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Fine structure and function of the osmotin gene promoter.

作者信息

Liu D, Narasimhan M L, Xu Y, Raghothama K G, Hasegawa P M, Bressan R A

机构信息

Center for Plant Environmental Stress Physiology, Purdue University, West Lafayette, IN 47907-1165, USA.

出版信息

Plant Mol Biol. 1995 Dec;29(5):1015-26. doi: 10.1007/BF00014974.

DOI:10.1007/BF00014974
PMID:8555445
Abstract

The gene encoding osmotin, a tobacco pathogenesis-related protein, has been shown to be regulated by an array of hormonal and environmental signals. The osmotin promoter fragment -248 to -108 upstream of the transcription start site (fragment A), was sufficient to direct reporter gene expression when fused to a minimal CaMV 35S promoter in transient assays using microprojectile bombardment. This was consistent with previous 5'-deletion analyses of the osmotin promoter which showed that the promoter sequence from -248 to -108 is absolutely required for reporter gene activity. Nuclear protein factors from salt-adapted tobacco cells, ABA-treated unadapted cells, and young cultured tobacco leaves were shown to interact with fragment A by gel mobility-shift assays. DNase I footprinting revealed that three conserved promoter elements in fragment A interact specifically with nuclear factors. These elements are: (1) a cluster of G-box-like sequences (G sequence); (2) an AT-1 box-like sequence, 5'-AATTATTTTATG-3' (AT sequence); (3) a sequence highly conserved in ethylene-induced PR gene promoters, 5'-TAAGA/CGCCGCC-3' (PR sequence). Transient expression assays performed with fragment A deletions fused to GUS indicated that osmotin promoter activity correlated with the presence of these elements. UV cross-linking analysis showed that the protein complex bound to fragment A consisted of at least four individual proteins with approximate molecular masses of 28, 29, 40 and 42 kDa. One component of this protein complex, which was associated with the G sequence, was a 14-3-3 like protein.

摘要

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本文引用的文献

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Plant Mol Biol. 1988 Sep;10(5):401-12. doi: 10.1007/BF00014946.
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Transgenic Plants with Enhanced Resistance to the Fungal Pathogen Rhizoctonia solani.转抗真菌病原体腐霉菌基因植物。
Science. 1991 Nov 22;254(5035):1194-7. doi: 10.1126/science.254.5035.1194.
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Isolation and Characterization of the Genes Encoding Basic and Acidic Chitinase in Arabidopsis thaliana.拟南芥碱性和酸性几丁质酶基因的分离与鉴定。
14-3-3 Proteins are components of the transcription complex of the ATEM1 promoter in Arabidopsis.
14-3-3蛋白是拟南芥中ATEM1启动子转录复合体的组成成分。
Planta. 2007 Dec;227(1):167-75. doi: 10.1007/s00425-007-0604-1. Epub 2007 Aug 16.
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Differences in spatial expression between 14-3-3 isoforms in germinating barley embryos.萌发大麦胚中14-3-3亚型之间的空间表达差异。
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Plant Mol Biol. 1999 Jun;40(3):455-65. doi: 10.1023/a:1006213324555.
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A nitrilase-like protein interacts with GCC box DNA-binding proteins involved in ethylene and defense responses.一种腈水解酶样蛋白与参与乙烯和防御反应的GCC盒DNA结合蛋白相互作用。
Plant Physiol. 1998 Nov;118(3):867-74. doi: 10.1104/pp.118.3.867.
7
Tissue-specific activation of the osmotin gene by ABA, C2H4 and NaCl involves the same promoter region.脱落酸、乙烯和氯化钠对渗透素基因的组织特异性激活涉及相同的启动子区域。
Plant Mol Biol. 1997 Jun;34(3):393-402. doi: 10.1023/a:1005812217945.
8
Differential expression of TPS11, a phosphate starvation-induced gene in tomato.TPS11(一种番茄中由磷饥饿诱导的基因)的差异表达
Plant Mol Biol. 1997 Mar;33(5):867-74. doi: 10.1023/a:1005729309569.
Plant Physiol. 1990 Jul;93(3):907-14. doi: 10.1104/pp.93.3.907.
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Molecular Cloning of Osmotin and Regulation of Its Expression by ABA and Adaptation to Low Water Potential.渗透素的分子克隆及其对 ABA 和低水势适应的表达调控。
Plant Physiol. 1989 Jul;90(3):1096-101. doi: 10.1104/pp.90.3.1096.
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Osmotin gene expression is posttranscriptionally regulated.渗透素基因表达受转录后调控。
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