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研究碳水化合物 - 蛋白质相互作用的分析方法的演变简述。

A brief account of evolution of assays to study carbohydrate-protein interaction.

作者信息

Ballal Suhas

机构信息

Department of Chemistry and Biochemistry, Jain (Deemed to be) University, Bengaluru, India.

出版信息

J Mol Recognit. 2024 Jan;37(1):e3065. doi: 10.1002/jmr.3065. Epub 2023 Oct 20.

Abstract

Molecular recognition remains one of the most desirable means of cellular communication. Each cell offers a unique surface pattern of biomolecules that makes it very specific about the nature of molecules that interact with the cell. Protein-glycan interaction has been one of the most common forms of cell signaling. Glycans expressed on the cell surface interact with an exogenous protein, and in many cases lead to a physiological response. These carbohydrate-binding proteins, commonly known as lectins, are very specific to the glycan they bind to. An exogenous lectin interacting with an animal cell surface glycan is generally studied using the classical hemagglutination assay. However, this method presents certain challenges that make it imperative to design and develop novel methods that are more specific and efficient in their interaction. In the last decade, a few methods have been developed to analyze more diverse reactions and use a lesser amount of sample. In some cases, the processing of the sample is also reduced. This review discusses how the methods have evolved over the decades and how they have reduced error while becoming more efficient.

摘要

分子识别仍然是细胞通讯最理想的方式之一。每个细胞都呈现出独特的生物分子表面模式,这使得细胞对与自身相互作用的分子性质具有高度特异性。蛋白质-聚糖相互作用一直是细胞信号传导最常见的形式之一。细胞表面表达的聚糖与外源蛋白质相互作用,在许多情况下会引发生理反应。这些碳水化合物结合蛋白,通常被称为凝集素,对它们所结合的聚糖具有高度特异性。与动物细胞表面聚糖相互作用的外源凝集素一般通过经典的血细胞凝集试验进行研究。然而,这种方法存在一定的挑战,因此迫切需要设计和开发在相互作用方面更具特异性和高效性的新方法。在过去十年中,已经开发了一些方法来分析更多样化的反应并减少样品用量。在某些情况下,样品处理过程也得到了简化。本文综述了这些方法在几十年间是如何演变的,以及它们在提高效率的同时如何减少误差。

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