Live attenuated Salmonella displaying HIV-1 10E8 epitope on fimbriae: systemic and mucosal immune responses in BALB/c mice by mucosal administration

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作者
Qing-Hai Li
Gang Jin
Jia-Ye Wang
Hai-Ning Li
Huidi Liu
Xiao-Yun Chang
Fu-Xiang Wang
Shu-Lin Liu
机构
[1] Systemomics Center,Department of Microbiology
[2] College of Pharmacy and Genomics Research Center (State-Province Key Laboratories of Biomedicine-Pharmaceutics of China),Department of Infectious Diseases
[3] Harbin Medical University,Department of Infectious Diseases
[4] Harbin Medical University,Department of Microbiology
[5] The Fourth Affiliated Hospital of Harbin Medical University,undefined
[6] The First Affiliated Hospital,undefined
[7] Harbin Medical University,undefined
[8] Immunology and Infectious Diseases,undefined
[9] University of Calgary,undefined
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The HIV-1 membrane proximal external region (MPER) that is targeted by several broadly neutralizing antibodies (BNAbs) has been considered a potential immunogen for vaccine development. However, to date the immunogenicity of these BNAb epitopes has not been made sufficiently adequate. In the present work, we used live attenuated Salmonella as a platform to present the HIV-1 MPER 10E8 epitope in the fimbriae. The insertion of the 10E8 epitope into the fimbriae had no significant influence on the expression and the absorption capacity of bacterial fimbriae, nor on the virulence and invasiveness of the attenuated Salmonella. After oral administration of the vaccine construct to mice followed by 10E8 epitope peptide boost, specific antibody responses in serum and mucosa as well as memory lymphocytes in spleen and plasma cells in bone marrow were induced. We also found that the live attenuated Salmonella vector directed the immunity toward Th1 bias, induced Th1 and Th2 cytokine responses and stimulated significant B cell differentiation into GC B, memory B and plasma cells. Therefore, we propose that the live attenuated Salmonella constitutively expressing HIV-1 BNAb epitopes on the fimbriae will be an effective approach to improving immune microenvironment and enhancing the immunogenicity of HIV-1 epitope vaccines.
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