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纤维二糖对嗜热栖热放线菌celC操纵子的诱导作用。

Induction of the celC operon of Clostridium thermocellum by laminaribiose.

作者信息

Newcomb Michael, Chen Chun-Yu, Wu J H David

机构信息

Department of Chemical Engineering, University of Rochester, Rochester, NY 14627-0166, USA.

出版信息

Proc Natl Acad Sci U S A. 2007 Mar 6;104(10):3747-52. doi: 10.1073/pnas.0700087104. Epub 2007 Feb 27.

Abstract

Clostridium thermocellum is an anaerobic, thermophilic, cellulolytic, and ethanogenic bacterium. It produces an extracellular multiprotein complex termed the cellulosome, which consists of >70 subunits, most of them glycosyl hydrolases. It also produces many free glycosyl hydrolases. How the organism commands such a large number of genes and proteins for biomass degradation is an intriguing yet unresolved question. We identified glyR3, which is cotranscribed with the cellulase/hemicellulase genes celC and licA, as a potential cellulase transcription regulator. The gel-shift assay (EMSA) revealed that the recombinant GlyR3 bound specifically to the celC promoter region. GlyR3 was also identified from the lysate of the lichenan-grown cells, which bound to the same sequence. DNase I footprinting and competitive EMSA showed the binding site to be an 18-bp palindromic sequence with one mismatch. The DNA-binding activity was specifically inhibited by laminaribiose, a beta-1-3 linked glucose dimer, in a dose-dependent manner. In in vitro transcription analysis, celC expression was repressed by rGlyR3 in a dose-dependent manner. The repression was relieved by laminaribiose, also in a dose-dependent manner. These results indicate that GlyR3 is a negative regulator of the celC operon consisting of celC, glyR3, and licA, and inducible by laminaribiose. Thus, the bacterium may modulate the biosynthesis of its enzyme components to optimize its activity on an available biomass substrate, in this case, beta-1-3 glucan, because both CelC and LicA are active on the substrate. The results further indicate that, despite the insolubility of the biomass substrate, regulation of the degradative enzymes can be accomplished through soluble sugars generated by the action of the enzymes.

摘要

嗜热栖热菌是一种厌氧、嗜热、能分解纤维素并产乙醇的细菌。它产生一种称为纤维小体的细胞外多蛋白复合物,该复合物由70多个亚基组成,其中大多数是糖基水解酶。它还产生许多游离的糖基水解酶。该生物体如何调控如此大量的基因和蛋白质来进行生物质降解,是一个引人入胜但尚未解决的问题。我们鉴定出与纤维素酶/半纤维素酶基因celC和licA共转录的glyR3,它是一种潜在的纤维素酶转录调节因子。凝胶迁移试验(EMSA)表明,重组的GlyR3特异性结合celC启动子区域。从地衣聚糖培养细胞的裂解物中也鉴定出GlyR3,它能结合相同的序列。DNA酶I足迹法和竞争性EMSA表明,结合位点是一个有一个错配的18碱基对回文序列。层叠寡糖(一种β-1,3连接的葡萄糖二聚体)以剂量依赖的方式特异性抑制DNA结合活性。在体外转录分析中,rGlyR3以剂量依赖的方式抑制celC表达。层叠寡糖也以剂量依赖的方式缓解这种抑制。这些结果表明,GlyR3是由celC、glyR3和licA组成的celC操纵子的负调节因子,可被层叠寡糖诱导。因此,该细菌可能会调节其酶组分的生物合成,以优化其在可用生物质底物上的活性,在这种情况下是β-1,3葡聚糖,因为CelC和LicA对该底物都有活性。结果还进一步表明,尽管生物质底物不溶性,但降解酶的调节可以通过酶作用产生的可溶性糖来实现。

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