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海洋硅藻三角褐指藻中具有 CREB/ATF 样基本拉链结构域的转录因子靶向的 CO(2)-cAMP 反应性顺式元件。

CO(2)-cAMP-responsive cis-elements targeted by a transcription factor with CREB/ATF-like basic zipper domain in the marine diatom Phaeodactylum tricornutum.

机构信息

Research Center for Environmental Bioscience, Department of Bioscience, Kwansei-Gakuin University, Sanda, Hyogo 669-1337, Japan.

出版信息

Plant Physiol. 2012 Jan;158(1):499-513. doi: 10.1104/pp.111.190249. Epub 2011 Nov 17.

Abstract

Expression controls of the carbon acquisition system in marine diatoms in response to environmental factors are an essential issue to understand the changes in marine primary productivity. A pyrenoidal β-carbonic anhydrase, PtCA1, is one of the most important candidates to investigate the control mechanisms of the CO(2) acquisition system in the marine diatom Phaeodactylum tricornutum. A detailed functional assay was carried out on the putative core regulatory region of the ptca1 promoter using a β-glucuronidase reporter in P. tricornutum cells under changing CO(2) conditions. A set of loss-of-function assays led to the identification of three CO(2)-responsive elements, TGACGT, ACGTCA, and TGACGC, at a region -86 to -42 relative to the transcription start site. Treatment with a cyclic (c)AMP analog, dibutyryl cAMP, revealed these three elements to be under the control of cAMP; thus, we designated them, from 5' to 3', as CO(2)-cAMP-Responsive Element1 (CCRE1), CCRE2, and CCRE3. Because the sequence TGACGT is known to be a typical target of human Activating Transcription Factor6 (ATF6), we searched for genes containing a basic zipper (bZIP) region homologous to that of ATF6 in the genome of P. tricornutum. Gel-shift assays using CCRE pentamers as labeled probes showed that at least one candidate of bZIP proteins, PtbZIP11, bound specifically to CCREs. A series of gain-of-function assays with CCREs fused to a minimal promoter strongly suggested that the alternative combination of CCRE1/2 or CCRE2/3 at proper distances from the minimal promoter is required as a potential target of PtbZIP11 for an effective CO(2) response of the ptca1 gene.

摘要

海洋硅藻中碳获取系统对环境因子的表达调控是理解海洋初级生产力变化的一个重要问题。一个石碳酸酐酶,PtCA1,是研究海洋硅藻三角褐指藻 CO2 摄取系统调控机制的重要候选蛋白之一。我们在三角褐指藻细胞中,通过β-葡萄糖醛酸酶报告基因,对 PtCA1 启动子的假定核心调控区进行了详细的功能分析,同时改变 CO2 条件。一系列功能丧失实验鉴定了三个 CO2 响应元件,TGACGT、ACGTCA 和 TGACGC,位于转录起始位点前 -86 至 -42 位。环磷酸腺苷(cAMP)类似物二丁酰环磷酸腺苷(db-cAMP)的处理表明这三个元件受 cAMP 调控;因此,我们将它们从 5'到 3'命名为 CO2-cAMP-Responsive Element1(CCRE1)、CCRE2 和 CCRE3。由于 TGACGT 序列是人类激活转录因子 6(ATF6)的典型靶标,我们在三角褐指藻基因组中搜索了含有与 ATF6 同源的碱性拉链(bZIP)区域的基因。使用 CCRE 五聚体作为标记探针的凝胶迁移实验表明,至少有一种 bZIP 蛋白候选物 PtbZIP11 特异性结合 CCREs。一系列与最小启动子融合的 CCRE 功能获得实验强烈表明,适当距离的 CCRE1/2 或 CCRE2/3 的替代组合是 PtbZIP11 作为 PtCA1 基因有效 CO2 响应的潜在靶标所必需的。

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