用于定量检测人血浆中脂蛋白脂肪酶质量的直接夹心酶联免疫吸附测定法的开发与评估

Development and evaluation of a direct sandwich enzyme-linked immunosorbent assay for the quantification of lipoprotein lipase mass in human plasma.

作者信息

Kimura H, Ohkaru Y, Katoh K, Ishii H, Sunahara N, Takagi A, Ikeda Y

机构信息

The Division of Laboratory Products, Dainippon Pharmaceutical Co., Suita, Osaka, Japan.

出版信息

Clin Biochem. 1999 Feb;32(1):15-23. doi: 10.1016/s0009-9120(98)00081-2.

DOI:10.1016/s0009-9120(98)00081-2

PMID:10074887

Abstract

OBJECTIVE

The purpose of this study was to develop and evaluate a direct sandwich enzyme-linked immunosorbent assay (ELISA) for quantification of the lipoprotein lipase (LPL) immunoreactive mass in human plasma using monoclonal antibodies (MAbs) directed against LPL purified from human postheparin plasma (PHP) [corrected].

METHODS AND RESULTS

The direct sandwich-ELISA was performed using a combination of two distinct types of MAbs that recognize different epitopes on the LPL molecule. The immunoreactive mass of human LPL was specifically measured using a horseradish peroxidase-labeled anti-human LPL MAb [1(1)D2B2] as an enzyme-linked MAb, and an anti-human LPL MAb [2(10)F8F9] coated on a polystyrene microtiter plate as a solid-phase MAb. Purified human PHP-LPL was used as a standard material. The detection range of the sandwich-ELISA was 3.6-460 ng of LPL protein per mL of plasma. The intra- and interassay coefficients of variation were less than 5.9% and 3.3%, respectively. The validity of this method was additionally assured by the recovery test, which resulted in the variation only between 97.5% and 105.1%, and also by the interference test, which resulted in noninterference of LPL assay with a high concentration of triglyceride, hemoglobin, bilirubin, uric acid, or creatinine. To assess the reliability of the LPL mass values obtained with the direct sandwich-ELISA, they were compared with LPL mass values determined by the one-step sandwich-EIA (MARKIT-F LPL EIA kit) previously established by us. This comparison showed a highly significant correlation (r = +0.990) between the two sets of values. The LPL mass concentrations in PHP from 33 healthy subjects were 267 +/- 53 and 257 +/- 59 ng/mL (mean +/- SD), respectively.

CONCLUSION

The present direct sandwich-ELISA is useful for rapidly identifying certain abnormalities of LPL in PHP samples from patients with hypertriglyceridemia [corrected].

摘要

目的

本研究旨在开发并评估一种直接夹心酶联免疫吸附测定法（ELISA），该方法使用针对从人肝素后血浆（PHP）中纯化的脂蛋白脂肪酶（LPL）的单克隆抗体（MAb）来定量人血浆中LPL的免疫反应性质量[已校正]。

方法与结果

直接夹心ELISA使用两种不同类型的MAb组合进行，这两种MAb识别LPL分子上不同的表位。使用辣根过氧化物酶标记的抗人LPL单克隆抗体[1(1)D2B2]作为酶联单克隆抗体，以及包被在聚苯乙烯微量滴定板上的抗人LPL单克隆抗体[2(10)F8F9]作为固相单克隆抗体，特异性测量人LPL的免疫反应性质量。纯化的人PHP-LPL用作标准物质。夹心ELISA的检测范围为每毫升血浆中3.6 - 460 ng的LPL蛋白。批内和批间变异系数分别小于5.9%和3.3%。回收率测试进一步确保了该方法的有效性，回收率仅在97.5%至105.1%之间变化，干扰测试也表明高浓度的甘油三酯、血红蛋白、胆红素、尿酸或肌酐对LPL测定无干扰。为评估通过直接夹心ELISA获得的LPL质量值的可靠性，将其与我们之前建立的一步夹心酶免疫测定法（MARKIT-F LPL EIA试剂盒）测定的LPL质量值进行比较。这种比较显示两组值之间具有高度显著的相关性（r = +0.990）。33名健康受试者的PHP中LPL质量浓度分别为267±53和257±59 ng/mL（平均值±标准差）。