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Molecular Pharmacology

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Research ArticleArticle

Analysis of Random Recombination between Human MDR1 and Mouse Mdr1a cDNA in a pHaMDR-Dihydrofolate Reductase Bicistronic Expression System

Tzipora Shoshani, Shudong Zhang, Saibal Dey, Ira Pastan and Michael M. Gottesman
Molecular Pharmacology October 1998, 54 (4) 623-630;
Tzipora Shoshani
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Shudong Zhang
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Saibal Dey
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Ira Pastan
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Michael M. Gottesman
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Abstract

Human P-glycoprotein (Pgp) confers multidrug resistance (MDR) to otherwise sensitive cells. The homologous mouse Pgps, which are encoded by mouse mdr1a (also known as mdr3) andmdr1b (also known as mdr1), confer different degrees of resistance to the same MDR drugs and inhibitors. To create recombinants for the study of sequences responsible for these differences in drug-resistance, chimeric cDNA libraries can be constructed by homologous recombination of pools of related sequences. This mutagenesis approach is called DNA shuffling. To select for chimeric Pgp with an altered resistance profile, DNA shuffling between the homologous but not identical drug interacting transmembrane domains 5 and 6 of human MDR1 and mouse mdr1a was used. The chimeric proteins were expressed in human KB-3-1 cells. One recombinant Pgp (clone 3-4) with a novel phenotype was analyzed in detail. Inhibitors of Pgp, including verapamil and cyclosporin A, were less effective in reversing resistance of the chimeric Pgp compared with wild-type Pgp, for certain drugs. However, [125I]iodoarylazidoprazosin photoaffinity labeling of the chimeric Pgp and its binding competition with cyclosporin A, showed that cyclosporin A competed for the photoaffinity labeling. The chimeric Pgp cells stained less well with human-specific anti-Pgp mAb MRK16 than wild-type Pgp, despite having the described epitopes for MRK16. Staining with human-specific mAb UIC2 was increased when the chimeric protein was compared with wild-type Pgp. These results suggest an alteration in exposure of human Pgp specific epitopes in this chimeric Pgp, as well as a change in the interaction of reversing agents with the chimeric protein.

Footnotes

  • Send reprint requests to: Dr. Michael M. Gottesman, Lab of Cell Biology, NCI/NIH, Building 37, Room 1AO9, 37 Convent Dr MSC4255, Bethesda, MD 20892-4255. E-mail: mgottesman{at}nih.gov

  • ↵1 Current affiliation: Division of Oncology, Room 6318-University Wing, The Hospital for Sick Children, 555 University Avenue, Toronto, Ontario, M5G 1X8, Canada

  • Abbreviations:
    Pgp
    P-glycoprotein
    MDR
    multidrug resistance
    PCR
    polymerase chain reaction
    TM
    transmembrane
    MTX
    methotrexate
    IRES
    internal ribosome entry site
    DHFR
    dihydrofolate reductase
    FACS
    fluorescence-activated cell-sorting
    IAAP
    iodoarylazidoprazosin
    AM
    acetoxymethyl ester
    • Received January 14, 1998.
    • Accepted June 23, 1998.
  • The American Society for Pharmacology and Experimental Therapeutics
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Molecular Pharmacology: 54 (4)
Molecular Pharmacology
Vol. 54, Issue 4
1 Oct 1998
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Research ArticleArticle

Analysis of Random Recombination between Human MDR1 and Mouse Mdr1a cDNA in a pHaMDR-Dihydrofolate Reductase Bicistronic Expression System

Tzipora Shoshani, Shudong Zhang, Saibal Dey, Ira Pastan and Michael M. Gottesman
Molecular Pharmacology October 1, 1998, 54 (4) 623-630;

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Research ArticleArticle

Analysis of Random Recombination between Human MDR1 and Mouse Mdr1a cDNA in a pHaMDR-Dihydrofolate Reductase Bicistronic Expression System

Tzipora Shoshani, Shudong Zhang, Saibal Dey, Ira Pastan and Michael M. Gottesman
Molecular Pharmacology October 1, 1998, 54 (4) 623-630;
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