Sadegh-Nasseri S, Dessi V, Sercarz E E
Eur J Immunol. 1986 May;16(5):486-92. doi: 10.1002/eji.1830160504.
Immune responsiveness to lysozyme in H-2b mice is under the control of H-2-linked Ir genes, with T suppressor (Ts) cells playing a dominant role in strains such as C57BL/6 (B6), C57BL/10 and A.BY. However, non-H-2-genes were found to be capable of specific reversal of the effect of the H-2-linked genes in responsiveness to chicken lysozyme (HEL), but not to human lysozyme (HUL). Therefore, studies were performed to identify any lesion in the suppressor circuit in BALB.B. It was known that HUL-induced suppressor cells could cross-suppress the anti-HEL response in B10.Q mice, which are responsive to HEL but nonresponsive to HUL. Similarly, BALB.B Ts cells were able to suppress the anti-HEL response, using as T helper (Th) source a T cell line (BB-1), derived from HEL-primed BALB.B periaortic and inguinal lymph node cells. A protocol designed to examine the in vivo suppression by the use of HUL-induced suppressor cells also demonstrated a significant suppression of the anti-HEL response. Since the suppressive circuitry seemed intact in the BALB.B, the possibility was examined that a step in T-B cell collaboration was more efficient in this strain than in the B6 nonresponder. With a B6-derived HEL-specific T cell line, BO1H, the B cell and antigen-presenting (B/APC) populations from B6 required addition of concanavalin A supernatant for anti-HEL antibody formation, whereas BALB.B B/APC were capable of responding to HEL in culture without the addition of concanavalin A supernatant. In agreement with this finding, when B/APC cell populations from BALB.B and B6 were compared for their extent of anti-HEL responsiveness, as measured with BB-1 Th cells, BALB.B B/APC populations responded significantly higher than B6 populations when the responses were activated by picogram/nanogram amounts of HEL. The response level of (BALB.B X B6)F1 B/APC measured in the same assay resembled that of B6. However, when HEL was used at the microgram level, both B6 and BALB.B strains responded equivalently. The above data are consistent with the expression of the reversing non-H-2 Ir gene(s) resulting from the balance of antigen presentation to Th and Ts cells in the H-2b mouse. In the B6, processing and handling of antigen may be inefficient in activating response-enhancing Th, and more effective in triggering Ts cells, while the reverse may be true for the BALB.B.
H-2b小鼠对溶菌酶的免疫反应性受H-2连锁Ir基因的控制,在C57BL/6(B6)、C57BL/10和A.BY等品系中,T抑制(Ts)细胞起主导作用。然而,发现非H-2基因能够特异性逆转H-2连锁基因对鸡溶菌酶(HEL)反应性的影响,但对人溶菌酶(HUL)则不然。因此,进行了研究以确定BALB.B抑制回路中的任何损伤。已知HUL诱导的抑制细胞可以交叉抑制B10.Q小鼠中的抗HEL反应,B10.Q小鼠对HEL有反应但对HUL无反应。同样,BALB.B Ts细胞能够抑制抗HEL反应,使用来自经HEL致敏的BALB.B主动脉周和腹股沟淋巴结细胞的T细胞系(BB-1)作为T辅助(Th)细胞来源。一项旨在通过使用HUL诱导的抑制细胞来检测体内抑制作用的方案也证明了抗HEL反应受到显著抑制。由于BALB.B中的抑制回路似乎完整,因此研究了T-B细胞协作中的一个步骤在该品系中比在B6无反应者中更有效的可能性。使用源自B6的HEL特异性T细胞系BO1H,B6的B细胞和抗原呈递(B/APC)群体形成抗HEL抗体需要添加伴刀豆球蛋白A上清液,而BALB.B B/APC在培养中无需添加伴刀豆球蛋白A上清液就能对HEL作出反应。与此发现一致的是,当比较来自BALB.B和B6的B/APC细胞群体对抗HEL反应性的程度时,用BB-1 Th细胞测量,当反应由皮克/纳克量的HEL激活时,BALB.B B/APC群体的反应明显高于B6群体。在相同测定中测量的(BALB.B×B6)F1 B/APC的反应水平与B6相似。然而,当使用微克水平的HEL时,B6和BALB.B品系的反应相当。上述数据与由H-2b小鼠中抗原呈递给Th和Ts细胞的平衡所导致的逆转非H-2 Ir基因的表达一致。在B6中,抗原的加工和处理在激活增强反应的Th方面可能效率低下,而在触发Ts细胞方面更有效,而对于BALB.B则可能相反。
