Kohler J, Martin S, Pflugfelder U, Ruh H, Vollmer J, Weltzien H U
Max-Planck-Institut für Immunbiologie, Freiburg, FRG.
Eur J Immunol. 1995 Jan;25(1):92-101. doi: 10.1002/eji.1830250118.
The induction of contact sensitivity in mice by hapten reagents such as trinitrochlorobenzene (TNCB) involves the activation of class II major histocompatibility complex (MHC)-restricted, hapten-specific, CD4+ T cells. Reports from different laboratories have indicated that the relevant antigenic epitopes in such reactions might include hapten-conjugated, MHC class II-associated peptides. This study for the first time directly demonstrates that hapten-peptides account for the majority of determinants recognized by trinitrophenyl (TNP)-specific CD4+ T lymphocytes. The sequences of those TNP carrier peptides do not have to be related to mouse proteins. Thus, we show that TNP-modified peptides derived from mouse IgG, pigeon cytochrome c or staphylococcal nuclease known to bind to I-Ab or from lambda repressor with specificity to I-Ad as well as TNP-proteins such as bovine serum albumin, ovalbumin or keyhole limpet hemocyanin all create class II-restricted hapten determinants for a number of TNP-specific T cell clones and hybridomas. All of these cells were induced with cells modified by trinitrobenzene sulfonic acid (TNBS). In addition, we present arguments indicating that individual TNP-specific helper T cells may cross-react with different TNP-peptides bound to identical class II molecules. Chemical treatment of antigen-presenting cells with TNCB or TNBS may thus result in a limited number of particularly repetitive immunodominant hapten epitopes. Immunodominant epitopes were also indicated by an overrepresentation of the TCR elements V beta 2 and V alpha 10 in I-Ab/TNP-specific T cells. Most importantly, however, we demonstrate that TNP attached to lysine 97 in the staphylococcal nuclease peptide 93-105 (i.e. a clearly "non-self" sequence) is able to prime mice for subsequent elicitation of contact sensitivity by TNCB in the absence of foreign protein. We take this to indicate that those TNP-peptide determinants defined by us as immuno-dominant are responsible for the induction of contact sensitivity to haptens.
用诸如三硝基氯苯(TNCB)等半抗原试剂在小鼠中诱导接触敏感性涉及II类主要组织相容性复合体(MHC)限制的、半抗原特异性的CD4 + T细胞的激活。不同实验室的报告表明,此类反应中相关的抗原表位可能包括半抗原结合的、与MHC II类相关的肽段。本研究首次直接证明,半抗原肽占三硝基苯基(TNP)特异性CD4 + T淋巴细胞识别的决定簇的大部分。那些TNP载体肽的序列不必与小鼠蛋白相关。因此,我们表明,源自已知与I - Ab结合的小鼠IgG、鸽细胞色素c或葡萄球菌核酸酶或源自对I - Ad具有特异性的λ阻遏物的TNP修饰肽,以及诸如牛血清白蛋白、卵清蛋白或钥孔戚血蓝蛋白等TNP蛋白,均为许多TNP特异性T细胞克隆和杂交瘤产生II类限制的半抗原决定簇。所有这些细胞均用经三硝基苯磺酸(TNBS)修饰的细胞诱导。此外,我们提出的论据表明,单个TNP特异性辅助性T细胞可能与结合到相同II类分子上的不同TNP肽发生交叉反应。用TNCB或TNBS对抗抗原呈递细胞进行化学处理可能因此导致数量有限的特别重复的免疫显性半抗原表位。I - Ab/TNP特异性T细胞中TCR元件Vβ2和Vα10的过度表达也表明了免疫显性表位。然而,最重要的是,我们证明,附着于葡萄球菌核酸酶肽93 - 105中赖氨酸97的TNP(即一个明显的“非自身”序列)能够使小鼠致敏,以便随后在无外源蛋白的情况下由TNCB引发接触敏感性。我们据此认为,我们定义为免疫显性的那些TNP肽决定簇负责对半抗原的接触敏感性的诱导。
