Dransfield I, Cabañas C, Craig A, Hogg N
Macrophage Laboratory, Imperial Cancer Research Fund, London, England.
J Cell Biol. 1992 Jan;116(1):219-26. doi: 10.1083/jcb.116.1.219.
The integrin lymphocyte function-associated antigen-1 (LFA-1) expressed on T cells serves as a useful model for analysis of leukocyte integrin functional activity. We have assessed the role of divalent cations Mg2+, Ca2+, and Mn2+ in LFA-1 binding to ligand intercellular adhesion molecule-1 (ICAM-1) and induction of the divalent cation-dependent epitope recognized by mAb 24. Manganese strongly promoted both expression of the 24 epitope and T cell binding to ICAM-1 via LFA-1, suggesting that Mn2+ is able to directly alter the conformation of LFA-1 in a manner that favors ligand binding. Since Mn2+ also promotes functional activity of other integrins, parallels in mechanism of ligand binding may span the integrin family. In contrast, induction of 24 epitope expression by Mg2+ required removal of Ca2+ from T cell LFA-1 with EGTA. Furthermore, binding of mAb 24 to T cell LFA-1 in the presence of either Mn2+ or Mg2+ was found to be specifically inhibited by Ca2+, suggestive of a negative regulatory role for Ca2+ in the control of leukocyte integrin function. Analysis of T cell binding to ICAM-1 via LFA-1 in the presence of Mg2+ or Mn2+, confirmed that Ca2+ exerted inhibitory effects upon LFA-1 function. The implication of our findings is that Ca2+ bound with relatively high affinity to LFA-1 may serve to maintain an inactive state. Thus induction of function and 24 epitope expression may occur as a result of displacement of Ca2+ from leukocyte integrins or alternatively, such activators may be able to impose the required conformational change in the presence of bound Ca2+.
T 细胞上表达的整合素淋巴细胞功能相关抗原-1(LFA-1)是分析白细胞整合素功能活性的有用模型。我们评估了二价阳离子 Mg2+、Ca2+ 和 Mn2+ 在 LFA-1 与配体细胞间黏附分子-1(ICAM-1)结合以及诱导单克隆抗体 24 识别的二价阳离子依赖性表位中的作用。锰强烈促进 24 表位的表达以及 T 细胞通过 LFA-1 与 ICAM-1 的结合,这表明 Mn2+ 能够以有利于配体结合的方式直接改变 LFA-1 的构象。由于 Mn2+ 也促进其他整合素的功能活性,配体结合机制的相似性可能贯穿整合素家族。相比之下,Mg2+ 诱导 24 表位表达需要用乙二醇双四乙酸(EGTA)从 T 细胞 LFA-1 中去除 Ca2+。此外,发现在存在 Mn2+ 或 Mg2+ 的情况下,单克隆抗体 24 与 T 细胞 LFA-1 的结合被 Ca2+ 特异性抑制,提示 Ca2+ 在白细胞整合素功能控制中起负调节作用。在存在 Mg2+ 或 Mn2+ 的情况下分析 T 细胞通过 LFA-1 与 ICAM-1 的结合,证实 Ca2+ 对 LFA-1 功能发挥抑制作用。我们研究结果的意义在于,以相对高亲和力与 LFA-1 结合的 Ca2+ 可能用于维持非活性状态。因此,功能诱导和 24 表位表达可能是由于 Ca2+ 从白细胞整合素中被置换所致,或者,此类激活剂可能能够在结合 Ca2+ 的情况下引发所需的构象变化。