Weber C, Alon R, Moser B, Springer T A
Center for Blood Research, Harvard Medical School, Boston, Massachusetts 02115, USA.
J Cell Biol. 1996 Aug;134(4):1063-73. doi: 10.1083/jcb.134.4.1063.
Leukocyte emigration possibly requires dynamic regulation of integrin adhesiveness for endothelial and extracellular matrix ligands. Adhesion assays on purified vascular cell adhension molecule (VCAM)-1, fibronectin, and fibronectin fragments revealed distinct kinetic patterns for the regulation of very late antigen (VLA)-4 (alpha 4 beta 1) and VLA-5 (alpha 5 beta 1) avidity by the CC chemokines monocyte inflammatory protein (MIP)-1 alpha, RANTES (regulated on activation, normal T expressed and secreted), or monocyte chemoattractant protein (MCP)-1 in monocytes. CC chemokines induced early activation and subsequent deactivation of VLA-4, whereas upregulation of VLA-5 avidity occurred later and persisted. Controlled detachment assays in shear flow suggested that adhesive strength of VLA-4 for VCAM-1 or the 40-kD fragment of fibronectin (FN40) is more rapidly increased and subsequently reduced by MCP-1 than by MIP-1 alpha, and confirmed late and sustained activation of the adhesive strength of VLA-5 for the 120-kD fragment of fibronectin (FN120). Mn2+ or the stimulating beta 1 mAb TS2/16 strongly and stably enhanced monocyte binding to VCAM-1 or fibronectin, and locked beta 1 integrins in a high avidity state, which was not further modulated by CC chemokines. Mn2+ and mAb TS2/16 inhibited CC chemokine-induced transendothelial migration, particularly chemotaxis across stimulated endothelium that involved VLA-4 and VCAM-1. VLA-4 on Jurkat cells is of constitutively high avidity and interfered with migration across barriers expressing VCAM-1. Low but not high site densities of VCAM-1 or FN40 promoted, while FN120 impaired, beta 1 integrin-dependent monocyte chemotaxis to MCP-1 across filters coated with these substrates. Thus, we show that CC chemokines can differentially and selectively regulate avidity of integrins sharing common beta subunits. Transient activation and deactivation of VLA-4 may serve to facilitate transendothelial diapedesis, whereas late and prolonged activation of VLA-5 may mediate subsequent interactions with the basement membrane and extracellular matrix.
白细胞渗出可能需要对整合素与内皮细胞和细胞外基质配体的黏附性进行动态调节。对纯化的血管细胞黏附分子(VCAM)-1、纤连蛋白及纤连蛋白片段进行的黏附试验揭示了CC趋化因子单核细胞炎性蛋白(MIP)-1α、调节激活正常T细胞表达和分泌因子(RANTES)或单核细胞趋化蛋白(MCP)-1对单核细胞中极迟抗原(VLA)-4(α4β1)和VLA-5(α5β1)亲和力调节的不同动力学模式。CC趋化因子诱导VLA-4早期激活及随后的失活,而VLA-5亲和力的上调出现较晚且持续存在。剪切流中的可控脱离试验表明,MCP-1比MIP-1α更快速地增加并随后降低VLA-4对VCAM-1或纤连蛋白40kD片段(FN40)的黏附强度,并证实了VLA-5对纤连蛋白120kD片段(FN120)黏附强度的晚期和持续激活。Mn2+或刺激性β1单克隆抗体TS2/16强烈且稳定地增强单核细胞与VCAM-1或纤连蛋白的结合,并将β1整合素锁定在高亲和力状态,而CC趋化因子不会对其进行进一步调节。Mn2+和单克隆抗体TS2/16抑制CC趋化因子诱导的跨内皮迁移,尤其是涉及VLA-4和VCAM-1的跨刺激内皮细胞的趋化作用。Jurkat细胞上的VLA-4具有组成性高亲和力,并干扰跨表达VCAM-1屏障的迁移。低而非高位点密度的VCAM-1或FN40促进,而FN120损害β1整合素依赖性单核细胞对MCP-1穿过包被这些底物的滤膜时的趋化作用。因此,我们表明CC趋化因子可以差异性和选择性地调节共享共同β亚基的整合素的亲和力。VLA-4的短暂激活和失活可能有助于促进跨内皮细胞渗出,而VLA-5的晚期和延长激活可能介导随后与基底膜和细胞外基质的相互作用。
