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尿素通道的质子门控机制。

Mechanism of proton gating of a urea channel.

作者信息

Weeks David L, Gushansky Gene, Scott David R, Sachs George

机构信息

Department of Veterans Affairs Greater Los Angeles Healthcare System, Los Angeles, California 90073, USA.

出版信息

J Biol Chem. 2004 Mar 12;279(11):9944-50. doi: 10.1074/jbc.M312680200. Epub 2003 Dec 29.

DOI:10.1074/jbc.M312680200
PMID:14701805
Abstract

The size and complexity of many pH-gated channels have frustrated the development of specific structural models. The small acid-activated six-membrane segment urea channel of Helicobacter hepaticus (HhUreI), homologous to the essential UreI of the gastric pathogen Helicobacter pylori, enables identification of all the periplasmic sites of proton gating by site-directed mutagenesis. Exposure to external acidity enhances [(14)C]urea uptake by Xenopus oocytes expressing HhUreI, with half-maximal activity (pH(0.5)) at pH 6.8. A downward shift of pH(0.5) in single site mutants identified four of six protonatable periplasmic residues (His-50 at the boundary of the second transmembrane segment TM2, Glu-56 in the first periplasmic loop, Asp-59 at the boundary of TM3, and His-170 at the boundary of TM6) that affect proton gating. Asp-59 was the only site at which a protonatable residue appeared to be essential for pH gating. Mutation of Glu-110 or Glu-114 in PL2 did not affect the pH(0.5) of gating. A chimera, where the entire periplasmic domain of HhUreI was fused to the membrane domain of Streptococcus salivarius UreI (SsUreI), retained the pH-independent properties of SsUreI. Hence, proton gating of HhUreI likely depends upon the formation of hydrogen bonds by periplasmic residues that in turn produce conformational changes of the transmembrane domain. Further studies on HhUreI may facilitate understanding of other physiologically important pH-responsive channels.

摘要

许多pH门控通道的大小和复杂性阻碍了特定结构模型的发展。肝螺杆菌的小型酸激活六膜段尿素通道(HhUreI)与胃病原体幽门螺杆菌的必需UreI同源,通过定点诱变能够识别质子门控的所有周质位点。暴露于外部酸性环境会增强表达HhUreI的非洲爪蟾卵母细胞对[¹⁴C]尿素的摄取,在pH 6.8时具有半数最大活性(pH(0.5))。单一位点突变体中pH(0.5)的下移确定了六个可质子化周质残基中的四个(第二个跨膜段TM2边界处的His-50、第一个周质环中的Glu-56、TM3边界处的Asp-59以及TM6边界处的His-170),这些残基影响质子门控。Asp-59是唯一一个可质子化残基似乎对pH门控至关重要的位点。PL2中Glu-110或Glu-114的突变不影响门控的pH(0.5)。一种嵌合体,其中HhUreI的整个周质结构域与唾液链球菌UreI(SsUreI)的膜结构域融合,保留了SsUreI的pH非依赖性特性。因此,HhUreI的质子门控可能取决于周质残基形成氢键,进而导致跨膜结构域的构象变化。对HhUreI的进一步研究可能有助于理解其他生理上重要的pH响应通道。

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