首页> 外文OA文献 >Allelic Diversity of the Two Transferrin Binding Protein B Gene Isotypes among a Collection of Neisseria meningitidis Strains Representative of Serogroup B Disease: Implication for the Composition of a Recombinant TbpB-Based Vaccine
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Allelic Diversity of the Two Transferrin Binding Protein B Gene Isotypes among a Collection of Neisseria meningitidis Strains Representative of Serogroup B Disease: Implication for the Composition of a Recombinant TbpB-Based Vaccine

机译:脑膜炎奈瑟氏菌菌株代表血清型B疾病的集合中的两个转铁蛋白结合蛋白B基因同种型的等位基因多样性:对基于重组TbpB的疫苗的组成的影响。

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摘要

The distribution of the two isotypes of tbpB in a collection of 108 serogroup B meningococcal strains belonging to the four major clonal groups associated with epidemic and hyperendemic disease (the ET-37 complex, the ET-5 complex, lineage III, and cluster A4) was determined. Isotype I strains (with a 1.8-kb tbpB gene) was less represented than isotype II strains (19.4 versus 80.6%). Isotype I was restricted to the ET-37 complex strains, while isotype II was found in all four clonal complexes. The extent of the allelic diversity of tbpB in these two groups was studied by PCR restriction analysis and sequencing of 10 new tbpB genes. Four major tbpB gene variants were characterized: B16B6 (representative of isotype I) and M982, BZ83, and 8680 (representative of isotype II). The relevance of these variants was assessed at the antigenic level by the determination of cross-bactericidal activity of purified immunoglobulin G preparations raised to the corresponding recombinant TbpB (rTbpB) protein against a panel of 27 strains (5 of isotype I and 22 of isotype II). The results indicated that rTbpB corresponding to each variant was able to induce cross-bactericidal antibodies. However, the number of strains killed with an anti-rTbpB serum was slightly lower than that obtained with an anti-TbpA+B complex. None of the sera tested raised against an isotype I strain was able to kill an isotype II strain and vice versa. None of the specific antisera tested (anti-rTbpB or anti-TbpA+B complex) was able to kill all of the 22 isotype II strains tested. Moreover, using sera raised against the C-terminus domain of TbpB M982 (amino acids 352 to 691) or BZ83 (amino acids 329 to 669) fused to the maltose-binding protein, cross-bactericidal activity was detected against 12 and 7 isotype II strains, respectively, of the 22 tested. These results suggest surface accessibility of the C-terminal end of TbpB. Altogether, these results show that although more than one rTbpB will be required in the composition of a TbpB-based vaccine to achieve a fully cross-bactericidal activity, rTbpB and its C terminus were able by themselves to induce cross-bactericidal antibodies.
机译:tbpB的两个同种型在108个B组脑膜炎球菌菌株中的分布,这些菌株属于与流行病和高流行病有关的四个主要克隆组(ET-37复合体,ET-5复合体,谱系III和簇A4)被确定。与同型II菌株相比,同型I菌株(具有1.8-kb tbpB基因)的代表较少(19.4比80.6%)。 I型仅限于ET-37复合株,而II型则在所有四个克隆复合物中均发现。通过PCR限制性酶切分析和10个新的tbpB基因测序,研究了两组中tbpB的等位基因多样性程度。表征了四个主要的tbpB基因变体:B16B6(代表同种型I)和M982,BZ83和8680(代表同种型II)。通过确定纯化的免疫球蛋白G制剂对27种菌株(5种同型I和22种同种II型)产生的相应重组TbpB(rTbpB)蛋白的交叉杀菌活性,在抗原水平上评估了这些变体的相关性)。结果表明对应于每个变体的rTbpB能够诱导交叉杀菌抗体。但是,用抗rTbpB血清杀死的菌株的数量略少于用抗TbpA + B复合物获得的菌株的数量。针对I型同种菌株产生的测试血清均不能杀死II型同种菌株,反之亦然。测试的所有特定抗血清(抗rTbpB或抗TbpA + B复合物)均无法杀死所有22种同型II菌株。此外,使用针对与麦芽糖结合蛋白融合的TbpB M982(氨基酸352至691)或BZ83(氨基酸329至669)的C末端结构域产生的血清,检测到针对12和7个同种型II的交叉杀菌活性分别测试了22个菌株。这些结果表明TbpB的C末端的表面可及性。总的来说,这些结果表明,尽管在基于TbpB的疫苗的组成中需要一个以上的rTbpB才能实现完全的交叉杀菌活性,但是rTbpB及其C末端本身能够诱导交叉杀菌抗体。

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