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一种带有截短鞭毛蛋白的嵌合疟疾抗原引发的快速和持久的体液免疫。

Prompt and Robust Humoral Immunity Elicited by a Conjugated Chimeric Malaria Antigen with a Truncated Flagellin.

机构信息

National Key Laboratory of Biochemical Engineering, Institute of Process Engineering , Chinese Academy of Sciences , Beijing 100190 , PR China.

University of Chinese Academy of Sciences , Beijing 100049 , PR China.

出版信息

Bioconjug Chem. 2018 Mar 21;29(3):761-770. doi: 10.1021/acs.bioconjchem.7b00320. Epub 2017 Aug 22.

Abstract

As one of the pathogen-associated molecular patterns (PAMPs), flagellin is recently utilized as a potent adjuvant for many subunit vaccines. In this study, a truncated flagellin (tFL) with deletion of the hypervariable regions was adopted as a carrier-adjuvant by chemical conjugation with a chimeric malaria antigen M.RCAg-1 (M312) via a heterobifunctional polyethylene glycol (PEG) linker. After booster immunization in mice without any extra adjuvants, the M312-PEG-tFL conjugates elicited M312-specific antibody titers 100-1000 times higher than M312 and 10-100 times higher than the physical mixture of M312 and tFL. The elicited specific antibodies could recognize the native parasites, and the immunofluorescence assay (IFA) titer was 2100 for M312-P5k-tFL, which was about 7 times higher than M312. Furthermore, the IFA titers of the conjugates were comparable to the positive control of complete Freund's adjuvant (CFA). Compared to M312, the M312-PEG-tFL conjugates enhanced the proliferation index, lymphocyte activation, and memory T-cell generation. IgG subclasses of sera and cytokines analysis of splenocytes showed that conjugation with tFL could slightly trigger the Th1 polarization, while the antigen alone predominantly induced a Th2-biased immune response. Furthermore, a more-efficient innate immune response was provoked by the M312-PEG-tFL conjugates, as determined by the detection of antigen-specific TNF-α secretion by splenocytes. Our results indicated that tFL mainly retained the function as an agonist of TLR5. Conjugation of antigen to tFL could induce strong humoral and moderate cellular immune responses. Thus, conjugation of antigen to tFL as a potent carrier-adjuvant is an effective strategy for developing a promising protein-based vaccine.

摘要

作为一种病原体相关分子模式(PAMPs),鞭毛蛋白最近被用作许多亚单位疫苗的有效佐剂。在这项研究中,通过化学偶联,将缺失超变区的截短鞭毛蛋白(tFL)与嵌合疟疾抗原 M.RCAg-1(M312)通过杂双功能聚乙二醇(PEG)接头连接在一起,作为载体-佐剂。在没有任何额外佐剂的情况下,对小鼠进行加强免疫后,M312-PEG-tFL 缀合物引起的 M312 特异性抗体滴度比 M312 高 100-1000 倍,比 M312 和 tFL 的物理混合物高 10-100 倍。诱导的特异性抗体可识别天然寄生虫,免疫荧光分析(IFA)滴度为 M312-P5k-tFL 为 2100,约比 M312 高 7 倍。此外,缀合物的 IFA 滴度与完全弗氏佐剂(CFA)的阳性对照相当。与 M312 相比,M312-PEG-tFL 缀合物增强了增殖指数、淋巴细胞活化和记忆 T 细胞生成。血清 IgG 亚类和脾细胞细胞因子分析表明,与 tFL 缀合可轻微触发 Th1 极化,而抗原本身主要诱导 Th2 偏向免疫反应。此外,通过检测脾细胞中抗原特异性 TNF-α的分泌,M312-PEG-tFL 缀合物引起了更有效的先天免疫反应。我们的结果表明,tFL 主要保留作为 TLR5 激动剂的功能。抗原与 tFL 的缀合可以诱导强烈的体液和适度的细胞免疫反应。因此,将抗原与 tFL 缀合作为一种有效的载体-佐剂,是开发有前途的蛋白质疫苗的有效策略。

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