T cell recognition of lysozyme. II. Shift in specificity during long-term culture determined by synthetic overlapping peptides comprising the entire protein chain.

G S Bixler, T Yoshida, M Z Atassi
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引用次数: 9

Abstract

Recently, by using a comprehensive synthetic strategy developed in this laboratory, we localized four sites (T sites) within the polypeptide chain of lysozyme recognized by T cells from two high responder mouse strains, DBA/1 and B10.BR. However, to detect minor specificities, the selective enrichment of lysozyme reactive cells, would be required. T cells from long-term cultures maintained by repeated stimulation with antigen are selectively enriched for that antigen. It is not known whether maintaining T cells for extended periods of time in vitro has any consequences on the profile of T cell recognition. In the present study, T cells from long-term cultures, derived from these two high responder lysozyme-primed mouse strains, were examined for their responsiveness to a series of synthetic overlapping peptides encompassing the entire polypeptide chain of the lysozyme molecule. We have found that the profile of T cell recognition of the long-term cultures may not reflect that of the lysozyme primed lymph node cells, but that it is subject to a shift in specificity towards submolecular features of the molecule. In addition, we have identified in B10.BR mice another region within the polypeptide chain of lysozyme (residues 72-84) which may potentially harbor a previously undetected (in lymph node cells) minor T site.

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T细胞识别溶菌酶。2在长期培养过程中,特异性的转变由合成重叠肽组成的整个蛋白质链决定。
最近,通过本实验室开发的综合合成策略,我们在两个高反应小鼠菌株DBA/1和B10.BR的T细胞识别的溶菌酶多肽链中定位了四个位点(T位点)。然而,为了检测次要特异性,需要选择性富集溶菌酶反应细胞。通过反复刺激长期培养的T细胞可以选择性地富集该抗原。目前尚不清楚在体外长时间维持T细胞是否对T细胞识别的特征有任何影响。在本研究中,来自这两种高反应性溶菌酶引物小鼠菌株的长期培养的T细胞,被检测对一系列合成的覆盖整个溶菌酶分子多肽链的重叠肽的反应性。我们发现,长期培养的T细胞识别谱可能不能反映溶菌酶引发的淋巴结细胞的识别谱,但它受到分子亚分子特征特异性转变的影响。另外,我们已经在B10中进行了识别。BR小鼠溶菌酶多肽链中的另一个区域(残基72-84),可能含有以前未被发现的(在淋巴结细胞中)小T位点。
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