Neumann Anthony P, Weimer Paul J, Suen Garret
1Department of Bacteriology, University of Wisconsin-Madison, Madison, WI USA.
2Agricultural Research Service, United States Department of Agriculture, Madison, WI USA.
Biotechnol Biofuels. 2018 Oct 27;11:295. doi: 10.1186/s13068-018-1290-x. eCollection 2018.
Cellulose is the most abundant biological polymer on earth, making it an attractive substrate for the production of next-generation biofuels and commodity chemicals. However, the economics of cellulose utilization are currently unfavorable due to a lack of efficient methods for its hydrolysis. strain S85, originally isolated from the bovine rumen, is among the most actively cellulolytic mesophilic bacteria known, producing succinate as its major fermentation product. In this study, we examined the transcriptome of S85 grown in continuous culture at several dilution rates on cellulose, cellobiose, or glucose to gain a system-level understanding of cellulose degradation by this bacterium.
Several patterns of gene expression were observed for the major cellulases produced by S85. A large proportion of cellulase genes were constitutively expressed, including the gene encoding for Cel51A, the major cellulose-binding endoglucanase produced by this bacterium. Moreover, other cellulase genes displayed elevated expression during growth on cellulose relative to growth on soluble sugars. Growth rate had a strong effect on global gene expression, particularly with regard to genes predicted to encode carbohydrate-binding modules and glycoside hydrolases implicated in hemicellulose degradation. Expression of hemicellulase genes was tightly regulated, with these genes displaying elevated expression only during slow growth on soluble sugars. Clear differences in gene expression were also observed between adherent and planktonic populations within continuous cultures growing on cellulose.
This work emphasizes the complexity of the fiber-degrading system utilized by S85, and reinforces the complementary role of hemicellulases for accessing cellulose by these bacteria. We report for the first time evidence of global differences in gene expression between adherent and planktonic populations of an anaerobic bacterium growing on cellulose at steady state during continuous cultivation. Finally, our results also highlight the importance of controlling for growth rate in investigations of gene expression.
纤维素是地球上最丰富的生物聚合物,使其成为生产下一代生物燃料和商品化学品的有吸引力的底物。然而,由于缺乏有效的纤维素水解方法,目前纤维素利用的经济性不佳。菌株S85最初从牛瘤胃中分离出来,是已知最活跃的纤维素分解嗜温细菌之一,其主要发酵产物为琥珀酸。在本研究中,我们检测了S85在连续培养中以几种稀释率在纤维素、纤维二糖或葡萄糖上生长时的转录组,以从系统水平了解该细菌对纤维素的降解。
观察到S85产生的主要纤维素酶有几种基因表达模式。很大一部分纤维素酶基因是组成型表达的,包括编码Cel51A的基因,Cel51A是该细菌产生的主要纤维素结合内切葡聚糖酶。此外,相对于在可溶性糖上生长,其他纤维素酶基因在纤维素上生长期间表达升高。生长速率对全局基因表达有很强的影响,特别是对于预测编码参与半纤维素降解的碳水化合物结合模块和糖苷水解酶的基因。半纤维素酶基因的表达受到严格调控,这些基因仅在以可溶性糖缓慢生长期间表达升高。在以纤维素为生长底物的连续培养物中,附着群体和浮游群体之间也观察到明显的基因表达差异。
这项工作强调了S85利用的纤维降解系统的复杂性,并强化了半纤维素酶对这些细菌获取纤维素的互补作用。我们首次报道了在连续培养期间,厌氧细菌在纤维素上稳定生长时,附着群体和浮游群体之间基因表达存在全局差异的证据。最后,我们的结果还突出了在基因表达研究中控制生长速率的重要性。
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