HIGH-EFFICIENCY IDENTIFICATION OF GENES BY FUNCTIONAL-ANALYSIS FROM A RETROVIRAL CDNA EXPRESSION LIBRARY

被引:38
作者
WONG, BY
CHEN, H
CHUNG, SW
WONG, PMC
机构
[1] TEMPLE UNIV,FELS INST CANC RES & MOLEC BIOL,DEPT BIOCHEM,PHILADELPHIA,PA 19140
[2] TEMPLE UNIV,DEPT MICROBIOL,PHILADELPHIA,PA 19140
[3] TEMPLE UNIV,DEPT IMMUNOL,PHILADELPHIA,PA 19140
[4] SUNY HLTH SCI CTR,MORSE INST MOLEC GENET,DEPT IMMUNOL & MICROBIOL,BROOKLYN,NY 11203
关键词
D O I
10.1128/JVI.68.9.5523-5531.1994
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Retroviral gene transfer efficiently delivers genes of interest stably into target cells, and expression cDNA cloning has been shown to be highly successful. Considering these two advantages, we now report a method by which one can identify genes stimulating cell growth through functional analysis. The first step requires the construction of a retroviral cDNA expression library and the optimization of transfection of vector DNA into virus packaging cells. The second step involves the cocultivation of target cells with libraries of retrovirus-producing cells, resulting in the amplification of target cells transduced with a gene(s) stimulating cell growth. Under standardized conditions of transfection, we detected an average of 4,000 independent clones per dish, among which expression of a retroviral beta-galactosidase gene at an abundance of 0.2% could be detected. Next, we demonstrated the augmentation of the sensitivity of the assay by retroviral infection and functional analysis. We did this by cocultivating factor-dependent (FD) cells with dishes of GP/E cells transfected with plasmids containing various molar ratios of pN2-IL3 DNA and retroviral library cDNA and by determining the highest dilution of pN2-IL3 which Still resulted in the conversion of FD cells to factor independence. The retroviral interleukin-3 gene at an abundance as low as 0.001% could be detected. Indeed, we were able to detect from FD cells the development of factor-independent colonies with different phenotypes after retroviral transfer of cDNAs from an immortalized hemopoietic stem cell line. Thus, the combination of a standardized high-efficiency DNA transfection and retrovirus-mediated gene transfer should facilitate the identification of genes capable of conferring to target FD cells a detectable new function or phenotype. By scaling up the size of the experiment realistically during screening, the assay can detect cDNA at an abundance of lower than 0.0001%.
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页码:5523 / 5531
页数:9
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