Comparative analysis of synthetic DNA promoters for high-level gene expression in plants

Comparative analysis of synthetic DNA promoters for high-level gene expression in plants

MAIN CONCLUSION : We have designed two near- constitutive and stress-inducible promoters (CmYLCV9.11 and CmYLCV4); those are highly efficient in both dicot and monocot plants and have prospective to substitute the CaMV 35S promoter. We performed structural and functional studies of the full-length t...

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Veröffentlicht in:Planta 2014-10, Vol.240 (4), p.855-875
Hauptverfasser: Sahoo, Dipak Kumar, Sarkar, Shayan, Raha, Sumita, Maiti, Indu B, Dey, Nrisingha
Format: Artikel
Sprache:eng
Schlagworte:
abiotic stress
Agriculture
Allium cepa
Arabidopsis
Arabidopsis - genetics
Arabidopsis - physiology
beta-glucuronidase
Biomedical and Life Sciences
Biotechnology
biotic stress
Caulimovirus - physiology
Cestrum
corn
correlation
DNA
DNA probes
Ecology
Enzymatic activity
Flowers - genetics
Flowers - physiology
Forestry
Gene Expression
Gene Expression Regulation, Plant - genetics
Genes
Genes, Reporter
leaf curling
Leaves
Life Sciences
Liliopsida
Nicotiana - genetics
Nicotiana - physiology
onions
Onions - genetics
Onions - physiology
Original Article
Plant cells
Plant Diseases - immunology
Plant roots
Plant Roots - genetics
Plant Roots - physiology
Plant Sciences
Plants
Promoter regions
Promoter Regions, Genetic - genetics
Protoplasts
Recombinant Proteins
reporter genes
Seedlings
Seedlings - genetics
Seedlings - physiology
Stress, Physiological
Tobacco
transcription factors
Transgenic plants
viruses
Zea mays
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Zusammenfassung:MAIN CONCLUSION : We have designed two near- constitutive and stress-inducible promoters (CmYLCV9.11 and CmYLCV4); those are highly efficient in both dicot and monocot plants and have prospective to substitute the CaMV 35S promoter. We performed structural and functional studies of the full-length transcript promoter from Cestrum yellow leaf curling virus (CmYLCV) employing promoter/leader deletion and activating cis-sequence analysis. We designed a 465-bp long CmYLCV9.11 promoter fragment (−329 to +137 from transcription start site) that showed enhanced promoter activity and was highly responsive to both biotic and abiotic stresses. The CmYLCV9.11 promoter was about 28-fold stronger than the CaMV35S promoter in transient and stable transgenic assays using β-glucuronidase (GUS) reporter gene. The CmYLCV9.11 promoter also demonstrated stronger activity than the previously reported CmYLCV promoter fragments, CmpC (−341 to +5) and CmpS (−349 to +59) in transient systems like maize protoplasts and onion epidermal cells as well as transgenic systems. A good correlation between CmYLCV9.11 promoter-driven GUS-accumulation/enzymatic activities with corresponding uidA-mRNA level in transgenic tobacco plants was shown. Histochemical (X-Gluc) staining of transgenic seedlings, root and floral parts expressing the GUS under the control of CmYLCV9.11, CaMV35S, CmpC and CmpS promoters also support the above findings. The CmYLCV9.11 promoter is a constitutive promoter and the expression level in tissues of transgenic tobacco plants was in the following order: root > leaf > stem. The tobacco transcription factor TGA1a was found to bind strongly to the CmYLCV9.11 promoter region, as shown by Gel-shift assay and South-Western blot analysis. In addition, the CmYLCV9.11 promoter was regulated by a number of abiotic and biotic stresses as studied in transgenic Arabidopsis and tobacco plants. The newly derived CmYLCV9.11 promoter is an efficient tool for biotechnological applications.
ISSN:0032-0935
1432-2048
DOI:10.1007/s00425-014-2135-x