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Streptococcus salivarius ATCC 25975 possesses at least two genes coding for primer-independent glucosyltransferases.

机译:唾液链球菌ATCC 25975具有至少两个编码不依赖引物的葡糖基转移酶的基因。

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摘要

Fractionation of the culture medium showed that Streptococcus salivarius ATCC 25975 secreted a glucosyltransferase (Gtf) that was primer independent. On the basis of this observation, a gene library of S. salivarius chromosomal DNA cloned into lambda L47.1 was screened for a gene(s) coding for such an activity. As a result of this screening process, two new gtf genes, gtfL and gtfM, both of which coded for primer-independent Gtf activities, were isolated. GtfL produced an insoluble glucan that was refractory to digestion by the endo-(1-->6)-alpha-D-glucanase. of Chaetonium gracile, while GtfM produced a soluble glucan that was readily degraded by the glucanase. Comparison of the deduced amino acid sequences of gtfL and gtfM with 10 other available Gtf sequences allowed the relatedness of the conserved catalytic regions to be assessed. This analysis showed that the 12 enzymes did not form clusters based on their primer dependencies or on their product solubilities. Further analysis of the YG repeats in the C-terminal glucan-binding domains of GtfJ, GtfK, GtfL, and GtfM from S. salivarius showed that there was strong homology between a block of contiguous triplet YG repeats present in the four alleles. These blocks of YG repeats were coded for by a region of each gene that appeared to have arisen as a result of a recent duplication event(s).
机译:分离培养基显示唾液链球菌ATCC 25975分泌了不依赖引物的葡糖基转移酶(Gtf)。基于该观察结果,筛选克隆到λL47.1中的唾液链球菌染色体DNA的基因文库,以寻找编码这种活性的基因。作为该筛选过程的结果,分离了两个新的gtf基因gtfL和gtfM,这两个基因均编码不依赖引物的Gtf活性。 GtfL产生了一种不溶性葡聚糖,该葡聚糖对内切(1-> 6)-α-D-葡聚糖酶的消化具有抵抗力。 ,而GtfM产生的可溶性葡聚糖很容易被葡聚糖酶降解。推导的gtfL和gtfM氨基酸序列与其他10个可用的Gtf序列的比较,可以评估保守催化区域的相关性。该分析表明,基于其引物依赖性或产物溶解度,这12种酶均未形成簇。对来自唾液链球菌的GtfJ,GtfK,GtfL和GtfM的C端葡聚糖结合结构域中的YG重复序列的进一步分析表明,在四个等位基因中存在的连续三联体YG重复序列之间存在很强的同源性。 YG重复序列的这些区块由每个基因的某个区域编码,这些区域似乎是由于最近的复制事件而出现的。

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