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首页> 外文期刊>Journal of Molecular Biology >Is 2-phosphoglycerate-dependent automodification of bacterial enolases implicated in their export?
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Is 2-phosphoglycerate-dependent automodification of bacterial enolases implicated in their export?

机译:细菌烯醇酶的2-磷酸甘油酸酯依赖性自动修饰与它们的出口有关吗?

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摘要

We observed that in vivo and in vitro a small fraction of the glycolytic enzyme enolase became covalently modified by its substrate 2-phosphoglycerate (2-PG). In modified Escherichia coli enolase, 2-PG was bound to Lys341, which is located in the active site. An identical reversible modification was observed with other bacterial enolases, but also with enolase from Saccharomyces cerevisiae and rabbit muscle. An equivalent of Lys341, which plays an important role in catalysis, is present in enolase of all organisms. Covalent binding of 2-PG to this amino acid rendered the enzyme inactive. Replacement of Lys341 of E. coli enolase with other amino acids prevented the automodification and in most cases strongly reduced the activity. As reported for other bacteria, a significant fraction of E. coli enolase was found to be exported into the medium. Interestingly, all Lys341 substitutions prevented not only the automodification, but also the export of enolase. The K341E mutant enolase was almost as active as the wild-type enzyme and therefore allowed us to establish that the loss of enolase export correlates with the loss of modification and not the loss of glycolytic activity. (C) 2004 Elsevier Ltd. All rights reserved. [References: 43]
机译:我们观察到在体内和体外,一小部分的糖酵解酶烯醇酶被其底物2-磷酸甘油酸酯(2-PG)共价修饰。在修饰的大肠杆菌烯醇化酶中,2-PG与位于活性位点的Lys341结合。用其他细菌烯醇酶观察到相同的可逆修饰,但是用酿酒酵母和兔肌肉的烯醇酶观察到相同的可逆修饰。在所有生物的烯醇酶中都存在与Lys341等价的物质,在催化中起重要作用。 2-PG与该氨基酸的共价结合使该酶失活。用其他氨基酸替换大肠杆菌烯醇酶的Lys341可以防止自修饰,并且在大多数情况下会大大降低其活性。如对其他细菌的报道,发现很大一部分大肠杆菌烯醇化酶被出口到培养基中。有趣的是,所有Lys341取代不仅阻止了自动修饰,而且阻止了烯醇酶的输出。 K341E突变型烯醇酶的活性几乎与野生型酶相同,因此使我们能够确定烯醇酶输出的丧失与修饰的丧失而不是糖酵解活性的丧失有关。 (C)2004 Elsevier Ltd.保留所有权利。 [参考:43]

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