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曼氏血吸虫P28谷胱甘肽S-转移酶肽段115-131多个串联拷贝作为C末端与破伤风毒素片段C融合在减毒活疫苗菌株鼠伤寒沙门氏菌aro中的构建、表达及免疫原性

Construction, expression, and immunogenicity of multiple tandem copies of the Schistosoma mansoni peptide 115-131 of the P28 glutathione S-transferase expressed as C-terminal fusions to tetanus toxin fragment C in a live aro-attenuated vaccine strain of Salmonella.

作者信息

Khan C M, Villarreal-Ramos B, Pierce R J, Demarco de Hormaeche R, McNeill H, Ali T, Chatfield S, Capron A, Dougan G, Hormaeche C E

机构信息

Department of Pathology, University of Cambridge, UK.

出版信息

J Immunol. 1994 Dec 15;153(12):5634-42.

PMID:7527446
Abstract

Genetic fusions have been constructed between the highly immunogenic but atoxic fragment C of tetanus toxin and a guest peptide, aa115-131, from the protective 28-kDa glutathione S-transferase Ag of Schistosoma mansoni. Fusions have been assembled to express one, two, four, and eight tandem copies of the peptide. The recombinant vectors have been electroporated into the nonvirulent aroA strain of Salmonella typhimurium SL3261. The fusion proteins are soluble and stably expressed in Salmonella as evaluated by Western blotting with fragment C and glutathione S-transferase antisera. Mice have been immunized i.v. with a single dose of the live recombinant salmonellae. The strains are stable in mice and elicit Ab responses directed against fragment C, as determined by enzyme-linked immunosorbent assays. Ab responses were also detected against the guest peptide. The Ab responses improved dramatically toward the aa115-131 peptide with increasing copy number, with the octameric "repitope" fusion displaying the greatest potency. This approach may represent a general strategy for eliciting immune responses against peptides in live bacterial vaccines.

摘要

已构建了破伤风毒素高免疫原性但无毒的C片段与来自曼氏血吸虫保护性28 kDa谷胱甘肽S-转移酶Ag的客体肽(aa115 - 131)之间的基因融合体。已组装融合体以表达该肽的一、二、四和八个串联拷贝。将重组载体电穿孔导入鼠伤寒沙门氏菌SL3261的无毒aroA菌株中。通过用C片段和谷胱甘肽S-转移酶抗血清进行蛋白质印迹分析评估,融合蛋白在沙门氏菌中可溶且稳定表达。已通过静脉内注射单剂量的活重组沙门氏菌对小鼠进行免疫。这些菌株在小鼠体内稳定,并引发针对C片段的抗体反应,这通过酶联免疫吸附测定法确定。还检测到针对客体肽的抗体反应。随着拷贝数增加,针对aa115 - 131肽的抗体反应显著改善,八聚体“重复表位”融合体显示出最大效力。这种方法可能代表了在活细菌疫苗中引发针对肽的免疫反应的一种通用策略。

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