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大肠杆菌的耐酸性:pH 感应、氯离子激活以及 GadB 中的自抑制作用

Escherichia coli acid resistance: pH-sensing, activation by chloride and autoinhibition in GadB.

作者信息

Gut Heinz, Pennacchietti Eugenia, John Robert A, Bossa Francesco, Capitani Guido, De Biase Daniela, Grütter Markus G

机构信息

Biochemisches Institut der Universität Zürich, Zürich, Switzerland.

出版信息

EMBO J. 2006 Jun 7;25(11):2643-51. doi: 10.1038/sj.emboj.7601107. Epub 2006 May 4.

Abstract

Escherichia coli and other enterobacteria exploit the H+ -consuming reaction catalysed by glutamate decarboxylase to survive the stomach acidity before reaching the intestine. Here we show that chloride, extremely abundant in gastric secretions, is an allosteric activator producing a 10-fold increase in the decarboxylase activity at pH 5.6. Cooperativity and sensitivity to chloride were lost when the N-terminal 14 residues, involved in the formation of two triple-helix bundles, were deleted by mutagenesis. X-ray structures, obtained in the presence of the substrate analogue acetate, identified halide-binding sites at the base of each N-terminal helix, showed how halide binding is responsible for bundle stability and demonstrated that the interconversion between active and inactive forms of the enzyme is a stepwise process. We also discovered an entirely novel structure of the cofactor pyridoxal 5'-phosphate (aldamine) to be responsible for the reversibly inactivated enzyme. Our results link the entry of chloride ions, via the H+/Cl- exchange activities of ClC-ec1, to the trigger of the acid stress response in the cell when the intracellular proton concentration has not yet reached fatal values.

摘要

大肠杆菌和其他肠杆菌利用谷氨酸脱羧酶催化的消耗氢离子的反应,在到达肠道之前在胃酸环境中存活下来。我们在此表明,胃分泌物中含量极为丰富的氯离子是一种变构激活剂,在pH 5.6时可使脱羧酶活性提高10倍。当通过诱变删除参与形成两个三螺旋束的N端14个残基时,协同性和对氯离子的敏感性丧失。在存在底物类似物乙酸盐的情况下获得的X射线结构,确定了每个N端螺旋底部的卤化物结合位点,展示了卤化物结合如何导致螺旋束稳定性,并证明酶的活性形式与非活性形式之间的相互转化是一个逐步过程。我们还发现了辅因子磷酸吡哆醛(醛胺)的一种全新结构,它是导致酶可逆失活的原因。我们的结果将氯离子通过ClC-ec1的H⁺/Cl⁻交换活性进入细胞,与细胞内质子浓度尚未达到致命值时酸应激反应的触发联系起来。

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