4.3 Article

A Kluyveromyces marxianus 2-deoxyglucose-resistant mutant with enhanced activity of xylose utilization

期刊

INTERNATIONAL MICROBIOLOGY
卷 18, 期 4, 页码 235-244

出版社

INST ESTUDIS CATALANS
DOI: 10.2436/20.1501.01.255

关键词

Kluyveromyces marxianus; glucose repression; 2-deoxyglucose-resistant mutants; ethanol fermentation on xylose; thermotolerant yeast

资金

  1. Directorate General of Resources for Science, Technology and Higher Education (DIKTI) scholarship
  2. Ministry of Research, Technology and Higher Education of Indonesia
  3. Brawijaya University, Indonesia
  4. Special Coordination Funds for Promoting Science Technology
  5. Ministry of Education, Culture, Sports, Science Technology
  6. Advanced Low Carbon Technology Research and Development Program, Japan Science and Technology Agency

向作者/读者索取更多资源

Thermotolerant ethanologenic yeast Kluyveromyces marxianus is capable of fermenting various sugars including xylose but glucose represses to hamper the utilization of other sugars. To acquire glucose repression-defective strains, 33 isolates as 2-deoxyglucose (2-DOG)-resistant mutants were acquired from about 100 colonies grown on plates containing 2-DOG, which were derived from an efficient strain DMKU 3-1042. According to the characteristics of sugar consumption abilities and cell growth and ethanol accumulation along with cultivation time, they were classified into three groups. The first group (3 isolates) utilized glucose and xylose in similar patterns along with cultivation to those of the parental strain, presumably due to reduction of the uptake of 2-DOG or enhancement of its export. The second group (29 isolates) showed greatly delayed utilization of glucose, presumably by reduction of the uptake or initial catabolism of glucose. The last group, only one isolate, showed enhanced utilization ability of xylose in the presence of glucose. Further analysis revealed that the isolate had a single nucleotide mutation to cause amino acid substitution (G270S) in RAG5 encoding hexokinase and exhibited very low activity of the enzyme. The possible mechanism of defectiveness of glucose repression in the mutant is discussed in this paper.

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