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6-磷酸葡萄糖胺脱氨酶(NagB)的变构调节与大肠杆菌利用葡萄糖胺的生长

Allosteric regulation of glucosamine-6-phosphate deaminase (NagB) and growth of Escherichia coli on glucosamine.

作者信息

Alvarez-Añorve Laura I, Bustos-Jaimes Ismael, Calcagno Mario L, Plumbridge Jacqueline

机构信息

Institut de Biologie Physico-Chimique, (UPR9073-CNRS), 13 rue Pierre et Marie Curie, 75005 Paris, France.

出版信息

J Bacteriol. 2009 Oct;191(20):6401-7. doi: 10.1128/JB.00633-09. Epub 2009 Aug 21.

Abstract

Growth on N-acetylglucosamine (GlcNAc) produces intracellular N-acetylglucosamine-6-phosphate (GlcNAc6P), which affects the regulation of the catabolism of amino sugars in Escherichia coli in two ways. First, GlcNAc6P is the inducing signal for the NagC repressor, and thus it increases the expression of the enzymes of the nagE-nagBACD operon. Second, it is the allosteric activator of glucosamine-6P (GlcN6P) deaminase, NagB, and thus increases the catalytic capacity of this key enzyme in the metabolism of amino sugars. We showed previously that both the level of expression of the nagB gene and the transport of glucosamine were limiting the growth rate on GlcN (L. I. Alvarez-Añorve et al., J. Bacteriol. 187:2974-2982, 2005). We were unable to conclude if the lack of allosteric activation of wild-type NagB was also contributing to the slower growth rate on GlcN. Using a single-copy plasmid, with a constitutive promoter, we have separated the effects of GlcNAc6P on the NagB protein level and on deaminase activity. We show that over a range of intracellular NagB concentrations it is the quantity of the substrate, GlcN6P, which is limiting growth rather than the concentration of the allosteric activator, GlcNAc6P. On the other hand, the F174A mutant of NagB, which requires higher concentrations of GlcNAc6P for activity in vitro, grew better on GlcN in the presence of GlcNAc6P. However, wild-type NagB behaves as if it is already fully allosterically activated during growth on GlcN, and we present evidence suggesting that sufficient GlcNAc6P for allosteric activation is derived from the recycling of peptidoglycan.

摘要

在N - 乙酰葡糖胺(GlcNAc)上生长会产生细胞内的N - 乙酰葡糖胺 - 6 - 磷酸(GlcNAc6P),它以两种方式影响大肠杆菌中氨基糖分解代谢的调节。首先,GlcNAc6P是NagC阻遏物的诱导信号,因此它会增加nagE - nagBACD操纵子中酶的表达。其次,它是葡糖胺 - 6 - 磷酸(GlcN6P)脱氨酶NagB的变构激活剂,从而增加了这种氨基糖代谢关键酶的催化能力。我们之前表明,nagB基因的表达水平和葡糖胺的转运都限制了在GlcN上的生长速率(L. I. Alvarez - Añorve等人,《细菌学杂志》187:2974 - 2982,2005年)。我们无法确定野生型NagB缺乏变构激活是否也导致了在GlcN上生长速率较慢。使用带有组成型启动子的单拷贝质粒,我们分离了GlcNAc6P对NagB蛋白水平和脱氨酶活性的影响。我们表明,在一系列细胞内NagB浓度范围内,限制生长的是底物GlcN6P的量,而不是变构激活剂GlcNAc6P的浓度。另一方面,NagB的F174A突变体在体外需要更高浓度的GlcNAc6P才能有活性,在有GlcNAc6P存在的情况下,它在GlcN上生长得更好。然而,野生型NagB在GlcN上生长时表现得好像已经完全被变构激活了,并且我们提供的证据表明,用于变构激活的足够的GlcNAc6P来自肽聚糖的循环利用。

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