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网格蛋白片段与被膜小泡膜的关联。

The association of clathrin fragments with coated vesicle membranes.

作者信息

Hanspal M, Luna E, Branton D

出版信息

J Biol Chem. 1984 Sep 10;259(17):11075-82.

PMID:6147350
Abstract

The association between clathrin triskelions and the clathrin-stripped membranes of coated vesicles has been investigated using a filter assay to separate bound from unbound clathrin. The filter assay is more sensitive and less cumbersome than a sedimentation assay used previously (1). While confirming the high affinity interaction between clathrin and the vesicle membrane, our results yield Scatchard plots that are curvilinear and consistent with a positively cooperative interaction between clathrin and the vesicle membranes. Controlled digestion with trypsin removes the distal portions of the triskelion legs leaving the proximal 31 nm portions that form the hub of the triskelions. These hubs are trimers of large 112,000- and 124,000-dalton fragments of clathrin heavy chains. They competitively inhibit the binding of 125I-labeled intact triskelions to stripped vesicles with a KI identical to the KD for the association of 125I-labeled intact triskelions to stripped vesicles. Furthermore, these large fragment trimers bind to stripped vesicles with approximately the same high affinity as do intact triskelions and also show evidence of a positively cooperative interaction. It is concluded that clathrin binds to coated vesicles by an interaction that is mediated by the proximal 112,000-dalton fragment of the clathrin heavy chains.

摘要

利用一种过滤分析法来分离结合的网格蛋白和未结合的网格蛋白,从而研究了网格蛋白三脚复合体与被剥离网格蛋白的包被小泡膜之间的关联。这种过滤分析法比之前使用的沉降分析法更灵敏且更简便(1)。在证实网格蛋白与小泡膜之间存在高亲和力相互作用的同时,我们的结果得出的斯卡查德图呈曲线状,这与网格蛋白和小泡膜之间的正协同相互作用一致。用胰蛋白酶进行的控制性消化去除了三脚复合体腿的远端部分,留下近端31纳米的部分,这些部分形成了三脚复合体的中心。这些中心是由112,000道尔顿和124,000道尔顿的网格蛋白重链大片段组成的三聚体。它们以与125I标记的完整三脚复合体与被剥离小泡结合的解离常数相同的抑制常数,竞争性抑制125I标记的完整三脚复合体与被剥离小泡的结合。此外,这些大片段三聚体与被剥离小泡的结合亲和力与完整三脚复合体大致相同,并且也显示出正协同相互作用的证据。得出的结论是,网格蛋白通过由网格蛋白重链近端112,000道尔顿片段介导的相互作用与包被小泡结合。

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