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一种用于测量人体液中总α-抗胰蛋白酶水平的新 ELISA 方法。

A new ELISA method for the measurement of total α-plasmin inhibitor level in human body fluids.

机构信息

Division of Clinical Laboratory Science, Department of Laboratory Medicine, Faculty of Medicine, University of Debrecen, 98. Nagyerdei krt., Debrecen H-4032, Hungary.

Borsod-Abaúj-Zemplén County Hospital and University Teaching Hospital, Miskolc, Hungary.

出版信息

J Immunol Methods. 2019 Aug;471:27-33. doi: 10.1016/j.jim.2019.05.004. Epub 2019 May 24.

Abstract

The ever-increasing research efforts to develop new antithrombotic therapies have led to the reassessment of the role of alpha-2-plasmin inhibitor (α-PI) in pathological conditions. In particular, experimental stroke studies have suggested correlation between increased free α2-PI level and mortality. However there are only a small number of well-characterized and specific assays available for the measurements of free α-PI. In plasma α-PI undergoes both N- and/or C-terminal cleavages resulting four isoforms with modified susceptibility to FXIII catalyzed cross-linking to fibrin and/or loss of plasmin(ogen) binding. Present paper describes a new sandwich ELISA method for the determination of free total α-PI in plasma and other body fluids. A newly generated biotinylated monoclonal antibody recognizes and captures all the four N- and/or C-terminally modified isoforms of α-PI while HRPO-labeled polyclonal anti-α-PI antibody detects the captured antigen. Performing the 2-step assay in streptavidin-coated microplate can be completed within three hours. The assay is well reproducible, total (within laboratory) imprecision in the normal, pathological and very low ranges were 7.4%, 9.1% and < 19%, respectively. When examining the plasma samples of 197 healthy volunteers, 100 acute ischemic stroke patients and 102 patients with venous thrombosis, strong correlation was observed between total α2-PI antigen levels and α2-PI activity for each group. Using the assay a reference interval of 45-86 mg/L was established for total α-PI mass concentration in the plasma. α-PI levels were also measured in cerebrospinal fluid samples of 47 individuals the median value and range was 132 (36-379) μg/L. In conclusion, our ELISA enables accurate and fast measurement of total free α-PI in human body fluids.

摘要

为了开发新的抗血栓疗法,人们进行了越来越多的研究,这导致了对 α-2-纤溶酶抑制剂 (α-PI) 在病理情况下的作用的重新评估。特别是,实验性中风研究表明,游离 α2-PI 水平升高与死亡率之间存在相关性。然而,目前只有少数经过良好特征描述和特异性检测的方法可用于测量游离 α-PI。在血浆中,α-PI 会经历 N-和/或 C-末端的裂解,从而产生四种具有不同纤维蛋白 XIII 催化交联和/或纤溶酶原结合能力的同工型。本文描述了一种用于测定血浆和其他体液中游离总 α-PI 的新的夹心 ELISA 方法。新生成的生物素化单克隆抗体识别并捕获所有四种 N-和/或 C-末端修饰的 α-PI 同工型,而 HRPO 标记的多克隆抗-α-PI 抗体则检测捕获的抗原。在链霉亲和素包被的微孔板中进行 2 步检测,可在 3 小时内完成。该检测方法具有良好的可重复性,正常、病理和极低范围内的总(实验室内部)精密度分别为 7.4%、9.1%和<19%。在检查 197 名健康志愿者、100 名急性缺血性中风患者和 102 名静脉血栓形成患者的血浆样本时,观察到各组中总 α2-PI 抗原水平与 α2-PI 活性之间存在强相关性。使用该检测方法,建立了血浆中总 α-PI 质量浓度的参考区间为 45-86mg/L。还测量了 47 名个体的脑脊液样本中的 α-PI 水平,中位数和范围为 132(36-379)μg/L。总之,我们的 ELISA 能够准确、快速地测量人体体液中的总游离 α-PI。

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