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Identification of gene function by cyclical packaging rescue of retroviral cDNA libraries

机译:逆转录病毒cDNA文库的循环包装拯救鉴定基因功能

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摘要

Genes regulating responses in mammalian cells are often difficult to identify by functional cloning strategies limited to a single round of selection. Here we describe a strategy, cyclical packaging rescue (CPR), which allows rapid recovery and retransmission of retroviral cDNA libraries. CPR can be used not only with immortalized cell lines such as fibroblasts and Jurkat T cells, but also with primary B lymphocytes, which can be maintained only in short-term cultures. CPR allows for multiple rounds of selection and enrichment to identify cDNAs regulating responses in mammalian cells. Using CPR, five cDNAs were functionally cloned, which conferred protection against tumor necrosis factor α (TNFα)-induced apoptosis in RelA−/− fibroblasts. Three of the genes, RelA, cellular FLICE-like inhibitory protein (c-FLIP), and a dominant-negative mutant of TNF receptor 1 arising through CPR afforded strong protection against apoptosis. Two of the genes identified, Dbs and Fas-associated death domain protein (FADD), previously identified as a proapoptotic molecule, afforded partial protection against TNFα-induced apoptosis. These results suggest that CPR is a versatile method that permits functional identification of both wild-type and dominant-negative gene products that regulate cellular responses.
机译:限制哺乳动物细胞反应的基因通常难以通过限于单轮选择的功能性克隆策略来鉴定。在这里,我们描述了一种策略,循环包装救援(CPR),它可以快速恢复和重新传递逆转录病毒cDNA文库。 CPR不仅可以用于永生化细胞系,例如成纤维细胞和Jurkat T细胞,而且可以与原代B淋巴细胞一起使用,后者只能在短期培养中才能维持。 CPR允许进行多轮选择和富集,以鉴定调节哺乳动物细胞反应的cDNA。使用CPR,从功能上克隆了五个cDNA,赋予了针对肿瘤坏死因子α(TNFα)诱导的RelA -/-成纤维细胞凋亡的保护作用。通过CPR产生的三个基因RelA,细胞FLICE样抑制蛋白(c-FLIP)和TNF受体1的显性负突变提供了针对凋亡的强大保护作用。已鉴定的两个基因,Dbs和Fas相关的死亡域蛋白(FADD),先前被鉴定为促凋亡分子,提供了针对TNFα诱导的细胞凋亡的部分保护。这些结果表明,CPR是一种通用的方法,可以对调节细胞反应的野生型和显性阴性基因产物进行功能鉴定。

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