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首页> 外文期刊>Journal of Extracellular Vesicles >Proteome‐minimized outer membrane vesicles from Escherichia coli as a generalized vaccine platform
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Proteome‐minimized outer membrane vesicles from Escherichia coli as a generalized vaccine platform

机译:来自<斜体>大肠杆菌的蛋白质组最小化的外膜囊泡作为广义疫苗平台的

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Because of their potent adjuvanticity, ease of manipulation and simplicity of production Gram‐negative Outer Membrane Vesicles OMVs have the potential to become a highly effective vaccine platform. However, some optimization is required, including the reduction of the number of endogenous proteins, the increase of the loading capacity with respect to heterologous antigens, the enhancement of productivity in terms of number of vesicles per culture volume. In this work we describe the use of Synthetic Biology to create Escherichia coli BL21(DE3)Δ60, a strain releasing OMVs (OMVs _(Δ60)) deprived of 59 endogenous proteins. The strain produces large quantities of vesicles (&?40?mg/L under laboratory conditions), which can accommodate recombinant proteins to a level ranging from 5% to 30% of total OMV proteins. Moreover, also thanks to the absence of immune responses toward the inactivated endogenous proteins, OMVs _(Δ60) decorated with heterologous antigens/epitopes elicit elevated antigens/epitopes‐specific antibody titers and high frequencies of epitope‐specific IFN‐γ‐producing CD8 ~(+) T cells. Altogether, we believe that E. coli BL21(DE3)Δ60 have the potential to become a workhorse factory for novel OMV‐based vaccines.
机译:由于它们有效的辅助性,易于操纵和生产革兰氏阴性外膜囊泡OMV的易于操纵和简单性具有潜力成为一个高效的疫苗平台。然而,需要一些优化,包括减少内源蛋白的数量,相对于异源抗原的负载能力的增加,在每种培养体积的囊泡数量方面提高生产率。在这项工作中,我们描述了合成生物学的使用来创建大肠杆菌BL21(DE3)Δ60,脱离59个内源蛋白的菌株释放OMV(OMVS _(Δ60))。该菌株在实验室条件下产生大量的囊泡(& 40×mg / L),其可以容纳重组蛋白质,从总OMV蛋白的5%〜30%的水平。此外,还由于没有对灭活内源蛋白的免疫应答,OMVS _(Δ60)用异源抗原/表位引起升高的抗原/表位特异性抗体滴度和高频特异性IFN-γ-产生CD8〜的高频率(+)T细胞。完全,我们认为E. Coli BL21(DE3)Δ60有可能成为新型OMV的疫苗的工作厂。
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