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Biochemical evidence for the rapid assembly and disassembly of processed antigen-major histocompatibility complex class II complexes in acidic vesicles of B cells

机译:B细胞酸性囊泡中加工过的抗原-主要组织相容性复合物II类复合物快速组装和拆卸的生化证据

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摘要

Helper T cell recognition of antigen requires that it be processed within antigen-presenting cells (APC) to peptide fragments that subsequently bind to major histocompatibility complex (MHC) class II molecules and are displayed on the APC surface. Heretofore, processed antigen-MHC class II complexes have been detected by functional assays, measuring the activation of specific T cells. We now report direct, biochemical evidence for the assembly of processed antigen-MHC class II complexes within splenic B cells as APC. The I-Ek MHC class II molecules were immunoprecipitated from B cells that had processed the model protein antigen cytochrome c radiolabeled across its entire length by reductive methylation of lysine residues and covalently coupled to Ig-specific antibodies, allowing internalization after binding to surface Ig. Our previous studies showed that I-Ek immunoaffinity purified from B cells that had processed cytochrome c contains functional processed antigen--MHC class II complexes and that approximately 0.2% of the I-Ek molecules are specifically associated with one of two predominant processed antigenic fragments. Here we show that these complexes are rapidly assembled, within 30-60 min after antigen binding to surface Ig on splenic B cells. Maximal numbers of complexes are assembled by 2 h in a process that is sensitive to acidic vesicle inhibitors but not to inhibitors of protein synthesis. The processed antigen-I-Ek complexes have a relatively short half-life of 2- 4 h and are disassembled or degraded within 8 h after antigen is first internalized. The disassembly or degradation of the processed antigen-I- Ek complexes requires acidic vesicle function, and in the presence of an acidic vesicle inhibitor the complexes are long lived. Thus, using a biochemical assay to monitor processed antigen-I-Ek complexes, we find that, in B cells, processed antigen is relatively rapidly associated in acidic vesicles with preexisting MHC class II molecules, and the complexes are disassembled 4-6 h later in processes that also require acid vesicle function.
机译:抗原的辅助T细胞识别需要在抗原呈递细胞(APC)中加工成肽片段,该肽片段随后与主要的组织相容性复合物(MHC)II类分子结合并显示在APC表面。迄今为止,已通过功能测定法检测了加工过的抗原-MHC II类复合物,从而测量了特异性T细胞的活化。我们现在报告直接生化证据为脾脏B细胞作为APC组装的抗原MHC II类复合物的加工。 I-Ek MHC II类分子从B细胞免疫沉淀,该B细胞已通过赖氨酸残基的还原甲基化在整个长度上对模型蛋白抗原细胞色素c进行了放射性标记,并与Ig特异性抗体共价偶联,从而在与表面Ig结合后得以内在化。我们以前的研究表明,从已加工细胞色素c的B细胞纯化的I-Ek免疫亲和力包含功能性加工的抗原-MHC II类复合物,并且大约0.2%的I-Ek分子与两个主要加工的抗原片段之一特异性结合。在这里,我们显示这些复合物在抗原结合脾B细胞上的表面Ig后的30-60分钟内迅速组装。在对酸性囊泡抑制剂敏感但对蛋白质合成抑制剂不敏感的过程中,最大数量的复合物要在2 h内组装完毕。加工过的抗原-I-Ek复合物的半衰期相对较短,为2-4小时,在抗原首次被内化后的8小时内被分解或降解。加工的抗原-I-Ek复合物的分解或降解需要酸性囊泡功能,并且在酸性囊泡抑制剂的存在下,复合物寿命长。因此,使用生化分析监测加工的抗原-I-Ek复合物,我们发现,在B细胞中,加工的抗原在酸性囊泡中与先前存在的MHC II类分子相对较快地缔合,并且该复合物在4-6小时后分解在还需要酸性囊泡功能的过程中。

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  • 年度 1992
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