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Production of Xylitol from d-Xylose by a Xylitol Dehydrogenase Gene-Disrupted Mutant of Candida tropicalis

机译:由木糖醇脱氢酶基因破坏的热带念珠菌突变体从d-木糖生产木糖醇

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摘要

Xylitol dehydrogenase (XDH) is one of the key enzymes in d-xylose metabolism, catalyzing the oxidation of xylitol to d-xylulose. Two copies of the XYL2 gene encoding XDH in the diploid yeast Candida tropicalis were sequentially disrupted using the Ura-blasting method. The XYL2-disrupted mutant, BSXDH-3, did not grow on a minimal medium containing d-xylose as a sole carbon source. An enzyme assay experiment indicated that BSXDH-3 lost apparently all XDH activity. Xylitol production by BSXDH-3 was evaluated using a xylitol fermentation medium with glucose as a cosubstrate. As glucose was found to be an insufficient cosubstrate, various carbon sources were screened for efficient cofactor regeneration, and glycerol was found to be the best cosubstrate. BSXDH-3 produced xylitol with a volumetric productivity of 3.23 g liter−1 h−1, a specific productivity of 0.76 g g−1 h−1, and a xylitol yield of 98%. This is the first report of gene disruption of C. tropicalis for enhancing the efficiency of xylitol production.
机译:木糖醇脱氢酶(XDH)是D-木糖代谢中的关键酶之一,催化木糖醇氧化为D-木酮糖。使用Ura-blasting方法依次破坏了二倍体酵母热带假丝酵母中编码XDH的XYL2基因的两个副本。 XYL2中断的突变体BSXDH-3,没有在含有d-木糖作为唯一碳源的基本培养基上生长。酶分析实验表明,BSXDH-3显然丧失了所有XDH活性。使用木糖醇发酵培养基,以葡萄糖作为共底物,评估了BSXDH-3产生的木糖醇。由于发现葡萄糖不足以形成辅助底物,因此筛选了各种碳源以进行有效的辅因子再生,并且发现甘油是最好的辅助底物。 BSXDH-3生产的木糖醇的容积生产率为3.23 g升 -1 h -1 ,比生产率为0.76 gg -1 h < sup> -1 ,木糖醇收率为98%。这是首次报道了热带假丝酵母基因破坏以提高木糖醇生产效率的报道。

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