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抗原加工突变体T2表明MHC连锁基因在II类抗原呈递中发挥作用。

The antigen-processing mutant T2 suggests a role for MHC-linked genes in class II antigen presentation.

作者信息

Riberdy J M, Cresswell P

机构信息

Howard Hughes Medical Institute, Yale University School of Medicine, New Haven, CT 06510.

出版信息

J Immunol. 1992 Apr 15;148(8):2586-90.

PMID:1373173
Abstract

.174xCEM.T2 (T2) is a human cell hybrid that has a large homozygous deletion within the MHC, including all of the functional class II genes. We have generated stable HLA-DR3 and H-2 I-Ak transfectants of T2 that express parental levels of class II molecules at the cell surface. T2.Ak transfectants fail to stimulate a hen egg lysozyme (HEL)-specific, I-Ak-restricted T cell when incubated with intact HEL. However, stimulation occurs if the appropriate HEL peptide is provided. The T2 cell line therefore has a defect in class II-restricted Ag processing. Biosynthetic studies demonstrate that the kinetics of I-Ak transport in T2.Ak are similar to the parental rates of transport, although the percentage of I-Ak molecules transported appears somewhat lower. I-Ak glycoproteins in T2.Ak associate normally with the I-chain, which appears to be proteolytically cleaved after transport through the Golgi apparatus in a similar fashion to that in the parent cell line, .174xCEM.T1 (T1). The DR alpha beta heterodimers in T2 differ from the parental phenotype in two ways. First, HLA-DR3 expressed in T2 does not have the epitope recognized by the DR3-specific mAb 16.23, although DR3 expressed in the parent does have the epitope. Second, the alpha beta subunits in the parent remain associated when exposed to SDS at room temperature, although those in T2 dissociate.

摘要

.174xCEM.T2(T2)是一种人类细胞杂交体,其主要组织相容性复合体(MHC)内存在一个大的纯合缺失,包括所有功能性Ⅱ类基因。我们已经构建了T2细胞的稳定HLA - DR3和H - 2 I - Ak转染体,它们在细胞表面表达亲本水平的Ⅱ类分子。当与完整的溶菌酶(HEL)一起孵育时,T2.Ak转染体不能刺激HEL特异性、I - Ak限制性T细胞。然而,如果提供合适的HEL肽,则会发生刺激。因此,T2细胞系在Ⅱ类限制性抗原加工方面存在缺陷。生物合成研究表明,T2.Ak中I - Ak的转运动力学与亲本转运速率相似,尽管转运的I - Ak分子百分比似乎略低。T2.Ak中的I - Ak糖蛋白通常与I链结合,在通过高尔基体转运后,I链似乎以与亲本细胞系.174xCEM.T1(T1)相似的方式被蛋白水解切割。T2中的DRαβ异二聚体在两个方面与亲本表型不同。首先,T2中表达的HLA - DR3不具有DR3特异性单克隆抗体16.23识别的表位,尽管亲本中表达的DR3具有该表位。其次,当在室温下暴露于SDS时,亲本中的αβ亚基保持结合状态,而T2中的αβ亚基则解离。

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