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Regulation of Gene Expression in Neurospora crassa with a Copper Responsive Promoter

机译:铜响应启动子调控神经孢菌中基因表达的调控

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Precise control of gene expression is a powerful method to elucidate biological function, and protein overexpression is an important tool for industry and biochemistry. Expression of the Neurospora crassa tcu-1 gene (NCU00830), encoding a high-affinity copper transporter, is tightly controlled by copper availability. Excess copper represses, and copper depletion, via the use of a copper chelator, activates expression. The kinetics of induction and repression of tcu-1 are rapid, and the effects are long lived. We constructed a plasmid carrying the bar gene (for glufosinate selection) fused to the tcu-1 promoter. This plasmid permits the generation of DNA fragments that can direct integration of P tcu-1 into any desired locus. We use this strategy to integrate P tcu-1 in front of wc-1 , a circadian oscillator and photoreceptor gene. The addition of excess copper to the P tcu-1 :: wc-1 strain phenocopies a Δwc-1 strain, and the addition of the copper chelator, bathocuproinedisulfonic acid, phenocopies a wc-1 overexpression strain. To test whether copper repression can recapitulate the loss of viability that an essential gene knockout causes, we placed P tcu-1 upstream of the essential gene, hpt-1 . The addition of excess copper drastically reduced the growth rate as expected. Thus, this strategy will be useful to probe the biological function of any N. crassa gene through controlled expression.
机译:精确控制基因表达是阐明生物学功能的有力方法,蛋白质过表达是工业和生物化学的重要工具。编码高亲和力铜转运蛋白的Crus Neurospora crassa tcu-1基因(NCU00830)的表达受到铜可用性的严格控制。过量的铜抑制和铜耗尽通过使用铜螯合剂激活表达。 tcu-1的诱导和抑制动力学是迅速的,并且作用是长期的。我们构建了携带与tcu-1启动子融合的bar基因(用于草铵膦选择)的质粒。该质粒允许生成可指导P tcu-1整合到任何所需基因座中的DNA片段。我们使用这种策略在wc-1,昼夜节律振荡器和感光基因之前整合P tcu-1。向P tcu-1 :: wc-1菌株中添加过量的铜表型复制了Δwc-1菌株,并且向铜螯合剂,浴铜基二磺酸添加了表型复制了wc-1过表达菌株。为了测试铜抑制是否可以概括必需基因敲除导致的生存力丧失,我们将P tcu-1置于必需基因hpt-1的上游。多余的铜的添加极大地降低了预期的增长率。因此,该策略将可用于通过受控表达来探测任何克雷萨氏猪笼草基因的生物学功能。

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