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来自卡氏棘阿米巴的肌动蛋白缺乏氨基末端加工。

Lack of NH2-terminal processing of actin from Acanthamoeba castellanii.

作者信息

Redman K L, Martin D J, Korn E D, Rubenstein P A

出版信息

J Biol Chem. 1985 Nov 25;260(27):14857-61.

PMID:4055803
Abstract

Acanthamoeba actin is the only actin sequenced to date that has neither an NH2-terminal Ac-Asp nor Ac-Glu residue. The protein begins with an Ac-Gly-Asp and is coded for by a gene that specifies a polypeptide beginning Met-Gly-Asp. Thus, the Acanthamoeba actin gene would appear to specify a class II actin with the usual NH2-terminal Cys replaced with a Gly. Previous studies (Rubenstein, P. A., and Martin, D. J. (1983) J. Biol. Chem. 258, 11354-11360) revealed that for class II actins the Met is probably removed early in translation and the Cys is removed post-translationally as an Ac-Cys residue. Two possibilities might explain why Acanthamoeba actin is not processed in a similar fashion. Either Ac-Gly is not a substrate for the enzyme or the enzyme is absent from the organism. To test these alternatives, Acanthamoeba actin was labeled in vivo with [35S]methionine and incubated with processing enzyme from rat liver, rabbit reticulocytes, and Dictyostelium. In no case did the processing reaction occur, indicating that Ac-Gly is not recognized by the enzyme as a substrate. Furthermore, we could not reproducibly detect the presence of a processing enzyme in Acanthamoeba. We were, however, able to show the presence of such an enzyme in Dictyostelium, the first demonstration of this activity in a lower eukaryote.

摘要

棘阿米巴肌动蛋白是迄今为止唯一一种既没有NH2末端的乙酰天冬氨酸残基也没有乙酰谷氨酸残基的已测序肌动蛋白。该蛋白质以乙酰甘氨酰天冬氨酸开头,由一个编码从甲硫氨酸-甘氨酰天冬氨酸开始的多肽的基因编码。因此,棘阿米巴肌动蛋白基因似乎指定了一种II类肌动蛋白,其通常的NH2末端半胱氨酸被甘氨酸取代。先前的研究(鲁宾斯坦,P.A.,和马丁,D.J.(1983年)《生物化学杂志》258,11354 - 11360)表明,对于II类肌动蛋白,甲硫氨酸可能在翻译早期被去除,半胱氨酸在翻译后作为乙酰半胱氨酸残基被去除。有两种可能性可以解释为什么棘阿米巴肌动蛋白没有以类似的方式进行加工。要么乙酰甘氨酸不是该酶的底物,要么该生物体中不存在这种酶。为了测试这些可能性,棘阿米巴肌动蛋白在体内用[35S]甲硫氨酸标记,并与来自大鼠肝脏、兔网织红细胞和盘基网柄菌的加工酶一起孵育。在任何情况下加工反应都没有发生,这表明乙酰甘氨酸不被该酶识别为底物。此外,我们无法在棘阿米巴中可重复地检测到加工酶的存在。然而,我们能够在盘基网柄菌中显示出这种酶的存在,这是在低等真核生物中首次证明这种活性。

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