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间隙连接蛋白氨基末端的结构。

Structure of the amino terminus of a gap junction protein.

作者信息

Purnick P E, Benjamin D C, Verselis V K, Bargiello T A, Dowd T L

机构信息

Department of Neuroscience, Albert Einstein College of Medicine, Bronx, New York 10461, USA.

出版信息

Arch Biochem Biophys. 2000 Sep 15;381(2):181-90. doi: 10.1006/abbi.2000.1989.

DOI:10.1006/abbi.2000.1989
PMID:11032405
Abstract

Charged amino acid residues in the amino terminus of gap junction forming proteins (connexins) form part, if not all, of the transjunctional voltage sensor of gap junction channels and play a fundamental role in ion permeation. Results from studies of the voltage dependence of N-terminal mutants predict that residues 1-10 of Group I connexins lie within the channel pore and that the N-terminus forms the channel vestibule by the creation of a turn initiated by the conserved G12 residue. Here we report that intercellular channels containing mutations of G12 in Cx32 to residues that are likely to interfere with flexibility of this locus (G12S, G12Y, and G12V) do not express junctional currents, whereas a connexin containing a proline residue at G12 (Cx32G12P), which is expected to maintain a structure similar to that of the G12 locus, forms nearly wild-type channels. We have solved the structure of an N-terminal peptide of Cx26 (MDWGTLQSILGGVNK) using 1H 2D NMR. The peptide contains two structured domains connected by a flexible hinge (domain-hinge-domain motif) that would allow the placement of the amino terminus within the channel pore. Residues 1-10 adopt a helical conformation and line the channel entrance while residues 12-15 form an open turn. Overall, there is good agreement between the structural and dynamic features of the N-terminal peptide provided by NMR and the functional studies of the voltage dependence of channels formed by wild-type and N-terminal mutations.

摘要

间隙连接形成蛋白(连接蛋白)氨基末端的带电荷氨基酸残基,即便不是间隙连接通道跨连接电压传感器的全部组成部分,也是其一部分,并且在离子通透中发挥着重要作用。对氨基末端突变体电压依赖性的研究结果预测,I 组连接蛋白的 1 - 10 位残基位于通道孔内,并且氨基末端通过由保守的 G12 残基引发的一个转角的形成而构成通道前庭。在此我们报告,在 Cx32 中含有 G12 突变为可能干扰该位点灵活性的残基(G12S、G12Y 和 G12V)的细胞间通道不表达连接电流,而在 G12 处含有脯氨酸残基的连接蛋白(Cx32G12P),预计其维持与 G12 位点相似的结构,能形成近乎野生型的通道。我们使用 1H 2D NMR 解析了 Cx26 的氨基末端肽(MDWGTLQSILGGVNK)的结构。该肽包含两个由柔性铰链连接的结构化结构域(结构域 - 铰链 - 结构域基序),这将允许氨基末端置于通道孔内。1 - 10 位残基呈螺旋构象并排列在通道入口处,而 12 - 15 位残基形成一个开放转角。总体而言,NMR 提供的氨基末端肽的结构和动态特征与野生型和氨基末端突变体形成的通道电压依赖性的功能研究之间存在良好的一致性。

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Structure of the amino terminus of a gap junction protein.间隙连接蛋白氨基末端的结构。
Arch Biochem Biophys. 2000 Sep 15;381(2):181-90. doi: 10.1006/abbi.2000.1989.
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Structural studies of N-terminal mutants of connexin 32 using (1)H NMR spectroscopy.使用(1)H NMR 光谱学研究连接蛋白 32 的 N 端突变体。
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Emerging issues of connexin channels: biophysics fills the gap.连接蛋白通道的新问题:生物物理学填补空白。
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The role of a conserved proline residue in mediating conformational changes associated with voltage gating of Cx32 gap junctions.一个保守脯氨酸残基在介导与Cx32间隙连接电压门控相关的构象变化中的作用。
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