Cultured rat cells deficient in endogenous thymidine kinase activity (tk) were stably transformed with a recombination-indicator DNA substrate constructed in vitro by rearrangement of the herpes simplex virus tk gene sequences into a partially redundant permutation of the functional gene. The recombination-indicator DNA did not express tk, but was designed to allow formation of a functional tk gene via homologous recombination. A clonal cell line (519) was isolated that harbored several permuted herpes simplex virus tk genes. 519 cells spontaneously produced progeny that survived in medium containing hypoxanthine, aminopterin, and thymidine. Acquisition of resistance to hypoxanthine, aminopterin, and thymidine was accompanied by the rearrangement of the defective tk gene to functional configuration. The rearrangement apparently occurred by unequal exchange between one permuted tk gene and a replicated copy of itself. Recombination was between 500-base-pair tracts of DNA sequence homology that were separated by 3.4 kilobases. Exchanges occurred spontaneously at a frequency of approximately 5 X 10(-6) events per cell per generation. Recombination also mediated reversion to the tk- phenotype; however, the predominant mechanism by which cells escaped death in the presence of drugs rendered toxic by thymidine kinase was not recombination, but rather inactivation of the intact tk gene.
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机译:通过将单纯疱疹病毒tk基因序列重排成功能基因的部分冗余排列,用体外构建的重组指示剂DNA底物稳定转化缺乏内源胸苷激酶活性(tk)的培养大鼠细胞。重组指示剂DNA不表达tk,但是被设计成允许通过同源重组形成功能性tk基因。分离出克隆的细胞系(519),其中包含几个排列的单纯疱疹病毒tk基因。 519个细胞自发产生后代,该后代在含有次黄嘌呤,氨基蝶呤和胸苷的培养基中存活。获得对次黄嘌呤,氨基蝶呤和胸苷的抗性伴随有缺陷的tk基因重排至功能构型。这种重排显然是由于一个排列的tk基因与其自身复制副本之间的交换不平等而发生的。重组是在DNA序列同源性的500个碱基对之间,相隔3.4个碱基。交换自发地发生在每个世代每个细胞大约5 X 10(-6)个事件的频率上。重组也介导了tk表型的回复。然而,在存在被胸苷激酶毒性的药物存在下,细胞逃脱死亡的主要机制不是重组,而是完整的tk基因失活。
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