Oeda K, Horiuchi T, Sekiguchi M
Mol Gen Genet. 1981;184(2):191-9. doi: 10.1007/BF00272904.
The uvrD gene of Escherichia coli that controls UV sensitivity and spontaneous mutation frequency has been cloned with phage lambda as vector. The increased sensitivity to ultraviolet light (UV) of uvrD3, uvrE502, recL152, and pdeB41 mutants, high mutability of uvrD3 and pdeB41 mutants, and conditional lethality of strain TS41 that carried pdeB41, polA1, and supl26 mutations were all suppressed by lysogenization of the mutant cells with lambda uvrD+. These results were consistent with the idea that the uvrD, uvrE, recL, and pdeB mutations are alleles of the uvrD gene. In addition to the uvrD gene, lambda uvrD+ carried the corA gene that controls transport of Mg++, Mn++, and Co++ through the cell membrane. Hybrid plasmids carrying both uvrD and corA genes were also constructed by using pKY2289 as a cloning vehicle. Orientational isomers that carried the same 12.0 kb fragment in the opposite direction were equally efficient in complementing the UvrD- as well as CorA- defects of the transformed host cells, suggesting that the DNA insert contains all the genetic signals needed to express the two gene products. Insertion of the gamma delta sequence into recombinant plasmids was performed to generate appropriate restriction endonuclease target sites in the cloned DNA fragments.
以噬菌体λ为载体克隆了大肠杆菌中控制紫外线敏感性和自发突变频率的uvrD基因。uvrD3、uvrE502、recL152和pdeB41突变体对紫外线(UV)的敏感性增加、uvrD3和pdeB41突变体的高突变率以及携带pdeB41、polA1和sup126突变的TS41菌株的条件致死性,都通过用λuvrD+对突变细胞进行溶原化而得到抑制。这些结果与uvrD、uvrE、recL和pdeB突变是uvrD基因的等位基因这一观点一致。除uvrD基因外,λuvrD+还携带控制Mg++、Mn++和Co++通过细胞膜运输的corA基因。还以pKY2289为克隆载体构建了携带uvrD和corA基因的杂交质粒。携带相同12.0 kb片段但方向相反的定向异构体在互补转化宿主细胞的UvrD-和CorA-缺陷方面同样有效,这表明DNA插入片段包含表达这两种基因产物所需的所有遗传信号。将γδ序列插入重组质粒以在克隆的DNA片段中产生合适的限制性内切酶靶位点。
