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首页> 外文期刊>Eukaryotic cell >Copper Response Element and Crr1-Dependent Ni2+-Responsive Promoter for Induced, Reversible Gene Expression in Chlamydomonas reinhardtii
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Copper Response Element and Crr1-Dependent Ni2+-Responsive Promoter for Induced, Reversible Gene Expression in Chlamydomonas reinhardtii

机译:铜响应元件和依赖Crr1的Ni2 +响应启动子在莱茵衣藻中诱导,可逆的基因表达。

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The Cpx1 and Cyc6 genes of Chlamydomonas reinhardtii are activated in copper-deficient cells via a signal transduction pathway that requires copper response elements (CuREs) and a copper response regulator defined by the CRR1 locus. The two genes can also be activated by provision of nickel or cobalt ions in the medium. The response to nickel ions requires at least one CuRE and also CRR1 function, suggesting that nickel interferes with a component in the nutritional copper signal transduction pathway. Nickel does not act by preventing copper uptake/utilization because (i) holoplastocyanin formation is unaffected in Ni2+-treated cells and (ii) provision of excess copper cannot reverse the Ni-dependent activation of the target genes. The CuRE is sufficient for conferring Ni-responsive expression to a reporter gene, which suggests that the system has practical application as a vehicle for inducible gene expression. The inducer can be removed either by replacing the medium or by chelating the inducer with excess EDTA, either of which treatments reverses the activation of the target genes.
机译:弱衣藻的 Cpx1 Cyc6 基因在缺铜细胞中通过信号传导途径被激活,该信号传导途径需要铜反应元件(CuREs)和由 CRR1 基因座定义的铜响应调节剂。还可以通过在培养基中提供镍或钴离子来激活这两个基因。对镍离子的响应需要至少一种CuRE以及 CRR1 功能,这表明镍会干扰营养铜信号传导途径中的一种成分。镍不能通过阻止铜的吸收/利用来起作用,因为(i)整体质蓝蛋白的形成在Ni 2 + 处理的细胞中不受影响,并且(ii)提供过量的铜不能逆转靶标的Ni依赖性活化基因。 CuRE足以赋予报告基因Ni响应性表达,这表明该系统作为诱导型基因表达的载体具有实际应用。可以通过替换培养基或通过用过量的EDTA螯合诱导剂来去除诱导剂,这两种方法都可以逆转靶基因的激活。

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