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大肠杆菌K-12 srl区域的遗传分析。

Genetic analysis of the Escherichia coli K-12 srl region.

作者信息

McEntee K

出版信息

J Bacteriol. 1977 Dec;132(3):904-11. doi: 10.1128/jb.132.3.904-911.1977.

Abstract

Specialized transducing lambda derivatives, deletion mapping, and Plkc transductional crosses have been used to analyze the genetic organization and regulation of the srl genes. Transducing phages obtained from a secondary site lambda insertion in srlA are of two types: lambdapsrlC1 and lambdaprecA are substituted in the b2 region of the lambda chromosome (galtype) and carry the srlC gene but not srlD; lambdapsrlD is substituted in the early region of the phage deoxyribonucleic acid (biotype) and carries the srlD gene but not srlC. The lambdapsrlC1 phage, which lysogenizes at attlambda, complements srlC mutants in trans, indicating that this gene codes for a diffusable positive regulatory element. The srl genes have been ordered relative to the cysC, recA, and alaS genes by two- and three-factor P1kc crosses. The order, cysC...srlD-srlA-srlC-recA-alaS, has been obtained. The srlA and srlD genes comprise an operon with srlD operator distal. From the secondary site lysogen, it has been possible to obtain deletion mutants of this region that are sensitive to ultraviolet light and are recombination deficient. Genetic evidence suggests that these deletions extend from srl into the recA gene.

摘要

已使用特异性转导λ衍生物、缺失作图和P1kc转导杂交来分析srl基因的遗传组织和调控。从srlA中λ的二次位点插入获得的转导噬菌体有两种类型:λpsrlC1和λprecA在λ染色体的b2区域(gal型)被取代,并携带srlC基因但不携带srlD;λpsrlD在噬菌体脱氧核糖核酸的早期区域(生物型)被取代,并携带srlD基因但不携带srlC。在attλ处溶原化的λpsrlC1噬菌体可反式互补srlC突变体,表明该基因编码一种可扩散的正向调控元件。通过双因子和三因子P1kc杂交,已确定srl基因相对于cysC、recA和alaS基因的顺序。已获得的顺序为:cysC...srlD-srlA-srlC-recA-alaS。srlA和srlD基因组成一个操纵子,srlD在操纵基因远端。从二次位点溶原菌中,已获得该区域对紫外线敏感且重组缺陷的缺失突变体。遗传证据表明这些缺失从srl延伸到recA基因。

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Genetic analysis of the Escherichia coli K-12 srl region.大肠杆菌K-12 srl区域的遗传分析。
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