Miki T, Kimura M, Hiraga S, Nagata T, Yura T
J Bacteriol. 1979 Dec;140(3):817-24. doi: 10.1128/jb.140.3.817-824.1979.
The dnaA gene of Escherichia coli K-12, supposedly present in the deoxyribonucleic acid (DNA) of specialized transducing phase lambda i21 dnaA-2, was cloned onto plasmid pBR322. The new plasmid was named pMCR501. Physical analyses of DNAs of lambda i21 dnaA-2 and pMCR501 revealed the following. The lambda i21 dnaA-2 DNA retained the delta sr I lambda 1-2 and ninR5 deletions and imm21 substitution which were originally present in the parental phage. The size reduction was compensated for by the insertion-substitution segment (tna-dnaA region) in lambda i21 dnaA-2 DNA. The fractional size of this segment was approximately 7 megadaltons (Md), or 10 kilobases, which was found to be the sum of the tna insertion subsegment of ca. 3.5 Md and the dnaA substitution subsegment of ca. 3.5 Md. Phage P1-mediated transductional mapping between the dnaA46 and tna mutations gave a cotransduction frequency of 84%, corresponding to approximately 5 kilobases. Thus, it is strongly suggested that the dnaA gene resides in the lambda i21 dnaA-2 DNA. Cleavage mapping with the restriction endonuclease of pMCR501 DNA confirmed that it was constructed by excising a BamHI fragment of 4.29 Md, containing the 3.5-Md dnaA substitution segment, from the lambda i21 dnaA-2 DNA, inserting it into the sole BamHI cleavage site on pBR322.
据推测存在于特异性转导噬菌体λi21 dnaA - 2的脱氧核糖核酸(DNA)中的大肠杆菌K - 12的dnaA基因,被克隆到质粒pBR322上。新质粒被命名为pMCR501。对λi21 dnaA - 2和pMCR501的DNA进行的物理分析结果如下。λi21 dnaA - 2 DNA保留了最初存在于亲代噬菌体中的δsr I λ1 - 2和ninR5缺失以及imm21取代。λi21 dnaA - 2 DNA中大小的减小由插入 - 取代片段(tna - dnaA区域)补偿。该片段的分子量约为7兆道尔顿(Md),即10千碱基,发现它是约3.5 Md的tna插入子片段和约3.5 Md的dnaA取代子片段之和。噬菌体P1介导的dnaA46和tna突变之间的转导作图给出了84%的共转导频率,对应于约5千碱基。因此,强烈提示dnaA基因存在于λi21 dnaA - 2 DNA中。用pMCR501 DNA的限制性内切酶进行的切割作图证实,它是通过从λi21 dnaA - 2 DNA中切除一个4.29 Md的BamHI片段(包含3.5 - Md的dnaA取代片段),并将其插入pBR322上唯一的BamHI切割位点而构建的。
