Weltzien H U, Kempkes B, Jankovic D L, Eichmann K
Eur J Immunol. 1986 Jun;16(6):631-9. doi: 10.1002/eji.1830160608.
Two experimental systems have demonstrated somatic variation of antigen recognition specificity of long-term cytotoxic T cell (CTL) clones. System 1 used CTL clone BT7.4.1 with strict specificity for Kb/TNP, which had been continuously cultured for 15 months in the presence of H-2b/TNP stimulator cells and interleukin 2. Upon removal of the TNP antigen from the cultures, 99% of the clone cells within about 10 cell divisions lost their ability to grow in the presence of antigen and interleukin 2 (lethal variants). Of the surviving 1%, about 60% retained the ability to lyse target cells in the presence of lectins but only 12% could be considered as "wild type" BT7.4.1 cells, i.e. they still specifically lysed H-2b/TNP-bearing target cells. The majority of the growing cells, thus, had to be considered as specificity loss variants. Several specificity loss variants were established in culture and were shown to express membrane-bound T cell "receptor" heterodimer similar to their TNP-specific ancestor, BT7.4.1. Principally the same types of variants were generated in cultures growing in the presence of TNP antigen, although in quantitatively reduced numbers. Under these conditions the specific stimulator cells appeared to impose a significant selective advantage for "wild type" CTL since even after 15 months the cultures fully retained their specificity for the nominal antigen. In system 2, the development of cytolytic fine specificity of a panel of 42 individual Kb/TNP-specific CTL clones was followed over a period of 8 months of in vitro culture. At the beginning of the test, 37 of these clones exhibited significant cross-reactivity for lysis of H-2k/TNP target cells. This number of cross-reactive clones continuously diminished with time and dropped to only 4 clones after 8 months in culture. All 42 clones retained their original Kb/TNP specificity and after losing their reactivity for H-2k/TNP usually showed no decrease but rather an increase in their cytotoxic activity towards Kb/TNP target cells. Loss of H-2k/TNP cross-reactivity was not accompanied by loss of Lyt-2 or of LFA-1 surface antigens or by loss of sensitivity of the cytotoxicity to inhibition by anti-Lyt-2 or by anti-LFA-1 antibody. We conclude from these observations that in vitro cultivated CTL clones, at least those of C57BL/6 anti-TNP-C57BL/6 specificity, are not stable in terms of their antigen recognition specificity.(ABSTRACT TRUNCATED AT 400 WORDS)
两个实验系统已证明长期细胞毒性T细胞(CTL)克隆的抗原识别特异性存在体细胞变异。系统1使用对Kb/TNP具有严格特异性的CTL克隆BT7.4.1,该克隆在H-2b/TNP刺激细胞和白细胞介素2存在的情况下连续培养了15个月。从培养物中去除TNP抗原后,约10个细胞分裂内99%的克隆细胞在有抗原和白细胞介素2存在的情况下失去了生长能力(致死变异体)。在存活的1%中,约60%在有凝集素存在的情况下保留了裂解靶细胞的能力,但只有12%可被视为“野生型”BT7.4.1细胞,即它们仍能特异性裂解携带H-2b/TNP的靶细胞。因此,大多数生长的细胞必须被视为特异性丧失变异体。在培养中建立了几个特异性丧失变异体,并显示它们表达与TNP特异性祖先BT7.4.1相似的膜结合T细胞“受体”异二聚体。在有TNP抗原存在的情况下生长的培养物中也产生了大致相同类型的变异体,尽管数量上有所减少。在这些条件下,特异性刺激细胞似乎赋予“野生型”CTL显著的选择优势,因为即使在15个月后,培养物仍完全保留其对名义抗原的特异性。在系统2中,对一组42个个体的Kb/TNP特异性CTL克隆的溶细胞精细特异性在体外培养8个月的时间内进行了跟踪。在测试开始时,这些克隆中有37个对裂解H-2k/TNP靶细胞表现出显著的交叉反应性。这种交叉反应性克隆的数量随时间持续减少,培养8个月后降至仅4个克隆。所有42个克隆都保留了其原始的Kb/TNP特异性,在失去对H-2k/TNP的反应性后,它们对Kb/TNP靶细胞的细胞毒性活性通常没有降低,反而有所增加。H-2k/TNP交叉反应性的丧失并未伴随着Lyt-2或LFA-1表面抗原的丧失,也未伴随着细胞毒性对抗Lyt-2或抗LFA-1抗体抑制的敏感性丧失。我们从这些观察结果得出结论,体外培养的CTL克隆,至少那些具有C57BL/6抗TNP-C57BL/6特异性的克隆,在抗原识别特异性方面是不稳定的。(摘要截断于400字)
