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LacR 突变在中间链球菌中经常观察到,并且与增加中间溶菌素的产生和毒力有关。

LacR mutations are frequently observed in Streptococcus intermedius and are responsible for increased intermedilysin production and virulence.

机构信息

Department of Biological Science and Technology, Institute of Technology and Science, The University of Tokushima Graduate School, Tokushima, Japan.

出版信息

Infect Immun. 2013 Sep;81(9):3276-86. doi: 10.1128/IAI.00638-13. Epub 2013 Jun 24.

Abstract

Streptococcus intermedius secretes a human-specific cytolysin, intermedilysin (ILY), which is considered to be the major virulence factor of this pathogen. We screened for a repressor of ily expression by using random gene disruption in a low-ILY-producing strain (PC574). Three independent high-ILY-producing colonies that had plasmid insertions within a gene that has high homology to lacR were isolated. Validation of these observations was achieved through disruption of lacR in strain PC574 with an erythromycin cassette, which also led to higher hemolytic activity, increased transcription of ily, and higher cytotoxicity against HepG2 cells, compared to the parental strain. The direct binding of LacR within the ily promoter region was shown by a biotinylated DNA probe pulldown assay, and the amount of ILY secreted into the culture supernatant by PC574 cells was increased by adding lactose or galactose to the medium as a carbon source. Furthermore, we examined lacR nucleotide sequences and the hemolytic activity of 50 strains isolated from clinical infections and 7 strains isolated from dental plaque. Of the 50 strains isolated from infections, 13 showed high ILY production, 11 of these 13 strains had one or more point mutations and/or an insertion mutation in LacR, and almost all mutations were associated with a marked decline in LacR function. These results strongly suggest that mutation in lacR is required for the overproduction of ILY, which is associated with an increase in pathogenicity of S. intermedius.

摘要

中间链球菌分泌一种人类特异性细胞毒素,即中介溶素(ILY),被认为是该病原体的主要毒力因子。我们通过在低 ILY 产生菌株(PC574)中进行随机基因敲除来筛选 ILY 表达的抑制剂。从三个独立的高 ILY 产生菌落中分离出了一个与 lacR 高度同源的基因内的质粒插入。通过在含有红霉素盒的 PC574 菌株中敲除 lacR 来验证这些观察结果,这也导致了更高的溶血活性、ILY 的转录增加以及对 HepG2 细胞的更高细胞毒性,与亲本菌株相比。通过生物素化 DNA 探针下拉测定证实了 LacR 在 ILY 启动子区域内的直接结合,并且通过将乳糖或半乳糖添加到培养基中作为碳源,PC574 细胞分泌到培养上清液中的 ILY 量增加。此外,我们检查了 50 株从临床感染中分离的菌株和 7 株从牙菌斑中分离的菌株的 lacR 核苷酸序列和溶血活性。在从感染中分离的 50 株菌株中,有 13 株表现出高 ILY 产生,其中 11 株在 LacR 中有一个或多个点突变和/或插入突变,几乎所有突变都与 LacR 功能的显著下降有关。这些结果强烈表明 lacR 中的突变是 ILY 过度产生所必需的,这与中间链球菌致病性的增加有关。

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