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控制大肠杆菌高温调节子的一个基因的分子克隆与表达

Molecular cloning and expression of a gene that controls the high-temperature regulon of Escherichia coli.

作者信息

Neidhardt F C, VanBogelen R A, Lau E T

出版信息

J Bacteriol. 1983 Feb;153(2):597-603. doi: 10.1128/jb.153.2.597-603.1983.

Abstract

The high-temperature production (HTP) regulon of Escherichia coli consists of a set of operons that are induced coordinately by a shift to a high temperature under the control of a single chromosomal gene called htpR or hin. To identify more components of this regulon, the rates of synthesis of many polypeptides resolved on two-dimensional polyacrylamide gels were measured in various strains by pulse-labeling after a temperature shift-up. A total of 13 polypeptides were found to be heat inducible only in cells bearing a normal htpR gene on the chromosome or on a plasmid; on this basis these polypeptides were designated products of the HTP regulon. Several hybrid plasmids that contain segments of the E. coli chromosome in the 75-min region were found to carry the htpR gene. A restriction map of this region was constructed, and selected fragments were subcloned and tested for the ability to complement an htpR mutant. The polypeptides encoded by these fragments were detected by permitting expression in maxicells, minicells, and chloramphenicol-treated cells. Complementation was accompanied by production of a polypeptide having a molecular weight of approximately 33,000. This polypeptide, designated F33.4, was markedly reduced in amount in an htpR mutant expected to contain very little htpR gene product. Polypeptide F33.4 is postulated to be the product of htpR and to be an effector that controls heat induction of the HTP regulon.

摘要

大肠杆菌的高温生产(HTP)调节子由一组操纵子组成,这些操纵子在一个名为htpR或hin的单一染色体基因的控制下,通过转移到高温而被协同诱导。为了鉴定这个调节子的更多组成部分,在温度升高后,通过脉冲标记法在各种菌株中测量了二维聚丙烯酰胺凝胶上分离出的许多多肽的合成速率。总共发现有13种多肽仅在染色体或质粒上携带正常htpR基因的细胞中是热诱导的;基于此,这些多肽被指定为HTP调节子的产物。发现几个含有大肠杆菌染色体75分钟区域片段的杂交质粒携带htpR基因。构建了该区域的限制酶图谱,并将选定的片段进行亚克隆,并测试其互补htpR突变体的能力。通过在大细胞、小细胞和氯霉素处理的细胞中表达来检测这些片段编码的多肽。互补作用伴随着一种分子量约为33000的多肽的产生。这种多肽被命名为F33.4,在一个预计含有极少htpR基因产物的htpR突变体中,其含量明显减少。推测多肽F33.4是htpR的产物,并且是控制HTP调节子热诱导的效应物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/17fc/221674/f3ea1d274b74/jbacter00249-0030-a.jpg

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