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Identification of a Gene Cluster for the Biosynthesis of a Long Galactose-Rich Exopolysaccharide in Lactobacillus rhamnosus GG and Functional Analysis of the Priming Glycosyltransferase

机译:鼠李糖乳杆菌GG中长半乳糖丰富的外多糖生物合成的基因簇的鉴定和糖基转移酶的功能分析

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摘要

Cell surface polysaccharides have an established role as virulence factors in human bacterial pathogens. Less documented are the biosynthesis and biological functions of surface polysaccharides in beneficial bacteria. We identified a gene cluster that encodes the enzymes and regulatory and transporter proteins for the different steps in the biosynthesis of extracellular polysaccharides (EPS) of the well-documented probiotic strain Lactobacillus rhamnosus GG. Subsequent mutation of the welE gene, encoding the priming glycosyltransferase within this cluster, and comparative phenotypic analyses of wild-type versus mutant strains confirmed the specific function of this gene cluster in the biosynthesis of high-molecular-weight, galactose-rich heteropolymeric EPS molecules. The phenotypic analyses included monomer composition determination, estimation of the polymer length of the isolated EPS molecules, and single-molecule force spectroscopy of the surface polysaccharides. Further characterization of the welE mutant also showed that deprivation of these long, galactose-rich EPS molecules results in an increased adherence and biofilm formation capacity of L. rhamnosus GG, possibly because of less shielding of adhesins such as fimbria-like structures.
机译:细胞表面多糖在人类细菌病原体中具有确定的毒力因子作用。有益细菌中表面多糖的生物合成和生物学功能文献较少。我们确定了一个基因簇,该簇编码了酶和调控蛋白以及转运蛋白,这些蛋白在众所周知的益生菌鼠李糖乳杆菌GG的细胞外多糖(EPS)的生物合成中的不同步骤中起作用。 welE基因的随后突变,在该簇中编码启动糖基转移酶,并对野生型与突变菌株进行比较表型分析,证实了该基因簇在高分子量,富含半乳糖的杂聚EPS分子生物合成中的特定功能。 。表型分析包括单体组成测定,分离的EPS分子的聚合物长度估计和表面多糖的单分子力光谱学。 welE突变体的进一步特征还表明,剥夺这些长的,富含半乳糖的EPS分子会导致鼠李糖乳杆菌GG的粘附和生物膜形成能力增强,这可能是由于对粘附素(如菌毛状结构)的屏蔽作用降低了。

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