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Poly(glucosyl-N-acetylgalactosamine 1-phosphate), a wall teichoic acid of Bacillus subtilis 168: its biosynthetic pathway and mode of attachment to peptidoglycan

机译:poly(葡萄糖基 - 乙酰甘氨酸胺1-磷酸盐),枯草芽孢杆菌168的壁噻虫酸:其生物合成途径和肽聚糖的附着模式

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The ggaAB operon of Bacillus subtilis 168 encodes enzymes responsible for the synthesis of poly(glucosyl N-acetylgalactosamine 1-phosphate) [poly(GlcGalNAc 1-P)], a wall teichoic acid (WTA). Analysis of the nucleotide sequence revealed that both GgaA and GgaB contained the motif characteristic of sugar transferases, while GgaB was most likely to be bifunctional, being endowed with an additional motif present in glucosyl/glycerophosphate transferases. Transcription of the operon was thermosensitive, and took place from an unusually distant σA-controlled promoter. The incorporation of the poly(GlcGalNAc 1-P) precursors by various mutants deficient in the synthesis of poly(glycerol phosphate), which is the most abundant WTA of strain 168, revealed that both WTAs were most likely to be attached to peptidoglycan (PG) through the same linkage unit (LU). The incorporation of poly(GlcGalNAc 1-P) precursors by protoplasts confirmed the existence of this LU, and provided further evidence that incorporation takes place at the outer surface of the protoplast membrane. The data presented here strengthen the view that biosynthesis of the LU, and the hooking of the LU-endowed polymer to PG, offer distinct widespread targets for antibiotics specific to Gram-positive bacteria.
机译:枯草芽孢杆菌168的GGAAB操纵子编码负责聚(葡萄糖基N-丙基酰胺1-磷酸葡萄糖1-磷酸葡萄糖)[聚(GlcGalnac 1-P)]的合成酶,壁噻吩酸(WTA)。核苷酸序列的分析显示,GGAA和GGAB含有糖转移酶的基序特征,而GGAB最有可能是双官能的,并且赋予葡萄糖基/甘油磷酸盐转移酶中的另外的基序。操纵子的转录是热敏,并从异常的远处ΣA控制的启动子发生。通过各种突变体掺入缺乏聚(甘油磷酸盐)的各种突变体,其是最丰富的菌株168 WTA,揭示了两种WTA最有可能附着在肽聚糖上(PG )通过相同的联动单元(Lu)。通过原生质体掺入poly(glcgalnac 1-p)前体证实了该Lu的存在,并且提供了进一步证据,即掺入在原生质体膜的外表面上。这里呈现的数据增强了Lu的生物合成和Lu禀赋聚合物的钩钩,为PG提供了明显的抗生素抗生素的不同靶标。

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