OA17472A - Pharmaceutical composition comprising albumin-binding arginine deiminase for cancer targeting treatment. - Google Patents
Pharmaceutical composition comprising albumin-binding arginine deiminase for cancer targeting treatment. Download PDFInfo
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- OA17472A OA17472A OA1201500352 OA17472A OA 17472 A OA17472 A OA 17472A OA 1201500352 OA1201500352 OA 1201500352 OA 17472 A OA17472 A OA 17472A
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- Prior art keywords
- albumin
- fusion protein
- binding
- arginine deiminase
- cancer
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Abstract
The present invention provides a pharmaceutical composition containing albuminbinding arginine deiminase fusion protein (AAD) for treating cancer or other arginine-dependent diseases. The AAD fusion protein can be purified from both soluble and insoluble fractions of crude proteins, it binds to human serum albumin (HSA) and has its high activity with longer half life for efficient depletion of arginine in cancer cells. The specific activities of wild-type ADI and AAD in the present invention are 8.4 and 9.2 U/mg (at physiological pH 7.4), respectively. The AAD used in the present invention can be used in the treatment of various cancers (e.g. pancreatic cancer, leukemia, head and neck cancer, colorectal cancer, lung cancer, breast cancer, liver cancer, nasopharyngeal cancer, esophageal cancer, prostate cancer, stomach cancer and brain cancer) and curing arginine-dependent diseases. The composition can be used alone or in combination with at least one chemotherapeutic agent to give a synergistic effect on cancer treatment and/or inhibiting metastasis.
Description
PHARMACEUTICAL COMPOSITION COMPRISING ALBUMIN-BINDING ARGININE DEIMINASE FOR CANCER TARGETING TREATMENT
Cross-reference to Related Application [0001] The présent application claims benefit from US provisional patent application serial number 61/773,214 filed March 6, 2013 and US non-provisional patent application serial number 14/197,236 filed March 5, 2014, and the disclosures of which are incorporated herein by reference in its entirety.
Technical Field [0002] The présent invention describes albumin-binding arginine deiminase (AAD) fusion protein that has been genetically modified to create a material having high activity and long in vivo half-life. The présent invention further describes the designs for DNA and protein engineering for creating different AAD fusion proteins. The AAD fusion proteins can be isolated and purified from soluble fraction and insoluble fraction (inclusion bodies) of the crude proteins. The présent invention further relates to albumin-binding arginine deiminase-containing pharmaceutical compositions for cancer targeting treatment and curing arginine-dependent diseases in humans and other animais.
Background of the Invention [0003] The incidence of pancreatic cancer, colon cancer, liver cancer, melanoma and cervical cancer in the worldwide population is increasing. Effective treatments for these diseases are urgently needed. In many types of cancer including leukemia, melanoma, pancreatic, colon, rénal cell carcinoma, lung, prostate, breast, brain, cervical and liver cancers, the cancer cells are auxotrophic for arginine since they lack of expression of argininosuccinate synthetase (ASS), making these cancers excellent targets for arginine déplétion therapy.
[0004] Arginine is a semi-essential amino acid for humans and other mammals. It can be synthesized from citrulline via a two step process catalyzed by the urea cycle enzymes argininosuccinate synthase (ASS) and argininosuccinate lyase (ASL). Arginine can be metabolized to omithine by the enzyme arginase, and omithine can be converted to citrulline by omithine carbamoyltransferase (OTC) in the mitochondria. The citrulline can be utilized to synthesize arginine again. Normal cells usually do not require an exogenous supply of arginine for growth because of the abundant catalytic activity of ASS and ASL. In contrast, many types of cancers do not express ASS and therefore are auxotrophic for arginine. Their growth is dépendent on arginine solely obtained from blood circulation. Therefore, targeting circulating arginine by using arginine-degrading enzymes is a feasible strategy to inhibit ASS-negative tumor growth [Feun et al., Curr. Pharm. Des. 14:1049-1057 (2008); Kuo et al., Oncotarget. 1:246-251 (2010)] [0005] Arginine can be degraded by arginase, arginine decarboxylase, and arginine deiminase (ADI). Among them, arginine deiminase (ADI) appears to hâve the highest affmity for arginine (a low Km value). ADI converts arginine to citrulline and ammonia, the métabolites of the urea cycle. Unfortunately, ADI can only be found in prokaryotes e.g. Mycoplasma sp. There are some problems associated with the isolation and purification of ADI from prokaryotes. ADI isolated from Pseudomonas pudita fails to exhibit efficacy in vivo because of its low enzymatic activity in neutral pH. ADI produced from Escherichia coli is enzymatically inactive and subsequently requires multiple dénaturation and renaturation process which raises the subséquent cost of production.
[0006] As the native ADI is found in microorganisms, it is antigenic and rapidly cleared from circulation in a patient. The native form of ADI is immunogenic upon injection into human circulation with a short half-life (~4 hours) and elicits neutralizing antibodies [Ensor et al., Cancer Res. 62:5443-5450 (2002); Izzo et al., J. Clin. Oncol. 22:1815-1822 (2004)]. These shortcomings can be remedied by pegylation. Among various forms of pegylated ADI, ADI bound with PEG (molecular weight 20,000) via succinimidyl succinate (ADI-PEG 20) has been found to be an effïcacious formulation. However, the activity of ADI after pegylation is greatly decreased on the order of 50% [Ensor et al., Cancer Res. 62:5443-5450 (2002)]. The previous attempts to create pegylated ADI resulted in materials that are not homogenous (due to the random attachment of PEG on protein surface Lys residues) and also difficult to characterize and perform quality control during the manufacturing process. Also, PEG is very expensive, greatly increasing the production cost. After the intravenous injection of pegylated ADI in vivo, leakage or detachment of free PEG is observed and the ADI (without PEG) can elicit the immunogenicity problem. Therefore, there is a need for improved cancer-treatment compositions, particularly, improved cancer-treatment compositions that hâve enhanced activity and in vivo half-life. Ύ
Summary of the Invention [0007] In the présent invention, albumin-binding arginine deiminase (AAD) fusion protein has increased its activity and plasma half-life in order to efficiently deplete arginine in cancer cells. Native ADI may be found in microorganisms and is antigenic and rapidly cleared from circulation in a patient. The présent invention constructs different AAD fusion proteins with one or two albumin-binding proteins to maintain high activity with longer in vivo half-life (at least 5 days of arginine déplétion after one injection). In the présent invention, the albumin binding protein in the AAD fusion protein product does not appear to influence its spécifie enzyme activity but instead appears to increase the circulating half-life. The spécifie activities of wildtype ADI and AAD fusion protein in the présent invention are 8.4 and 9.2 U/mg (at physiological pH 7.4), respectively.
[0008] In its broadest sense, the présent invention provides an albumin-binding arginine deiminase fusion protein comprising a first portion comprising one or two components selected from an albumin-binding domain, an albumin-binding peptide or an albumin-binding protein(s) fused to a second portion comprising arginine deiminase to form the albumin-binding arginine deiminase fusion protein such that the albumin-binding arginine deiminase fusion protein retains the activity of arginine deiminase and is also able to bind sérum albumin.
[0009] The présent invention further relates to albumin-binding arginine deiminase (AAD) fusion protein -containing pharmaceutical compositions for targeted cancer treatment in humans and other animais. The first aspect of the présent invention is to construct the modified AAD fusion protein with high activity against cancer cells. The second aspect of the présent invention is to purify AAD fusion protein with high purity from both soluble and insoluble fractions of the crude proteins. The third aspect of the présent invention is to lengthen the half-life of AAD fusion protein as it can bind to albumin very well in the circulation. The fourth aspect of the présent invention is to provide a method of using the AAD-containing pharmaceutical composition of the présent invention for treating cancer by administering said composition to a subject in need thereof suffering from various tumors, cancers or diseases associated with tumors or cancers or other arginine-dependent diseases.
[0010] The AAD fusion protein of the présent invention is also modified to avoid dissociation into albumin-binding protein and ADI such that it becomes more stable and has a longer half-life in circulation. ADI is fused to an albumin-binding domain/peptide/protein in AAD fusion product to extend the plasma half-life and reduce the immunogenicity of the fusion product. γ
Albumin binding domain (ABD) is a peptide that binds albumin in the blood. There are different variants of ABD showing different or improved human sérum albumin (HSA) affmities.
Different variants of ABD can be constructed and can be fused to ADI. Unlike the naturally occurring ADI, this longer half-life property facilitâtes the déplétion of arginine efficiently in cancerous cells, cancer stem cells and/or cancer progenitor cells.
[0011] The pharmaceutical composition containing AAD fusion protein can be used for intravenous (i.v.) injection (for rapid-acting dosage of médication) and intramuscular (i.m.) injection (for fairly rapid-acting and long-lasting dosage of médication). The application of AAD fusion protein in the présent invention can be used in the treatment of various cancers such as pancreatic cancer, leukemia, head and neck cancer, colorectal cancer, lung cancer, breast cancer, prostate cancer, cervical cancer, liver cancer, nasopharyngeal cancer, esophageal cancer and brain cancer. The présent invention is directed to AAD fusion proteins, to methods of treating cancer, to methods of treating and/or inhibiting metastasis of cancerous tissue, and to methods of curing arginine-dependent diseases.
[00 f 2] The method of the présent invention also includes using a combination of different chemotherapeutic drugs and/or radiotherapy with the AAD fusion protein of the présent invention to give a synergistic effect on cancer treatment.
Brief Description of the Drawings [0013] FIG. 1 shows the design approach for construction of different AAD fusion proteins with one or two albumin-binding domain/peptide/protein(s) in three-dimensional structure. One or two albumin-binding domain/peptide/protein(s) can be fused to ADI to form the AAD fusion protein. The position of albumin-binding domain/peptide/protein is far from the ADI active site. The albumin-binding domain/peptide/protein can be fused to the N-terminus or/and C-terminus of ADI. The structure in this figure is based on the Mycoplasma arginini ADI structure (Protein Data Bank: 1LXY). (A) Native ADI; (B) AAD fusion protein with two ABD or ABD1; (C) AAD fusion protein with one ABD or ABD1 at N-terminus; (D) AAD fusion protein with one ABD or ABD1 at C-terminus.
[0014] FIG. 2 shows the sequence alignment for ADI in some bacterial species including Mycoplasma arginini (SEQ ID No. 23), Lactococcus lactis (SEQ ID No. 24), Bacillus cereus (SEQ ID No. 25) and Bacillus licheniformis (SEQ ID No. 26).
[0015] FIG. 3 shows the designs and amino acid sequences for different AAD fusion proteins originated from Mycoplasma arginini (A to E) and AAD fusion protein originated from Bacillus cereus (F).
[0016] FIG. 4 shows the création of AAD fusion protein in two embodiments (A) and (B) by the use of intein-fusion proteins and expressed protein ligation (CBD, chitin binding domain) under the following schemes; (C) C-terminal fusion; (D) N-terminal fusion; (E) Intein-mediated protein ligation.
[0017] FIG. 5 shows the plasmid map of the expression vector constructed for producing AAD fusion protein.
[0018] FIG. 6 shows the (A) gene map, (B) nucléotide sequence (SEQ ID No. 44) and (C) amino acid sequence (SEQ ID No. 40) of His-ABD-PolyN-ADI. (ADI: the Mycoplasma arginini ADI) [0019] FIG. 7 shows the (A) gene map, (B) nucléotide sequence (SEQ ID No. 45) and (C) amino acid sequence (SEQ ID No. 41) of His-ABD-PolyN-bcADI. (bcADI, the Bacillus cereus ADI) [0020] FIG. 8 shows the expression and purification of AAD fusion protein: (A) AAD is -90% soluble when expressed at 20°C (lanes 2 and 3) and -90% insoluble (inclusion body) when expressed at 37°C (lanes 4 and 5); (B) The purified AAD fusion protein in sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) gel: lane 1, purified AAD fusion protein (52.8 kDa); lane 2, molecular weight marker.
[0021] FIG. 9 illustrâtes that AAD fusion protein depletes arginine efficiently and inhibits the growth of various types of human cancer cell lines in in vitro tissue culture studies, including human melanoma (A375), human colon carcinoma (HCT116), and human pancreatic cancer (Panel).
[0022] FIG. 10 shows the albumin binding results of AAD fusion protein: (A) A non-denaturing native polyacrylamide gel (12%) showing the increase in the amount of HSA+AAD complex when the amount of AAD fusion protein (the amino acid sequence is shown in SEQ ID NO: 36; FIG. 3A) added increases. The mole ratios of human sérum albumin (HSA): AAD in lanes 3-6 are 1:1, 1:2, 1:5, and 1:15, respectively. Lanes 1 and 2 represent HSA and AAD at 6 and 30 pmole, respectively; (B) In another experiment based on AAD fusion protein (SEQ ID NO: 40; FIG. 3E), an albumin: AAD ratio of 1:8 is sufficient to bind ail the albumin présent (lane 5).
[0023] FIG. 11 is a graph showing the dose response of AAD fusion protein on plasma arginine levels in mice. A dose of 100 pg of AAD is sufficient to deplete plasma arginine for at least 5 days.
Définitions [0024] The term “cancer stem cell” refers to the biologically distinct cell within the neoplastic clone that is capable of initiating and sustaining tumor growth in vivo (i.e. the cancer-initiating cell).
Detailed Description of the Invention [0025] Arginine is a semi-essential amino acid for humans and other mammals. It can be synthesized from citrulline via a two step process catalyzed by urea cycle enzymes argininosuccinate synthase (ASS) and argininosuccinate lyase (ASL). Arginine can be metabolized to omithine by the enzyme arginase, and omithine can be converted to citrulline by omithine carbamoyltransferase (OTC) in the mitochondria. The citrulline can be utilized to synthesize arginine again. Normal cells do not typically require an exogenous supply of arginine for growth because of the abundant catalytic activity of ASS and ASL. In contrast, many types of cancers do not express ASS and are therefore auxotrophic for arginine. Their growth is solely dépendent on arginine from circulation. Therefore, targeting circulating arginine by using arginine-degrading enzymes is a feasible strategy to inhibit ASS-negative tumor growth.
[0026] Arginine can be degraded by arginine deiminase (ADI). ADI converts arginine to citrulline and ammonia, the métabolites of the urea cycle. Unfortunately, ADI can only be found in prokaryotes e.g. Mycoplasma sp. There are many problems associated with the isolation and purification of arginine deiminase from prokaryotes. ADI isolated from Pseudomonas pudita failed to exhibit efficacy in vivo because of its low enzymatic activity in neutral pH. ADI produced from Escherichia coli is enzymatically inactive and subsequently requires multiple dénaturation and renaturation process which raised the subséquent cost of production. The plasma half-life of the native form of ADI is short (~4 hours) upon injection into human circulation [Ensor et al., Cancer Res. 62:5443-5450 (2002); Izzo et al., J. Clin. Oncol. 22:18151822 (2004)]. These shortcomings can be partially remedied by pegylation. Among various forms of pegylated ADI, ADI bound with PEG (molecular weight 20,000) via succinimidyl succinate (ADI-PEG 20) has been found to be an efficacious formulation. However, the activity of ADI after pegylation is greatly decreased (by -50%) [Ensor et al., Cancer Res. 62:5443-5450 (2002); Wang et al., Bioconjug. Chem. 17:1447-1459 (2006)]. Also, the succinimidyl succinate PEG linker can easily be hydrolyzed and detached from the protein, causing immunogenic problems after a short period of use in the body. Therefore, there is a need for improved cancertreatment compositions, particularly, improved cancer-treatment compositions with enhanced activity.
[0027] ADI isolated from P. pudita failed to exhibit efficacy in vivo because it had little enzyme activity at a neutral pH and was rapidly cleared from the circulation of experimental animais. ADI derived from Mycoplasma arginini is described, for example, by Takaku et al, Int. J. Cancer, 51:244-249 (1992), and U.S. Pat. No. 5,474,928. However, a problem associated with the therapeutic use of such a heterologous protein is its antigenicity. The chemical modification of ADI from Mycoplasma arginini, via a cyanuric chloride linking group, with polyethylene glycol (PEG) was described by Takaku et al., Jpn. J. Cancer Res., 84:1195-1200 (1993). However, the modified protein was toxic when metabolized due to the release of cyanide from the cyanuric chloride linking group. In contrast, even for the ADI-PEG20, the PEG linker can easily be hydrolyzed and detached from the protein, causing immunogenic problems after a short period of use in the body. Therefore, there is a need for compositions which dégradé non-essential amino acids and which do not hâve the problems associated with the prior art.
[0028] In many types of cancer including melanoma, pancreatic, colon, leukemia, breast, prostate, rénal cell carcinoma and liver cancers, cancer cells are auxotrophic for arginine since they lack of expression of argininosuccinate synthetase (ASS), making them excellent targets for arginine déplétion therapy. In this invention, albumin-binding arginine deiminase (AAD) fusion proteins hâve high activity with long half-lives for efficient déplétion of arginine in cancer cells.
[0029] The size of the monomer for ADI is on the order of 45 kDa and it exists as dimer (on the order of 90 kDa) [Das et al., Structure. 12:657-667 (2004)]. A design for construction of an AAD fusion protein is shown in FIG. 1. One or two albumin-binding domain/peptide/protein(s) with or without linker(s), SEQ ID NO: 46-49, are fused to ADI to form the AAD fusion protein. It is noteworthy that the sélection of one or two particular albumin-binding domain/peptide/protein(s) can be made depending upon the type of cancer tissue to be targeted, the desired size and halflife of the resulting fusion protein, and whether a domain or entire protein is selected. Further, vi the selected albumin-binding material may be the same or different. That is, a protein and a peptide can be fused, two proteins, two domains, a domain and a protein, etc., as long as the résultant molécule retains the activity of the ADI and is also able to bind sérum albumin with neither function of one portion of the fusion protein being interfered with by the other portion of the fusion protein. The position of the albumin-binding domain/peptide/protein is far from the active site. The albumin-binding domain/peptide/protein can be fused to the N-terminus or/and C-terminus of ADI. There are different variants of ABD showing different or improved human sérum albumin (HSA) affmities. Different variants of ABD can be constructed and can be fused to ADI. Some micro-organisms endowed with ADI (for example Pseudomonas sp) cannot be used, due to their potential pathogenicity and pyrogenicity. The source of ADI can be from, but not limited to, different microorganisms, e.g. Mycoplasma (e.g. Mycoplasma arginini, Mycoplasma arthritidis, Mycoplasma hominis), Lactococcus (e.g. Lactococcus lactis), Pseudomonas (e.g. Pseudomonas plecoglossicida, Pseudomonas putida, Pseudomonas aeruginosa), Steptococcus (e.g. Streptococcus pyogenes, Streptococcus pneumonia, Streptococcus pneumoniae), Escherichia, Mycobacterium (e.g. Mycobacterium tuberculosis) and Bacillus (e.g. Bacillus licheniformis, Bacillus cereus). It is preferred that ADI is cloned from Mycoplasma arginini, Lactococcus lactis, Bacillus licheniformis, Bacillus cereus, or any combination thereof. Their amino acid sequences with SEQ ID (SEQ ID NO: 23-35) and the sequence alignment for some of the amino acid sequences in FIG. 2 are disclosed herein and also in the literature [Das et al., Structure. 12:657-667 (2004); Wang et al., Bioconjug. Chem. 17:1447-1459 (2006); Ni et al., Appl. Microbiol. Biotechnol. 90:193-201 (2011)].
[0030] The design and amino acid sequence for (A) native Mycoplasma arginini ADI protein (SEQ ID NO: 23), (B) different AAD fusion proteins originated from the Mycoplasma arginini ADI (SEQ ID NO: 36-40) and (C) AAD fusion protein originated from the Bacillus cereus ADI (SEQ ID NO: 41) are shown in FIG. 3. Different AAD fusion proteins are successfully constructed. A linker is inserted between the albumin-binding protein and ADI in the AAD fusion protein in these embodiments.
[0031 ] On the other hand, a novel AAD fusion protein is also created by the use of intein-fusion proteins and expressed protein ligation (FIG. 4). The novel AAD fusion protein can be formed (1) by reacting the ADI having a N-terminal cysteine residue with a reactive thioester at C-terminus of the ABD, or (2) by reacting the ABD having a N-terminal cysteine residue with a reactive thioester at C-terminus of the ADI so that the ADI and the ABD are linked by a covalent bond,
In FIG. 4E, ADI with N-terminal cysteine residue reacts with reactive thioester at the C-terminus of ABD. The thioester tag at the C-terminus of ABD, and an α-cysteine at the N-terminus of ADI are required to facilitate protein ligation. These fragments are produced using a pTWIN l vector (New England Biolabs) according to the manufacturer’s manual. In particular, the gene coding for the ABD-Intein-CBD fusion protein is synthesized and it is cloned into the vector under the control of T7 promoter for expression in E. coli (FIG. 4C). The ABD-Intein-CBD fusion protein produced binds to chitin in a column. The amino acid sequence of ABD-InteinCBD (SEQ ID NO: 42) is shown in FIG. 4A. After thiol-inducible cleavage and elution from the column, the ABD with reactive thioester at its C-terminus is obtained (FIG. 4C). On the other hand, the gene coding for the CBD-Intein-ADI fusion protein is synthesized and cloned into the vector under the control of the T7 promoter for expression in E. coli (FIG. 4D). The CBD-InteinADI fusion protein produced binds to chitin in a column. The amino acid sequence of the CBDIntein-ADI (SEQ ID NO: 43) is shown in FIG. 4B. After cleavage at pH 7 and 25°C, and elution from the column, the ADI with α-cysteine at its N-terminus is obtained (FIG. 4D). Finally, the AAD fusion protein is produced by the protein ligation reaction as shown in FIG. 4E.
[0032] Importantly, AAD fusion proteins can be produced and purified in a convenient manner. For example, an AAD fusion protein is successfully expressed and purified from E. coli both in soluble fraction and insoluble fraction, and this resuit is shown in FIG. 8. Furthermore, FIG. 8 shows the purified AAD fusion protein analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). The size of the purified AAD fusion protein is determined as 52.8 kDa.
[0033] The pharmaceutical composition of the présent invention contains AAD fusion protein with high activity for depleting arginine in tumor cells for cancer treatment. The spécifie activity of the purified AAD fusion protein is found to be similar to that of the wild-type ADI. IC50 is the half maximal inhibitory concentration, that is, it represents the concentration of AAD fusion protein that is required for 50% inhibition of a cancer cell line. The IC50 is a measure of the effectiveness of a drug. The IC50 of AAD fusion protein (amino acid sequence is shown in SEQ ID NO: 40, FIG. 3E) for different cancer cell lines (human melanoma, A375 & SK-mel-28; human colon carcinoma, HCTl 16; human pancreatic cancer, Panel; human liver cancer, Sk-hepl; human cervical cancer, C-33A) is shown in TABLE 1. The in vitro efficacy of AAD fusion protein on different cancer cell lines is demonstrated in FIG. 9. It illustrâtes that AAD fusion protein can kill many cancer types, including human melanoma, human colon carcinoma and pancreatic cancer cell lines.
[0034] TABLE 1
| Cancer cell line | IC50 of AAD (μ§/ιη1) |
| A375 (human melanoma) | 0.104 |
| SK-mel-28 (human melanoma) | 1.92 |
| Panel (human pancreatic cancer) | 1 |
| Sk-hepl (human liver cancer) | 10 |
| C-33A (human cervical cancer) | 0.063 |
| HCT116 (human colon carcinoma) | 1.30 |
[0035] For the albumin binding study, we hâve demonstrated successfully that the engineered
AAD fusion protein can bind to human sérum albumin (HSA). FIG. 10 shows that the AAD fusion protein (amino acid sequence is shown in SEQ ID NO: 40, FIG. 3E) binds to HSA readily. At a mole ratio of 1:5 or 1:15, the formation of the HSA-AAD complex forms according to the construct of FIG. 1 using the linker molécule design. It is expected that the circulating half-life of 10 AAD fusion protein in the blood is increased by the non-covalent HSA-AAD complex formation.
Therefore, a long-lasting version of AAD fusion protein has been successfully created.
[0036] No commercial products show high efficacy when compared to the AAD fusion proteincontaining pharmaceutical composition prepared in this invention. For uses in cancer treatment, the AAD fusion protein-containing pharmaceutical composition of the présent invention serves 15 as an anti-cancer agent to deplete the arginine in tumor tissues. AAD fusion protein is a good candidate to be used in combination with other molecular targeting or cytotoxic agents.
Examples [0037] The following examples are provided by way of describing spécifie embodiments of this invention without intending to limit the scope of this invention in any way.
[0038] Several of the Examples below relate to methods of making an albumin-binding arginine deiminase fusion protein. Various techniques can be used including cloning and intein-mediated protein ligation. As used herein, the term “cloning” is broadly used and comprises constructing a fusion gene coding for the albumin-binding arginine deiminase fusion protein, inserting the fusion gene into a vector, inserting the vector into a host organism and expressing a protein that includes an albumin-binding arginine deiminase fusion protein. Numerous variants on this technique can be performed and still fall within the cloning contemplated by the présent invention.
[0039] Example 1 [0040] Construction of the gene coding for albumin-binding domain/peptide/protein (ABD) [0041] The gene coding for ABD is constructed by two rounds of PCR. In the first round, the PCR reaction mixture (total volume of 25 μΐ) contains the following materials:
x iProof PCR buffer (Bio-Rad) μΜ dNTP mixture
0.5 unit of iProof DNA Polymerase (Bio-Rad) nM of each of the following oligos
ABD-F1 forwardprimer (SEQ ID NO: 01):
5' -CATGATGCGAATTCCTTAGCTGAAGCTAAAGTCTTAGCTAACAGAGAACT-3 '
ABD-R2 reverse primer (SEQ ID NO: 02):
' -TAGTCACTTACTCCATATTTGTCAAGTTCTCTGTTAGCTAAGACTTTAGC-3 '
ABD-F3 forwardprimer (SEQ ID NO: 03):
' -GAACTTGACAAATATGGAGTAAGTGACTATTACAAGAACCTAATCAACAA-3 '
ABD-R4 reverse primer (SEQ ID NO: 04):
' -TACACCTTCAACAGTTTTGGCATTGTTGATTAGGTTCTTGTAATAGTCAC-3 '
ABD-F5 forwardprimer (SEQ ID NO: 05):
' -GCCAAAACTGTTGAAGGTGTAAAAGCACTGATAGATGAAATTTTAGCTGC - 3 '
ABD-R6 reverse primer (SEQ ID NO: 06):
' - AGCTACGATAAGCTTAAGGTAATGCAGCTAAAATTTCATCTATCAGTG - 3 '
The following PCR program is used:
98°C 30 s; 20 cycles of {98°C 10 s, 50°C 20 s, 72°C 20 s} [0042] In the second round of PCR, the PCR mixture (total volume of 50 μΐ) contains the following materials:
x iProof PCR buffer (Bio-Rad);
μΜ dNTP mixture;
μΐ of PCR reactant as DNA template from the first round;
unit of iProof DNA Polymerase (Bio-Rad);
200 nM of each of the following oligos:
ABD-F7forwardprimer (SEQ ID NO: 07):
5' -CATGATGCGAATTCCTTAGCTGAAGCTAAAGTCTTAGCTAACAGAGAACT-3 '
ABD-R8 reverse primer (SEQ ID NO: 08):
' -AGCTACGATAAGCTTAAGGTAATGCAGCTAAAATTTCATCTATCAGTG- 3 '
The following PCR program is used:
98°C 30 s; 35 cycles of {98°C 10 s, 60°C 20 s, 72°C 20 s}; 72°C 5 min [0043] A PCR product containîng the DNA sequence of ABD (169 bp) is obtained and purified by Qiagen DNA Gel Extraction Kit for cloning purpose.
[0044] Example 2A [0045] Construction of the fusion gene coding for the AAD fusion protein [0046] In the first PCR, the PCR mixture (total volume of 50 μΐ) contains the following materials:
x iProof PCR buffer (Bio-Rad);
μΜ dNTP mixture;
ng of Mycoplasma arginini genomic DNA; gb l unit of iProof DNA Polymerase (Bio-Rad);
200 nM of each of the following oligos:
ADINde-Fforwardprimer (SEQ ID NO: 09):
' -ATCGATCGATGTCTGTATTTGACAGTAAATTTAAAGG- 3 ’
ADIhis-R reverse primer (SEQ ID NO: 10):
’ -AGCTAAGGAATTCGCATCATGATGGTGATGGTGGTGGCTACCCCACTTAAC-3 '
The following PCR program is used:
98°C 1 min; 35 cycles of {98°C 10s, 50°C 20s, 72°C 40s}; 72°C 5 min
A PCR product of 1280 bp long is obtained and purified by Qiagen DNA Gel Extraction Kit. After that, the second PCR is performed. The PCR mixture (total volume of 50 μΐ) contains the following materials:
x iProof PCR buffer (Bio-Rad);
μΜ dNTP mixture;
ng of the 1280 bp PCR product;
ng of the 169 bp PCR product;
unit of iProof DNA Polymerase (Bio-Rad);
200 nM of each of the following oligos:
ADINde-Fforwardprimer (SEQ ID NO: 11):
' -ATCGATCGATGTCTGTATTTGACAGTAAATTTAAAGG- 3 '
ABD-R10 reverse primer (SEQ ID NO: 12):
' -AGCTACGATAAGCTTAAGGTAATGCAGCTAAAATTTCATCTATCAGTG-3 '
The following PCR program is used:
98°C 1 min; 35 cycles of {98°C 10s, 50°C 20s, 72°C 45s}; 72°C 5 min [0047] A PCR product of 1428 bp is obtained and purified by Qiagen DNA Gel Extraction Kit. Then it is digested with restriction enzymes Ndel and HindlII, and ligated to plasmid pREST A (Invitrogen) that is predigested with the same enzymes. The ligation product is then transformed into E. coli BL21 (DE3) cells. The sequence of the constructed fusion gene is confirmed by DNA sequencing.
[0048] Example 2B [0049] Cloning of His-ABD-PolyN-ADI [0050] The construction of His-ABD-PolyN-ADI (SEQ ID NO: 40, in FIG. 3E) is done by two steps of overlapping PCR, the PCR fragment obtained from the last step is inserted into the vector pET3a between the Ndel and BamHI sites. The gene map, nucléotide sequence and amino acid sequence of His-ABD-PolyN-ADI are shown in FIG. 6.
Primers involved in construction of His-ABD-PolyN-ADI:
hisABDNde-Fforwardprimer (SEQ ID NO: 13):
' -GGAGATATACATATGCATCATCACCATCACCATGATGAAGCCGTGGATG- 3 '
ABDnn-Rl reverse primer (SEQ ID NO: 14):
' -TTGTTATTATTGTTGTTACTACCCGAAGGTAATGCAGCTAAAATTTCATC- 3 ’
ABDn-R2 reverse primer (SEQ ID NO: 15):
’ -AGAACCGCCGCTACCATTGTTATTATTGTTGTTACTACCCGA- 3 ’
ADln-Fforwardprimer (SEQ ID NO: 16):
’ -AATAATAACAATGGTAGCGGCGGTTCTGTATTTGACAGTAAATTTAAAGG-3 '
ADIBam-R reverse primer (SEQ ID NO: 17):
’ -TAGATCAATGGATCCTTACCACTTAACATCTTTACGTGATAAAG-3 ' [0051] In the first round of PCR, 50 μΐ of reaction volume contaîning the known concentration of components are prepared in two PCR tubes. In each of the tubes, dNTP, iProof buffer (BIORAD), iProof DNA polymerase (BIO-RAD), primers and DNA template are mixed and added up to 50 μΐ by ddl^O. The DNA template used in the reaction is a pET3a vector contaîning the gene jZ'' of ADI from Mycoplasma arginini with a removal of an internai Ndel site mutation without altering the protein sequence of the ADI gene.
[0052] The two reaction tubes contain the primer mixtures of (A) 10 pmol hisABDNde-F (SEQ ID NO: 13), 0.5 pmol ABDnn-Rl (SEQ ID NO: 14) and 10 pmol ABDn-R2 (SEQ ID NO: 15); and (B) 10 pmol ADIn-F (SEQ ID NO: 16) and 10 pmol ADIBam-R (SEQ ID NO: 17), respectively.
[0053] The PCR program is set according to the recommended steps in the manual with an annealing and extension température (time) at 50 °C (20 s) and 72 °C (40 s), respectively. The two products generated by PCR with the size of 237 bp and 1278 bp. The products are extracted and applied as template for the next round of PCR.
[0054] In the second overlapping step, the reaction mixture is prepared in a similar way to the first round except the template used was the mixture of 1 pmol of the 237 bp PCR product and 1 pmol of the 1278 bp PCR product from the first round PCR. Primers used are changed to 10 pmol hisABDNde-F (SEQ ID NO: 13) and 10 pmol ADIBam-R (SEQ ID NO: 17).
[0055] The annealing and extension température (time) are 50 °C (20 s) and 72 °C (60 s), respectively. A PCR product with the size of 1484 bp is generated from the reaction. The PCR product is purified and digested with Ndel and BamHI and then ligated into the pre-digested pET3a plasmid. The ligated product is then transformed into E. coli BL21 (DE3) for the production of recombinant protein.
[0056] Example 2C [0057] Cloning of His-ABD-PolyN-bcADI [0058] The construction of His-ABD-PolyN-bcADI (SEQ ID NO: 41, in FIG. 3F) is done by two steps of overlapping PCR, the PCR fragment obtained from the last step is inserted into the vector pET3a between the Ndel and BamHI sites. The gene map, nucléotide sequence and amino acid sequence of His-ABD-PolyN-bcADI are shown in FIG. 7.
Primers involved in construction of His-ABD-PolyN-bcADI:
hisABDNde-F2 forwardprimer (SEQ ID NO: 18):
5' -GGAGATATACATATGCATCATCACCATCACCATGATGAAGCCGTGGATG-3' bcABDnn-Rl reverse primer (SEQ ID NO: 19):
’ -TTGTTATTATTGTTGTTACTACCCGAAGGTAATGCAGCTAAAATTTCATC- 3 ’ bcABDn-R2 reverse primer (SEQ ID NO: 20):
' -TTTACCGCCGCTACCATTGTTATTATTGTTGTTACTACCCGA-3 ' bcADln-Fforwardprimer (SEQ ID NO: 21):
' -AATAATAACAATGGTAGCGGCGGTAAACATCCGATACATGTTACTTCAGA- 3 ' bcADIBam-R reverse primer (SEQ ID NO: 22):
' -TAGATCAATGGATCCCTAAATATCTTTACGAACAATTGGC ATAC- 3 ' [0059] In the first round of PCR, 50 μΐ of reaction volume containing the known concentration of components are prepared in two PCR tubes. In each of the tubes, dNTP, iProof buffer (BIORAD), iProof DNA polymerase (BIO-RAD), primers and DNA template are mixed and added up to 50 μΐ by ddHîO. The DNA template used in the reaction is a pET3a vector containing the gene of ADI from Bacillius cereus with a removal of an internai Ndel site mutation without altering the protein sequence of the ADI gene.
[0060] The two reaction tubes contain the primer mixtures of (A) 10 pmol hisABDNde-F2 (SEQ ID NO: 18), 0.5 pmol bcABDnn-Rl (SEQ ID NO: 19) and 10 pmol bcABDn-R2 (SEQ ID NO: 20); and (B) 10 pmol bcADIn-F (SEQ ID NO: 21) and 10 pmol bcADIBam-R (SEQ ID NO: 22), respectively. The PCR program is set according to the recommended steps in the manual with an annealing and extension température (time) at 50 °C (20 s) and 72 °C (40 s), respectively. The two products are generated by PCR with the size of 237 bp and 1250 bp. The products are extracted and applied as template for the next round of PCR.
[0061] In the second overlapping step, the reaction mixture is prepared in a similar way to the first round except the template used is the mixture of 1 pmol of the 237 bp PCR product and 1 pmol of the 1250 bp PCR product from the first round PCR. Primers used are changed to 10 pmol hisABDNde-F2 (SEQ ID NO: 18) and 10 pmol bcADIBam-R (SEQ ID NO: 22).
[0062] The annealing and extension température (time) are 50 °C (20 s) and 72 °C (60 s), respectively. A PCR product with the size of 1512 bp is generated from the reaction. The PCR Y product is purified and digested with Ndel and BamHl and then ligated into the pre-digested pET3a plasmid. The ligated product is then transformed into E. coli BL2l (DE3) for the production of recombinant protein.
[0063] Example 3 [0064] Expression and purification of the AAD fusion protein [0065] For preparing the seed culture, the strain E. coli BL2l(DE3) carrying the plasmid encoding the AAD fusion protein (FIG. 5) is eultured in 5 ml of 2xTY medium, 30°C, 250 rpm, ovemight. The ovemight seed culture (2.5 ml) is added to 250 ml of 2xTY, 37°C, 250 rpm, 2.5 h (until ODéoo ~ 0.6-0.7). When the ODôoo reached, IPTG is added to the culture (0.2 mM final concentration). The growth is continued for 22 more hours at 20°C and then the cells are collected by centrifugation. The cell pellet is resuspended in 25 ml of 10 mM sodium phosphate buffer, pH 7.4. The cells are lysed by sonication. The soluble portion is collected after centrifugation. The fusion protein (containing a His tag) is then purified by nickel affinity chromatography. TABLE 2 shows that cultivation température is an important factor in affecting the solubility of AAD fusion protein (amino acid sequence is shown in SEQ ID NO: 40, FIG. 3E) obtained from the expression host.
[0066] For isolating the soluble fraction of AAD fusion protein, the cell pellet is resuspended in 25 ml of 10 mM sodium phosphate buffer, pH 7.4. The cells are lysed by sonication. The soluble portion is collected after centrifugation. The AAD fùsion protein (contains a His tag) is then purified by nickel affinity chromatography.
[0067] For isolating the insoluble fraction of AAD fusion protein, the cell pellet is resuspended in 25 ml of 20 mM Tris-HCl, pH 7.4, 1% Triton X-100. The cells are lysed by sonication. The insoluble portion (inclusion bodies) is collected by centrifugation. The protein is unfolded by resuspending in 10 ml of 20 mM Tris-HCl, pH 7.4, 6 M Guanidine HCl, and vortexed until it becomes soluble. The protein is refolded by adding the unfolded protein solution drop by drop into a fast stirring solution of 100 ml of 20 mM Sodium phosphate buffer, pH 7.4. The insoluble materials are removed by centrifugation. Salting out of the protein is performed by adding solid ammonium sulphate powder into the supernatant to achieve 70% saturation. The insoluble portion is collected by centrifugation and it is resuspended in 10 ml of 20 mM sodium phosphate buffer. The AAD fusion protein (contains a His tag) is then purified by nickel affinity chromatography.
[0068] TABLE 2
| AAD | 1 | 2 | 3 |
| Cultivation température (°C) | 30 | 20 | 37 |
| Yield (mg) / 250ml culture | -0.66 | -12.0 | -7.0 |
| solubility | 50% soluble | 90% soluble | 90% inclusion body |
| IC50 (gg/ml) on A375 cells | 0.10 | 0.68 | 0.23 |
[0069] Example 4 [0070] Enzyme activity assay and Enzyme kinetics for AAD fusion protein [0071] To détermine the enzyme activity for wild-type ADI and AAD fusion protein in the présent invention, the diacetyl monoxime (DAM) - thiosemicarbazide (TSC) assay for citrulline détection is used. The reaction is shown below.
[0072] L-Arginine or aad fusion protein > L_Citrulline + Ammonia [0073] This assay is run by adding sample to a color reagent, which is made by mixing acidic ferrie chloride solution with DAM-TSC solution. Briefly, enzyme is incubated with 20 mM arginine, 10 mM sodium phosphate pH 7.4 for 5 min at 37°C. The reaction mixture is heated at 100°C for 5 min to develop the color and read at 540 nm (light path = 1 cm). A standard curve is constructed using various concentrations of citrulline. One unit of the ADI native enzyme is the amount of enzyme activity that converts 1 pmol of arginine to 1 pmol of citrulline per minute at 37°C under the assay conditions. The spécifie activities of wild-type ADI and AAD fusion protein in the présent invention are 8.4 and 9.2 U/mg (at pH 7.4, physiological pH) respectively. The spécifie activities for wild-type ADI and AAD fusion protein at different pH range (from pH 5.5 to 9.5) are also determined, and the optimum pH is at 6.5. Therefore, the results indicate that AAD fusion protein depletes arginine efficiently, as the fusion with albumin-binding protein does not affect enzyme activity of ADI. vkA [0074] The Michaelis constant Km is the substrate concentration at which the reaction rate is at half-maximum, and is an inverse measure of the substrate's affinity for the enzyme. A small Km indicates high affinity for the substrate, and it means that the rate will approach the maximum reaction rate more quickly. For détermination of the enzyme kinetics or Km value, the activity of wild-type ADI and AAD fusion protein are measured under different concentration of substrate arginine (2000 μΜ, 1000 μΜ, 500 μΜ, 250 μΜ, 125 μΜ, 62.5 μΜ) at ρΗ 7.4. The measured Km values of the AAD fusion protein shown in FIG. 3E (SEQ ID NO: 40, ADI protein is originated from Mycoplasma arginini) and AAD fusion protein shown in FIG. 3F (SEQ ID NO: 41, ADI protein is originated from Bacillus cereus) are 0.0041 mM and 0.132 mM respectively. The results suggest that the fusion to ABD did not affect the binding affinity of the different AAD fusion proteins to arginine.
[0075] Example 5 [0076] Cell prolifération assay and in vitro effïcacy of AAD fusion protein on cancer cell lines [0077] Culture medium DMEM is used to grow the human melanoma A375 & SK-mel-28, human pancreatic cancer Panel and human cervical cancer C-33A cell lines. The EMEM medium is used to culture the SK-hep 1 liver cancer and C-33A cervical cancer cell line. Cancer cells (2-5 X 103) in 100 μΐ culture medium are seeded to the wells of 96-well plates and incubated for 24 h. The culture medium is replaced with medium containing different concentrations of AAD fusion protein. The plates are incubated for an additional 3 days at 37°C in an atmosphère of 95% air/5% CO2. MTT assay is performed to estimate the number of viable cells in the culture according to manufacturer’s instructions. The amount of enzyme needed to achieve 50% inhibition of cell growth is defined as IC50.
[0078] As shown in TABLE 1 and FIG. 9, the results indicate that AAD fusion protein depletes arginine efficiently and inhibits the growth of various types of human cancer cell lines in in vitro tissue culture studies. For example, human melanoma, human colon carcinoma, human pancreatic cancer, human liver cancer and human cervical cancer, ail hâve low values of IC50 (see TABLE 1), as these cancer types are ail inhibited by AAD fusion protein readily. As predicted, AAD fusion protein would inhibit ail cancer types that are arginine-dependent (for example, the ASS-negative cancers). vY [0079] Example 6 [0080] In vivo half-life détermination of AAD fusion protein [0081] Balb/c mice (5-7 weeks) are used in this study and they are allowed to acclimatize for a week before the experiment. Mice (n=3) are separated into four groups and injected with 0, 100, 500 or 1000 pg of AAD fusion protein (SEQ ID NO: 40, FIG. 3E) in 100 μΐ PBS intraperitoneally, respectively. Blood of each mouse is collected at 0 h and Day 1-7. Sera are obtained after centrifugation. The sera are then deproteinised and analyzed by amino acid analyzer for arginine.
[0082] As shown in FIG. 11, AAD fusion protein (SEQ ID NO: 40, FIG. 3E), even at the lowest dosage of 100 pg, depletes plasma arginine efficiently at Day 1, 3 and 5, suggesting that AAD can deplete arginine in vivo efficiently for at least 5 days. The arginine level retums to normal gradually at Day 6 and Day 7 in ail treatment groups.
[0083] Example 7 [0084] In vivo efficacy of AAD fusion protein on cancer cell xenografts [0085] Nude balb/c mice (5-7 weeks) are used in this study and they are allowed to acclimatize for a week before the experiment. Mice are inoculated subcutaneously with 2x106 cancer cells in 100 μΐ of fresh culture medium. Ten days later, the mice are randomly separated into control and treatment group. Control group receives 100 μΐ PBS and treatment group receives 100 μΐ AAD fusion protein intraperitoneally weekly. Tumor size is measured by caliper and tumor volume is calculated using formula: (length x width2)/2. Blood draw are obtained at Day 5 after each treatment for plasma measurement of arginine.
Claims (28)
1. An albumin-binding arginine deiminase fusion protein comprising a first portion comprising one or two components selected from an albumin-binding domain, an albumin-binding peptide or an albumin-binding protein(s) fused to a second portion comprising arginine deiminase to form the albumin-binding arginine deiminase fusion protein, and one or more linker molécules; the first portion being positioned far from active site of the second portion by said linker molécule such that the albumin-binding arginine deiminase fusion protein retains the activity of arginine deiminase and binds sérum albumin with neither function of one portion of the fusion protein being interfered with by the other portion of the fusion protein, wherein the albuminbinding arginine deiminase fusion protein comprises an amino acid sequence selected from SEQ ID NO: 36, 37, 38, 39, 40, or 4L
2. An albumin-binding arginine deiminase fusion protein according to claim l wherein the two components are the same.
3. An albumin-binding arginine deiminase fusion protein according to claim l wherein the two components are different.
4. An albumin-binding arginine deiminase fusion protein according to claim l wherein the albumin-binding domain is SEQ ID NO. 46, 47, 48, 49 or an active portion thereof.
5. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the albumin binding peptide is SEQ ID NO. 46, 47, 48, 49 or an active portion thereof.
6. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the albumin binding protein is SEQ ID NO. 46, 47, 48, 49 or an active portion thereof.
7. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the linker molécule includes a sequence selected from SEQ ID NO. 50, 51, 52, 53, or serine-glycineserine (SGS) amino acid sequence.
8. An albumin-binding arginine deiminase fusion protein according to claim l further comprising at least one of Poly-N or a His tag.
9. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the fusion includes a remaining portion of an intein-mediated protein ligation between the first portion and the second portion.
10. An albumin-binding arginine deiminase fusion protein according to claim 9 wherein the intein-mediated protein includes a chitin binding domain.
11. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the arginine deiminase is selected from arginine deiminase produced from a Mycoplasma, Lactococcus, Pseudomonas, Steptococcus, Escherichia, Mycobacterium or Bacillus microorganism.
12. An albumin-binding arginine deiminase fusion protein according to claim 11 wherein the arginine deiminase is produced from Mycoplasma arginini, Lactococcus lactis, Bacillus licheniforrais, Bacillus cereus, Mycoplasma arthritidis, Mycoplasma hominis, Streptococcus pyogenes, Streptococcus pneumonia, Streptococcus pneumoniae, Mycobacterium tuberculosis, Pseudomonas plecoglossicida, Pseudomonas putida, Pseudomonas aeruginosa or a combination thereof.
13. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the fusion protein is formed by reacting the arginine deiminase having a N-terminal cysteine residue with a reactive thioester at C-terminus of the albumin-binding domain so that the arginine deiminase and the albumin-binding domain are linked by a covalent bond.
14. An albumin-binding arginine deiminase fusion protein according to claim 1 wherein the fusion protein is formed by reacting the albumin-binding domain having a N-terminal cysteine residue with a reactive thioester at C-terminus of the arginine deiminase so that the arginine deiminase and the albumin-binding domain are linked by a covalent bond. Λ/-
15. An albumin-binding arginine deiminase fusion protein according to claim l wherein the fusion protein is formed by using SEQ ID NOS. 42 and 43 and by reacting the arginine deiminase having a N-terminal cysteine residue with a reactive thioester at C-terminus of the albumin-binding domain so that the arginine deiminase and the albumin-binding domain are linked by a covalent bond.
16. Use of the albumin-binding arginine deiminase fusion protein according to any one of claims 1 to 15 in préparation of a médicament for treating a cancer in a patient comprising administering a clinically effective amount of the fusion protein to the patient to reduce the availability of circulating arginine.
17. The use according to claim 16 wherein the cancer is pancreatic cancer, leukemia, head and neck cancer, colorectal cancer, lung cancer, breast cancer, liver cancer, nasopharyngeal cancer, esophageal cancer, prostate cancer, stomach cancer or brain cancer.
18. Use of the albumin-binding arginine deiminase fusion protein according to any one of claims 1 to 15 in préparation of a médicament for treating arginine-dependent diseases in a patient comprising administering a clinically effective amount of the fusion protein to the patient to reduce the availability of circulating arginine.
19. A method of making the albumin-binding arginine deiminase fusion protein of claim 1 comprising constructing a fusion gene coding for the albumin-binding arginine deiminase fusion protein, inserting the fusion gene into a vector, inserting the vector into a host organism and expressing a protein including the albumin-binding arginine deiminase fusion protein of claim 1.
20. The method of making the albumin-binding arginine deiminase fusion protein according to claim 19 further comprising purifying the fusion protein.
21. The method of making the albumin-binding arginine deiminase fusion protein according to claim 20 wherein the purifying is performed by chromatography.
22. The method of making the albumin-binding arginine deiminase fusion protein according to claim 20 wherein the purifying is performed from soluble fractions of crude proteins.
23. The method of making the albumin-binding arginine deiminase fusion protein according to claim 20 wherein the purifying is performed from insoluble fractions of crude proteins.
24. A method of making the albumin-binding deiminase fusion protein of claim l by intein mediated protein ligation between the albumin-binding domain, albumin-binding peptide or albumin-binding protein(s) and the second portion comprising arginine deiminase.
25. A pharmaceutical composition comprising the albumin-binding arginine deiminase fusion protein of claim l in a pharmaceutically-acceptable carrier.
26. The pharmaceutical composition of claim 25 wherein the composition has a pH in a range of
5.5 to 9.5.
27. The pharmaceutical composition of claim 25 wherein the composition has a pH of 7.4.
28. The pharmaceutical composition of claim 25 wherein the composition has a pH of 6.5. tfj'
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US61/773214 | 2013-03-06 | ||
| US14/197236 | 2014-03-05 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| OA17472A true OA17472A (en) | 2016-12-30 |
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