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中间链球菌唾液酸酶:一种潜在的修饰糖链的致病因子。

Sialidase of Streptococcus intermedius: a putative virulence factor modifying sugar chains.

机构信息

Department of Oral Bacteriology, Tsurumi University, Japan.

出版信息

Microbiol Immunol. 2010 Oct;54(10):584-95. doi: 10.1111/j.1348-0421.2010.00257.x.

DOI:10.1111/j.1348-0421.2010.00257.x
PMID:21118296
Abstract

A sialidase gene of Streptococcus intermedius was cloned. It was most similar to nanA, a major sialidase gene in Streptococcus pneumoniae, and was expressed in Escherichia coli. Since the gene-knockout S. intermedius strain lost detectable sialidase activity, the gene might code, either solely or mainly, the glycosidase in the bacterial genome. Polymerase chain reaction using the primers for the nanA homologue in S. intermedius (described as nanA below) showed that this sialidase gene was commonly distributed within the isolates of S. intermedius, but not found in the strains of other species among the anginosus group. In biofilm formation assay under cultivation with mucin, the nanA-deleted S. intermedius maintained the amount of biofilm for 72 hr, while that of the parent strain decreased during incubation from 24 to 72 hr. Since sialidase activity in the parent strain increased during that time period, sialidase might contribute to the degradation of biofilm under sialic acid-rich conditions. When S. intermedius was added into the HepG2 hepatoma culture, the calculated disassociation constant (K(d)) of EDTA-releasable bacterial adhesion to the cells was higher in the nanA-deleted strain than in the parent. Furthermore, the rate constant, assuming endocytosis of the bacterium mediated by ASGP-R in HepG2 cells, seemed to be increased by sialidase pretreatment of the bacterial cells before addition to the cell culture. According to the results, modification of sugar chains by sialidase on the bacterial surface and in the surrounding environment might influence both bacterial interaction and host-bacterial interaction in S. intermedius.

摘要

中间链球菌唾液酸酶基因被克隆。它与肺炎链球菌中主要的唾液酸酶基因 nanA 最为相似,并在大肠杆菌中表达。由于基因敲除中间链球菌菌株失去了可检测的唾液酸酶活性,该基因可能单独或主要编码细菌基因组中的糖苷酶。使用中间链球菌 nanA 同源物(下文称为 nanA)的引物进行聚合酶链反应表明,这种唾液酸酶基因在中间链球菌的分离株中广泛分布,但在其他种属的菌株中未发现。在含有粘蛋白的条件下进行生物膜形成试验时,缺失 nanA 的中间链球菌在 72 小时的孵育过程中保持生物膜的量,而亲本菌株在 24 至 72 小时的孵育过程中减少。由于亲本菌株在此期间唾液酸酶活性增加,因此唾液酸酶可能有助于在富含唾液酸的条件下降解生物膜。当中间链球菌被添加到 HepG2 肝癌培养物中时,EDTA 释放的细菌与细胞的分离常数(K(d))在缺失 nanA 的菌株中高于亲本菌株。此外,假设通过 HepG2 细胞中的 ASGP-R 介导细菌内吞作用,假设细菌细胞在添加到细胞培养物之前进行唾液酸酶预处理,则细菌内吞作用的速率常数似乎增加。根据这些结果,细菌表面和周围环境中唾液酸酶对糖链的修饰可能会影响中间链球菌的细菌相互作用和宿主-细菌相互作用。

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