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适用于肌肉组织蛋白质组学分析的蛋白质提取方法。

Protein Extraction Methods Suitable for Muscle Tissue Proteomic Analysis.

作者信息

Vantaggiato Lorenza, Landi Claudia, Shaba Enxhi, Rossi Daniela, Sorrentino Vincenzo, Bini Luca

机构信息

Functional Proteomics Lab., Department Life Sciences, University of Siena, Via Aldo Moro 2, 53100 Siena, Italy.

Department of Molecular and Developmental Medicine, University of Siena, Via Aldo Moro 2, 53100 Siena, Italy.

出版信息

Proteomes. 2024 Sep 25;12(4):27. doi: 10.3390/proteomes12040027.

Abstract

Muscle tissue is one of the most dynamic and plastic tissues of the mammalian body and covers different roles, such as force generation and metabolic control. Muscular proteomics provides an important opportunity to reveal the molecular mechanisms behind muscle pathophysiology. To ensure successful proteomic analysis, it is necessary to have an efficient and reproducible protein extraction method. This study aimed to evaluate the efficacy of two different extraction protocols of muscle samples for two-dimensional gel electrophoresis. In particular, mouse muscle proteins were extracted by an SDS-based buffer (Method A) and by a UREA/CHAPS/DTE/TRIS solution (Method B). The efficacies of the methods were assessed by performing an image analysis of the 2DE gels and by statistical and multivariate analyses. The 2DE gels in both preparations showed good resolution and good spot overlapping. Methods A and B produced 2DE gels with different means of total spots, higher for B. Image analysis showed different patterns of protein abundance between the protocols. The results showed that the two methods extract and solubilize proteins with different chemical-physical characteristics and different cellular localizations. These results attest the efficacy and reproducibility of both protein extraction methods, which can be parallelly applied for comprehensive proteomic profiling of muscle tissue.

摘要

肌肉组织是哺乳动物体内最具活力和可塑性的组织之一,具有多种功能,如产生力量和控制代谢。肌肉蛋白质组学为揭示肌肉病理生理学背后的分子机制提供了重要契机。为确保蛋白质组学分析的成功,需要一种高效且可重复的蛋白质提取方法。本研究旨在评估两种不同的肌肉样本提取方案用于二维凝胶电泳的效果。具体而言,小鼠肌肉蛋白分别用基于SDS的缓冲液(方法A)和尿素/CHAPS/DTE/Tris溶液(方法B)进行提取。通过对二维凝胶进行图像分析以及统计和多变量分析来评估这些方法的效果。两种制备方法的二维凝胶均显示出良好的分辨率和斑点重叠。方法A和方法B产生的二维凝胶总斑点数均值不同,方法B的更高。图像分析显示两种方案之间蛋白质丰度模式不同。结果表明,这两种方法提取和溶解具有不同化学物理特性和不同细胞定位的蛋白质。这些结果证明了两种蛋白质提取方法的有效性和可重复性,它们可并行应用于肌肉组织的全面蛋白质组分析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f109/11503273/f24b40313eec/proteomes-12-00027-g001.jpg

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