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基于荧光显微镜的 GLUT4 易位定量分析。

Fluorescence microscopy-based quantitation of GLUT4 translocation.

机构信息

University of Applied Sciences Upper Austria, School of Engineering and Environmental Sciences, Stelzhamerstraße 23, 4600 Wels, Austria.

FFoQSI GmbH-Austrian Competence Centre for Feed and Food Quality, Safety and Innovation, Technopark 1D, 3430 Tulln, Austria.

出版信息

Methods Appl Fluoresc. 2022 Jan 21;10(2). doi: 10.1088/2050-6120/ac4998.


DOI:10.1088/2050-6120/ac4998
PMID:35008072
Abstract

Postprandial insulin-stimulated glucose uptake into target tissue is crucial for the maintenance of normal blood glucose homeostasis. This step is rate-limited by the number of facilitative glucose transporters type 4 (GLUT4) present in the plasma membrane. Since insulin resistance and impaired GLUT4 translocation are associated with the development of metabolic disorders such as type 2 diabetes, this transporter has become an important target of antidiabetic drug research. The application of screening approaches that are based on the analysis of GLUT4 translocation to the plasma membrane to identify substances with insulinomimetic properties has gained global research interest in recent years. Here, we review methods that have been implemented to quantitate the translocation of GLUT4 to the plasma membrane. These methods can be broadly divided into two sections: microscopy-based technologies (e.g., immunoelectron, confocal or total internal reflection fluorescence microscopy) and biochemical and spectrometric approaches (e.g., membrane fractionation, photoaffinity labeling or flow cytometry). In this review, we discuss the most relevant approaches applied to GLUT4 thus far, highlighting the advantages and disadvantages of these approaches, and we provide a critical discussion and outlook into new methodological opportunities.

摘要

餐后胰岛素刺激靶组织葡萄糖摄取对于维持正常血糖稳态至关重要。这一步骤受到质膜中存在的易化葡萄糖转运蛋白 4 (GLUT4)数量的限制。由于胰岛素抵抗和 GLUT4 易位受损与 2 型糖尿病等代谢紊乱的发展有关,因此该转运蛋白已成为抗糖尿病药物研究的重要靶点。近年来,基于分析 GLUT4 易位至质膜的筛选方法在识别具有胰岛素模拟特性的物质方面引起了全球研究兴趣。在这里,我们回顾了用于定量 GLUT4 易位至质膜的方法。这些方法可以大致分为两类:基于显微镜的技术(例如,免疫电子显微镜、共聚焦或全内反射荧光显微镜)和生化及光谱方法(例如,膜分离、光亲和标记或流式细胞术)。在这篇综述中,我们讨论了迄今为止应用于 GLUT4 的最相关方法,强调了这些方法的优缺点,并对新的方法学机会进行了批判性讨论和展望。

相似文献

[1]
Fluorescence microscopy-based quantitation of GLUT4 translocation.

Methods Appl Fluoresc. 2022-1-21

[2]
Fluorescence Microscopy-Based Quantitation of GLUT4 Translocation: High Throughput or High Content?

Int J Mol Sci. 2020-10-27

[3]
Identification of novel insulin mimetic drugs by quantitative total internal reflection fluorescence (TIRF) microscopy.

Br J Pharmacol. 2014-12

[4]
Insulin-Mimetic Activity of Herbal Extracts Identified with Large-Scale Total Internal Reflection Fluorescence Microscopy.

Nutrients. 2024-7-9

[5]
Intracellular organization of insulin signaling and GLUT4 translocation.

Recent Prog Horm Res. 2001

[6]
Real time qualitative and quantitative GLUT4 translocation assay.

Methods Enzymol. 2012

[7]
A pre-docking role for microtubules in insulin-stimulated glucose transporter 4 translocation.

FEBS J. 2008-2

[8]
Biomolecular Characterization of Putative Antidiabetic Herbal Extracts.

PLoS One. 2016-1-28

[9]
Quantitative measurement of GLUT4 translocation to the plasma membrane by flow cytometry.

J Vis Exp. 2010-11-7

[10]
Total Internal Reflection Fluorescence Microscopy to Study GLUT4 Trafficking.

Methods Mol Biol. 2018

引用本文的文献

[1]
Mechanisms and therapeutics of insulin signaling transduction genes in diabetic cardiomyopathy: a comprehensive updated review.

Front Endocrinol (Lausanne). 2025-7-17

[2]
Live-cell GLUT4 translocation assay reveals Per3 as a novel regulator of circadian insulin sensitivity in skeletal muscle cells.

Biol Open. 2025-7-15

[3]
Identification of Plant Phenolics from and as Novel PPARγ Partial Agonists and Hypoglycemic Agents.

J Agric Food Chem. 2025-6-4

[4]
A comprehensive / screening toolbox for the elucidation of glucose homeostasis modulating properties of plant extracts (from roots) and its bioactives.

Front Pharmacol. 2024-6-26

[5]
Flow cytometry protocol for GLUT4-myc detection on cell surfaces.

Biosci Rep. 2024-4-24

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