Kappert Kai, Meyborg Heike, Baumann Bernadette, Furundzija Vesna, Kaufmann Jan, Graf Kristof, Stibenz Dietger, Fleck Eckart, Stawowy Philipp
Department of Medicine/Cardiology, Deutsches Herzzentrum Berlin, Augustenburger Platz 1, Berlin, Germany.
Int J Biochem Cell Biol. 2009 Jul;41(7):1511-7. doi: 10.1016/j.biocel.2009.01.004. Epub 2009 Jan 8.
Vascular smooth muscle cell (VSMC) invasion is a key element in atherogenesis and restenosis, requiring integrins for adhesion/de-adhesion as well as matrix metalloproteinases (MMPs) for focalized proteolysis. Among the MMP family, pro-MMP-2 is unique in its activation, depending on the formation of a multiprotein complex with MT1-MMP/TIMP-2 at the cell surface, in which integrin alphavbeta3 participates. Integrin alphav and MT1-MMP are synthesized from precursors via furin-dependent cleavage of their pro-peptide. Furin is the prototypical proprotein convertase highly expressed in VSMCs and human atherosclerotic lesions. Its precise role in the tight network involving MMPs/integrins and their coordination and cooperation required for VSMC invasion is unknown. We demonstrate that furin-inhibition with decanoyl-RVKR-chloromethylketone inhibits VSMC invasion in a comparable degree to MMP inhibitors, which reduce the MT1-MMP-MMP-2 proteolytic cascade. Furin-inhibition did not prevent MT1-MMP/MMP-2 maturation. In contrast, it strongly reduced pro-alphav cleavage, but did not lessen its cell membrane expression. However, inhibition of pro-alphav processing via furin-inhibition strongly reduced pro-MMP-2 binding to the cell surface, thereby lessening its full maturation and diminishing the cell surface in situ proteolysis required for invasion. Thus, our data demonstrate a novel mechanism of furin-dependent alphav cleavage that enhances pro-MMP-2 binding and activation at the cell membrane in cooperation with MT1-MMP in primary VSMCs. Processing of alphav by furin contributes to the recruitment of enzymatic energy to the cell surface, thereby providing focalized proteolysis associated with VSMC invasion.
血管平滑肌细胞(VSMC)的侵袭是动脉粥样硬化和再狭窄的关键因素,这一过程需要整合素进行黏附/去黏附,以及基质金属蛋白酶(MMPs)进行局部蛋白水解。在MMP家族中,前MMP-2的激活方式独特,它依赖于在细胞表面与MT1-MMP/TIMP-2形成多蛋白复合物,整合素αvβ3也参与其中。整合素αv和MT1-MMP是通过弗林蛋白酶对其前体肽的切割从前体合成的。弗林蛋白酶是在VSMC和人类动脉粥样硬化病变中高度表达的典型前体蛋白转化酶。其在涉及MMPs/整合素及其协调合作的紧密网络中,对于VSMC侵袭所起的确切作用尚不清楚。我们证明,用癸酰-RVKR-氯甲基酮抑制弗林蛋白酶,对VSMC侵袭的抑制程度与MMP抑制剂相当,MMP抑制剂可减少MT1-MMP-MMP-2蛋白水解级联反应。抑制弗林蛋白酶并不能阻止MT1-MMP/MMP-2的成熟。相反,它强烈降低了前αv的切割,但并未减少其细胞膜表达。然而,通过抑制弗林蛋白酶来抑制前αv的加工,会强烈减少前MMP-2与细胞表面的结合,从而减少其完全成熟,并减少侵袭所需的细胞表面原位蛋白水解。因此,我们的数据证明了一种新的弗林蛋白酶依赖性αv切割机制,该机制与原代VSMC中的MT1-MMP协同作用,增强前MMP-2在细胞膜上的结合和激活。弗林蛋白酶对αv的加工有助于将酶促能量募集到细胞表面,从而提供与VSMC侵袭相关的局部蛋白水解。
