Screening of monoclonal antibodies against specific phosphonylation sites and analysis of serum samples exposed to soman and VX using an indirect competitive enzyme-linked immunosorbent assay

Qiao Lv; Hui-Lan Yu; Yang Yang; Fan-Hua Meng; Xian-Dong Dai; Pei-Yu Jiang; Chang-Cai Liu

doi:10.1007/s00216-022-03914-x

Screening of monoclonal antibodies against specific phosphonylation sites and analysis of serum samples exposed to soman and VX using an indirect competitive enzyme-linked immunosorbent assay

Anal Bioanal Chem. 2022 Mar;414(8):2713-2724. doi: 10.1007/s00216-022-03914-x. Epub 2022 Jan 26.

Authors

Qiao Lv^{1

2}, Hui-Lan Yu^{3

4}, Yang Yang^{1

2}, Fan-Hua Meng¹, Xian-Dong Dai¹, Pei-Yu Jiang^{1

2}, Chang-Cai Liu^{5

6}

Affiliations

¹ State Key Laboratory of NBC Protection for Civilian, Beijing, 102205, China.
² Laboratory of Analytical Chemistry, Research Institute of Chemical Defence, Beijing, 102205, China.
³ State Key Laboratory of NBC Protection for Civilian, Beijing, 102205, China. yuhuilan1@163.com.
⁴ Laboratory of Analytical Chemistry, Research Institute of Chemical Defence, Beijing, 102205, China. yuhuilan1@163.com.
⁵ State Key Laboratory of NBC Protection for Civilian, Beijing, 102205, China. liuchangcai@sklnbcpc.cn.
⁶ Laboratory of Analytical Chemistry, Research Institute of Chemical Defence, Beijing, 102205, China. liuchangcai@sklnbcpc.cn.

PMID: 35083511
DOI: 10.1007/s00216-022-03914-x

Abstract

Organophosphorus nerve agents (OPNAs) covalently bind to tyrosine 411 of human serum albumin (HSA) and the formed adducts are stable biomarkers of OPNA exposure. The detection of these adducts has been limited to mass spectrometry techniques combined with protein digestion. Here, we developed indirect competitive ELISA (icELISA) methods to verify OPNA exposure by the detection of OPNA-phosphonylated adducts at tyrosine 411 residue (OPNA-HSA adducts), in which monoclonal antibodies (mAbs) against phosphonylation sites at tyrosine 411 were introduced. The two mAbs were prepared by the fourth generation of rabbit mAb technology using the phosphonylated peptides of LVRY^{(GD or VX)}TKKVPQC as the haptens. These mAbs were screened using our developed competitive ELISA method and then selected based on their individual affinity and selectivity. As a result, we obtained two mAbs that recognized the HSA Tyr 411 adduct of GD (mAb-5G2) or VX (mAb-12B9), respectively. They shared the highest affinity exhibiting a Kd value of about 10^-6 mol/L of the OPNA exposure concentration. They also had remarkable selectivity, which could especially recognize their individual OPNA-HSA adducts in a native state but did not recognize other OPNA-HSAs and unadducted HSAs. Especially for mAb-12B9, it could clearly distinguish VX-HSA and GB-HSA between which there was only one alkyl difference in their phosphonyl portion of the adducted sites. The two mAbs were then used to build the icELISA method for analysis of the serum samples exposed to OPNA. It was found that the detectable lowest GD- and VX-exposed concentrations in serum samples were respectively 1.0 × 10^-6 mol/L and 10.0 × 10^-6 mol/L. This study provides one novel approach and strategy for the retrospective detection of OPNA exposure, and the two mAbs have great potential to be extended for point-of-care testing of OPNA intoxication.

Keywords: Albumin adduct; Competitive ELISA; Immunodetection; Organophosphorus nerve agents; Recombinant monoclonal antibody.

MeSH terms

Animals
Antibodies, Monoclonal
Enzyme-Linked Immunosorbent Assay
Organothiophosphorus Compounds
Rabbits
Retrospective Studies
Soman*

Substances

Antibodies, Monoclonal
Organothiophosphorus Compounds
Soman
VX