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A vector carrying the GFP gene (Green fluorescent protein) as a yeast marker for fermentation processes

机译:带有GFP基因(绿色荧光蛋白)作为酵母菌发酵过程标记的载体

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Contaminant yeasts spoil pure culture fermentations and cause great losses in quality and product yields. They can be detected by a variety of methods although none being so efficient for early detection of contaminant yeast cells that appear at low frequency. Pure cultures bearing genetic markers can ease the direct identification of cells and colonies among contaminants. Fast and easy detection are desired and morphological markers would even help the direct visualization of marked pure cultures among contaminants. The GFP gene for green fluorescent protein of Aquorea victoria, proved to be a very efficient marker to visualize transformed cells in mixed populations and tissues. To test this marker in the study of contaminated yeast fermentations, the GFP gene was used to construct a vector under the control of the ADH2 promoter (pYGFP3). Since ADH2 is repressed by glucose the expression of the protein would not interfere in the course of fermentation. The transformed yeasts with the vector pYGFP3 showed high stability and high bioluminescence to permit identification of marked cells among a mixed population of cells. The vector opens the possibility to conduct further studies aiming to develop an efficient method for early detection of spoilage yeasts in industrial fermentative processes.
机译:污染的酵母破坏了纯培养物的发酵,并导致质量和产品产量的巨大损失。可以通过多种方法检测它们,尽管没有一种方法能如此有效地早期检测低频率出现的污染酵母细胞。带有遗传标记的纯培养物可简化污染物中细胞和菌落的直接鉴定。需要快速且容易的检测,形态标记甚至可以帮助直接可视化污染物中标记的纯培养物。维多利亚水绿色荧光蛋白的GFP基因被证明是可视化混合种群和组织中转化细胞的非常有效的标记。为了在受污染的酵母发酵研究中测试该标记,GFP基因用于在ADH2启动子(pYGFP3)控制下构建载体。由于ADH2被葡萄糖抑制,因此蛋白质的表达不会干扰发酵过程。具有载体pYGFP3的转化酵母显示出高稳定性和高生物发光性,从而可以在混合细胞群中鉴定标记细胞。该载体为开展进一步的研究提供了可能,目的是开发一种在工业发酵过程中早期检测腐败酵母的有效方法。

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    《Scientia Agricola》 |2000年第4期|共4页
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