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镁 - 三磷酸腺苷酶与电鳐胆碱能突触小泡

Mg-ATPase and Torpedo cholinergic synaptic vesicles.

作者信息

Diebler M F, Lazereg S

出版信息

J Neurochem. 1985 May;44(5):1633-41. doi: 10.1111/j.1471-4159.1985.tb08806.x.

Abstract

The reported presence of Mg-ATPase activity in cholinergic synaptic vesicles from the electric organ of Torpedo marmorata was reinvestigated in view of possible contamination of vesicles by other subcellular fractions. After dilution in concentrated sucrose, the vesicular fraction isolated on a sedimentation sucrose gradient was purified further on a flotation density gradient. It appears that this treatment allows separation of the vesicles according to their content. The two vesicular content markers, acetylcholine and ATP, are recovered as sharp coincident peaks at a density close to 0.48 M sucrose. Empty vesicles are identified in denser regions by the protein pattern on gel electrophoresis which is identical to the pattern obtained for filled vesicles. Refractionation of vesicles depleted of their acetylcholine content by valinomycin leads to an extreme picture, with a massive shift of the vesicles toward denser regions. We have then shown that a ouabain-insensitive Mg-ATPase is indeed associated with the vesicle membrane, but the activity is fully apparent only when vesicles are permeabilized either as the result of the fractionation procedure or after detergent treatment. The relative insensitivity of the Mg-ATPase associated with the synaptic vesicles to oligomycin, N,N'-dicyclohexylcarbodiimide, and azide indicates that this enzyme differs from the classic F1F0 mitochondrial enzyme. The most striking finding is the sensitivity to vanadate of the vesicular Mg-ATPase, which suggests the involvement of a phosphorylated intermediate. On the basis of both the difference in inhibitor sensitivity between untreated and detergent-treated vesicles and of the pronase experiments, the possibility that the enzyme has an inward orientation is discussed.

摘要

鉴于电鳐电器官的胆碱能突触小泡可能被其他亚细胞组分污染,我们重新研究了已报道的该突触小泡中镁 - ATP酶活性的存在情况。在浓蔗糖中稀释后,通过沉降蔗糖梯度分离得到的小泡组分在浮选密度梯度上进一步纯化。看来这种处理能够根据小泡的内容物进行分离。两种小泡内容物标记物,乙酰胆碱和ATP,在密度接近0.48M蔗糖处作为尖锐的重合峰被回收。空泡通过凝胶电泳上的蛋白质图谱在密度更高的区域被鉴定出来,该图谱与充满小泡所获得的图谱相同。用缬氨霉素耗尽乙酰胆碱含量的小泡再分级导致了一种极端情况,小泡大量向密度更高的区域移动。然后我们表明,一种哇巴因不敏感的镁 - ATP酶确实与小泡膜相关,但只有当小泡由于分级分离过程或去污剂处理而通透性增加时,该活性才会完全显现。与突触小泡相关的镁 - ATP酶对寡霉素、N,N'-二环己基碳二亚胺和叠氮化物的相对不敏感性表明该酶不同于经典的F1F0线粒体酶。最引人注目的发现是小泡镁 - ATP酶对钒酸盐敏感,这表明涉及一个磷酸化中间体。基于未处理和经去污剂处理的小泡之间抑制剂敏感性的差异以及链霉蛋白酶实验结果,讨论了该酶具有向内取向的可能性。

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