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以色列放线菌口腔菌株产生的葡聚糖酶的特性研究

Characterization of a dextranase produced by an oral strain of Actinomyces israelii.

作者信息

Staat R H, Schachtele C F

出版信息

Infect Immun. 1975 Sep;12(3):556-63. doi: 10.1128/iai.12.3.556-563.1975.

Abstract

A dextranase-producing, gram-positive, anaerobic, rod-shaped bacterium isolated from human dental plaque was identified as Actinomyces israeli. Although the extracellular dextranase (EC 3.2.1.11) formed by this microbe appeared to be constitutively produced, the bacterium did not utilize the reaction products as a carbon source during growth. A striking feature of the dextranase was the formation of two distinct groups of oligosaccharide end products. The two groups presumably correspond to the limit dextran and the released reaction product which appeared to be cleaved from the end(s) of larger dextran molecules. Low levels of dextranase activity were measured by [3H]NaBH4 reduction and alcohol fixation of the large, tritiated end products on filter paper disks. Of the carbohydrate substrates tested, only alpha-1,6-linked glucans were cleaved. The enzyme did not exhibit any metal ion requirements, and its pH optimum was 6.3. It is suggested that the A. israelii dextranase may function as a regulatory factor during extracellular in vivo glucan synthesis from sucrose by various plaque microbes.

摘要

从人类牙菌斑中分离出的一种产葡聚糖酶、革兰氏阳性、厌氧、杆状细菌被鉴定为衣氏放线菌。尽管这种微生物形成的细胞外葡聚糖酶(EC 3.2.1.11)似乎是组成型产生的,但该细菌在生长过程中并未将反应产物用作碳源。葡聚糖酶的一个显著特征是形成了两组不同的寡糖终产物。这两组产物可能分别对应于极限葡聚糖和从较大葡聚糖分子末端裂解出来的释放反应产物。通过用[3H]NaBH4还原并将大的、经氚标记的终产物在滤纸片上进行乙醇固定来测定低水平的葡聚糖酶活性。在所测试的碳水化合物底物中,只有α-1,6-连接的葡聚糖被裂解。该酶不需要任何金属离子,其最适pH为6.3。有人提出,衣氏放线菌葡聚糖酶可能在各种菌斑微生物从蔗糖进行细胞外体内葡聚糖合成过程中作为一种调节因子发挥作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4eea/415323/49e64811e6fe/iai00237-0110-a.jpg

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