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Improved secretory expression of lignocellulolytic enzymes in Kluyveromyces marxianus by promoter and signal sequence engineering

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바이오화학분류
    • 바이오플라스틱
      1. 플라스틱
    • 바이오정밀화학
      1. 용매
      2. 화학제품
      3. 연료
    • 화장품용 기능성소재
      1. 계면활성제⁄증점제
    • 의료용 화학소재
      1. 식품첨가제
논문

Improved secretory expression of lignocellulolytic enzymes in Kluyveromyces marxianus by promoter and signal sequence engineering

학술지

Biotechnology for biofuels

저자명

Zhou, Jungang; Zhu, Peixia; Hu, Xiaoyue; Lu, Hong; Yu, Yao

초록

<P><B>Background</B></P><P>Taking into account its thermotolerance, high growth rate, and broad substrate spectrum, <I>Kluyveromyces marxianus</I> can be considered an ideal consolidated bioprocessing (CBP). A major obstacle to ethanol production using <I>K. marxianus</I> is the low production of lignocellulolytic enzymes, which reduces the cellulose hydrolysis and ethanol production. Thus, further improvement of enzyme expression and secretion is essential.</P><P><B>Results</B></P><P>To improve the expression of lignocellulolytic enzymes, the inulinase promoter and signal sequence from <I>K. marxianus</I> was optimized through mutagenesis. A T(-361)A mutation inside the promoter, a deletion of AT-rich region inside 5′UTR (UTR&#x2206;A), and a P10L substitution in the signal sequence increased the secretory expression of the feruloyl esterase Est1E by up to sixfold. T(-361)A and UTR&#x2206;A increased the mRNA expression, while the P10L substitution extended the hydrophobic core of signal sequence and promoted secretion of mature protein. P10L and T(-361)A mutations increased secretory expressions of other types of lignocellulolytic enzymes by up to threefold, including endo-1,4-&beta;-glucanase RuCelA, endo-1,4-&beta;-endoxylanase Xyn-CDBFV, and endo-1,4-&beta;-mannanase MAN330. During the fed-batch fermentation of strains carrying optimized modules, the peak activities of RuCelA, Xyn-CDBFV, MAN330, and Est1E reached 24&nbsp;U/mL, 25,600&nbsp;U/mL, 10,200&nbsp;U/mL, and 1220&nbsp;U/mL, respectively. Importantly, higher yield of enzymes by optimized promoter and signal sequence were achieved in all tested carbon sources, including the major end products of lignocellulose saccharification and fermentation, with growth on xylose resulting in the highest production.</P><P><B>Conclusions</B></P><P>The engineered promoter and signal sequence presented increased secretory expressions of different lignocellulolytic enzymes in <I>K. marxianus</I> by means of various carbon resources. Activities of lignocellulolytic enzymes in fed-batch fermentation were the highest activities reported for <I>K. marxianus</I> so far. Our engineered modules are valuable in producing lignocellulolytic enzymes by <I>K. marxianus</I> and in constructing efficient CBP strains for cellulosic ethanol production.</P><P><B>Electronic supplementary material</B></P><P>The online version of this article (10.1186/s13068-018-1232-7) contains supplementary material, which is available to authorized users.</P>

발행연도

2018

발행기관

BioMed Central

라이선스

cc-by

ISSN

1754-6834

11

페이지

pp.235

주제어

Kluyveromyces marxianus; Inulinase; Lignocellulolytic enzymes; Signal sequence; Promoter optimization

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1 2023-12-11

논문; 2018-08-29

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