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用于血红蛋白病研究的过氧化物酶/单克隆抗体结合物。

Peroxidase/monoclonal antibody conjugates for the study of hemoglobinopathies.

作者信息

Moscoso H, Kiefer C R, Shyamala M, Garver F A

机构信息

Department of Immunology and Microbiology, Medical College of Georgia, Augusta 30912-2400.

出版信息

J Clin Lab Anal. 1993;7(4):214-9. doi: 10.1002/jcla.1860070405.

Abstract

Monoclonal antibodies (mAbs) to normal human hemoglobins (Hbs) A and F and to variant Hbs C and G-Philadelphia were conjugated to horseradish peroxidase (HRP) and used in qualitative or quantitative enzyme-linked immunosorbent assays (ELISAs). Conjugates with output molar HRP/IgG ratios close to 2.0 had higher avidity for the cognate antigens than those with ratios above or below 2.0. The analytical sensitivities of the conjugates ranged from 0.2 to 4 ng of hemolysate containing the target hemoglobin, and it was not related to the input or the output HRP/IgG ratios. The overall imprecision for the qualitative ELISA was below 8%, and the accuracy for the identification of Hbs C and G-Philadelphia was 100% as compared with established methods. Quantitative determinations of HbA based upon direct dose-response curves showed an analytical sensitivity of 1% and an imprecision < or = 11%. The most significant application of the HbA assay was in the differential diagnosis of hemoglobinopathies associated with partial or total suppression of HbA synthesis. Competitive dose-response curves for the HRP/anti-gamma conjugate allowed the quantification of HbF in the clinically significant range of 0.5-10%, with an imprecision < or = 12%. It is concluded that the incorporation of HRP/mAb conjugates into the ELISA technique offers a simpler, more rapid, yet specific alternative for the measurement of hemoglobins.

摘要

将针对正常人血红蛋白(Hb)A和F以及变异型Hb C和G-费城的单克隆抗体(mAb)与辣根过氧化物酶(HRP)偶联,并用于定性或定量酶联免疫吸附测定(ELISA)。输出摩尔HRP/IgG比率接近2.0的偶联物对同源抗原的亲和力高于比率高于或低于2.0的偶联物。偶联物的分析灵敏度范围为0.2至4 ng含有目标血红蛋白的溶血产物,且与输入或输出HRP/IgG比率无关。定性ELISA的总体不精密度低于8%,与既定方法相比,Hb C和G-费城的鉴定准确率为100%。基于直接剂量反应曲线的HbA定量测定显示分析灵敏度为1%,不精密度≤11%。HbA测定最显著的应用在于与HbA合成部分或完全抑制相关的血红蛋白病的鉴别诊断。HRP/抗γ偶联物的竞争剂量反应曲线能够在0.5 - 10%的临床显著范围内对HbF进行定量,不精密度≤12%。得出的结论是,将HRP/mAb偶联物纳入ELISA技术为血红蛋白的测量提供了一种更简单、更快速且特异的替代方法。

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