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变形链球菌生物膜形成:利用gtfB启动子-绿色荧光蛋白(PgtfB::gfp)构建体监测其发育情况。

Streptococcus mutans biofilm formation: utilization of a gtfB promoter-green fluorescent protein (PgtfB::gfp) construct to monitor development.

作者信息

Yoshida Akihiro, Kuramitsu Howard K

机构信息

Department of Oral Biology, State University of New York, 3435 Main St, Buffalo NY 14214, USA1.

出版信息

Microbiology (Reading). 2002 Nov;148(Pt 11):3385-3394. doi: 10.1099/00221287-148-11-3385.

DOI:10.1099/00221287-148-11-3385
PMID:12427930
Abstract

The glucosyltransferases of Streptococcus mutans are recognized as important virulence factors for this cariogenic bacterium. To study the expression of the gtfB gene of S. mutans in biofilms, a gtfB promoter (PgtfB)-green fluorescent protein (GFP) reporter system was developed. A Streptococcus-Escherichia coli shuttle vector harbouring a PGTFB::gfp cassette was introduced into S. mutans GS-5, and the expression of GFP by the transformed S. mutans cells was confirmed by fluorescence microscopy. Furthermore, confocal laser scanning microscopy was carried out on biofilms attached to polystyrene plates; enhanced gtfB expression was observed in various microcolonies across these biofilms. To further test the hypothesis that gtfB expression is upregulated in biofilms, flow cytometry analysis was done on planktonic and biofilm cells; this analysis showed an approximately five-fold increase in gtfB expression in the biofilm cells relative to the planktonic cells. Real-time (TaqMan) PCR analysis confirmed that gtfB expression in the biofilm cells was enhanced relative to the planktonic cells. Previously, it has been suggested that the S. mutans gtfC gene might be co-transcribed with gtfB. Therefore, RT-PCR analysis was performed on gtfB-expressing S. mutans; this analysis demonstrated that gtfC was co-transcribed with gtfB. These results indicated that GFP expression can be utilized to examine gene regulation in S. mutans biofilm formation.

摘要

变形链球菌的葡糖基转移酶被认为是这种致龋菌的重要毒力因子。为了研究变形链球菌gtfB基因在生物膜中的表达,构建了gtfB启动子(PgtfB)-绿色荧光蛋白(GFP)报告系统。将携带PGTFB::gfp盒的链球菌-大肠杆菌穿梭载体导入变形链球菌GS-5,并通过荧光显微镜确认转化后的变形链球菌细胞中GFP的表达。此外,对附着在聚苯乙烯平板上的生物膜进行了共聚焦激光扫描显微镜观察;在这些生物膜的各个微菌落中观察到gtfB表达增强。为了进一步验证gtfB在生物膜中表达上调的假说,对浮游细胞和生物膜细胞进行了流式细胞术分析;该分析表明,生物膜细胞中gtfB的表达相对于浮游细胞增加了约5倍。实时(TaqMan)PCR分析证实,生物膜细胞中gtfB的表达相对于浮游细胞有所增强。此前有研究表明,变形链球菌gtfC基因可能与gtfB共转录。因此,对表达gtfB的变形链球菌进行了RT-PCR分析;该分析表明gtfC与gtfB共转录。这些结果表明,GFP表达可用于研究变形链球菌生物膜形成过程中的基因调控。

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