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跨膜结构域1中的氨基酸替换影响大肠杆菌传感器激酶KdpD的渗透感应,但不影响钾离子感应。

Amino acid replacements in transmembrane domain 1 influence osmosensing but not K+ sensing by the sensor kinase KdpD of Escherichia coli.

作者信息

Stallkamp Iris, Altendorf Karlheinz, Jung Kirsten

机构信息

Universität Osnabrück, Fachbereich Biologie/Chemie, Abteilung Mikrobiologie, 49069 Osnabrück, Germany.

出版信息

Arch Microbiol. 2002 Dec;178(6):525-30. doi: 10.1007/s00203-002-0485-4. Epub 2002 Oct 3.

Abstract

Expression of the kdpFABC operon coding for the high affinity K+ -translocating KdpFABC complex of Escherichia coli is induced by K+ limitation or high osmolality. This process is controlled by the sensor kinase/response regulator system KdpD/KdpE. To study the importance of the transmembrane domains of KdpD for stimulus perception, each amino acid residue of the transmembrane domain 1 and Asp-424 of the adjacent periplasmic loop were replaced with Cys in a KdpD derivative devoid of native Cys residues. In vivo analysis of KdpD proteins with a single Cys residue revealed that 14 out of 18 amino acid replacements caused an altered response towards an osmotic upshift imposed by NaCl, whereby only four replacements also altered the response towards changes in the K+ concentration. The in vitro activities of most of the KdpD derivatives were in the range of KdpD devoid of native Cys residues. The results reveal that the osmosensing and K+ -sensing properties of KdpD can be dissected. Furthermore, the data support the hypothesis that osmosensing involves amino acid residues of the transmembrane domains.

摘要

编码大肠杆菌高亲和力钾离子转运KdpFABC复合体的kdpFABC操纵子的表达受钾离子限制或高渗透压诱导。这一过程由传感激酶/反应调节系统KdpD/KdpE控制。为了研究KdpD跨膜结构域对刺激感知的重要性,在一个不含天然半胱氨酸残基的KdpD衍生物中,将跨膜结构域1的每个氨基酸残基和相邻周质环的Asp-424替换为半胱氨酸。对具有单个半胱氨酸残基的KdpD蛋白进行体内分析发现,18个氨基酸替换中有14个导致对NaCl引起的渗透压升高的反应改变,其中只有4个替换也改变了对钾离子浓度变化的反应。大多数KdpD衍生物的体外活性与不含天然半胱氨酸残基的KdpD活性范围相同。结果表明,KdpD的渗透压感知和钾离子感知特性可以被区分。此外,数据支持渗透压感知涉及跨膜结构域氨基酸残基的假说。

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