Development of efficient synthetic promoters derived from pararetrovirus suitable for translational research

Dipinte Gupta; Nrisingha Dey; Sadhu Leelavathi; Rajiv Ranjan

doi:10.1007/s00425-021-03565-9

Development of efficient synthetic promoters derived from pararetrovirus suitable for translational research

Planta. 2021 Jan 21;253(2):42. doi: 10.1007/s00425-021-03565-9.

Authors

Dipinte Gupta¹, Nrisingha Dey², Sadhu Leelavathi³, Rajiv Ranjan⁴

Affiliations

¹ Plant Biotechnology Lab, Department of Botany, Faculty of Science, Dayalbagh Educational Institute (Deemed University), Dayalbagh, Agra, 282005, India.
² Institute of Life Science, Nalco Square, Bhubaneshwar, Odisha, 751023, India.
³ Plant Biology: Plant Transformation Research Group, International Centre for Genetic Engineering and Biotechnology (ICGEB), New Delhi, 110067, India.
⁴ Plant Biotechnology Lab, Department of Botany, Faculty of Science, Dayalbagh Educational Institute (Deemed University), Dayalbagh, Agra, 282005, India. rajivranjanbt@gmail.com.

PMID: 33475866
DOI: 10.1007/s00425-021-03565-9

Abstract

In this study, useful hybrid promoters were developed for efficient ectopic gene expression in monocot and dicot plants, and they hold strong prominence in both transgenic research and biotech industries. This study deals with developing novel synthetic promoters derived from Rice Tungro Bacilliform Virus (RTBV) and Mirabilis Mosaic Virus (MMV). Despite numerous availability, there is a severe scarcity of promoters universally suitable for monocot and dicot plants. Here, eight chimeric promoter constructs were synthesized as gBlocks gene fragments through domain swapping and hybridization by incorporating important domains of previously characterized RTBV and MMV promoters. The developed promoter constructs were assessed for transient GUS expression in tobacco protoplast (Xanthi Brad) and agro-infiltrated tobacco, petunia, rice and pearl millet. Protoplast expression analysis showed that two promoter constructs, namely pUPMA-RP1-MP1GUS and pUPMA-RP4-MP1GUS exhibited 3.56 and 2.5 times higher activities than that of the CaMV35S promoter. We had observed the similar type of expression patterns of these promoters in agroinfiltration-based transient studies. RP1-MP1 and RP4-MP1 promoters exhibited 1.87- and 1.68-fold increase expression in transgenic tobacco plants; while, a 1.95-fold increase was found in RP1-MP1 transgenic rice plants when compared their activities with CaMV35S promoter. Furthermore, on evaluating these promoter constructs for their expression in the bacterial system, pUPMA-RP1-MP1GFP was found to have the highest GFP expression. Moreover, the promoter construct was also evaluated for its capacity to express the HMP3 gene. Biobeads of encapsulated bacterial cells expressing HMP3 gene under control of the pUPMA-RP4-MP1 promoter were found to reduce 72.9% copper and 29.2% zinc concentration from wastewater. Our results had demonstrated that the developed promoter constructs could be used for translational research in dicot, monocot plants and bacterial systems for efficient gene expression.

Keywords: Cis elements; Mirabilis mosaic virus; Rice tungro bacilliform virus; Synthetic promoter.

MeSH terms

Caulimovirus* / genetics
Nicotiana / genetics
Plants, Genetically Modified / genetics
Promoter Regions, Genetic* / genetics
Protein Biosynthesis*

Grants and funding

37(1)/14/40/20l4-BRNS/l423 dated 24/08/20l4/DAE-BRNS