Endothelial fibrinolytic response onto an evolving matrix of fibrin.

Q2 Medicine BMC Hematology Pub Date : 2016-04-14 eCollection Date: 2016-01-01 DOI:10.1186/s12878-016-0048-6
O Castillo, H Rojas, Z Domínguez, E Anglés-Cano, R Marchi
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引用次数: 5

Abstract

Background: Fibrin provides a temporary matrix at the site of vascular injury. The aims of the present work were (1) to follow fibrin formation and lysis onto the surface of human dermal microvascular endothelial cells (HMEC-1), and (2) to quantify the secretion of fibrinolytic components in the presence of fibrin.

Methods: Fibrin clots at different fibrinogen concentrations were formed on top of (model 1) or beneath (model 2) the endothelial cells. Fibrin formation or lysis onto the surface of HMEC-1 cells, was followed by turbidity. Clot structure was visualized by laser scanning confocal microscopy (LSCM). The secretion of uPA and PAI-1 by HMEC-1 cells was quantified by ELISA.

Results: The rate of fibrin formation increased approximately 1.5-fold at low fibrinogen content (0.5 and 1 mg/mL; p < 0.05) compared to the condition without cells; however, it was decreased at 2 mg/mL fibrinogen (p < 0.05) and no differences were found at higher fibrinogen concentrations (3 and 5 mg/mL). HMEC-1 retarded dissolution of clots formed onto their surface at 0.5 to 3 mg/mL fibrinogen (p < 0.05). Secretion of uPA was 13 × 10(-6) ng/mL per cell in the absence of RGD and 8 × 10(-6) ng/mL per cell in the presence of RGD, when clots were formed on the top of HMEC-1. However, the opposite was found when cells were grown over fibrin: 6 × 10(-6) ng/mL per cell without RGD vs. 17 × 10(-6) ng/mL per cell with RGD. The secretion of PAI-1 by HMEC-1 cells was unrelated to the presence of fibrin or RGD, 7 × 10(-6) μg/mL per cell and 5 × 10(-6) μg/mL per cell, for the apical (model 1) and basal clots (model 2), respectively.

Conclusions: HMEC-1 cells influence fibrin formation and dissolution as a function of the fibrin content of clots. Clot degradation was accentuated at high fibrin concentrations. The secretion of fibrinolytic components by HMEC-1 cells seemed to be modulated by integrins that bind RGD ligands.

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内皮纤维蛋白溶解反应对纤维蛋白基质的进化。
背景:纤维蛋白在血管损伤部位提供临时基质。本研究的目的是:(1)跟踪纤维蛋白在人皮肤微血管内皮细胞(HMEC-1)表面的形成和裂解,(2)量化纤维蛋白存在时纤维蛋白溶解成分的分泌。方法:不同纤维蛋白原浓度的纤维蛋白凝块形成于内皮细胞的顶部(模型1)或下方(模型2)。纤维蛋白形成或溶解到HMEC-1细胞表面,然后混浊。用激光扫描共聚焦显微镜(LSCM)观察血块结构。ELISA法测定HMEC-1细胞分泌uPA和PAI-1的水平。结果:低纤维蛋白原含量(0.5和1 mg/mL)时,纤维蛋白形成率提高约1.5倍;p结论:HMEC-1细胞影响凝块纤维蛋白含量的纤维蛋白形成和溶解。在高纤维蛋白浓度下,凝块降解加剧。HMEC-1细胞分泌的纤溶成分似乎受到结合RGD配体的整合素的调节。
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来源期刊
BMC Hematology
BMC Hematology Medicine-Hematology
CiteScore
4.10
自引率
0.00%
发文量
0
期刊介绍: BMC Hematology is an open access, peer-reviewed journal that considers articles on basic, experimental and clinical research related to hematology. The journal welcomes submissions on non-malignant and malignant hematological diseases, hemostasis and thrombosis, hematopoiesis, stem cells and transplantation.
期刊最新文献
Correction to: Rapid and reliable detection of α-globin copy number variations by quantitative real-time PCR Correction to: Patterns of bone marrow aspiration confirmed hematological malignancies in Eritrean National Health Laboratory. Correction to: The impact of helicobacter pylori eradication on platelet counts of adult patients with idiopathic thrombocytopenic purpura. Assessment of knowledge, attitude and practice and associated factors of blood donation among health care workers in Ethiopia: a cross-sectional study. Health-related quality of life of adolescents with sickle cell disease in sub-Saharan Africa: a cross-sectional study.
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