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用于葡萄糖依赖性胰岛素促分泌肽 1-42(肠降血糖素激素的活性形式)的双克隆夹心免疫分析法。

Dual-monoclonal, sandwich immunoassay specific for glucose-dependent insulinotropic peptide1-42, the active form of the incretin hormone.

机构信息

Lilly Research Laboratories, Eli Lilly and Company, Indianapolis, IN, USA.

出版信息

Clin Chem. 2011 Jun;57(6):849-55. doi: 10.1373/clinchem.2010.159954. Epub 2011 Apr 22.

DOI:10.1373/clinchem.2010.159954
PMID:21515744
Abstract

BACKGROUND

Glucose-dependent insulinotropic peptide (GIP) is an incretin peptide secreted by intestinal K cells that stimulates insulin secretion in a glucose-dependent manner. It is secreted as an active, intact 42-amino acid peptide GIP(1-42), which is rapidly degraded by dipeptidyl peptidase 4 to GIP(3-42), which is inactive. There is currently no described monoclonal antibody-based sandwich immunoassay to quantify concentrations of GIP(1-42), the active form of the peptide.

METHODS

To create a sandwich ELISA for GIP(1-42), we generated a monoclonal antibody specific for the intact N-terminus of the peptide, which was further optimized to increase its affinity. We used this antibody as a conjugate antibody in a sandwich ELISA and paired it with an anti-total GIP capture monoclonal antibody to create a dual monoclonal sandwich ELISA for GIP(1-42).

RESULTS

The sandwich ELISA was highly specific for GIP(1-42) and did not recognize GIP(3-42). The ELISA demonstrated a broad dynamic range and a lower limit of quantification of 5 ng/L. Using the ELISA, we were able to show that GIP(1-42) concentrations in healthy volunteers increased dramatically in the postprandial state compared to the fasting state. GIP(1-42) values were correlated with total GIP values overall; however, there was substantial interindividual variation.

CONCLUSIONS

The use of an N-terminal-specific monoclonal antibody in a sandwich ELISA format provides a robust and convenient method for measuring concentrations of GIP(1-42), the active form of the incretin hormone. This ELISA should help to improve our understanding of the role of GIP(1-42) in regulating glucose-dependent insulin secretion.

摘要

背景

葡萄糖依赖性胰岛素促泌肽(GIP)是一种由肠道 K 细胞分泌的肠促胰岛素肽,以葡萄糖依赖性的方式刺激胰岛素分泌。它作为一种活性的、完整的 42 个氨基酸肽 GIP(1-42)分泌,该肽迅速被二肽基肽酶 4 降解为无活性的 GIP(3-42)。目前没有描述基于单克隆抗体的夹心免疫测定法来定量 GIP(1-42)的浓度,即肽的活性形式。

方法

为了创建 GIP(1-42)的夹心 ELISA,我们生成了一种针对肽完整 N 端的单克隆抗体,进一步优化了该抗体以增加其亲和力。我们将该抗体用作夹心 ELISA 的缀合抗体,并将其与抗总 GIP 捕获单克隆抗体配对,以创建用于 GIP(1-42)的双单克隆夹心 ELISA。

结果

夹心 ELISA 对 GIP(1-42)具有高度特异性,并且不识别 GIP(3-42)。该 ELISA 表现出广泛的动态范围和 5ng/L 的定量下限。使用 ELISA,我们能够表明健康志愿者的 GIP(1-42)浓度在餐后状态下与空腹状态相比急剧增加。GIP(1-42)值与总 GIP 值总体相关;然而,个体间存在很大差异。

结论

在夹心 ELISA 格式中使用 N 端特异性单克隆抗体提供了一种强大且方便的方法来测量 GIP(1-42)的浓度,即肠促胰岛素的活性形式。该 ELISA 应该有助于提高我们对 GIP(1-42)在调节葡萄糖依赖性胰岛素分泌中的作用的理解。

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