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A reporter gene construct for studying the regulation of manganese peroxidase gene expression.

机译:用于研究锰过氧化物酶基因表达调控的报道基因构建体。

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摘要

The orotidylate decarboxylase (ODase) gene (ura1) from Schizophyllum commune was utilized as a reporter for studying Mn regulation of the manganese peroxidase (MnP) gene (mnp) from the lignin-degrading basidiomycete Phanerochaete chrysosporium. A 1,500-bp fragment of the mnp1 promoter was fused upstream of the coding region of the ODase gene in a plasmid (pAMO) containing the S. commune ade5 gene as a selectable marker. pAMO was used to transform a P. chrysosporium ade1 ura11 mutant lacking endogenous ODase activity. When the P. chrysosporium transformant was grown in nitrogen-limited, Mn(II)-sufficient cultures, ODase activity was detected only during secondary metabolic growth and the pattern of ODase expression was similar to that of endogenous MnP. When Mn was added to 6-day-old nitrogen-limited, Mn-deficient cultures, both ODase activity and MnP activity were induced synchronously with maximal activity at 30 h. Growth in high-nitrogen-concentration medium suppressed the induction of both the ODase and endogenous MnP. These results indicate that this promoter-reporter construct can be used to study the regulation of the mnp gene.
机译:Schizophyllum comorune的Orotidylate脱羧酶(ODase)基因(ura1)被用作报道分子,用于研究木质素降解的担子菌Phanerochaete chrysosporium的锰过氧化物酶(MnP)基因(mnp)的Mn调控。在含有S.commune ade5基因作为选择标记的质粒(pAMO)中,在ODase基因编码区的上游融合了一个1,500bp的mnp1启动子片段。 pAMO用于转化缺乏内源性ODase活性的金黄色葡萄球菌ade1 ura11突变体。当P. chrysosporium转化子在氮有限,Mn(II)充足的培养物中生长时,仅在二次代谢生长过程中才检测到ODase活性,并且ODase表达的模式与内源性MnP相似。当将锰添加到6天龄的缺氮,缺锰培养物中时,ODase活性和MnP活性都在30 h时以最大活性同步诱导。在高氮浓度培养基中的生长抑制了ODase和内源性MnP的诱导。这些结果表明,该启动子-报告子构建体可用于研究mnp基因的调控。

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