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Recognition of the lipid intermediate for arabinogalactan/arabinomannan biosynthesis and its relation to the mode of action of ethambutol on mycobacteria.阿拉伯半乳聚糖/阿拉伯甘露聚糖生物合成中脂质中间体的识别及其与乙胺丁醇对分枝杆菌作用方式的关系。
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Inhibition of synthesis of arabinogalactan by ethambutol in Mycobacterium smegmatis.乙胺丁醇对耻垢分枝杆菌中阿拉伯半乳聚糖合成的抑制作用。
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分枝杆菌细胞壁阿拉伯糖基残基的生物合成起源。

Biosynthetic origin of mycobacterial cell wall arabinosyl residues.

作者信息

Scherman M, Weston A, Duncan K, Whittington A, Upton R, Deng L, Comber R, Friedrich J D, McNeil M

机构信息

Department of Microbiology, Colorado State University, Fort Collins 80523, USA.

出版信息

J Bacteriol. 1995 Dec;177(24):7125-30. doi: 10.1128/jb.177.24.7125-7130.1995.

DOI:10.1128/jb.177.24.7125-7130.1995
PMID:8522519
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC177591/
Abstract

Designing new drugs that inhibit the biosynthesis of the D-arabinan moiety of the mycobacterial cell wall arabinogalactan is one important basic approach for treatment of mycobacterial diseases. However, the biosynthetic origin of the D-arabinosyl monosaccharide residues themselves is not known. To obtain information on this issue, mycobacteria growing in culture were fed glucose labeled with 14C or 3H in specific positions. The resulting radiolabeled cell walls were isolated and hydrolyzed, the arabinose and galactose were separated by high-pressure liquid chromatography, and the radioactivity in each sugar was determined. [U-14C]glucose, [6-3H]glucose, [6-14C]glucose, and [1-14C]glucose were all converted to cell wall arabinosyl residues with equal retention of radioactivity. The positions of the labeled atoms in the arabinose made from [1-14C]glucose and [6-3H]glucose were shown to be C-1 and H-5, respectively. These results demonstrated that the arabinose carbon skeleton is formed via the nonoxidative pentose shunt and not via hexose decarboxylation or via triose condensations. Since the pentose shunt product, ribulose-5-phosphate, is converted to arabinose-5-phosphate as the first step in 3-keto-D-manno-octulosonic acid biosynthesis by gram-negative bacteria, such a conversion was then searched for in mycobacteria. However, cell-free enzymatic analysis using both phosphorous nuclear magnetic resonance spectrometry and colorimetric methods failed to detect the conversion. Thus, the conversion of the pentose shunt intermediates to the D-arabino stereochemistry is not via the expected isomerase but rather must occur via novel metabolic transformations.

摘要

设计能够抑制分枝杆菌细胞壁阿拉伯半乳聚糖中D - 阿拉伯聚糖部分生物合成的新型药物,是治疗分枝杆菌疾病的一种重要基础方法。然而,D - 阿拉伯糖基单糖残基本身的生物合成起源尚不清楚。为了获取关于这个问题的信息,用在特定位置标记了14C或3H的葡萄糖培养分枝杆菌。分离并水解得到的放射性标记细胞壁,通过高压液相色谱法分离阿拉伯糖和半乳糖,并测定每种糖中的放射性。[U - 14C]葡萄糖、[6 - 3H]葡萄糖、[6 - 14C]葡萄糖和[1 - 14C]葡萄糖都以相同的放射性保留率转化为细胞壁阿拉伯糖基残基。由[1 - 14C]葡萄糖和[6 - 3H]葡萄糖生成的阿拉伯糖中标记原子的位置分别显示为C - 1和H - 5。这些结果表明,阿拉伯糖碳骨架是通过非氧化戊糖支路形成的,而不是通过己糖脱羧或通过丙糖缩合形成的。由于戊糖支路产物5 - 磷酸核酮糖在革兰氏阴性菌3 - 酮 - D - 甘露糖 - 辛酮糖酸生物合成中作为第一步转化为5 - 磷酸阿拉伯糖,因此随后在分枝杆菌中寻找这种转化。然而,使用磷核磁共振光谱法和比色法的无细胞酶分析未能检测到这种转化。因此,戊糖支路中间体向D - 阿拉伯糖立体化学的转化不是通过预期的异构酶,而是必须通过新的代谢转化发生。