首页> 外文OA文献 >Deletion of Cg-emb in Corynebacterianeae leads to a novel truncated cell wall arabinogalactan, whereas inactivation of Cg-ubiA results in an arabinan-deficient mutant with a cell wall galactan core
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Deletion of Cg-emb in Corynebacterianeae leads to a novel truncated cell wall arabinogalactan, whereas inactivation of Cg-ubiA results in an arabinan-deficient mutant with a cell wall galactan core

机译:棒状杆菌中Cg-emb的缺失会导致一种新型的截短的阿拉伯半乳聚糖细胞壁,而Cg-ubiA的失活会导致带有阿拉伯半乳聚糖核心且具有细胞壁半乳聚糖核心的突变体

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摘要

The cell wall of Mycobacterium tuberculosis has a complex ultrastructure that consists of mycolic acids connected to peptidoglycan via arabinogalactan (AG) and abbreviated as the mAGP complex. The mAGP complex is crucial for the survival and pathogenicity of M. tuberculosis and is the target of several anti-tubercular agents. Apart from sharing a similar mAGP and the availability of the complete genome sequence, Corynebacterium glutamicum has proven useful in the study of orthologous M. tuberculosis genes essential for viability. Here we examined the effects of particular genes involved in AG polymerization by gene deletion in C. glutamicum. The anti-tuberculosis drug ethambutol is thought to target a set of arabinofuranosyltransferases (Emb) that are involved in arabinan polymerization. Deletion of emb in C. glutamicum results in a slow growing mutant with profound morphological changes. Chemical analysis revealed a dramatic reduction of arabinose resulting in a novel truncated AG structure possessing only terminal arabinofuranoside (t-Araf) residues with a corresponding loss of cell wall bound mycolic acids. Treatment of wild-type C. glutamicum with ethambutol and subsequent cell wall analyses resulted in an identical phenotype comparable to the C. glutamicum emb deletion mutant. Additionally, disruption of ubiA in C. glutamicum, the first enzyme involved in the biosynthesis of the sugar donor decaprenol phosphoarabinose (DPA), resulted in a complete loss of cell wall arabinan. Herein, we establish for the first time, (i) that in contrast to M. tuberculosis embA and embB mutants, deletion of C. glutamicum emb leads to a highly truncated AG possessing t-Araf residues, (ii) the exact site of attachment of arabinan chains in AG, and (iii) DPA is the only Araf sugar donor in AG biosynthesis suggesting the presence of a novel enzyme responsible for "priming" the galactan domain for further elaboration by Emb, resulting in the final maturation of the native AG polysaccharide.
机译:结核分枝杆菌的细胞壁具有复杂的超微结构,该超微结构由通过阿拉伯半乳聚糖(AG)连接至肽聚糖的霉菌酸组成,缩写为mAGP复合物。 mAGP复合物对于结核分枝杆菌的生存和致病性至关重要,并且是多种抗结核药的目标。除了共享相似的mAGP和完整基因组序列的可用性外,谷氨酸棒杆菌还被证明可用于研究生存力必不可少的直系结核分枝杆菌基因。在这里,我们通过谷氨酸棒杆菌中的基因缺失检查了参与AG聚合的特定基因的作用。抗结核药乙胺丁醇被认为靶向一组涉及阿拉伯聚糖聚合的阿拉伯呋喃糖基转移酶(Emb)。谷氨酸棒状杆菌中emb的缺失导致突变体缓慢生长,具有深刻的形态学变化。化学分析表明,阿拉伯糖显着减少,导致一种新型的截短的AG结构,仅具有末端阿拉伯呋喃糖苷(t-Araf)残基,而细胞壁结合的霉菌酸则相应丢失。用乙胺丁醇处理野生型谷氨酸棒状杆菌和随后的细胞壁分析产生与谷氨酸棒状杆菌emb缺失突变体相当的相同表型。此外,谷氨酸棒杆菌中的ubiA的破坏是糖供体癸癸酚磷酸阿拉伯糖(DPA)生物合成中涉及的第一个酶,导致细胞壁阿拉伯聚糖的完全丧失。在此,我们首次确定:(i)与结核分枝杆菌embA和embB突变体相反,谷氨酸棒状杆菌emb的缺失导致具有t-Araf残基的高度截短的AG,(ii)确切的附着位点(iii)DPA是AG生物合成中唯一的Araf糖供体,表明存在一种新型酶,该酶负责“引发”半乳聚糖结构域,以供Emb进一步修饰,从而导致天然AG的最终成熟多糖。

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