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志贺氏菌血清型 1 型 O-多糖基因重组稳定表达于活的口服沙门氏菌疫苗载体 Ty21a 染色体中。

Stable expression of Shigella sonnei form I O-polysaccharide genes recombineered into the chromosome of live Salmonella oral vaccine vector Ty21a.

机构信息

Laboratory of Enteric and Sexually Transmitted Diseases, U.S. FDA-Center for Biologics Evaluation and Research, NIH campus Bldg. 29, 8800 Rockville Pike, Mail Code HFM440, Bethesda, MD 20892, USA.

出版信息

Int J Med Microbiol. 2013 Apr;303(3):105-13. doi: 10.1016/j.ijmm.2013.01.001. Epub 2013 Mar 7.

DOI:10.1016/j.ijmm.2013.01.001
PMID:23474241
Abstract

Live, attenuated Salmonella enterica serovar Typhi strain Ty21a, a licensed oral typhoid fever vaccine, has also been employed for use as a vector to deliver protective antigens of Shigella and other pathogens. Importantly, lipopolysaccharide (LPS) alone has been shown to be a potent antigen for specific protection against shigellosis. We reported previously the plasmid cloning of heterologous LPS biosynthetic genes and the expression in Ty21a of either S. sonnei or of S. dysenteriae 1 LPS's. The resulting plasmids encoding Shigella LPS's were reasonably stable for >50 generations of growth in nonselective media, but still contained an antibiotic resistance marker that is objectionable to vaccine regulatory authorities. Deletion of this antibiotic-resistance marker inexplicably resulted in significant plasmid instability. Thus, we sought a method to insert the large ∼12kb S. sonnei LPS gene region into the chromosome, that would allow for subsequent removal of a selectable marker and would result in 100% genetic stability. Toward this objective, we optimized an existing recombination method to mediate the insertion of a ∼12kb region encoding the S. sonnei LPS genes into the Ty21a genome in a region that is nonfunctional due to mutation. The resulting strain Ty21a-Ss simultaneously expresses both homologous Ty21a and heterologous S. sonnei O-antigens. This chromosomal insert was shown to be 100% genetically stable in vitro and in vivo. Moreover, Ty21a-Ss elicited strong dual anti-LPS serum immune responses and 100% protection in mice against a virulent S. sonnei challenge. This new vaccine candidate, absolutely stable for vaccine manufacture, should provide combined protection against enteric fevers due to Salmonella serovar Typhi as shown previously (and some Paratyphi infections) and against shigellosis due to S. sonnei.

摘要

活减毒伤寒沙门氏菌血清型 Ty21a 菌株,一种已获许可的口服伤寒疫苗,也被用作载体,传递志贺氏菌和其他病原体的保护性抗原。重要的是,单独的脂多糖(LPS)已被证明是针对志贺氏菌病的特异性保护的有效抗原。我们之前曾报道过异源 LPS 生物合成基因的质粒克隆,并在 Ty21a 中表达 S. sonnei 或 S. dysenteriae 1 LPS。编码志贺氏菌 LPS 的质粒在非选择性培养基中生长超过 50 代时相对稳定,但仍含有疫苗监管机构反对的抗生素抗性标记。令人费解的是,删除这个抗生素抗性标记会导致质粒严重不稳定。因此,我们寻求一种方法将大型约 12kb S. sonnei LPS 基因区域插入染色体中,以便随后去除选择标记,并实现 100%的遗传稳定性。为了实现这一目标,我们优化了一种现有的重组方法,以介导约 12kb 区域的插入,该区域编码 S. sonnei LPS 基因到 Ty21a 基因组中的一个由于突变而无功能的区域。由此产生的 Ty21a-Ss 株同时表达同源的 Ty21a 和异源的 S. sonnei O-抗原。这种染色体插入在体外和体内均显示出 100%的遗传稳定性。此外,Ty21a-Ss 在小鼠中引发强烈的双重抗 LPS 血清免疫反应,并 100%保护免受强毒 S. sonnei 攻击。这种新的候选疫苗在制造疫苗时绝对稳定,应提供针对伤寒沙门氏菌血清型 Typhi 的联合保护(如前所述,还有一些 Paratyphi 感染)和针对 S. sonnei 的志贺氏菌病的联合保护。

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