WO1989012109A1 - Gene therapy using gene fusions for genetic or acquired disorders - Google Patents

Gene therapy using gene fusions for genetic or acquired disorders Download PDF

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Publication number
WO1989012109A1
WO1989012109A1 PCT/US1989/002450 US8902450W WO8912109A1 WO 1989012109 A1 WO1989012109 A1 WO 1989012109A1 US 8902450 W US8902450 W US 8902450W WO 8912109 A1 WO8912109 A1 WO 8912109A1
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gene
cells
ada
transfected
coding sequence
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PCT/US1989/002450
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French (fr)
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Ira H. Pastan
Michael M. Gottesman
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The United States Of America, As Represented By Th
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Priority to EP89907509A priority Critical patent/EP0420911B1/en
Priority to DE68927104T priority patent/DE68927104T2/en
Publication of WO1989012109A1 publication Critical patent/WO1989012109A1/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/11DNA or RNA fragments; Modified forms thereof; Non-coding nucleic acids having a biological activity
    • C12N15/62DNA sequences coding for fusion proteins
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/435Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/63Introduction of foreign genetic material using vectors; Vectors; Use of hosts therefor; Regulation of expression
    • C12N15/79Vectors or expression systems specially adapted for eukaryotic hosts
    • C12N15/85Vectors or expression systems specially adapted for eukaryotic hosts for animal cells
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    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/14Hydrolases (3)
    • C12N9/78Hydrolases (3) acting on carbon to nitrogen bonds other than peptide bonds (3.5)
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K48/00Medicinal preparations containing genetic material which is inserted into cells of the living body to treat genetic diseases; Gene therapy
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    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K2319/00Fusion polypeptide

Definitions

  • the present invention is related generally to the construction of fusion genes. More particularly, the present invention is related to the construction of a fusion gene comprising a coding sequence for a selectable marker linked by fusion to another coding sequence, the product of which is desired to be expressed in recipient cells. BACKGROUND OF THE INVENTION
  • an object of the present invention to provide an efficient and reproducibly reliable method of introducing genes into animal or human cells to treat genetic or acquired disorders or defects caused by enzyme deficiency.
  • ADA adenosine deaminase
  • Figures 1 A,B,C schematically represent the construction of a re roviral expression vector pHaMDRlADA which encodes a human P-glycoprotein-adenosine deaminase chimeric protein (it is noted that in Figures 1 A,B,C, MDRADA represents MDR1ADA) ;
  • Figure 2 shows Southern analysis of genomic DNAs of transfected KB cells.
  • Genomic DNA was digested with EcoRI, separated on a 0 .1% aqueous gel, transferred to nitrocellulose, and hybridized to a MDR 1-specific probe (pHDR5A) .
  • Panel A shows individually picked cell clones.
  • Lane 1 KB-A, mock-transfected, grown at 6 ng/ml colchicine.
  • Lane 2 KB-MDR1A, pHaMDRl transfected, grown at 6 ng/ml colchicine. Lanes 3 and 4: KB-MDR1ADA-I, pHAMDRIA transfected, grown at 6 ng/ml (3) and 12 ng/ml (4) colchicine. Panel B shows pooled cell populations.
  • Lanes 1 and 2 pHaMDRl transfected, grown at 6 ng/ml (1) and 24 ng/ml (2) colchicine. Lanes 3 and 4: pHaMDRlADA transfected, grown at 6 ng/ml (3) and 24 ng/ml (4) colchicine.
  • Lane 5 non-transfected parental KB-3-1 cell line, colchicine-sensitive
  • FIG. 3 shows the results of immunoprecipitations of cell lysates. Cultures were labeled with S-methionine for 16 hours. Cell lysates were immunoprecipitated using anti-P-glycoprotein antiserum (lanes 1 - 7) or preimmune serum (lanes 8 - 12) and protein A sepharose. Fluoro- gra s of the resulting SDS-polyacrylamide gels are shown. Arrows indicate the 170 kD P-glycoprotein (MDRl gene product) and the 210 kD P-glycoprotein-ADA fusion protein (MDR1ADA) . Lane 1: drug-sensitive KB-3-1 control cell line, labelled and immunoprecipitated in parallel.
  • MDRl gene product anti-P-glycoprotein antiserum
  • MDR1ADA preimmune serum
  • Lane 2 vinblastine-selected KB-V1 control cell line.
  • Lanes 3 and 8 pHaMDRl transfected KB cell population grown at 24 ng/ml colchicine.
  • Lanes 4, 5, 9, 10 pHaMDRlADA transfected KB cell popu ⁇ lations grown at 6 ng/ml (4 and 9) and 24 ng/ml (5 and 10) colchicine.
  • Lanes 6, 7, 11, 12 pHaMDRlADA transfected clone KB- MDR1ADA-I grown at 6 ng/ml (6 and 11) and 12 ng/ml (7 and 12) colchicine;
  • Figure 4 shows killing curves for control and pHaMDRlADA cell lines.
  • 300 cells were plated in a 60 mm dish containing 5 ml culture medium supplemented with 1.1 M adenosine, 1.0 mM uridine, 0.05 mM alanosine and variable amounts of 2'-deoxycoformycin. After a grown period of ten days at 37°C and 7% C0 2 , cells were stained with methylene blue and colonies were counted.
  • Figure 4A shows individual clones selected at 6 ng/ml colchicine.
  • Figure 4B shows collected cell populations grown at 16 ng/ml (circles) and 24 ng/ml (triangles) colchicine. Dashed lines and open symbols (o,A) represent pHaMDRl transfected cells, and solid lines and closed symbols (#,_A) are pHaMDRlADA transfected cells.
  • a chimeric gene comprising a selectable marker gene fused, linked or associated in tandem or otherwise with another gene, the expression of which is desired in the recipient cell.
  • fusion gene is defined herein as a DNA segment in which two or more genes are fused result ⁇ ing in a single open reading frame for coding two or more proteins that as a result of this fusion are joined by one or more peptide bonds.
  • ADA adenosine deaminase
  • E.C. 3.5.4.4 adenosine aminohydrolase
  • This disease is invariably fatal unless effectively treated.
  • ADA catalyzes the irre ⁇ versible deamination of adenosine and deoxyadenosine to inosine and deoxyinosine, respectively. Most ADA deficient patients produce a catalytically defective enzyme.
  • the cytotoxic ADA substrates, adenosine and deoxyadenosine, as well as their meta ⁇ bolites, particularly deoxyadenosine 5'-triphosphate, are accumulated intracellularly. This leads to the specific destruction of T-lymphocytes and, to a lesser extent, B- lymphocytes, with consequent severe immunological dysfunction.
  • One of the therapies available for ADA deficiency is bone marrow transplantation from a normal histocompatible donor. However, for many patients, there are no suitable bone marrow donors.
  • Alternative forms of treatment such as enzyme replacement by repeated erythro- cyte transfusions or repeated intramuscular injection of polyethylene glycol-modified bovine ADA are also avail ⁇ able, but these can lead to severe complications during long-term therapy.
  • Retrovirus-mediated transfer and expression of the ADA gene has been reported in a variety of human T and B lymphocyte cell lines, diploid human skin fibro- blasts, as well as in murine NIH 3T3 and lymphoid cells. More recently, a Moloney murine leukemia virus- based recombinant retrovirus has been used to express ADA in " murine hematopoietic stem cells (Lim, et al, 1987, Mol. Cell. Biol. 7, 3459). Such retroviral constructs, however, contained no dominant marker gene which would allow selection and thus efficient enrichment of ADA expressing cells.
  • a dominant selectable marker gene e.g., neo- mycin phosphotransferase, hypoxanthine phosphoribosyl transferase or dihydrofolate reductase
  • ADA _in_ vitro but failed to express ADA _in_ vivo, i.e., in stem cells of experimental animals (Williams, et al, 1986, Proc. Natl. Acad. Sci. USA 83, 2566; Mclvor, et al, 1987, Mol. Cell Biol. _7_ 838; Zwiebel, et al, 1986, Blood 68, 307).
  • the present invention is the first to directly link the expression of the selectable marker gene (e.g., MDRl) to the expression of the ADA gene by creating a fusion MDRl-ADA gene which directs the synthesis of a bifunctional chimeric protein in the recipient cells of the host simultaneously conferring multidrug resistance and efficient ADA activity.
  • MDRl selectable marker gene
  • a 1.1 kb Asp 718 - Hhal fragment encoding a carboxylterminal region of the MDRl gene product P-glycoprotein (ranging from Val-926 to Lys-1278) was isolated from plasmid pMDRl 104-2.
  • the adapter encodes the two carboxyl terminal amino acid residues of P-glycoprotein.
  • MDRl and ADA genes were fused at the newly created single Sail site located at the 3' end of the P-glycoprotein coding region (pAHSH-1) and at the 5' end of the ADA structural gene (pESE-13). Concomitantly, the fusion gene was inserted into the pGEM-2 vector (Promega) . To this end a 2.9 kb EcoRI - Sad fragment (containing pGEM- 2 plasmid sequences) and a 2.9 kb Sacl - Asp 718 fragment encoding the aminoterinal part of P-glycoprotein) were isolated from pMDRl 2000XS (Ueda, et al, 1987, Acad. Sci.
  • pMDRADAS was partially cut with EcoRI to linearize the molecule, filled in using the Klenow fragment of DNA polymerase I, and ligated with non-phosphorylated Xhol - linkers.
  • the fusion gene was then excised from pMDRADA XS as a 5.45 kb SacII-XhoI fragment and ligated with the 10.7 kb SacII - Xhol frag ⁇ ment derived from pHaMDRl and containing the retroviral vector sequences.
  • the final construct is designated pHaMDRlADA and carries the human MDR1-ADA fusion gene between the 5' and 3' LTRs of Harvey murine sarcoma virus .
  • the MDR1-ADA fusion gene is the only functional eucaryotic gene in this vector and encodes a chimeric protein with an expected Mr of 210 kD. It consists of P- glycoprotein which is connected at the carboxyl-terminal amino acid Gln-1280 to the initiator-methionine of ADA by the tripeptide Gly-Arg-Pro.
  • a deposit of the pHaMDRlADA has been made at the American Type Culture Collection (ATCC), 12301 Parklawn Drive, Rockville, Maryland, U.S.A. on May 18, 1988 under the accession number 67699.
  • the deposit shall be viably maintained, replacing it if it becomes non- viable, for a period of 30 years from the date of the deposit, or for 5 years from the last date of request for a sample of the deposit, whichever is longer, and made available to the public without restriction in accordance with the provisions of the law.
  • the Commissioner of Patents and Trademarks, upon request, shall have access to the deposit.
  • Drug-sensitive human KB-3-1 cells were trans- fected with pHaMDRlADA DNA. Negative control cells received no DNA whereas positive control cells were transfected with pHaMDRl which represents full-length human MDRl DNA in the same Harvey murine sarcoma virus expression vector (see Fig. 1C) . This plasmid represents full-length human MDRl cDNA in the same Harvey murine sarcoma virus expression vector (see Fig. 10). This plasmid confers the full phenotype of multidrug resistance to a variety of mouse and human cell lines as mentioned in application S/N 07/062,583. Plasmid DNA used for cell trans ections was isolated by standard alkaline lysis followed by cesium chloride gradient centrifugation.
  • Drug-sensitive human KB-3-1 cells were transfected by the standard calcium phosphate precipitation method. 10 ⁇ g of plasmid DNA were used to transfeet 5 x lOg cells per 10 cm dish. Sixteen hours after transfection cells were washed twice and 24 hrs later they were split 1:5 into medium contain ⁇ ing the selective drug colchicine at a concentration of 6 ng/ml. After a growth period of ten days, two dishes of cells were stained with 0.5% (w/v) methylene blue in 10% (v/v) ethanol and individual colonies counted. The data presented in Table I show the relative transfection efficiencies of plasmids pHaMDRlADA and pHaMDRl.
  • genomic DNA was isolated from transfected and control KB cells by standard procedures (Chen, et al, 1986, Cell 47, 381). Equal amounts of genomic DNA were analyzed by restriction endonuclease digestion using EcoRI, followed by agarose gel electrophoresis, Southern transfer and hybridization to a MDRl-specific probe. A 3 kb fragment of pHaMDRl transfected cells and a 4 kb frag ⁇ ment of pHaMDRlADA transfected cells were expected to give rise to a hybridization signal. Indeed, as shown in Fig.
  • pHaMDRl pHaMDRl transfected cells
  • the immunoprecipitated protein from pHaMDRlADA transfected cells has a higher Mr which is in good agreement with the calculated Mr of 210 kD of the MDRIADA fusion protein.
  • the levels of the chimeric protein seem to increase along with the colchicine resistance of the cells.
  • dCF 2'-deoxycoformycin
  • dCF Under conditions where ADA activity is required (such as in the presence of cyto- toxic amounts of adenosine) dCF can be used to estimate intracellular ADA levels.
  • the amounts of dCF necessary to inhibit cell growth correlated with the amounts of functional ADA.
  • Killing curves were performed by growing a constant number of dels (initially 300 cells were plated in a 60 mm dish) in culture medium supplemented with 1.1 mM adenosine, 1.0 mM uridine, 0.05 mM alanosine and variable amounts of dCF.
  • Alanosine was added to block de novo AMP synthesis and uridine to alleviate the block in UMP synthesis caused by the high adenosine con ⁇ centration.
  • MDRl is only an example of a selectable marker gene.
  • any selectable marker gene can be similarly employed to produce a chimeric gene.
  • the linked gene which is introduced by fusion with the selectable marker gene may be altered (for example by mutation) and the effect of such alternations determined in intact living cells. Such manipulations allow the determination of the effect of the alternation and the verification that the mutant gene is in fact introduced and expressed as a poly- peptide.
  • the human MDRl gene linked to the ADA gene could be used to introduce mutant ADA proteins into cells for determining the function of different parts of the ADA molecule.
  • ADA is also a selectable marker gene in tissue culture cells via the deoxycoformycin selection
  • ADA can be used as the select ⁇ able marker to introduce an altered MDRl gene into cells thereby allowing the determination of the function of various modifications of the MDRl protein.
  • pHaMDRlADA (5 ⁇ g) 75 pHaMDRlADA (10 ⁇ g) 125 pHaMDRl (5 ⁇ g) 330 pHaMDRl (10 ⁇ g) 550 no DNA 5
  • KB-3-1 cells were plated at 5 x 10 5 cells/10 cm dish and transfected the next day with the indicated DNAs. After 2 days cells were trypsinized and split 1:5 into culture medium supplemented with 6 ng/ml colchicine. Ten days later colonies were stained with methylene blue and counted.
  • KB-A, KB-MDR1, KB-MDRIADA G, and KB-MDRIADA I are indi ⁇ vidual clones.
  • ADA assays were performed according to Yeung, C.-y., Ingolia, D. E., Bobonis, C, Dunbar, B. S., Riser, M. E., Siciliano, M. J., and Kellems, R. E. (1983) J. Biol. Che . 258, 8338-8345.
  • ADA activity in the membrane or cytosolic fraction cells were collected by scraping into PBS, washed twice with PBS, resuspended in hypotonic lysis buffer (10 mM Tris HCl pH 7.5, 10 mM NaCl, 1 mM MgCl 2 ) at a concentration of 2 x 10 7 cells/ml and incubated in an ice-bath for 15 min.
  • hypotonic lysis buffer (10 mM Tris HCl pH 7.5, 10 mM NaCl, 1 mM MgCl 2 ) at a concentration of 2 x 10 7 cells/ml and incubated in an ice-bath for 15 min.
  • the swollen cells were disrupted with 20 strokes in a tightly fitting Dounce homogenizer and the nuclei removed by centrifuga- tion at 400 xg for 10 min at 4°C.
  • the pellet obtained by subsequent centrifugation at 30,000 xg for 30 min at 4°C was used as the crude

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Abstract

Gene therapy utilizing an MDR1 linked fusion coding sequence has been disclosed. ADA activity has been introduced into cells using MDR1 linked fusion gene.

Description

GENE THERAPY USING GENE FUSIONS FOR GENETIC OR ACQUIRED DISORDERS
The present invention is related generally to the construction of fusion genes. More particularly, the present invention is related to the construction of a fusion gene comprising a coding sequence for a selectable marker linked by fusion to another coding sequence, the product of which is desired to be expressed in recipient cells. BACKGROUND OF THE INVENTION
Development in recombinant DNA technology and the need to treat genetic disorders has led to the con¬ cept of "gene therapy." To this end, methods have been developed for the introduction and expression of foreign genes into somatic cells. However, a fusion gene per se as described herein has not heretofore been produced and the expression of the delivered gene in the recipient cell in accordance with the prevalent methods is usually found to be either very low or quite variable. SUMMARY OF THE INVENTION
It is, therefore, an object of the present invention to provide an efficient and reproducibly reliable method of introducing genes into animal or human cells to treat genetic or acquired disorders or defects caused by enzyme deficiency.
It is a further object of the present invention to provide a selectable marker-linked fusion gene for transfer and expression of a desired gene in human cells without introducing a non-human antigen. It is another object of the present invention to provide gene therapy for the treatment of severe com¬ bined immunodeficiency caused by adenosine deaminase (ADA) deficiency.
Other objects and advantages will become evi- dent from the following detailed description of the invention.
BRIEF DESCRIPTION OF THE DRAWINGS These and other objects, features and many of the attendant advantages of the invention will be better understood upon a reading of the following detailed description when considered in connection with the accompanying drawings wherein: Figures 1 A,B,C schematically represent the construction of a re roviral expression vector pHaMDRlADA which encodes a human P-glycoprotein-adenosine deaminase chimeric protein (it is noted that in Figures 1 A,B,C, MDRADA represents MDR1ADA) ; Figure 2 shows Southern analysis of genomic DNAs of transfected KB cells. Genomic DNA was digested with EcoRI, separated on a 0 .1% aqueous gel, transferred to nitrocellulose, and hybridized to a MDR 1-specific probe (pHDR5A) . Panel A shows individually picked cell clones. Lane 1: KB-A, mock-transfected, grown at 6 ng/ml colchicine.
Lane 2: KB-MDR1A, pHaMDRl transfected, grown at 6 ng/ml colchicine. Lanes 3 and 4: KB-MDR1ADA-I, pHAMDRIA transfected, grown at 6 ng/ml (3) and 12 ng/ml (4) colchicine. Panel B shows pooled cell populations.
Lanes 1 and 2: pHaMDRl transfected, grown at 6 ng/ml (1) and 24 ng/ml (2) colchicine. Lanes 3 and 4: pHaMDRlADA transfected, grown at 6 ng/ml (3) and 24 ng/ml (4) colchicine.
Lane 5: non-transfected parental KB-3-1 cell line, colchicine-sensitive;
Figure 3 shows the results of immunoprecipitations of cell lysates. Cultures were labeled with S-methionine for 16 hours. Cell lysates were immunoprecipitated using anti-P-glycoprotein antiserum (lanes 1 - 7) or preimmune serum (lanes 8 - 12) and protein A sepharose. Fluoro- gra s of the resulting SDS-polyacrylamide gels are shown. Arrows indicate the 170 kD P-glycoprotein (MDRl gene product) and the 210 kD P-glycoprotein-ADA fusion protein (MDR1ADA) . Lane 1: drug-sensitive KB-3-1 control cell line, labelled and immunoprecipitated in parallel. Lane 2: vinblastine-selected KB-V1 control cell line. Lanes 3 and 8: pHaMDRl transfected KB cell population grown at 24 ng/ml colchicine. Lanes 4, 5, 9, 10: pHaMDRlADA transfected KB cell popu¬ lations grown at 6 ng/ml (4 and 9) and 24 ng/ml (5 and 10) colchicine.
Lanes 6, 7, 11, 12: pHaMDRlADA transfected clone KB- MDR1ADA-I grown at 6 ng/ml (6 and 11) and 12 ng/ml (7 and 12) colchicine; and
Figure 4 shows killing curves for control and pHaMDRlADA cell lines. In each experiment 300 cells were plated in a 60 mm dish containing 5 ml culture medium supplemented with 1.1 M adenosine, 1.0 mM uridine, 0.05 mM alanosine and variable amounts of 2'-deoxycoformycin. After a grown period of ten days at 37°C and 7% C02, cells were stained with methylene blue and colonies were counted. Figure 4A shows individual clones selected at 6 ng/ml colchicine. (A) KB-A, mock-transfected clones.
(o) KB-MDR-A, pHaMDRl transfected clone.
(A) KB-MDR1ADA-G, pHaMDRlADA transfected clone. -
(♦) KB-MDR1ADA-I, pHaMDRlADA transfected clone; and
Figure 4B shows collected cell populations grown at 16 ng/ml (circles) and 24 ng/ml (triangles) colchicine. Dashed lines and open symbols (o,A) represent pHaMDRl transfected cells, and solid lines and closed symbols (#,_A) are pHaMDRlADA transfected cells.
DETAILED DESCRIPTION OF THE INVENTION The above and various other objects and advantages of the present invention are achieved by a chimeric gene comprising a selectable marker gene fused, linked or associated in tandem or otherwise with another gene, the expression of which is desired in the recipient cell.
Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, the preferred methods and materials are now described. All publications mentioned hereunder are incorporated herein by reference. Unless mentioned otherwise, the techniques employed herein are standard methodologies well known to one of ordinary skill in the art.
The term "fusion gene" is defined herein as a DNA segment in which two or more genes are fused result¬ ing in a single open reading frame for coding two or more proteins that as a result of this fusion are joined by one or more peptide bonds.
The concept of "gene therapy" utilizing the gene fusion expression system of the present invention is now exemplified by the construction, transfer and reliably efficient expression of the ADA gene si ul- taneously with a selectable marker gene such as the MDRl gene, producing a bifunctional chimeric protein in the host cells.
The ADA gene was chosen for the illustrative purposes herein because adenosine deaminase (ADA; adenosine aminohydrolase: E.C. 3.5.4.4) deficiency is a genetic disorder which is associated with approximately one quarter of all cases of severe combined immuno¬ deficiency (Hirschhorn, et al, 1979, Clin. Immunol. Immunopatho1, 14:107). This disease is invariably fatal unless effectively treated. ADA catalyzes the irre¬ versible deamination of adenosine and deoxyadenosine to inosine and deoxyinosine, respectively. Most ADA deficient patients produce a catalytically defective enzyme. As a consequence, the cytotoxic ADA substrates, adenosine and deoxyadenosine, as well as their meta¬ bolites, particularly deoxyadenosine 5'-triphosphate, are accumulated intracellularly. This leads to the specific destruction of T-lymphocytes and, to a lesser extent, B- lymphocytes, with consequent severe immunological dysfunction.
One of the therapies available for ADA deficiency is bone marrow transplantation from a normal histocompatible donor. However, for many patients, there are no suitable bone marrow donors. Alternative forms of treatment such as enzyme replacement by repeated erythro- cyte transfusions or repeated intramuscular injection of polyethylene glycol-modified bovine ADA are also avail¬ able, but these can lead to severe complications during long-term therapy.
Retrovirus-mediated transfer and expression of the ADA gene has been reported in a variety of human T and B lymphocyte cell lines, diploid human skin fibro- blasts, as well as in murine NIH 3T3 and lymphoid cells. More recently, a Moloney murine leukemia virus- based recombinant retrovirus has been used to express ADA in "murine hematopoietic stem cells (Lim, et al, 1987, Mol. Cell. Biol. 7, 3459). Such retroviral constructs, however, contained no dominant marker gene which would allow selection and thus efficient enrichment of ADA expressing cells.
It is noteworthy that all recombinant retro- viral constructs made so far carry, in addition to the ADA gene, a dominant selectable marker gene (e.g., neo- mycin phosphotransferase, hypoxanthine phosphoribosyl transferase or dihydrofolate reductase) and consistently expressed ADA _in_ vitro, but failed to express ADA _in_ vivo, i.e., in stem cells of experimental animals (Williams, et al, 1986, Proc. Natl. Acad. Sci. USA 83, 2566; Mclvor, et al, 1987, Mol. Cell Biol. _7_ 838; Zwiebel, et al, 1986, Blood 68, 307).
The present invention is the first to directly link the expression of the selectable marker gene (e.g., MDRl) to the expression of the ADA gene by creating a fusion MDRl-ADA gene which directs the synthesis of a bifunctional chimeric protein in the recipient cells of the host simultaneously conferring multidrug resistance and efficient ADA activity.
EXAMPLE - 1 CONSTRUCTION OF A RETROVIRAL VECTOR
CONTAINING A MDRl-ADA FUSION GENE
The cloning strategies for MDRl related con¬ structions have been fully described in application S/N 07/062,583 which is incorporated herein by reference. Further strategies are now set forth. As shown sche¬ matically in Fig. 1, a human MDRl cDNA was fused to a human ADA cDNA by a synthetic linker and placed between the 5' and 3' long terminal repeats (LTRs) of the Harvey murine sarcoma virus expression vector pC06-HX following standard procedures such as described by Velu, et al, 1987, Science 238, 1408. All intermediates as well as the final constructs were characterized by restriction endonuclease mapping.
As a first step (Fig. 1A) , a 1.1 kb Asp 718 - Hhal fragment encoding a carboxylterminal region of the MDRl gene product P-glycoprotein (ranging from Val-926 to Lys-1278) was isolated from plasmid pMDRl 104-2. Two oligonucleotides, a 12-mer and an 18-mer, were synthe¬ sized and annealed to give an adapter with Hhal and Hindlll compatible ends and containing a single Sail restriction site. The adapter encodes the two carboxyl terminal amino acid residues of P-glycoprotein.
In a second step shown in Fig. IB full-length human ADA cDNA corresponding to ADA 211 cDNA as described by Adrian, et al, 1984, Hum. Genet. 68, 169, was sub- cloned as a 1.5 kb EcoRI fragment into the plasmid pUC8. Clone pUC8 ADA was then partially digested with Ncol to yield two types of linearized molecules which were both isolated by agarose gel electrophoresis. The desired linearized form of pUC8 ADA was cleaved within the codon for the initiator-methionine of ADA. In order to restore this condon, the ends of the linearized plasmid were filled in using the Klenow fragment of DNA polymerase I . Then a non-phosphorylated Sail-linker [carrying the new amino acids (Arg-Pro) of the final tripeptide-junction between P-glycoprotein and ADA] was added by ligation and plasmid pESE-13 was obtained. In the next step outlined in Fig. 1C, the human
MDRl and ADA genes were fused at the newly created single Sail site located at the 3' end of the P-glycoprotein coding region (pAHSH-1) and at the 5' end of the ADA structural gene (pESE-13). Concomitantly, the fusion gene was inserted into the pGEM-2 vector (Promega) . To this end a 2.9 kb EcoRI - Sad fragment (containing pGEM- 2 plasmid sequences) and a 2.9 kb Sacl - Asp 718 fragment encoding the aminoterinal part of P-glycoprotein) were isolated from pMDRl 2000XS (Ueda, et al, 1987, Acad. Sci. USA 84, 3004) and ligated with a 1.1. kb Asp 718 - Sail fragment of pAHSH-1 (carrying the coding region for the carboxylterminal part of P-glycoprotein) and a 1.4 kb Sail - EcoRI fragment isolated from pESE-13 (containing the structural gene for ADA) . In the resulting plasmid (pMDRADAS) a single SacII site was present at the 5' end of the fusion gene and could be used for its transfer into the retroviral expression vector pC06-HX (Velu, et al, 1987, Science 238, 1408).
For this purpose, however, a second site, a single Xhol site, had to be newly created at the 3' end of the fusion gene. Therefore, pMDRADAS was partially cut with EcoRI to linearize the molecule, filled in using the Klenow fragment of DNA polymerase I, and ligated with non-phosphorylated Xhol - linkers. The fusion gene was then excised from pMDRADA XS as a 5.45 kb SacII-XhoI fragment and ligated with the 10.7 kb SacII - Xhol frag¬ ment derived from pHaMDRl and containing the retroviral vector sequences. The final construct is designated pHaMDRlADA and carries the human MDR1-ADA fusion gene between the 5' and 3' LTRs of Harvey murine sarcoma virus . The MDR1-ADA fusion gene is the only functional eucaryotic gene in this vector and encodes a chimeric protein with an expected Mr of 210 kD. It consists of P- glycoprotein which is connected at the carboxyl-terminal amino acid Gln-1280 to the initiator-methionine of ADA by the tripeptide Gly-Arg-Pro. A deposit of the pHaMDRlADA has been made at the American Type Culture Collection (ATCC), 12301 Parklawn Drive, Rockville, Maryland, U.S.A. on May 18, 1988 under the accession number 67699. The deposit shall be viably maintained, replacing it if it becomes non- viable, for a period of 30 years from the date of the deposit, or for 5 years from the last date of request for a sample of the deposit, whichever is longer, and made available to the public without restriction in accordance with the provisions of the law. The Commissioner of Patents and Trademarks, upon request, shall have access to the deposit.
TRANSFECTION OF DRUG-SENSITIVE HUMAN KB CELLS AND COLCHICINE SELECTION
Drug-sensitive human KB-3-1 cells were trans- fected with pHaMDRlADA DNA. Negative control cells received no DNA whereas positive control cells were transfected with pHaMDRl which represents full-length human MDRl DNA in the same Harvey murine sarcoma virus expression vector (see Fig. 1C) . This plasmid represents full-length human MDRl cDNA in the same Harvey murine sarcoma virus expression vector (see Fig. 10). This plasmid confers the full phenotype of multidrug resistance to a variety of mouse and human cell lines as mentioned in application S/N 07/062,583. Plasmid DNA used for cell trans ections was isolated by standard alkaline lysis followed by cesium chloride gradient centrifugation. Drug-sensitive human KB-3-1 cells were transfected by the standard calcium phosphate precipitation method. 10 μ g of plasmid DNA were used to transfeet 5 x lOg cells per 10 cm dish. Sixteen hours after transfection cells were washed twice and 24 hrs later they were split 1:5 into medium contain¬ ing the selective drug colchicine at a concentration of 6 ng/ml. After a growth period of ten days, two dishes of cells were stained with 0.5% (w/v) methylene blue in 10% (v/v) ethanol and individual colonies counted. The data presented in Table I show the relative transfection efficiencies of plasmids pHaMDRlADA and pHaMDRl.
From three non-stained dishes six individual colchicine-resistant colonies were picked and represen¬ tative cell pools were collected. Both individual clones and cell populations were grown for at least ten more days in the presence of 6 ng/ml colchicine. It has been shown that due to amplification of the endogenous MDRl gene, human multidrug resistant cell lines become increasingly drug resistant when the concentration of the selective drug in the growth medium is raised. Hence, to investigate whether the transferred MDRl or MDRIADA DNA sequences are also amplified, the concentration of colchicine in the culture medium of transfected cells was raised stepwise in two-fold increments up to 96 ng colchicine/ml. Both individual clones and cell populations were passaged twice in appropriate drug con¬ centrations before being plated in the next higher concentration. No difference in growth rate at any con¬ centration of colchicine was observed between pHaMDRl and pHaMDRlADA transfected KB cells, indicating that the ADA fusion does not affect the functional activity of P- glycoprotein in the chimeric protein.
GENOMIC DNA ANALYSIS OF TRANSFECTED KB CELLS
In order to confirm the presence of the intro¬ duced MDRl or MDRIADA genes and to investigate their copy number, genomic DNA was isolated from transfected and control KB cells by standard procedures (Chen, et al, 1986, Cell 47, 381). Equal amounts of genomic DNA were analyzed by restriction endonuclease digestion using EcoRI, followed by agarose gel electrophoresis, Southern transfer and hybridization to a MDRl-specific probe. A 3 kb fragment of pHaMDRl transfected cells and a 4 kb frag¬ ment of pHaMDRlADA transfected cells were expected to give rise to a hybridization signal. Indeed, as shown in Fig. 2, strong hybridization signals of the correct size were obtained both for transfected individual clones and cell populations indicating that the integrated DNA sequences were intact. A weak 1.8 kb hybridization signal was detected in all investigated cells including the parental KB-3-1 cell line a a mock-transfected KB clone. Without being bound to any theory, it is postu¬ lated that this signal is probably derived from the endo- genous single-copy MDRl gene. The intensity of the 3 kb and 4 kb hybridization signals indicate that the pHaMDRl and pHaMDRlADA transfected cells contain multiple copies of the introduced DNA sequences. However, from the data presented in Fig. 3, it cannot be definitively concluded whether increasing concentrations of colchicine in the culture medium caused further amplification in the cell populations (Fig. 2B, lanes 2 and 4) could simply be a reflection of an enrichment for cells which express high levels of the MDRl or MDRIADA gene even at low concentra- tions of colchicine. Moreover, a potential rearrangement of the introduced DNA sequences in pHaMDRlADA transfected cells (Fig. 2B, lane 4) is also possible.
ANALYSIS OF THE PROTEINS PRODUCED BY TRANSFECTED KB CELLS Having confirmed the presence of the introduced
DNA sequences in pHaMDRlADA and pHaMDRl transfected KB cells, it was important to investigate their ex¬ pression. To this end immunoprecipitations using a poly- clonal rabbit antiserum against the carboxyl terminal regions of P-glycoprotein were performed. Cell cultures were radiolabeled with [JJS]-methionine for 16 hours and cell lysates prepared. Antigen-antibody complexes were allowed to form for 18 hours at 4°C and were then pre¬ cipitated with Protein A Sepharose. The precipitated proteins were analyzed by electrophoresis on a SDS - 7% polyacrylamide gel followed by fluorography. As shown in Fig. 3, P-glycoprotein with a Mr of 170 kD was detected in pHaMDRl transfected cells. The immunoprecipitated protein from pHaMDRlADA transfected cells has a higher Mr which is in good agreement with the calculated Mr of 210 kD of the MDRIADA fusion protein. Furthermore, the levels of the chimeric protein seem to increase along with the colchicine resistance of the cells.
ANALYSIS OF ADA ACTIVITY IN TRANSFECTED KB CELLS
After the expressed MDRIADA fusion protein was demonstrated to be intact, it was essential to test whether the ADA part was functionally active. To de on- strate ADA function, the sensitivity of pHaMDRlADA trans¬ fected cells to 2'-deoxycoformycin (dCF) was investigated in the presence of toxic concentrations of adenosine and compared to the sensitivity of pHaMDRl transfected cells. dCF is a tight-binding transition-state analog inhibitor of ADA (Dd = 2.5 x 10"12, Agarwal, et al, 1977, Biochem. Pharmacol. 26, 359; Frieden, et al, 1980, Biochemistry 19, 5303). Under conditions where ADA activity is required (such as in the presence of cyto- toxic amounts of adenosine) dCF can be used to estimate intracellular ADA levels. The amounts of dCF necessary to inhibit cell growth correlated with the amounts of functional ADA. Killing curves were performed by growing a constant number of dels (initially 300 cells were plated in a 60 mm dish) in culture medium supplemented with 1.1 mM adenosine, 1.0 mM uridine, 0.05 mM alanosine and variable amounts of dCF. Alanosine was added to block de novo AMP synthesis and uridine to alleviate the block in UMP synthesis caused by the high adenosine con¬ centration. After incubation at 37°C in 7% C02 for 10 days, the cells were stained with 0.5% (w/v) methylene blue in 50% (v/v) ethanol and colonies were counted. The results are presented in Fig. 4 and ID-^n values are shown in Table II. The ID-^g value corresponds to the concen¬ tration of dCF which reduces plating efficiency to 50% of the control without dCF. The data clearly indicate that pHaMDRlADA transfected cells survive higher concentra¬ tions of dCF than pHaMDRl transfected cells or mock- transfected control cells. Hence, it is concluded that ADA, as part of the chimeric MDRl-ADA fusion protein, is functional. Evidence for enzymatic activity, located primarily in the membrane fraction of transfected cells, is shown in Table III.
It should be noted that MDRl is only an example of a selectable marker gene. Given the illustrative methodology described herein, of course any selectable marker gene can be similarly employed to produce a chimeric gene. Furthermore, the linked gene which is introduced by fusion with the selectable marker gene may be altered (for example by mutation) and the effect of such alternations determined in intact living cells. Such manipulations allow the determination of the effect of the alternation and the verification that the mutant gene is in fact introduced and expressed as a poly- peptide. In the current example, the human MDRl gene linked to the ADA gene could be used to introduce mutant ADA proteins into cells for determining the function of different parts of the ADA molecule. Since ADA is also a selectable marker gene in tissue culture cells via the deoxycoformycin selection, ADA can be used as the select¬ able marker to introduce an altered MDRl gene into cells thereby allowing the determination of the function of various modifications of the MDRl protein.
It is understood that the examples and embodi¬ ments described herein are for illustrative purposes only and that various modifications or changes in light there¬ of will be suggested to persons skilled in the art and are to be included within the spirit and purview of this application and scope of the appended claims. TABLE I: Transfections of human KB-3-1 cells with pHaMDRlADA and pHaMDRl
DNA (amount) Colonies/5 x 105 cell.
pHaMDRlADA (5 μg) 75 pHaMDRlADA (10 μg) 125 pHaMDRl (5 μg) 330 pHaMDRl (10 μg) 550 no DNA 5
KB-3-1 cells were plated at 5 x 105 cells/10 cm dish and transfected the next day with the indicated DNAs. After 2 days cells were trypsinized and split 1:5 into culture medium supplemented with 6 ng/ml colchicine. Ten days later colonies were stained with methylene blue and counted.
TABLE II: Sensitivity of transfected KB cell lines to 2'-deoxycoformycin in the presence of toxic concentrations of adenosine
Colchicine
DNA Used for Concentration
Cell Line Transfection of Selection ID50 Value (ng/ml) (nM dCF)
KB-A None 6 0.13
KB-MDR1-A pHaMDRl 6 0.11
KB-MDR1ADA-G pHaMDRlADA 6 0.40
KB-MDR1ADA-I pHaMDRlADA 6 0.80
KB-MDRl Pool pHaMDRlADA 6 0.13
KB-MDR1 Pool pHaMDRl 24 0.11
KB-MDRIADA Pool pHaMDRlADA 6 0.42
KB-MDRIADA Pool pHaMDRlADA 24 2.0
KB-A, KB-MDR1, KB-MDRIADA G, and KB-MDRIADA I are indi¬ vidual clones.
TABLE III
ADA ACTIVITY OF CRUDE MEMBRANE AND CYTOSOLIC FRACTIONS OF PARENTAL AND TRANSFECTED KB CELL LINES
Colchicine ADA Activity
DNA Used Concentra- (nmol Inosine/min/mg) for Trans- tion for Cell line fection Selection (ng/ml) Cytosol Membranes
KB-3-1 None 0 18.2 3.0
KB-MDR1 pHaMDRl 6 13.6 2.0
Pool
KB-MDRl pHaMDRl 48 15.6 1.8
Pool
KB-MDRIADA pHaMDRlADA 6 15.8 1.9
Pool
KB-MDRIADA pHaMDRlADA 24 13.3 94.9
Pool
KB-MDRIADA pHaMDRlADA 48 17.1 153.4
Pool
ADA assays were performed according to Yeung, C.-y., Ingolia, D. E., Bobonis, C, Dunbar, B. S., Riser, M. E., Siciliano, M. J., and Kellems, R. E. (1983) J. Biol. Che . 258, 8338-8345. To determine ADA activity in the membrane or cytosolic fraction, cells were collected by scraping into PBS, washed twice with PBS, resuspended in hypotonic lysis buffer (10 mM Tris HCl pH 7.5, 10 mM NaCl, 1 mM MgCl2) at a concentration of 2 x 107 cells/ml and incubated in an ice-bath for 15 min. The swollen cells were disrupted with 20 strokes in a tightly fitting Dounce homogenizer and the nuclei removed by centrifuga- tion at 400 xg for 10 min at 4°C. The pellet obtained by subsequent centrifugation at 30,000 xg for 30 min at 4°C was used as the crude membrane fraction and the super¬ natant was used as the cytosolic fraction.

Claims

WHAT IS CLAIMED IS:
1. A fusion gene comprising a coding sequence for a selectable marker fused to another coding sequence which is desired to be expressed in recipient cells.
2. The f sion gene of claim 1 wherein said selectable marker coding sequence is human MDRl gene.
3. The fusion gene of claim 1 wherein said another coding sequence is ADA gene.
4. The fusion gene of claim 1 being MDRIADA. -
5. The fusion gene of claim 4 cloned in an expression vector.
6. The fusion gene of claim 1 having the identifying characteristics of ATCC 67699.
7. A method for expressing in vivo a desired gene, comprising introducing into cells of a host a fusion gene comprising a selectable marker coding sequence fused to. a gene whose expression is desired in vivo in recipient cells to alleviate conditions resulting from genetic or acquired disorder related to said gene.
8. The fusion gene of claim 1 wherein the selectable marker coding sequence or said another coding sequence is altered to determine resultant effect there¬ of.
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EP0451157A1 (en) * 1988-10-21 1991-10-16 THE UNITED STATES OF AMERICA as represented by the Secretary UNITED STATES DEPARTMENT OF COMMERCE Transgenic animals for testing multidrug resistance
EP0451157A4 (en) * 1988-10-21 1992-01-02 Us Health Transgenic animals for testing multidrug resistance
US6627615B1 (en) 1991-12-17 2003-09-30 The Regents Of The University Of California Methods and compositions for in vivo gene therapy
US6468798B1 (en) 1991-12-17 2002-10-22 The Regents Of The University Of California Expression of cloned genes in the lung by aerosol and liposome-based delivery
US5858784A (en) * 1991-12-17 1999-01-12 The Regents Of The University Of California Expression of cloned genes in the lung by aerosol- and liposome-based delivery
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