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稳定转染的B淋巴瘤细胞将IgG2a抗原呈递给II类限制性T细胞。

Presentation of IgG2a antigens to class II-restricted T cells by stably transfected B lymphoma cells.

作者信息

Bikoff E K, Eckhardt L A

机构信息

Department of Obstetrics, Gynecology and Reproductive Sciences, Mount Sinai School of Medicine, New York, NY 10029.

出版信息

Eur J Immunol. 1989 Oct;19(10):1903-9. doi: 10.1002/eji.1830191022.

Abstract

Here we describe a panel of BALB/c T cells specific for IgG2a of the b allotype in association with I-Ad. We used DNA-mediated gene transfer techniques to localize antigenic determinants recognized by responding T cells. Initially a truncated IgG2aa gene comprising a variable domain and the CH3 domain (not including the membrane exons) from the BALB/c IgG2aa heavy chain was introduced into myeloma cells. The V-CH3 protein was expressed at high levels under control of the Ig heavy chain enhancer. Secretion of the V-CH3 protein did not require assembly of H-H dimers or an association with light chains. To generate stably transfected B cell lines that would stimulate our class II-restricted T cells, we replaced most of the BALB/c IgG2aa CH3 exon with CH3 coding sequences from a C57BL/6 IgG2ab cDNA clone and introduced these constructs into Ia+ B lymphoma cells. The IgG2ab CH3-transfected B cells were recognized by BALB/c Igh-1b-specific T cell hybrids in the absence of exogenous antigen. Experiments using glutaraldehyde-fixed cells as stimulators indicate that presentation of the secreted form of V-IgG2ab CH3 requires processing. We found that a significant fraction of the endogenously synthesized V-IgG2ab CH3 protein was, however, present as already processed antigen.

摘要

在此,我们描述了一组与I-Ad相关的、对b同种异型IgG2a具有特异性的BALB/c T细胞。我们使用DNA介导的基因转移技术来定位反应性T细胞识别的抗原决定簇。最初,将一个截短的IgG2aa基因导入骨髓瘤细胞,该基因包含来自BALB/c IgG2aa重链的一个可变结构域和CH3结构域(不包括膜外显子)。V-CH3蛋白在Ig重链增强子的控制下高水平表达。V-CH3蛋白的分泌不需要H-H二聚体的组装或与轻链的结合。为了产生能够刺激我们的II类限制性T细胞的稳定转染B细胞系,我们用来自C57BL/6 IgG2ab cDNA克隆的CH3编码序列替换了大部分BALB/c IgG2aa CH3外显子,并将这些构建体导入Ia+B淋巴瘤细胞。在没有外源性抗原的情况下,IgG2ab CH3转染的B细胞被BALB/c Igh-1b特异性T细胞杂交瘤识别。使用戊二醛固定细胞作为刺激剂的实验表明,分泌形式的V-IgG2ab CH3的呈递需要加工。然而,我们发现内源性合成的V-IgG2ab CH3蛋白中有很大一部分是以已经加工的抗原形式存在的。

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