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从酵母细胞中分离纯酵母细胞壁蛋白的可靠方法。

Reliable Approach for Pure Yeast Cell Wall Protein Isolation from Yeast Cells.

作者信息

Yammine Marie, Bray Fabrice, Flament Stéphanie, Picavet Antoine, Lacroix Jean-Marie, Poilpré Emmanuel, Mouly Isabelle, Rolando Christian

机构信息

Univ. Lille, CNRS, USR 3290, MSAP, Miniaturisation pour la Synthèse, l'Analyse et la Protéomique, F-59000 Lille, France.

Lesaffre international, Research and Development department, 77 rue de Menin, F-59520 Marquette-lez-Lille, France.

出版信息

ACS Omega. 2022 Aug 15;7(34):29702-29713. doi: 10.1021/acsomega.2c02176. eCollection 2022 Aug 30.

Abstract

yeast is a fungus presenting a peripheral organelle called the cell wall. The cell wall protects the yeast cell from stress and provides means for communication with the surrounding environment. It has a complex molecular structure, composed of an internal part of cross-linked polysaccharides and an external part of mannoproteins. These latter are very interesting owing to their functional properties, dependent on their molecular features with massive mannosylations. Therefore, the molecular characterization of mannoproteins is a must relying on the optimal isolation and preparation of the cell wall fraction. Multiple methods are well reported for yeast cell wall isolation. The most applied one consists of yeast cell lysis by mechanical disruption. However, applying this classical approach to S288C yeast cells showed considerable contamination with noncell wall proteins, mainly comprising mitochondrial proteins. Herein, we tried to further purify the yeast cell wall preparation by two means: ultracentrifugation and Triton X-100 addition. While the first strategy showed limited outcomes in mitochondrial protein removal, the second strategy showed optimal results when Triton X-100 was added at 5%, allowing the identification of more mannoproteins and significantly enriching their amounts. This promising method could be reliably implemented on the lab scale for identification of mannoproteins and molecular characterization and industrial processes for "pure" cell wall isolation.

摘要

酵母是一种具有称为细胞壁的外周细胞器的真菌。细胞壁保护酵母细胞免受压力,并提供与周围环境进行交流的方式。它具有复杂的分子结构,由交联多糖的内部部分和甘露糖蛋白的外部部分组成。由于其功能特性,后者非常有趣,这些功能特性取决于其具有大量甘露糖基化的分子特征。因此,甘露糖蛋白的分子表征必须依赖于细胞壁组分的最佳分离和制备。关于酵母细胞壁分离的多种方法已有充分报道。应用最广泛的方法是通过机械破碎使酵母细胞裂解。然而,将这种经典方法应用于S288C酵母细胞时,发现存在大量非细胞壁蛋白污染,主要是线粒体蛋白。在此,我们尝试通过两种方法进一步纯化酵母细胞壁制剂:超速离心和添加Triton X-100。虽然第一种策略在去除线粒体蛋白方面效果有限,但当添加5%的Triton X-100时,第二种策略显示出最佳结果,能够鉴定出更多的甘露糖蛋白并显著增加其含量。这种有前景的方法可以在实验室规模上可靠地实施,用于甘露糖蛋白的鉴定和分子表征,以及“纯”细胞壁分离的工业过程。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e2c0/9435031/74ba25b73bcf/ao2c02176_0002.jpg

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