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用于鉴定人嗜铬粒蛋白A抗原区域的肽微阵列。

Peptide microarrays for the characterization of antigenic regions of human chromogranin A.

作者信息

Chiari Marcella, Cretich Marina, Corti Angelo, Damin Francesco, Pirri Giovanna, Longhi Renato

机构信息

Istituto di Chimica del Riconoscimento Molecolare, Milan, Italy.

出版信息

Proteomics. 2005 Sep;5(14):3600-3. doi: 10.1002/pmic.200401216.

Abstract

Microarraying peptides is a powerful proteomics technique for studying molecular recognition events. Since peptides have small molecular mass, they are not easily accessible when adsorbed onto solid supports. Moreover, peptides can lack a well-defined three-dimensional structure, and therefore a correct orientation is essential to promote the interaction with their target. In this work, we investigated the suitability as a peptide array substrate of a glass slide coated with a copolymer of N,N-dimethylacrylamide, N,N-acryloyloxysuccinimide, and [3-(methacryloyl-oxy)propyl]trimethoxysilyl. This polymeric surface was used as substrate for peptides in the characterization of linear antigenic sites of human chromogranin A, a useful tissue and serum marker for neuroendocrine tumors and a precursor of many biologically active peptides. The microarray support provided sufficient accessibility of the ligand, with no need for a spacer, as the polymer chains prevent interaction of immobilized peptides with substrate. In addition, the polymeric surface constitutes an aqueous micro-environment in which linear epitopes are freely exposed despite peptide random orientation. The results reported in this article are in accordance with those obtained in conventional ELISA assays using biotinylated and non-biotinylated peptides.

摘要

肽微阵列是一种用于研究分子识别事件的强大蛋白质组学技术。由于肽的分子量较小,当它们吸附到固体支持物上时不易接近。此外,肽可能缺乏明确的三维结构,因此正确的方向对于促进与靶标的相互作用至关重要。在这项工作中,我们研究了涂有N,N-二甲基丙烯酰胺、N,N-丙烯酰氧基琥珀酰亚胺和[3-(甲基丙烯酰氧基)丙基]三甲氧基硅烷共聚物的载玻片作为肽阵列底物的适用性。这种聚合物表面被用作肽的底物,用于表征人嗜铬粒蛋白A的线性抗原位点,人嗜铬粒蛋白A是神经内分泌肿瘤的一种有用的组织和血清标志物,也是许多生物活性肽的前体。微阵列支持物提供了足够的配体可及性,无需间隔物,因为聚合物链可防止固定化肽与底物相互作用。此外,聚合物表面构成了一个水性微环境,尽管肽的取向是随机的,但线性表位仍可自由暴露。本文报道的结果与使用生物素化和非生物素化肽的传统ELISA分析中获得的结果一致。

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