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含有来自鸡卵清溶菌酶(HEL74-90)的两个半胱氨酸残基的T细胞表位的加工与反应性

Processing and reactivity of T cell epitopes containing two cysteine residues from hen egg-white lysozyme (HEL74-90).

作者信息

Kang H K, Mikszta J A, Deng H, Sercarz E E, Jensen P E, Kim B S

机构信息

Department of Microbiology, Northwestern University Medical School, Chicago, IL 60611, USA.

出版信息

J Immunol. 2000 Feb 15;164(4):1775-82. doi: 10.4049/jimmunol.164.4.1775.

Abstract

The Ag processing and structural requirements involved in the generation of a major T cell epitope from the hen egg-white lysozyme protein (HEL74-88), containing two cysteine residues at positions 76 and 80, were investigated. Several T cell hybridomas derived from both low responder (I-Ab) and high responder (I-Ak) mice recognize this region. These hybridomas are strongly responsive to native HEL, but unresponsive to the reduced and carboxymethylated protein. Air-oxidized HEL74-88 peptide was unable to bind I-Ak molecules and failed to stimulate T cells in the absence of intracellular Ag processing. Further functional competition assays showed that alkylation of cysteine residues with bulky methyl groups interferes with the contacts for the MHC class II molecules (I-Ak) of high responder mice and the I-Ab-restricted TCR of low responder mice. Serine substitutions of the cysteine residues of HEL74-88 either enhanced or abrogated T cell stimulation by the peptides without significant alterations in the class II binding. These results suggest that the cysteine residues of peptides must be free from disulfide bonding for efficient stimulation of T cells and yet frequently used modifications of cysteine residues may not be suitable for peptide-based vaccine development.

摘要

研究了从含有位于76和80位两个半胱氨酸残基的鸡蛋清溶菌酶蛋白(HEL74 - 88)产生主要T细胞表位所涉及的抗原(Ag)加工和结构要求。从低反应性(I - Ab)和高反应性(I - Ak)小鼠衍生的几种T细胞杂交瘤识别该区域。这些杂交瘤对天然HEL强烈反应,但对还原和羧甲基化蛋白无反应。空气氧化的HEL74 - 88肽不能结合I - Ak分子,并且在没有细胞内抗原加工的情况下不能刺激T细胞。进一步的功能竞争试验表明,用大体积甲基对半胱氨酸残基进行烷基化会干扰高反应性小鼠的MHC II类分子(I - Ak)和低反应性小鼠的I - Ab限制性TCR的接触。HEL74 - 88半胱氨酸残基的丝氨酸替代要么增强要么消除了肽对T细胞的刺激,而II类结合没有明显改变。这些结果表明,肽的半胱氨酸残基必须没有二硫键才能有效刺激T细胞,然而,半胱氨酸残基常用的修饰可能不适用于基于肽的疫苗开发。

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