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一种用于在戈登氏链球菌中进行异源基因表达的宿主-载体系统。

A host-vector system for heterologous gene expression in Streptococcus gordonii.

作者信息

Oggioni M R, Pozzi G

机构信息

Sezione di Microbiologia, Dipartimento di Biologia Molecolare, Università di Siena, Italy.

出版信息

Gene. 1996 Feb 22;169(1):85-90. doi: 10.1016/0378-1119(95)00775-x.

Abstract

We have developed a host-vector system for heterologous expression in Streptococcus gordonii (Sg) Challis (formerly Streptococcus sanguis), a commensal bacterium of the human oral cavity. The system is based on (i) integration of plasmid insertion vectors into the chromosome of specially engineered recipient hosts, and (ii) the use of the M6-protein-encoding gene (emm6) as a partner for construction of translational gene fusions. M6 is a streptococcal surface protein already proven useful as a fusion partner for the delivery of foreign antigens to the surface of Sg [Pozzi et al., Infect. Immun. 60 (1992) 1902-1907]. Insertion vectors carry a drug-resistance marker, different portions of emm6 and a multiple cloning site to allow construction of a variety of emm6-based fusions. Upon transformation of a recipient host with an insertion vector, 100% of transformants acquire both the drug-resistance marker and the capacity of displaying the M6 molecule on the cell surface. Chromosomal integration occurred at high frequency in recipient host GP1221. Transformation with 1 microgram of insertion vector DNA yielded 8.1 X 10(5) transformants per ml of competent cells.

摘要

我们开发了一种宿主-载体系统,用于在戈登链球菌(Sg)Challis(以前称为血链球菌)中进行异源表达,该菌是人类口腔中的一种共生细菌。该系统基于:(i)将质粒插入载体整合到经过特殊工程改造的受体宿主的染色体中,以及(ii)使用编码M6蛋白的基因(emm6)作为构建翻译基因融合体的伙伴。M6是一种链球菌表面蛋白,已被证明可作为融合伙伴,用于将外源抗原递送至Sg表面[Pozzi等人,《感染与免疫》60(1992)1902 - 1907]。插入载体携带一个耐药标记、emm6的不同部分以及一个多克隆位点,以允许构建多种基于emm6的融合体。用插入载体转化受体宿主后,100%的转化体同时获得耐药标记和在细胞表面展示M6分子的能力。染色体整合在受体宿主GP1221中高频发生。用1微克插入载体DNA进行转化,每毫升感受态细胞可产生8.1×10⁵个转化体。

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