Literature DB >> 14660650

Sequence and spacing of TATA box elements are critical for accurate initiation from the beta-phaseolin promoter.

Margaret L Grace1, Mahesh B Chandrasekharan, Timothy C Hall, Alison J Crowe.   

Abstract

The beta-phaseolin (phas) gene, which encodes one of the major seed storage proteins of P. vulgaris, is tightly regulated at the transcription level resulting in strict tissue-specific and spatial expression during embryonic development. The phas proximal promoter contains a complex arrangement of core promoter elements including three TATA boxes as well as several putative initiator elements. To delineate the respective contributions of the core promoter elements to transcription initiation we have performed site-directed mutagenesis of the phas promoter. In vivo expression studies were performed on transgenic Arabidopsis harboring phas promoter mutants driving expression of the beta-glucuronidase (gus) reporter gene. Quantitative assessment of GUS activity in seeds bearing the promoter mutants indicated that both sequence and spacing of the TATA elements influenced the efficiency of transcription. Substitution, insertion or deletion mutations had no effect on histochemical staining patterns indicating that strict spacing requirements are not essential for correct spatial expression of phas during embryogenesis. Further evaluation of the phas promoter by in vitro transcription analysis revealed the presence of multiple TATA-dependent transcription initiation start sites. The distance between TATA elements and transcription start sites was maintained in insertion and deletion mutants through the creation of novel initiation sites, indicating that positioning of the TATA elements rather than DNA sequence was the primary determinant of start site location. We conclude that, while dispensable for proper spatial distribution, the complex architecture of the phas promoter is required to ensure high levels of accurate phas transcription initiation in the developing embryo.

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Year:  2003        PMID: 14660650     DOI: 10.1074/jbc.M309376200

Source DB:  PubMed          Journal:  J Biol Chem        ISSN: 0021-9258            Impact factor:   5.157


  32 in total

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4.  Comparative functional analysis of three abiotic stress-inducible promoters in transgenic rice.

Authors:  Mayank Rai; Chengkun He; Ray Wu
Journal:  Transgenic Res       Date:  2009-04-09       Impact factor: 2.788

5.  Regulation of the rose Rh-PIP2;1 promoter by hormones and abiotic stresses in Arabidopsis.

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Journal:  Plant Cell Rep       Date:  2008-11-05       Impact factor: 4.570

6.  Identification of cis-elements and evaluation of upstream regulatory region of a rice anther-specific gene, OSIPP3, conferring pollen-specific expression in Oryza sativa (L.) ssp. indica.

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7.  Genome-wide characterization of phenylalanine ammonia-lyase gene family in watermelon (Citrullus lanatus).

Authors:  Chun-Juan Dong; Qing-Mao Shang
Journal:  Planta       Date:  2013-04-02       Impact factor: 4.116

8.  Highly conserved motifs in non-coding regions of Sirevirus retrotransposons: the key for their pattern of distribution within and across plants?

Authors:  Alexandros Bousios; Nikos Darzentas; Athanasios Tsaftaris; Stephen R Pearce
Journal:  BMC Genomics       Date:  2010-02-04       Impact factor: 3.969

9.  Identification and functional characterization of the BBX24 promoter and gene from chrysanthemum in Arabidopsis.

Authors:  Muhammad Imtiaz; Yingjie Yang; Ruixue Liu; Yanjie Xu; Muhammad Ali Khan; Qian Wei; Junping Gao; Bo Hong
Journal:  Plant Mol Biol       Date:  2015-08-08       Impact factor: 4.076

10.  A T9G mutation in the prototype TATA-box TCACTATATATAG determines nucleosome formation and synergy with upstream activator sequences in plant promoters.

Authors:  Amol Ranjan; Suraiya A Ansari; Rakesh Srivastava; Shrikant Mantri; Mehar H Asif; Samir V Sawant; Rakesh Tuli
Journal:  Plant Physiol       Date:  2009-10-07       Impact factor: 8.340

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