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玉米胚特异杂种 PRP 的细胞定位及其基因启动子调控元件的特性。

Cellular localization of the embryo-specific hybrid PRP from Zea mays, and characterization of promoter regulatory elements of its gene.

机构信息

Centre de Recerca en Agrigenòmica (CRAG), CSIC-IRTA-UAB-UB, Edifici CRAG, Campus UAB, Bellaterra (Cerdanyola del Vallés), 081993 Barcelona, Spain,

出版信息

Plant Mol Biol. 2012 Oct;80(3):325-35. doi: 10.1007/s11103-012-9951-9. Epub 2012 Aug 23.

Abstract

The expression, regulation and cellular localization of ZmHyPRP, a gene marker of embryo differentiation whose expression declines after ABA induction, was studied. ZmHyPRP is a proline-rich protein with a C-terminal domain having eight cysteines in a CM8 pattern. Transient expression in onion epidermal cells, transformed with a 2x35S::ZmHyPRP-GFP construction, indicated the protein is present in vesicles lining the membrane of the cell. The ZmHyPRP gene expression is under the control of classic promoter seed-specific regulatory elements such as Sph/RY and G-boxes, suggesting regulation by B3 and b-ZIP transcription factors. Promoter deletion analysis, by particle-bombardment transient transformation of maize immature embryos with serial deletions of the promoter fused to GUS, showed the presence of two negative regulatory elements, NE1 (-2070 to -1280) and NE2 (-232 to -178), in the ZmHyPRP promoter. By selective deletion or mutation of ZmHyPRP regulatory promoter elements we conclude that the promoter expression is attenuated by the NE2 element as well as by the G-box2 and the Sph1-2 box together with the G-box2.

摘要

研究了 ZmHyPRP 的表达、调控和细胞定位,该基因是胚胎分化的标志基因,其表达在 ABA 诱导后下降。ZmHyPRP 是一种富含脯氨酸的蛋白,其 C 端结构域具有 CM8 模式的 8 个半胱氨酸。用 2x35S::ZmHyPRP-GFP 构建体转化洋葱表皮细胞的瞬时表达表明,该蛋白存在于细胞膜的囊泡中。ZmHyPRP 基因的表达受经典启动子种子特异性调控元件的控制,如 Sph/RY 和 G-盒,提示其受 B3 和 b-ZIP 转录因子的调控。通过用粒子轰击瞬时转化玉米未成熟胚,对启动子进行串联缺失与 GUS 融合,对启动子进行缺失分析,发现 ZmHyPRP 启动子中存在两个负调控元件 NE1(-2070 至-1280)和 NE2(-232 至-178)。通过选择性缺失或突变 ZmHyPRP 调控启动子元件,我们得出结论,启动子表达受到 NE2 元件以及 G-box2 和 Sph1-2 盒与 G-box2 共同的衰减作用。

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