Detection of Calcitonin Gene-related Peptide Based on Increased Antigen-Driven Interaction with Antibody Variable Regions Provisionally Accepted
Yueqing Cheng1
Yujie Gao1
Shengshuo Zhang1
Yujie Zou1
Guangwei Zhao2
Liyuan Zheng3
Binghui Hou4
Mei Li1*
Jinhua Dong5*
- 1Shandong Second Medical University, China
- 2Shandong University, China
- 3The University of Rehabilitation, China
- 4Qingdao University, China
- 5University of Health and Rehabilitation Sciences, China
Introduction: Calcitonin gene-related peptide (CGRP) is involved in trigeminal neuralgia and migraine, and measuring the CGRP concentration in the serum is crucial for the early prediction of these conditions. Current methods for CGRP detection are primarily competitive enzyme-linked immunosorbent assays (ELISA), which have a narrow detection range. Methods: The genes of anti-CGRP antibody variable regions were cloned into pDong1 vector to obtain pDong1-CGRP/Fab, with which phage-Fab was prepared, and the concentration of CGRP was detected by competitive ELISA. The pDong1-CGRP/Fab was modified to obtain pDong1-CGRP/OS, with which the co-expression solution containing phage-displayed heavy chain variable fragments (phage-VH) and light chain was obtained. CGRP was detected by OS-ELISA based on phage-VH, antibody light chain, and anti-light chain antibody. The VL gene was cloned into the pMAL vector to obtain pMAL-VL(CGRP), with which maltose binding protein fused with VL (MBP-VL) was prepared. CGRP was detected by OS-ELISA employing MBP-VL and phage-VH. Results: OS-ELISAs that measure the CGRP concentration by quantifying the interaction between variable regions were investigated. OS-ELISA using phage-VH and secreted light chains in the same culture system exhibited a limit of detection (LOD) of 0.05 nM, offering higher sensitivity than competitive assay with an LOD of 2.07 nM, whereas using phage-VH and separately prepared MBP-VL exhibited an LOD of 0.15 nM and a broader detection range of 0.15-500 nM than competitive ELISA, whose detection range was 0.75-10 nM. Discussion: The combination of the two OS assays achieved high sensitivity and a broad detection range for CGRP, which may have significance in clinical applications.
Keywords: Migraine, CGRP, detection, antibody, Open sandwich ELISA
Received: 03 Mar 2024;
Accepted: 08 May 2024.
Copyright: © 2024 Cheng, Gao, Zhang, Zou, Zhao, Zheng, Hou, Li and Dong. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
* Correspondence:
Prof. Mei Li, Shandong Second Medical University, Weifang, China
Prof. Jinhua Dong, University of Health and Rehabilitation Sciences, Qingdao, China