Sandwich enzyme-linked immunosorbent assay (ELISA) to quantify monoclonal antibody (B[a]P-13) for herbal medicine products

IF 0.7 Q4 CHEMISTRY, MEDICINAL

Natural Products Journal Pub Date : 2022-11-04 DOI:10.2174/2210315513666221104154116

Han-Seung Shin, Yong-Yeon Kim

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引用次数: 0

Abstract

Sandwich enzyme-linked immunosorbent assay (ELISA) to quantify monoclonal antibody (B[a]P-13) Only a few studies have focused on the analysis using specific antibodies in the sandwich ELISA method to each B[a]P in herbal medicine products. In contrast to the sandwich ELISA method, many competitive ELISA methods using specific antibodies such as benzo[a]pyrene monoclonal antibody (B[a]P-13) and a goat anti-mouse IgG (H+L) cross-adsorbed secondary antibody, horseradish peroxidase (HRP) were developed. The objective of this study was to develop and validate the method for the response of the benzo[a]pyrene monoclonal antibody (B[a]P-13) and goat anti-mouse IgG (H+L) cross-adsorbed secondary antibody (HRP) to prepare the immunogen and its application to detect the benzo[a]pyrene in various herbal medicine products. This research method includes preparation of B[a]P-protein conjugates, sampling and extraction procedure for herbal medicines, sandwich ELISA procedure, evaluation of cross-reactivity for determination, matrix effect of the organic solvents, correlation of benzo[a]pyrene detection ELISA compared to HPLC-FLD in herbal medicine products. The sandwich ELISA method for B[a]P was validated in linearity (R2 > 0.99), the limit of detection (LOD) (0.080.19 μg/kg) and limit of quantification (LOQ) (0.240.57 μg/kg), accuracy (95.58117.06 %), and precision (3.8010.26 %). The cross-reactivity (CR) was found for B[a]P (100%), CHR (39%), B[b]F (27%), and B[a]A (41%). As a solvent, acetonitrile (MeCN) was used to express the normalized sandwich ELISA calibration curves with benzo[a]pyrene monoclonal antibody (B[a]P-13). The antigen-antibody binding in sandwich ELISA was decreased about 10 times with increasing the salt content (0.0060.18 mol/L phosphate to 20400 mmol/L). The pH range from 6 to 9 was not considered to affect the performance of the sandwich ELISA. Correlation of B[a]P detection in herbal medicines with ELISA compared to HPLC-FLD expressed good correlation (R2 = 0.991) and the slope of the graph for the ELISA (B[a]P-equivalents μg/kg) value divided by the HPLC-FLD (B[a]P μg/kg) value was 0.7292. Therefore, sandwich ELISA method using benzo[a]pyrene monoclonal antibody (B[a]P-13) could be an alternative screening method for detection of B[a]P in herbal medicine products.

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夹心酶联免疫吸附试验（ELISA）用于定量草药产品的单克隆抗体（B[a]P-13）

用于定量单克隆抗体（B[a]P-13）的夹心酶联免疫吸附试验（ELISA）只有少数研究集中于在夹心ELISA方法中使用特异性抗体对草药产品中的每种B[a]P进行分析。与夹心ELISA法不同，开发了许多使用特异性抗体的竞争性ELISA法，如苯并[a]芘单克隆抗体（B[a]P-13）和山羊抗小鼠IgG（H+L）交叉吸附的第二抗体辣根过氧化物酶（HRP）。本研究的目的是开发和验证苯并[a]芘单克隆抗体（B[a]P-13）和山羊抗小鼠IgG（H+L）交叉吸附二抗（HRP）制备免疫原的方法及其在检测各种草药产品中苯并[a]芘中的应用。该研究方法包括B[a]P-蛋白偶联物的制备、中草药的取样和提取程序、夹心ELISA程序、用于测定的交叉反应性评估、有机溶剂的基质效应、检测中草药产品中苯并[a]芘的ELISA与HPLC-FLD的相关性。夹心ELISA法对B[a]P的线性度（R2>0.99）、检出限（LOD）（0.080.19μg/kg）和定量限（LOQ）（0.240.57μg/kg），准确度（95.58117.06%），精密度（3.8010.26%）。发现B[a]P（100%）、CHR（39%）、B[B]F（27%）和B[a]a（41%）的交叉反应性（CR）。使用乙腈（MeCN）作为溶剂，用苯并[a]芘单克隆抗体（B[a]P-13）表达标准化的夹心ELISA校准曲线。随着盐含量的增加，夹心ELISA中抗原-抗体结合降低了约10倍（0.0060.18mol/L磷酸盐至20400mmol/L）。pH范围从6到9不被认为影响夹心ELISA的性能。与HPLC-FLD相比，草药中的B[a]P检测与ELISA的相关性表现出良好的相关性（R2=0.991），ELISA（B[a]P-当量μ，苯并[a]芘单克隆抗体（B[a]P-13）夹心ELISA法是检测中草药产品中B[a]P的一种替代方法。

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来源期刊

Natural Products Journal CHEMISTRY, MEDICINAL-

CiteScore

1.70

自引率

0.00%

发文量

期刊介绍： The Natural Products Journal a peer reviewed journal, aims to publish all the latest and outstanding developments in natural products. The Natural Products Journal publishes original research articles, full-length/mini reviews, letters and guest edited issues on all aspects of research and development in the field including: isolation, purification, structure elucidation, synthesis and bioactivity of chemical compounds found in nature.