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宋内志贺氏菌I型O多糖基因的分子克隆与特性分析:推测的生物合成途径及其在减毒活沙门氏菌疫苗载体中的稳定表达

Molecular cloning and characterization of genes for Shigella sonnei form I O polysaccharide: proposed biosynthetic pathway and stable expression in a live salmonella vaccine vector.

作者信息

Xu De-Qi, Cisar John O, Ambulos Nicholas, Burr Donald H, Kopecko Dennis J

机构信息

Oral Infection and Immunity Branch, National Institute of Dental and Craniofacial Research, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

Infect Immun. 2002 Aug;70(8):4414-23. doi: 10.1128/IAI.70.8.4414-4423.2002.

Abstract

The gene region for biosynthesis of Shigella sonnei form I O polysaccharide (O-Ps) and flanking sequences, totaling >18 kb, was characterized by deletion analysis to define a minimal construct for development of Salmonella-based live vaccine vector strains. Lipopolysaccharide (LPS) expression and DNA sequence studies of plasmid deletion derivatives indicated form I O-Ps expression from a 12.3-kb region containing a putative promoter and 10 contiguous open reading frames (ORFs), one of which is the transposase of IS630. A detailed biosynthetic pathway, consistent with the predicted functions of eight of the nine essential ORFs and the form I O-Ps structure, is proposed. Further sequencing identified partial IS elements (i.e., IS91 and IS630) and wzz upstream of the form I coding region and a fragment of aqpZ and additional full or partial IS elements (i.e., IS629, IS91, and IS911) downstream of this region. The stability of plasmid-based form I O-Ps expression was greater from low-copy vectors than from high-copy vectors and was enhanced by deletion of the downstream IS91 from plasmid inserts. Both core-linked (i.e., LPS) and non-core-linked (i.e., capsule-like) surface expression of form I O-Ps were detected by Western blotting and silver staining of polyacrylamide gel electrophoresis-separated Shigella and Escherichia coli extracts. However, salmonellae, which have a core that is chemically dissimilar to that of shigellae, expressed only non-core-linked surface-associated form I O-Ps. Finally, attenuated Salmonella enterica serovar Typhi live vaccine vector candidates, containing minimal-sized form I operon constructs, elicited immune protection in mice against virulent S. sonnei challenge, thereby supporting the promise of live, oral vaccines for the prevention of shigellosis.

摘要

宋内志贺菌I型O多糖(O-Ps)生物合成的基因区域及侧翼序列,总长>18 kb,通过缺失分析进行了表征,以确定用于开发基于沙门氏菌的活疫苗载体菌株的最小构建体。质粒缺失衍生物的脂多糖(LPS)表达和DNA序列研究表明,I型O-Ps表达来自一个12.3 kb的区域,该区域包含一个推定的启动子和10个连续的开放阅读框(ORF),其中之一是IS630的转座酶。提出了一个详细的生物合成途径,与九个必需ORF中的八个的预测功能和I型O-Ps结构一致。进一步测序确定了I型编码区域上游的部分IS元件(即IS91和IS630)和wz z,以及该区域下游的aqpZ片段和其他完整或部分IS元件(即IS629、IS91和IS911)。基于质粒的I型O-Ps表达的稳定性在低拷贝载体中比在高拷贝载体中更高,并且通过从质粒插入物中缺失下游的IS91而增强。通过对聚丙烯酰胺凝胶电泳分离的志贺菌和大肠杆菌提取物进行蛋白质印迹和银染,检测到了I型O-Ps的核心连接(即LPS)和非核心连接(即类荚膜)表面表达。然而,沙门氏菌的核心与志贺菌的核心在化学上不同,仅表达非核心连接的表面相关I型O-Ps。最后,含有最小尺寸I型操纵子构建体的减毒伤寒沙门氏菌活疫苗载体候选物在小鼠中引发了针对强毒宋内志贺菌攻击的免疫保护,从而支持了用于预防志贺菌病的口服活疫苗的前景。

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