白细胞介素1（IL-1）对人大型颗粒淋巴细胞系中IL-1受体表达的下调作用及内化的125I标记IL-1β的去向

Down-regulation of interleukin 1 (IL 1) receptor expression by IL 1 and fate of internalized 125I-labeled IL 1 beta in a human large granular lymphocyte cell line.

作者信息

Matsushima K, Yodoi J, Tagaya Y, Oppenheim J J

出版信息

J Immunol. 1986 Nov 15;137(10):3183-8.

Abstract

The regulation of interleukin 1 (IL 1) receptor expression on a human large granular lymphocyte cell line, YT, and fate of internalized 125I-labeled IL 1 beta (125I-IL 1 beta) were studied. YT cells were selected for this study, because this cell line expresses a large number of specific high-affinity receptor for IL 1, responds biologically to exogenously added IL 1 by expressing high-affinity IL 2 receptors, and does not produce IL 1. YT cells constitutively express approximately 7 X 10(3) IL 1 receptors/cell with a Kd approximately 10(-10) M. Neither IL 2, phorbol myristic acid, nor lipopolysaccharide affected the total binding of 125I-IL 1 beta by YT cells. In contrast, the capacity of YT cells to bind 125I-IL 1 beta when incubated at 37 degrees C for 3 to 16 hr with a low dose of purified IL 1 beta (approximately 6 U/ml) was reduced by greater than 80%. The loss of binding capability gradually recovered by 16 hr after removal of IL 1 beta from cultured YT cells. The apparent loss of IL 1 receptor expression was accompanied by the internalization of 125I-IL 1 beta into cells. Acid treatment of YT cells to remove bound 125I-IL 1 beta at 4 degrees C showed that 50% of the 125I-IL 1 beta bound to cells could no longer be recovered after 30 min at 37 degrees C, and this increased to 80% after 3 hr at 37 degrees C. Fractionation of cell extracts on Percoll gradient additionally showed 125I-IL 1 beta to appear intracellularly after receptor binding on plasma membranes, and to be successively transferred to some membranous organelles (d approximately equal to 1.037) through an intermediate density organelle (d approximately equal to 1.050), and to finally end up in lysosomal cell fractions (d approximately equal to 1.05 to 1.08) after approximately 3 hr at 37 degrees C. Only approximately 5% of internalized 125I-IL 1 beta was released into culture media by 6 hr of incubation at 37 degrees C. However, the radioactivity in the TCA soluble fraction of the culture media increased gradually by 6 hr and a lysosomotropic enzyme, ethylamine, significantly inhibited both the transfer of internalized 125I-IL 1 beta to the lysosomal fraction and the degradation of 125I-IL 1 beta. This study represents the first evidence of autoregulation of IL 1 receptors by IL 1 and internalization of IL 1 molecules after binding to receptors.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

研究了白细胞介素1（IL-1）受体在人大型颗粒淋巴细胞系YT上的表达调控以及内化的125I标记的IL-1β（125I-IL-1β）的命运。选择YT细胞进行本研究，因为该细胞系表达大量特异性高亲和力的IL-1受体，对外源添加的IL-1有生物学反应，通过表达高亲和力的IL-2受体作出反应，且不产生IL-1。YT细胞组成性地表达约7×10³个IL-1受体/细胞，解离常数约为10⁻¹⁰M。IL-2、佛波醇肉豆蔻酸酯和脂多糖均不影响YT细胞对125I-IL-1β的总结合。相反，当用低剂量的纯化IL-1β（约6U/ml）在37℃孵育3至16小时时，YT细胞结合125I-IL-1β的能力降低了80%以上。从培养的YT细胞中去除IL-1β后，结合能力的丧失在16小时后逐渐恢复。IL-1受体表达的明显丧失伴随着125I-IL-1β内化进入细胞。在4℃对YT细胞进行酸处理以去除结合的125I-IL-1β，结果显示，与细胞结合的125I-IL-1β在37℃孵育30分钟后有50%无法再回收，在37℃孵育3小时后这一比例增加到80%。在Percoll梯度上对细胞提取物进行分级分离还显示，125I-IL-1β在质膜上与受体结合后出现在细胞内，并通过一个中等密度的细胞器（密度约为1.050）依次转移到一些膜性细胞器（密度约为1.037），并在37℃孵育约3小时后最终进入溶酶体细胞组分（密度约为1.05至1.08）。在37℃孵育6小时后，只有约5%内化的125I-IL-1β释放到培养基中。然而，培养基中三氯乙酸可溶性部分的放射性在6小时内逐渐增加，一种溶酶体促酶乙胺显著抑制内化的125I-IL-1β向溶酶体组分的转移以及125I-IL-1β的降解。本研究首次证明了IL-1对IL-1受体的自身调节以及IL-1分子与受体结合后的内化。（摘要截短于400字）