcagg gtcagggtg).
SEQ ID NO: 46 is an oligonucleotide for site directed mutagenesis for the preparation of pGST-azu 88-113 (gttcttctgc acctagccgg gccactccg).
SEQ ID NO: 47 is an oligonucleotide for site directed mutagenesis for the preparation of pGST-azu 88-1 13 (cggagtggcc cggctaggtg cagaagaac). SEQ ID NO: 48 is the amino acid sequence of the 96-113 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr).
SEQ ID NO: 49 is the amino acid sequence of the 88-113 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (GIy Ser GIy GIu Lys Asp Ser VaI Thr Phe Asp VaI Ser Lys Leu Lys GIu GIy GIu GIn Tyr Met Phe Phe Cys Thr).
SEQ ID NO: 50 is the amino acid sequence of the 36-88 amino acid fragment of wt- azurin from Pseudomonas aeruginosa (Pro GIy Asn Leu Pro Lys Asn VaI Met GIy His Asn Trp VaI Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp Ser Arg VaI He Ala His Thr Lys Leu Ue GIy).
SEQ ID NO: 51 is the amino acid sequence of a variant of the azurin truncation p28 (Leu Ser Thr Ala Ala Asp Met GIn Ala VaI VaI Thr Asp Thr Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 52 is the amino acid sequence of a variant of the azurin truncation p28 (Leu Ser Thr Ala Ala Asp Leu GIn GIy VaI VaI Thr Asp GIy Leu Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 53 is the amino acid sequence of a variant of the azurin truncation p28 (Leu Ser Thr Ala Ala Asp VaI GIn GIy VaI VaI Thr Asp GIy VaI Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 54 is the amino acid sequence of a modified cupredoxin derived peptide
(Asp Asp Pro Lys Leu Tyr Asp Lys Asp Leu GIy Ser Ala Met GIy Asp Thr VaI VaI GIy GIn Met Asp Ala Ala Thr Ser Leu).
SEQ ID NO: 55 is the amino acid sequence of a modified cupredoxin derived peptide (Acetylation- Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp-amidation).
SEQ ID NO: 56 is the amino acid sequence of a hexapeptide (VaI Ser Pro Pro Ala Arg).
SEQ ID NO: 57 is the amino acid sequence of a hexapeptide (Tyr Thr Pro Pro Ala Leu). SEQ ID NO: 58 is the amino acid sequence of a hexapeptide (Phe Ser Phe Phe Ala
Phe). SEQ ID NO: 59 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Thr Pro GIy Cys).
SEQ ID NO: 60 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Cys GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 61 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Cys Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 62 is the amino acid sequence of a modified cupredoxin-derived peptide
(Leu Ser Thr Ala Cys Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 63 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Thr Met GIn Cys VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 64 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Thr Met GIn GIy Cys VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 65 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asn Thr GIn GIy Cys VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 66 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asn Thr GIn GIy VaI Cys Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 67 is the amino acid sequence of a modified cupredoxin-derived peptide
(Leu Ser Thr Ala Ala Asp Met Thr Ala VaI Cys Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 68 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Thr Ala VaI VaI Cys Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 69 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn Thr VaI VaI Cys Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 70 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn Thr VaI VaI Thr Cys GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 71 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn Ala Thr VaI Thr Cys GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 72 is the amino acid sequence of a modified cupredoxin-derived peptide
(Leu Ser Thr Ala Ala Asp Met GIn Ala Thr VaI Thr Asp Cys Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 73 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI Thr Ala Asp Cys Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 74 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI Thr Ala Asp GIy Cys Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 75 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asn GIy Cys Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 76 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Ala Thr Met GIy Ser GIy Leu Cys Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 77 is the amino acid sequence of a modified cupredoxin-derived peptide
(Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp Leu Thr Ala Ser GIy Leu Cys Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 78 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met GIn GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 79 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Trp GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 80 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Trp Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 81 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Thr Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 82 is the amino acid sequence of a modified cupredoxin-derived peptide
(Leu Ser Trp Ala Ala Asp Met Trp GIy VaI VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 83 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met GIn GIy VaI VaI Trp Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 84 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met GIn GIy VaI VaI Thr Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 85 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Trp GIy VaI VaI Trp Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 86 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Thr Ala Ala Asp Met Trp GIy VaI VaI Thr Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 87 is the amino acid sequence of a modified cupredoxin-derived peptide
(Leu Ser Thr Ala Ala Asp Met GIn GIy VaI VaI Trp Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 88 is the amino acid sequence of a modified cupredoxin-derived peptide (Leu Ser Trp Ala Ala Asp Met Trp GIy VaI VaI Trp Asp Trp Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp). SEQ ID NO: 89 is the amino acid sequence of a modified cupredoxin-derived peptide (X1 Ser X2 Ala Ala Asp X3 X4 X5 VaI VaI X6 Asp X7X8 Ala Ser GIy Leu Asp Lys Asp Tyr Leu Ly s Pro Asp X9).
SEQ ID NO: 90 is the amino acid sequence of a modified cupredoxin-derived peptide (Xi Asp Pro Lys Leu Tyr Asp Lys Asp Leu GIy Ser Ala X2 X3 Asp X4 VaI VaI X5 X6 X7 Asp Ala Ala X8 Ser X9 ).
SEQ ID NO: 91 is the amino acid sequence of pi 8b, the 60-77 amino acid fragment of wt-azurin from Pseudomonas aeruginosa (VaI Thr Asp GIy Met Ala Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp) SEQ ID NO: 92 is the amino acid sequence of the 10 C-terminal amino acids of p28
(Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
SEQ ID NO: 93 is the amino acid sequence of the 12 C-terminal amino acids of p28 (Ser GIy Leu Asp Lys Asp Tyr Leu Lys Pro Asp Asp).
BRIEF DESCRIPTION OF THE FIGURES
Figure 1. Figure 1 depicts confocal microscopy images of malignant and normal cells incubated with p28 labeled with Alexafluor® 568 and the cells are then stained with DAPI. The indicated cell lines were incubated in the absence (negative control) or presence (p28) of 20μM Alexafluor® 568 labeled p28 for 2h at 37°C. The images are indicative of amount of cellular entry observed. Figure IA depicts the Alexafluor 568 fluorescence and control fluorescence of human melanoma, pancreatic, breast (BCA-I), breast (MCF-7), glioblastoma, astrocytoma, lung and prostrate cancer cells. Figure IB depicts the Alexafluor® 568 fluorescence and control fluorescence of human normal fibroblast, pancreas and breast cells. Figure 1C depicts the Alexafluor® 568 fluorescence and control fluorescence of human umbilical vein endothelial cells (HUVEC).
Figure 2. Figure 2 depicts the capillary tube formation by HUVEC cells plated on Matrigel® in the presence or absence of p28. Culture media contained 20ng/ml VEGF. Figure 2A shows images of HUVEC cells incubated for 4h at 37°C with 0.1 OμM, 0.30μM, 0.92μM, 2.77μM, 8.33μM, 25μM and 75μM of p28, and then stained with calcein AM and visualized using fluorescence microscopy. In Figure 2B, the graph shows the average number of tubes formed in peptide treated and control (untreated) cells.
Figure 3. Figure 3 depicts the results of the scratch wound HUVEC migration assay. In Figures 3A-C show the fixed cells that were stained for F-actin and nuclei. In Figure 3 A, HUVEC cells at 90% confluence were scratched using a 1 ml plastic pipette tip. In Figure 3B, the HUVEC cells were scratched and then incubated in the culture media containing 20ng/ml VEGF for 24h at 37°C in the absence of p28. In Figure 3 C, the HUVEC cells were scratched and then incubated for 24h at 37°C in the presence of 25 μM p28. The insets of Figures 3A-C show the cell density in the area away from the scored area. In Figure 3D, a bar graph indicates the average # of cells in 20 different fields (20X) of the scratched area in control and p28 treated wells (Figures 3B and C). Data represent mean ± SEM. * indicates the differences are statistically significant.
Figure 4. Figure 4 depicts the images of the localization of cell structural proteins with and without p28 treatment. HUVEC cells were plated on Matrigel®-coated cover slips, incubated in the culture media containing 20ng/ml VEGF in the presence or absence of p28 peptide (25μM) for 4 and 24h, fixed, and processed for staining of CD31 /PECAM-I, paxillin, Fak (focal adhesion kinase), vinculin, WASP (Wiskott Aldrich Syndrome protein) and β- catenin. Each figure pertains to the detection of particular structural protein: Figure 4 A is CD31/PECAM-1; Figure 4B is paxillin; Figure 4C is Fak; Figure 4D is WASP; Figure 4E is vinculin; and Figure 4F is β-catenin. Each figure is divided into four panes which show the image of the localization of the fluorescent markers used. Each pane is numbered to indicate the fluorescent marker detected: 1 = F-actin; 2 = DAPI; 3 = FITC-Protein of interest; 4 = merged image. Arrows indicate the localization of the protein of interest.
Figure 5. Figure 5 depicts Mel-2 cells which were treated with increasing concentrations of p28 for 24, 48, and 72 hours. The number of cells in treated and control wells were counted using a Coulter counter. Data represent percentage of cell growth inhibition when compared to control cultures at the time point.
Figure 6. Depicts the results when Mel-2 cells were injected subcutaneously in the left flank (about 1 million cells/animal). Animals received p28 at the indicated dose at the time of injection. Figure 6A shows the incidence of tumor occurrence after initiation of treatment with a graph indicating % of tumor free animals at days post treatment with Mel-2 cells. Figure 6B shows the rumor size after initiation of treatment with a graph indicating the average volume of the tumors (cm3) at days post treatment with Mel-2 cells.
Figure 7. Figure 7 depicts surface plasmon resonance binding titrations depicting the interactions of Azurin, H.8-azurin (H.8-Az), Laz, and GST-azurin (GST- Azu) constructs with MSPl -19 and MSP 1-42. (A) Binding curves demonstrating the interactions of azurin and its analogues with MSPl -19 immobilized on carboxymethyldextran coated gold sensor chips (MSPl -19-CM5). Concentration dependent binding of the azurin proteins to MSPl -19 was determined via injection of various concentrations (0.05-300 nM) over the sensor surface and the extent of binding was evaluated as a function of the equilibrium resonance response value measured in resonance units (RU). While H.8-Az and Laz bound somewhat more strongly than azurin, no binding was seen with GST or H.8-GST. (B) In vitro binding titrations for immobilized MSP 1-42 with azurin and its analogues was followed in a similar manner to that for MSPl -19 as shown in (A). Relative binding affinities were determined via fitting the data to Req = Rmax/(l+(Kd/C)) with the curve fits connecting the data points in the graphs. The MSPl -19 binding Kd values are: 32.2 ± 2.4 nM (azurin), 26.2 ± 2.4 nM (Laz), 11.8 ± 0.3 nM (H.8-Az), and those for MSPl -42 binding are: 54.3 ± 7.6 nM (azurin), 45.6 ± 2.4 nM (Laz) and 14.3 ± 1.7 nM (H.8-Az). (C) Binding titrations for the interactions of GST-Azu fusion proteins over the MSP1-19-CM5 sensors surface demonstrate the recognition of GST-Azu 36-128 and GST-Azu 36-89 with MSP1-19. No binding was seen with GST or GST-Azu 88-113.
Figure 8. Figure 8 depicts inhibition of P. falciparum parasitemia (parasite growth within the RBC) by different concentrations, as shown, of Azurin, H.8-azurin (H.8-Az) and Laz. In these experiments, normal red blood cells were infected with schizonts in absence or in presence of the proteins at different concentrations, incubated overnight and the number of intracellular parasites was scored by thin blood smear and Giemsa staining.
Figure 9. Figure 9 depicts surface plasmon resonance binding curves for the binding of ICAMs (ICAM-I, ICAM-2, ICAM-3 and NCAM, inset) with immobilized azurin. Due to large nonspecific binding to the bare Au-CM5 chip, CM5 was added as an eluent to the running buffer (1 mg/ml CM5 to HBS-EP buffer). The selective recognition of azurin with ICAM-3, but not with ICAM-I or ICAM-2, is notable and the binding strength was 19.5 ± 5.4 nM. The Kd for NCAM binding with azurin, as shown in the inset, was 20 ± 5.0 nM. Figure 10. Figure 10 depicts the inhibition of HIV-I viral growth by azurin, H.8- azurin (H.8-Az) and Laz. These three proteins were incubated at different concentrations with PBMC followed by addition of the three subtypes of HIV-I. After 2 h incubation, the virus was removed but the proteins added back as described in Example 18. Suppression of virus growth was determined by ELISA assays of p24.
Figure 11. Figure 11 depicts surface plasmon resonance binding curves depicting the binding patterns of cupredoxins with CD4 and HIV-I gpl20. (A) SPR titration curves showing novel and specific binding of azurin, and GST-Azu 36-128 (shown as an inset) with immobilized CD4 on carboxymethyldextran coated gold sensor chips (CD4-CM5). HIV-I gpl20, HIV-I gag, and HIV-I nef served as the positive and negative controls respectively. Relative binding affinities were determined via fitting the data to Req = Rmax/(l+(Kd/C)) with the curve fits connecting the data points above. The CD4 binding Kd values are: 36.9 ± 2.0 nM (azurin), 0.34 ± 0.04 nM (GST-Azu 36-128), and 48.1 ± 3.1 nM (HIV-I gpl20). (B) The binding titrations when immobilized azurin (Az-CM5) is in contact with HIV proteins. Due to large nonspecific binding to the bare Au-CM5 chip, CM5 was added as an eluent to the running buffer (1 mg/ml CM5 to HBS-EP buffer). Curve fits gave Kd's of 25.1 ± 3.1 nM (CD4), and 8.9 ± 0.8 nM (HIV-I gpl20). (C) SPR curves for the binding of ICAMs (ICAM- 1, ICAM-2, ICAM-3 and NCAM, inset) with immobilized azurin were determined under similar conditions as for experiments in part (B). The selective recognition of azurin with ICAM-3, but not with ICAM-I or ICAM-2, is notable and the binding strength was 19.5 ± 5.4 nM. The Kd for NCAM binding with azurin, as shown in the inset, was 20 + 5.0 nM. (D) SPR binding competition studies with CD4 immobilized on CM5 sensor chips. Azurin + HIV-I gpl20 solutions were added at different azurin concentrations (0-4500 nM, [HIV-I gpl20] is 242 nM) to the sensor surface and the data were plotted as a ratio of resonances, % total response [Req (azurin+HIV-1 gpl20)/(Req/(HIV-l gpl20))]. GST- Azu 36-128 was titrated with HIV-I gpl20 to immobilized CD4 and analyzed in a similar manner. Competition data suggests 1 :1 stoichiometry of binding between azurin and GST- Azu 36-128 with immobilized CD4. Figure 12. Figure 12 depicts surface plasmon resonance binding titrations depicting the interactions of azurin, and GST- Azurin fusions with DC-SIGN. (A) Concentration dependent binding of azurin, ICAM-3, and GST- Azu 36-89 with DC-SIGN were determined via injection of various concentrations of the proteins (0 - 100 nM) over a DC-SIGN modified CM5 sensor surface and the extent of binding was evaluated as a function of the equilibrium resonance response value measured in resonance units (RU). (B) The binding titration curve of GST- Azu 88-113 with DC-SIGN using the same sensor chip and protocol as described for azurin in part A. The positive interaction of GST- Azu 88-113 with DC-SIGN suggests its potential role as the recognition sequence for azurin. The binding affinities (Kd) for azurin, ICAM-3 and GST- Azu 88-113 were determined by fitting the data to Req = Rmax/(l+(Kd/C)) and the curve fits connect the data points in these plots. The extrapolated Kd values are 0.83 ± 0.05 nM (azurin), 0.93 ± 0.39 nM (ICAM-3), and 5.98 ± 1.13 nM (GST- Azu 88-113).
Figure 13. Figure 13 depicts the effects of cupredoxin peptides on cancer cell viability. (In Fig. 13 A, effect of azurin (Azu 96-113) and plastocyanin (PIc 70-84) synthetic peptides on cell viability of Astrocytoma CCF-STTGl and Glioblastoma LN-229 cancer cell lines. In Fig. 13B, effect of different concentrations of plastocyanin (PIc 70-84) synthetic peptide on Melanoma UISO-Mel-2 cell viability. Cancer cells (2 x 104 cells per well in 96- well plates) were treated with the synthetic peptides at different concentrations for 24 h at 37°C. Data are presented as the percentage of cell viability as compared to that of untreated control (100% viability) In Fig. 13 C, cytotoxic activity of Azu 96-113 synthetic peptide towards Glioblastoma LN-229 cells. Cytotoxicity effects were determined by MTT assay. Cancer (2 x 104 cells per well in 96-well plates) were treated with various concentrations of Azu 96-113 (10, 25, 50, 75, 100 μM) for 24 h at 37°C. Percent cytotoxicity is expressed as percentage of cell death as compared to that of untreated control (0% cytotoxicity).
Figure 14. Effect of GST- Azu 36-128 and GST- Azu 88-113 on cell viability of MCF-7 cells. GST- Azu peptides were added at increasing concentrations (1.25, 6.25 and 12.5 μM) into 96 well plates containing 8 x 103 cancer cells per well, incubated at 37°C for 48 h and subsequently analyzed using MTT assay. GST and GST-Azu 36-89 at the same concentrations and untreated cells were run in parallel with GST-Azu 36-128 and GST-Azu 88-113 as controls.
Figures 15 A-C. Depict photographs showing penetration of azurin derived peptides, pi 8 and p28, into cancer cell lines of diverse histogenesis and their normal counterparts. (A) Photos showing penetration of Alexafluor 568 labeled p28 or pi 8 after 2hrs at 37°C. The cationic Arg8 was used as a control. (B) Graphs depicting flow cytometric analysis of the penetration of Alexafluor 568 labeled p28 or pl8 into the same cell lines after 2hrs at 37°C. (C) Graphs depicting fold increase over fluorescence from normal cells. Similar observations of p28 or pi 8 entry into 4 melanoma cell lines show a several fold increase over fluorescence from normal cells.
Figures 16 A and B. Depict photographs showing entry of azu 60-77 (pl8b) and azu 66-77 (pl2) into cancer and normal cells. Cells were incubated with alexafluor 568 labeled p 18b (A) or pi 2 (B) at 37°C for 2 hrs and images recorded by confocal microscopy. Figures 17 A and B. Graphs depicting cellular membrane toxicity of azurin and its peptides. (A) LDH leakage assay of UISOMeI- 2 cells exposure for 10 min to different concentrations of p28, pi 8 and azurin at 37°C. A standard lysis buffer (cytotox-one reagent) was included as a positive control. Changes in fluorescence following exposure were measured at k,x 560nm and kem 590nm. Lysis buffer was defined as 100% LDH release. Data represent % of positive fluorescence of control. Data are shown as mean ± SEM. (B) Hemoglobin leakage from human erythrocytes incubated with p28, pi 8 and azurin. Human erythrocytes were incubated with peptide for 30 min at 37°C and absorbance at 540 nm determined. Hemoglobin release following 0.1% Triton X-100 was defined as 100% hemoglobin release. Data represent mean ± SEM of triplicate determinations. Figures 18 A-D. Depict photographs showing temperature dependent and competitive internalization of p28 and pi 8 into UISO-Mel-2 cells. Penetration of Alexafluor 568 labeled p28 (A) or pi 8 (B) at 201 IM was evaluated by confocal microscopy at different temperatures. (C) and (D) Confocal analysis of entry of Alexafluor 568 labeled p28 (C) or pi 8 (D) at 5 μM into UISO-Mel-2 cells after 30min at 37° C in the presence/absence of unlabeled peptide (200 fold excess).
Figures 19 A-D . (A) Depicts photographs showing confocal analysis of 28, pl8 (20 μM) and Arg8 (10 μM) entry into UISO-Mel-2 cells after 1 hr at 37°C in the presence/absence of heparin sulfate (lOOμg/ml). (B) Graphs showing flow cytometric analysis of p28 or pl8 entry in the presence of inhibitors. Cell fluorescence intensity in the absence of inhibitor (control) was considered as 100%. (C) Graphs depicting FRCS analysis of p28 and pi 8 entry into fibroblasts in presence of inhibitors. (D) Depicts photographs showing colocalization of pi 8 and p28 with caveolin I (Panel 1 ). UISO-Mel-2 cells were incubated with Alexafluor 568 labeled pi 8 or p28 (20μM) or media for 2hrs at 37°C. Cells were fixed and processed for anti-caveolin 1 immunostaining. Confocal analysis of entry of Alexafluor 568 labeled pi 8 or p28 (20μM) into UISO-Mel-2 cells after 2hrs at 370C followed by antigolgin 97 antibodies (Panel 2 ). Colocalization of Alexafluor 568 labeled azurin, p28 and pi 8 (red) with mitotracker (green) (Panel 3 ) and Lysotracker (green) (Panel 4) dyes in
UISO-Mel-2 cells. Cells were incubated at 37°C with 20μM azurin, p28, pi 8 or media only. After 90 min incubation, mitotracker/lysotracker probes were added and cells incubated for 30min. Cells were counterstained with DAPI (blue). Colocalization of azurin, p28 or pi 8 appears as a yellow florescence. Figures 20 A and B. Graphs depicting UISO-Mel-2 cells that were incubated with increasing concentrations of azurin, p28, or pl8 at 37°C for 72hrs. MTT (A); Direct cell count (B). Cell viability (MTT) or cell number in control wells were considered as 100%. Data represent mean ± SEM.
Figure 21, (A) through (C). Graphs and charts depicting peptide binding and entry into cells. (A) UISO-Mel-2 or fibroblast cells (3x105cells) were suspended in MEME media without phenol red. Reactions were started by adding Alexafluor 568-conjugated p28 at 10, 50, 100, 150, 250, 300 and 400 μM for 30, 60, 90 and 120 sec on ice. Cells were analyzed by flow cytometry. (B) The Km and Vmax were calculated by plotting peptide concentration (μM) vs velocity (MFI/sec). (C) Peptide binding and entry was determined using whole Mel2 cells (50,000 cells/ml), were incubated for 30 min at 37°C with increasing concentrations (0-175nM) of radiolabeled azurin in the presence/absence of 1000 fold excess of unlabeled p28, or azurin, and radioactivity remaining in the cell pellet counted using a gamma counter. Radioactivity in cells incubated with 125I azurin alone was considered total binding; radioactivity in the presence of unlabeled azurin or p28 was considered nonspecific binding. Specific binding was determined by subtracting nonspecific binding from total binding and Scatchard plots generated. Figure 22, (A) through (C). Depict side and back photographs of mice with melanoma MEL-23 tumors taken after injection with p28 dye complex at 60 μmolar concentration in 250 μL scans and after injection with control PBS at (A) 24 hours and (B) 48 hours. (C) depics side and back photographs of mice with melanoma MEL-23 tumors taken after injection with p28 at 200 μM concentration at 24 and 48 hours. Figure 23, (A) through (C). Depict side and back photographs of mice with melanoma MEL-23 tumors taken after injection with pi 8 at 60 μmolar concentration at (A) 17 hours, (B) 24 hours, and (C) 46 hours. (C) also depicts photographs of mouse organs, including the heart, lung, liver, kidney, spleen, and brain, taken 46 hours after injection of pl8. Figure 24, (A) and (B). (A) Depicts side and back photographs of mice with tumors taken 12 hours after injection with pi 8, p28, and arg-8 at 60 μmolar concentration. (B) Depicts photographs of mouse organs, including mouse brains, taken 12 hours after injection with pi 8, p28, and arg-8.
Figure 25, (A) and (B). (A) Depicts side and back photographs of mice with melanoma MEL-6 tumors taken 40 hours after injections of 600 μM concentrations of pi 8 and arg-8 into tail veins. Animals treated with pi 8 received 0.5 million cells, and animals treated with arg-8 received 1 million cells. (B) Depicts photographs of mouse organs taken 40 hours after injections of 600 μM concentrations of pi 8 and arg-8.
Figure 26, (A) and (B). (A) Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 16 hours after injections of 60 μM concentrations of p28, pi 8, and arg-8. (B) Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 24 hours after injections of 60 μM concentrations of p28, pl8, and arg-8.
Figure 27. Depicts photographs of mouse organs taken 48 hours after injection of 60 μM concentrations of p28 and pi 8 dye peptide complex into mice with melanoma MEL-23. Figure 28. Depicts photographs of mouse organs taken 24 hours after injection of 60 μM concentrations of p28 into mice with MEL-23 tumors and organs. Figure 29. Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 16 hours after injections of 60 μM concentrations of p28 and arg-8.
Figure 30. Depicts side and back photographs of mice with melanoma MEL-23 tumors taken 16 hours after injections of 60 μM concentrations of pi 8. Figure 31. Depicts side photographs of mice with tumors taken 10 and 24 hours after high dose treatment with 240 μM concentrations of pi 8, p28, and arg-8.
Figure 32. Depicts side and back photographs of mice with MCF-7 tumors and organs taken 28 hours after high dose treatment with 240 μM concentrations of pi 8, p28, and arg-8. Also depicts photographs of mouse organs with MCF-7 taken 28 hours after high dose treatment with 240 μM concentrations of pi 8, p28, and arg-8.
Figure 33. Depicts side and back photographs of mice with tumors taken 50 hours after high dose treatment with 240 μM concentrations of pi 8, p28, and arg-8.
Figure 34. Depicts photographs of mouse organs taken 24 hours after injection of 120 μM concentrations of pi 8, p28, and arg-8 into the tail veins of mice with HCT-116 tumors and organs.
Figure 35, (A) and (B). (A) Depicts photographs of mouse organs taken 24 hours after injection of 120 μM concentrations of pi 8, p28, and arg-8 into the tail veins of mice with HCT-116 tumors and organs. (B) Depicts side photographs of mice with HCT-116 tumors taken 21 hours after injection of 120 μM concentrations of pi 8, p28, and arg-8 into their tail veins.
Figure 36, (A) and (B). (A) Depicts side and back photographs of mice with HCT- 116 24 hours after injection with 120 μM concentrations of p28, 47 days after injection of 1 million cells into tail veins. (B) Depicts photographs of mouse organs taken from mice with HCT-116 4 hours after injection with 120 μM concentrations of p28, 47 days after injection of 1 million cells into tail veins.
Figure 37. Depicts photographs of organs from MEL-6 mice taken 24 hours after treatment with 120 μM concentrations of pi 8, p28, and arg-8.
Figure 38, (A) and (B). (A) Depicts side and back photographs of MEL-6 mice taken 22 hours after injection of 120 μM concentrations of pi 8, p28, and arg-8, and 60 60 μM concentration of arg-8. (B) Depicts photographs of MEL-6 mouse organs after treatment with 120 μM concentrations of pi 8, p28, and arg-8, and 60 μM concentration of arg-8. Figure 39, (A) and (B). (A) Depicts photographs of organs from HT- 1080 mice taken 22 hours after treatment with 60 and 120 μM concentrations of pl8, p28, and arg-8. (B) Depicts side-by-side photographs of brains from HT- 1080 mice taken 22 hours after treatment with 60 and 120 μM concentrations of pl8, p28, and arg-8, demonstrating the differences between uptake of pi 8 and p28 into the brain.
Figure 40. Depicts side and back photographs of HT- 1080 mice during Doxorubicin vs. p28 study taken 16 hours after treatment with 60 and 120 μM concentrations of pi 8, p28, and arg-8.
Figure 41, (A) and (B). (A) Depicts photographs of organs from HT-1080 mice taken 22 hours after treatment with 60 and 120 μM concentrations of p28 and arg-8. (B) Depicts side-by-side photographs of brains from HT-1080 mice taken 22 hours after treatment with 60 and 120 μM concentrations of p28 and arg-8.
Figure 42, (A) and (B). (A) Depicts photographs of organs from HT-1080 mice taken 22 hours after treatment with 60 and 120 μM concentrations of pi 8 and arg-8. (B) Depicts side-by-side photographs of brains from HT-1080 mice taken 22 hours after treatment with 60 and 120 μM concentrations of pl8 and arg-8.
Figure 43, (A) through (E). Depicts photographs of HT-1080 mice with lung metastases treated via their tail veins with (A) 3mg/kg Doxorubicin IP, 3 treatments; (B) 5mg/kg IP p28 daily; (C) PBS control, PBS IP daily; (D) 10 mg/kg IP p28 daily; (E) 20 mg/kg IP daily.
Figure 44, (A) and (B). (A) Depicts photographs of organs from HT-1080 mice in an animal study, whereby 1x106 cells are injected into tail veins (43 days) and all treated mice have lung metastases, taken 24 and 26 hours after 60 μM concentrations of p28 injected into tail veins. Animal 6982 was dead when photographed. (B) Depicts side and back photographs of HT-1080 mice in an animal study, whereby 1x106 cells are injected into tail veins (43 days), taken 22 hours after 60 μM concentrations of p28 injected into tail veins. Animal 6982 was dead when photographed.
Figure 45. Depicts side and back photographs of HT-1080 mice in an animal study, whereby 1x106 cells are injected into tail veins (43 days), taken 26 hours after 60 μM concentrations of p28 injected into tail veins. Figure 46, (A) and (B). Depicts photographs of (A) organs from mice and (B) back views of mice in BaIb-C peptide study taken 12 hours after treatment with 60 and 120 μM concentrations of pi 8, p28, and arg-8.
Figure 47, (A) and (B). Depicts photographs of (A) organs from mice and (B) side views of mice in BaIb-C peptide study taken 24 hours after treatment with 60 and 120 μM concentrations of pi 8, p28, and arg-8.
Figure 48. Depicts side and back photographs of MEL-6 mice (0.5 million cells injected via tail vein) 16 hours after injection into tail veins of 60 μM concentrations of pi 8 and arg-8. Figure 49, (A) through (D). Depicts photographs of mouse organs, and specifically mouse brains, after treatment with pi 8 and p28.
Figure 50. Depicts photographs of organs from MEL-6 mice taken 24 hours after treatment with p28, pi 8, and arg-8.
Figure 51, (A) through (C). (A) Depicts side and back photographs of MEL-6 mice 3 hours after injection with 60 μM concentrations of pi 8, p28, and arg-8. (B) Depicts side and back photographs of MEL-6 mice, and photographs of organs from MEL-6 mice, taken 22 hours after injection with 60 μM concentrations of pi 8, p28, and arg-8. (C) Depicts photographs of organs from MEL-6 mice 24 hours after injection with 60 μM concentrations of pl8, p28, and arg-8. Figure 52, (A) and (B). Depict uptake of pi 8 and p28 into (A) mouse brains and (B) mouse organs).
Figure 53. Depicts side and back photographs of MEL-6 mice in study whereby 0.5 million cells injected LV. into tail vein (44 days post), taken 120 hours after injection into tail vein of 24 μM concentrations of pi 8 and arg-8. Figure 54. Depicts photographs of organs from MEL-6 mice taken 168 hours after tratment with pi 8.
Figure 55. Depicts side and back photographs of MEL-6 mice taken after injection of arg-8 and pi 8, 72 hrs, day 41 post injection.
Figure 56. Depicts back photographs of mice taken after injection of arg-8 and pi 8. Figure 57. Depicts side and front photographs of mice taken 3, 24, and 48 hours after injection of arg-8 and pi 8. DETAILED DESCRIPTION OF THE INVENTION Definitions
As used herein, the term "cell" includes either the singular or the plural of the term, unless specifically described as a "single cell." As used herein, the terms "polypeptide," "peptide," and "protein" are used interchangeably to refer to a polymer of amino acid residues. The terms apply to amino acid polymers in which one or more amino acid residue is an artificial chemical analogue of a corresponding naturally occurring amino acid. The terms also apply to naturally occurring amino acid polymers. The terms "polypeptide," "peptide," and "protein" are also inclusive of modifications including, but not limited to, glycosylation, lipid attachment, sulfation, gamma- carboxylation of glutamic acid residues, hydroxylation and ADP-ribosylation. It will be appreciated that polypeptides are not always entirely linear. For instance, polypeptides may be branched as a result of ubiquitination and they may be circular (with or without branching), generally as a result of post-translation events, including natural processing event and events brought about by human manipulation which do not occur naturally. Circular, branched and branched circular polypeptides may be synthesized by non-translation natural process and by entirely synthetic methods as well.
As used herein, the term "pharmacologic activity" means the effect of a drug or other chemical on a biological system. The effect of chemical may be beneficial (therapeutic) or harmful (toxic). The pure chemicals or mixtures may be of natural origin (plant, animal, or mineral) or may be synthetic compounds.
As used herein, the term "premalignant" means precancerous, or before abnormal cells divide without control.
As used herein, the term "lesion" means an area of abnormal tissue. As used herein, the term "pathological condition" includes anatomic and physiological deviations from the normal that constitute an impairment of the normal state of the living animal or one of its parts, that interrupts or modifies the performance of the bodily functions, and is a response to various factors (as malnutrition, industrial hazards, or climate), to specific infective agents (as worms, parasitic protozoa, bacteria, or viruses), to inherent defects of the organism (as genetic anomalies), or to combinations of these factors.
As used herein, the term "condition" includes anatomic and physiological deviations from the normal that constitute an impairment of the normal state of the living animal or one of its parts, that interrupts or modifies the performance of the bodily functions. A "condition" may be, but is not limited to an ailment, disease, infection or illness.
As used herein, the term "suffering from" includes presently exhibiting the symptoms of a pathological condition, having a pathological condition even without observable symptoms, in recovery from a pathological condition, or recovered from a pathological condition.
As used herein, the term "chemoprevention" is the use of drugs, vitamins, or other agents to try to reduce the risk of, or delay the development or recurrence of, cancer.
A used herein, the term "treatment" includes preventing, lowering, stopping, or reversing the progression or severity of the condition or symptoms associated with a condition being treated. As such, the term "treatment" includes medical, therapeutic, and/or prophylactic administration, as appropriate. Treatment may also include preventing or lessening the development of a condition, such as cancer.
As used herein, the term "inhibit cell growth" means the slowing or ceasing of cell division and/or cell expansion. This term also includes the inhibition of cell development or increases in cell death.
As used herein, the term "inhibit the growth of HIV infection" means any means by which HIV infection is decreased, or prevented from increasing in the human body. These means can include, but are not limited to, inhibition of replication of the HIV genome, inhibition of synthesis and/or assembly of the HIV coat proteins, and inhibition of HIV entry into uninfected cells. This definition includes any the method of action of any of the currently known HIV therapies.
As used herein, "anti-malarial activity" includes any activity that decreases the infectivity, the reproduction, or inhibits the progress of the lifecycle of a malaria parasite. "Anti-malarial activity" includes inhibition of the growth of malaria infection by all of the means of observed with current anti-malarial drugs.
As used herein, the term "anti-malarial drug" refers to drugs with anti-malarial activity that may be used to decrease the infectivity, the reproduction, or inhibit the progress of the lifecycle of a malaria parasite. As used herein, the term "anti-HIV drug" refers to drugs with anti-HIV activity HIV by which HIV infection in mammals is decreased, or prevented from increasing in the human body, by any means including, but are not limited to, inhibition of replication of the HIV genome, inhibition of synthesis and/or assembly of the HIV coat proteins, and inhibition of HIV entry into uninfected cells.
As used herein, the term "inhibit angiogenesis" refers to the slowing, ceasing or reverse of the formation of blood vessels in a particular cells, tissues, or location of the body. The inhibition of angiogenesis may be due to direct or indirect effects on endothelial cells. The inhibition may also be at any stage of the angiogenesis process. For example, the inhibition may be due to preventing a tumor from producing Vascular Endothelial Growth Factor (VEGF), direct inhibition of endothelial cell proliferation and/or migration, acting as an antagonist of angiogenesis growth factors, inhibition of endothelial-specific integrin/survival signaling, or chelation of copper. The inhibition of angiogenesis may be by any means by which the formation of blood vessels is slowed, ceased or reversed, including any means currently used by any anti-angiogenesis drug under development or on the market.
As used herein, the term "inappropriate angiogenesis" refers to any occurrence of angiogenesis that is undesirable. Inappropriate angiogenesis may be angiogenesis that is associated with a condition in a mammal. The inappropriate angiogenesis may be either the cause or the symptom of such a condition. Inappropriate angiogenesis in a broader sense may be any angiogenesis that is unwanted, even though it may be within the realm of normal mammalian physiology.
A "therapeutically effective amount" is an amount effective to prevent or slow the development of, or to partially or totally alleviate the existing symptoms in a particular condition for which the subject is being treated. Determination of a therapeutically effective amount is well within the capability of those skilled in the art.
The term "substantially pure," as used herein, when used to modify a protein or other cellular product of the invention, refers to, for example, a protein isolated from the growth medium or cellular contents, in a form substantially free of, or unadulterated by, other proteins and/or other compounds. The term "substantially pure" refers to a factor in an amount of at least about 75%, by dry weight, of isolated fraction, or at least "75% substantially pure." More specifically, the term "substantially pure" refers to a compound of at least about 85%, by dry weight, of isolated fraction, or at least "85% substantially pure." Most specifically, the term "substantially pure" refers to a compound of at least about 95%, by dry weight, of isolated fraction, or at least "95% substantially pure." The term "substantially pure" may also be used to modify a synthetically-made protein or compound of the invention, where, for example, the synthetic protein is isolated from the reagents and byproducts of the synthesis reaction(s).
The term "pharmaceutical grade," as used herein, when referring to a peptide or compound of the invention, is a peptide or compound that is isolated substantially or essentially from components which normally accompany the material as it is found in its natural state, including synthesis reagents and by-products, and substantially or essentially isolated from components that would impair its use as a pharmaceutical. For example, a "pharmaceutical grade" peptide may be isolated from any carcinogen. In some instances, "pharmaceutical grade" may be modified by the intended method of administration, such as "intravenous pharmaceutical grade," in order to specify a peptide or compound that is substantially or essentially isolated from any substance that would render the composition unsuitable for intravenous administration to a patient. For example, an "intravenous pharmaceutical grade" peptide may be isolated from detergents, such as SDS, and antibacterial agents, such as azide. The terms "isolated," "purified" or "biologically pure" refer to material which is substantially or essentially free from components which normally accompany the material as it is found in its native state. Thus, isolated peptides in accordance with the invention preferably do not contain materials normally associated with the peptides in their in situ environment. An "isolated" region of a polypeptide refers to a region that does not include the whole sequence of the polypeptide from which the region was derived. An "isolated" nucleic acid, protein, or respective fragment thereof has been substantially removed from its in vivo environment so that it may be manipulated by the skilled artisan, such as but not limited to, nucleotide sequencing, restriction digestion, site-directed mutagenesis, and subcloning into expression vectors for a nucleic acid fragment as well as obtaining the protein or protein fragment in substantially pure quantities.
The term "substantially pure", when used to modify the term a polypeptide or other compound, as used herein, refers to a polypeptide or compound, for example, a polypeptide isolated from the growth medium, in a form substantially free of, or unadulterated by, active inhibitory agents. The term "substantially pure" refers to a compound in an amount of at least about 75%, by dry weight, of isolated fraction, or "75% substantially pure." More specifically, the term "substantially pure" refers to a compound of at least about 85%, by dry weight, active compound, or "85% substantially pure." Most specifically, the term "substantially pure" refers to a compound of at least about 95%, by dry weight, active compound, or "95% substantially pure." The substantially pure cupredoxin or cytochrome or a variant or derivative thereof can be used in combination with one or more other substantially pure compounds, or another isolated cupredoxin or cytochrome. The term "variant" as used herein with respect to a peptide, refers to amino acid sequence variants which may have amino acids replaced, deleted, or inserted as compared to the wild-type polypeptide. Variants may be truncations of the wild-type peptide. A "deletion" is the removal of one or more amino acids from within the polypeptide, while a "truncation" is the removal of one or more amino acids from one or both ends of the polypeptide. Thus, a variant peptide may be made by manipulation of genes encoding the polypeptide. A variant may be made by altering the basic composition or characteristics of the polypeptide, but not at least some of its pharmacologic activities. For example, a "variant" of azurin can be a mutated azurin that retains its ability to inhibit the development of premalignant mammalian cells. In some cases, a variant peptide is synthesized with non- natural amino acids, such as ε-(3,5-dinitrobenzoyl)-Lys residues. Ghadiri & Fernholz, J. Am. Chem. Soc, 112:9633-9635 (1990). In another example, a "variant" of azurin can be a mutated azurin that retains its ability to inhibit the growth of HIV infection in mammalian cells. In another example, a "variant" of azurin can be a mutated azurin that retains its ability to inhibit parasitemia in malaria-infected human red blood cells. In some embodiments, the variant has not more than 20 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 15 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 10 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 6 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 5 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. In some embodiments, the variant has not more than 3 amino acids replaced, deleted or inserted compared to wild-type peptide or part thereof. The term "amino acid," as used herein, means an amino acid moiety that comprises any naturally-occurring or non-naturally occurring or synthetic amino acid residue, i.e., any moiety comprising at least one carboxyl and at least one amino residue directly linked by one, two three or more carbon atoms, typically one (α) carbon atom.
The term "derivative" as used herein with respect to a peptide refers to a peptide that is derived from the subject peptide. A derivation includes chemical modifications of the peptide such that the peptide still retains some of its fundamental activities. For example, a "derivative" of azurin can, for example, be a chemically modified azurin that retains its ability to inhibit angiogenesis in mammalian cells. Chemical modifications of interest include, but are not limited to, amidation, acetylation, sulfation, polyethylene glycol (PEG) modification, phosphorylation or glycosylation of the peptide. In addition, a derivative peptide may be a fusion of a polypeptide or fragment thereof to a chemical compound, such as but not limited to, another peptide, drug molecule or other therapeutic or pharmaceutical agent or a detectable probe.
The term "percent (%) amino acid sequence identity" is defined as the percentage of amino acid residues in a polypeptide that are identical with amino acid residues in a candidate sequence when the two sequences are aligned. To determine % amino acid identity, sequences are aligned and if necessary, gaps are introduced to achieve the maximum % sequence identity; conservative substitutions are not considered as part of the sequence identity. Amino acid sequence alignment procedures to determine percent identity are well known to those of skill in the art. Often publicly available computer software such as BLAST, BLAST2, ALIGN2 or Megalign (DNASTAR) software is used to align peptide sequences. In a specific embodiment, Blastp (available from the National Center for Biotechnology Information, Bethesda MD) is used using the default parameters of long complexity filter, expect 10, word size 3, existence 11 and extension 1.
When amino acid sequences are aligned, the % amino acid sequence identity of a given amino acid sequence A to, with, or against a given amino acid sequence B (which can alternatively be phrased as a given amino acid sequence A that has or comprises a certain % amino acid sequence identity to, with, or against a given amino acid sequence B) can be calculated as:
% amino acid sequence identity = X/Y*100 where
X is the number of amino acid residues scored as identical matches by the sequence alignment program's or algorithm's alignment of A and B and Y is the total number of amino acid residues in B.
If the length of amino acid sequence A is not equal to the length of amino acid sequence B, the % amino acid sequence identity of A to B will not equal the % amino acid sequence identity of B to A. When comparing longer sequences to shorter sequences, the shorter sequence will be the "B" sequence. For example, when comparing truncated peptides to the corresponding wild-type polypeptide, the truncated peptide will be the "B" sequence.
General
The present invention provides compositions comprising cupredoxin or cytochrome, and variants, derivatives, truncations, and structural equivalents of cupredoxin or cytochrome, and methods to treat and/or prevent two or more conditions in mammalian cells.
The invention also provides methods to administer to a patient to treat and/or prevent two or more diseases in a patient, comprising administering to the patient with one peptide or at least two peptides that are a cupredoxin, cytochrome and variants, derivatives, truncations, and structural equivalents of cupredoxin or cytochrome.
Specifically, the invention provides compositions comprising Pseudomonas aeruginosa azurin, variants, derivatives, truncations, and structural equivalents of azurin, and their use to concurrently treat and/or prevent two or more conditions in a patient. More specifically, the present invention provides compositions for the concurrent treatment and/or prevention of conditions such as cancer, inappropriate angiogenesis, HIV and malaria, and patients at a higher risk of acquiring these conditions than the general population. Members of the cupredoxin family, specifically azurin from Pseudomonas aeruginosa, are promising compounds for therapeutic and preventative treatment of numerous diseases or conditions. For example, azurin is known to inhibit angiogenesis in human umbilical vascular endothelium cells (HUVECs). U.S. Patent Application Serial No. 11/488,693, filed July 19, 2006, which is hereby incorporated by reference in its entirety herein. Azurin from P. aeruginosa is also known for its ability to inhibit the growth of HIV- 1 infection in peripheral blood mononuclear cells and to inhibit parasitemia of malaria- infected mammalian red blood cells . Chaudhari et al, Cell Cycle. 5: 1642-1648 (2006). Azurin from P. aeruginosa is also known to interfere with the ephrin signaling system in various mammalian cells and tissues. U.S. Patent Application No. 11/436,592, filed May 19, 2006, which is hereby incorporated by reference in its entirety herein. Furthermore, two redox proteins elaborated by Pseudomonas aeruginosa, the cupredoxin azurin and cytochrome C551, both enter J774 lung cancer cells and show significant cytotoxic activity toward the cancer cells as compared to normal cells. Zaborina et ah, Microbiology 146:2521-2530 (2000). Azurin can also selectively enter and kill human melanoma UISO-Mel-2 or human breast cancer MCF-7 cells. Yamada et a\., PNAS 99:14098-14103 (2002); Punj et ah, Oncogene 23:2367-2378 (2004). Azurin from P. aeruginosa preferentially enters J774 murine reticulum cell sarcoma cells, forms a complex with and stabilizes the tumor suppressor protein p53, enhances the intracellular concentration of p53, and induces apoptosis. Yamada et ah, Infection and Immunity 70:7054-7062 (2002). Detailed studies of various domains of the azurin molecule showed that amino acids 50-77 (p28) (SEQ ID NO: 29) represented a protein transduction domain (PTD) critical for internalization and subsequent apoptotic activity. Yamada et ah, Cell. Microbial. 7:1418- 1431 (2005). Azurin also caused a significant increase of apoptosis in human osteosarcoma cells as compared to non-cancerous cells. Ye et ah, Ai Zheng 24:298-304 (2003). Moreover, other members of the Cupredoxin family are promising compounds for therapeutic and preventative treatment of numerous diseases or conditions. Rusticyanin from Thiobacillus ferrooxidans can also enter macrophages and induce apoptosis. Yamada et ah, Cell Cycle 3:1182-1187 (2004); Yamada et ah, Cell. Micro. 7:1418-1431 (2005). Plastocyanin from Phormidium laminosum and pseudoazurin form Achromobacter cycloclastes also are cytotoxic towards macrophages. U.S. Pat. Pub. No. 20060040269, published Feb. 23, 2006.
The temperature dependent entry of cationic cell penetrating peptides ("CPPs"), which supports an endocytotic component to cell penetration, is reflected in the entry of azurin and aa fragment 50-77 (p28). Yamada, T., et ah, Cell Microbiol 7: 1418-1431 (2005). The entry of 50-67 of azurin (pl8) into normal and malignant cells appears accelerated relative to p28. The lower Km and higher Vmax of pi 8 suggest that aa 50-67 define an amphipathic structure when associated with phospholipid membranes that more closely represents the actual PTD of azurin. However, an energy dependent endocytotic or pore related process is not the only entry mechanism available to these peptides. For example, the metabolic and membrane potential inhibitors sodium azide and ouabain (Na+ K+ ATPase inhibitor), which inhibit the entry- of cationic peptides , did not impair the entry of either pi 8 or p28 into UISO-Mel-2 cells or fibroblasts (Figure 19 B,C), suggesting that either peptide may penetrate the cell membrane directly.
Depletion of cholesterol from the plasma membrane with β-methylcylodextran, filipin or nystatin to disrupt lipid rafts, plasma membrane domains that provide fluid platforms to segregate membrane components and compartmentalize membranes, significantly inhibited the penetration of pl8 (50%) and p28 (-60%) into UISO-Mel-2 cells and fibroblasts (35% and 42%, respectively) demonstrating that a significant percentage (-60%) of pi 8 and p28 penetrates the plasma membrane via caveolae. Caveolae are a 50- to 100-nm omega-shaped subset of lipid raft invaginations of the plasma membrane defined by the presence of caveolin specific proteins (caveolin- 1, -2, or -3) that function as regulators of signal transduction.
Brefeldin A disrupts the Golgi apparatus and inhibited pi 8 accumulation, so it follows that this pathway is also utilized in pi 8 and p28 entry and intracellular transport. Cell penetration of pi 8 and p28 via caveolae comports with the evidence that inhibitors of N- glycosylation reduce cell entry by ~ 60% in UISO-Mel-2 cells and 25% and 35% respectively in fibroblasts. The percentile differences between pi 8 and p28 entry relate to the numbers of N-glycosylation membrane structures in cancer vs normal cells and the relative route of entry of p28 and pi 8 via this mechanism. Figure 19 B, C.
Azurin, p28, and pi 8 all bind to cancer cells with high affinity and high capacity relative to many other potential anti-cancer peptides. It is believed that after binding, this protein/receptor complex localizes in caveolae and is internalized, eventually moving (via caveosomes) to the golgi, ER, and nucleus. In addition to caveolar-mediated entry, kinetic analysis also demonstrates that p28 and pi 8 penetrate the plasma membrane via a non- clathrin caveolae mediated process. A clathrin- and caveolin-independent pathway can exist as a constitutive internalization mechanism, such as for the interleukin 2 receptor and for certain glycosyl-phosphatidylinositol (GPI)-anchored proteins. Lamaze, C, et al, MoI Cell 7: 661-671 (2001); Sabharanjak, S., et al, Dev Cell, 2: 411-423 (2002). An increase in caveolin- 1 expression in cancer cells over normal cells is not likely to be the sole basis for the preferential entry of azurin, p28 and pi 8 into cancer cells. Fibroblasts and a number of other normal cells also have significant numbers of caveolae on their surface. The findings reflected in Examples 25-31 demonstrate that the cellular penetration of aa 50-67 and 50-77 of azurin is unique relative to all current CPPs in its preference for cancer cells, and show that the C-terminal 10-12 amino acids of p28, aa 50-77 of azurin, contain the domain primarily responsible for cell cycle inhibition and apoptitic activity. pi 8 and p28 are able to enter cancer cells, tumors, and mammalian organs, as is shown in Figures 21 through 57. Surprisingly, pi 8 and p28 are also able to penetrate the blood-brain barrier and enter mammalian brains, as demonstrated by, for example, Figures 24A, 24B, 25B, 27, 28, 32, 34, 35A, 36B, 37, 38B, 39A-B, 41 A-C, 42A-C, 44A, 46A, 47 A, 49 A-D, 50, 5 IB, 52A-B, and 54. As such, these peptides may be used to treat conditions in mammalian brains and brain cells.
It is also now known that synthesized p28 not only enters into a variety of malignant cell lines (melanoma (Mel-2), MCF-7, pancreatic, astrocytoma, glioblastoma, among others), but also non-cancerous human umbilical vein endothelial cells (HUVEC). See Example 1. p28 enters into these cells in a temperature dependent manner, but does not enter normal cells (fibroblast, normal mammary epithelium). As HUVEC cells are known to instigate angiogenesis in human embryos, the entry of p28 into HUVEC cells prompted an examination of the effect of p28 on angiogenesis. HUVEC cells (20,000 cells) were plated on Matrigel® coated wells and incubated in media containing 0-75 μM of p28. Cultures were examined under light microscopy at 4h and 24h post-treatment. The p28 peptide inhibited capillary tube formation of the HUVEC in a dose dependent manner, suggesting that p28 inhibits the capillary tube formation step of angiogenesis. See Example 2. Further, p28 inhibited the migration of HUVEC cells on Matrigel® in a scratch wound migration assay, indicating that p28 also inhibits the migration step of angiogenesis. See Example 3. Thus, in in vitro studies with an established angiogenesis model system, HUVEC cells on Matrigel®, p28 inhibits two critical steps in angiogenesis, capillary tube formation and cell migration.
It is also now known that azurin, and peptides derived from azurin, such as p28, have chemopreventative properties. It is now known that azurin, and p28, prevent the formation of premalignant preneoplastic lesions in mouse mammary gland organ culture. In a mouse mammary gland organ culture model, azurin at 50 μg/ml was found to inhibit the formation of alveolar lesions by 67%. Likewise, p28 at 25 μg/ml was found to inhibit the formation of alveolar lesions by 67%. Further, azurin at 50 μg/ml was found to inhibit the formation of ductal lesions by 79%, and p28 at 25 μg/ml inhibited the formation of ductal lesions by 71%. Confocal microscopy and FAC showed that azurin and p28 entered normal murine mammary epithelial cells (MM3MG) and mammary cancer cells (4Tl). It is therefore now known that azurin and variants of azurin may be used to inhibit the formation of premalignant preneoplastic lesions, and thus the development of cancer, and specifically breast cancer, in mammalian patients.
It is also now known that cupredoxins and cytochromes will inhibit in vitro parasitemia in human red blood cells by the malaria parasite Plasmodium falciparum. In particular, the cupredoxins azurin and Laz inhibit parasitemia in P. falciparum by about 50% and about 75% respectively. See, Example 14. Further, rusticyanin and cytochromes c and f inhibited parasitemia by 20-30 %. See, Example 9. Further, it is now known that azurin has a discernable structural homology to the Fab fragment of Gl 7.12 mouse monoclonal antibody when complexed to the PfMSP 1-19 fragment of the MSP 1 surface protein of P. falciparum . While not limiting the mode of inhibition to any one means, it is thought that azurin may inhibit parasitemia of P. falciparum by interaction with the MSPl protein on the parasite's surface.
It is also now known that azurin and Laz bind both the PfMSP 1-19 and PfMSP 1-42 P. falciparum surface proteins in vitro. Further, it is now known that azurin amino acid residues 36-89 are required for binding to PfMSPl -19 and PfMSPl -42. Further, it is now known that the H.8 domain of Laz from N. gonorrhea increases both the binding of a fused azurin to PfMSPl -19 as well as inhibition of parasitemia by P. falciparum. See, Examples 13 and 14. It has also been learned that P. aeruginosa cytochrome C551, human cytochrome c and Phormidium laminosum cytochrome f will inhibit parasitemia in malaria- infected human red blood cells. In a specific embodiment, the cytochrome is cytochrome C551 from P. aeruginosa, human cytochrome c or cytochrome f. In other specific embodiments, the cytochrome comprises an amino acid sequence that is SEQ ID NO: 19-21.
It is also now known that azurin can induce about a 90% suppression of growth of HIV-I in peripheral blood mononuclear cell (PBMC) cultures. See, Example 18. Azurin is now known to inhibit the growth of three strains of HIV-I, BaI (the most predominant clade B circulating in the US and Western Europe), a clade B African isolate RW/92/008/RE1, and a clade C Indian isolate IN/2167 D 15. See, Example 18. Additionally, a cupredoxin-like protein from Neisseria, Laz, is now also known to inhibit the growth of these three HIV-I strains, as well as a fusion of the H.8 region of the Laz protein with P. aeruginosa azurin. See, Example 18. Finally, it is now known that M44KM64E mutant of azurin and cytochrome c551 from P. aeruginosa can inhibit HIV infection in HIV-infected human blood lymphocytes. See, Example 16.
Due to the high degree of structural similarity between cupredoxins, it is likely that other cupredoxins may treat and/or prevent numerous diseases. In some embodiments, the cupredoxin may be, but is not limited to, azurin, pseudoazurin, plastocyanin, auracyanin, Laz, rusticyanin, stellacyanin or cucumber basic protein. In a more specific embodiment, the cupredoxin may be azurin. In a specific embodiment, the cupredoxin or azurin may be derived from Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp. , Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas fluorescens, Pseudomonas chlor or aphis, Bordetella pertussis, Pseudomonas syringae, Xylella fastidiosa and Vibrio parahaemolyticus. In a most specific embodiment, the azurin is from P. aeruginosa. In other specific embodiments, the cupredoxin comprises an amino acid sequence that is SEQ ID NOs: 1, 5-12, 18 and 23. Several cupredoxins are known to have pharmacokinetic activities similar to those of azurin from Pseudomonas aeruginosa. For example, rusticyanin from Thiobacillus ferrooxidans can also enter macrophages and induce apoptosis. Yamada et al, Cell Cycle 3:1182-1187 (2004); Yamada et ah, Cell. Micro. 7:1418—1431 (2005). Plastocyanin from P hormidium laminosum and pseudoazurin form Achromobacter cycloclastes also are cytotoxic towards macrophages. U.S. Pat. Pub. No. 20060040269, published Feb. 23, 2006. It is therefore contemplated that other cupredoxins may be used in the compositions and methods of the invention. Further, variants, derivatives, and structural equivalents of cupredoxins that retain the ability to inhibit the formation of cancer in mammals may also be used in the compositions and methods of the invention. These variants and derivatives may include, but are not limited to, truncations of a cupredoxin, conservative substitutions of amino acids and proteins modifications such as PEGylation, all-hydrocarbon stabling of α-helices, and other methods and techniques disclosed herein.
Moreover, because of the structural homology between the cytochromes, it is contemplated that other cytochromes will have the same ability to treat and/or prevent more than one condition as P. aeruginosa cytochrome C551 and human cytochrome c. In some embodiments, the cytochrome is from a pathogenic bacterium. In another specific embodiment, the cytochrome inhibits parasitism in malaria-infected red blood cells, and more specifically, human red blood cells. In another embodiment, the cytochrome inhibits viral infection such as HIV. In another specific embodiment, the cytochrome inhibits cell cycle progression in a mammalian cancer cell, and more specifically in a J774 cell.
Compositions of the Invention The invention provides for peptides that are cupredoxins and/or cytochromes, and/or variants, derivatives or structural equivalents of cupredoxin or cytochrome. In some embodiments, the peptide is isolated. In some embodiments, the peptide is substantially pure or pharmaceutical grade. In other embodiments, the peptide is in a composition that comprises, or consists essentially of, the peptide. In another specific embodiment, the peptide is non-antigenic and does not raise an immune response in a mammal, and more specifically a human. In some embodiments, the peptide is less than a full-length cupredoxin or cytochrome, and retains some of the pharmacologic activities of the cupredoxin or cytochrome. In one specific embodiment, the peptide may retain the ability to concurrently treat and/or prevent two or more conditions in a mammalian cell or a patient. In some embodiments, the peptide retains the ability to inhibit the growth of viral or bacterial infection. In some embodiments, the peptide retains the ability to inhibit specifically HIV-I infection in peripheral blood mononuclear cells, or parasitemia in malaria- infected red blood cells, or P. falciparium infection in human red blood cells or inhibit angiogenesis in HUVECs on Matrigel®, or inhibit cancer in malignant cells. The invention also provides compositions comprising at least one peptide that is a cupredoxin, or variant, derivative, truncation, or structural equivalent of a cupredoxin. The invention also provides compositions comprising at least one peptide that is a cytochrome, or variant, derivative, truncation, or structural equivalent of a cytochrome. In other embodiments, the composition consists essentially of the peptide. In some embodiments, the cupredoxin is selected from the group consisting of azurin, pseudoazurin, plastocyanin, rusticyanin, Laz, auracyanin, stellacyanin and cucumber basic protein. In some embodiments, the cupredoxin is from an organism selected from the group consisting of Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp. , Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas βuorescens, Pseudomonas chlororaphis, Bordetella pertussis, Pseudomonas syringae, Xylella fastidiosa and Vibrio parahaemolyticus. In a very specific embodiment, the cupredoxin is from Pseudomonas aeruginosa. In one embodiment, the cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof, is fused to a H.8 region of Laz from Neisseria meningitides or Neisseria gonorrhea. One example of such a peptide is the H.8-Paz fusion protein. In a specific embodiment, the H.8 is fused to the C-terminus of the cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof. In another specific embodiment, the H.8 region is SEQ ID NO: 22, or a variant, derivative, truncation, or structural equivalent thereof.
In another embodiment, the variant or derivative of cupredoxin has a significant structural homology to the Fab fragment of G 17.12 mouse monoclonal antibody. An example of how this structural similarity can be determined can be found in Example 11. Specifically, significant structural homology between a cupredoxin and the Fab fragment of Gl 7.12 mouse monoclonal antibody can be determined by using the VAST algorithm (Gibrat et al, id.; Madej et al, id.). In specific embodiments, the VAST p-value from a structural comparison of a cupredoxin to the Fab fragment of Gl 7.12 mouse monoclonal antibody can be less than about 10"4, less than about 10"5, less than about 10"6, or less than about 10"7. In other specific embodiments, the VAST score from a structural comparison of a cupredoxin to the Fab fragment of G 17.12 mouse monoclonal antibody can be greater than about 9, greater than about 10, greater than about 11 or greater than about 12.
In some embodiments, the variant, derivative, truncation, or structural equivalent thereof has some of the functional characteristics of the P. aeruginosa azurin, P. aeruginosa cytochrome C551, human cytochrome c or cyanobacterial cytochrome f. In a specific embodiment, the peptide of the invention inhibits parasitemia by malaria in malaria-infected red blood cells, and more specifically parasitemia by P. falciparum in P. falciparum-infected human red blood cells. The invention also provides for the variants, derivatives and structural equivalents of cupredoxin and cytochrome C551 that retain the ability to inhibit parasitemia in malaria-infected red blood cells, and more specifically parasitemia by P. falciparum in P. falciparum-infected human red blood cells. The inhibition of parasitemia by P. falciparum in P. falciparum-infected human red blood cells may be determined by the method described in Example 14. The invention provides for amino acid sequence variants of a cupredoxin or cytochrome which have amino acids replaced, deleted, or inserted as compared to the wild- type polypeptide. Variants of the invention may be truncations of the wild-type polypeptide. In some embodiments, the composition comprises a peptide that consists of a region of a cupredoxin or cytochrome that is less than the full length wild-type polypeptide. In some embodiments, the composition comprises a peptide that consists of more than about 10 residues, more than about 15 residues or more than about 20 residues of a truncated cupredoxin or cytochrome. In some embodiments, the composition comprises a peptide that consists of not more than about 100 residues, not more than about 50 residues, not more than about 40 residues or not more than about 30 residues of a truncated cupredoxin or cytochrome. In some embodiments, the composition comprises a peptide to which a cupredoxin or cytochrome, and more specifically to SEQ ID NOS. :1, 5-12, 18 and 23, and has at least about 90% amino acid sequence identity, at least about 95% amino acid sequence identity or at least about 99% amino acid sequence identity or is a mutant of SEQ ID NOS.: 1, 5-12, 18 and 23.
In specific embodiments, the variant of cupredoxin comprises Pseudomonas aeruginosa azurin residues 50-77 (p28, SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (pi 8, SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio par ahaemolyticus azurin residues 52-78 (SEQ ID NO: 27), Pseudomonas syringae azurin residues 51-77 (SEQ ID NO: 25), Bordetella bronchiseptica azurin residues 51-77 (SEQ ID NO: 28), and Pseudomonas aeruginosa azurin residues 36-77 (SEQ ID NO: 33).
In other embodiments, the variant of cupredoxin consists of Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio par ahaemolyticus azurin residues 52-78 (SEQ ID NO: 27), Pseudomonas syringae azurin residues 51-77 (SEQ ID NO: 25), Bordetella bronchiseptica azurin residues 51-77 (SEQ ID NO: 28), and Pseudomonas aeruginosa azurin residues 36-77 (SEQ ID NO: 33). In other specific embodiments, the variant consists of the equivalent residues of a cupredoxin.
It is also contemplated that other cupredoxin variants can be designed that have a similar pharmacological activity to Pseudomonas aeruginosa azurin residues 50-77 (SEQ ID NO: 29), Pseudomonas aeruginosa azurin residues 50-67 (SEQ ID NO: 30), Pseudomonas aeruginosa azurin residues 36-88 (SEQ ID NO: 50), Pseudomonas aeruginosa azurin residues 36-128 (SEQ ID NO: 31), Pseudomonas aeruginosa azurin residues 88-113 (SEQ ID NO: 49), Pseudomonas aeruginosa azurin residues 36-89 (SEQ ID NO: 32), and Pseudomonas aeruginosa azurin residues 96-113 (SEQ ID NO: 48), Vibrio parahaemolyticus azurin residues 52-78 (SEQ ID NO: 27), Pseudomonas syringae azurin residues 51-77 (SEQ ID NO: 25), Bordetella bronchiseptica azurin residues 51-77 (SEQ ID NO: 28), and Pseudomonas aeruginosa azurin residues 36-77 (SEQ ID NO: 33). To do this, the subject cupredoxin amino acid sequence will be aligned to the Pseudomonas aeruginosa azurin sequence using BLAST, BLAST2, ALIGN2 or Megalign (DNASTAR), the relevant residues located on the P. aeruginosa azurin amino acid sequence, and the equivalent residues found on the subject cupredoxin sequence, and the equivalent peptide thus designed.
The variants also include peptides made with synthetic amino acids not naturally occurring. For example, non-naturally occurring amino acids may be integrated into the variant peptide to extend or optimize the half-life of the composition in the bloodstream. Such variants include, but are not limited to, D,L-peptides (diastereomer), (Futaki et al., J. Biol. Chem. 276(8):5836-40 (2001); Papo et al, Cancer Res. 64(16):5779-86 (2004); Miller et al, Biochem. Pharmacol. 36(l):169-76, (1987); peptides containing unusual amino acids (Lee et al., J. Pept. Res. 63(2):69-84 (2004)), and incorporation of olefin-containing non- natural amino acid followed by hydrocarbon stapling (Schafmeister et al, J. Am. Chem. Soc. 122:5891-5892 (2000); Walenski et al, Science 305:1466-1470 (2004)), and peptides comprising ε-(3,5-dinitrobenzoyl)-Lys residues.
The invention also provides compositions comprising one peptide or at least two peptides that are a cupredoxin, cytochrome, or variant, derivative, truncation, or structural equivalent of a cupredoxin or cytochrome in a pharmaceutical composition. In some embodiments, the cupredoxin is in a pharmaceutical composition and is from an organism selected from the group consisting of Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidans ssp. denitrificans I, Bordetella bronchiseptica, Methylomonas sp., Neisseria meningitides, Neisseria gonorrhea, P seudomonas fluoresceins, Pseudomonas chlor or aphis, Bordetella pertussis, Pseudomonas chlor or aphis, Xylellafastidiosa, Ulva pertussis or Vibrio par ahaemolyticus. In a specific embodiment, the cupredoxin is from Pseudomonas aeruginosa. In another specific embodiment, the cupredoxin or cytochrome is selected from the group consisting of SEQ ID NOS: 1, 5-12, 18, 23, 25, 27-33 and 48-50 in a pharmaceutical composition. In another specific embodiment, the cupredoxin may comprise SEQ ID NO: 30.
In other embodiments, the peptide of the invention is a derivative of a cupredoxin or cytochrome. The derivatives of cupredoxin or cytochrome are chemical modifications of the peptide such that the peptide still retains some of its fundamental activities. For example, a "derivative" of azurin can be a chemically modified azurin that retains its ability to treat and/or prevent more than one condition in a mammalian cell. Chemical modifications of interest include, but are not limited to, amidation, acetylation, sulfation, polyethylene glycol (PEG) modification, phosphorylation, glycosylation of the peptide, and other modifications disclosed herein. In addition, a derivative peptide maybe a fusion of a cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof to a chemical compound, such as but not limited to, another peptide, drug molecule or other therapeutic or pharmaceutical agent or a detectable probe. Derivatives of interest include chemical modifications by which the half-life in the bloodstream of the peptides and compositions of the invention can be extended or optimized, such as by several methods well known to those in the art, including but not limited to, circularized peptides (Monk et al. , BioDrugs 19(4):261-78, (2005); DeFreest et al., J. Pept. Res. 63(5):409-19 (2004)), N- and C- terminal modifications (Labrie et al., Clin. Invest. Med. 13(5):275-8, (1990)), and incorporation of olefin-containing non-natural amino acid followed by hydrocarbon stapling (Schafmeister et al, J. Am. Chem. Soc. 122:5891-5892 (2000); Walenski et al, Science 305:1466-1470 (2004)).
It is contemplated that the peptide of the composition of invention may be more than one of a variant, derivative and structural equivalent of a cupredoxin or cytochrome. For example, the peptide may be a truncation of azurin that has been PEGylated, thus making it both a variant and a derivative. In one embodiment, the peptides of the invention are synthesized with α,α-disubstituted non-natural amino acids containing olefin-bearing tethers, followed by an all-hydrocarbon "staple" by ruthenium catalyzed olefin metathesis. (Scharmeister et ai, J. Am. Chem. Soc. 122:5891-5892 (2000); Walensky et al., Science 305:1466-1470 (2004)). Additionally, peptides that are structural equivalents of azurin may be fused to other peptides, thus making a peptide that is both a structural equivalent and a derivative. These examples are merely to illustrate and not to limit the invention. Variants, derivatives or structural equivalents of cupredoxin or cytochrome may or may not bind copper.
In some embodiments, the cupredoxin may be varied using methods that include, but are not limited to, those which decrease the hydrolysis of the peptide, decrease the deamidation of the peptide, decrease the oxidation, decrease the immunogenicity and/or increase the structural stability of the peptide. It is contemplated that two or more of the modifications described herein may be combined in one modified cupredoxin derived peptide, as well as combinations of one or more modifications described herein with other modification to improve pharmacokinetic properties that are well know to those in the art. Many methods to design such variants and derivatives are well known in the art, and some are discussed below and herein.
Biotransformation
One approach to improving the pharmacokinetic properties of cupredoxins, cytochromes, and variants, derivatives, truncations, and structural equivalents thereof, particularly cupredoxin-derived peptides such as truncations of azurin, is to create variants and derivatives of the cupredoxin derived peptides that are less susceptible to biotransformation. Biotransformation may decrease the pharmacologic activity of the peptide as well as increase the rate at which it is eliminated from the patient's body. One way of achieving this is to determine the amino acids and/or amino acid sequences that are most likely to be biotransformed and to replace these amino acids with ones that are not susceptible to that particular transformative process.
In some embodiments, the cupredoxin derived peptides may include unnatural amino acids or modified amino acids. In some embodiments, the introduction of certain unnatural amino acids enhances the pharmcaokinetic properties of the cupredoxin derived peptide. Such introduction may be site-specific and may be done to avoid certain biochemical modifications in vivo. Exemplary unnatural amino acids include b-amino acids (e.g., b3 and b2), homo-amino acids, cyclic amino acids, aromatic amino acids, Pro and Pyr derivatives, 3- substituted Alanine derivatives, Glycine derivatives, Ring-substituted Phe and Tyr Derivatives, Linear Core Amino Acids and Diamino Acids. Such unnatural amino acids may be incorporated into peptides by site directed modification, ribosomal translation, or by chemical synthesis of the peptide. Each of these methods may be applied in synthesizing cupredoxin derived peptides.
For example, modified cupredoxin derived peptides may be synthesized by the use of wild-type Aminoacyl-tRNA synthetases (AARSs) with unnatural amino acids building for the production of unnatural cupredoxin variants. See Hartman, et al, PLoS One, 2(10): e972 (2007); Miranda, et al, J. Am. Chem. Soc. 129: 13153-13159 (2007). The specificity of the ribosomal translation apparatus limits the diversity of unnatural amino acids that may be incorporated into peptides using ribosomal translation. Over ninety unnatural building blocks that are AARS substates have been uncovered including side chain and backbone analogs. Hartman, et al, PLoS One, 2(10): e972 (2007). Over fifty unnatural amino acids may be incorporated into peptides with high efficiency using an all-en2ymatic translation system, with peptides containing up to thirteen different unnatural amino acids. Hartman, et al, PLoS One, 2(10): e972 (2007). In some embodiments, such amino acids may be incorporated in cupredoxin derived peptides.
Other modifications may include the use of optically active α-amino acids. The use of optically active α-amino acids and their derivatives is being expanded for their use in pharmaceuticals, agrochemicals and as chiral ligands. In particular, chiral glycine and alanine equivalents plan an important role. At least one stereoselective strategy for constructing α-amino acids has been proposed, allowing for enantiopure α-amino acids in predetermined stereochemistry. Lu, et al "Asymmetric Synthesis of α-amino acids: Preparation and alkylation of monocyclic iminolactones derived from α-Methyl trans- cinnamaldehyde" published on the Internet on Sept. 11 , 2008 (to be published in J. Org. Chem.), the disclosure of which is incorporated by reference herein. The modified cupredoxin derived peptides may be synthesized using the optically active α-amino acids to produce enantiomerically enriched iterations.
Hydrolysis is generally a problem in peptides containing aspartate. Aspartate is susceptible to dehydration to form a cyclic imide intermediate, causing the aspartate to be converted to the potentially inactive iso-aspartate analog, and ultimately cleaving the peptide chain. For example, in the presence of aspartic acid— proline in the peptide sequence, the acid catalyzed formation of cyclic imide intermediate can result to cleavage of the peptide chain. Similarly, in the presence of aspartic acid— glycine in the peptide sequence, the cyclic intermediate can be hydrolyzed either into the original aspartate form (harmless) or into the iso-aspartate analog. Eventually, all of the aspartate form can be completely converted into the iso-aspartate analog. Similarly sequences with serine can also be dehydrated to form a cyclic imide intermediate that can cleave the peptide chain. Cleavage of the peptide may result in reduced plasma half-life as well as reduced specific pharmacologic activity of the peptide.
It is contemplated that substituting other amino acids for asparagine and/or serine in the sequence of the cupredoxin derived peptide may result in a peptide with improved pharmacokinetic properties such as a longer plasma half-life and increased specific activity of a pharmacologic activity of the peptide. In one contemplated variant, at one or more asparagine residues of the cupredoxin derived peptide may be replaced with another amino acid residue, and specifically a glutamic acid residue. In another contemplated variant, one or more serine residues of the cupredoxin derived peptide may be replaced with another amino acid residue, and specifically a threonine residue. In some variants of cupredoxin derived peptide, one or more asparagine residues and one or more serine residues are substituted. In some embodiments, conservative substitutions are made. In other embodiments, non-conservative substitutions are made. Deamidation of amino acid residues is a particular problem in biotransformation.
This base-catalyzed reaction frequently occurs in sequences containing asparagine— glycine or glutamine— glycine and follows a mechanism analogous to the aspartic acid— glycine sequence above. The de-amidation of the asparagine— glycine sequence forms a cyclic imide intermediate that is subsequently hydrolyzed to form the aspartate or iso-asparate analog of asparagine. In addition, the cyclic imide intermediate can lead to racemization into D- aspartic acid or D-iso-aspartic acid analogs of asparagine, all of which can potentially lead to inactive forms of the peptide.
It is contemplated that deamidation in the cupredoxin peptides may be prevented by replacing a glycine, asparagine and/or glutamine of the asparagine— glycine or glutamine — glycine sequences of the cupredoxin with another amino acid and may result in a peptide with improved pharmacokinetic properties, such as a longer plasma half-life and increased specific activity of a pharmacologic activity of the peptide. In some embodiments, the one or more glycine residues of the cupredoxin derived peptide are replaced by another amino acid residue. In specific embodiments, one or more glycine residues of the cupredoxin derived peptide are replaced with a threonine or an alanine residue. In some embodiments, the one or more asparagine or glutamine residues of the cupredoxin derived peptide are replaced by another amino acid residue. In specific embodiments, one or more asparagine or glutamine residues of the cupredoxin derived peptide are replaced with an alanine residue. In other specific embodiments, the glycine at residues 58 and/or 63 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent glycines of other cupredoxins, are replaced with an alanine or a threonine. In other specific embodiments, the methionine at residue 59 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent methionine residue of another cupredoxin derived peptide, is replaced by an alanine residue. In other specific embodiments, the glycine at residue 63 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent glycine residue of another cupredoxin derived peptide, is replaced by a threonine residue. In some embodiments, conservative substitutions are made. In other embodiments, non-conservative substitutions are made. In specific embodiments, the modified cupredoxin derived peptide of the invention comprises the following sequence, wherein the underlined amino acids are substituted into the wildtype Pseudomonas aeruginosa p28 sequence
LSTAADMQAVVTDTMASGLDKDYLKPDD (SEQ ID NO: 51). Reversible and irreversible oxidation of amino acids are other biotransformative processes that may also pose a problem that may reduce the pharmacologic activity, and/or plasma half-life of cupredoxin derived peptides. The cysteine and methionine residues are the predominant residues that undergo reversible oxidation. Oxidation of cysteine is accelerated at higher pH, where the thiol is more easily deprotonated and readily forms intra- chain or inter-chain disulfide bonds. These disulfide bonds can be readily reversed in vitro by treatment with dithiothreitol (DTT) or tris(2-carboxyethylphosphine) hydrochloride (TCEP). Methionine oxidizes by both chemical and photochemical pathways to form methionine sufoxide and further into methionine sulfone, both of which are almost impossible to reverse.
It is contemplated that oxidation in the cupredoxin derived peptides may be prevented by replacing methionine and/or cysteine residues with other residues. In some embodiments, one or more methionine and/or cysteine residues of the cupredoxin derived peptide are replaced by another amino acid residue. In specific embodiments, the methionine residue is replaced with a leucine or valine residue. In other specific embodiments, one or more of the methionines at residues 56 and 64 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent methionine residues in other cupredoxin derived peptides, are replaced with leucine or valine. In some embodiments, conservative substitutions are made. In other embodiments, non- conservative substitutions are made. In specific embodiments, the cupredoxin peptides of the invention comprise one of the following sequences, wherein the underlined amino acid is substituted into the wildtype Pseudomonas aeruginosa p28 sequence:
LSTAADLQGVVTDGLASGLDKDYLKPDD (SEQ ID NO: 52) or LSTAADVQGVVTDGVASGLDKDYLKPDD (SEQ ID NO: 53). Another biotransformative process that may affect the pharmacologic activity, plasma half-life and/or immunogenicity of the cupredoxin derived peptides is diketopiperazine and pyroglutamic acid formation. Diketopiperazine formation usually occurs when glycine is in the third position from the N-terminus, and more especially if proline or glycine is in position 1 or 2. The reaction involves nucleophilic attack of the N-terminal nitrogen on the amide carbonyl between the second and third amino acid, which leads to the cleavage of the first two amino acids in the form of a diketopiperazine. On the other hand, pyroglutamic acid formation may be almost inevitable if glutamine is in the N-terminus. This is an analogous reaction where the N-terminal nitrogen attacks the side chain carbonyl carbon of glutamine to form a deaminated pyroglutamayl peptide analog. This conversion also occurs in peptide containing asparagine in the N-terminus, but to a much lesser extent.
It is contemplated that diketopiperazine and pyroglutamic acid formation may be decreased in cupredoxin derived peptides by replacing glycine in position 1 , 2, or 3 from the N-terminus, proline in position 3 from the N-terminus, or asparagine at the N-terminus of the peptide with another amino acid residue. In some embodiments, a glycine in positions 1, 2, or 3 from the N-terminus of the cupredoxin derived peptide is replaced with another amino acid residue. In specific embodiments, the glycine residue is replaced by a threonine or alanine residue. In another embodiment, a proline at position 3 from the N-terminus of the cupredoxin derived peptide is replaced with another amino acid residue. In specific embodiments, the proline is replaced by an alanine residue. In another embodiment, an asparagine at the N-terminus is replaced with another amino acid residue. In specific embodiments, the asparagine residue is replaced by a glutamine residue. In some embodiments, conservative substitutions are made. In other embodiments, non-conservative substitutions are made.
Another biotransformative process that may affect the pharmacologic activity, plasma half-life and/or immunigenicity of the cupredoxin derived peptide is racemization. This term is loosely used to refer to the overall loss of chiral integrity of the amino acid or peptide.
Racemization involves the base-catalyzed conversion of one enantiomer (usually the L-form) of an amino acid into a 1 : 1 mixture of L- and D-enantiomers. One way to improve stability of the peptide in general is by making a retro-inverso (D-isomer) peptide. The double inversion of peptide structure often leaves the surface topology of the side-chain intact and has been used extensively to stabilize biologically active peptides. Snyder et al, PLoS Biol. 2:0186-0193 (2004). A D-amino acid substituted Tat is internalized into cells as well as the L- amino acid peptide. Futaki et al, J. Biol. Chem. 276:5836-5840 (2001); Huq et al, Biochemistry 38:5172-5177 (1999). In some embodiments, one or more amino acid residues of the cupredoxin derived peptide are replaced by the D-isomer of that amino acid residue. In other embodiments, all of the amino acid residues of the cupredoxin derived peptide are replaced with D-isomers of those residues. In one embodiment, the modified cupredoxin derived peptide is a retro-inverso (D-isomer) version of the cupredoxin derived peptide. In a specific embodiment, the modified cupredoxin derived peptide is
DDPKLYDKDLGSAMGDTVVGQMDAATSL (SEQ ID NO: 54). Other methods to protect a cupredoxin derived peptide from biotransformative degradation are N-acetylation and C-amidation. These derivatives may protect the peptide from degradation and may make the cupredoxin derived peptide more closely mimic the charge state of the alpha amino and carboxyl groups in the native protein. Peptides with the N-acetylation and/or C-amidation can be provided by commercial suppliers. In one embodiment of the invention, the N-terminus of the cupredoxin derived peptide may be acetylated. In another embodiment of the invention, the C-terminus of the cupredoxin derived peptides may be amidated. In one specific embodiment, the modified cupredoxin derived peptide is
Acetylation-LSTAADMQGVVTDGMASGLDKDYLKPDD-amidation (SEQ ID NO: 55).
Cyclization is an additional manner of biotransformation that may be beneficial to therapeutic peptides including the cupredoxins as described herein. Cyclization may stabilize therapeutic peptides, allowing them to be stored longer, be administered at lower doses and be administered less frequently. Cyclization has been shown to protect peptides against peptidase and protease degradation. Cyclization can be done chemically or enzymatically. Enzymatic cyclization is generally less problematic than chemical cyclization, as chemical cyclization can lack in regio- and stereospecificity, can lead to multimerization in lieu of cyclization and can require complicated multistep processes. Indeed, it has been shown that thioether cyclization is more protective and stable than a disulfide bond against proteolytic enzymes.
Enzymatic cyclization has been shown in lantibiotics - (mehtlyl)lanthionine- containing bacterial peptides. E.g., R. Rink, et al., "Lantibiotic Structures as Guidelines for the Design of Peptides That Can Be Modified by Lantibioitic Enzymes" 44 Biochem., 8873- 82 (2005); R. Rink, et al., "Production of Dehydroamino Acid-Containing Peptides by Lactococcus lactis" 73:6 Applied and Environmental Microbiology, 1792-96 (2007); R. Rink, et al., "NisC, the Cylcase of the Lantibiotic Nisin, Can Catalyze Cyclization of Designed Nonlantibiotic Peptides" 46 Biochem., 13179-89 (2007) (each of which is hereby incorporated by reference in its entirety). Lantibiotics are produced by and inhibit the growth of gram-positive bacteria. In lantibiotics, dehydroalanine and dehydrobutyrine are created by enzyme mediated dehydration of serine and threonine residues. Cysteines are then enzymatically coupled to the dehydrated serine and threonine residues to form thioether cyclizations. Naturally occurring lantibiotics show such couplings via thioether bonds between residues that are up to 19 residues apart. Thioether ring formation depends upon the leader peptide. The location of the cyclization depends upon the cyclase mediated regio- and stereospecific ring closure and the positions of the dehydratable serine and threonine residues. The best characterized of the lantibiotics is nisin — a pentacyclic peptide antiobiotic produced by Lactococcus lactis. Nisin is composed of four methyllanthionines, one lanthionine, two dehydroalanines, one dehydrobutyrine, and twenty-six unmodified amino acids. Nisin's five thioether cross-links are formed by the addition of cysteine residues to dehydroalanine and dehydrobutyrine residues that originate from serine and threonine. Nisin contains thioether-containing amino acids that are posttranslationally introduced by a membrane-associated enzyme complex. This enzyme complex includes: transporter NisT, serine and threonine dehydratase NisB, and cyclase NisC. NisB dehydrates serine and threonine residues, converting them into dehydroalanine and dehydrobutyrine, respectively. This is followed by NisC catalyzed enantioselective coupling of cysteines to the formed dehydoresidues. NisT facilitates the export of the modified prenisin. Another enzyme, NisP cleaves the nisin leader peptide from prenisin. The cyclase NisC has been well characterized. Li et al, "Structure and Mechanism of the Lantibiotic Cylclase Involved in Nisin Biosynthesis" 311 Science, 1464-67 (2006) (hereby incorporated by reference in its entirety).
An analysis of cyclization in lantibiotics has led to the identification of amino acid sequences and characteristics in peptides that favor cyclization. It has been shown that the NisB enzyme dehydrates more often where certain amino acids flank the serine and threonine residues. It has been shown that cyclization occurs more often in lantibiotic propeptides where hydrophobic, nonaromatic residues are in proximity to the serine and threonine residues. The flanking residues of the modified cysteines are typically less hydrophobic than the flanking residues of the modified threonines and serines. Exceptions have been found, including hexapeptides VSPPAR (SEQ ID NO: 56), YTPPAL (SEQ ID NO: 57) and FSFFAF (SEQ ID NO: 58). The hexapeptides suggest that the presence of a proline at position 3 or 4 or having phenylalanine flanking both sides may prohbit dehydration. The rings are typically formed by coupling a dehydrated residue to a C-terminally located cysteine. However, rings may be formed by coupling a dehydrate residue to a N-terminally located cysteine.
It has also been shown that the nisin dehydrating and transport enzymes are not specific to nisin and may, in fact, be used to modify non-nisin peptides (and non-lantibiotic peptides). NisB has been shown to dehydrate serine and threonine residues in peptides such as human peptide hormones when such peptides are N-terminally fused to the lantibiotic leader peptide. On non-lantibiotic peptides, similar ring formation characteristics apply; namely, the extent of dehydration can be controlled by the amino acid context of the flanking region of the dehydratable serine and threonine residues. The presence of hydrophobic flanking residues (e.g., alanine and valine) around the serines and threonines allowed full dehydration and therefore enhanced thioether ring formation. The presence of an N-terminal aspartate and C-terminally flanked arginine prevented dehydration. It also shown that the presence of proline residues and phenylalanine residues is disfavorable for dehydration. Generally, the presence of hydrophilic flanking residues prevented dehydration of the serine and threonine residues. Hydrophobic flanking favors dehydration; hydrophilic flanking disfavors dehydration. Studies have shown that where dehydration does occur, the average hydrophobicity of the flanking residues of serines and threonine is positive ~ .40 on the N- terminal side and .13 on the C-terminal side. Also, the average hydrophobicity of the residues flanking serines and threonines that are not dehydrated is negative — .36 on the N- terminal side and -1.03 on the C-terminal side. Deydration is not restricted by the presence of a series of flanking threonine residues and is not restricted by the distance bteween the nisin leader peptide and the residue to be dehydrated.
NisC has been shown to catalyze the regiospecifϊc formation of thioether rings in peptides unrelated to naturally occuring lantibiotics. Generally, such peptides must be fused to the nisin leader peptide. In some cases, thioether rings may form spontaneously, for example where a dehydroalanine is spaced by two amino acids from a cysteine. Unlike spontaneous cyclization, NisC catalyzed cyclization is stereospecific for dehydrated pre- nisin. Consequently, the methyllanthionines and lanthionine in nisin are in the DL configuration. It is thought that cyclization in nonlantibiotic peptides will also be stereospecific
These principles can be applied to the compounds described herein, including cupredoxins, cytochromes, and variants derivatives, truncations, and structural equivalents thereof.
Thioether Bridges
In nature, lantibiotic-enzyme-induced thioether bridges occur with up to 19 amino acids under the bridge. Thioether bridges with 2 to 4 amino acids under the bridge are abundant. In some embodiments, the cupredoxins and cytochromes and derivatives, variants, truncations, or structural equivalents thereof, such as truncated azurin, may be modified by introducing thioether bridges into the structure. The azurin truncation p28 (SEQ ID NO: 29), for example, may be modified using this method. Extended molecular dynamics simulations (70 ns) using software package GROMACS (www.gromacs.org) suggest that, at 37°C, the region of the p28 alpha helix from position 6 to 16 is unstable, and that the peptide tends to adopt a beta sheet conformation. This, together with the fact that the part of the molecule presumed to be responsible for interaction with p53 remains solvent exposed, suggests that introduction of a thioether bridge in this region of the p28 peptide may not affect its functionality.
Figure imgf000064_0001
Structure 1 : Azurin truncation with alpha-helical structure
Figure imgf000064_0002
Structure 2: Result of 70 ns simulation.
The amino acid sequence of p28 is SEQ ID NO: 29
(LSTAADMQGVVIDGMASGLDKDYLKPDD). The amino acid sequence known as pi 8 is SEQ ID NO: 30 (LSTAADMQGVVTDGMASG). Thioether bridges can be formed between Ser/Thr on the N-side to Cys on the C-side. The serine/threonine is dehydrated and subsequently coupled to the cysteine. Threonines are preferred since they are more easily dehydrated than serines. Generally, hydrophobic flanking residues (at least one) to the threonine are preferred since they enhance the extent of dehydration. Negatively charged amino acids, glutamate and aspartate, that are flanking residues have a strong negative effect on dehydration. Generally, hydrophilic flanking residues, especially glycin, do not favor dehydration. Preceding the Cys there is a slight preference for charged hydrophilic residues, especially glutamate/aspartate. Depending on the size of the thioether ring, the bulkiness of the amino acids that participate in the ring matters.
In one embodiment, the truncated azurin sequence is LSTAADMQGVVTDGMASGLDKDYLTPGC (SEQ ID NO: 59). A thioether bridge is formed between positions 25 and 28 of p28, and will be fully protected against carboxyetidases. Positions 2, 3 and 25 will be dehydrated, but neither the import sequence, nor the sequence thought to be relevant for interaction with p53, is altered by thioether ring introduction. As such, peptide activity should not be altered. The threonine is between two hydrophobic amino acids and hence is expected to be fully dehydrated by dehydratase, NisB, according to specific guidelines. See Rink et al., Biochemistry 2005. The same guidelines also predict cyclization involving positions 25 and 28 by cyclase NisC, especially because of the aspartate located before the cysteine.
In another embodiment, the truncated azurin sequence is LSTAADCQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 60) and the thioether bridge is formed between positions 3 and 7. The ring between position 3 and 7 mimics ring A of nisin and makes use of the existing threonine at position 2. The aspartate at position 6 will favor cyclization.
In another embodiment, the truncated azurin sequence is LSTAACMQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 61), and the threonine in position 2 is utilized to form a thioether bridge.
In another embodiment, two or more of the thioether rings in the truncated azurins described in the paragraphs above are combined into one peptide.
In another embodiment, many truncated azurin sequences can be created and screened for threonine rings by analyzing the peptides with a ring of one lanthionine and two to three additional amino acids under the sulfur bridge. This might involve one or combinations of the sequences below: LSTACDMQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 62) LSTAATMQCVVTDGMASGLDKDYLKPDD (SEQ ID NO: 63) LSTAATMQGCVTDGMASGLDKDYLKPDD (SEQ ID NO: 64) LSTAANTQGCVTDGMASGLDKDYLKPDD (SEQ ID NO: 65) LSTAANTQGVCTDGMASGLDKDYLKPDD (SEQ ID NO: 66) LSTAADMTAVCTDGMASGLDKDYLKPDD (SEQ ID NO: 67) LSTAADMTAVVCDGMASGLDKDYLKPDD (SEQ ID NO: 68) LSTAADMQTVVCDGMASGLDKDYLKPDD (SEQ ID NO: 69) LSTAADMQTVVTCGMASGLDKDYLKPDD (SEQ ID NO: 70) LSTAADMQATVTCGMASGLDKDYLKPDD (SEQ ID NO: 71) LSTAADMQATVTDCMASGLDKDYLKPDD (SEQ ID NO: 72) LSTAADMQGVTADCMASGLDKDYLKPDD (SEQ ID NO: 73) LSTAADMQGVTADGCASGLDKDYLKPDD (SEQ ID NO: 74) LSTAADMQGVVTNGCASGLDKDYLKPDD (SEQ ID NO: 75)
A practical approach would be to genetically make a large number of such sequences and select a group for purification on the basis of extent of modification and level of production.
In another embodiment, a thioether bridge is formed between a threonine at position 12 in p28 (SEQ ID NO: 29) and the c-terminus of the peptide. The distance between the Ca of position 13 and the aspartate at position 28 might be 17.52 angstroms, larger than 1.5 nanometers, implying significant alteration of the structure of the peptide.
Figure imgf000067_0001
Structure 3: Measurement of thioether bridge positions based on distances between Ca atoms in a simulated structure.
In another embodiment, the peptide sequence is
LSTAADMQGVVTATMGSGLCKDYLKPDD (SEQ ID NO: 76), with a thioether bridge from position 14 to position 2 at a distance of 4.38 angstroms. The mutation of aspartate at position 13 to alanine favors dehydration of threonine at position 14. Mutation of alanine at position 16 to glycine completely prevents dehydration of serine at position 17 and enhances cyclization.
In another embodiment, the peptide sequence is
LSTAADMQGVVTDLTASGLCKDYLKPDD (SEQ ID NO: 77), with the thioether bridge from position 15 to position 20 at a distance of 5.83 angstroms. In this situation, mutation of glycine at position 14 to leucine favors dehydration of threonine at position 15.
Tertiary Structure Stabilization
The stability of the tertiary structure of the cupredoxin, cytochrome, or variant, derivative, truncation, or structural equivalent thereof will affect most aspects of the pharmacokinetics, including the pharmacologic activity, plasma half-life, and/or immunogenicity among others. See Kanovsky et al, Cancer Chemother. Pharmacol. 52:202- 208 (2003); Kanovsky et al, PNAS 23:12438-12443 (2001). Peptide helices often fall apart into random coils, becoming more susceptible to protease attack and may not penetrate cell membrane well. Schafmeister et al, J. Am. Chem. Soc. 122:5891-5892 (2000). Therefore, one way to stabilize the overall structure of a peptide such as a cupredoxin is to stabilize the α-helix structure of the peptide. The intra-molecular hydrogen bonding associated with helix formation reduces the exposure of the polar amide backbone, thereby reducing the barrier to membrane penetration in a transport peptide, and thus increasing related pharmacologic activities and increasing the resistance of the peptide to protease cleavage. Id. Pseudomonas aeruginosa azurin (SEQ ID NO: 1) has α-helices at residues 53-56, 58-64 and 68-70.
One method to stabilize an α-helix is to replace in the α-helix helix breaking amino acid residues such as glycine, proline, serine and aspartic acid, or helix neutral amino acid residues such as alanine, threonine, valine, glutamine, asparagine, cysteine, histidine, lysine or arginine, with helix forming residues, such as leucine, isoleucine, phenylalanine, glutamic acid, tyrosine, tryptophan and methionine or helix favoring amino acid residue substitutions, for example α-amino-isobutyric acid (Aib). See Miranda et al, J. Med. Chem., 51, 2758- 2765 (2008), the disclosure of which is incorporated by reference herein. It is contemplated that the α-helix of cupredoxin derived peptides may be stabilized by replacing one or more glycine, proline, serine and/or aspartic acid residues with other amino acids. In specific embodiments, the glycine, proline, serine, aspartic acid, alanine, threonine, valine, glutamine, asparagine, cysteine, histidine, lysine and/or arginine residues are replaced by leucine, isoleucine, phenylalanine, glutamic acid, tyrosine, tryptophan, Aib and/or methionine residues. See Lee et al, Cancer Cell Intl. 11:21 (2005). In other specific embodiments, one or more serine or glutamine residues in the α-helices of a cupredoxin derived peptide may be substituted. In still more specific embodiments, the serine and/or glutamine residues in residues 53-56, 58-64 and 68-70 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides, may be replaced. In another specific embodiment, the glutamine residue at amino acid residue 57 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan. In another specific embodiment, the threonine residue at amino acid residue 52 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan. In another specific embodiment, the threonine residue at amino acid residue 61 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan. In another specific embodiment, the glycine residue at amino acid residue 63 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan. In another specific embodiment, one or more threonine, glutamine or glycine residues at amino acid residues 52, 57, 61 or 63 of P. aeruginosa azurin (SEQ ID NO: 1), or an equivalent residue of another cupredoxin derived peptide, may be replaced, more specifically replaced with tryptophan. In specific embodiments, the cupredoxin peptide comprises one of the following sequences wherein the underlined amino acid is substituted into the wildtype Pseudomonas aeruginosa p28 sequence:
LSWAADMQGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 78);
LSTAADMWGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 79); LSTAADMQGVVWDGMASGLDKD YLKPDD (SEQ ID NO: 80);
LSTAADMQGVVTDWMASGLDKDYLKPDD (SEQ ID NO: 81);
LSWAADMWGVVTDGMASGLDKDYLKPDD (SEQ ID NO: 82);
LSWAADMQGVVWDGMASGLDKDYLKPDD (SEQ ID NO: 83);
LSWAADMQGVVTDWMASGLDKDYLKPDD (SEQ ID NO: 84); LSTAADMWGVVWDGMASGLDKDYLKPDD (SEQ ID NO: 85);
LSTAADMWGVVTDWMASGLDKDYLKPDD (SEQ ID NO: 86);
LSTAADMQGVVWDWMASGLDKDYLKPDD (SEQ ID NO: 87); or
LSWAADMWGVVWDWMASGLDKDYLKPDD (SEQ ID NO: 88).
In other embodiments, equivalent amino acids in other cupredoxin derived peptides are substituted with tryptophan.
Another method to stabilize an α-helix tertiary structure involves using unnatural amino acid residues capable of π-stacking. For example, in Andrews and Tabor (Tetrahedron 55:11711-1 1743 (1999)), pairs of ε-(3,5-dinitrobenzoyl)-Lys residues were substituted into the α-helix region of a peptide at different spacings. The overall results showed that the ι,(/'+4) spacing was the most effective stabilizing arrangement. Increasing the percentage of water, up to 90%, increased the helical content of the peptide. Pairs of ε-acyl-Lys residues in the same /,0+4) spacing had no stabilizing effect, indicating that the majority of the stabilization arises from π-π interactions. In one embodiment, the cupredoxin derived peptide may be modified so that the lysine residues are substituted by ε-(3,5-dinitrobenzoyl)-Lys residues. In a specific embodiment, the lysine residues may be substituted by ε-(3,5- dinitrobenzoyl)-Lys in a /,(/+4) spacing. Another method to stabilize an α-helix tertiary structure uses the electrostatic interactions between side-chains in the α-helix. When His-Cys or His-His residue pairs were substituted in into peptides in an /,(/+4) arrangement, the peptides changed from about 50% helical to about 90% helical on the addition of Cu, Zn or Cd ions. When ruthenium (Ru) salts were added to the His-His peptides, an exchange-inert complex was formed, a macrocyclic cw-[Ru-(NH3)4L2]3+ complex where L2 are the side chains of two histidines, which improved the helix stability. Ghadiri and Fernholz, J. Am. Chem. Soc. 112, 9633-9635 (1990). In some embodiments, the cupredoxin derived peptides may comprise macrocyclic cw-[Ru- (NH3)4L2]3+ complexes where L2 is the side chains of two histidines. In some embodiments, one or more histidine-cysteine or histidine-histidine residue pairs may be substituted an i,(i+4) arrangement into the α-helices of the cupredoxin derived peptide. In other embodiments, one or more histidine-cysteine or histidine-histidine residue pairs may be substituted an i,(i+4) arrangement in residues 53-56, 58-64 and 68-70 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides. In some embodiments, the cupredoxin derived peptide may further comprise Cu, Zn, Cd and/or Ru ions.
Another method to stabilize an α-helix tertiary structure involves disulfide bond formation between side-chains of the α-helix. It is also possible to stabilize helical structures by means of formal covalent bonds between residues separated in the peptide sequence. The commonly employed natural method is to use disulfide bonds. Pierret et al., Intl. J. Pept. Prot. Res., 46:471-479 (1995). In some embodiments, one or more cysteine residue pairs are substituted into the α-helices of the cupredoxin derived peptide. In other embodiments, one or more cysteine residue pairs are substituted at residues 53-56, 58-64 and 68-70 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides. Another method to stabilize an α-helical tertiary structure involves the use of side chain lactam bridges. A lactam is a cyclic amide which can form from the cyclisation of amino acids. Side chain to side chain bridges have been successfully used as constraints in a variety of peptides and peptide analogues, such as amphipathic or model α-helical peptides, oxytocin antagonists, melanoptropin analogues, glucagon, and SDF-I peptide analogues. For example, the Glucagon-like Peptide- 1 (GLP-I) gradually assumes a helical conformation under certain helix-favoring conditions and can be stabilized using lactam bridging. Miranda et al, J. Med. Chem., 51, 2758-2765 (2008). These lactam bridges may be varied in size, effecting stability and binding affinity. Id. Such modifications improved the stability of the compounds in plasma. Id. Depending on the space between the cyclization sites and choice of residues, lactam bridges can be used to induce and stabilize turn or helical conformations. In some embodiments, one or more cupredoxin or variant analogues are prepared with lactam bridging between nearby amino acids (such as i to i+4 glutamic acid-lysine constraints). In some embodiments, the cupredoxin derived peptide may comprise such modifications to enhance α-helix content.
Another method to stabilize an α-helix tertiary structure is the all-carbon cross-link method. The all-hydrocarbon cross-link method is proven to increase the stabilization of helical structure, protease resistant and cell-permeability. Walensky et al, Science, 305, 1466-1470 (2004). α,α- disubstituted non-natural amino acids containing olefin-bearing tethers are incorporated into peptides. Ruthenium catalyzed olefin metathesis generates an all-hydrocarbon "staple" to cross-link the helix. Schafmeister et al, J. Am. Chem. Soc, 122, 5891-5892 (2000); Walensky et ah, id.. Non-natural amino acids containing olefin-bearing tethers may be synthesized according to methodology provided in Schafmeister et al (id.) and Williams and Im (J. Am. Chem. Soc, 113:9276-9286 (1991)). In some embodiments, the cupredoxin derived peptides are stabilized by all-hydrocarbon staples. In specific embodiments, one or more pairs of α,α- disubstituted non-natural amino acids containing olefin-bearing tethers corresponding to the native amino acids are substituted into the α- helices of the cupredoxin derived peptide. In other embodiments, one or more pairs of α,α- disubstituted non-natural amino acids containing olefin-bearing tethers corresponded to the native amino acids are substituted into residues 53-56, 58-64 and 68-70 of P. aeruginosa azurin (SEQ ID NO: 1), or equivalent residues of other cupredoxin derived peptides. In some embodiments, the modified cupredoxin derived peptide may comprise XISX2AADX3X4X5VVX6DX7X8ASGLDKDYLKPDX9 (SEQ ID NO: 89), where Xi is L or acetylated-L, X2 is T or W, X3 is M, L or V, X4 is Q or W, X5 is G or A, X6 is T or W, X7 is G, T or W, X8 is M, L or V, and Xg is D or amidated-D. In other embodiments, the modified cupredoxin derived peptide may consist of
XI SX2AADX3X4X5VVX6DX7X8ASGLDKDYLKPDX9 (SEQ ID NO: 89), where X, is L or acetylated-L, X2 is T or W, X3 is M, L or V, X4 is Q or W, X5 is G or A, X6 is T or W, X7 is G, T or W, X8 is M, L or V, and X9 is D or amidated-D. In other embodiments, the modified cupredoxin derived peptide may comprise
X1DPKLYDKDLGSAX2X3DX4VVX5X6X7DAAX8SX9 (SEQ ID NO: 90), where Xi is D or acetylated-D, X2 is M, L or V, X3 is G, T or W, X4 is T or W, X5 is G or A, X6 is Q or W, X7 is M, L or V, X8 is T or W, and X9 is L or amidated-L. In other embodiments, the modified cupredoxin derived peptide may consist of XIDPKLYDKDLGSAX2X3DX4VVX5X6X7DAAX8SX9 (SEQ ID NO: 90), where Xj is D or acetylated-D, X2 is M, L or V, X3 is G, T or W, X4 is T or W, X5 is G or A, X6 is Q or W, X7 is M, L or V, X8 is T or W, and X9 is L or amidated-L. Specific peptides of interest are listed in Table 3.
PEGylation
Covalent attachment of PEG to drugs of therapeutic and diagnostic importance has extended the plasma half-life of the drug in vivo, and/or reduced their immunogenicity and antigenicity. Harris and Chess, Nature Reviews Drug Discovery 2:214-221 (2003). For example, PEG attachment has improved the pharmacokinetic properties of many therapeutic proteins, including interleukins (Kaufman et al, J. Biol. Chem. 263:15064 (1988); Tsutsumi et al, J. Controlled Release 33:447 (1995)), interferons (Kita et al, Drug Des. Delivery 6:157 (1990)), catalase (Abuchowski et al, J. Biol. Chem. 252:3582 (1977)), superoxide dismutase (Beauchamp et al, Anal. Biochem. 131 :25 (1983)), and adenosine deanimase (Chen et al, Biochem. Biophys. Acta 660:293 (1981)), among others. The FDA has approved PEG for use as a vehicle or base in foods, cosmetics and pharmaceuticals, including injectable, topical, rectal and nasal formulations. PEG shows little toxicity, and is eliminated from the body intact by either the kidneys (for PEGs < 30 kDa) or in the feces (for PEGs > 20 kDa). PEG is highly soluble in water.
PEGylation of cupredoxins, cytochromes, and/or variants, derivatives, truncations, and structural equivalents thereof, particularly cupredoxin-derived peptides such as truncations of azurin, may be used to increase the lifetime of the peptide in the bloodstream of the patient by reducing renal ultrafiltration, and thus reduce elimination of the drug from the body. Charge masking may affect renal permeation. Charge masking may be a consequence of the paramchemical modification of protein ionizable functional group, namely amines or carboxyls. In particular, the most common procedures for producing protein-PEG derivatives involves the conversion of protein amino groups into amides with the consequent loss of positive charges, and this can alter protein ultrafiltration. Since anionic macromolecules have been found to be cleared by renal ultrafiltration more slowly than neutral or positive ones, it could be expected that PEG conjugation to amino groups prolongs the permanence of the PEGylated peptide in the bloodstream.
Molecular size and globular ultrafiltration may also affect renal ultrafiltration of therapeutic peptides. The molecular weight cut off for kidney elimination of native globular proteins is considered to be about 70 kDa, which is close to the molecular weight of serum albumin. Thus, proteins with molecular weight exceeding 70 kDa are mainly eliminated from the body by pathways other than renal ultrafiltration, such as liver uptake, proteolytic digestion and clearance by the immune system. Therefore, increasing the size of a therapeutic peptide by PEGylation may decrease renal ultrafiltration of that peptide form the bloodstream of the patient.
Additionally, PEGylation of a peptide may decrease the immunogenicity of that peptide, as well as protect the peptide from proteolytic enzymes, phagocytic cells, and other factors that require direct contact with the therapeutic peptide. The umbrella-like structure of branched PEG in particular has been found to give better protection than linear PEG towards approaching proteolytic enzymes, antibodies, phagocytic cells, etc. Caliceti and Veronese, Adv. Drug. Deliv. Rev. 55:1261-12778 (2003).
In some embodiments, the cupredoxin derived peptides are modified to have one or more PEG molecules covalently bonded to a cysteine molecule. The covalent bonding does not necessarily need to be a covalent bond directly from the PEG molecule to the cupredoxin derived peptide, but may be covalently bonded to one or more linker molecules which in turn are covalently bonded to each other and/or the cupredoxin derived peptide. In some embodiments, the cupredoxin derived peptide have site-specific PEGylation. In specific embodiments, the PEG molecule(s) may be covalently bonded to the cysteine residues 3, 26 and/or 112 of P. aeruginosa azurin (SEQ ID NO: 1). In other embodiments, one or more cysteine residues may be substituted into the cupredoxin derived peptide and is PEGylated. In some embodiments, the method to PEGylate the cupredoxin derived peptide may be NHS, reductive animation, malimid or epoxid, among others. In other embodiments, the cupredoxin derived peptides may be PEGylated on one or more lysine, cysteine, histidine, arginine, aspartic acid, glutamic acid, serine, threonine, or tyrosine, or the N-terminal amino group or the C-terminal carboxylic acid. In more specific embodiments, the cupredoxin derived peptides may be PEGylated on one or more lysines or N-terminal amino groups. In other embodiments, one or more lysine, cysteine, histidine, arginine, aspartic acid, glutamic acid, serine, threonine, or tyrosine residue are substituted into the cupredoxin derived peptides and are PEGylated. In other embodiments, the cupredoxin derived peptides may be PEGylated on one or more amino groups. In other embodiments, the cupredoxin derived peptides may be PEGylated in a random, non-site specific manner. In some embodiments, the cupredoxin derived peptides may have an average molecular weight of PEG-based polymers of about 200 daltons to about 100,000 daltons, about 2,000 daltons to about 20,000 daltons, or about 2,000 daltons to about 5,000 daltons. In other embodiments, the cupredoxin derived peptides may be comprised of one or more PEG molecules that is branched, specifically a branched PEG molecule that is about 50 kDa. In other embodiments, the cupredoxin derived peptides may comprise one or more linear PEG molecules, specifically a linear PEG molecule that is about 5 kDa.
In another embodiment, the chemopreventive agent is a peptide that is a cupredoxin, or variant, truncation, structural equivalent, or derivative thereof that is a conjugate of Pep42, a cyclic 13-mer oligopeptide that specifically binds to glucose-regulated protein 78 (GRP78) and is internalized into cancer cells. The cupredoxin or variant, structural equivalent, or derivative of cupredoxin may be conjugated with Pep42 pursuant to the synthesis methods disclosed in Yoneda et al, "A cell-penetrating peptidic GRP78 ligand for tumor cell-specific prodrug therapy," Bioorganic & Medicinal Chemistry Letters 18: 1632-1636 (2008), the disclosure of which is incorporated in its entirety herein. In another embodiment, the peptide is a structural equivalent of a cupredoxin or cytochrome. Examples of studies that determine significant structural homology between cupredoxins and cytochromes and other proteins include Toth et al. {Developmental Cell 1 :82-92 (2001)). Specifically, significant structural homology between a cupredoxin or cytochrome and its structural equivalents are determined by using the VAST algorithm (Gibrat et al, Curr Opin Struct Biol 6:377-385 (1996); Madej et al, Proteins 23:356-3690 (1995)). In specific embodiments, the VAST p value from a structural comparison of a cupredoxin or cytochrome to the structural equivalent is less than about 10"3, less than about 10"5, or less than about 10"7. In other embodiments, significant structural homology between a cupredoxin or cytochrome and its structural equivalents are determined by using the DALI algorithm (Holm & Sander, J. MoI. Biol. 233:123-138 (1993)). In specific embodiments, the DALI Z score for a pairwise structural comparison is at least about 3.5, at least about 7.0, or at least about 10.0. In some embodiments, the cupredoxin, or variant, derivative, truncation, or structural equivalent thereof has some of the pharmacologic activities of the P. aeruginosa azurin, and p28. In a specific embodiment, the cupredoxins and variants, derivatives and structural equivalents of cupredoxins that may inhibit prevent the development of premalignant lesions in mammalian cells, tissues or animals, and specifically but not limited to, mammary gland cells. The invention also provides for the cupredoxins and variants, derivatives and structural equivalents of cupredoxins that may have the ability to inhibit the development of mammalian premalignant lesions, and specifically but not limited to, melanoma, breast, pancreas, glioblastoma, astrocytoma, lung, colorectal, neck and head, bladder, prostate, skin and cervical cancer cells. Inhibition of the development of cancer cells is any decrease, or lessening of the rate of increase, of the development of premalignant lesions that is statistically significant as compared to control treatments.
In some embodiments, the cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalent thereof has some of the functional characteristics of the P. aeruginosa azurin or cytochrome. In a specific embodiment, the cupredoxin or cytochrome inhibits the growth of viral or bacterial infection, and specifically HIV infection in mammalian cells, more specifically in peripheral blood mononuclear cells infected with HIV. The invention also provides for the variants, derivatives and structural equivalents of cupredoxin and cytochrome C551 that retain the ability to inhibit the growth of viral or bacterial infection, and specifically HIV infection in mammalian cells. The growth of HIV-I infection in the cells may be determined by measuring the change in the production of HIV-I p24 antigen in the cell culture supernatant by a commercial p24 enzyme immunoassay (PerkinElmer Life Sciences, Inc., Wellesley, Mass.)- Inhibition of a growth of infection is any decrease or lessening of the rate of increase of that infection that is statistically signification as compared to control treatments.
In some specific embodiments, the peptide of the invention may also induce apoptosis in a mammalian cancer cell, more specifically a J774 cell. The ability of a cupredoxin or other polypeptide to induce apoptosis may be observed by mitosensor Apo Alert confocal microscopy using a MITOSENSOR™ APOLERT™ Mitochondrial Membrane Sensor kit (Clontech Laboratories, Inc., Palo Alto, California, U.S.A.), by measuring caspase-8, caspase-9 and caspase-3 activity using the method described in Zou et al. (J. Biol. Chem. 274: 11549-11556 (1999)), and by detecting apoptosis-induced nuclear DNA fragmentation using, for example, the APOLERT™ DNA fragmentation kit (Clontech Laboratories, Inc., Palo Alto, California, U.S.A.).
In another specific embodiment, the peptide of the invention may also induce cellular growth arrest in a mammalian cancer cell, more specifically a J774 cell. Cellular growth arrest can be determined by measuring the extent of inhibition of cell cycle progression, such as by the method found in Yamada et al. (PNAS 101 :4770-4775 (2004)). In another specific embodiment, the cupredoxin or cytochrome C551, or variant, derivative, truncation, or structural equivalent thereof inhibits cell cycle progression in a mammalian cancer cell, more specifically a J774 cell.
In some specific embodiments, the cupredoxin, cytochrome or variant, derivative, truncation, or structural thereof, is administered to a patient for the concurrent treatment and/or prevention of two or more conditions such as interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papilloma virus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, heφes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus, arena virus, Dhori virus, poliovirus, rubella virus, dengue virus; SIV, Mycobacterium tuberculosis and cancer. More specifically, the cancer may be melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors or prostate cancer.
In a specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural thereof, is administered to a patient for the concurrent treatment and/or prevention of two or more conditions selected from the group consisting of cancer, HIV, malaria and inappropriate angiogenesis.
In another specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, may be in a composition as a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from HIV, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, cancer or inappropriate angiogenesis.
In another specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, may be in a composition as a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from malaria, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as malaria, cancer or inappropriate angiogenesis.
In another specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, may be in a composition as a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from HIV, malaria or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, malaria or inappropriate angiogenesis.
In another specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, may be in a composition as a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from HIV, cancer or malaria or has a higher risk than the general population of acquiring a condition such as HIV, cancer or malaria. In another specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, may be in a composition with, may be coadministered, or may be administered at about the same time as another drug. Such drugs may include, but are not limited to an anti-malarial drug, an anti-HIV drug, an anti-cancer drug, or an anti-angiogenesis drug.
In another specific embodiment, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, may be in a composition that is administered by a mode of intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection and oral.
Cupredoxins
These small blue copper proteins (cupredoxins) are electron transfer proteins (10-20 kDa) that participate in bacterial electron transfer chains or are of unknown function. The copper ion is solely bound by the protein matrix. A special distorted trigonal planar arrangement to two histidine and one cystine ligands around the copper gives rise to very peculiar electronic properties of the metal site and an intense blue color. A number of cupredoxins have been crystallographically characterized at medium to high resolution.
The cupredoxins in general have a low sequence homology but high structural homology. (Gough & Clothia, Structure 12:917-925 (2004); De Rienzo et al, Protein Science 9:1439-1454 (2000)). For example, the amino acid sequence of azurin is 31% identical to that of auracyanin B, 16.3% to that of rusticyanin, 20.3 % to that of plastocyanin, and 17.3% to that of pseudoazurin. See Table 1. However, the structural similarity of these proteins is more pronounced. The VAST p value for the comparison of the structure of azurin to auracyanin B is 10"74, azurin to rusticyanin is 10"5, azurin to plastocyanin is 10"5 6, and azurin to psuedoazurin is 10"4 -1.
All of the cupredoxins possess an eight-stranded Greek key beta-barrel or beta-sandwich fold and have a highly conserved site architecture. (De Rienzo et al, Protein Science 9:1439- 1454 (2000)). A prominent hydrophobic patch, due to the presence of many long chain aliphatic residues such as methionines and leucines, is present around the copper site in azurins, amicyanins, cyanobacterial plastocyanins, cucumber basic protein and to a lesser extent, pseudoazurin and eukaryotic plastocyanins. Id. Hydrophobic patches are also found to a lesser extent in stellacyanin and rusticyanin copper sites, but have different features. Id. Table 1. Sequence and structure alignment of azurin (IJZG) from P. aeruginosa to other proteins using VAST algorithm.
PDB Alignment % aa P-value2 Score3 length1 identity RMSD4 Description
IAOZ A 2 82 18.3 10 e-7 12.2 1.9 Ascorbate oxidase
1QHQ_A 113 31 10e-7.4 12.1
1.9 AuracyaninB
1V54 B 1 79 20.3 10e-6.0 11.2 2.1 Cytocrome c oxidase
1GY2 A 92 16.3 10e-5.0 11.1
1.8 Rusticyanin
3MSP A 74 8.1 10e-6.7 10.9 2.5 Motile Major Sperm
Protein5
HUZ 74 20.3 10e-5.6 10.3
2.3 Plastocyanin
IKGY E 90 5.6 10e-4.6 10.1
3.4 Ephrinb2
IPMY 75 17.3 10e-4.1 9.8
2.3 Pseudoazurin
'Aligned Length: The number of equivalent pairs of C-alpha atoms superimposed between the two structures, i.e. how many residues have been used to calculate the 3D superposition.
2P-VAL: The VAST p value is a measure of the significance of the comparison, expressed as a probability. For example, if the p value is 0.001, then the odds are 1000 to 1 against seeing a match of this quality by pure chance. The p value from VAST is adjusted for the effects of multiple comparisons using the assumption that there are 500 independent and unrelated types of domains in the MMDB database. The p value shown thus corresponds to the p value for the pairwise comparison of each domain pair, divided by 500.
3Score: The VAST structure-similarity score. This number is related to the number of secondary structure elements superimposed and the quality of that superposition. Higher VAST scores correlate with higher similarity.
4RMSD: The root mean square superposition residual in Angstroms. This number is calculated after optimal superposition of two structures, as the square root of the mean square distances between equivalent C-alpha atoms. Note that the RMSD value scales with the extent of the structural alignments and that this size must be taken into consideration when using RMSD as a descriptor of overall structural similarity. 5 C. elegcms major sperm protein proved to be an ephrin antagonist in oocyte maturation (Kuwabara, 2003 "The multifaceted C. elegans major sperm protein: an ephrin signaling antagonist in oocyte maturation" Genes and Development, 17:155-161.
Azurin
The azurins are copper containing proteins of 128 amino acid residues which belong to the family of cupredoxins involved in electron transfer in plants and certain bacteria. The azurins include those from P. aeruginosa (PA) (SEQ ID NO: 1), A. xylosoxidans, and A. denitrificans (SEQ ID NO: 6). (Murphy et al., J. MoI Biol. 315:859-871 (2002)) The amino acid sequence identity between the azurins varies between 60-90%, these proteins showed a strong structural homology. All azurins have a characteristic β-sandwich with Greek key motif and the single copper atom is always placed at the same region of the protein. In addition, azurins possess an essentially neutral hydrophobic patch surrounding the copper site. Id.
Plastocyanins
The plastocyanins are soluble proteins of cyanobacteria, algae and plants that contain one molecule of copper per molecule and are blue in their oxidized form. They occur in the chloroplast, where they function as electron carriers. Since the determination of the structure of poplar plastocyanin in 1978, the structure of algal (Scenedesmus, Enteromorpha,
Chlamydomonas) and plant (French bean) plastocyanins has been determined either by crystallographic or NMR methods, and the poplar structure has been refined to 1.33 A resolution. SEQ ID NO: 2 shows the amino acid sequence of plastocyanin from Phormidium laminosum, a thermophilic cyanobacterium. Despite the sequence divergence among plastocyanins of algae and vascular plants (e.g., 62% sequence identity between the Chlamydomonas and poplar proteins), the three-dimensional structures are conserved (e.g., 0.76 A rms deviation in the C alpha positions between the Chlamydomonas and Poplar proteins). Structural features include a distorted tetrahedral copper binding site at one end of an eight-stranded antiparallel beta-barrel, a pronounced negative patch, and a flat hydrophobic surface. The copper site is optimized for its electron transfer function, and the negative and hydrophobic patches are proposed to be involved in recognition of physiological reaction partners. Chemical modification, cross-linking, and site-directed mutagenesis experiments have confirmed the importance of the negative and hydrophobic patches in binding interactions with cytochrome f , and validated the model of two functionally significant electron transfer paths involving plastocyanin. One putative electron transfer path is relatively short (approximately 4 A) and involves the solvent- exposed copper ligand His-87 in the hydrophobic patch, while the other is more lengthy (approximately 12-15 A) and involves the nearly conserved residue Tyr-83 in the negative patch, Redinbo et ah, J. Bioenerg. Biomembr. 26:49-66 (1994).
Rusticyanins Rusticyanins are blue-copper containing single-chain polypeptides obtained from a
Thiobacillus (now called Acidithiobacillus). The X-ray crystal structure of the oxidized form of the extremely stable and highly oxidizing cupredoxin rusticyanin from Thiobacillus ferrooxidans (SEQ ID NO: 3) has been determined by multi wavelength anomalous diffraction and refined to 1.9A resolution. The rusticyanins are composed of a core beta- sandwich fold composed of a six- and a seven-stranded b-sheet. Like other cupredoxins, the copper ion is coordinated by a cluster of four conserved residues (His 85, Cysl38, Hisl43, Met 148) arranged in a distorted tetrahedron. Walter, R.L. et al., J. MoI. Biol., vol. 263, pp- 730-51 (1996).
Pseudoazurins
The pseudoazurins are a family of blue-copper containing single-chain polypeptide. The amino acid sequence of pseudoazurin obtained from Achromobacter cycloclastes is shown in SEQ ID NO: 4. The X-ray structure analysis of pseudoazurin shows that it has a similar structure to the azurins although there is low sequence homology between these proteins. Two main differences exist between the overall structure of the pseudoazurins and azurins. There is a carboxy terminus extension in the pseudoazurins, relative to the azurins, consisting of two alpha-helices. In the mid-peptide region azurins contain an extended loop, shortened in the pseudoazurins, which forms a flap containing a short α-helix. The only major differences at the copper atom site are the conformation of the MET side-chain and the Met-S copper bond length, which is significantly shorter in pseudoazurin than in azurin. Phytocyanins
The proteins identifiable as phytocyanins include, but are not limited to, cucumber basic protein, stellacyanin, mavicyanin, umecyanin, a cucumber peeling cupredoxin, a putative blue copper protein in pea pods, and a blue copper protein from Arabidopsis thaliana. In all except cucumber basic protein and the pea-pod protein, the axial methionine ligand normally found at blue copper sites is replaced by glutamine.
Auracyanin Three small blue copper proteins designated auracyanin A, auracyanin B-I, and auracyanin B-2 have been isolated from the thermophilic green gliding photosynthetic bacterium Chloroflexus aurantiacus. The two B forms are glycoproteins and have almost identical properties to each other, but are distinct from the A form. The sodium dodecyl sulfate-polyacrylamide gel electrophoresis demonstrates apparent monomer molecular masses as 14 (A), 18 (B-2), and 22 (B-I) kDa.
The amino acid sequence of auracyanin A has been determined and showed auracyanin A to be a polypeptide of 139 residues. (Van Dreissche et ah, Protein Science 8:947-957 (1999).) His58, Cysl23, Hisl28, and Metl32 are spaced in a way to be expected if they are the evolutionary conserved metal ligands as in the known small copper proteins plastocyanin and azurin. Secondary structure prediction also indicates that auracyanin has a general beta-barrel structure similar to that of azurin from Pseudomonas aeruginosa and plastocyanin from poplar leaves. However, auracyanin appears to have sequence characteristics of both small copper protein sequence classes. The overall similarity with a consensus sequence of azurin is roughly the same as that with a consensus sequence of plastocyanin, namely 30.5%. The N-terminal sequence region 1-18 of auracyanin is remarkably rich in glycine and hydroxy amino acids. Id. See exemplary amino acid sequence SEQ ID NO: 14 for chain A of auracyanin from Chloroflexus aurantiacus (NCBI Protein Data Bank Accession No. AAMl 2874).
The auracyanin B molecule has a standard cupredoxin fold. The crystal structure of auracyanin B from Chloroflexus aurantiacus has been studied. (Bond et ah, J. MoI. Biol. 306:47-67 (2001).) With the exception of an additional N-terminal strand, the molecule is very similar to that of the bacterial cupredoxin, azurin. As in other cupredoxins, one of the Cu ligands lies on strand 4 of the polypeptide, and the other three lie along a large loop between strands 7 and 8. The Cu site geometry is discussed with reference to the amino acid spacing between the latter three ligands. The crystallographically characterized Cu-binding domain of auracyanin B is probably tethered to the periplasmic side of the cytoplasmic membrane by an N-terminal tail that exhibits significant sequence identity with known tethers in several other membrane-associated electron-transfer proteins. The amino acid sequences of the B forms are presented in McManus et al. (J Biol Chem. 267:6531-6540 (1992).). See exemplary amino acid sequence SEQ ID NO: 15 for chain B of auracyanin from Chloroflexus aurantiacus (NCBI Protein Data Bank Accession No. IQHQA).
Stellacyanin
Stellacyanins are a subclass of phytocyanins, a ubiquitous family of plant cupredoxins. An exemplary sequence of a stellacyanin is included herein as SEQ ID NO: 13. The crystal structure of umecyanin, a stellacyanin from horseradish root (Koch et al, J. Am. Chem. Soc. 127:158-166 (2005)) and cucumber stellacyanin (Hart el al., Protein Science
5:2175-2183 (1996).). The protein has an overall fold similar to the other phytocyanins. The ephrin B2 protein ectodomain tertiary structure bears a significant similarity to stellacyanin. (Toth et al, Developmental Cell 1 :83-92 (2001).) An exemplary amino acid sequence of a stellacyanin is found in the National Center for Biotechnology Information Protein Data Bank as Accession No . 1 JER, SEQ ID NO : 13.
Cucumber basic protein
An exemplary amino acid sequence from a cucumber basic protein is included herein as SEQ ID NO: 16. The crystal structure of the cucumber basic protein (CBP), a type 1 blue copper protein, has been refined at 1.8 A resolution. The molecule resembles other blue copper proteins in having a Greek key beta-barrel structure, except that the barrel is open on one side and is better described as a "beta-sandwich" or "beta-taco". (Guss et al, J. MoI Biol. 262:686-705 (1996).) The ephrinB2 protein ectodomain tertiary structure bears a high similarity (rms deviation 1.5A for the 50 α carbons) to the cucumber basic protein. (Toth et al, Developmental Cell 1 :83-92 (2001).)
The Cu atom has the normal blue copper NNSS' co-ordination with bond lengths Cu- N(His39) = 1.93 A, Cu-S(Cys79) = 2.16 A, Cu-N(His84) = 1.95 A, Cu-S(Met89) = 2.61 A. A disulphide link, (Cys52)-S-S-(Cys85), appears to play an important role in stabilizing the molecular structure. The polypeptide fold is typical of a sub-family of blue copper proteins (phytocyanins) as well as a non-metalloprotein, ragweed allergen Ra3, with which CBP has a high degree of sequence identity. The proteins currently identifiable as phytocyanins are CBP, stellacyanin, mavicyanin, umecyanin, a cucumber peeling cupredoxin, a putative blue copper protein in pea pods, and a blue copper protein from Arabidopsis thaliana. In all except CBP and the pea-pod protein, the axial methionine ligand normally found at blue copper sites is replaced by glutamine. An exemplary sequence for cucumber basic protein is found in NCBI Protein Data Bank Accession No. 2CBP, SEQ ID NO: 16.
Cytochromes
Cytochrome C551
Cytochrome C551 from P. aeruginosa (Pa-C551) is a monomeric redox protein of 82 amino-acid residues (SEQ ID NO: 21), involved in dissimilative denitrification as the physiological electron donor of nitrite reductase. The functional properties of Pa-C551 have been extensively investigated. The reactions with non-physiological small inorganic redox reactants and with other macromolecules, like blue copper proteins, eukaryotic cytochrome c and the physiological partner nitrite reductase have provided a test for protein-protein electron transfer. The three-dimensional structure of Pa-C551, which is a member of bacterial class I cytochromes, shows a single low-spin heme with His-Met ligation and the typical polypeptide fold which however leaves the edges of pyrrole rings II and III of the heme exposed (Cutruzzola et al, J. Morgan. Chem. 88:353-61 (2002)). The lack of a 20-residue omega loop, present in the mammalian class I cytochromes, causes further exposure of the heme edge at the level of propionate 13. The distribution of charged residues on the surface of Pa-C551 is very anisotropic: one side is richer in acidic residues whereas the other displays a ring of positive side chains, mainly lysines, located at the border of a hydrophobic patch which surrounds the heme crevice. This patch comprises residues Glyll, VaI 13, Alal4, Met22, Val23, Pro58, Ile59, Pro60, Pro62, Pro63 and Ala65. The anisotropic charge distribution leads to a large dipolar moment which is important for electron transfer complex formation. The charge distribution described above for Pa-C551 has been reported for other electron transfer proteins and their electron acceptors. Moreover, modification by site- directed mutagenesis of residues within the hydrophobic or charged patch has shown for different proteins the importance of surface complementarity for binding and electron transfer. As an example, evidence for the relevance of the hydrophobic patch for the electron transfer properties of azurin from P. aeruginosa came from the studies carried out on mutants of residues Met44 and Met64 changed to positively and negatively charged amino acids. Id The cytochrome c-type domain has a fold consisting of a series of alpha helices and reverse turns that serve to envelop the covalently bound haem within a hydrophobic pocket. This domain can be found in monodomain cytochrome c proteins, such as cytochrome c6, cytochrome C552, cytochrome c459 and mitochondrial cytochrome c. The cytochrome c-type domain occurs in a number of other proteins, such as in cytochrome cdl -nitrite reductase as the N-terminal haem c domain, in quinoprotein alcohol dehydrogenase as the C-terminal domain, in Quinohemoprotein amine dehydrogenase A chain as domains 1 and 2, and in the cytochrome bcj complex as the cytochrome bet domain. Structural analysis with VAST algorithm (cytochrome C551 from Pseudomonas aeruginosa as a query) showed significant structural neighbors (P values between 10"1 to 10"4 5) only for cytochromes.
Methods of Use The invention provides methods to administer to a patient the compositions comprising cupredoxin or cytochrome, and variants, derivatives and structural equivalents of cupredoxin or cytochrome. Specifically, the invention provides methods to administer to a patient a composition comprising at least one peptide, or at least two peptides that are a cupredoxin, cytochrome and variants, derivatives and structural equivalents of cupredoxin or cytochrome. More specifically, the invention provides methods to administer to a human a composition comprising at least one peptide that is a cupredoxin, cytochrome and variants, derivatives and structural equivalents of cupredoxin or cytochrome. The invention provides methods to administer to a patient compositions comprising cupredoxin or cytochrome and variants, derivatives and structural equivalents of cupredoxin or cytochrome, and their use to concurrently treat and/or prevent two or more conditions in a patient. In a specific embodiment, the methods may utilize pharmaceutical compositions for the administration to a patient. In another specific embodiment, the invention provides methods for the concurrent prevention and/or treatment of two or more conditions such as interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papillomavirus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), Para influenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus, arena virus, Dhori virus, poliovirus, rubella virus, dengue virus; SIV, Mycobacterium tuberculosis, melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors and prostate cancer. In another specific embodiment, the methods may utilize compositions administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from one or more of the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
Members of the Cupredoxin family, specifically azurin from Pseudomonas aeruginosa, are promising compounds for therapeutic and preventative treatment of numerous conditions. Such conditions may include, but are not limited to HIV, malaria, cancer and inappropriate angiogenesis. For example, two redox proteins elaborated by P. aeruginosa, the cupredoxin azurin and cytochrome CsS1 (Cyt Cs51), both enter J774 cells and show significant cytotoxic activity towards the human cancer cells as compared to normal cells. Zaborina et ah, Microbiology 146: 2521-2530 (2000). Azurin can also enter human melanoma UISO-Mel-2 or human breast cancer MCF-7 cells. Yamada et al, PNAS
99:14098-14103 (2002); Punj et al, Oncogene 23:2367-2378 (2004); Yamada et al, Cell. Biol. 7:14181431 (2005). In addition, azurin from P. aeruginosa preferentially enters J774 murine reticulum cell sarcoma cells, forms a complex with and stabilizes the tumor suppressor protein p53, enhances the intracellular concentration of p53, and induces apoptosis . Yamada et al, Infection and Immunity, 70:7054-7062 (2002). Azurin also caused a significant increase of apoptosis in human osteosarcoma cells as compared to noncancerous cells. Ye et al, Ai Zheng 24:298-304 (2003). Rusticyanin from Thiobacillus ferrooxidans can also enter macrophages and induce apoptosis. Yamada et al. , Cell Cycle 3:1182-1187 (2004); Yamada et al., Cell. Micro. 7:1418-1431 (2005). Plastocyanin from Phormidium laminosum and pseudoazurin form Achromobacter cycloclastes also are cytotoxic towards macrophages. U.S. Pat. Pub. No. 20060040269, published Feb. 23, 2006. Azurin is also known to have other pharmacologic activities of therapeutic importance. It is known to inhibit angiogenesis in human umbilical vascular endothelium cells (HUVECs). U.S. Patent Application No. 11/488,693, filed July 19, 2006. Azurin from P. aeruginosa is also known for its ability to inhibit the growth of HIV-I infection in peripheral blood mononuclear cells and to inhibit parasitemia of malaria-infected mammalian red blood cells . Chaudhari et al, Cell Cycle. 5: 1642-1648 (2006). Azurin from P. aeruginosa is also known to interfere with the ephrin signaling system in various mammalian cells and tissues. U.S. Patent Application No. 11/436,592, filed May 19, 2006.
In another specific embodiment, the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, wherein the patient has at least one "high risk feature." "High risk features" may be factors of the patient that increase the risk of a patient developing one or more conditions or where the patient has a higher risk than the general population.
The increased risk may be due to numerous variables or factors such as, but not limited to, environmental and behavioral factors, increased risk caused from other conditions, and genetic predisposition.
For example, an HIV infected patient is associated with an increased risk of acquiring large cell lymphoma or Kaposi's sarcoma. The Merck Manual of Diagnosis and Therapy (Beers et al., 18 edition, Merck Research Laboratories, 2006). For another example, a female patient that acquires human papillomavirus has an increased risk of acquiring cervical carcinoma. Id.
Environmental factors may include, but are not limited to, a patient's lifestyle, eating habits and/or geographic location. For example, co-infections with HIV and malaria are very common in many areas of the world, and in particular sub-Saharan Africa
Behavioral factors may include actions by the patient that predispose a patient to many conditions. For example, the risk of acquiring cancer and heart disease may be increased due to factors such as, but not limited to, smoking, diet, alcohol consumption, hormone replacement therapy and higher body mass index. Genetic predisposition may play a factor in a patient acquiring numerous conditions. For example, it is known that when a person carries a particular cystic fibrosis transmembrane regulator (CFTK) mutation, that person has a higher risk for cystic fibrosis and pancreatic cancer. Weiss et al., Gut; 54: 1456-1460 (2005). For another example, genetic factors that predispose a patient to various forms of cancer include, but are not limited to, a family history of cancer, gene carrier status of BRCAl and BRCA2, prior history of breast neoplasia, familial adenomatous polyposis (FAP), hereditary nonpolyposis colorectal cancer (HNPCC), red or blond hair and fair-skinned phenotype, xeroderma pigmentosum, and ethnicity. Patients with high risk features, such as higher risk to develop cancer than the general population may be patients with premalignant lesions, and patients that have been cured of their initial cancer or definitively treated for their premalignant lesions. See generally Tsao et al. , CA Cancer J Clin 54: 150-180 (2004). Additionally, patients at a higher risk of developing cancer may be determined by the use of various risk models that have been developed for certain kinds of cancer. For example, patients predisposed to breast cancer may be determined using the Gail risk model, or the Claus model, among others. See Gail et al, J Natl Cancer Inst 81 :1879-1886 (1989); Cuzick, Breast 12:405-411 (2003); Huang et al, Am J Epidemiol 151 :703-714 (2000).
In a specific embodiment, the methods may utilize compositions to be administered to a patient for the concurrent treatment and/or prevention of two or more conditions where the patient has a higher risk than the general population of acquiring a condition. Such conditions may include, but are not limited to, cancer, HIV, malaria or inappropriate angiogenesis.
In a specific embodiment, the methods may comprise a composition including a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of malaria, wherein the patient is additionally suffering from HIV, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, cancer or inappropriate angiogenesis.
In another specific embodiment, the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of HIV, wherein the patient is additionally suffering from malaria, cancer or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as malaria, cancer or inappropriate angiogenesis.
In another specific embodiment, the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of cancer, wherein the patient is additionally suffering from HIV, malaria or inappropriate angiogenesis or has a higher risk than the general population of acquiring a condition such as HIV, malaria or inappropriate angiogenesis.
. In another specific embodiment, the methods may utilize a composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof, as a therapeutic agent for the treatment of inappropriate angiogenesis, wherein the patient is additionally suffering from HIV, cancer or malaria or has a higher risk than the general population of acquiring a condition such as HIV, cancer or malaria.
The compositions comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be administered to the patient by many routes and in many regimens that will be well known to those in the art. In specific embodiments, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof is administered intravenously, intramuscularly, subcutaneously, topically, orally, or by inhalation.
In another specific embodiment, the methods may utilize compositions that additionally comprise another drug. In a specific embodiment, the additional drug may be an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
In one specific embodiment, the methods may comprise co-administering to a patient one unit dose of a composition comprising a cupredoxin, cytochrome or a variant, derivative, truncation, or structural equivalent of cupredoxin or cytochrome and one unit dose of a composition comprising another drug, in either order, administered at about the same time, or within about a given time following the administration of the other, for example, about one minute to about 60 minutes following the administration of the other drug, or about 1 hour to about 12 hours following the administration of the other drug. In another embodiment, the other drug may be, but is not limited to an anti-malarial drug, an anti-HIV drug, an anti- cancer drug, and an anti-angiogenesis drug.
Anti-malarial drugs of interest include, but are not limited to, proguanil, chlorproguanil, trimethoprim, chloroquine, mefloquine, lumefantrine, atovaquone, pyrimethamine-sulfadoxine, pyrimethamine-dapsone, halofantrine, quinine, quinidine, amodiaquine, amopyroquine, sulphonamides, artemisinin, arteflene, artemether, artesunate, primaquine, pyronaridine, proguanil, chloroquine, mefloquine, pyrimethamine-sulfadoxine, pyrimethamine-dapsone, halofantrine, quinine, proguanil, chloroquine, mefloquine, 1,16- hexadecamethylenebis(N-methylpyrrolidinium)dibromide, and combinations thereof.
Anti-HIV drugs include, but are not limited to, reverse transcriptase inhibitors: AZT (zidovudine [Retrovir]), ddC (zalcitabine [Hivid], dideoxyinosine), d4T (stavudine [Zerit]), and 3TC (lamivudine [Epivir]), nonnucleoside reverse transcriptase inhibitors (NNRTIS): delavirdine (Rescriptor) and nevirapine (Viramune), protease inhibitors: ritonavir (Norvir), a lopinavir and ritonavir combination (Kaletra), saquinavir (Invirase), indinavir sulphate (Crixivan), amprenavir (Agenerase), and nelfinavir (Viracept). In some embodiments, a combination of several drugs called highly active antiretro viral therapy (HAART) is used to treat people with HIV.
Anti-cancer and/or anti-angiogenesis drugs of interest include, but are not limited to, tamoxifen, aromatase inhibitors such as letrozole and anastrozole (Arimidex j, retinoids such as N-[4-hydroxyphenyl] retinamide (4-HPR, fenretinide), nonsteriodal anti-inflammatory agents (NSAIDs) such as aspirin and sulindac, celecoxib (COX-2 inhibitor), defluoromethylornithing (DFMO), ursodeoxycholic acid, 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors, EKI-785 (EGFR inhibitor), bevacizumab (antibody to VEGF-receptor), cetuximab (antibody to EGFR), retinol such as vitamin A, beta-carotene, 13-cis retinoic acid, isotretinoin and retinyl palmitate, α-tocopherol, interferon, oncolytic adenovirus dll520 (ONYX-Ol 5), gefitinib, etretinate, finasteride, indole-3-carbinol, resveratrol, chlorogenic acid, raloxifene, and oltipraz.
Pharmaceutical Compositions Comprising Cupredoxin, Or Variant, Derivative, Truncation, Or Structural Equivalent Thereof
Pharmaceutical compositions comprising cupredoxin or cytochrome, or variant, derivative, truncation, or structural equivalents thereof, can be manufactured in any conventional manner, e.g., by conventional mixing, dissolving, granulating, dragee-making, emulsifying, encapsulating, entrapping, or lyophilizing processes. The substantially pure or pharmaceutical grade cupredoxin, cytochrome or variants, derivatives and structural equivalents thereof can be readily combined with a pharmaceutically acceptable carrier well- known in the art. Such carriers enable the preparation to be formulated as a tablet, pill, dragee, capsule, liquid, gel, syrup, slurry, suspension, and the like. Suitable carriers or excipients can also include, for example, fillers and cellulose preparations. Other excipients can include, for example, flavoring agents, coloring agents, detackifϊers, thickeners, and other acceptable additives, adjuvants, or binders. In some embodiments, the pharmaceutical preparation is substantially free of preservatives. In other embodiments, the pharmaceutical preparation may contain at least one preservative. General methodology on pharmaceutical dosage forms is found in Ansel et ah, Pharmaceutical Dosage Forms and Drug Delivery Systems (Lippencott Williams & Wilkins, Baltimore MD (1999)).
The composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof used in the invention may be administered in a variety of ways, including by injection (e.g., intradermal, subcutaneous, intramuscular, intraperitoneal and the like), by inhalation, by topical administration, by suppository, by using a transdermal patch or by mouth. General information on drug delivery systems can be found in Ansel et al, id.. In some embodiments, the composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be formulated and used directly as injectables, for subcutaneous and intravenous injection, among others. The injectable formulation, in particular, can advantageously be used to prevent and/or treat patients with more than one condition. The composition comprising a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can also be taken orally after mixing with protective agents such as polypropylene glycols or similar coating agents.
When administration is by injection, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be formulated in aqueous solutions, specifically in physiologically compatible buffers such as Hanks solution, Ringer's solution, or physiological saline buffer. The solution may contain formulatory agents such as suspending, stabilizing and/or dispersing agents. Alternatively, the cupredoxin or variant, derivative, truncation, or structural equivalent thereof may be in powder form for constitution with a suitable vehicle, e.g. , sterile pyrogen-free water, before use. In some embodiments, the pharmaceutical composition does not comprise an adjuvant or any other substance added to enhance the immune response stimulated by the peptide. In some embodiments, the pharmaceutical composition comprises a substance that inhibits an immune response to the peptide. When administration is by intravenous fluids, the intravenous fluids for use administering the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be composed of crystalloids or colloids. Crystalloids as used herein are aqueous solutions of mineral salts or other water-soluble molecules. Colloids as used herein contain larger insoluble molecules, such as gelatin. Intravenous fluids may be sterile. Crystalloid fluids that may be used for intravenous administration include but are not limited to, normal saline (a solution of sodium chloride at 0.9% concentration), Ringer's lactate or Ringer's solution, and a solution of 5% dextrose in water sometimes called D5W, as described in Table 2.
Table 2. Composition of Common Crystalloid Solutions
Solution Other Name [Na+] [Cl ] [Glucose]
D5W 5% Dextrose 0 0 252
2/3 & 1/3 3.3% Dextrose 51 51 168 / 0.3% saline
Half-normal 0.45% NaCl 77 77 0 saline
Normal saline 0.9% NaCl 154 154 0
Ringer's Ringer's 130 109 0 lactate* solution
*Ringer's lactate also has 28 mmol/L lactate, 4 mmol/L K+ and 3 mmol/L Ca' 2+ When administration is by inhalation, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be delivered in the form of an aerosol spray from pressurized packs or a nebulizer with the use of a suitable propellant, e.g., dichlorodifluoromethane, trichlorofluoromethane, carbon dioxide or other suitable gas. In the case of a pressurized aerosol, the dosage unit may be determined by providing a valve to deliver a metered amount. Capsules and cartridges of, e.g., gelatin, for use in an inhaler or insufflator may be formulated containing a powder mix of the proteins and a suitable powder base such as lactose or starch.
When administration is by topical administration, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof may be formulated as solutions, gels, ointments, creams, jellies, suspensions, and the like, as are well known in the art. In some embodiments, administration is by means of a transdermal patch. When administration is by suppository (e.g., rectal or vaginal), cupredoxin, cytochrome or variants and derivatives thereof compositions may also be formulated in compositions containing conventional suppository bases.
When administration is oral, a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be readily formulated by combining the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof with pharmaceutically acceptable carriers well known in the art. A solid carrier, such as mannitol, lactose, magnesium stearate, and the like may be employed; such carriers enable the cupredoxin and variants, derivatives or structural equivalent thereof to be formulated as tablets, pills, dragees, capsules, liquids, gels, syrups, slurries, suspensions and the like, for oral ingestion by a subject to be treated. For oral solid formulations such as, for example, powders, capsules and tablets, suitable excipients include fillers such as sugars, cellulose preparation, granulating agents, and binding agents.
Other convenient carriers, as well-known in the art, also include multivalent carriers, such as bacterial capsular polysaccharide, a dextran or a genetically engineered vector. In addition, sustained-release formulations that include a cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof allow for the release of cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof over extended periods of time, such that without the sustained release formulation, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof would be cleared from a subject's system, and/or degraded by, for example, proteases and simple hydrolysis before eliciting or enhancing a therapeutic effect.
The half-life in the bloodstream of the compositions of the invention can be extended or optimized by several methods well known to those in the art, including but not limited to, circularized peptides (Monk et al, BioDrugs 19(4):261-78, (2005); DeFreest et al., J. Pept. Res. 63(5):409-19 (2004)), D,L-peptides (diastereomer), (Futaki et al, J. Biol. Chem. Feb 23;276(8):5836-40 (2001); Papo et al, Cancer Res. 64(16):5779-86 (2004); Miller et al, Biochem. Pharmacol. 36(l):169-76, (1987)); peptides containing unusual amino acids (Lee et al, J. Pept. Res. 63(2):69-84 (2004)), N- and C- terminal modifications (Labrie et al, Clin. Invest. Med. 13(5):275-8, (1990)), and hydrocarbon stapling (Schafmeister et al, J. Am. Chem. Soc. 122:5891-5892 (2000); Walenski et al, Science 305:1466-1470 (2004)). Of particular interest are d-isomerization (substitution) and modification of peptide stability via D-substitution or L- amino acid substitution and hydrocarbon stapling
In various embodiments, the pharmaceutical composition includes carriers and excipients (including but not limited to buffers, carbohydrates, mannitol, proteins, polypeptides or amino acids such as glycine, antioxidants, bacteriostats, chelating agents, suspending agents, thickening agents and/or preservatives), water, oils, saline solutions, aqueous dextrose and glycerol solutions, other pharmaceutically acceptable auxiliary substances as required to approximate physiological conditions, such as buffering agents, tonicity adjusting agents, wetting agents and the like. It will be recognized that, while any suitable carrier known to those of ordinary skill in the art may be employed to administer the compositions of this invention, the type of carrier will vary depending on the mode of administration. Compounds may also be encapsulated within liposomes using well-known technology. Biodegradable microspheres may also be employed as carriers for the pharmaceutical compositions of this invention. Suitable biodegradable microspheres are disclosed, for example, in U.S. Patent Nos. 4,897,268; 5,075,109; 5,928,647; 5,811,128; 5,820,883; 5,853,763; 5,814,344 and 5,942,252.
The pharmaceutical compositions may be sterilized by conventional, well-known sterilization techniques, or may be sterile filtered. The resulting aqueous solutions may be packaged for use as is, or lyophilized, the lyophilized preparation being combined with a sterile solution prior to administration. Administration of Cupredoxin And/Or Cytochrome And Variants And Derivatives And Structural Equivalents Thereof
The cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof can be administered formulated as pharmaceutical compositions and administered by any suitable route, for example, by oral, buccal, inhalation, sublingual, rectal, vaginal, transurethral, nasal, topical, percutaneous, i.e., transdermal or parenteral (including intravenous, intramuscular, subcutaneous and intracoronary) or vitreous administration. The pharmaceutical formulations thereof can be administered in any amount effective to achieve its intended purpose. More specifically, the composition is administered in a therapeutically effective amount. In specific embodiments, the therapeutically effective amount is generally from about 0.01-20 mg/day/kg of body weight.
The compounds comprising cupredoxin or variant, derivative, truncation, or structural equivalent thereof are useful for the prevention and/or treatment of more than one condition, alone or in combination with other active agents. The appropriate dosage will, of course, vary depending upon, for example, the compound of cupredoxin or variant, derivative, truncation, or structural equivalent thereof employed, the host, the mode of administration and the nature and severity of the potential cancer. However, in general, satisfactory results in humans are indicated to be obtained at daily dosages from about 0.01-20 mg/kg of body weight. An indicated daily dosage in humans is in the range from about 0.7 mg to about 1400 mg of a compound of cupredoxin or variant, derivative, truncation, or structural equivalent thereof conveniently administered, for example, in daily doses, weekly doses, monthly doses, and/or continuous dosing. Daily doses can be in discrete dosages from 1 to 12 times per day. Alternatively, doses can be administered every other day, every third day, every fourth day, every fifth day, every sixth day, every week, and similarly in day increments up to 31 days or over. Alternatively, dosing can be continuous using patches, i.v. administration and the like.
The exact formulation, route of administration, and dosage is determined by the attending physician in view of the patient's condition. Dosage amount and interval can be adjusted individually to provide plasma levels of the active cupredoxin or variant, derivative, truncation, or structural equivalent thereof which are sufficient to maintain therapeutic effect. Generally, the desired cupredoxin or variant, derivative, truncation, or structural equivalent thereof is administered in an admixture with a pharmaceutical carrier selected with regard to the intended route of administration and standard pharmaceutical practice. In one aspect, the cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof is delivered as DNA such that the polypeptide is generated in situ. In one embodiment, the DNA is "naked," as described, for example, in Ulmer et al., (Science 259:1745-1749 (1993)) and reviewed by Cohen (Science 259:1691-1692 (1993)). The uptake of naked DNA may be increased by coating the DNA onto a carrier, e.g., biodegradable beads, which are then efficiently transported into the cells. In such methods, the DNA may be present within any of a variety of delivery systems known to those of ordinary skill in the art, including nucleic acid expression systems, bacterial and viral expression systems. Techniques for incorporating DNA into such expression systems are well known to those of ordinary skill in the art. See, e.g. , WO90/11092, WO93/24640, WO 93/17706, and U.S. Pat. No. 5,736,524.
Vectors, used to shuttle genetic material from organism to organism, can be divided into two general classes: Cloning vectors are replicating plasmid or phage with regions that are essential for propagation in an appropriate host cell and into which foreign DNA can be inserted; the foreign DNA is replicated and propagated as if it were a component of the vector. An expression vector (such as a plasmid, yeast, or animal virus genome) is used to introduce foreign genetic material into a host cell or tissue in order to transcribe and translate the foreign DNA, such as the DNA of a cupredoxia In expression vectors, the introduced DNA is operably-linked to elements such as promoters that signal to the host cell to highly transcribe the inserted DNA. Some promoters are exceptionally useful, such as inducible promoters that control gene transcription in response to specific factors. Operably-linking a cupredoxin and variants and derivatives thereof polynucleotide to an inducible promoter can control the expression of the cupredoxin and variants and derivatives thereof in response to specific factors. Examples of classic inducible promoters include those that are responsive to α-interferon, heat shock, heavy metal ions, and steroids such as glucocorticoids (Kaufman, Methods Enzymol. 185:487-511 (1990)) and tetracycline. Other desirable inducible promoters include those that are not endogenous to the cells in which the construct is being introduced, but, are responsive in those cells when the induction agent is exogenously supplied. In general, useful expression vectors are often plasmids. However, other forms of expression vectors, such as viral vectors (e.g., replication defective retroviruses, adenoviruses and adeno-associated viruses) are contemplated Vector choice is dictated by the organism or cells being used and the desired fate of the vector. In general, vectors comprise signal sequences, origins of replication, marker genes, polylinker sites, enhancer elements, promoters, and transcription termination sequences. The exact formulation, route of administration, and dosage is determined by the attending physician in view of the patient's condition. Dosage amount and interval can be adjusted individually to provide plasma levels of the active cupredoxin and/or cytochrome and variants and derivatives thereof which are sufficient to treat the patient and/or maintain therapeutic effect. Generally, the desired cupredoxin and/or cytochrome and variants and derivatives thereof can be administered in an admixture with a pharmaceutical carrier selected with regard to the intended route of administration and standard pharmaceutical practice. Pharmaceutical compositions used in accordance with the present invention can be formulated in a conventional manner using one or more physiologically acceptable carriers comprising excipients and auxiliaries that facilitate processing of the cupredoxin and/or cytochrome and variants and derivatives thereof, active agents, for inhibiting or stimulating the secretion of cupredoxin and/or cytochrome and variants and derivatives thereof, or a mixture thereof into preparations which can be used therapeutically.
Kits Comprising Cupredoxin, And/Or Cytochrome, Or Variant, Derivative, Truncation, Or Structural Equivalent Thereof
In one aspect, the invention provides regimens or kits comprising one or more of the following in a package or container: (1) a pharmacologically active composition comprising at least one cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalent thereof; (2) an additional chemopreventive drug, (3) apparatus to administer the biologically active composition to the patient, such as a syringe, nebulizer etc..
When a kit is supplied, the different components of the composition may be packaged in separate containers, if appropriate, and admixed immediately before use. Such packaging of the components separately may permit long-term storage without losing the active components' functions. The reagents included in the kits can be supplied in containers of any sort such that the life of the different components are preserved and are not adsorbed or altered by the materials of the container. For example, sealed glass ampoules may contain lyophilized cupredoxin and variants, derivatives and structural equivalents thereof, or buffers that have been packaged under a neutral, non-reacting gas, such as nitrogea Ampoules may consist of any suitable material, such as glass, organic polymers, such as polycarbonate, polystyrene, etc., ceramic, metal or any other material typically employed to hold similar reagents. Other examples of suitable containers include simple bottles that may be fabricated from similar substances as ampoules, and envelopes, that may comprise foil-lined interiors, such as aluminum or an alloy. Other containers include test tubes, vials, flasks, bottles, syringes, or the like. Containers may have a sterile access port, such as a bottle having a stopper that can be pierced by a hypodermic injection needle. Other containers may have two compartments that are separated by a readily removable membrane that upon removal permits the components to be mixed. Removable membranes may be glass, plastic, rubber, etc.
Kits may also be supplied with instructional materials. Instructions may be printed on paper or other substrate, and/or may be supplied as an electronic-readable medium, such as a floppy disc, CD-ROM, DVD-ROM, Zip disc, videotape, audiotape, flash memory device etc. Detailed instructions may not be physically associated with the kit; instead, a user may be directed to an internet web site specified by the manufacturer or distributor of the kit, or supplied as electronic mail.
Modification of Cupredoxin and Variants, Derivatives and Structural Equivalents Thereof
Cupredoxin, cytochrome or variant, derivative, truncation, or structural equivalents thereof may be chemically modified or genetically altered to produce variants and derivatives as explained above. Such variants and derivatives may be synthesized by standard techniques. In addition to naturally-occurring allelic variants of cupredoxin, changes can be introduced by mutation into cupredoxin coding sequence that incur alterations in the amino acid sequences of the encoded cupredoxin that do not significantly alter the ability of cupredoxin to inhibit the development of premalignant lesions. A "non-essential" amino acid residue is a residue that can be altered from the wild-type sequences of the cupredoxin without altering pharmacologic activity, whereas an "essential" amino acid residue is required for such pharmacologic activity. For example, amino acid residues that are conserved among the cupredoxins are predicted to be particularly non-amenable to alteration, and thus "essential."
Amino acids for which conservative substitutions that do not change the pharmacologic activity of the polypeptide can be made are well known in the art. Useful conservative substitutions are shown in Table 3, "Preferred substitutions." Conservative substitutions whereby an amino acid of one class is replaced with another amino acid of the same type fall within the scope of the invention so long as the substitution does not materially alter the pharmacologic activity of the compound.
Table 3. Preferred substitutions
Preferred
Original residue Exemplary substitutions substitutions
Ala (A) VaI, Leu, He VaI
Arg (R) Lys, GIn, Asn Lys
Asn (N) GIn, His, Lys, Arg GIn
Asp (D) GIu GIu
Cys (C) Ser Ser
GIn (Q) Asn Asn
GIu (E) Asp Asp
GIy (G) Pro, Ala Ala
His (H) Asn, GIn, Lys, Arg Arg
Leu, VaI, Met, Ala, Phe,
He (I) Leu Norleucine
Norleucine, He, VaI, Met, Ala,
Leu (L) He Phe
Lys (K) Arg, GIn, Asn Arg
Met (M) Leu, Phe, He Leu
Phe (F) Leu, VaI, He, Ala, Tyr Leu
Pro (P) Ala Ala
Ser (S) Thr Thr
Thr (T) Ser Ser
Tip (W) Tyr, Phe Tyr
Tyr (Y) Trp, Phe, Thr, Ser Phe
He, Leu, Met, Phe, Ala,
VaI (V) Leu Norleucine
Non-conservative substitutions that affect (1) the structure of the polypeptide backbone, such as a β-sheet or α-helical conformation, (2) the charge, (3) hydrophobicity, or (4) the bulk of the side chain of the target site can modify the pharmacologic activity. Residues are divided into groups based on common side-chain properties as denoted in Table 4. Non-conservative substitutions entail exchanging a member of one of these classes for another class. Substitutions may be introduced into conservative substitution sites or more specifically into non-conserved sites.
Table 4. Amino acid classes
Class Amino acids hydrophobic Norleucine, Met, Ala, VaI, Leu, He neutral hydrophilic Cys, Ser, Thr acidic Asp, GIu basic Asn, GIn, His, Lys, Arg disrupt chain conformation GIy, Pro aromatic Trp, Tyr, Phe
The variant polypeptides can be made using methods known in the art such as oligonucleotide-mediated (site-directed) mutagenesis, alanine scanning, and PCR mutagenesis. Site-directed mutagenesis (Carter, Biochem J. 237:1-7 (1986); Zoller and Smith, Methods Enzymol. 154:329-350 (1987)), cassette mutagenesis, restriction selection mutagenesis (Wells et al, Gene 34:315-323 (1985)) or other known techniques can be performed on the cloned DNA to produce the cupredoxin variant DNA.
Known mutations of cupredoxins and cytochrome can also be used to create variant cupredoxin and cytochrome to be used in the methods of the invention. For example, the C 112D and M44KM64E mutants of azurin are known to have cytotoxic and growth arresting activity that is different from the native azurin, and such altered activity can be useful in the treatment and/or prevention methods of the present invention.
A more complete understanding of the present invention can be obtained by reference to the following specific Examples. The Examples are described solely for purposes of illustration and are not intended to limit the scope of the invention. Changes in form and substitution of equivalents are contemplated as circumstances may suggest or render expedient. Although specific terms have been employed herein, such terms are intended in a descriptive sense and not for purposes of limitations. Modifications and variations of the invention as hereinbefore set forth can be made without departing from the spirit and scope thereof. EXAMPLES
Example 1. Entry of p28 into human umbilical vein endothelial cells. p28 was labeled with 20μM Alexafluor® 568 (Molecular Probes, Eugene, OR). Indicated cell lines were cultured on cell culture coated cover slips overnight at 37°C. Pre- warmed media containing labeled peptide was added at indicated concentrations. After incubation with the labeled peptide, the cover slips were washed 3X with PBS and fixed in formalin for 5 minutes. Cover slips were then mounted in media containing 1.5 μg ml"1 DAPI for nuclear staining (VECTASHIELD®, Vector Laboratories, Burlingame, CA). Analysis was performed with a confocal microscope (Model LC510, Carl Zeiss, Thornwood, NY). p28 effectively entered malignant cell lines originating from melanoma, breast, pancreas, glioblastoma, astrocytoma, and lung (Fig. IA). p28 was also efficiently entered HUVEC cells (Fig. 1C). No significant entry was observed in other "normal" cell lines originating from skin fibroblasts, breast and pancreas Fig. IB). Therefore, in addition to specifically entering mammalian cancer cells, p28 also specifically enters HUVEC cells.
This experiment shows that the P. aeruginosa azurin 50-77 peptide has activity that inhibits capillary tube formation in endothelial cells, one step in angiogenesis. The P. aeruginosa azurin 50-77 peptide can therefore be used to control angiogenesis and hence be utilized as a cancer treatment, and treatment of other conditions related to inappropriate angiogenesis.
Example 2. Effects of p28 on HUVEC capillary tube formation on Matrigel .
Matrigel® Matrix (Becton Dickinson Biosciences, San Jose CA) is a solubulized basement membrane preparation extracted from EHS mouse sarcoma, a tumor rich in ECM proteins. Its major component is laminin, followed by collagen IV, heparan sulfate proteoglycans, and entactin 1. At room temperature, Matrigel Matrix polymerizes to produce biologically active matrix material resembling the mammalian cellular basement membrane. Cells behave as they do in vivo when they are cultured on Matrigel® Matrix. It provides a physiologically relevant environment for studies of cell morphology, biochemical function, migration or invasion, and gene expression. Matrigel® Matrix serves as a substrate for in vitro endothelial cell invasion and tube formation assays. The effects of p28 on the capillary tube formation of HUVEC cells were investigated using Matrigel®. HUVEC cells were plated (15,000 cells/well) on Matrigel® coated 8 well chamber slides with 20ng/ml VEGF and in the presence or absence of peptide. p28 concentrations of OμM (control), O.lOμM, 0.30μM, 0.92μM, 2.77μM, 8.33μM, 25μM and 75 μM were used. Cells were stained 4h and 24h post-treatment with calcein AM, and capillary tube formation was examined using a fluorescence microscope (Fig. 2A). The results show that as little as O.lOμM prevented capillary tube formation by HUVEC cells by about 50% (Fig. 2A). p28 therefore inhibits tube formation of HUVEC cells, and will therefore also inhibit the capillary tube formation related to angiogenesis.
Example 3. Effects of p28 on HUVEC motility.
The effects of p28 on HUVEC motility was investigated with the scratch wound migration assay. HUVEC cells were plated in 60mm tissue culture dishes and allowed to reach 90% confluence. After removing the media, cell layers were wounded using a 1 ml sterile plastic pipette tip. Plates were rinsed with culture media. Media with 20ng/ml VEGF alone or media with 20ng/ml VEGF and containing p28 peptide was then added to the plates. One dish was scratched as above and fixed immediately in order to mark exact wound area. Figure 3 A. After 24h, cultures were fixed and stained for F-actin and nuclei using Phalloidin and Hoechst stain. Scratched areas were examined using a florescence microscope and photographed. The number of cells that migrated into the scratched area was counted in the control (Fig. 3B) and peptide treated dishes (Fig. 3C).
The number of HUVECs that migrated into the scratch wound in the cells treated with p28 was about half that of those that migrated into the scratch wound in the control. Figure D. Therefore, the presence of p28 inhibited the motility of HUVECs undergoing angiogenesis
Example 4. Effects of p28 on HUVEC structural proteins.
The effects of p28 on HUVEC structural proteins was studied to gain a better understanding of the way p28 affects these cells. HUVEC cells plated on Matrigel® coated cover slips were incubated with 20ng/ml VEGF in the presence or absence of 25μM p28 peptide for 4h or 24h. After incubation, cells were rinsed in PBS, fixed in buffered formalin and permeablized in 0.2% triton in PBS. Cells were incubated with indicated antibodies for 90min, and if necessary incubated with a specific secondary antibody, and then mounted in DAPI containing mounting media. Analysis was performed with a confocal microscope (model LC510, Carl Zeiss). Proteins examined are as follows: CD-31 (protein present at intercellular junctions that is necessary for cell to cell attachment), Fak (focal adhesion kinase), Paxillin, Vinculin (critical adhesion assembly proteins), WASP (Wiskott Aldrich Syndrome protein, required for nucleation and elongation of F-actin fibers), β-catenin (required for cell survival, regulation of cell surface proteins).
In the CD31/PECAM1 detected cells, pronounced CD31/PECAM localization was found at cell/cell junctions in p28 treated cells as compared to control (Fig. 4A). In the paxillin detected cell, the paxillin was mainly localized on cell surface of the control cells, however it was more often found on F-actin fibers in the p28 treated cells (Fig. 4B). In the Fak detected cells, Fak was mainly on localized cell surface of the control cells, while it was more often found on F-actin fibers of the p28 treated cells (Fig. 4C). In the WASP detected cells, at 4h WASP localization was mostly nuclear in control cells, while WASP was localized on the nucleus and at the cell surface in p28 treated cells (Fig. 4 D). At 24h, WASP was mostly localized at the cell surface in control cells, while it was mostly localized in the nucleus in p28 treated cells (Fig. 4D). In the vinculin detected cells, vinculin was localized mainly on the cell surface in control cells, while vinculin was more often localized on F-actin fibers in p28 treated cells (Fig. 4E). In β-catenin detected cells, at 4h, β-catenin localization was mostly cytoplasmic with some on the cell surface in the control cells, while β-catenin was mostly localized on the cell membrane with some in the perinuclear space in the p28 treated cells. At 24h, β-catenin localization was mostly on the cell membrane and in the nucleus in the control cells, while β-catenin was localized on the cell membrane and perinuclear area in p28 treated cells. Therefore, the presence of p28 prevented the structural changes normally found in HUVECs undergoing angiogenesis.
Example 5. In vitro growth inhibition of human melanoma cells by p28.
The ability of p28 to inhibit the growth of human melanoma Mel-2 cells in vitro was determined. Mel-2 cells were plated in 24 well culture plates at 10,000-12,000 cells/well and allowed to attach to the plate overnight. Cells were then incubated at 370C in media alone (MEM-E with 10% FBS) or media containing p28 peptide. p28 was added at 5 μM, 50 μM, and 100 μM. The number of cells in each well was counted at Oh, 24h, 48h and 72h. The number of cells in each well was counted using a Coulter counter at the indicated time.
The results show that p28 inhibits growth of Mel-2 cells in a concentration dependent manner. p28 inhibited the Mel-2 cell growth by about 50% at 100 μM and 24h (Fig. 5). These results indicate that p28 inhibits the growth of cancer cells, specifically human melanoma-2 cells.
Example 6. In vivo anti-tumor activity of p28 peptides.
One million Mel-2 cells were injected subcutaneously into the dorsal flank of 3-4 week old athymic mice (n=13 per group). Animals received daily i.p. injections of PBS only, 8mg, or 16mg per kg body weight (b.w.) of p28 peptide in PBS. Animals were examined daily for the development of palpable tumors. Once the tumor developed, tumor size was measured using a caliper and tumor volume was determined. p28 inhibited the tumor incidence and growth in the mice. With the treatment of 16mg/kg b.w., about 50% of the animal were tumor-free 40 days after the mel-2 cells were injected, while only about 95% of the control animals had tumors 22 days after the mel-2 cells were injected (Fig. 6A). p28 also inhibited the growth of the tumors by about 30% at 20 days post treatment with 16 mg/kg b.w. p28 (Fig. 6B). These results indicate that p28 can prevent the slow and prevent the develop of tumors, as well as slow the growth of existing tumors in vivo, and thus would make an effective therapeutic for cancer prevention and treatment in humans.
Example 7: Efficacy of the synthetic peptides derived from azurin and plastocyanin.
T he efficacy of the synthetic peptides derived from azurin and plastocyanin have been analyzed. An 18-mer azurin peptide with the following sequence has been synthesized by standard techniques:
TFDVSKLKEGEQYMFFCT (SEQ ID NO: 48)
MCF-7 breast cancer cells were incubated in 16-well plates with 5 and 50 ug/ml of the 18-mer azurin peptide for 0, 24, 48 and 72 hours, after which the number of MCF-7 cells were counted in a coulter counter. The peptide was seen at 50 ug/ml to inhibit MCF-7 cell growth by 50% in 48 to 72 hours, as compared to cells without the synthetic peptide treatment. The extent of cell growth inhibition was about 25% at 5 ug/ml of the 18-mer synthetic peptide as compared to untreated control. This experiment shows that the synthetic peptide d does in fact inhibit the cancer cell progression promoted by the B-2 ephrin.
Example 8: In vitro measurement of effect of cupredoxins on the growth of Mel-2 and MCF-7 cells.
The growth of cells treated with cupredoxins was measured using a 16-well plate. Mel-2 or MCF-7 cells (5 x 105 cells per well) were allowed to adhere to multiwell (16-well, in this instance) plates for 24 hours. After adherence, the growth medium was siphoned off. PBS (phosphate-buffered saline) or various cupredoxins/cytochromes at concentrations of 0.1 to 10 μM in PBS were then added to the wells containing fresh growth media and the growth of the cancer cells was followed for 24, 48 and 72 hours. After the incubation period, trypan blue was added to the culture and the number of dead floating cells was counted. Both live and dead floating cells were counted to determine the IC50 at various cupredoxin doses. The IC50 is the concentration of protein that inhibits the cell culture growth by 50%. At 500,000 cells per well at 24 hours of growth, enough cells were present for reproducible counts. In the cupredoxin-minus control cell cultures, as the cells grew, they had less space to adhere to the bottom of the well, began to die and became floating cells. In the cupredoxin-treated cell cultures, both the Mel-2 and MCF-7 cell line growth was inhibited leading to very few floating cells.
Example 9: In Vitro Inhibition of P. falciparum Parasitemia by Cupredoxin and Cytochrome.
The cupredoxins bacterial wt azurin, M44KM64E azurin, rusticyanin and cyanobacterial plastocyanin, as well as the cytochromes Pseudomonas aeruginosa cytochrome C551, human cytochrome c and Phormidium laminosum cytochrome f were tested in a normal red blood cell (RBC) assay at 200 μg/ml concentrations at 30 hours post inoculation. In these experiments, the normal RBCs were washed twice in serum free media and resuspended to 10% hematocrit in complete RPMI. 200 μl of 10% Hct RBCs were added to each of 24 wells (final 2% Hct at ImI) in addition to 30 μl complete RPMI containing recombinant cupredoxin or cytochrome proteins at 666 μM for a final concentration of 200 μM. Schizont-stage parasites were prepared by centrifuging a late-stage culture through a Percoll cushion at 3200 rpm for 10 minutes. For infection, 4 x 106 parasites/well in 500 μl volume were added at t=0 hr.. The plate was incubated for 30 hours and scored by thin blood smear and Giemsa stain at that time.
The control showed 9.5% parasitemia (standard error 1.3%), wt azurin 6.9% (s.e. 1.4%), M44KM64E azurin 9.1% (s.e. 1.0%), rusticyanin 7.2% (s.e. 0.7%), cytochrome C551 7.5% (s.e. 1.5%), human cytochrome c 8.4% (s.e. 0.4%), plastocyanin 8.1% (s.e. 1.3%) and cytochrome f 6.6% (s.e. 1.0%), suggesting that cupredoxins such as wt azurin and rusticyanin and cytochromes such as cytochrome for cytochrome C551 demonstrated 20 to 30% inhibition of parasitemia.
When the cupredoxins were tested for their effects at various stages of the parasite life cycle (0 - 24 hours, ring formation; 24-36 hours, trophozoite; 36-48 hours, schizont), the control showed 0.1% average ring formation and 9.4% trophozoite formation while wt azurin showed no ring formation but 6.9% trophozoite formation; cytochrome f showed 0.2% ring formation but had significantly low (6.3%) trophozoite formation. Remarkably, rusticyanin exhibited very high (2.0%) ring formation and significantly reduced (5.2%) trophozoite formation. The others had no significant effect. The parasites in rusticyanin - treated samples looked sick and dying as compared to the rest of the samples, showing a significant inhibitory and toxic effect of rusticyanin on parasite development.
Example 10: Inhibition In Vitro of P. falciparum Intracellular Replication by Rusticyanin.
To determine if the bacterial redox proteins can inhibit intracellular replication of the malarial parasites, red blood cells were loaded to an intracellular recombinant protein concentration of 200 μg/ml using a hypotonic ghost preparation. Cells where then washed, resuspended and infected with schizont-stage parasites (P. falciparum) as described in Example 9. The red blood cell ghosts were incubated for 19 hours and 40 hours and giemsa smears were made.
Compared to the infections of normal red blood cells in Example 9, only rusticyanin decreased total parasitemia in loaded cell ghost cultures. At 19 hours, there was no significant difference in invasion and ring formation, with empty ghosts at 5.0 ± 0.4% and rusticyanin-loaded ghosts at 4.5 ± 1.0%. However, at 40 hours, rusticyanin-loaded ghosts had a lower level of infection. No major effects were seen at 19 hour with any of the bacterial proteins. However, at 40 hours, control untreated ghosts showed 4.6 ± 0.3% parasitemia while rusticyanin-treated ghosts had 2.7 ± 0.8% parasitemia, an almost 50% reduction. See, Table 5. Wt azurin, M44KM64E mutant azurin, plastocyanin, cytochrome C551, human cytochrome c and cynobacterial cytochrome f proteins showed parasitemia varying from 4.2 to 5.4% .
Table 5. Cupredoxin and cytochrome inhibition of P. falciparum infection of red blood cell ghosts.
Figure imgf000107_0001
Example 11: Structural Homology between Azurin and Fab Fragment of G17.12 Monoclonal Antibody Complexed with Pf MSP1-19.
Previous studies have shown that cupredoxins show structural similarity to the variable domains of the immunoglobulin superfamily members. (Gough & Chothia, Structure 12:917-925 (2004); Stevens et ai, J. MoI. Recognit. 18:150-157 (2005)) The DALI algorithm (Holm & Park, Bioinformatics 16:566-567 (2000)) was used to search the 3D databases for structural homologs of azurin (IJZG) from P. aeruginosa. Azurin exhibits structural similarity to the Fab fragment of G 17.12 monoclonal antibody in complexation with Pf MSP 1 - 19 fragment of the MSP 1 merozoite surface protein of P. falciparum. (Pizarro et al, J. MoI. Biol. 328:1091-1103 (2003).) (Table 6) Azurin also demonstrates structural similarity to CD4 (Table 5), the primary host cell surface receptor for HIV-I. (Maddon et al., Cell 47:333-348 (1986)). Azurin also exhibits a structural similarity to ICAM-I (Table 6), which is involved in cerebral malaria and implicated as a receptor on the endothelial cells in the micro vasculture of the brain and other tissues for sequestering P. f ale iparum-m' t ected erythrocytes. (Smith et al, Proc. Natl. Acad. Sci. USA 97:1766-1771 (2000); Franke-Fayard et al, Proc. Natl. Acad. Sci. USA 102: 11468-11473 (2005)). ICAM-I is also found in HIV- 1 particles during their passage through the host cells and is known to enhance HIV-I infectivity by enhancing cytosolic delivery of the viral materials. (Fortin et ah, J. Virol. 71 :3588-3596 (1997); Tardif & Tremblay, J. Virol. 77:12299-12309 (2003)) ICAM-I is known also to be subverted as receptors for major groups of rhino viruses and coxsackie viruses. (Bella & Rossmann, J. Struct. Biol. 128:69-74 (1999))
This example shows that cupredoxins including azurin demonstrate structural similarities in having two anti-parallel β sheets packed face to face and linked by a disulfide bridge to the variable domains of the immunoglobulin superfamily members as well as extracellular domains of the intercellular adhesion molecules (ICAM) and their ligands.
Table 6. Structural similarity of P. aeruginosa azurin with various pathogenesis- related proteins
Azurin (ljzg)
PDB Annotation Reference DALI z score(1)
IVCA Human Vascular Cell Adhesion Molecule-
17 3.5 Bl 1, VCAM-I
IZXQl The Crystal Structure of ICAM-2 19 3.3
HAMl Structure of The Two Amino-Terminal
20 3.0 Domains of, ICAM-I
IOBI Crystal Structure of a Fab complex with
21 2.9 Al Plasmodium falciparum MSP1-19
ITOP B The complex Structure of Binding Domains
22 2.5 of ICAM-3 and Alphabeta2
1 CDH CD4 (D1D2 Fragment)
18 3.4 Type 1 Crystal Form
2NCM Neural Cell Adhesion Molecule, NCAM 23 2.4
(1) - Structural alignment to azurin were made using DALI (16). Structure pairs with DALI z scores <2 are considered dissimilar.
Example 12. Cloning And Expression of the Laz and H.8-Azurin Fusion Genes.
The laz gene from Neisseria gonorrhoeae was cloned based on its known sequence (SEQ ID NO: 22). The P. aeruginosa azurin gene (SEQ ID NO: 1), termed paz, and the sequence of the H.8 epitope of laz from TV. gonorrhoeae (SEQ ID NO: 23), were used to clone in frame the H.8 epitope gene in the 5'-end of paz to produce H.S-paz or in the 3'-end of paz to generate paz-H.8. Table 7. Cancer cells, bacterial strains and genetic constructs
Figure imgf000109_0001
Figure imgf000110_0001
*Ap, ampicillin; Km, kanamycin; GST, Glutathione S-transferase.
Cloning and Expression of the paz and laz Genes. The cloning and hyperexpression of the azurin gene has been described. (Yamada, et al., Proc. Natl. Acad. Sci. USA 99:14098-14103 (2002); Punj, et al, Oncogene 23:2367-2378 (2004)) The Laz- encoding gene (laz) of Neisseria gonorrhoeae was amplified by PCR with genomic DNA of N. gonorrhoeae strain F62 as template DNA. The forward and reverse primers used were 5'-CCGGAATTCCGGCAGGGATGTTGTAAATATCCG-S' (SEQ ID NO: 34) and 5'-GGGGTACCGCCGTGGCAGGCATACAGCATTTCAATCGG-S' (SEQ ID NO: 35) where the additionally introduced restriction sites of EcoRI and Kpnl sites are underlined respectively. The amplified DNA fragment of 1.0 kb, digested with EcoRI and Kpnl, was inserted into the corresponding sites of pUC18 vector (Yanisch-Perron, et al., Gene 33:103- 119 (1985)) so that the laz gene was placed downstream of the lac promoter to yield an expression plasmid pUC18-/αz (Table 7). The plasmids expressing fusion H.8 of N. gonorrhoeae Laz and azurin of P. aeruginosa (Paz) were constructed by PCR with pUC19-/?αz and pUCl S-laz as templates. For H.8-Paz fusion, a 3.1 kb fragment was amplified with pUC18-/αz as a template and primers, 5'-(phosphorylated)GGCAGCAGGGGCTTCGGCAGCATCTGC-3' (SEQ ID NO: 36) and 5'-CTGCAGGTCGACTCTAGAGGATCCCG-S' (SEQ ID NO: 37) where a Sail site is underlined. A PCR amplified a 0.4 kb fragment was obtained from p\JC\9-paz as a template and primers, 5'-(phosphorylated)GCCGAGTGCTCGGTGGACATCCAGG-3' (SEQ ID NO: 38) and 5'-TACTCGAGTC ACTTC AGGGTC AGGGTG-3' (SEQ ID NO: 39) where a Xhol site is underlined. A Sail digested PCR fragment from pUC 1 S-laz and Xhol digested PCR fragment from pUC19-/?αz were cloned to yield an expression plasmid pUC18-H.8-pαz (Table 7).
E. coli JM 109 was used as a host strain for expression of azurin and its derivative genes. Recombinant E. coli strains were cultivated in 2 X YT medium containing 100 μg/ml ampicillin, 0.1 mM IPTG and 0.5 mM CuSO4 for 16 h at 37°C to produce the azurin proteins. When E. coli strains harboring these plasmids were grown in presence of IPTG, cells lysed and the proteins purified as described for azurin (Yamada, et al., Proc. Natl. Acad. Sci. USA 99:14098-14103 (2002); Punj, et al, Oncogene 23:2367-2378 (2004);Yamada, et al, Cell. Microbiol. 7:1418-1431 (2005)), the various azurin derivatives migrated on SDS-PAGE as single components, although the H.8 containing proteins (about 17 kDa) showed anomalous migrations, as noted before (Cannon, Clin. Microbiol. Rev. 2:S1-S4 (1989); Fisette, et al., J. Biol. Chem. 278 :46252-46260 (2003)).
Plasmid Construction for Fusion GST Proteins. Plasmids expressing fusion glutathione S-transferase (GST)-truncated wt-azurin (azu) derivatives were constructed by a polymerase chain reaction using proofreading DNA polymerase. For pGST- azu 36-128, an amplified PCR fragment was introduced into the BamHl and EcoRl sites of the commercial GST expression vector pGEX-5X (Amersham Biosciences, Piscataway, NJ). The fragment was amplified with pUC19-azu as a template and primers, 5'-CGGGATCC CCG GCA ACC TGC CGA AGA ACG TCA TGG GC-3'(SEQ ID NO: 40) and 5'- CGGAATTC GCA TCA CTT CAG GGT CAG GG-3' (SEQ ID NO: 41), where the additionally introduced BamHl and EcoRI sites are underlined respectively. Carboxyl- terminus truncation of azu gene was cumulatively performed by introducing a stop codon using QuickChange site-direct mutagenesis kit (Stratagene, La Jolla, CA).
For pGST-azu 36-89, a stop codon were introduced into Gly90. The plasmid carrying pGST-azu 36-128 was used as template DNA. Three sets of oligonucleotides for site-direct mutagenesis are shown as follows. For pGST-azu 36-89: 5'-CCA AGC TGA TCG GCT CGT GAG AGA AGG ACT CGG TGA CC-3' (SEQ ID NO: 42), and 5'-GGT CAC CGA GTC CTT CTC TCA CGA GCC GAT CAG CTT GG-3 (SEQ ID NO: 43).
For pGST-azu 88-113, carboxyl terminus truncation of azu gene was cumulatively performed by introducing stop codon using QuickChange site directed mutagenesis kit (Stratagene, La Jolla, CA). For pGST-azu 88-113, a stop codon was introduced into Phel 14. The plasmid carrying pGST-azu 88-128 was used as the template. For pGST-azu 88-128 an amplified PCR fragment was introduced into the BamHl and EcoRl sites of the commercial GST expression vector pGEX-5X (Amersham Biosciences). The fragment was amplified with pUC19-azu as the template and primers, 5'-CGGGGATCC CCG GCT CGG GCG AGA AGG AC-3' (SEQ ID NO: 44) and 5'-CGGGAATTC TCC ACT TCA GGG TCA GGG TG- 3' (SEQ ID NO: 45) where the additionally introduced BamHl and EcoRl sites are underlined respectively. One set of oligonucleotides for site directed mutagenesis are shown as follows for the preparation of pGST-azu 88-113: 5'-GTT CTT CTG CAC CTA GCC GGG CCA CTC CG- 3' (SEQ ID NO: 46) and 5'-CGG' AGT GGC CCG GCT AGG TGC AGA AGA AC-3' (SEQ ID NO: 47). pGST-azu 88-113 was used to transform E. coli XL-I Blue strains. Plasmid extraction was performed using a commercial kit (Qiagen, Venlo, The Netherlands) and PCR sequencing were performed to assess plasmid insertion and transfection.
E. coli BL21 (DE3) was used as a host strain for expression of the gst and its fusions derivatives. E. coli strain XLl -Blue transformed with pGST-azu plasmids was grown in LB media with ampicillin for three hours at 37°C upon which IPTG induction (0.4 mM) was performed an subsequent incubation for 2-4 h at 37°C to maximize the expression levels. Cells were isolated by centrifugation, resuspended in 25 mL of IX PBS buffer. Subsequent cell lysis involved two sequential treatments of the cell suspension via sonication (20 min on ice) and heat-cold shock in acetone-dry ice bath (using the appropriate protease inhibitors). Supernatants of the cell lysis mixture were isolated and passed through a freshly packed and PBS equilibrated 1 mL glutathione-sepharose 4B (Amersham Biosciences) column. After column washing and subsequent elution of GST-azu product using 10 mM glutathione in 20 mM Tris-HCl pH 8. GST-Azu 88-113 purity was tested via electrophoresis using a 10% SDS-PAGE Tris-Gly gel stained with Coomassie Brilliant Blue R reagent. Protein concentration was determined using the Bradford Method.
Example 13. Azurin Binds to the C-Terminal Fragments MSP1-19 and MSP1-42 of the P. falciparum Merozoite Surface Protein MSPl.
Given the structural similarity (Table 6) between azurin and the fab fragment of the monoclonal antibody G17.12 in complexation with Pf MSP1-19 (Pizarro et al, id), the ability of azurin to form a complex with Pf MSP 1-42 or Pf MSP 1-19 was determined. Two derivatives of azurin, Laz, an azurin-like protein from gonnococci and meningococci such as Neisseria meningitides with an additional 39 amino acid epitope called an H.8 epitope (Gotschlich & Seiff, FEMS Microbiol. Lett. 43:253-255 (1987); Kawula et al, MoI. Microbiol. 1 : 179-185 (1987)) and H.8-azurin, where the H.8 epitope of Laz has been fused in the N-terminal part of P. aeruginosa azurin in frame (as described in Example 12) were tested. - I l l -
In vitro protein-protein interactions were evaluated using a Biacore X spectrometer from Biacore AB International. All experiments were conducted at 25°C in HBS-EP running buffer (0.01 M HEPES, pH 7.4, 0.15 M NaCl, 3 mM EDTA, 0.005% v/v Surfactant P20) using Au-CM5 sensor chips (Biacore). Protein immobilizations on CM5 chips were conducted according to the amine coupling procedure. Proteins were immobilized after NHS/EDC preactivation of the CM5 surface: 50 μl injections of azurin (510 μM). Subsequent treatment of CM5 surface with ethanolamine (IM, pH 8.8) removed uncrosslinked proteins. Binding studies were performed by injecting protein eluents (50 μl) over the protein-CM5 surface at flow rates of 30 μl/min with a 120 sec time delay at the end of the injections. Protein eluents included GST-azurin fusion proteins (GST, GST- Azu 36- 128, GST-Azu 36-89, and GST-Azu 88-113, as described in Example 12). Sensor chip surfaces were regenerated between protein injections using 100 mM NaOH (10 μl injection pulse). All binding studies were run in parallel against a negative flow channel with bare Au- CM5 sensor surface to correct for nonspecific binding to the chips. To generate binding constant data, titration experiments were designed via injection of increasing concentrations of protein eluents (0.05-2000 nM). The SPR data were fit to a Langmuir (1.1) equilibrium binding model [Req = Rmax/(1 + Kd/C] as specified in the Biacore software from which binding constants (Kd) were extrapolated.
Specific interactions of the Pf MSPl-19 and Pf MSP 1-42 proteins with azurin, H.8- azurin and Laz were determined by surface plasmon resonance (SPR) analysis and the data are presented in Figure 7. SPR sensorgrams for binding of immobilized Pf MSPl -19 and Pf MSP 1-42 with azurin and its derivatives indicated selective recognition among these proteins. While nanomolar concentrations of azurin allowed significant binding with the immobilized MSP1-19 (Fig. 7A) or MSP1-42 (Fig. 7B), both H.8-azurin and Laz demonstrated a higher affinity of binding with the merozoite surface protein MSPl cleavage products, with characteristic Kd values of 32.2 nM between azurin and MSP1-19 and 54.3 nM between azurin and MSP1-42. The Kd values between H.8-azurin and MSP1-19 and MSP1-42 were 11.8 nM and 14.3 nM while such values between Laz and MSPl -19 and MSP1-42 ranged from 26.2 nM and 45.6 nM respectively. To examine if the H.8 epitope might facilitate binding of the H.8-azurin or Laz to the
PfMSPl -19 or PfMSP 1-42 moieties, the ability of glutathione S-transferase (GST) and a fusion derivative H.8-GST where the H.8 epitope was fused in the N-terminal of GST (see Example 12), to bind MSPl-19 or MSP 1-42 was tested. Neither the GST nor the H.8-GST bound PfMSPl-19 (Fig. 7A) or MSP1-42 (Fig. 7B), although H.8-GST showed a weak binding with MSP 1-42.
Glutathione S transferase (GST) and some of the fusion proteins where parts of azurin were fused to GST (Yamada et al. , Cell. Microbiol. 7: 1418-1431 (2005), and Example 4) were tested for their ability to bind to MSP.1-19. GST alone, or GST-Azu 88-113, where the azurin amino acid sequence 88 to 113 out of 128 amino acids of azurin was fused to GST in frame, did not show any binding (Fig. 7C) while GST-Azu 36-89 with amino acid sequence 36 to 89 and GST-Azu 36-128 with amino acid sequence 36 to 128 showed significant binding with MSP1-19 with Kd values of 20.9 nM and 24.5 nM respectively.
Example 14. Inhibition of Plasmodium falciparum Parasitemia by Azurin, H.8- Azurin and Laz.
The extent of parasitemia was determined using schizont stage parasites and normal red blood cells (RBC). Normal red blood cells (RBCs) were washed twice in serum-free medium and resuspended to 10% hematocrit in complete RPMI. 200 μl of 10% hematocrit RBCs were added to each of 24 wells in addition to 300 μl complete RPMI without or with azurin, H.8-azurin or Laz at various concentrations. Schizont stage P. falciparum parasites were prepared by centrifuging a late-stage culture through a Percoll cushion at 3200 rpm for 10 min. For infection, 4x106 parasites per well in 500 μl volume were added at time zero. The plate was incubated overnight (about 16 h) and then scored by thin blood smear and Giemsa stain at that time.
Azurin, H.8-azurin or Laz all demonstrated significant inhibition of parasitemia in a dose-dependent manner (Fig. 8), although at relatively high concentrations (about 50 μM). Such high concentrations presumably reflect the multiple ways the malarial parasites invade the erythrocytes (Cowman et al., FEBS Lett. 476:84-88 (2000); Baum et al., J. Biol. Chem. 281 :5197-5208 (2006)) and a high concentration of azurin or Laz is necessary to interfere in the entry process. As indicated by their enhanced binding affinities to MSP1-19, both H.8- azurin and Neisserial Laz protein showed a higher level of inhibition of P. falciparum parasitemia as compared to azurin (Fig. 8).
When azurin was labeled with the red fluorescent dye Alexafluor 568 and used during the invasion assay, very little red fluorescence was detectable inside the RBC, suggesting that azurin seems not to enter the RBC as part of bound MSPl -19, or more likely, that the RBCs that showed the presence of the schizonts were the ones where azurin failed to bind with the MSP 1-19. These data fully agree with our previous observation (Yamada et al, Cell. Microbiol. 7: 1418-1431 (2005)) that azurin does not enter normal cells such as macrophages, mast cells, etc, and the effect of azurin, H.8-azurin or Laz is at the entry level rather than the intracellular replication of the parasite. Taken together, the data in Fig. 8 demonstrate the potential antimalarial action of azurin, H.8-azurin and Laz through interference in the invasion of the RBC by the parasites.
Example 15. Azurin binds ICAMs
An interesting structural similarity between azurin and ICAMs (Table 6) that are known to be involved as receptors for P. falciparum-infected erythrocytes (Wassmer et al. , PIoS Med. 2:885-890 (2005); Dormeyer et al, Antimicrob. Agents Chemotherap. 50:724-730 (2006)) prompted test analysis of protein-protein interactions as measured by SPR between azurin and ICAMs such as ICAM-I , ICAM-2, ICAM-3 and NCAM. With immobilized azurin on the CM5 chip, ICAM-3 (Fig. 9, Kd - 19.5 + 5.4 nM) and NCAM (Fig. 9, inset), but interestingly not ICAM-I and ICAM-2, showed strong binding. While not limiting the manner in which the invention operates, part of effect of azurin on inhibition of P. falciparum parasitemia might also be mediated through its interaction with ICAM-3 or NCAM.
Example 16. In Vivo Inhibition Of HIV Infection Of Lymphocytes By Azurin Mutant And Cytochrome C551.
The M44KM64E mutant of azurin was mixed with cytochrome C551 on a 1 :1 basis (1 μM azurin : 1 μM cytochrome C551). HIV-infected human blood lymphocytes were incubated with the mixed azurin/cytochrome C551 proteins at concentrations of 0, 500 to 1000 μg/ml protein for 7 days. The HIV p24 levels were then measured in the infected lymphocytes. p24 levels are known to be colinear with HIV virus levels in infected blood. Measuring the change in p24 concentrations in blood will indicate the change of HIV virus titer in the blood. Controls with non-infected human blood lymphocytes were also run in a parallel manner. After the 7 day incubation, the HIV p24 levels in the infected lymphocytes were reduced by 25% to 90% as compared to the control infected lymphocytes with 0 μg/ml azurin and cytochrome C551- In the non-infected control cells, after 7 days of incubation with the protein mixture, neither cell death nor cytotoxicity was found.
Example 17. Effect of Azurin, H.8-Azurin and Laz on HIV-I Entry and Viral Growth. The effect of various concentrations of azurin, H.8-azurin and Laz on the growth of three subtypes of HIV-I in peripheral blood mononuclear cells (PBMCs), BaI, RW/92/008/RE1 clade A and IN/2157 D15 clade C.
Example 18. Effect of Azurin, H.8-Azurin and Laz on HIV-I Entry and Viral Growth. The effect of various concentrations of azurin, H.8 -azurin and Laz on the growth of three subtypes of HIV-I in peripheral blood mononuclear cells (PBMCs), BaI, RW/92/008/RE1 clade A and IN/2157 D15 clade C. Plasmid construction and expression of Azurin, H.8-Azurin and Laz were performed as in Example 12.
HIV-I Suppression Assay. Azurin, H.8-azurin and Laz were filter sterilized through a 0.45 μM filter. Peripheral blood mononuclear cells (PBMC) were treated with polybrene (5 μg/ml) for 1 h and seeded at 250,000 cells/well in a microtiter plate. The plate was spun at 800 rpm for 5 min to collect the cells. The supernatant was taken off and media with protein (at concentrations of 0.3, 0.6, 1.2, 6.0 and 30 μM) was added (100 μl). The cells were then incubated for 1 h. AZT (25 μM) was used as a control. The proteins were left on cells and 100 μl of virus (BaI, 2167, or RW/92/008/RE1) was added and incubated for 2 h. The plate was spun again at 800 rpm for 5 minutes and protein and virus was removed. Protein and media were added back for a total volume of 100 μl and incubated for 5 days. At the end of the 5 day period, the culture supernatant was tested for HIV/p24 by ELISA.
The results in Figure 10 show that azurin at a concentration of 6.0 μM shows about 90% suppression of the growth of HIV-I BaI, the most predominant clade B circulating in the US and Western Europe, a clade B African isolate RW/92/008/RE1 and a clade C Indian isolate IN/2167 D15. However, H.8-azurin (azurin with the H.8 epitope in the N-terminal) had high inhibitory activity against all the three subtypes at concentrations as low as 0.3 μM, particularly for the African and the Indian subtypes (Fig.10). The Neisserial protein Laz, which also harbors the H.8 epitope in the N-terminal part of the Neisserial azurin homolog (Gotschlich & Seiff FEMS Microbiol. Lett. 43:253-255 (1987); Kawula et al, MoI. Microbiol. 1 :179-185 (1987)), had similar inhibitory activity for the three subtypes, particularly for the African and the Indian subtypes (Fig. 10), demonstrating a role of the H.8 epitope in promoting enhanced anti-HIV-1 activity by azurin. No effect on host cell (PBMC) death by MTT assay (Yamada et al., Proc. Natl. Acad. Sci. USA 99:14098-14103 (2002); Punj et al., Oncogene 23:2367-2378 (2004)) was discernible for all concentrations of these three proteins, suggesting that inhibition of HIV-I growth was not due to death of the host cells.
Example 19. Azurin Binding with gpl20 and CD4 as Studied by Surface Plasmon Resonance. Surface Plasmon Resonance experiments were conducted to determine the extent of azurin binding not only to CD4 but also to HIV-I surface proteins such as gpl20 or gp41 known to be involved in HIV-I entry and other proteins such as Nef or Gag that are involved in intracellular virus multiplication.
Surface Plasmon Resonance (SPR) Studies. In vitro protein-protein interactions were evaluated using a Biacore X spectrometer from Biacore AB International (Uppsala, Sweden). All experiments were conducted at 25°C in HBS-EP running buffer (0.01 M HEPES, pH 7.4, 0.15 M NaCl, 3 mM EDTA, 0.005% v/v Surfactant P20)) using Au-CM5 sensor chips purchased from Biacore. Protein stock solutions were prepared in PBS after desalting on G-75 column and lyophilizaiton in order to preconcentrate and exchange the buffer.
Protein immobilizations on CM5 chips were conducted according to the amine coupling procedure. Due to differences in protein crosslinking efficiencies, proteins were immobilized under various conditions after NHS/EDC preactivation of the CM5 surface: 50 μl injections of azurin (510 μM), or 35 μl injections of CD4 (25 μM, 2x), or HIV-I gpl20 (10 μM). Subsequent treatment of CM5 surface with ethanolamine (IM, pH 8.8) removed uncrosslinked proteins prior to binding studies. Binding studies were performed by injecting protein eluents (50 μl) over the protein-CM5 surface at flow rates of 30 μl/min with a 120 sec time delay at the end of the injections. Protein eluents included CD4 (Protein Sciences Corp., Meriden, CT), HIV-I gpl20 (Immunodiagnostics Inc., Woburn, MA), HIV-I gp41 (Bioclone Inc., San Diego, CA), HIV-I gag and HIV- 1 -nef (Chemicon International, Temecula, CA) and GST-azurin fusion proteins (GST, GST- Azu 36-128, GST- Azu 36-89, and GST- Azu 88- 113, expressed in inventor's laboratory). Sensor chip surfaces were regenerated between protein injections using 100 raM NaOH (10 μl injection pulse). All binding studies were run against a negative flow channel containing bare Au-CM5 to correct for nonspecific binding effects. For the binding experiments wherein CD4 and HIV-I gpl20 served as the eluents (not immobilized), 1 mg/mL of carboxymethyldextran (CarboMer Inc., San Diego CA) was added to the running buffer in order to reduce nonspecific protein binding to the bare Au- CM5 flow channel surface.
To generate binding constant data, titration experiments were designed via injection of increasing concentrations of protein eluents (0.05-2000 nM) and the data collected. The SPR data could be fit to a Langmuir equilibrium binding model [Req = Rmax/(1 + Kd/C] form which binding constants (Kd) were determined. Similar to the binding constant studies described above, competition studies with CD4-CM5 were performed using similar protocols but with injections of HIV-I gpl20 + the competitor proteins (azurin, GST-Azu 36-128 and GST-Azu 88-113).
With CD4 immobilized in the sensor chip, both azurin and gρl20 showed significant binding to CD4 (Fig. 1 IA). Azurin demonstrated a higher affinity for binding CD4 (Kd = 36.9 nM) than the HIV-I ligand gpl20 (Kd = 48.1 nM). While a GST-azurin fusion such as GST-Azu 88-113 showed no binding (Fig. 1 IA), another GST-azurin fusion protein, GST- Azu 36-128 showed even stronger binding than azurin itself with a Kd value of 0.34 nM, suggesting that parts of azurin might retain a stronger binding affinity than the full length protein. When azurin was immobilized on the sensor chip, gpl20 showed somewhat stronger binding to azurin than CD4 (Fig. HB), clearly demonstrating that azurin binds both to gpl20 and CD4 with a high affinity. Interestingly, gp41, also involved in HIV-I entry into the host cell, did not show any binding to azurin (Fig. 1 IB). Similar lack of binding was demonstrated for Gag and Nef.
Example 20. Azurin Binding with ICAMs and CD5 as Studied by Surface Plasmon Resonance.
There is a structural similarity between azurin and ICAMs (Table 6) that are known to be involved as receptors HIV-I infections. (Liao et al.,. AIDS Res. Hum. Retroviruses 16:355-366 (2000); Hioe et al, J. Virol. 75:1077-1082 (2001)) ICAM-3 has been implicated in stimulating HIV-I transcription and viral production, thereby contributing additionally to intracellular viral growth. (Barat et al, J. Virol. 78, 6692-6697 (2004)) Protein-protein interactions as measured by SPR between azurin and ICAMs such as ICAM- 1, ICAM-2, ICAM-3 and NCAM were therefore studied. With immobilized azurin on the CM5 chip, ICAM-3 (Fig. 2C, K41 = 19.5 ± 5.4 nM) and NCAM (Fig. 11C, inset), but not ICAM-I and ICAM-2, showed strong binding. While not limiting the operation of the invention to any one mechanism, part of azurin suppression of HIV-I growth might also be mediated through its interaction with ICAM-3 or NCAM.
Example 21. Azurin Competition with gpl20 for CD4 as Studied by Surface Plasmon Resonance. Due to the higher affinity of binding of azurin to CD4, as compared to gpl20 (Fig.
1 IA), a competition experiment was performed to see if azurin can interfere in gpl20 binding with its cognate receptor CD4. As the concentration of the competitor protein (azurin, GST- Azu 36-128 or GST-Azu 88-113) was increased in presence of a fixed concentration of gpl20 adsorbed to the immobilized CD4 chip, both azurin and GST-Azu 36-128 demonstrated significant decrease in the total protein binding of gpl20 from the CD4-CM5 chip (Fig. 1 ID). Such apparent displacement of gpl20 from the chip was not observed in case of GST-Azu 88-113 (Fig. 1 ID). GST-Azu 88-113 is known not to bind CD4 (Fig. 1 IA). While not limiting the operation of the invention to any one mechanism, this indicates that azurin or GST-Azu 36-128 fusion protein may successfully inhibit the complex formation between gpl20 and CD4.
Example 22. Azurin and ICAM-3 Binding with DC-SIGN as Studied by Surface Plasmon Resonance.
The strong binding of azurin with gpl20, CD4 and ICAM-3 (Fig. 11) mimics the binding of another very important HIV-I binding protein present on the surface of dendritic cells (DC) known as DC-SIGN (DC-specific intercellular adhesion molecule 3-grabbing nonintegrin) and a related protein called DC-SIGN/R. DC-SIGN is expressed abundantly on DC while DC-SIGN/R is expressed primarily on sinusoidal and endothelial cells. DC-SIGN plays a major role in HIV-I immunopathogenesis by allowing DC, which are professional antigen presenting cells, to capture and present pathogens including HIV-I to resting T cells through their interactions with ICAM-3 on the T cell surface. (Geijtenbeek et al, Cell 100, 575-585 (2000); Soilleux, Clin. Sci. 104, 437-446 (2003); Geijtenbeek et al., Placenta 22, S19-S23 (2001)). DC-SIGN has also been shown to bind avidly to HIV-I envelope protein gpl20, thereby capturing HIV-I and transporting it to CD4+ T cells, where HIV-I can replicate freely. (Snyder et al., J. Virol. 79:4589-4598 (2005))
In SPR experiments with immobilized DC-SIGN on the sensor chip, both azurin (Kd=0.83±0.05 nM) and ICAM-3 (Kd=0.93± 0.39 nM) bound strongly to DC-SIGN (Fig. 12A). While the GST-fusion derivative GST-Azu 36-89 showed very little binding (Fig. 12A), another GST-fusion derivative GST-Azu 88-113 exhibited relatively strong binding (Kd=5.98+1.13 nM), demonstrating the involvement of the C-terminal part of azurin in DC- SIGN binding (Fig. 12B). GST-Azu 88-113, however, does not bind with CD4 (Fig. 1 IA), suggesting that different parts of azurin have different binding specificities.
While not limiting the operation of the invention to any one mechanism, such binding with DC-SIGN demonstrates azurin's potential ability to interfere in the binding of HIV-I with DCs. Thus DC-SIGN, a critical molecule on DC surface responsible for transmitting HIV-I from the mucosal cells to the lymphoid T cells, may well find a strong competitor in azurin or Laz that can also avidly bind gpl20, CD4 and ICAM-3.
Example 23. Azurin/Laz Acts in the Entry Stage of HIV-I Infection.
To determine if azurin acts at the entry or post entry step of HIV-I infection, the effect of Laz on the Indian isolate IN/2167 of HIV-I was investigated. In one experiment, activated PBMC (25,000 cells/well) were incubated with 6.0 μM Laz and HIV-I for 2 h. The mixture was centrifuged to remove Laz and HIV-I, fresh medium without Laz was added back, and the culture was grown for 5 days. HIV-I growth was monitored by measurement of p24 in the culture supernatant. Under this condition, Laz (6.0 μM) suppressed the HIV-I growth by 43%. With higher concentration of Laz (30 μM), the extent of suppression was 76%. In a parallel experiment, when the Laz (6 or 30 μM) was added to the PBMC after the HIV-I infection and its removal, very little suppression of viral growth was observed. As a positive control, when Laz (6.0 μM) was present both during infection and after removal of the virus with fresh medium during 5 days of the culture, the extent of inhibition was about 93%. While not limiting the operation of the invention to any one mechanism, such data clearly indicate that azurin or Laz exerts its effect primarily at the entry stage of infection. Example 24. Treatment of more than one disease such as patients infected with Malaria and HIV.
Twenty four patients, aged 22-50, who exhibit a history of preexisting antibodies to blood-stage P. falciparum parasites (as determined by immunofluorescent assay) and infected with AIDS presents with low to non-detectable HIV viral loads (RNA PCR) in the plasma as measured by PCR techniques, and increased CD4+ counts. Next, CD4+RO+ cells are enriched by magnetic separation and FACS sorting, and assayed to determine infectivity with respect to naive and uninfected cell co-culture experiments. This analysis of CD4+RO+ memory cells shows the presence of infective HIV. The patients are injected with a pharmaceutical preparation of purified P. aeruginosa azurin. Two such patients serve as treated controls.
The sterile pharmaceutical preparation is in the form of 0.5 ml single-dose ampoules of sterile P. aeruginosa azurin in a pharmaceutical preparation designed for intravenous administration, as will be well known to those in the art.. The pharmaceutical preparation is stored at 4° C. and protected from light before administration. In one clinical trial, P. aeruginosa azurin is prepared at five different concentrations: 10 μg, 30 μg, 100 μg, 300 μg and 800 μg azurin/cytochrome c55i (1 :1 on molecule basis) per 0.5 ml dose.
The pharmaceutical preparation is given intravenously to twenty two patients for each 10 doses. Patients receive primary treatment at day 0 and subsequent doses identical doses for a period of 3 months until CD4+ cells, including memory cells, are at low levels
Volunteers are observed for immediate toxic effects for twenty minutes after injection. Two patients receive placebo injections. During administration of azurin and for a period of approximately 1 -2 months thereafter, or until CD4+ cells recover, the patients are maintained with antibiotics and antifungal therapy. Stem cell or precursor cell replacement is provided through a bone marrow transplant and cytokine therapy, both of which are performed according to conventional techniques. Twenty-four and forty-eight hours later, they are examined for evidence of fever, local tenderness, erythema, warmth, induration and lymphadenopathy, and are asked about complaints of headache, fever, chills, malaise, local pain, nausea and joint pain. Before each dose, blood and urine samples are taken for full laboratory examination. Complete blood count and serum chemistry profiles are rechecked two days after each dose. The presence of the malaria parasite are determined by light microscopic examination (ME) of the stained blood smears, or the ICT Malaria P.f./P.v. test kits ( Binax, Inc., Portland, ME) . The patients are also followed at frequent intervals and monitored for CD34 cell level, reestablishment of CD4+ cells and quantitation of CD4+RO+ cells. Additionally, the patients' plasma is assayed for viral load by cell co-culture experiments. On reducing virus load in active and memory CD4+ T cells to low or non- detectable concentrations, the patients are weaned from azurin. After 3 months, the patients are weaned from antibiotic and antifungal therapy. Following this, the patients are followed at 6 month intervals and assayed for viral content. The results demonstrate the effectiveness of azurin therapy for patients with HIV infection. The results demonstrate the effectiveness of the therapy.
Example 25 - Entry of pl8 and p28 Into Human Cell Lines
Cell Culture and Cell Lines: Human cancer and non-cancer (immortalized and non- immortalized) cell lines were obtained from ATCC [lung cancer (A549 and NCI-H23 adenocarcinoma), normal lung (CCD- 13 Lu), prostate cancers (DU 145 and LN-CAP), normal prostate (CRLl 1611), breast cancer (MCF-7), normal breast (MCF-IOA), colon cancer
(HCTl 16), normal colon (CCD33Co), fibrosarcoma (HTl 080), and ovarian cancer (SK-OV3 adenocarcinoma)]. Normal fibroblasts isolated from skin were established. Normal ovarian cells (HOSE6-3) were donated by Dr. S. W. Tsao (University of Hong Kong). Melanoma lines (UISO-Mel-2, 23, 29) were established and characterized. All cells except UISO-Mel-2 were cultured in MEM-E (Invitrogen, Carlsbad, CA) supplemented with 10% heat- inactivated fetal bovine serum (Atlanta Biological Inc., Lawrenceville, GA), 100 units/ml penicillin and lOOμg/ml streptomycin at 37C in 5% CO2 or air.
Proliferation assays/Cell growth: Melanoma cells were seeded (four replicates) in flat bottom 24 well plates (Becton Dickinson, Franklin Lakes, NJ) at a density of 12x103 cells/well. After 24 hrs media was changed and fresh p 18, p28 , azurin or a similar volume of media without peptide (eight replicates) added daily for 72 hr. Cells were then counted in a Beckman Coulter (Z 1 coulter particle counter). Values represent the mean ± SD of 4 replicates.
MITT Assay: Melanoma cells were seeded at a density of 2000 cells/well in flat- bottomed 96 well plates (Becton Dickinson, Franklin Lakes, NJ) and allowed to attach for 24 hrs. Freshly prepared peptide (10 μl) or culture medium was then added to each well. After 24 hrs, medium was changed and pi 8, p28 or azurin added daily. After 72 hr incubation, lOμl of MTT reagent (Trevigen, Gaithersburg, MD) was added to each well, the samples incubated for 3hr, RT/sig 100 μl of detergent added to each well, and the samples incubated for an additional 3hr at 37°C. Absorbance was measured with a SpectraMax 340 plate reader (Molecular Devices Corporation, Sunnyvale, CA) and percent change in the absorbance at 570 nm in treated cells relative to untreated controls determined. Values represent the mean ±- SD. Significance between control and treated groups was determined by Student's t-test.
Peptide synthesis: All azurin derived peptides including pi 8, Leu50-Gly67 LSTAADMQGVVTDGMASG (SEQ ID NO. 30), p28 Leu50-Asp77 LSTAADMQGVVTDGMASGLDKDYLKPDD (SEQ ID NO. 29), p 18b VaI60- Asp77 VTDGMASGLDKDYLKPDD (SEQ ID NO. 91 ), MAP, Mastoparan-7, and poly arginine (Arg8) were synthesized by C S Bio, Inc. (MeIo Park, CA). Peptides were received as lyophilized powder aliquoted and stored at -2O0C in air-tight desiccators. All peptides were subsequently analyzed by mass spectrometry and reverse phase HPLC as >95% purity and mass balance. Predictive modeling for azurin peptides: GENETYX software (ver. 6.1) was used to generate Robson structure models for azurin derived peptides. Gamier, J., Osguthorpe, D. J., and Robson, B., J MoI Biol, 120: 97-120 (1978). The MAPAS Software was used to predict a given protein structure for strong membrane contacts and define regions of the protein surface that most likely form such contacts. Sharikov, Y. et al, Nat Methods, 5: 119 (2008). If a protein, i.e., azurin, has a membranephilic residue score (MRS) > 3, membranephilic area score (MAS) > 60%, and coefficient of membranephilic asymmetry (Kmpha) > 2.5, there is a high probability that the protein has a true membrane-contacting region..
Peptide/Protein labeling: Peptides were dissolved in ImI PBS mixed with Alexafluor 568 dye (Molecular Probes, Eugene, OR) at a 1 :2 protein:dye ratio, lOOμl sodium bicarbonate added, and the mixture incubated overnight at 4°C with continuous stirring. Labeled peptide was separated from free dye by dialyzing against cold-PBS using Slide- A- Lyzerg Dialysis Cassettes 1000 MWCO for pl2 and 2000 MWCO for others (Pierce Biotechnology, Rockford, IL).
Cell penetrationfconfocal analysis: Cells were seeded on glass coverslips and allowed to attach overnight at 37°C under 5% CO2. Cells were rinsed with fresh media and incubated at 370C for 2 hrs in pre-warmed media containing Alexafluor 568 labeled azurin peptides (20 μM) or Arg8 (5 μM), or media alone. Following incubation, coverslips were rinsed 3x with PBS, cells fixed in 2.5% formalin for 5 min, and washed 2x in PBS, once in d.i. H2O, and coverslips mounted in media containing 1.5μg/ml DAPI for nuclear counter staining (VECTASHIELD® Vector Laboratories, Burlingame CA). Cellular uptake and distribution were photographed under an inverted confocal laser scanning microscope ('Model LC510, Carl Zeiss Inc., Gottingen, Germany).
Peptide co-localization with lysosomes or mitochondria was determined by incubating cells growing on a glass coverslip for 2 hrs at 37° with Alexafluor 568 labeled azurin or peptides. Mitrotracker (MitroTracker® Green FM Invitrogen Corporation, Carlsbad, CA) or lysotracker (LysoTracker® Green DND-26 Invitrogen Corporation, Carlsbad, CA) was added (final concentraion 1 μM) for the last 30 mins of incubation. Cells were rinsed 3x with PBS, fixed in 2.5 % formalin for 5 mins, washed 2x with PBS and incubated in 0.1% Triton-XlOO in PBS for 15 min. Cells were then incubated with 1 μg/ml rabbit anti-human golgin 97 or anti-human caveolin I (Abeam, Cambridge, MA) in PBS with 1% BSA. After 1 hr incubation at 4°C, coverslips were washed once with PBS, incubated 10 min in PBS containing Alexafluor 468 conjugated goat anti-rabbit antibody, washed 2x in PBS and once in d.i.H20. Coverslips were then mounted in media containing 1.5 μg/mlDAPI for nuclear counter staining. Colocalization (yellow) of Alexafluor 568 (red) and Alexafluor 468 (green) was analyzed and photographed.
UISO-Mel-2 cells on coverslips were preincubated in MEM-E containing 100 μg/ml heparin sulfate (Sigma-Aldrich, St. Louis, MO) for 30 min and pi 8, p28 or Arg8 added to bring the final concentration to 20 μM. After lhr, coverslips were washed, fixed, and analyzed as described above.
Cell penetration by FFACS: Cells (1.0 x 106/500 μl PBS) were incubated for 2 hrs at 37°C with Alexafluor 568 labeled pi 8 or p28 (20μM), Argg (5μM), or media alone, washed 3x in PBS, fixed in 2.5% formalin for 5 min, washed twice in PBS, resuspended in 200 μl PBS, and passed through a screen to obtain a single cell suspension. Samples were analyzed with a MoFIo Cell Sorter (Dako, Glostrup, Denmark) λeX 568 nm and λem 603 nm and the fold increase of the mean fluorescence intensity over background levels calculated. Results represent mean fluorescence of three separate experiments. Entry inhibitors: UISO-Mel-2 cells (3xlO5 per 300 μl), maintained in phenol red-, serum-free MEM-E at 370C, were pretreated with inhibitors, including: Chloropromazine (inhibitor of clathrin-mediatied endocytosis, 10 μg/ml, 60 min); Amiloride (macropinocytosis inhibitor, 50 μM, 30 min); Nystatin (50 μg/ml, 30 min); Methyl-β-cyclodextrin (MβCD, 5mM, 60 min); Filipin (inhibitor of caveolae-mediated endocytosis, 3 μg/ml, 60 min); Taxol (microtubule stabilizer, 20 μM, 30 min); Staurosporine (cell cycle inhibitor, 250 nM, 10 min); Sodium azide (metabolic inhibitor, 1 mM, 60 min); Oauabain (ATPase-dependent Na+/K+ pump inhibitor, 50 mM, 60 min); Brefeldin A (BFA; Golgi apparatus disruptor, 100 μM, 60 min); Wortmannin (early endosome inhibitor, 100 nM, 30 min); Monensin (inhibits at late endosome/lysosome, 10 μM, 60 min); Nocodazole (inhibits caveosome formation, 10 μM, 60 min); Cytochalasin D (actin filament and microtubule disruptor, 5 μM, 30 min); Benzyl 2-acetamido-2-deoxy-α-D-galactopyranoside (BnGalNac; O-linked glycosylation inhibitor, 3mM, 48 hrs); Tunicamycin (N-linked glycosylation inhibitor, 20μg/ml, 48hrs); and Neuraminidase (cleave sialic acid residues from proteins, IU/ml, 30min). Final concentrations were derived from the dose response curves of individual inhibitors. Alexafluor 568 labeled pi 8 or p28 (20 μM) were then added, incubated for 1 hr, and the cells washed, fixed and prepared for flow cytometric analysis as described above. Cell Membrane Toxicity Assays/LDH Leakage Assay: An LDH leakage assay was performed according to the manufacturer's instructions (CytoTox-One, Promega, WI) with lOOμl of UISO-Mel-2 cells (5x 103). Cells without peptides/proteins were used as a negative control. Experiments were carried out in triplicate (data represent mean ± SEM).
Hemolysis assay: Human whole blood samples (2-3ml) were centrifuged for 10 min at 1000xg, and the pellets washed once with PBS and once with HKR buffer pH7.4 ( 18). Cell pellets were then resuspended in HKR buffer to 4% erythrocytes, 50μl transferred to a 1.5ml tube with 950μl of peptides, azurin (5, 50 and lOOμM) or 0.1% Triton X-100 in HRK buffer to completely disrupt the RBC membrane. MAP and Mastoparan7 (Bachem California, Inc., Torrance, CA) were used as positive controls. After 30 min incubation at 370C with rotation, tubes were centrifuged for 2 min at 1000xg, 300μl of supernatants transferred to a 96-well plate and absorbance recorded at 540 nm.
Kinetics of Entry: UISO-Mel-2 cells (5x 105cells) in 1.5 ml tubes were suspended in MEME media without phenol red. Reactions were started by adding either Alexa fluor 568- conjugated p 18 at 0, 10, 20, 50, 100, 150 and 200μM for 5, 10, 15 and 20 sec ., or Alexafluor 568-conjugated p28 at 1, 10, 25, 50, 100, 150 and 200μM for 30 , 60, 90 and 120 sec on ice. After incubation, 1 ml of cold-PBS was added to the 250μl reaction in mixture. Cells were centrifuged twice at 600xg for 2 min at 4°C. At least 10,000 fixed cells were analyzed by flow cytometry in each reaction and their background and relative fluorescence calculated.
I125 Labeling of Azurin and Competition Assays: Peptide binding and entry was determined using a whole cell assay with UISO-Mel-2 cells in HEPES solution (50,000 cells/ml ), were incubated for 30 min at 370C with increasing concentrations (0-175nM) of radiolabeled a zurin in the presence/absence of 1000 fold excess of unlabeled pi 8, p28, or azurin, then washed 3 times with ice cold PBS, and radioactively remaining in the cell pellet counted using a gamma counter. Radioactivity in cells incubated with I125 azurin alone was considered total binding; radioactivity in the presence of unlabeled azurin, pi 8, or p28 was considered nonspecific binding. Specific binding was determined by subtracting nonspecific binding from total binding and Scatchard plots generated.
Example 26 -Domain of p28 responsible for preferential entry into cancer cells
Initial data from peptide-GST constructs defined aa 50-77 of azurin as a putative PTD for cell penetration, which fits well with structural evidence for an α-helical region encompassing residues 54-67 of azurin stabilizing the azurin molecule. Confocal analyses initially suggested that p28 and pi 8 of p28/azurin (Figure 15 A) penetrated human melanoma, prostate, lung, breast and ovarian cancer cells with relatively similar efficiency, but did not penetrate histologically matched normal cell lines to the same degree (Figure 15 A). A singular exception was CCD 13-Lu, a cell line derived from lung fibroblasts. The cationic Arg8 was rapidly and efficiently taken up into fibroblasts (Figure 15 A) and all other normal cell lines tested (data not shown).
These observations were essentially confirmed by a more sensitive FACs analyses (Figure 15 B) where p28 fluorescence was about 0.5-6 and pi 8 about 0.5-3 fold higher than the corresponding normal cell line, with the exception of lung cancer. A similar pattern in intracellular fluorescence intensity was observed within a histopathologic subtype, melanoma, where the relative intensity of pi 8 was about 50% of that observed with p28 (Figure 15 C). Fluorescence intensity over background was also consistently lower in normal and cancer cell pairs exposed to pi 8 than p28 (data not shown), again suggesting less p 18 entered individual cells. In all cases, the degree of entry of pi 8 and p28 into either cancer or normal cells was significantly less than that observed with Arg8, where no preference for entry was observed (Figure 15 A). The predicted Robson structure (data not shown) of pi 8 suggests that the C-terminal amino acids form a partial β-sheet. This and the shorter length of pi 8, which lacks the hydrophilic C-terminal 10 amino acids (aa 68-77, SEQ ID NO: 92) of p28, suggests that pi 8, as a putative PTD for azurin, may have a more rapid entry into cancer and normal cells via a non-endocytotic over an endocytotic or membrane receptor mediated process. MAPAS data (MRS 3.74, MAS 87.1, Kmpha 2.37) predict that aa's 69, 70, 75, 76, 85 of azurin provide the best opportunity for membrane contact, suggesting the C-terminal region of p28, not present on pi 8 (aa 50-67) is most likely to contact specific residues on the cell membrane, irrespective of a cell's status.
The preferential penetration of pi 8 and p28 was confirmed by exposing the same cell lines to azurin 60-77 (pi 8b), or aa 66-77 (SEQ ID NO: 93), the C-terminal 12 aa of p28 (Figure 16 A, B). Here, the preferential penetration observed with pi 8 and p28 was completely abolished, pi 8b (theoretical p/4.13) has a short α-helix and partial β-sheet, and is extremely hydrophilic which together may negate preferential entry, pi 2 (theoretical p/ 4.33) lacks a secondary α -helical structure, but is also hydrophilic suggesting overall hydrophilicity may be a major contributor to the decrease in selectivity of cell penetration.
Example 27 - Cell penetration is not a result of membrane disruption
Cell penetration by azurin, p28, and p 18 does not result from membrane disruption. An LDH leakage assay using UISO-Mel-2 cells in the presence of 5-100 μM p28, pi 8 or azurin (Figure 17 A) suggested that neither peptide nor azurin entered cells by altering plasma membrane integrity. The lack of membrane disruption was confirmed by determining the hemolytic activity of azurin, p28, and pi 8 on human erythrocytes against the receptor mimetic MAP and mast cell degranulating peptide mastoparan 7, which translocates cell membranes as an amphipathic alpha-helix, and activates heterotrimeric G proteins. Mastoparan 7 caused complete cell lysis at 25 μM, while azurin, p28, and pi 8 had no hemolytic effect when compared to control (no peptide) (Figure 13 B).
Example 28 - pl8/p28 penetration is energy dependent and saturable
The penetration of p28 (Figure 18 A) and pl8 (Figure 18 B) into UISO-Mel-2 cells is temperature dependent. Cell penetration and intracellular transport occurs relatively slowly over 3 hr at 40C, while entry and intracellular transport through various compartments is rapid at 22 and 370C as pl8 and p28 were present in the nucleus of UISO-Mel-2 cells within 2 hrs post exposure. The penetration of 5 μM p28 (Figure 18 C) or pi 8 (Figure 18 D) into UISO- Mel-2 cells after 30 min in the presence of a 200 fold excess of unlabeled peptide was severely curtailed, suggesting that entry was a saturable process and specific receptors or cell surface proteins or specific residues were, at least in part, responsible for initial entry.
Example 29 - Kinetics of p28 and pl8
The kinetics of p28 and pi 8 entry into UISO-Mel-2 cells relative to human fibroblasts was calculated after incubation, when cells were fixed and mean fluorescence intensity (MFI) determined. The Km and Vmax of each peptide were calculated by plotting peptide concentration (μM) vs velocity (MFI/sec) or by Scatchard analysis. Although the penetration of azurin fragments 50-67 (pl8: Vmax 2.46, Km 101.6) and 50-77 (p28: Vmax 1.87, Km 159.1) into cancer and normal cells (Vmax 2.88, Km 102.1 and Vmax 1.89, Km 166.0, respectively) differs significantly from each other, with pi 8 entering -42% faster, the rate of the entry of each peptide into normal and cancer cells is virtually identical. The increase in amount of fluorescence following exposure of cancer cells to p28 relative to p 18 is likely due to the increase in the amount of p28 entering malignant cells. 125I azurin and pi 8 bound to UISO-Mel-2 cells with a similar affinity. In contrast, significantly more p28 (Kd 2.5μm, Bmax 3.0 pm) bound to UISO-Mel-2 cells with a higher affinity when exposed for a longer period of time (20 min vs 2 min) at a higher temperature (37°C vs 40C) than either pi 8 (Kj 18 min, Bmax 0.51 pm) or azurin (Kd 10 nm and 0.48 pm). These results suggest that azurin, p28, and pi 8 all bind with relatively high affinity and capacity to a site on the cancer and normal cell surface prior to entry, but may enter via more than one mechanism.
Example 30 - pl8/p28 penetration involves Caveolae and the Golgi Complex Peptides called cell-penetrating peptides (CPPs) or cell-delivery vectors (CDVs), such as penetratin, transportan, Tat (amino acids 47-57 or 48-60), and the model amphipathic peptide MAP, are short, amphipathic and cationic peptides and peptide derivatives, usually containing multiple lysine and arginine residues. Fischer, P. M., Med Res Rev, 27: 755-795 (2007). They form a class of small molecules receiving significant attention as potential transport agents or delivery vehicles for a variety of cargoes, including cytotoxic drugs, anti- sense oligo-nucleotides, proteins, and peptides, in gene therapy, and as decoy peptides. Hallbrink, M. et al. Biochim. Biophys. Acta 1515: 101-109 (2001); Lindgren, M., et al. Trends Pharmacol. Sci. 21 : 99-103 (2000); Gusarova, et al, J Clin Invest, 117: 99-111 (2007); Melnick, A., Biochem Soc Trans, 35: 802-806 (2007); Astriab-Fisher et al, Pharm Res, 19: 744-754 (2002); El-Andaloussi et al, J Gene Med, 8: 1262-1273 (2006); Cashman et al, MoI Ther, 6: 813-823 (2002). As a class, cationic CPPs such as pTat and Arg8 enter cells by initially binding to anionic, sulfated proteoglycans prior to endocytosis. Incubation of p28 and pi 8 and Arg8 with UISO-Mel-2 cells under serum free conditions in the presence/absence of lOOμg/ml heparin sulfite (HS) significantly reduced the amount of intracellular Arg8, but did not alter the entry of either p28 or pl8 (Figure 19 A). The penetration of pl8 and p28 into UISO-MeI- 2 cells in the presence or absence of a specific inhibitor of O-linked glycosylation,
BnGalNac, and neruaminidase, which cleaves sialic acid residues, was further characterized (Figure 19 B), and no inhibition of penetration was observed. However, tunicamycin, an inhibitor of N-linked glycosylation, significantly reduced the penetration of pi 8 and p28 across the cell membrane. The entry of pi 8 and p28 into UISO-MeI -2 cells was also analyzed using inhibitors of energy dependent transport mechanisms, i.e., ATP. Sodium azide (Figure 19 B) and ouabain (Na+K+ ATPase pump) did not significantly inhibit the penetration of either peptide suggesting non endocytosic pathways might also be involved in the penetration of these peptides. Chlorpromazine (CPZ), a specific inhibitor of clathrin mediated endocytosis, also had no effect on penetration, nor did the macropinocytosis inhibitor amiloride. (Figure 15 B). Stabilization of microtubules with taxol had no effect on penetration , but disruption of actin filaments and macropinocytosis with Cytochalasin D produced a small (-20%), reproducible inhibition of the penetration of pi 8 and p28. The lack of effect of amiloride suggests that the inhibitory activity of Cytochalasin D is probably through its effect on actin filaments. Inhibition of the cell cycle with staurosporine did not block penetration, suggesting that penetration was not cell cycle specific. The lack of effect of staurosporine on pi 8 and p28 penetration of the cancer cell plasma membrane also suggests that a Src kinase/tyrosine kinase dependent pathway was not involved in penetration, was dynamin independent, and hence independent of caveolae budding. Neither pl8 nor p28 co-localized with flotillin-1 (data not shown) a protein that resides within the plasma membrane and in a specific population of endocytic intermediates , again arguing against a role for flotillin and dynamin in internalization . In contrast, nocodazole, which disrupts caveolae transport and inhibitors of cholesterol mobilization and hence, caveolae-mediated endocytosis, inhibited penetration 50-65%.
The intracellular disposition of pi 8 and p28 was then analyzed using wortmannin, an inhibitor of early endosome formation, monensin, which inhibits late endosome/lysosome, and brefeldin A (BFA), a disruptor of the Golgi apparatus. Wortmannin did not block the intracellular accumulation of either pi 8 or p28 suggesting that, unlike cholera toxin, a caveolae to early endosome pathway is not involved in the intracellular trafficking of pi 8 and p28. The lack of early endosome involvement in the intracellular trafficking of pi 8 and p28 also suggests that clathrin mediated endocytosis is not involved in internalization of these peptides.
However, monensin (Figure 19 B) and BFA reduced the intracellular accumulation of both peptides with a greater inhibitory effect on p28 (-30%) than pi 8 (-10%) (Figure 19 B). The penetration of p28 and pi 8 into fibroblasts was also inhibited by MβCD, nocodazole, monensin and tunicamycin, but not by amiloride, sodium azide, and CPZ (Figure 19 C). This suggests that at least one mechanism of entry into cancer and normal cells may be similar, but additional preferential accumulation into cancer cells may be a function of the number of common membrane receptors or structures, ie., caveolae (Figure 19 D, panels 1, 2). Alexafluor 568 labeled pi 8 and p28 co-localized with caveolin-1 and golgin 97 antibodies (Figure 19 D panels 1,2). This confirms that these organelles are involved in the intracellular trafficking of pl8 and p28. Interestingly, azurin, but neither pl8 nor p28 colocalized with mitochondrial specific fluorescence (Figure 19 D panel 3). In contrast, p28 and azurin, but not pi 8, co-localized with lysosomes ( Figure 19 D panel 4).
Example 31 - Functional Analysis of p28 and pl8 Azurin inhibits the growth of several human cancer cell lines in vitro and in vivo.
Figures 20 A and B illustrate the effect of pi 8 and p28 relative to azurin and dacarbazine (DTIC) on UISO-Mel-2 cells as determined by MTT and cell count. After 72hrs exposure, azurin decreased (p<0.05) cell survival at 100 and 200μM -15% (Figure 20 A). p28 had inhibited cell survival 14 and 22% (p 0.05) at 100 and 200μM, respectively. In contrast, pi 8 had no effect, while dacarbazine (DTIC) produced a significant dose-related decrease on UISO-Mel-2 survival. Azurin and p28 (200μM) also significantly decreased the survival of UISO-Mel-23 and 29 cells, pi 8 had no effect on UISO-Mel-2 cell proliferation. The apparent increase (-30-35%; UISO-Mel-2) in p28 and azurin inhibition of melanoma cell proliferation, as measured by direct cell counting, suggests that the inhibitory effect may reside primarily at the level of cell cycle with apoptosis subsequent to any delay. Although pi 8 penetrated cancer cells preferentially, unlike p28, it had virtually no inhibitory activity on cell proliferation. This result indicates that the cytostatic and cytotoxic activity of p28 likely lies in the C-terminal 10-12 aa of the sequence.

Claims

What is claimed is:
1. An isolated. peptide that is a cupredoxin or cytochrome or a variant, derivative or truncation thereof and that may treat and/or prevent two or more conditions in mammalian cells.
2. The isolated peptide of claim 1, wherein said cupredoxin is azurin.
3. The isolated peptide of claim 1, wherein said cupredoxin is from an organism selected from the group consisting of Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp. , Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas βuorescens, Pseudomonas chlororaphis, Bordetella pertussis, Pseudomonas syringae, Xylella fastidiosa and Vibrio par ahaemolyticus.
4. The isolated peptide of claim 1, wherein the peptide is selected from the group consisting of SEQ ID NOS: 1, 5-12, 18 and 23.
5. The isolated peptide of claim 1, to which a sequence selected from the group consisting of SEQ ID NOS: 1, 5-12, 18 and 23 is a mutant or has at least 90% amino acid sequence identity.
6. The isolated peptide of claim 1 , wherein the peptide is a truncation of a peptide selected from the group consisting of SEQ ID NOS: 1, 5-12, 18 and 23.
7. The isolated peptide of claim 6, wherein the peptide comprises the sequence and/or the equivalent residues of a cupredoxin as a region selected from the group consisting of SEQ ID NOS: 25, 27-33, and 48-50.
8. A composition, comprising one or more cupredoxins, cytochromes or peptides of claim 1 in a pharmaceutical composition.
9. The composition of claim 8, wherein the cupredoxin is selected from one or more of the group consisting of SEQ ID NOS: 1, 5-12, 18, 23, 25, 27-33 and 48-50.
10. The composition of claim 8, wherein the cupredoxin comprises SEQ ID NO: 30.
11. The composition of claim 8, wherein the composition is administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, bacterial infection, Cytomegalovirus infection, human papillomavirus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), parainfluenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus, arena virus, Dhori virus, poliovirus, rubella virus, dengue virus; SIV, Mycobacterium tuberculosis and cancer.
12. The composition of claim 8, wherein the composition is administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
13. The composition of claim 12, wherein the patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
14. The composition of claim 8, which additionally comprises another drug selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
15. The composition of claim 8, wherein the pharmaceutical composition is coadministered with at least one other drug.
16. The composition of claim 15, wherein the other drug is selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti- angiogenesis drug.
17. A method to administer to a patient the pharmaceutical composition of claim 8.
18. The method of claim 17, wherein the patient is human.
19. The method of claim 17, wherein the composition is administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of interstitial cystitis (IC), lesions associated with inflammatory bowel disease (IBD), HIV infection, AIDS, central nervous system disorders, peripheral vascular diseases, viral diseases, degeneration of the central nervous system (Christopher Reeve's disease), Alzheimer's disease, malaria, inappropriate angiogenesis, cardiovascular disease, hypertension, Cytomegalovirus infection, human papillomavirus infection; Muscular Dystrophy, encephalopathy, dementia, Parkinson's disease, neuropathy, macular degeneration, diabetic retinopathy, rheumatoid arthritis, psoriasis, herpes simplex virus (HSV), Ebola virus, cytomeglovirus (CMV), parainfluenza viruses types A, B and C, hepatitis virus A, B, C, and G, the delta hepatitis virus (HDV), mumps virus, measles virus, respiratory syncytial virus, bunyvirus, arena virus, Dhori virus, poliovirus, rubella virus, dengue virus; SIV, Mycobacterium tuberculosis and cancer.
20. The method of claim 17, wherein said composition is administered to a patient for the concurrent prevention and/or treatment of two or more conditions selected from the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
21. The method of claim 20, wherein said patient has a higher risk than the general population of acquiring a condition selected from one or more of the group consisting of HIV, malaria, cancer and inappropriate angiogenesis.
22. The method of claim 17, wherein said composition additionally comprises another drug selected from the group consisting of an anti -malarial drug, an anti-HIV drug, an anti-cancer drug and an anti-angiogenesis drug.
23. The method of claim 17, wherein said pharmaceutical composition is coadministered with at least one other drug.
24. The method of claim 23, wherein said other drug is selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti- angiogenesis drug.
25. A kit comprising the composition of claim 8.
26. The isolated peptide of claim 1, wherein the cupredoxin is selected from the group consisting of azurin, pseudoazurin, plastocyanin, rusticyanin, Laz, auracyanin, stellacyanin and cucumber basic protein.
27. The isolated peptide of claim 1, which can inhibit parasitemia by malaria in P. falciparum-infected human red blood cells.
28. The isolated peptide of claim 1, which is fused to a H.8 region of Laz.
29. The isolated peptide of claim 1, which is a structural equivalent of monoclonal antibody G 17.12.
30. The isolated peptide of claim 1 , wherein the cytochrome is selected from one or more of the group consisting of cytochrome c, cytochrome f and cytochrome C551.
31. The isolated peptide of claim 30, wherein the cytochrome c is from an organism selected from the group consisting of human and Pseudomonas aeruginosa.
32. The isolated peptide of claim 30, wherein the cytochrome f is from a cyanobacteria.
33. The isolated peptide of claim 1 , which is a truncation of cupredoxin or cytochrome.
34. The isolated peptide of claim 33, wherein the peptide is more than about 10 residues and not more than about 100 residues.
35. The isolated peptide of claim 6, wherein the peptide consists of a sequence selected from the group consisting of SEQ ID NOS: 25, 27-33, and 48-50.
36. The composition of claim 8, wherein the cupredoxin is from an organism selected from the group consisting of Pseudomonas aeruginosa, Alcaligenes faecalis, Achromobacter xylosoxidan, Bordetella bronchiseptica, Methylomonas sp. , Neisseria meningitidis, Neisseria gonorrhea, Pseudomonas βuorescens, Pseudomonas chlororaphis, Bordetella pertussis, Pseudomonas syringae, Xylella fastidiosa and Vibrio par ahaemolyticus.
37. The composition of claim 36, wherein the cupredoxin is from Pseudomonas aeruginosa.
38. The composition of claim 8, wherein the pharmaceutical composition is administered by a mode selected from the group consisting of intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection and oral.
39. The composition of claim 8, wherein the pharmaceutical composition is administered at about the same time as another drug.
40. The composition of claim 39, wherein the other drug is selected from the group consisting of an anti -malarial drug, an anti-HIV drug, an anti-cancer drug and an anti- angiogenesis drug
41. The composition of claim 11 , wherein the cancer is selected from the group consisting of melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors and prostate cancer.
42. The method of claim 17, wherein the pharmaceutical composition is administered by a mode selected from the group consisting of intravenous injection, intramuscular injection, subcutaneous injection, inhalation, topical administration, transdermal patch, suppository, vitreous injection and oral.
43. The method of claim 17, wherein the pharmaceutical composition is administered at about the same time as another drug.
44. The method of claim 43, wherein the other drug is selected from the group consisting of an anti-malarial drug, an anti-HIV drug, an anti-cancer drug and an anti- angiogenesis drug.
45. The method of claim 19, wherein the cancer is selected from the group consisting of melanoma, leukemia, breast cancer, ovarian cancer, lung cancer, mesenchymal cancer, colon cancer, aerodigestive tract cancer, cervical cancer, brain tumors and prostate cancer.
PCT/US2008/013721 2007-12-14 2008-12-15 Compositions and methods to concurrently treat or prevent multiple diseases with cupredoxins WO2009078977A2 (en)

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
US1370907P 2007-12-14 2007-12-14
US61/013,709 2007-12-14

Publications (3)

Publication Number Publication Date
WO2009078977A2 true WO2009078977A2 (en) 2009-06-25
WO2009078977A3 WO2009078977A3 (en) 2009-08-27
WO2009078977A9 WO2009078977A9 (en) 2009-12-30

Family

ID=40796067

Family Applications (1)

Application Number Title Priority Date Filing Date
PCT/US2008/013721 WO2009078977A2 (en) 2007-12-14 2008-12-15 Compositions and methods to concurrently treat or prevent multiple diseases with cupredoxins

Country Status (1)

Country Link
WO (1) WO2009078977A2 (en)

Cited By (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US8017749B2 (en) * 2006-12-04 2011-09-13 The Board Of Trustees Of The University Of Illinois Compositions and methods to treat cancer with cupredoxins and CpG rich DNA
EP2379098A1 (en) * 2008-12-18 2011-10-26 CDG Therapeutics, Inc. Compositions and methods to prevent cancer with cupredoxins
US9161989B2 (en) 2004-10-07 2015-10-20 The Board Of Trustees Of The University Of Illinois Cupredoxin derived transport agents and methods of use thereof
US9309292B2 (en) 2004-10-07 2016-04-12 The Board Of Trustees Of The University Of Illinois Transport agents for crossing the blood-brain barrier and into brain cancer cells, and methods of use thereof
US9598470B2 (en) 2004-10-07 2017-03-21 Craig W. Beattie Compositions and methods to prevent cancer by stabilizing P53 through non MDM2-mediated pathways
US9957304B2 (en) 2001-02-15 2018-05-01 Ananda Chakrabarty Compositions and methods for treating conditions related to ephrin signaling with cupredoxins
US10675326B2 (en) 2004-10-07 2020-06-09 The Board Of Trustees Of The University Of Illinois Compositions comprising cupredoxins for treating cancer

Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20060149037A1 (en) * 2004-10-07 2006-07-06 Ananda Chakrabarty Cupredoxin derived transport agents and methods of use thereof
US20060251669A1 (en) * 2001-02-15 2006-11-09 Ananda Chakrabarty Compositions and methods for treating malaria with cupredoxin and cytochrome

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20060251669A1 (en) * 2001-02-15 2006-11-09 Ananda Chakrabarty Compositions and methods for treating malaria with cupredoxin and cytochrome
US20060149037A1 (en) * 2004-10-07 2006-07-06 Ananda Chakrabarty Cupredoxin derived transport agents and methods of use thereof

Cited By (12)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US9957304B2 (en) 2001-02-15 2018-05-01 Ananda Chakrabarty Compositions and methods for treating conditions related to ephrin signaling with cupredoxins
US10889621B2 (en) 2001-02-15 2021-01-12 The Board Of Trustees Of The University Of Illinois Compositions and methods for treating conditions related to ephrin signaling with Cupredoxins
US9161989B2 (en) 2004-10-07 2015-10-20 The Board Of Trustees Of The University Of Illinois Cupredoxin derived transport agents and methods of use thereof
US9309292B2 (en) 2004-10-07 2016-04-12 The Board Of Trustees Of The University Of Illinois Transport agents for crossing the blood-brain barrier and into brain cancer cells, and methods of use thereof
US9598470B2 (en) 2004-10-07 2017-03-21 Craig W. Beattie Compositions and methods to prevent cancer by stabilizing P53 through non MDM2-mediated pathways
US9968685B2 (en) 2004-10-07 2018-05-15 Brad N. Taylor Methods to treat cancer with cupredoxins
US10675326B2 (en) 2004-10-07 2020-06-09 The Board Of Trustees Of The University Of Illinois Compositions comprising cupredoxins for treating cancer
US8017749B2 (en) * 2006-12-04 2011-09-13 The Board Of Trustees Of The University Of Illinois Compositions and methods to treat cancer with cupredoxins and CpG rich DNA
US9969781B2 (en) 2006-12-04 2018-05-15 Tapas Das Gupta Compositions and methods to treat cancer with CpG rich DNA and cupredoxins
US11046733B2 (en) 2006-12-04 2021-06-29 The Board Of Trustees Of The University Of Illinois Compositions and methods to treat cancer with CpG rich DNA and cupredoxins
EP2379098A1 (en) * 2008-12-18 2011-10-26 CDG Therapeutics, Inc. Compositions and methods to prevent cancer with cupredoxins
EP2379098A4 (en) * 2008-12-18 2012-12-05 Cdg Therapeutics Inc Compositions and methods to prevent cancer with cupredoxins

Also Published As

Publication number Publication date
WO2009078977A9 (en) 2009-12-30
WO2009078977A3 (en) 2009-08-27

Similar Documents

Publication Publication Date Title
US7740857B2 (en) Compositions and methods for treating malaria with cupredoxin and cytochrome
US7301010B2 (en) Compositions and methods for treating HIV infection with cupredoxin and cytochrome c
US10351605B2 (en) Compositions and methods to prevent cancer by stabilizing p53 through non MDM2-mediated pathways
WO2009078977A2 (en) Compositions and methods to concurrently treat or prevent multiple diseases with cupredoxins
US10196428B2 (en) Modification of cupredoxin derived peptides
US20090208476A1 (en) Compositions and methods to concurrently treat or prevent multiple diseases with cupredoxins
US20140287990A1 (en) Compositions and methods to concurrently treat and/or prevent multiple diseases with cupredoxins
AU2010201360A1 (en) Compositions and methods for treating malaria with cupredoxin and cytochrome
US8158574B2 (en) Compositions and methods to prevent cancer with cupredoxins
EP1883650A2 (en) Compositions and methods for treating hiv infection with cupredoxin and cytochrome c
US10266868B2 (en) Compositions for treating HIV infection with cupredoxin and cytochrome C

Legal Events

Date Code Title Description
121 Ep: the epo has been informed by wipo that ep was designated in this application

Ref document number: 08860898

Country of ref document: EP

Kind code of ref document: A2

NENP Non-entry into the national phase

Ref country code: DE

122 Ep: pct application non-entry in european phase

Ref document number: 08860898

Country of ref document: EP

Kind code of ref document: A2