Live attenuated vector strains of Vibrio cholerae were derived from Peru-2, a Peruvian El Tor Inaba strain deleted for the cholera toxin genetic element and attRS1 sequences, which was developed as a live, oral vaccine strain. A promoterless gene encoding the Shiga-like toxin I B subunit (slt-IB) was inserted in the V. cholerae virulence gene irgA by in vivo marker exchange, such that slt-IB was under transcriptional control of the iron-regulated irgA promoter. slt-IB was also placed under transcriptional control of the V. cholerae heat shock promoter, htpGp, and introduced into either the irgA or lacZ locus, or both loci, on the chromosome of Peru-2, generating JRB10, JRB11, or JRB12, respectively. A new technique was used to perform allelic exchange with lacZ. This method uses plasmid p6891MCS, a pBR327 derivative containing cloned V. cholerae lacZ, to insert markers of interest into the V. cholerae chromosome. Recombinants can be detected by simple color screening and antibiotic selection. In vitro measurements of Slt-IB produced by the vector strains suggested that expression of Slt-IB from the irgA and htpG promoters was synergistic and that two copies of the gene for Slt-IB increased expression over a single copy. The V. cholerae vectors colonized the gastrointestinal mucosa of rabbits after oral immunization, as demonstrated by very high serum antibody responses to V. cholerae antigens. Comparison of the serologic responses to the B subunit of cholera toxin (CtxB) following orogastric inoculation either with the wild-type C6709 or with Peru-10, a strain containing ctxB regulated by htpGp, suggested that both the cholera toxin and heat shock promoters were active in vivo, provoking comparable immunologic responses. Orogastric inoculation of rabbits with vector strains evoked serum immunoglobulin G (IgG) responses to Slt-IB in two of the four strains tested; all four strains produced biliary IgA responses. No correlation was observed between the type of promoter expressing slt-IB and the level of serum IgG or biliary IgA response, but the vector strain containing two copies of the gene for slt-IB evoked greater serum IgG responses than strains containing a single copy, consistent with the increased expression of Slt-IB from this strain observed in vitro. A comparison of the serum and biliary antibody responses to Slt-IB expressed from htpGp versus CtxB expressed from the same promoter suggested that CtxB is a more effective orally delivered immunogen.
展开▼
机译:霍乱弧菌的减毒活毒株来自秘鲁-2,这是一种秘鲁霍乱毒素遗传元件和attRS1序列缺失的秘鲁El Tor Inaba毒株,被开发为口服活疫苗株。通过体内标记交换将编码志贺氏样毒素IB亚基(slt-IB)的无启动子基因插入霍乱弧菌毒力基因irgA,使得slt-IB处于铁调节的irgA启动子的转录控制下。 slt-IB也被置于霍乱弧菌热激启动子htpGp的转录控制下,并被引入Peru-2染色体上的irgA或lacZ基因座或两个基因座,从而产生JRB10,JRB11或JRB12,分别。一种新技术被用来与lacZ进行等位基因交换。该方法使用质粒p6891MCS(一种含有克隆的霍乱弧菌lacZ的pBR327衍生物)将感兴趣的标记插入霍乱弧菌染色体。可以通过简单的颜色筛选和抗生素选择来检测重组子。由载体菌株产生的Slt-IB的体外测量表明,来自irgA和htpG启动子的Slt-IB的表达是协同的,并且Slt-IB的基因的两个拷贝比单个拷贝增加了表达。口服免疫后,霍乱弧菌载体定居在兔的胃肠道粘膜上,这表现为对霍乱弧菌抗原的很高的血清抗体反应。比较野生型C6709或秘鲁10(经htpGp调节的ctxB菌株)经口胃接种后对霍乱毒素B亚基(CtxB)的血清学反应,表明霍乱毒素和热休克促进剂都是在体内活跃,引起类似的免疫反应。在四只测试菌株中的两只中,用载体菌株对家兔进行胃内接种,引起对Slt-IB的血清免疫球蛋白G(IgG)反应。所有四种菌株均产生胆汁IgA反应。在表达slt-IB的启动子类型与血清IgG或胆汁IgA反应的水平之间未发现相关性,但是包含slt-IB基因的两个拷贝的载体菌株引起的血清IgG反应比包含单个拷贝的菌株更大。与在体外观察到的该菌株中Slt-IB的表达增加一致。血清和胆汁抗体对htpGp表达的Slt-IB与相同启动子表达的CtxB的反应比较表明,CtxB是一种更有效的口服免疫原。
展开▼
