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解析幽门螺杆菌脂多糖A的异常酰化模式。

Deciphering the unusual acylation pattern of Helicobacter pylori lipid A.

作者信息

Stead Christopher M, Beasley Ashley, Cotter Robert J, Trent M Stephen

机构信息

Department of Biochemistry and Molecular Biology, Medical College of Georgia, Augusta, GA 30912, USA.

出版信息

J Bacteriol. 2008 Nov;190(21):7012-21. doi: 10.1128/JB.00667-08. Epub 2008 Aug 29.

Abstract

The synthesis of "typical" hexa-acylated lipid A occurs via a nine-step enzymatic pathway, which is generally well conserved throughout all gram-negative bacteria. One exception to the rule is Helicobacter pylori, which has only eight homologs to the nine lipid A biosynthetic enzymes. The discrepancy occurs toward the end of the pathway, with H. pylori containing only a single putative secondary acyltransferase encoded by jhp0265. In Escherichia coli K-12, two late acyltransferases, termed LpxL and LpxM, are required for the biosynthesis of hexa-acylated lipid A. Detailed biochemical and genetic analyses reveal that H. pylori Jhp0265 (the protein encoded by jhp0265) is in fact an LpxL homolog, capable of transferring a stearoyl group to the hydroxyl group of the 2' linked fatty acyl chain of lipid A. Despite the lack of a homolog to LpxM in the H. pylori genome, the organism synthesizes a hexa-acylated lipid A species, suggesting that an equivalent enzyme exists. Using radiolabeled lipid A substrates and acyl-acyl carrier protein as the fatty acyl donor, we were able to confirm the presence of a second H. pylori late acyl transferase by biochemical assays. After synthesis of the hexa-acylated lipid A species, several modification enzymes then function to produce the major lipid A species of H. pylori that is tetra-acylated. Jhp0634 was identified as an outer membrane deacylase that removes the 3'-linked acyl chains of H. pylori lipid A. Together, this work elucidates the biochemical machinery required for the acylation and deacylation of the lipid A domain of H. pylori lipopolysaccharide.

摘要

“典型的”六酰化脂多糖A的合成通过一条九步酶促途径进行,该途径在所有革兰氏阴性菌中通常都高度保守。该规则的一个例外是幽门螺杆菌,它与九种脂多糖A生物合成酶只有八个同源物。差异出现在该途径的末尾,幽门螺杆菌仅含有一种由jhp0265编码的假定的二级酰基转移酶。在大肠杆菌K-12中,六酰化脂多糖A的生物合成需要两种晚期酰基转移酶,即LpxL和LpxM。详细的生化和遗传分析表明,幽门螺杆菌Jhp0265(由jhp0265编码的蛋白质)实际上是一种LpxL同源物,能够将硬脂酰基转移到脂多糖A的2'连接的脂肪酰链的羟基上。尽管幽门螺杆菌基因组中缺乏LpxM的同源物,但该生物体仍能合成一种六酰化脂多糖A物种,这表明存在一种等效的酶。使用放射性标记的脂多糖A底物和酰基-酰基载体蛋白作为脂肪酰供体,我们能够通过生化分析证实幽门螺杆菌存在第二种晚期酰基转移酶。在合成六酰化脂多糖A物种后,几种修饰酶随后发挥作用,产生幽门螺杆菌的主要四酰化脂多糖A物种。Jhp0634被鉴定为一种外膜脱酰酶,可去除幽门螺杆菌脂多糖A的3'-连接的酰基链。这项工作共同阐明了幽门螺杆菌脂多糖脂多糖A结构域酰化和脱酰化所需的生化机制。

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