The Truncated Gene cfaD′ Positively Regulates CFA/Ⅰ Expression of Enterotoxigenic Escherichia coli

The gene cluster cfaABCED’ of enterotoxigenic Escherichia coli, encoding the fimbriae which is called colonization factor antigen located on a plasmid. It is positively regulated by cfaR, a member of the AraC family, and the cfaD’ gene region, which is located downstream of cfaE and is homologous to cfaR, had been described as a truncated cryptic gene. In the present study we observed that the CFA/ fimbriae subunit, cfaB, was expressed in lower amount by the cfaABCED’ clone pNTP513 in host E. coli HB101. The expression of CFA/ diminished by deletion of cfaD’ gene region from pNTP513, and was restored by acquisition of cfaD’ in trans. Furthermore, CFA/ expression by cfaD’ deletion mutant, the cfaABCE clone, was remarkably increased by the presence of cfaD’ in trans in a topoisomerase A deficient strain of E. coli DM800. These data suggest that cfaD’ region is a functional region of gene, that regulates the CFA/ expression with cfaR by unknown mechanism.

共表达ETEC CFA/Ⅰ、CS6福氏痢疾减毒株与单独表达CFA/Ⅰ及CS6混合疫苗株的免疫原性比较

目的 以减毒志贺菌为载体 ,研制肠毒素大肠杆菌 (enterotoxigenicEscherichiacoli,ETEC)多价疫苗可以有效防治细菌性腹泻。方法 以共表达肠毒素大肠杆菌定居因子CFA/Ⅰ和CS6的重组减毒福氏痢疾疫苗株FWL0 1(pZCF16 )和两种混合的表达CFA/Ⅰ的FWL0 1(pZHY2 1)和表达CS6的FWL0 1(pZLG6 )减毒福氏痢疾疫苗株 ,分别以同等剂量口服免疫BALB/c小鼠 ,比较二者肠毒素大肠杆菌定居因子的免疫效果。结果 免疫BALB/c小鼠全部产生了抗CFA/Ⅰ和CS6的特异性血清抗体IgG和分泌型抗体sIgA ,共表达CFA/Ⅰ、CS6的减毒福氏痢疾菌FWL0 1(pZCF16 )的免疫原性与混合的FWL0 1(pZHY2 1)和FWL0 1(pZLG6 )相似或稍高。结论 在同一菌株可以表达多种菌毛 。

共表达肠毒素大肠杆菌定居因子CFA/Ⅰ、CS6与单独表达CFA/Ⅰ、CS6痢疾载体候选疫苗株的免疫原性比较

目的 :评价同一菌株表达多种肠毒素大肠杆菌 (ETEC)定居因子时的免疫效果 ,为构建多价疫苗提供依据。方法 :以同等剂量分别口服免疫BALB/c小鼠 ,比较并评价共表达肠毒素大肠杆菌定居因子CFA/Ⅰ、CS6的减毒弗氏痢疾菌苗株FWL0 1(pZCF16 )与单独表达CFA/Ⅰ的FWL0 1(pZHY2 1)和表达CS6的FWL0 1(pZLG6 )免疫效果。结果 :免疫BALB/c小鼠全部产生了抗CFA/Ⅰ和 (或 )CS6的特异性血清抗体IgG和分泌性抗体sIgA。共表达CFA/Ⅰ、CS6的减毒弗氏痢疾菌苗株FWL0 1(pZCF16 )免疫动物后 ,血清和黏膜抗体滴度与单独表达CFA/Ⅰ的FWL0 1(pZHY2 1)和表达CS6的FWL0 1(pZLG6 )的免疫效果相似。结论 :共表达ETECCFA/Ⅰ和CS6的减毒弗氏痢疾菌苗株FWL0 1(pZCF16 )能够像单独表达相应抗原的菌苗株一样有效激发机体抗CFA/I和CS6的体液及肠道黏膜免疫应答 ,为构建ETEC多价疫苗奠定了基础。

产肠毒素大肠杆菌定居因子Ⅰ基因克隆与表达

目的:在大肠杆菌DH5α中表达产肠毒素大肠杆菌(Enterotoxigenio escherichia coli,ETEC)定居因子CFA/Ⅰ,检测重组表达的ETEC CFA/Ⅰ。方法:以质粒pBV220为基础,构建pBV220-CFA/Ⅰ重组载体,表达产物用SDS-PAGE鉴定,免疫原性实验验证。结果:成功构建了pBV220-CFA/Ⅰ重组载体,表达产物的分子量与天然蛋白相同,动物免疫试验表明重组菌具有免疫原性。结论:CFA/Ⅰ基因的成功克隆为今后的ETEC CFA/Ⅰ候选疫苗研制奠定了基础。