Welsh John D, Muthard Ryan W, Stalker Timothy J, Taliaferro Joshua P, Diamond Scott L, Brass Lawrence F
Department of Medicine and Department of Chemical and Biomolecular Engineering, University of Pennsylvania, Philadelphia, PA.
Department of Chemical and Biomolecular Engineering, University of Pennsylvania, Philadelphia, PA.
Blood. 2016 Mar 24;127(12):1598-605. doi: 10.1182/blood-2015-09-672188. Epub 2016 Jan 6.
Previous studies have shown that hemostatic thrombi formed in response to penetrating injuries have a core of densely packed, fibrin-associated platelets overlaid by a shell of less-activated, loosely packed platelets. Here we asked, first, how the diverse elements of this structure combine to stem the loss of plasma-borne molecules and, second, whether antiplatelet agents and anticoagulants that perturb thrombus structure affect the re-establishment of a tight vascular seal. The studies combined high-resolution intravital microscopy with a photo-activatable fluorescent albumin marker to simultaneously track thrombus formation and protein transport following injuries to mouse cremaster muscle venules. The results show that protein loss persists after red cell loss has ceased. Blocking platelet deposition with an αIIbβ3antagonist delays vessel sealing and increases extravascular protein accumulation, as does either inhibiting adenosine 5'-diphosphate (ADP) P2Y12receptors or reducing integrin-dependent signaling and retraction. In contrast, sealing was unaffected by introducing hirudin to block fibrin accumulation or a Gi2α gain-of-function mutation to expand the thrombus shell. Collectively, these observations describe a novel approach for studying vessel sealing after injury in real time in vivo and show that (1) the core/shell architecture previously observed in arterioles also occurs in venules, (2) plasma leakage persists well beyond red cell escape and mature thrombus formation, (3) the most critical events for limiting plasma extravasation are the stable accumulation of platelets, ADP-dependent signaling, and the emergence of a densely packed core, not the accumulation of fibrin, and (4) drugs that affect platelet accumulation and packing can delay vessel sealing, permitting protein escape to continue.
先前的研究表明,针对穿透性损伤形成的止血血栓具有一个核心,该核心由紧密堆积的、与纤维蛋白相关的血小板组成,其上方覆盖着一层活化程度较低、松散堆积的血小板外壳。在此,我们首先探究了这种结构的不同组成部分如何共同作用以阻止血浆中分子的流失,其次探究了扰乱血栓结构的抗血小板药物和抗凝剂是否会影响紧密血管密封的重新建立。这些研究将高分辨率活体显微镜检查与可光激活的荧光白蛋白标记物相结合,以在小鼠提睾肌小静脉损伤后同时追踪血栓形成和蛋白质运输。结果表明,在红细胞流失停止后,蛋白质流失仍会持续。用αIIbβ3拮抗剂阻断血小板沉积会延迟血管密封并增加血管外蛋白质的积累,抑制腺苷5'-二磷酸(ADP)P2Y12受体或减少整合素依赖性信号传导及收缩也会如此。相比之下,引入水蛭素以阻断纤维蛋白积累或引入Gi2α功能获得性突变以扩大血栓外壳对密封没有影响。总体而言,这些观察结果描述了一种在体内实时研究损伤后血管密封的新方法,并表明:(1)先前在小动脉中观察到的核心/外壳结构在小静脉中也会出现;(2)血浆渗漏在红细胞逸出和成熟血栓形成之后仍会持续很长时间;(3)限制血浆外渗的最关键事件是血小板的稳定积累、ADP依赖性信号传导以及紧密堆积核心的出现,而非纤维蛋白的积累;(4)影响血小板积累和堆积的药物会延迟血管密封,使蛋白质继续逸出。