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High copy and stable expression of the xylanase XynHB in Saccharomyces cerevisiae by rDNA-mediated integration

机译:木糖酶XynHB在酿酒酵母中的高拷贝和稳定表达通过rDNA介导的整合

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摘要

Xylanase is a widely-used additive in baking industry for enhancing dough and bread quality. Several xylanases used in baking industry were expressed in different systems, but their expression in antibiotic free vector system is highly essential and safe. In the present study, an alternative rDNA-mediated technology was developed to increase the copy number of target gene by integrating it into Saccharomyces cerevisiae genome. A xylanase-encoding gene xynHB from Bacillus sp. was cloned into pHBM367H and integrated into S. cerevisiae genome through rDNA-mediated recombination. Exogenous XynHB expressed by recombinant S. cerevisiae strain A13 exhibited higher degradation activity towards xylan than other transformants. The real-time PCR analysis on A13 genome revealed the presence of 13.64 copies of xynHB gene. Though no antibiotics have been used, the genetic stability and the xylanase activity of xynHB remained stable up to 1,011 generations of cultivation. S. cerevisiae strain A13 expressing xylanase reduced the required kneading time and increased the height and diameter of the dough size, which would be safe and effective in baking industry as no antibiotics-resistance risk. The new effective rDNA-mediated technology without using antibiotics here provides a way to clone other food related industrial enzymes for applications.
机译:木聚糖酶是烘焙行业中广泛使用的添加剂,可增强面团和面包的质量。烘焙工业中使用的几种木聚糖酶在不同的系统中表达,但是它们在无抗生素载体系统中的表达是高度必要和安全的。在本研究中,开发了一种替代性的rDNA介导技术,通过将其整合到啤酒酵母基因组中来增加目标基因的拷贝数。来自芽孢杆菌属的木聚糖酶编码基因xynHB。将其克隆到pHBM367H中,并通过rDNA介导的重组整合到酿酒酵母基因组中。由重组啤酒酵母菌株A13表达的外源XynHB表现出比其他转化体更高的对木聚糖的降解活性。对A13基因组的实时PCR分析显示存在13.64个拷贝的xynHB基因。尽管没有使用抗生素,但xynHB的遗传稳定性和木聚糖酶活性在1,011代的培养过程中仍保持稳定。表达木聚糖酶的酿酒酵母菌株A13减少了所需的捏合时间,并增加了面团尺寸的高度和直径,由于没有抗药性风险,因此在烘焙行业中是安全有效的。无需使用抗生素的新型有效rDNA介导技术在这里提供了一种克隆其他与食品相关的工业酶以进行应用的方法。

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