首页> 外文期刊>Applied and Environmental Microbiology >The cel3 gene of Agaricus bisporus codes for a modular cellulase and is transcriptionally regulated by the carbon source.
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The cel3 gene of Agaricus bisporus codes for a modular cellulase and is transcriptionally regulated by the carbon source.

机译:双孢蘑菇的cel3基因编码一种模块化的纤维素酶,并受碳源的转录调控。

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摘要

A 52-kDa protein, CEL3, has been separated from the culture filtrate of Agaricus bisporus during growth on cellulose. A PCR-derived probe was made, with a degenerate oligodeoxynucleotide derived from the amino acid sequence of a CEL3 CNBr cleavage product and was used to select cel3 cDNA clones from an A. bisporus cDNA library. Two allelic cDNAs were isolated. They showed 98.8% identity of their nucleotide sequences. The deduced amino acid sequence and domain architecture of CEL3 showed a high degree of similarity to those of cellobiohydrolase II of Trichoderma reesei. Functional expression of cel3 cDNA in Saccharomyces cerevisiae was achieved by placing it under the control of a constitutive promoter and fusing it to the yeast invertase signal sequence. Recombinant CEL3 secreted by yeast showed enzymatic activity towards crystalline cellulose. At long reaction times, CEL3 was also able to degrade carboxymethyl cellulose. Northern (RNA) analysis showed that cel3 gene expression was induced by cellulose and repressed by glucose, fructose, 2-deoxyglucose, and lactose. Glycerol, mannitol, sorbitol, and maltose were neutral carbon sources. Nuclear run-on analysis showed that the rate of synthesis of cel3 mRNA in cellulose-grown cultures was 13 times higher than that in glucose-grown cultures. A low basal rate of cel3 mRNA synthesis was observed in the nuclei isolated from glucose-grown mycelia.
机译:在纤维素上生长期间,已从双孢蘑菇的培养滤液中分离出52 kDa蛋白CEL3。用衍生自CEL3 CNBr裂解产物氨基酸序列的简并寡聚脱氧核苷酸制成PCR探针,并用于从双孢曲霉cDNA库中选择cel3 cDNA克隆。分离了两个等位基因cDNA。他们显示出98.8%的核苷酸序列同一性。推导的CEL3的氨基酸序列和结构域结构与里氏木霉的纤维二糖水解酶II具有高度相似性。 cel3 cDNA在啤酒酵母中的功能表达是通过将其置于组成型启动子的控制下并将其融合到酵母转化酶信号序列中来实现的。酵母分泌的重组CEL3对结晶纤维素表现出酶活性。在较长的反应时间下,CEL3还能够降解羧甲基纤维素。 Northern(RNA)分析表明,cel3基因表达被纤维素诱导,并被葡萄糖,果糖,2-脱氧葡萄糖和乳糖抑制。甘油,甘露醇,山梨糖醇和麦芽糖是中性碳源。核运行分析表明,纤维素生长培养物中cel3 mRNA的合成速率比葡萄糖生长培养物中的cel13 mRNA高13倍。在分离自葡萄糖生长的菌丝体的细胞核中观察到低的cel3 mRNA合成基础速率。

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