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霍奇金病患者淋巴结中存在抗纤维蛋白溶解的纤维蛋白沉积。

Fibrinolysis resistant fibrin deposits in lymph nodes with Hodgkin's disease.

作者信息

Adány R, Szegedi A, Ablin R J, Muszbek L

机构信息

Department of Clinical Chemistry, University School of Medicine, Debrecen, Hungary.

出版信息

Thromb Haemost. 1988 Oct 31;60(2):293-7.

PMID:3064359
Abstract

Extravasal fibrin deposition is frequently observed within and around tumorous tissues and has been implicated in various aspects of tumor growth. However, no adequate information has been available on the mechanism how intratumoral interstitial fibrin deposits escape a prompt elimination by the fibrinolytic system. In this study we provide immunomorphological evidence showing that fibrin deposits in lymph nodes with Hodgkin's disease are stabilized and made resistant to fibrinolysis by factor XIII (FXIII) of blood coagulation. By double immunofluorescent labelling systems fibrin deposits were simultaneously stained for alpha 2-antiplasmin (alpha 2-AP), the main physiological inhibitor of fibrinolysis and in a number of nodular areas they were also labelled for plasmin(ogen). The detection of alpha 2-antiplasmin-plasmin complex-neoantigen (alpha 2-AP-P-Neo) revealed that alpha 2-AP reacted with plasmin, i.e., alpha 2-AP covalently linked to fibrin indeed inhibited intratumoral fibrinolysis. In addition to fibrin deposits FXIII was also found in cellular elements characterized earlier as tumor associated macrophages. These cells were attached to fibrin strands suggesting that they are involved in the intratumoral fibrin formation and might be a source of fibrin stabilizing factor in the tumor stroma.

摘要

在肿瘤组织内部及其周围经常观察到血管外纤维蛋白沉积,并且其与肿瘤生长的各个方面都有关联。然而,关于肿瘤内间质纤维蛋白沉积物如何逃避纤维蛋白溶解系统的迅速清除这一机制,目前尚无充分的信息。在本研究中,我们提供了免疫形态学证据,表明霍奇金病淋巴结中的纤维蛋白沉积物通过凝血因子 XIII(FXIII)得以稳定,并对纤维蛋白溶解产生抗性。通过双重免疫荧光标记系统,纤维蛋白沉积物同时被染以α2 - 抗纤溶酶(α2 - AP),这是纤维蛋白溶解的主要生理抑制剂,并且在一些结节区域它们还被标记上纤溶酶(原)。α2 - 抗纤溶酶 - 纤溶酶复合物 - 新抗原(α2 - AP - P - Neo)的检测表明,α2 - AP 与纤溶酶发生反应,即与纤维蛋白共价连接的α2 - AP 确实抑制了肿瘤内的纤维蛋白溶解。除了纤维蛋白沉积物外,FXIII 还存在于先前被鉴定为肿瘤相关巨噬细胞的细胞成分中。这些细胞附着于纤维蛋白链上,表明它们参与肿瘤内纤维蛋白的形成,并且可能是肿瘤基质中纤维蛋白稳定因子的来源。

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