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首页> 外文期刊>Applied and Environmental Microbiology >Copper Induction of Laccase Isoenzymes in the Ligninolytic Fungus Pleurotus ostreatus
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Copper Induction of Laccase Isoenzymes in the Ligninolytic Fungus Pleurotus ostreatus

机译:木质素分解菌平菇菌漆酶同工酶的铜诱导

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Pleurotus ostreatus is a white rot basidiomycete that produces several extracellular laccase isoenzymes, including phenol oxidase A1b (POXA1b), POXA2, and POXC. POXC was the most abundant isoenzyme produced under all of the growth conditions examined in this study. Copper was the most efficient inducer of laccase activity among the putative inducers tested. The amounts of all of the previously described laccase isoenzymes increased substantially in copper-supplemented cultures. Under these conditions expression of POX isoenzymes was regulated at the level of gene transcription. It is worth noting that poxa1b mRNA was the most abundant induced transcript at all of the growth times analyzed, and the amount of this mRNA increased until day 7. The discrepancy between thepoxa1b transcript and protein amounts can be explained by the presence of a high level of the protein in P. ostreatuscellular extract, which indicated that the POXA1b isoenzyme could be inefficiently secreted and/or that its physiological activity could occur inside the cell or on the cell wall. Moreover, the POXA1b isoenzyme behaved uniquely, as its activity was maximal on the second day of growth and then decreased. An analysis performed with protease inhibitors revealed that the loss of extracellular POXA1b activity could have been due to the presence of specific proteases secreted into the copper-containing culture medium that affected the extracellular POXA1b isoenzyme.
机译:平菇是一种白色腐烂的担子菌,可产生几种细胞外漆酶同工酶,包括酚氧化酶A1b(POXA1b),POXA2和POXC。 POXC是在本研究中考察的所有生长条件下产生的最丰富的同工酶。铜是公认的漆酶活性最有效的诱导剂。在铜补充的培养物中,所有上述漆酶同工酶的量均显着增加。在这些条件下,POX同工酶的表达在基因转录水平上受到调节。值得注意的是,在所有分析的生长时间中,poxa1b mRNA是最丰富的诱导转录本,并且该mRNA的量一直增加到第7天。popoa1b转录本与蛋白质量之间的差异可以通过高水平的存在来解释。的研究表明,POXA1b同工酶可能被低效率地分泌,并且/或者其生理活性可能在细胞内或细胞壁上发生。此外,POXA1b同工酶表现独特,因为其活性在生长的第二天达到最大,然后下降。用蛋白酶抑制剂进行的分析表明,胞外POXA1b活性的丧失可能是由于分泌到含铜培养基中的特定蛋白酶的存在影响了胞外POXA1b同工酶。

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