Kost C, Stüber W, Ehrlich H J, Pannekoek H, Preissner K T
Haemostasis Research Unit, Kerckhoff-Klinik, Max-Planck-Gesellschaft, Bad Nauheim, Germany.
J Biol Chem. 1992 Jun 15;267(17):12098-105.
Vitronectin (VN) has been implicated as a major matrix-associated regulator component of plasminogen activation by serving as a potent stabilizing cofactor of plasminogen activator inhibitor-1 (PAI-1). The direct binding of heparin, plasminogen as well as PAI-1 in its latent and active form to immobilized VN was studied in the absence or presence of competitors. Monoclonal antibodies against the carboxyl-terminal portion of VN inhibited both PAI-1 and plasminogen binding, whereas heparin, heparan sulfate with a high degree of sulfation, or dextran sulfate interfered with PAI-1 binding (KD = 20 nM) only. Utilizing synthetic peptides encompassing overlapping sequences of the heparin-binding domain of VN, adjacent heparin and PAI-1-binding sites were localized within the sequence 348-370 of VN. Although a number of other serine protease inhibitors which do not form binary complexes with VN contain a reactive-site Ser at their P1'-position, a reactive-site P1' mutant of PAI-1 (Met----Ser) showed comparable if not increased binding to VN. Binding of Lys-plasminogen and active-site-blocked plasmin was at least 10-fold higher in affinity (KD = 85-100 nM) compared to Glu-plasminogen (KD approximately 1 microM) and could be inhibited by lysine analogs but not by glycosaminoglycans or PAI-1, indicating that heteropolar plasmin(ogen) binding of VN occurs to an adjacent segment upstream to the heparin and PAI-1-binding sites. This contention was further supported in binding studies with plasmin-modified VN which lost both heparin and PAI-1 binding but exhibited 2-3-fold higher capacity to bind plasminogen. The essential plasmin(ogen)-binding site was mapped by ligand blot analysis to the carboxyl-terminal portion of proteolytically trimmed VN (M(r) = 61,000). Moreover, treatment of the extracellular matrix of human umbilical vein endothelial cells with plasmin resulted in partial degradation of matrix-associated VN and concomitant release of PAI-1, but increased the ability of the matrix by about 2-fold to bind plasminogen. These results are indicative of differential interactions of VN with components of the plasminogen activation system, whereby plasmin itself may provoke the switch of VN from an anti-fibrinolytic into a pro-fibrinolytic cofactor. This process reflects a novel role for the adhesive protein and its degradation product(s) in the possible feedback regulation of localized plasmin formation at extracellular sites.
玻连蛋白(VN)作为纤溶酶原激活物抑制剂-1(PAI-1)的一种强效稳定辅因子,被认为是纤溶酶原激活的主要基质相关调节成分。在有无竞争者存在的情况下,研究了肝素、纤溶酶原以及潜伏和活性形式的PAI-1与固定化VN的直接结合。针对VN羧基末端部分的单克隆抗体抑制了PAI-1和纤溶酶原的结合,而肝素、高度硫酸化的硫酸乙酰肝素或硫酸葡聚糖仅干扰PAI-1的结合(解离常数KD = 20 nM)。利用包含VN肝素结合域重叠序列的合成肽,相邻的肝素和PAI-1结合位点定位于VN的348 - 370序列内。尽管许多其他不与VN形成二元复合物的丝氨酸蛋白酶抑制剂在其P1'位置含有反应位点Ser,但PAI-1的反应位点P1'突变体(Met→Ser)与VN的结合即使没有增加也相当。与谷氨酸纤溶酶原(KD约为1 μM)相比,赖氨酸纤溶酶原和活性位点被阻断的纤溶酶的结合亲和力至少高10倍(KD = 85 - 100 nM),并且可被赖氨酸类似物抑制,但不能被糖胺聚糖或PAI-1抑制,这表明VN的异极纤溶酶(原)结合发生在肝素和PAI-1结合位点上游的相邻片段。用纤溶酶修饰的VN进行的结合研究进一步支持了这一观点,该修饰后的VN失去了肝素和PAI-1结合,但结合纤溶酶原的能力提高了2 - 3倍。通过配体印迹分析将必需的纤溶酶(原)结合位点定位到蛋白水解切割后的VN(分子量Mr = 61,000)的羧基末端部分。此外,用纤溶酶处理人脐静脉内皮细胞的细胞外基质导致基质相关VN部分降解并伴随PAI-1释放,但使基质结合纤溶酶原的能力提高了约2倍。这些结果表明VN与纤溶酶原激活系统各成分之间存在差异相互作用,由此纤溶酶本身可能促使VN从抗纤溶转变为促纤溶辅因子。这一过程反映了这种粘附蛋白及其降解产物在细胞外位点局部纤溶酶形成的可能反馈调节中的新作用。
