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探究肌动蛋白的鬼笔环肽结合位点。

Probing the phalloidin binding site of actin.

作者信息

Faulstich H, Zobeley S, Heintz D, Drewes G

机构信息

Max-Planck-Institut für Medizinische Forschung, Heidelberg, Germany.

出版信息

FEBS Lett. 1993 Mar 8;318(3):218-22. doi: 10.1016/0014-5793(93)80515-v.

DOI:10.1016/0014-5793(93)80515-v
PMID:8440376
Abstract

Phallotoxins form tight complexes with filamentous actin and stabilize the polymer against shearing stress. In the present study a phalloidin derivative containing a thiol-capturing moiety was prepared and reacted with single thiol groups of monomeric muscle actin. Sites of attachment in the protein were Cys-374 next to the C-terminus and Cys-10, close to the N-terminus; the latter was recently shown to be uncovered during a slow but reversible conformational transition occurring in ADP-G-actin. Phalloidin bound to Cys-374 stabilizes filaments against shearing stress almost as effectively as free phalloidin, indicating that the phalloidin binding site cannot be far from the C-terminus of actin. Stabilization was also achieved when the phalloidin reagent was added to F-actin, however, the subsequent formation of a covalent linkage with Cys-374 was not observed, most likely due to a restricted mobility of the reactants. In contrast to the efficient stabilization of filaments by phalloidin linked to Cys-374 a destabilizing effect was observed when phalloidin was attached to Cys-10. It appears that phalloidin located close to the N-terminus is unable to bind to the normal binding site in its own filament. Pronounced gelification of this actin derivative suggests that the toxin is able to mediate crosslinking with neighbouring filaments. From these results we conclude that the phalloidin binding site of actin is distant from the N-terminus, but close to the C-terminus. Furthermore, the data provide evidence that binding of phalloidin reduces the mobility of the C-terminus.

摘要

鬼笔毒素与丝状肌动蛋白形成紧密复合物,并使聚合物稳定以抵抗剪切力。在本研究中,制备了一种含有硫醇捕获基团的鬼笔环肽衍生物,并使其与单体肌肉肌动蛋白的单个硫醇基团反应。蛋白质中的附着位点是靠近C末端的Cys-374和靠近N末端的Cys-10;最近发现,在ADP-G-肌动蛋白中发生的缓慢但可逆的构象转变过程中,后者会暴露出来。与Cys-374结合的鬼笔环肽稳定细丝抵抗剪切力的效果几乎与游离鬼笔环肽一样有效,这表明鬼笔环肽结合位点离肌动蛋白的C末端不远。当将鬼笔环肽试剂添加到F-肌动蛋白中时也实现了稳定化,然而,未观察到随后与Cys-374形成共价键,这很可能是由于反应物的迁移受限。与连接到Cys-374的鬼笔环肽对细丝的有效稳定作用相反,当鬼笔环肽连接到Cys-10时观察到了去稳定化作用。似乎位于靠近N末端的鬼笔环肽无法与其自身细丝中的正常结合位点结合。这种肌动蛋白衍生物明显的凝胶化表明该毒素能够介导与相邻细丝的交联。从这些结果我们得出结论,肌动蛋白的鬼笔环肽结合位点远离N末端,但靠近C末端。此外,数据提供了证据表明鬼笔环肽的结合降低了C末端的迁移率。

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