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噬菌体λ基因表达在远离该基因的位点的转录后调控。

Posttranscriptional control of bacteriophage lambda gene expression from a site distal to the gene.

作者信息

Guarneros G, Montañez C, Hernandez T, Court D

出版信息

Proc Natl Acad Sci U S A. 1982 Jan;79(2):238-42. doi: 10.1073/pnas.79.2.238.

Abstract

The bacteriophage lambda int gene product, integrase, recombines the phage DNA with the host DNA at specific sites on each to accomplish lysogeny. The int gene is transcribed from two promoters, PL and PI, each regulated positively by lambda proteins. The expression of integrase is also controlled from a site, sib, in the b region of the phage genome. This is a unique regulatory site because it is located distal to the structural gene in relation to the promoters. The expression of int from the PL promoter is inhibited when sib is present. This effect appears to be specific for PL because sib does not cause inhibition of PI-dependent int synthesis. lambda mutants that contain alterations in the site have been isolated. Sequence analyses of the mutations reveal single base changes, spanning 37 base pairs (bp) in the b region, some 240 bp beyond the int gene. Another mutant, hef13, which has a phenotype similar to that of sib, introduces a nucleotide change within the same 37-bp region. The sib and hef mutations cluster within a region of dyad symmetry. Regulation of int synthesis by sib occurs after transcription of the int gene. There is no difference in the rate of PL-promoted int mRNA synthesis in either sib+ or sib- phage infections, yet int mRNA is less stable in the sib+ infection. Because RNase III host mutants are defective in sib regulation, processing of the PL mRNA at sib by this endoribonuclease may cause int mRNA decay and decrease int synthesis.

摘要

噬菌体λ整合酶基因产物整合酶,可使噬菌体DNA与宿主DNA在各自特定位点发生重组,从而实现溶原化。整合酶基因由两个启动子PL和PI转录,每个启动子都受λ蛋白正向调控。整合酶的表达还受噬菌体基因组b区域内一个位点sib的控制。这是一个独特的调控位点,因为相对于启动子而言,它位于结构基因的远端。当存在sib时,来自PL启动子的整合酶表达受到抑制。这种效应似乎对PL具有特异性,因为sib不会抑制依赖PI的整合酶合成。已分离出在该位点发生改变的λ突变体。对这些突变的序列分析揭示了单个碱基变化,跨越b区域的37个碱基对(bp),位于整合酶基因下游约240 bp处。另一个突变体hef13,其表型与sib相似,在同一37 bp区域内引入了一个核苷酸变化。sib和hef突变聚集在一个二重对称区域内。sib对整合酶合成的调控发生在整合酶基因转录之后。在sib +或sib -噬菌体感染中,PL促进的整合酶mRNA合成速率没有差异,但在sib +感染中,整合酶mRNA不太稳定。由于RNase III宿主突变体在sib调控方面存在缺陷,这种核糖核酸内切酶在sib处对PL mRNA的加工可能导致整合酶mRNA降解并减少整合酶合成。

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Regulation of the integration-excision reaction by bacteriophage lambda.噬菌体λ对整合-切除反应的调控
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