抗β2-糖蛋白I和抗磷脂酰丝氨酸/凝血酶原抗体在外周血单核细胞和内皮细胞中具有相似的促血栓作用。

Q1 Medicine Auto-Immunity Highlights Pub Date : 2019-04-06 eCollection Date: 2019-12-01 DOI:10.1186/s13317-019-0113-9
A Cifù, R Domenis, C Pistis, F Curcio, M Fabris
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引用次数: 6

摘要

目的:在常规检测的抗磷脂(aPL)抗体中引入抗磷脂酰丝氨酸/凝血酶原(aPS/PT)抗体可改善抗磷脂综合征(aPS)的实验室诊断性能;然而,其致病机制仍未明确。为了支持临床数据和未来可能纳入的新标准抗体,我们设计了一项头对头的研究,直接比较aPS/PT和抗β2-糖蛋白I (a -β 2gpi)结构域1特异性抗体在体外维持的促凝作用。方法:用脂多糖(LPS)单独或联合从6例APS患者血清中分离的IgG组分刺激供血源性单核细胞和内皮细胞(HUVEC),仅a - β 2gpi或APS /PT抗体阳性。作为对照,细胞用LPS加从献血者中分离的IgG孵育。real-time PCR检测培养4 h后组织因子(TF) mRNA表达。用比色法测定细胞孵育16 h后上清液中一氧化氮(NO)的含量。结果:aPS/PT和a - β 2gpi IgG抗体在单核细胞和HUVEC中均表现出类似的增强lps诱导的TF mRNA表达的能力。与单独LPS相比,我们发现LPS加a - β 2gpi和aPS/PT IgG组分处理的HUVEC中NO水平强烈过量产生。结论:我们的数据支持aPS/PT在aPS患者血栓形成事件发病机制中的重要和独立作用,可能为仅存在aPS/PT IgG抗体的病例的治疗管理增加新的亮点。
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Anti-β2-glycoprotein I and anti-phosphatidylserine/prothrombin antibodies exert similar pro-thrombotic effects in peripheral blood monocytes and endothelial cells.

Purpose: The introduction of the anti-phosphatidylserine/prothrombin (aPS/PT) antibodies among the routinely investigated anti-phospholipid (aPL) antibodies led to an improvement in anti-phospholipid syndrome (APS) laboratory diagnostic performance; however, their pathogenic mechanism is still substantially undefined. To support clinical data and future inclusion as possible new criteria antibodies, we designed a head-to-head study to directly compare the procoagulant effects sustained in vitro by aPS/PT to those sustained by anti-β2-glycoprotein I (aβ2GpI) domain 1-specific antibodies.

Methods: Blood donors-derived monocytes and endothelial cells (HUVEC) were stimulated with lipopolysaccharides (LPS) alone or in combination with the IgG fractions isolated from the serum of six APS patients, positive only for aβ2GpI or for aPS/PT antibodies. As control, cells were incubated with LPS plus the IgG isolated from blood donors. Tissue factor (TF) mRNA expression was measured after four hours incubation by real-time PCR. Nitric oxide (NO) levels were measured in cells supernatant after 16 h incubation by colorimetric assay.

Results: aPS/PT and aβ2GpI IgG antibodies fractions showed comparable ability to enhance LPS-induced TF mRNA expression, either in monocytes and in HUVEC. Compared to LPS alone, we found that NO levels are strongly overproduced in HUVEC treated with LPS plus aβ2GpI and aPS/PT IgG fractions.

Conclusions: Our data support the significant and independent role of aPS/PT in the pathogenesis of the thrombotic events in APS patients, possibly adding new light to the therapeutic management of cases characterized by the sole presence of aPS/PT IgG antibodies.

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