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PhoE porin of Escherichia coli and phosphate reversal of acid damage and killing and of acid induction of the CadA gene product.大肠杆菌的PhoE孔蛋白以及酸损伤与杀伤的磷酸盐逆转和CadA基因产物的酸诱导
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LysP和CadC在介导大肠杆菌cad操纵子酸诱导所需赖氨酸中的作用。

Roles of LysP and CadC in mediating the lysine requirement for acid induction of the Escherichia coli cad operon.

作者信息

Neely M N, Dell C L, Olson E R

机构信息

Parke-Davis Pharmaceutical Research, Division of Warner-Lambert Co., Ann Arbor, Michigan 48105.

出版信息

J Bacteriol. 1994 Jun;176(11):3278-85. doi: 10.1128/jb.176.11.3278-3285.1994.

DOI:10.1128/jb.176.11.3278-3285.1994
PMID:8195083
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC205498/
Abstract

Expression of the Escherichia coli cadBA operon, encoding functions required for the conversion of lysine to cadaverine and for cadaverine excretion, requires at least two extracellular signals: low pH and a high concentration of lysine. To better understand the nature of the lysine-dependent signal, mutants were isolated which expressed a cadA-lacZ transcription fusion in the absence of lysine while retaining pH regulation. The responsible mutation in one of these isolates (EP310) was in cadC, a gene encoding a function necessary for transcriptional activation of cadBA. This mutation (cadC310) is in a part of the gene encoding the periplasmic domain of CadC and results in an Arg-to-Cys change at position 265, indicating that this part of the protein is involved in responding to the presence of lysine. Three other mutants had mutations mapping in or near lysP (cadR), a gene encoding a lysine transport protein that has previously been shown to regulate cadA expression. One of these mutations is an insertion in the lysP coding region. Thus, in the absence of exogenous lysine, LysP is a negative regulator of cadBA expression. Negative regulation by LysP was further demonstrated by showing that lysP expression from a high-copy-number plasmid rendered cadA-lacZ uninducible. Expression of cadA-lacZ in a strain carrying the cadC310 allele, however, was not affected by the plasmid-expressed lysP. Cadaverine was shown to inhibit expression of the cadA-lacZ fusion in cadC+ cells but not in a cadC310 background.

摘要

大肠杆菌cadBA操纵子的表达需要至少两种细胞外信号:低pH值和高浓度赖氨酸,该操纵子编码赖氨酸转化为尸胺以及尸胺排泄所需的功能。为了更好地理解赖氨酸依赖性信号的本质,我们分离出了一些突变体,这些突变体在没有赖氨酸的情况下表达cadA-lacZ转录融合体,同时保留pH调节功能。其中一个分离株(EP310)中的相关突变位于cadC基因,该基因编码cadBA转录激活所必需的功能。这个突变(cadC310)位于编码CadC周质结构域的基因部分,导致第265位的精氨酸变为半胱氨酸,表明该蛋白的这一部分参与了对赖氨酸存在的应答。另外三个突变体的突变位于lysP(cadR)基因内部或附近,lysP基因编码一种赖氨酸转运蛋白,先前已证明该蛋白可调节cadA的表达。其中一个突变是lysP编码区的插入。因此,在没有外源赖氨酸的情况下,LysP是cadBA表达的负调节因子。通过显示来自高拷贝数质粒的lysP表达使cadA-lacZ不可诱导,进一步证明了LysP的负调节作用。然而,携带cadC310等位基因的菌株中cadA-lacZ的表达不受质粒表达的lysP的影响。已证明尸胺可抑制cadC+细胞中cadA-lacZ融合体的表达,但在cadC310背景下则不会。