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顺式调控元件决定拟南芥精子细胞中异戊烯基转移酶基因的生殖系特异性和表达水平。

Cis-Regulatory Elements Determine Germline Specificity and Expression Level of an Isopentenyltransferase Gene in Sperm Cells of Arabidopsis.

作者信息

Zhang Jinghua, Yuan Tong, Duan Xiaomeng, Wei Xiaoping, Shi Tao, Li Jia, Russell Scott D, Gou Xiaoping

机构信息

Ministry of Education Key Laboratory of Cell Activities and Stress Adaptations, School of Life Sciences, Lanzhou University, Lanzhou 730000, China (J.Z., X.D., T.S., J.L., S.D.R., X.G.); Department of Microbiology and Plant Biology, University of Oklahoma, Norman, Oklahoma 73019 (T.Y., X.W., S.D.R.).

Ministry of Education Key Laboratory of Cell Activities and Stress Adaptations, School of Life Sciences, Lanzhou University, Lanzhou 730000, China (J.Z., X.D., T.S., J.L., S.D.R., X.G.); Department of Microbiology and Plant Biology, University of Oklahoma, Norman, Oklahoma 73019 (T.Y., X.W., S.D.R.)

出版信息

Plant Physiol. 2016 Mar;170(3):1524-34. doi: 10.1104/pp.15.01510. Epub 2016 Jan 6.

Abstract

Flowering plant sperm cells transcribe a divergent and complex complement of genes. To examine promoter function, we chose an isopentenyltransferase gene known as PzIPT1. This gene is highly selectively transcribed in one sperm cell morphotype of Plumbago zeylanica, which preferentially fuses with the central cell during fertilization and is thus a founding cell of the primary endosperm. In transgenic Arabidopsis (Arabidopsis thaliana), PzIPT1 promoter displays activity in both sperm cells and upon progressive promoter truncation from the 5'-end results in a progressive decrease in reporter production, consistent with occurrence of multiple enhancer sites. Cytokinin-dependent protein binding motifs are identified in the promoter sequence, which respond with stimulation by cytokinin. Expression of PzIPT1 promoter in sperm cells confers specificity independently of previously reported Germline Restrictive Silencer Factor binding sequence. Instead, a cis-acting regulatory region consisting of two duplicated 6-bp Male Gamete Selective Activation (MGSA) motifs occurs near the site of transcription initiation. Disruption of this sequence-specific site inactivates expression of a GFP reporter gene in sperm cells. Multiple copies of the MGSA motif fused with the minimal CaMV35S promoter elements confer reporter gene expression in sperm cells. Similar duplicated MGSA motifs are also identified from promoter sequences of sperm cell-expressed genes in Arabidopsis, suggesting selective activation is possibly a common mechanism for regulation of gene expression in sperm cells of flowering plants.

摘要

开花植物的精子细胞转录出一组不同且复杂的基因。为了研究启动子功能,我们选择了一个名为PzIPT1的异戊烯基转移酶基因。该基因在白花丹的一种精子细胞形态类型中高度选择性转录,这种精子细胞在受精过程中优先与中央细胞融合,因此是初生胚乳的起始细胞。在转基因拟南芥中,PzIPT1启动子在两个精子细胞中均显示活性,并且从5'端逐渐截断启动子会导致报告基因产物逐渐减少,这与多个增强子位点的存在一致。在启动子序列中鉴定出细胞分裂素依赖性蛋白结合基序,其对细胞分裂素的刺激有反应。PzIPT1启动子在精子细胞中的表达赋予特异性,独立于先前报道的生殖系限制性沉默因子结合序列。相反,在转录起始位点附近出现了一个由两个重复的6个碱基的雄配子选择性激活(MGSA)基序组成的顺式作用调节区域。破坏这个序列特异性位点会使精子细胞中绿色荧光蛋白报告基因的表达失活。多个MGSA基序拷贝与最小的CaMV35S启动子元件融合,赋予报告基因在精子细胞中的表达。在拟南芥精子细胞表达基因的启动子序列中也鉴定出类似的重复MGSA基序,这表明选择性激活可能是开花植物精子细胞中基因表达调控的一种常见机制。

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