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携带大肠杆菌K-12鞭毛基因的非缺陷型转导λ噬菌体的分离与鉴定

Isolation and characterization of nondefective transducing lambda bacteriophages carrying fla genes of Escherichia coli K-12.

作者信息

Kondoh H

出版信息

J Bacteriol. 1977 May;130(2):736-45. doi: 10.1128/jb.130.2.736-745.1977.

Abstract

In Escherichia coli K-12, 11 fla genes and a hag gene are located between his and uvrC, making two clusters at map positions 42.5 and 43.0 min. Nondefective transducing lambda phages for these genes were isolated. Low-frequency-transducing donors were constructed starting from lysogens of lambda cI857 in which the prophage is integrated at a secondary attachment site at 44 min on the E. coli map. Two strategies were used to delete the region between the prophage and the fla genes. Deletion mutants of the supD locus between fla and the prophage were isolated by selecting for loss of Su1+, an allele of supD. A strain with a deletion starting within the prophage and ending at a position close to the fla genes was isolated from heat-resistant derivatives of the lysogen. A lysogen of lambda b2 was then constructed in which the prophage had integrated at the site of the defective prophage by means of recombination with residual lambda deoxyribonucleic acid. From low-frequency-transducing lysate of the donor strains thus constructed, either directly or in combination with a procedure that extends the loci transduced, various lambda pfla's were isolated. lambda pflaL1 carries all nine fla genes at 43 min, and lambda pflaH14 carries hag and two fla genes at 42.5 min.

摘要

在大肠杆菌K-12中,11个鞭毛基因和1个hag基因位于his和uvrC之间,在图谱位置42.5分钟和43.0分钟处形成两个簇。分离出了这些基因的无缺陷转导λ噬菌体。从λcI857溶原菌构建低频转导供体,其中原噬菌体整合在大肠杆菌图谱上44分钟处的一个二级附着位点。使用了两种策略来删除原噬菌体和鞭毛基因之间的区域。通过选择supD的一个等位基因Su1+的缺失,分离出鞭毛基因和原噬菌体之间supD位点的缺失突变体。从溶原菌的耐热衍生物中分离出一种缺失菌株,其缺失从原噬菌体内部开始,到接近鞭毛基因的位置结束。然后构建了一个λb2溶原菌,其中原噬菌体通过与残留的λ脱氧核糖核酸重组而整合在缺陷原噬菌体的位点上。从如此构建的供体菌株的低频转导裂解物中,直接或与扩展转导位点的程序相结合,分离出了各种λpfla。λpflaL1在43分钟处携带所有9个鞭毛基因,λpflaH14在42.5分钟处携带hag和两个鞭毛基因。

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