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对由细胞毒性T淋巴细胞浸润的次要组织相容性抗原不相合同种异体移植物所表达的T细胞受体进行谱型分析。

Spectratyping of TCRs expressed by CTL-infiltrating minor histocompatibility antigen-disparate allografts.

作者信息

Johnston S L, Borson N D, Wettstein P J

机构信息

Department of Immunology, Mayo Foundation, Rochester, MN 55905, USA.

出版信息

J Immunol. 1997 Dec 1;159(11):5233-45.

PMID:9548462
Abstract

Minor histocompatibility Ags (HA) play prominent roles in stimulating allograft rejection and are recognized by CTLs that mediate this process. However, there is no information on the diversity of TCRs that are specific for single minor histocompatibility Ag peptides and expressed by CTLs in vivo. We have used the technique of spectratyping to study the diversity of Vbeta usage and beta complementarity-determining region 3 (CDR3) length of TCRs expressed by CTL-infiltrating skin allografts expressing the immunogenic H4 peptide during the process of rejection. Spectratyping revealed overall reduction in diversity of both Vbeta usage and CDR3 length, with sequential application of primary, second-set, and third-set H4-incompatible grafts. This dissection of the array of beta-chains expressed by graft-infiltrating CTLs allowed the direct sequencing of individual beta-chain PCR products. Beta CDR3s were characterized by a net negative charge, as we have observed previously with CDR3s expressed by H4-specific CTL clones selected in vitro. Identical and closely related CDR3 amino acid sequences could be identified that were shared by TCRs that 1) utilized different Vbeta genes, 2) derived from different mice, or 3) derived from different sequential sets of allografts on individual mice. Furthermore, a number of CDR3 sequences expressed by graft-infiltrating CTLs were identical or closely related to sequences we have identified previously in in vitro selected CTL clones that were specific for the H4 peptide.

摘要

次要组织相容性抗原(HA)在刺激同种异体移植排斥反应中起重要作用,并被介导这一过程的细胞毒性T淋巴细胞(CTL)识别。然而,关于体内CTL表达的、对单个次要组织相容性抗原肽具有特异性的T细胞受体(TCR)的多样性,尚无相关信息。我们利用光谱分型技术,研究了在排斥过程中表达免疫原性H4肽的CTL浸润的皮肤同种异体移植中,TCR表达的Vβ使用情况和β互补决定区3(CDR3)长度的多样性。光谱分型显示,随着初次、二次和三次H4不相容移植物的依次应用,Vβ使用情况和CDR3长度的多样性总体降低。对移植物浸润CTL表达的β链阵列进行分析,使得能够直接对单个β链PCR产物进行测序。正如我们之前在体外选择的H4特异性CTL克隆所表达的CDR3中观察到的那样,β CDR3的特征是净负电荷。可以鉴定出相同和密切相关的CDR3氨基酸序列,这些序列由以下TCR共享:1)使用不同Vβ基因的TCR;2)来自不同小鼠的TCR;3)来自单个小鼠不同顺序的同种异体移植物的TCR。此外,移植物浸润CTL表达的许多CDR3序列与我们之前在体外选择的、对H4肽具有特异性的CTL克隆中鉴定的序列相同或密切相关。

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