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鉴定微管上一类独特的长春碱结合位点。

Identification of a distinct class of vinblastine binding sites on microtubules.

作者信息

Jordan M A, Margolis R L, Himes R H, Wilson L

出版信息

J Mol Biol. 1986 Jan 5;187(1):61-73. doi: 10.1016/0022-2836(86)90406-7.

Abstract

Vinblastine, at concentrations above approximately 1 to 2 microM, causes depolymerization of steady-state bovine brain microtubules in vitro by a fraying of microtubule ends into protofilament-like spirals. Microtubule depolymerization is associated with the binding of vinblastine in approximately molar stoichiometry to tubulin in microtubules with apparent low affinity, as determined by binding experiments with radiolabeled vinblastine and by the ability of vinblastine to inhibit DEAE-dextran decoration of microtubule surfaces. Our data suggest that depolymerization occurs by a propagated mechanism, initially involving binding of vinblastine to a limited number of available sites on microtubule surfaces. This appears to cause loosening of protofilament associations which results in the exposure of new vinblastine-binding sites. Additional vinblastine binding in turn results in further loosening of protofilament associations. Such loosening, when it occurs at microtubule ends, results in protofilament-like splaying and end-wise depolymerization. Microtubule depolymerization appears mechanistically distinct from inhibition of microtubule polymerization by the drug, which is associated with the binding of vinblastine to small numbers of high-affinity binding sites on tubulin at one or both microtubule ends.

摘要

长春碱在浓度高于约1至2微摩尔时,会使体外稳态牛脑微管发生解聚,其方式是微管末端磨损成原纤维样螺旋。微管解聚与长春碱以近似摩尔化学计量比与微管中的微管蛋白结合有关,结合亲和力明显较低,这是通过用放射性标记的长春碱进行结合实验以及长春碱抑制微管表面二乙氨基乙基葡聚糖修饰的能力确定的。我们的数据表明,解聚是通过一种传播机制发生的,最初涉及长春碱与微管表面有限数量的可用位点结合。这似乎会导致原纤维结合松散,从而暴露出新的长春碱结合位点。额外的长春碱结合反过来又会导致原纤维结合进一步松散。当这种松散发生在微管末端时,会导致原纤维样展开和末端解聚。微管解聚在机制上似乎与该药物抑制微管聚合不同,后者与长春碱在一个或两个微管末端与微管蛋白上少量高亲和力结合位点的结合有关。

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