工程黑曲霉的胞外分泌物以从植物生物质生产纤维寡糖。
Engineering the secretome of Aspergillus niger for cellooligosaccharides production from plant biomass.
机构信息
Laboratory of Enzymology and Molecular Biology of Microorganisms (LEBIMO), Department of Biochemistry and Tissue Biology, Institute of Biology, Universidade Estadual de Campinas (UNICAMP), Campinas, SP, 13083-862, Brazil.
Department of Biotechnology and Biomedicine, Technical University of Denmark (DTU), Søltofts Plads, Building 223, Kongens Lyngby, 2800, Denmark.
出版信息
Microb Cell Fact. 2024 Nov 29;23(1):323. doi: 10.1186/s12934-024-02578-9.
BACKGROUND
Fermentation of sugars derived from plant biomass feedstock is crucial for sustainability. Hence, utilizing customized enzymatic cocktails to obtain oligosaccharides instead of monomers is an alternative fermentation strategy to produce prebiotics, cosmetics, and biofuels. This study developed an engineered strain of Aspergillus niger producing a tailored cellulolytic cocktail capable of partially degrading sugarcane straw to yield cellooligosaccharides.
RESULTS
The A. niger prtT∆ strain created resulted in a reduced extracellular protease production. The prtT∆ background was then used to create strains by deleting exoenzyme encoding genes involved in mono- or disaccharide formation. Consequently, we successfully generated a tailored prtT∆bglA∆ strain by eliminating a beta-glucosidase (bglA) gene and subsequently deleted two cellobiohydrolases and one beta-xylosidase encoding genes using a multiplex strategy, resulting in the Quintuple∆ strain (prtT∆; bglA∆; cbhA∆; cbhB∆; xlnD∆). When applied for sugarcane biomass degradation, the tailored secretomes produced by A. niger resulted in a higher ratio of cellobiose and cellotriose compared with glucose relative to the reference strain. Mass spectrometry revealed that the Quintuple∆ strain secreted alternative cellobiohydrolases and beta-glucosidases to compensate for the absence of major cellulases. Enzymes targeting minor polysaccharides in plant biomass were also upregulated in this tailored strain.
CONCLUSION
Tailored secretome use increased COS/glucose ratio during sugarcane biomass degradation showing that deleting some enzymatic components is an effective approach for producing customized enzymatic cocktails. Our findings highlight the plasticity of fungal genomes as enzymes that target minor components of plant cell walls, and alternative cellulases were produced by the mutant strain. Despite deletion of important secretome components, fungal growth was maintained in plant biomass.
背景
利用植物生物质原料中的糖进行发酵对于可持续性至关重要。因此,利用定制的酶混合物获得低聚糖而不是单体是一种替代发酵策略,可以用于生产益生元、化妆品和生物燃料。本研究开发了一种产黑曲霉工程菌株,能够产生定制的纤维素酶混合物,部分降解甘蔗秸秆以生成纤维寡糖。
结果
创建的 A. niger prtT∆ 菌株导致细胞外蛋白酶的产生减少。然后,在 prtT∆ 背景下,通过删除参与单糖或二糖形成的外切酶编码基因来创建菌株。因此,我们成功地通过消除一个β-葡萄糖苷酶(bglA)基因生成了定制的 prtT∆bglA∆ 菌株,然后使用多重策略删除了两个纤维二糖水解酶和一个β-木糖苷酶编码基因,得到 Quintuple∆ 菌株(prtT∆;bglA∆;cbhA∆;cbhB∆;xlnD∆)。当应用于甘蔗生物质降解时,与参考菌株相比,产黑曲霉产生的定制分泌酶导致相对于葡萄糖,纤维二糖和纤维三糖的比例更高。质谱分析表明,Quintuple∆ 菌株分泌替代的纤维二糖水解酶和β-葡萄糖苷酶来弥补主要纤维素酶的缺失。这种定制菌株中还上调了针对植物生物质中小多糖的酶。
结论
定制分泌酶的使用提高了甘蔗生物质降解过程中的 COS/葡萄糖比率,表明删除一些酶成分是生产定制酶混合物的有效方法。我们的研究结果强调了真菌基因组的可塑性,因为酶可以靶向植物细胞壁的次要成分,并且突变菌株产生了替代的纤维素酶。尽管删除了重要的分泌酶成分,但真菌在植物生物质中的生长仍得到维持。
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