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Characterization of serine proteinase expression in agaricus bisporus and coprinopsis cinerea by using green fluorescent protein and the A. bisporus SPR1 Promoter

机译:通过使用绿色荧光蛋白和双孢曲霉SPR1启动子表征双孢蘑菇和灰霉菌中丝氨酸蛋白酶的表达

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摘要

The Agaricus bisporus serine proteinase 1 (SPR1) appears to be significant in both mycelial nutrition and senescence of the fruiting body. We report on the construction of an SPR promoter::green fluorescent protein (GFP) fusion cassette, pGreen_hph1_SPR_GFP, for the investigation of temporal and developmental expression of SPR1 in homobasidiomycetes and to determine how expression is linked to physiological and environmental stimuli. Monitoring of A. bisporus pGreen_hph1_SPR_GFP transformants on media rich in ammonia or containing different nitrogen sources demonstrated that SPR1 is produced in response to available nitrogen. In A. bisporus fruiting bodies, GFP activity was localized to the stipe of postharvest senescing sporophores. pGreen_hph1_SPR_GFP was also transformed into the model basidiomycete Coprinopsis cinerea. Endogenous C. cinerea proteinase activity was profiled during liquid culture and fruiting body development. Maximum activity was observed in the mature cap, while activity dropped during autolysis. Analysis of the C. cinerea genome revealed seven genes showing significant homology to the A. bisporus SPR1 and SPR2 genes. These genes contain the aspartic acid, histidine, and serine residues common to serine proteinases. Analysis of the promoter regions revealed at least one CreA and several AreA regulatory motifs in all sequences. Fruiting was induced in C. cinerea dikaryons, and fluorescence was determined in different developmental stages. GFP expression was observed throughout the life cycle, demonstrating that serine proteinase can be active in all stages of C. cinerea fruiting body development. Serine proteinase expression (GFP fluorescence) was most concentrated during development of young tissue, which may be indicative of high protein turnover during cell differentiation
机译:双孢蘑菇丝氨酸蛋白酶1(SPR1)在菌丝营养和子实体的衰老中均具有重要意义。我们报告的SPR启动子::绿色荧光蛋白(GFP)融合盒,pGreen_hph1_SPR_GFP的建设,以调查同型单胞菌中SPR1的时间和发育表达,并确定表达如何与生理和环境刺激联系起来。在富含氨气或包含不同氮源的培养基上对双孢曲霉pGreen_hph1_SPR_GFP转化子的监测表明,SPR1是对可用氮的响应而产生的。在双孢蘑菇的子实体中,GFP活性位于收获后衰老的孢子体的柄上。 pGreen_hph1_SPR_GFP也被转化为灰葡萄孢菌的模型。在液体培养和子实体发育过程中分析了内源灰质曲霉的蛋白酶活性。在成熟帽中观察到最大活性,而在自溶过程中活性下降。对灰葡萄孢菌基因组的分析揭示了七个与双孢曲霉SPR1和SPR2基因显示出显着同源性的基因。这些基因含有丝氨酸蛋白酶常见的天冬氨酸,组氨酸和丝氨酸残基。启动子区域的分析揭示了在所有序列中至少一个CreA和几个AreA调节基序。在灰葡萄双核果中诱导结果,并在不同的发育阶段测定荧光。在整个生命周期中都观察到了GFP的表达,这表明丝氨酸蛋白酶可以在灰葡萄孢子实体发育的所有阶段中发挥作用。丝氨酸蛋白酶的表达(GFP荧光)在年轻组织的发育过程中最集中,这可能表明细胞分化过程中蛋白质的高转换

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