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内皮细胞膜联蛋白A2调节其结合伴侣S100A10/p11的多聚泛素化和降解。

Endothelial cell annexin A2 regulates polyubiquitination and degradation of its binding partner S100A10/p11.

作者信息

He Kai-Li, Deora Arunkumar B, Xiong Huabao, Ling Qi, Weksler Babette B, Niesvizky Ruben, Hajjar Katherine A

机构信息

Department of Cell and Developmental Biology, Weill Cornell Medical College, New York, New York 10065, USA.

出版信息

J Biol Chem. 2008 Jul 11;283(28):19192-200. doi: 10.1074/jbc.M800100200. Epub 2008 Apr 23.

Abstract

The annexin A2 (A2) heterotetramer, consisting of two copies of A2 and two copies of S100A10/p11, promotes fibrinolytic activity on the surface of vascular endothelial cells by assembling plasminogen and tissue plasminogen activator (tPA) and accelerating the generation of plasmin. In humans, overexpression of A2 by acute promyelocytic leukemia cells is associated with excessive fibrinolysis and hemorrhage, whereas anti-A2 autoantibodies appear to accentuate the risk of thrombosis in patients with anti-phospholipid syndrome. Complete deficiency of A2 in mice leads to a lack of tPA cofactor activity, accumulation of intravascular fibrin, and failure to clear arterial thrombi. Within the endothelial cell, p11 is required for Src kinase-mediated tyrosine phosphorylation of A2, which signals translocation of both proteins to the cell surface. Here we show that p11 is expressed at very low levels in the absence of A2 both in vitro and in vivo. We demonstrate further that unpartnered p11 becomes polyubiquitinated and degraded via a proteasome-dependent mechanism. A2 stabilizes intracellular p11 through direct binding, thus masking an autonomous p11 polyubiquitination signal that triggers proteasomal degradation. This interaction requires both the p11-binding N-terminal domain of A2 and the C-terminal domain of p11. This mechanism prevents accumulation of free p11 in the endothelial cell and suggests that regulation of tPA-dependent cell surface fibrinolytic activity is precisely tuned to the intracellular level of p11.

摘要

膜联蛋白A2(A2)异源四聚体由两个A2拷贝和两个S100A10/p11拷贝组成,通过组装纤溶酶原和组织纤溶酶原激活物(tPA)并加速纤溶酶的生成,促进血管内皮细胞表面的纤溶活性。在人类中,急性早幼粒细胞白血病细胞过度表达A2与过度纤溶和出血有关,而抗A2自身抗体似乎会增加抗磷脂综合征患者的血栓形成风险。小鼠体内A2完全缺乏会导致tPA辅因子活性缺失、血管内纤维蛋白积累以及无法清除动脉血栓。在内皮细胞中,p11是Src激酶介导的A2酪氨酸磷酸化所必需的,这一磷酸化促使两种蛋白转位至细胞表面。在此,我们发现无论在体外还是体内,在缺乏A2的情况下p11的表达水平都非常低。我们进一步证明,未与A2结合的p11会通过蛋白酶体依赖性机制发生多聚泛素化并降解。A2通过直接结合使细胞内的p11稳定,从而掩盖了触发蛋白酶体降解的p11自主多聚泛素化信号。这种相互作用需要A2的p11结合N末端结构域和p11的C末端结构域。该机制可防止内皮细胞中游离p11的积累,并表明tPA依赖性细胞表面纤溶活性的调节与细胞内p11水平精确匹配。

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