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一种氰酶受精氨酸转录调控,并参与大孢粪壳菌中的氰酸盐分解。

A cyanase is transcriptionally regulated by arginine and involved in cyanate decomposition in Sordaria macrospora.

作者信息

Elleuche Skander, Pöggeler Stefanie

机构信息

Institute of Microbiology and Genetics, Department of Genetics of Eukaryotic Microorganisms, Georg-August University, Grisebachstr. 8, D-37077 Göttingen, Germany.

出版信息

Fungal Genet Biol. 2008 Nov;45(11):1458-69. doi: 10.1016/j.fgb.2008.08.005. Epub 2008 Aug 29.

Abstract

Cyanase degrades toxic cyanate to NH3 and CO2 in a bicarbonate-dependent reaction. High concentrations of cyanate are fairly toxic to organisms. Here, we characterize a eukaryotic cyanase for the first time. We have isolated the cyn1 gene encoding a cyanase from the filamentous ascomycete Sordaria macrospora and functionally characterized the cyn1 product after heterologous expression in Escherichia coli. Site-directed mutagenesis confirmed a predicted catalytic centre of three conserved amino-acids. A Deltacyn1 knockout in S. macrospora was totally devoid of cyanase activity and showed an increased sensitivity to exogenously supplied cyanate in an arginine-depleted medium, defects in ascospore germination, but no other obvious morphological phenotype. By means of real-time PCR we have demonstrated that the transcriptional level of cyn1 is markedly elevated in the presence of cyanate and down-regulated by addition of arginine. The putative functions of cyanase in fungi are discussed.

摘要

氰酸酶在依赖碳酸氢盐的反应中将有毒的氰酸盐降解为NH₃和CO₂。高浓度的氰酸盐对生物体具有相当大的毒性。在此,我们首次对一种真核生物氰酸酶进行了表征。我们从丝状子囊菌大孢粪壳菌中分离出编码氰酸酶的cyn1基因,并在大肠杆菌中进行异源表达后对cyn1产物进行了功能表征。定点诱变证实了由三个保守氨基酸组成的预测催化中心。大孢粪壳菌中的Δcyn1基因敲除完全没有氰酸酶活性,并且在精氨酸耗尽的培养基中对外源提供的氰酸盐表现出更高的敏感性,在子囊孢子萌发方面存在缺陷,但没有其他明显的形态学表型。通过实时PCR我们证明,在存在氰酸盐的情况下,cyn1的转录水平显著升高,而添加精氨酸后则下调。文中讨论了氰酸酶在真菌中的假定功能。

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