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通过流式细胞术、蛋白质组分析和mRNA谱分析预测酿造酵母接种物的絮凝能力。

Prediction of flocculation ability of brewing yeast inoculates by flow cytometry, proteome analysis, and mRNA profiling.

作者信息

Heine Franziska, Stahl Frank, Sträuber Heike, Wiacek Claudia, Benndorf Dirk, Repenning Cornelia, Schmidt Frank, Scheper Thomas, von Bergen Martin, Harms Hauke, Müller Susann

机构信息

Helmholtz Centre for Environmental Research-UFZ, Department of Environmental Microbiology, Leipzig, Germany.

出版信息

Cytometry A. 2009 Feb;75(2):140-7. doi: 10.1002/cyto.a.20661.

DOI:10.1002/cyto.a.20661
PMID:19072835
Abstract

The ability of brewing yeast to flocculate is an important feature for brewing of qualitatively good beer. Flocculation involves two main cell wall structures, which are the flocculation proteins (flocculins) and mannans, to which these flocculins bind. Unfortunately, in practice, the flocculation ability may get lost after several repitches. Flow cytometry was employed to analyze glucose and mannose structures of the cell surface by application of fluorescent lectins. Validation of the expression of the flocculin genes Lg-FLO1, FLO1, FLO5, and FLO9 was carried out using microarray techniques. SDS-PAGE, western blot, and ESI-MS/MS analyses served to isolate and determine yeast cell flocculins. Mannose and glucose labeling with fluorescent lectins allowed differentiating powdery and flocculent yeast cells under laboratory conditions. Using microarray techniques and proteomics, the four flocculation genes Lg-FLO1, FLO1, FLO5, FLO9, and the protein Lg-Flo1p were identified as factors of major importance for flocculation. The expression of the genes was several times higher in flocculent yeast cells than in powdery ones. Flow cytometry is a fast and simple method to quantify the proportions of powdery and flocculent yeast cells in suspensions under defined cultivation conditions. However, differentiation under industrial conditions will require mRNA and protein expression profiling.

摘要

酿造酵母的絮凝能力是酿造优质啤酒的一个重要特性。絮凝涉及两种主要的细胞壁结构,即絮凝蛋白(絮凝素)和甘露聚糖,絮凝素可与甘露聚糖结合。遗憾的是,在实际操作中,经过几次转接培养后,絮凝能力可能会丧失。通过应用荧光凝集素,采用流式细胞术分析细胞表面的葡萄糖和甘露糖结构。利用微阵列技术对絮凝素基因Lg - FLO1、FLO1、FLO5和FLO9的表达进行验证。SDS - PAGE、蛋白质印迹和ESI - MS/MS分析用于分离和鉴定酵母细胞絮凝素。用荧光凝集素进行甘露糖和葡萄糖标记,可在实验室条件下区分粉状和絮凝状酵母细胞。利用微阵列技术和蛋白质组学,确定了四个絮凝基因Lg - FLO1、FLO1、FLO5、FLO9以及蛋白质Lg - Flo1p是絮凝的主要重要因素。絮凝酵母细胞中这些基因的表达比粉状酵母细胞中的表达高几倍。流式细胞术是一种快速简便的方法,可在规定培养条件下对悬浮液中粉状和絮凝状酵母细胞的比例进行定量。然而,在工业条件下进行区分将需要mRNA和蛋白质表达谱分析。

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Prediction of flocculation ability of brewing yeast inoculates by flow cytometry, proteome analysis, and mRNA profiling.通过流式细胞术、蛋白质组分析和mRNA谱分析预测酿造酵母接种物的絮凝能力。
Cytometry A. 2009 Feb;75(2):140-7. doi: 10.1002/cyto.a.20661.
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