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首页> 外文期刊>Journal of immunoassay >Development of a peptide-based sandwich ELISA for human tissue prokallikrein with no cross-reactivity from mature kallikrein.
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Development of a peptide-based sandwich ELISA for human tissue prokallikrein with no cross-reactivity from mature kallikrein.

机译:针对人组织原激肽释放酶的基于肽的夹心ELISA的开发,与成熟激肽释放酶没有交叉反应。

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摘要

Human tissue prokallikrein is the enzymatically inactive zymogen of a serine proteinase involved in the liberation of vasoactive kinin peptides, and it is supposed that an impaired prokallikrein-to-kallikrein conversion is closely related to certain hypertensive and inflammatory disorders. Progress in understanding the biological role of the proenzyme has been limited by the absence of an accurate assay for the kallikrein precursor. We describe a sandwich enzyme-linked immunosorbent assay to measure human tissue prokallikrein using monospecific anti-peptide antibodies raised against propeptide derivatives. This method could detect a minimum concentration of 60 pg/ml prokallikrein and displayed no cross-reactivity or interference with mature tissue kallikrein. The intra- and inter-assay precision varied from 8-15%, respectively, indicating a reasonable reproducibility of the method. The level of prokallikrein was defined in different human urine samples, and the corresponding dilution curves showed good linearity. The mean recovery of added zymogen was 104%. Prokallikrein immunoassay is the first reported tool for the direct and sensitive quantification of the precursor of tissue kallikrein and should facilitate the precise determination of prokallikrein levels in a variety of biological specimen.
机译:人组织原激肽释放酶是丝氨酸蛋白酶的无酶促酶原,与血管活性激肽释放有关,并且认为原激肽释放酶至激肽释放酶的转化受损与某些高血压和炎性疾病密切相关。由于缺乏对激肽释放酶前体的准确测定,限制了对酶原生物学作用的理解。我们描述了三明治酶联免疫吸附测定法,以使用针对前肽衍生物的单特异性抗肽抗体来测量人体组织原激肽释放酶。该方法可以检测到最低浓度为60 pg / ml的激肽释放酶原,并且没有交叉反应或对成熟的激肽释放酶产生干扰。测定内和测定间精密度分别在8-15%之间变化,表明该方法具有合理的重现性。在不同的人类尿液样品中确定了前激肽释放酶的水平,并且相应的稀释曲线显示出良好的线性。添加的酶原的平均回收率为104%。原激肽释放酶免疫测定是对组织激肽释放酶前体进行直接和灵敏定量的第一个报道工具,应有助于精确测定各种生物学标本中的激肽释放酶水平。

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