Muraoka S
Trudeau Institute, Saranac Lake, NY 12983.
Eur J Immunol. 1991 Sep;21(9):2095-103. doi: 10.1002/eji.1830210918.
Experiments were performed to determine whether CD4+ T cells are required for the generation of cytotoxic T lymphocytes (CTL) specific for the nonpolymorphic major histocompatibility complex (MHC) class I-like antigen, Qa-2. Splenic T cells from BALB/cBy (Qa-2b) mice that had been immunized with irradiated BALB/cJ (Qa-2a) splenocytes generated CTL following in vitro stimulation with BALB/cJ splenocytes. These CTL lysed all Qa-2+, but not Qa-2- targets, regardless of the H-2 haplotypes of target cells or their non-MHC backgrounds. This apparent MHC class I-unrestricted recognition of Qa-2 antigen was confirmed using Qa-2-specific CTL clones. The Qa-2-primed CTL precursor cells (CTLp) and CTL were found to be CD8+ T cells. Primed splenocytes depleted of CD4+ T cells prior to culture failed to generate CTL, but addition of lymphokines to the culture restored the CTL generation. Stimulation of primed splenic T cells with irradiated Qa-2+ T blast cells, instead of splenocytes or B blast cells, led to little to no CTL generation, suggesting that MHC class II molecules are involved in the presentation of Qa-2 antigen to CD4+ T cells. This was also supported by the results of experiments using Qa-2+, class II- thymoma cells of BALB/c origin. Stimulation of the thymoma-primed splenic T cells with the mitomycin C-treated thymoma cells resulted in no generation of anti-Qa-2 CTL, despite the fact that high levels of CTL specific for minor histocompatibility (H) antigens and H-2d were generated by immunizing the corresponding allogeneic hosts with the thymoma. However, the addition of lymphokines rendered thymoma-primed T cells capable of generating anti-Qa-2 CTL. Both CD4+ and CD8+ T cell populations, isolated from the BALB/cJ splenocyte-primed responder cells, proliferated in vitro in response to the Qa-2+ splenocytes, suggesting that Qa-2-reactive CD4+ T cells were present in the immunized mice. Depletion of CD4+ T cells from thymectomized BALB/cBy mice with anti-L3T4 monoclonal antibodies markedly reduced, but did not eliminate anti-Qa-2 CTL generation. In contrast, depletion of CD8+ T cells led to a complete abrogation of the CTL response. Addition of lymphokines to the culture of responder cells depleted of either T cell subset did not restore their reactivity. It is concluded that anti-Qa-2 CTLp need "help" from CD4+ T cells to become primed in vivo. Furthermore, primed CTLp also need "help" or lymphokines provided by CD4+ T cells to differentiate into effector CTL in vitro.(ABSTRACT TRUNCATED AT 400 WORDS)
进行实验以确定细胞毒性T淋巴细胞(CTL)产生针对非多态性主要组织相容性复合体(MHC)I类样抗原Qa-2的特异性反应时是否需要CD4 + T细胞。用经辐照的BALB/cJ(Qa-2a)脾细胞免疫的BALB/cBy(Qa-2b)小鼠的脾T细胞,在体外用BALB/cJ脾细胞刺激后产生了CTL。这些CTL能裂解所有Qa-2 +的靶细胞,但不能裂解Qa-2 -的靶细胞,无论靶细胞的H-2单倍型或其非MHC背景如何。使用Qa-2特异性CTL克隆证实了这种对Qa-2抗原明显的MHC I类非限制性识别。发现Qa-2致敏的CTL前体细胞(CTLp)和CTL是CD8 + T细胞。培养前耗尽CD4 + T细胞的致敏脾细胞不能产生CTL,但向培养物中添加淋巴因子可恢复CTL的产生。用经辐照的Qa-2 + T母细胞而不是脾细胞或B母细胞刺激致敏的脾T细胞,导致几乎没有或没有CTL产生,这表明MHC II类分子参与了Qa-2抗原向CD4 + T细胞的呈递。使用源自BALB/c的Qa-2 +、II类胸腺瘤细胞的实验结果也支持了这一点。用丝裂霉素C处理的胸腺瘤细胞刺激胸腺瘤致敏的脾T细胞,未产生抗Qa-2 CTL,尽管用胸腺瘤免疫相应的同种异体宿主可产生高水平的针对次要组织相容性(H)抗原和H-2d的特异性CTL。然而,添加淋巴因子使胸腺瘤致敏的T细胞能够产生抗Qa-2 CTL。从BALB/cJ脾细胞致敏的反应细胞中分离出的CD4 +和CD8 + T细胞群体,在体外用Qa-2 +脾细胞刺激后都发生增殖,这表明免疫小鼠中存在对Qa-2反应性的CD4 + T细胞。用抗L3T4单克隆抗体从胸腺切除的BALB/cBy小鼠中耗尽CD4 + T细胞,可显著降低但不能消除抗Qa-2 CTL的产生。相反,耗尽CD8 + T细胞导致CTL反应完全消除。向耗尽任一T细胞亚群的反应细胞培养物中添加淋巴因子不能恢复其反应性。结论是,抗Qa-2 CTLp在体内需要CD4 + T细胞的“帮助”才能被致敏。此外,致敏的CTLp在体外分化为效应CTL时也需要CD4 + T细胞提供 的“帮助”或淋巴因子。(摘要截断于400字)
