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抗噻虫啉单克隆抗体互补决定区可变区基因特征及关键识别位点的发现

Characterization of Variable Region Genes and Discovery of Key Recognition Sites in the Complementarity Determining Regions of the Anti-Thiacloprid Monoclonal Antibody.

机构信息

Institute of Pesticide and Environmental Toxicology, Ministry of Agriculture Key Laboratory of Molecular Biology of Crop Pathogens and Insects, Zhejiang University, Hangzhou 310058, China.

Department of Food Science and Nutrition, Zhejiang Key Laboratory for Agro-Food Processing, Zhejiang University, Hangzhou 310058, China.

出版信息

Int J Mol Sci. 2020 Sep 18;21(18):6857. doi: 10.3390/ijms21186857.

DOI:10.3390/ijms21186857
PMID:32962080
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7555632/
Abstract

Sequence-defined recombinant antibodies (rAbs) have emerged as alternatives to hybridoma-secreted monoclonal antibodies (mAbs) for performing immunoassays. However, the polyploidy nature of hybridomas often leads to the coexistence of aberrant or non-specific functional variable region (VR) gene transcripts, which complicates the identification of correct VR sequences. Herein, we introduced the use of LC-MS/MS combined with next-generation sequencing to characterize VR sequences in an anti-thiacloprid mAb, which was produced by a hybridoma with genetic antibody diversity. The certainty of VR sequences was verified by the functional analysis based on the recombinant antibody (rAb) expressed by HEK293 mammalian cells. The performance of the rAb was similar to that of the parental mAb, with IC values of 0.73 and 0.46 μg/L as measured by ELISAs. Moreover, molecular docking analysis revealed that Ser52 (H-CDR2), Trp98, and Trp93 (L-CDR3) residues in the complementarity determining regions (CDRs) of the identified VR sequences predominantly contributed to thiacloprid-specific recognition through hydrogen bonds and the CH-π interaction. Through single-site-directed alanine mutagenesis, we found that Trp98 and Trp93 (L-CDR3) showed high affinity to thiacloprid, while Ser52 (H-CDR2) had an auxiliary effect on the specific binding. This study presents an efficient and reliable way to determine the key recognition sites of hapten-specific mAbs, facilitating the improvement of antibody properties.

摘要

序列定义的重组抗体 (rAbs) 已成为杂交瘤分泌的单克隆抗体 (mAbs) 的替代品,可用于进行免疫分析。然而,杂交瘤的多倍体性质常常导致异常或非特异性功能可变区 (VR) 基因转录本的共存,这使得正确 VR 序列的鉴定变得复杂。在此,我们介绍了使用 LC-MS/MS 结合下一代测序来鉴定抗噻虫啉 mAb 的 VR 序列,该 mAb 由具有遗传抗体多样性的杂交瘤产生。通过基于 HEK293 哺乳动物细胞表达的重组抗体 (rAb) 的功能分析验证了 VR 序列的确定性。rAb 的性能与亲本 mAb 相似,ELISA 测量的 IC 值分别为 0.73 和 0.46 μg/L。此外,分子对接分析表明,鉴定的 VR 序列的互补决定区 (CDRs) 中的 Ser52 (H-CDR2)、Trp98 和 Trp93 (L-CDR3) 残基主要通过氢键和 CH-π 相互作用对噻虫啉特异性识别起作用。通过单点定向丙氨酸突变,我们发现 Trp98 和 Trp93 (L-CDR3) 对噻虫啉具有高亲和力,而 Ser52 (H-CDR2) 对特异性结合具有辅助作用。本研究提出了一种有效可靠的方法来确定半抗原特异性 mAbs 的关键识别位点,有利于改善抗体特性。

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