Frankel W, Potter T A, Rosenberg N, Lenz J, Rajan T V
Proc Natl Acad Sci U S A. 1985 Oct;82(19):6600-4. doi: 10.1073/pnas.82.19.6600.
A clonal murine cell line that is heterozygous at the beta 2-microglobulin locus (B2m) was obtained by Abelson murine leukemia virus (Ab-MuLV) transformation of liver cells from (C57BL/6 X BALB/c) F1 fetuses. To obtain proviral insertional mutants, we superinfected a subclone of these cells, which does not express the env surface protein of the Moloney leukemia virus (Mo-MuLV, the helper virus that was used to transmit the defective Ab-MuLV genome during transformation), with Mo-MuLV. Mutant clones that fail to express the C57BL/6 allele of B2m (B2mb) were then immunoselected by using a monoclonal antibody that specifically recognizes the B2mb gene product and not that of the B2ma allele. Of 22 independent clones obtained, one contains a proviral insertion that is near or in the first exon of the B2mb gene. Surprisingly, the insertion is of the Ab-MuLV genome and not of replication-competent Mo-MuLV. This indicates that superinfection with Mo-MuLV "rescued" the defective Ab-MuLV genome, which then inserted into the B2mb gene. We conclude that when an allele-specific selection procedure exists, proviral insertion is a potential method for obtaining mutations in heterozygous mammalian cells. This approach may thereby provide a method for molecular cloning of such selectable genes, using a retroviral hybridization probe.
通过用阿贝尔森鼠白血病病毒(Ab-MuLV)转化(C57BL/6×BALB/c)F1胎鼠的肝细胞,获得了一种在β2-微球蛋白基因座(B2m)杂合的克隆小鼠细胞系。为了获得前病毒插入突变体,我们用莫洛尼白血病病毒(Mo-MuLV,在转化过程中用于传递有缺陷的Ab-MuLV基因组的辅助病毒)对这些细胞的一个亚克隆进行了超感染,该亚克隆不表达莫洛尼白血病病毒的env表面蛋白。然后,通过使用一种单克隆抗体进行免疫筛选,该抗体特异性识别B2m的C57BL/6等位基因(B2mb)的基因产物,而不识别B2m的A等位基因(B2ma)的基因产物。在获得的22个独立克隆中,有一个克隆的前病毒插入位于B2mb基因的第一个外显子附近或之中。令人惊讶的是,插入的是Ab-MuLV基因组,而不是具有复制能力的Mo-MuLV基因组。这表明用Mo-MuLV进行超感染“拯救”了有缺陷的Ab-MuLV基因组,然后该基因组插入到了B2mb基因中。我们得出结论,当存在等位基因特异性选择程序时,前病毒插入是在杂合哺乳动物细胞中获得突变的一种潜在方法。因此,这种方法可能提供一种使用逆转录病毒杂交探针分子克隆此类可选择基因的方法。
