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细胞周围基质金属蛋白酶组织蛋白酶 G 和组织蛋白酶 H 通过跨膜丝氨酸蛋白酶激活肝细胞生长因子,但膜相关蛋白酶 uPA 则不能。

Pericellular activation of hepatocyte growth factor by the transmembrane serine proteases matriptase and hepsin, but not by the membrane-associated protease uPA.

机构信息

Biomedical Research Centre, School of Biological Sciences, University of East Anglia, Norwich NR4 7TJ, U.K.

出版信息

Biochem J. 2010 Feb 9;426(2):219-28. doi: 10.1042/BJ20091448.

DOI:10.1042/BJ20091448
PMID:20015050
Abstract

HGF (hepatocyte growth factor) is a pleiotropic cytokine homologous to the serine protease zymogen plasminogen that requires canonical proteolytic cleavage to gain functional activity. The activating proteases are key components of its regulation, but controversy surrounds their identity. Using quantitative analysis we found no evidence for activation by uPA (urokinase plasminogen activator), despite reports that this is a principal activator of pro-HGF. This was unaffected by a wide range of experimental conditions, including the use of various molecular forms of both HGF and uPA, and the presence of uPAR (uPA receptor) or heparin. In contrast the catalytic domains of the TTSPs (type-II transmembrane serine proteases) matriptase and hepsin were highly efficient activators (50% activation at 0.1 and 3.4 nM respectively), at least four orders of magnitude more efficient than uPA. PS-SCL (positional-scanning synthetic combinatorial peptide libraries) were used to identify consensus sequences for the TTSPs, which in the case of hepsin corresponded to the pro-HGF activation sequence, demonstrating a high specificity for this reaction. Both TTSPs were also found to be efficient activators at the cell surface. Activation of pro-HGF by PC3 prostate carcinoma cells was abolished by both protease inhibition and matriptase-targeting siRNA (small interfering RNA), and scattering of MDCK (Madin-Darby canine kidney) cells in the presence of pro-HGF was abolished by inhibition of matriptase. Hepsin-transfected HEK (human embryonic kidney)-293 cells also activated pro-HGF. These observations demonstrate that, in contrast with the uPA/uPAR system, the TTSPs matriptase and hepsin are direct pericellular activators of pro-HGF, and that together these proteins may form a pathway contributing to their involvement in pathological situations, including cancer.

摘要

HGF(肝细胞生长因子)是一种与丝氨酸蛋白酶原尿激酶纤溶酶原同源的多效细胞因子,需要经典的蛋白水解切割才能获得功能活性。激活蛋白酶是其调节的关键组成部分,但它们的身份存在争议。使用定量分析,我们没有发现证据表明 uPA(尿激酶纤溶酶原激活物)可以激活它,尽管有报道称 uPA 是 pro-HGF 的主要激活剂。这不受广泛的实验条件的影响,包括使用各种 HGF 和 uPA 的分子形式,以及 uPAR(uPA 受体)或肝素的存在。相比之下,TTSPs(II 型跨膜丝氨酸蛋白酶)matriptase 和 hepsin 的催化结构域是非常有效的激活剂(分别在 0.1 和 3.4 nM 时达到 50%的激活),至少比 uPA 高效四个数量级。使用 PS-SCL(位置扫描合成组合肽文库)来鉴定 TTSP 的共有序列,对于 hepsin 来说,它对应于 pro-HGF 的激活序列,证明了对该反应的高特异性。在细胞表面,两种 TTSP 也被发现是有效的激活剂。PC3 前列腺癌细胞中 pro-HGF 的激活被蛋白酶抑制和 matriptase 靶向 siRNA(小干扰 RNA)所阻断,而 pro-HGF 存在时 MDCK(Madin-Darby 犬肾)细胞的散射被 matriptase 抑制所阻断。转染了 hepsin 的 HEK(人胚肾)-293 细胞也可以激活 pro-HGF。这些观察结果表明,与 uPA/uPAR 系统相反,TTSPs matriptase 和 hepsin 是 pro-HGF 的直接细胞周激活剂,这些蛋白可能共同形成一条途径,有助于它们参与包括癌症在内的病理情况。

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