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首页> 外文期刊>Applied and Environmental Microbiology >Protease-mediated degradation of lignin peroxidase in liquid cultures of Phanerochaete chrysosporium.
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Protease-mediated degradation of lignin peroxidase in liquid cultures of Phanerochaete chrysosporium.

机译:蛋白酶介导的Phanerochaete chrysosporium液体培养物中木质素过氧化物酶的降解。

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摘要

The decline of lignin peroxidase (LiP) activity observed after day 6 in cultures of Phanerochaete chrysosporium was found to be correlated with the appearance of idiophasic extracellular protease activity. Daily addition of glucose started on day 6 resulted in low protease levels and in turn in stable LiP levels. Addition of cycloheximide to day 6 cultures resulted in virtually no change of LiP activity and extracellular protein and negligible levels of protease activity, indicating that this protease is synthesized de novo. LiP activity was found to be stable upon removal of the fungal pellets on day 6 and incubation of the extracellular fluid alone. An almost complete disappearance of LiP activity and LiP proteins and high levels of protease activity were observed upon incubation of 6-day extracellular fluid in the presence of fungal pellets. Moreover, incubation of crude or purified LiP isoenzymes with protease-rich extracellular fluid of day 11 or 11-day cell extracts resulted in a marked loss of activity. In contrast, incubation of crude LiP with boiled and clarified extracellular fluid of day 11 cultures resulted in virtually no loss of activity. These results indicate that protease-mediated degradation of LiP proteins is a major cause for the decay of LiP activity during late secondary metabolism in cultures of P. chrysosporium.
机译:发现在第6天后金黄色葡萄球菌培养物中观察到的木质素过氧化物酶(LiP)活性下降与特发性细胞外蛋白酶活性的出现有关。从第6天开始每天添加葡萄糖会导致蛋白酶水平降低,进而导致LiP稳定水平。在第6天的培养物中加入环己酰亚胺实际上导致LiP活性和细胞外蛋白无变化,蛋白酶活性水平可忽略不计,表明该蛋白酶是从头合成的。发现在第6天除去真菌沉淀并单独孵育细胞外液后,LiP活性稳定。在真菌沉淀存在下孵育6天的细胞外液后,观察到LiP活性和LiP蛋白质几乎完全消失,蛋白酶活性高水平。此外,将粗制或纯化的LiP同工酶与第11天或第11天细胞提取物的富含蛋白酶的细胞外液一起孵育会导致活性明显降低。相反,在第11天的培养中,将粗制的LiP与煮沸澄清的细胞外液一起孵育几乎不会导致活性降低。这些结果表明蛋白酶介导的LiP蛋白降解是在金孢假单胞菌培养物中后期次级代谢过程中LiP活性下降的主要原因。

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