Ianenko A S, Bogush V G, Kirsanov N B, Liapin M N, Krylov V N
Genetika. 1983 Nov;19(11):1760-8.
The hybrid plasmid RP4::D3112 becomes unstable in Escherichia coli K-12 cells under certain growth conditions. The deletion mutants of this plasmid are formed at a high frequency. All the deletions selected have a specific feature: they start in the left end, at the point of joining of plasmid and phage DNA, and remove different portions of the phage genome. The deletion mutants have been used for genetic mapping of D3112. We have localized the repressor gene cI (0-1.3 kb), 3 early genes (1.3-14.2 kb) and two groups of late genes (14.2-29.9 and 29.9-38 kb). Electron microscope studies of RP4::D3112 DNA and its deletion derivatives have shown that integration of D3112 genome in RP4 occurs through the ends of the genome, without permutations. It appears that bacterial nucleotide sequences joined to DNA from mature D3112 particles, to the right end of D3112 genome, are lost. Thus, transposable phages D3112 of Pseudomonas aeruginosa and E. coli Mu phage have some similarities in the genome organization and in the way of their integration into the host DNA.
在某些生长条件下,杂种质粒RP4::D3112在大肠杆菌K - 12细胞中变得不稳定。该质粒的缺失突变体高频形成。所有选择的缺失都有一个特定特征:它们始于左端,即质粒与噬菌体DNA的连接点,并去除噬菌体基因组的不同部分。这些缺失突变体已用于D3112的基因定位。我们已定位了阻遏基因cI(0 - 1.3 kb)、3个早期基因(1.3 - 14.2 kb)以及两组晚期基因(14.2 - 29.9和29.9 - 38 kb)。对RP4::D3112 DNA及其缺失衍生物的电子显微镜研究表明,D3112基因组在RP4中的整合是通过基因组末端进行的,没有重排。似乎与来自成熟D3112颗粒的DNA相连的细菌核苷酸序列,即D3112基因组右端的序列,丢失了。因此,铜绿假单胞菌的转座噬菌体D3112和大肠杆菌Mu噬菌体在基因组组织及其整合到宿主DNA的方式上有一些相似之处。
