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由分离的跨膜结构域和细胞质结构域形成CLC-0氯离子通道。

Formation of CLC-0 chloride channels from separated transmembrane and cytoplasmic domains.

作者信息

Maduke M, Williams C, Miller C

机构信息

Howard Hughes Medical Institute, Department of Biochemistry, Brandeis University, Waltham, Massachusetts, USA.

出版信息

Biochemistry. 1998 Feb 3;37(5):1315-21. doi: 10.1021/bi972418o.

Abstract

CLC-0, a member of the CLC family of Cl(-)-conducting ion channels, consists of an N-terminal hydrophobic core and a C-terminal region that is thought to be cytoplasmic. This study provides evidence that the C-terminal region is a mechanistically relevant cytoplasmic domain of the CLC-0 ion channel. Both a point mutation and a 37-residue deletion in this region cause drastic alterations in voltage-dependent gating of CLC-0 current expressed in Xenopus oocytes. CLC-0 current is not observed when the entire C-terminal region is deleted, but functional channels are efficiently reconstituted by co-injection of separate cRNA constructs encoding the N-terminal transmembrane and the C-terminal cytoplasmic domains. Moreover, reconstitution of CLC-0 can be achieved by co-injection of cRNA encoding the transmembrane domain along with Escherichia coli-expressed C-terminal domain polypeptide.

摘要

CLC-0是氯离子传导离子通道CLC家族的成员之一,由一个N端疏水核心和一个被认为位于细胞质的C端区域组成。本研究提供了证据表明,C端区域是CLC-0离子通道一个在机制上相关的细胞质结构域。该区域的一个点突变和一个37个残基的缺失都会导致非洲爪蟾卵母细胞中表达的CLC-0电流的电压依赖性门控发生剧烈改变。当整个C端区域被删除时,未观察到CLC-0电流,但通过共注射分别编码N端跨膜结构域和C端细胞质结构域的cRNA构建体,可以有效地重建功能性通道。此外,通过共注射编码跨膜结构域的cRNA与大肠杆菌表达的C端结构域多肽,可以实现CLC-0的重建。

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