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本文引用的文献

1
Isolation of cloned cDNAs to auxin-responsive poly(A)RNAs of elongating soybean hypocotyl.克隆 cDNA 对伸长的大豆下胚轴 auxin 反应性 poly(A)RNA 的分离。
Proc Natl Acad Sci U S A. 1982 Dec;79(23):7185-9. doi: 10.1073/pnas.79.23.7185.
2
An Auxin-Responsive Promoter Is Differentially Induced by Auxin Gradients during Tropisms.生长素梯度在向性运动过程中差异诱导生长素响应启动子。
Plant Cell. 1991 Nov;3(11):1167-1175. doi: 10.1105/tpc.3.11.1167.
3
Soybean GH3 promoter contains multiple auxin-inducible elements.大豆GH3启动子包含多个生长素诱导元件。
Plant Cell. 1994 May;6(5):645-57. doi: 10.1105/tpc.6.5.645.
4
Transcription, organization, and sequence of an auxin-regulated gene cluster in soybean.大豆中一个生长素调节基因簇的转录、组织及序列
Plant Cell. 1989 Feb;1(2):229-39. doi: 10.1105/tpc.1.2.229.
5
Auxin-induced expression of the soybean GH3 promoter in transgenic tobacco plants.生长素诱导大豆GH3启动子在转基因烟草植株中的表达。
Plant Mol Biol. 1991 Sep;17(3):567-79. doi: 10.1007/BF00040658.
6
Tissue-specific and organ-specific expression of soybean auxin-responsive transcripts GH3 and SAURs.大豆生长素响应转录本GH3和SAURs的组织特异性和器官特异性表达。
Plant Cell. 1991 Apr;3(4):419-30. doi: 10.1105/tpc.3.4.419.

大豆SAUR启动子中的一种生长素诱导元件。

An auxin-inducible element in soybean SAUR promoters.

作者信息

Li Y, Liu Z B, Shi X, Hagen G, Guilfoyle T J

机构信息

Department of Biochemistry, University of Missouri, Columbia 65211.

出版信息

Plant Physiol. 1994 Sep;106(1):37-43. doi: 10.1104/pp.106.1.37.

DOI:10.1104/pp.106.1.37
PMID:7972520
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC159496/
Abstract

The soybean SAUR (Small Auxin-Up RNA) genes are transcriptionally induced by exogenous auxins within a few minutes after hormone application. This response is specifically induced by auxins primarily in epidermal and cortical cells within elongation zones of hypocotyls and epicotyls. We have previously shown that an 832-bp soybean SAUR promoter/beta-glucuronidase (GUS) reporter gene fusion is responsive to auxin in transgenic tobacco plants (Y. Li, G. Hagen, T.J. Guilfoyle [1991] Plant Cell 3: 1167-1175). Similar results were obtained with an 868-bp SAUR 15A promoter-GUS reporter gene in transgenic tobacco (Y. Li, unpublished results). We have now analyzed a soybean SAUR 15A promoter in transgenic tobacco plants using 5' unidirectional deletions, internal deletions and mutations, and gain-of-function assays with a minimal cauliflower mosaic virus 35S promoter. Our results indicate that the distal upstream element/NdeI restriction endonuclease site element (NDE) (B.A. McClure, G. Hagen, C.S. Brown, M.A. Gee, T.J. Guilfoyle [1989] Plant Cell 1: 229-239) in the SAUR 15A promoter is necessary and sufficient for auxin induction. Our results also show that the 30-bp NDE portion of this element is responsible for most, if not all, of the auxin inducibility of the SAUR 15A promoter. The NDE contains two adjacent sequences, TGTCTC and GGTCCCAT, which have been previously identified as putative auxin-responsive elements. We propose that these elements might function independently or together, possibly with an additional element(s), to confer auxin inducibility to the SAUR promoters.

摘要

大豆SAUR(小生长素上调RNA)基因在施加外源生长素后几分钟内就会被转录诱导。这种反应主要由生长素特异性诱导,主要发生在下胚轴和上胚轴伸长区的表皮和皮层细胞中。我们之前已经表明,一个832 bp的大豆SAUR启动子/β-葡萄糖醛酸酶(GUS)报告基因融合体在转基因烟草植株中对生长素作出反应(Y. Li、G. Hagen、T.J. Guilfoyle [1991]《植物细胞》3: 1167 - 1175)。在转基因烟草中,一个868 bp的SAUR 15A启动子-GUS报告基因也得到了类似结果(Y. Li,未发表结果)。我们现在利用5'单向缺失、内部缺失和突变,以及与最小花椰菜花叶病毒35S启动子的功能获得分析,对转基因烟草植株中的大豆SAUR 15A启动子进行了分析。我们的结果表明,SAUR 15A启动子中的远端上游元件/NdeI限制性内切酶位点元件(NDE)(B.A. McClure、G. Hagen、C.S. Brown、M.A. Gee、T.J. Guilfoyle [1989]《植物细胞》1: 229 - 239)对于生长素诱导是必要且充分的。我们的结果还表明,该元件的30 bp NDE部分负责SAUR 15A启动子的大部分(如果不是全部)生长素诱导性。NDE包含两个相邻序列,TGTCTC和GGTCCCAT,它们之前已被鉴定为假定的生长素反应元件。我们提出,这些元件可能独立或共同发挥作用,可能还与其他元件一起,赋予SAUR启动子生长素诱导性。