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磷脂酶A2与脂质双层结合时脂质-蛋白质微界面的脱水作用。

Dehydration of the lipid-protein microinterface on binding of phospholipase A2 to lipid bilayers.

作者信息

Jain M K, Vaz W L

机构信息

Department of Chemistry, University of Delaware, Newark 19716.

出版信息

Biochim Biophys Acta. 1987 Nov 27;905(1):1-8. doi: 10.1016/0005-2736(87)90002-2.

Abstract

A novel method is described to demonstrate inaccessibility to the bulk aqueous phase of the microinterface between pig pancreatic phospholipase A2 and lipid bilayers to which this protein is bound. The method is based on the fact that the fluorescence emission quantum yields of the tryptophan residue of the protein and of a 5-dimethylaminonaphthalene-1-sulfonyl (dansyl) chromophore attached to a lipid are lower in water as compared to that in deuterated water. The fluorescence emission quantum yield of these chromophores is measured in water and in deuterated water under conditions where the protein is either bound or not bound to the surface of a lipid bilayer containing the dansyl chromophore. Under conditions where the protein is tightly bound to the surface of the bilayer, desolvation of both fluorophores abolishes the observed effect of deuterated water. The tryptophan residue in the bound phospholipase A2 also becomes inaccessible to fluorescence quenching by acrylamide or succinimide. Desolvation of the microinterface is observed only under conditions that are significant for the catalytic action of phospholipase A2 in the scooting mode and not in the hopping mode. Also, under similar conditions, binding of pro-phospholipase A2 to anionic vesicles does not cause dehydration of the microinterface. The mechanistic significance of these observations for lipid-protein interactions, in general, and for interfacial catalysis and interfacial activation, in particular, is discussed.

摘要

本文描述了一种新方法,用于证明猪胰磷脂酶A2与该蛋白所结合的脂质双层微界面的本体水相不可及。该方法基于以下事实:与在重水中相比,蛋白质中色氨酸残基以及连接到脂质上的5-二甲基氨基萘-1-磺酰基(丹磺酰)发色团在水中的荧光发射量子产率较低。在蛋白质与含有丹磺酰发色团的脂质双层表面结合或未结合的条件下,分别在水和重水中测量这些发色团的荧光发射量子产率。在蛋白质紧密结合到双层表面的条件下,两种荧光团的去溶剂化消除了观察到的重水效应。结合的磷脂酶A2中的色氨酸残基也无法被丙烯酰胺或琥珀酰亚胺进行荧光猝灭。仅在对磷脂酶A2以滑动模式而非跳跃模式进行催化作用具有重要意义的条件下,才观察到微界面的去溶剂化。同样,在类似条件下,前磷脂酶A2与阴离子囊泡的结合不会导致微界面脱水。本文讨论了这些观察结果对于一般脂质-蛋白质相互作用,特别是对于界面催化和界面活化的机制意义。

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