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Biosynthesis of D-alanyl-lipoteichoic acid in Lactobacillus casei: D-alanyl-lipophilic compounds as intermediates.

机译:干酪乳杆菌中D-丙氨酰-脂酸的生物合成:以D-丙氨酰-亲脂性化合物为中间体。

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摘要

D-Alanyl-lipoteichoic acid (D-alanyl-LTA) from Lactobacillus casei contains a poly(glycerol phosphate) moiety that is selectively acylated with D-alanine ester residues. To characterize further the mechanism of D-alanine substitution, intermediates were sought that participate in the assembly of this LTA. From the incorporation system utilizing either toluene-treated cells or a combination of membrane fragments and supernatant fraction, a series of membrane-associated D-[14C]alanyl-lipophilic compounds was found. The assay of these compounds depended on their extractability into monophasic chloroform-methanol-water (0.8:3.2:1.0, vol/vol/vol) and subsequent partitioning into chloroform. Four lines of evidence suggested that the D-alanyl-lipophilic compounds are intermediates in the synthesis of D-alanyl-LTA. First, partial degradation of the poly(glycerol phosphate) moiety of D-alanyl-LTA by phosphodiesterase II/phosphatase from Aspergillus niger generated a series of D-alanyl-lipophilic compounds similar to those extracted from the toluene-treated cells during the incorporation of D-alanine. Second, enzymatic degradation of the D-alanyl-lipophilic compounds by the above procedure gave D-alanyl-glycerol, the same degradation product obtained from D-alanyl-LTA. Third, the incorporation of D-alanine into these compounds required the same components as the incorporation of D-alanine into membrane-associated D-alanyl-LTA. Fourth, the phosphate-induced loss of D-[14C]alanine-labeled lipophilic compounds could be correlated with the stimulation of phosphatidylglycerol synthesis in the presence of excess phosphate. We interpreted these experiments to indicate that the D-alanyl-lipophilic compounds are D-alanyl-LTA with short polymer chains and are most likely intermediates in the assembly of the completed polymer, D-alanyl-LTA.
机译:来自干酪乳杆菌的D-丙氨酰-脂酸(D-丙氨酰-LTA)包含聚(甘油磷酸)部分,其被D-丙氨酸酯残基选择性地酰化。为了进一步表征D-丙氨酸取代的机制,寻求了参与该LTA组装的中间体。从利用甲苯处理的细胞或膜碎片和上清液部分组合的掺入系统中,发现了一系列与膜相关的D- [14C]丙氨酰-亲脂性化合物。这些化合物的测定取决于它们在单相氯仿-甲醇-水(0.8:3.2:1.0,vol / vol / vol)中的可萃取性,然后分配到氯仿中。四个证据表明,D-丙氨酰-亲脂性化合物是D-丙氨酰-LTA合成的中间体。首先,来自黑曲霉的磷酸二酯酶II /磷酸酶对D-丙氨酰-LTA的聚甘油磷酸酯部分降解,产生了一系列D-丙氨酰-亲脂性化合物,类似于从甲苯处理的细胞中掺入的化合物。 D-丙氨酸。其次,通过上述方法将D-丙氨酰-亲脂性化合物酶促降解,得到D-丙氨酰-甘油,其与从D-丙氨酰-LTA获得的相同降解产物。第三,将D-丙氨酸掺入到这些化合物中需要与将D-丙氨酸掺入到膜相关的D-丙氨酰-LTA中相同的组分。第四,在过量磷酸盐存在下,磷酸盐诱导的D- [14C]丙氨酸标记的亲脂性化合物的损失可能与刺激磷脂酰甘油合成有关。我们将这些实验解释为表明D-丙氨酰-亲脂性化合物是具有短聚合物链的D-丙氨酰-LTA,并且最有可能是完成的聚合物D-丙氨酰-LTA组装的中间体。

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