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ADP-核糖基精氨酸糖水解酶催化从霍乱毒素修饰的GTP结合蛋白α亚基中释放ADP-核糖。

ADP-ribosylarginine glycohydrolase catalyzing the release of ADP-ribose from the cholera toxin-modified alpha-subunits of GTP-binding proteins.

作者信息

Maehama T, Nishina H, Katada T

机构信息

Department of Life Science, Tokyo Institute of Technology, Yokohama.

出版信息

J Biochem. 1994 Nov;116(5):1134-8. doi: 10.1093/oxfordjournals.jbchem.a124639.

DOI:10.1093/oxfordjournals.jbchem.a124639
PMID:7896743
Abstract

A rat glycohydrolase which catalyzes the hydrolysis of ADP-ribosylarginine was expressed in Escherichia coli and purified to homogeneity for characterization of its enzymatic properties. The purified glycohydrolase catalyzed the hydrolysis of N-glycoside linked ADP-ribosylarginine on the alpha-subunits of stimulatory GTP-binding proteins (Gs) and cholera toxin A1-subunit that had been modified by cholera toxin and NAD. Nonmuscle actin of which an arginine residue was ADP-ribosylated by botulinum C2 toxin also served as a substrate of the glycohydrolase. On the other hand, the glycohydrolase did not hydrolyze ADP-ribosylated cysteine on the alpha-subunits of pertussis toxin-substrate GTP-binding proteins, ADP-ribosylated diphthamide on elongation factor 2, or ADP-ribosylated asparagine on rho GTP-binding proteins. The rate of the reaction catalyzed by the glycohydrolase was affected by nucleotide-binding form of the ADP-ribosylated substrate proteins; the GDP-bound form of the modified Gs-alpha was more rapidly hydrolyzed than the guanosine 5'-(3-O-thio)triphosphate-bound form. Interestingly, the glycohydrolase activity was markedly inhibited by mM order concentration of ATP in addition to ADP-ribose, the product of the enzyme reaction, though ADP had no inhibitory effect on the activity. Moreover, alpha NAD, but not beta NAD, inhibited the enzyme activity, suggesting that the glycohydrolase reaction was stereospecific for the alpha-anomer.

摘要

一种催化ADP - 核糖基精氨酸水解的大鼠糖水解酶在大肠杆菌中表达,并纯化至同质以表征其酶学性质。纯化的糖水解酶催化经霍乱毒素和NAD修饰的刺激性GTP结合蛋白(Gs)α亚基及霍乱毒素A1亚基上N - 糖苷键连接的ADP - 核糖基精氨酸的水解。肉毒杆菌C2毒素使精氨酸残基ADP - 核糖基化的非肌肉肌动蛋白也作为该糖水解酶的底物。另一方面,该糖水解酶不水解百日咳毒素底物GTP结合蛋白α亚基上的ADP - 核糖基化半胱氨酸、延伸因子2上的ADP - 核糖基化双氢酰胺或rho GTP结合蛋白上的ADP - 核糖基化天冬酰胺。糖水解酶催化的反应速率受ADP - 核糖基化底物蛋白的核苷酸结合形式影响;修饰的Gs - α的GDP结合形式比鸟苷5' -(3 - O - 硫代)三磷酸结合形式水解得更快。有趣的是,除了酶反应产物ADP - 核糖外,毫摩尔级浓度的ATP也显著抑制该糖水解酶活性,尽管ADP对该活性无抑制作用。此外,α - NAD而非β - NAD抑制酶活性,表明糖水解酶反应对α - 异头物具有立体特异性。

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