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表达γδ T细胞受体的人T淋巴细胞的分子与细胞分析

Molecular and cellular analysis of human T lymphocytes expressing gamma delta T-cell receptor.

作者信息

Moretta L, Ciccone E, Ferrini S, Pelicci P G, Mingari M C, Zeromski J, Bottino C, Grossi C, Moretta A

机构信息

Istituto Nazionale per la Ricerca sul Cancro, Genova, Italy.

出版信息

Immunol Rev. 1991 Apr;120:117-35. doi: 10.1111/j.1600-065x.1991.tb00590.x.

DOI:10.1111/j.1600-065x.1991.tb00590.x
PMID:1650757
Abstract

A minor subset of T lymphocytes expresses a CD3-associated TCR composed of gamma and delta chains. The majority of TCR gamma/delta+ cells lack surface CD4 and CD8 antigen and do not react with WT31 mAb. These negative criteria were utilized in early studies to identify TCR gamma/delta+ cells. More recently, mAb to TCR gamma/delta, selected in different laboratories, have permitted the direct identification of TCR gamma/delta+ cells and their subsets. TCR gamma/delta molecules were found to be heterogeneous in size and charge mobility. Two major forms of TCR gamma/delta could be identified that are characterized by the presence or absence of an inter-chain disulphide bond. Biochemical analysis originally suggested that a precise correlation existed between reactivity with BB3 or delta TCS1/A13 mAb and expression of a disulphide (C gamma 1-encoded) or non-disulphide linked (C gamma 2-encoded) form of TCR gamma/delta. However, more recent studies have indicated that these mAb react with the molecular product of V delta 2 or V delta 1, respectively, mAb directed to one or another form of TCR gamma/delta activate the functional program of the cell, leading to intracellular Ca++ mobilization, lymphokine production and triggering of the lytic machinery. Analysis of the target molecules for TCR gamma/delta-mediated recognition revealed that at least some TCR gamma/delta+ cells are capable of specific responses to (allo)antigen and that polymorphic determinants of class I molecules can be recognized (as shown by the specific lysis of P815 cells transfected with HLA-24 allele). Unlike TCR alpha/beta+ cells, TCR gamma/delta+ cells are homogeneously composed of cytolytic precursors, as shown by the analysis of a large panel of clones in both lectin-dependent and redirected killing assays. In spite of their LGL morphology, freshly isolated TCR gamma/delta+ cells do not lyse NK-sensitive targets but do so after exposure to rIL-2. A modest cytolytic activity, however, could be induced also in fresh cells by anti-TCR/CD3 mAb in a redirected killing assay. Analysis of the distribution of the subsets expressing different TCR gamma/delta types showed that BB3+ cells are prevalent in the peripheral blood and virtually absent in the thymus; in contrast, A13+ (delta TCS1+) cells represent the majority of TCR gamma/delta+ thymocytes. Electron microscopic analysis of fresh TCR gamma/delta+ cells showed an extended cytoplasm containing numerous electron-dense granules identifiable as primary lysosomes. Upon stimulation with IL-2, TCR gamma/delta+ cells, similar to other LAK cells, display an increase in their cytoplasmic granules together with a redistribution of cytoskeletal structures.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

一小部分T淋巴细胞表达由γ和δ链组成的与CD3相关的TCR。大多数TCRγ/δ+细胞缺乏表面CD4和CD8抗原,且不与WT31单克隆抗体发生反应。早期研究利用这些阴性标准来鉴定TCRγ/δ+细胞。最近,在不同实验室筛选出的针对TCRγ/δ的单克隆抗体,使得直接鉴定TCRγ/δ+细胞及其亚群成为可能。发现TCRγ/δ分子在大小和电荷迁移率方面具有异质性。可以鉴定出TCRγ/δ的两种主要形式,其特征在于链间二硫键的存在与否。生化分析最初表明,与BB3或δTCS1/A13单克隆抗体的反应性与二硫键连接(由Cγ1编码)或非二硫键连接(由Cγ2编码)形式的TCRγ/δ的表达之间存在精确的相关性。然而,最近的研究表明,这些单克隆抗体分别与Vδ2或Vδ1的分子产物发生反应,针对一种或另一种形式的TCRγ/δ的单克隆抗体激活细胞的功能程序,导致细胞内Ca++动员、淋巴因子产生以及溶细胞机制的触发。对TCRγ/δ介导的识别的靶分子分析表明,至少一些TCRγ/δ+细胞能够对(同种异体)抗原产生特异性反应,并且I类分子的多态性决定簇可以被识别(如用HLA - 24等位基因转染的P815细胞的特异性裂解所示)。与TCRα/β+细胞不同,TCRγ/δ+细胞均由溶细胞前体组成,这在凝集素依赖性和重定向杀伤试验中对大量克隆的分析中得到了证实。尽管它们具有大颗粒淋巴细胞(LGL)的形态,但新鲜分离的TCRγ/δ+细胞不会裂解NK敏感靶细胞,但在暴露于重组白细胞介素 - 2(rIL - 2)后会裂解。然而,在重定向杀伤试验中,抗TCR/CD3单克隆抗体也可以在新鲜细胞中诱导适度的溶细胞活性。对表达不同TCRγ/δ类型的亚群分布分析表明,BB3+细胞在外周血中普遍存在,而在胸腺中几乎不存在;相反,A13+(δTCS1+)细胞代表了大多数TCRγ/δ+胸腺细胞。对新鲜TCRγ/δ+细胞的电子显微镜分析显示,其细胞质延伸,含有许多可识别为初级溶酶体的电子致密颗粒。在用白细胞介素 - 2刺激后,TCRγ/δ+细胞与其他淋巴因子激活的杀伤(LAK)细胞类似,其细胞质颗粒增加,同时细胞骨架结构重新分布。(摘要截断于400字)

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