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卵和鞭毛动力蛋白的同源性。ATP结合位点与一级结构的比较。

Homology of egg and flagellar dynein. Comparison of ATP-binding sites and primary structure.

作者信息

Pratt M M

出版信息

J Biol Chem. 1986 Jan 15;261(2):956-64.

PMID:2934392
Abstract

Unfertilized sea urchin eggs contain a Mg2+-ATPase which shares physical and enzymatic characteristics with dynein, the enzyme which powers ciliary and flagellar movement. To further investigate the homology of the egg ATPase and axonemal dynein, ATP-binding subunits in preparations of each of the enzymes were identified using a photoaffinity probe of ATP, 8-azido-ATP (8-N3ATP), and three high molecular weight (HMW) polypeptide components of the two enzymes were compared by one-dimensional peptide mapping. Two heavy chains (A and B) of both the flagellar and egg ATPases bound [alpha-32P]8-N3ATP. The labeling of the HMW bands was specifically inhibited by ATP or ADP. Both the cytoplasmic ATPase and flagellar dynein utilized 8-N3ATP as a substrate indicating that the reagent binds to the active site. The two HMW ATP-binding polypeptides and one other HMW component of the egg ATPase were compared to flagellar dynein heavy chains by peptide mapping. Digestion of the egg versus flagellar HMW polypeptides with Staphylococcus V8 protease or alpha-chymotrypsin produced a highly similar group of peptides, and each pair of heavy chains was qualitatively estimated to be over 85% homologous. These data support the identification of the egg ATPase heavy chains as components of a cytoplasmic dynein and suggest that the HMW polypeptides form active enzymatic sites in flagellar and egg dynein which are substantially homologous.

摘要

未受精的海胆卵含有一种Mg2+ -ATP酶,它与动力蛋白在物理和酶学特性上有共同之处,动力蛋白是驱动纤毛和鞭毛运动的酶。为了进一步研究卵ATP酶与轴丝动力蛋白的同源性,使用ATP的光亲和探针8-叠氮基ATP(8-N3ATP)鉴定了每种酶制剂中的ATP结合亚基,并通过一维肽图比较了这两种酶的三种高分子量(HMW)多肽成分。鞭毛ATP酶和卵ATP酶的两条重链(A和B)都结合了[α-32P]8-N3ATP。HMW条带的标记被ATP或ADP特异性抑制。细胞质ATP酶和鞭毛动力蛋白都将8-N3ATP用作底物,这表明该试剂与活性位点结合。通过肽图将卵ATP酶的两种HMW ATP结合多肽和另一种HMW成分与鞭毛动力蛋白重链进行了比较。用葡萄球菌V8蛋白酶或α-胰凝乳蛋白酶消化卵与鞭毛的HMW多肽产生了一组高度相似的肽,并且定性估计每对重链的同源性超过85%。这些数据支持将卵ATP酶重链鉴定为细胞质动力蛋白的成分,并表明HMW多肽在鞭毛和卵动力蛋白中形成了基本同源的活性酶位点。

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