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Cellular Immune Responses to Recombinant Mycobacterium bovis BCG Constructs Expressing Major Antigens of Region of Difference 1 of Mycobacterium tuberculosis

机译:重组牛分枝杆菌BCG构建体对表达结核分枝杆菌差异1区域主要抗原的细胞的免疫应答

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摘要

Besides being the most widely used vaccine directed against tuberculosis (TB) worldwide, Mycobacterium bovis BCG is also the most controversial vaccine in current use. Its protective efficacy varies widely in different parts of the world. One approach to improving the current BCG vaccine might be to produce recombinant BCG strains that express major antigens encoded by genes that are present in the M. tuberculosis-specific region of difference 1 (RD1), such as pe35, cfp10, and esat6. In this study, pe35, cfp10, and esat6 genes were cloned into shuttle plasmid pDE22 to generate the recombinant plasmids PDE22-PE35, PDE22-CFP10, and PDE22-ESAT6, which were electroporated into BCG to generate recombinant BCGs (rBCGs). The cellular immune responses (antigen-induced proliferation and secretion of selected T helper 1 [Th1], Th2, and anti-inflammatory cytokines, i.e., gamma interferon [IFN-γ], interleukin 5 [IL-5], and IL-10, respectively) that are specific to the proteins of cloned genes were studied by using spleen cells from mice immunized with native BCGs and rBCGs and synthetic peptides covering the protein sequence of the cloned genes. The results showed that the spleen cells did not secrete IL-5, whereas IL-10 was secreted in response to peptides of all three proteins from mice immunized with rBCGs only, suggesting expression of the cloned genes and in vivo priming of spleen cells to the expressed proteins. However, in Th1 cell assays that correlate with protective cellular immune responses, i.e., antigen-induced proliferation and IFN-γ secretion, only mice immunized with rBCG-pDE22-PE35 yielded positive responses to the peptides of PE35. These results suggest that rBCG-PDE22-PE35 is the only one of the three vaccines used in this work that is worthy of consideration as a new vaccine candidate against TB.
机译:牛分枝杆菌卡介苗不仅是全球使用最广泛的针对结核病的疫苗,而且还是目前使用最有争议的疫苗。在世界各地,其保护功效差异很大。一种改进当前BCG疫苗的方法可能是生产重组BCG菌株,该菌株表达主要抗原,该主要抗原由存在于结核分枝杆菌特异性差异1(RD1)中的基因编码,例如pe35,cfp10和esat6。在这项研究中,将pe35,cfp10和esat6基因克隆到穿梭质粒pDE22中,以生成重组质粒PDE22-PE35,PDE22-CFP10和PDE22-ESAT6,将其电穿孔到BCG中以生成重组BCG(rBCG)。细胞免疫应答(抗原诱导的所选T辅助细胞1 [Th1],Th2和抗炎细胞因子,即γ干扰素[IFN-γ],白介素5 [IL-5]和IL-10的增殖和分泌通过使用天然BCG和rBCG免疫小鼠的脾细胞以及覆盖克隆基因蛋白质序列的合成肽,研究了对克隆基因蛋白质特异的特异性脾细胞。结果表明,脾细胞不分泌IL-5,而IL-10是仅对用rBCG免疫的小鼠的所有三种蛋白质的肽分泌的,这表明克隆基因的表达和脾细胞在体内启动表达的蛋白质。然而,在与保护性细胞免疫反应,即抗原诱导的增殖和IFN-γ分泌相关的Th1细胞测定中,仅用rBCG-pDE22-PE35免疫的小鼠对PE35的肽产生阳性反应。这些结果表明,rBCG-PDE22-PE35是这项工作中使用的三种疫苗中唯一值得考虑作为抗结核新疫苗的疫苗之一。

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