通过与主要组织相容性复合体 II 类分子的非肽结合区结合,用不变链片段增强免疫反应。
Boosting immune response with the invariant chain segments via association with non-peptide binding region of major histocompatibility complex class II molecules.
机构信息
Key Laboratory of Zoonoses of Anhui Province, Anhui Agricultural University, 130 Changjiang West Road, Hefei 230036, China.
出版信息
BMC Immunol. 2012 Sep 27;13:55. doi: 10.1186/1471-2172-13-55.
BACKGROUND
Based on binding of invariant chain (Ii) to major histocompatibility complex (MHC) class II molecules to form complexes, Ii-segment hybrids, Ii-key structure linking an epitope, or Ii class II-associated invariant chain peptide (CLIP) replaced with an epitope were used to increase immune response. It is currently unknown whether the Ii-segment cytosolic and transmembrane domains bind to the MHC non-peptide binding region (PBR) and consequently influence immune response. To investigate the potential role of Ii-segments in the immune response via MHC II/peptide complexes, a few hybrids containing Ii-segments and a multiepitope (F306) from Newcastle disease virus fusion protein (F) were constructed, and their binding effects on MHC II molecules and specific antibody production were compared using confocal microscopy, immunoprecipitation, western blotting and animal experiments.
RESULTS
One of the Ii-segment/F306 hybrids, containing ND (Asn-Asp) outside the F306 in the Ii-key structure (Ii-key/F306/ND), neither co-localized with MHC II molecules on plasma membrane nor bound to MHC II molecules to form complexes. However, stimulation of mice with the structure produced 4-fold higher antibody titers compared with F306 alone. The two other Ii-segment/F306 hybrids, in which the transmembrane and cytosolic domains of Ii were linked to this structure (Cyt/TM/Ii-key/F306/ND), partially co-localized on plasma membrane with MHC class II molecules and weakly bound MHC II molecules to form complexes. They induced mice to produce approximately 9-fold higher antibody titers compared with F306 alone. Furthermore, an Ii/F306 hybrid (F306 substituting CLIP) co-localized well with MHC II molecules on the membrane to form complexes, although it increased antibody titer about 3-fold relative to F306 alone.
CONCLUSIONS
These results suggest that Ii-segments improve specific immune response by binding to the non-PBR on MHC class II molecules and enabling membrane co-localization with MHC II molecules, resulting in the formation of relatively stable MHC II/peptide complexes on the plasma membrane, and signal transduction.
背景
基于不变链 (Ii) 与主要组织相容性复合体 (MHC) Ⅱ类分子结合形成复合物,Ii 片段杂合体、连接表位的Ii 键结构或替换为表位的Ii 类 II 相关不变链肽 (CLIP) 被用于增强免疫反应。目前尚不清楚 Ii 片段胞质和跨膜结构域是否与 MHC 非肽结合区 (PBR) 结合,从而影响免疫反应。为了通过 MHC II/肽复合物研究 Ii 片段在免疫反应中的潜在作用,构建了几个包含 Ii 片段和新城疫病毒融合蛋白 (F) 中多个表位 (F306) 的杂合体,并使用共聚焦显微镜、免疫沉淀、western blot 和动物实验比较了它们对 MHC II 分子的结合效应和特异性抗体的产生。
结果
Ii 键结构中的 F306 外部含有 ND (天冬酰胺-天冬氨酸) 的一个 Ii 片段/F306 杂合体 (Ii-key/F306/ND),既不在质膜上与 MHC II 分子共定位,也不与 MHC II 分子结合形成复合物。然而,用该结构刺激小鼠可使抗体滴度比单独使用 F306 高 4 倍。另外两个 Ii 片段/F306 杂合体,其中 Ii 的跨膜和胞质结构域与该结构相连 (Cyt/TM/Ii-key/F306/ND),部分在质膜上与 MHC Ⅱ类分子共定位,并与 MHC Ⅱ类分子弱结合形成复合物。与单独使用 F306 相比,它们诱导小鼠产生约 9 倍的高抗体滴度。此外,一个 Ii/F306 杂合体 (F306 取代 CLIP) 与膜上的 MHC II 分子很好地共定位形成复合物,尽管与单独使用 F306 相比,它使抗体滴度提高了约 3 倍。
结论
这些结果表明,Ii 片段通过与 MHC Ⅱ类分子的非 PBR 结合,并使 MHC Ⅱ分子与膜共定位,从而在质膜上形成相对稳定的 MHC II/肽复合物并进行信号转导,从而改善特异性免疫反应。
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