Genome-wide identification, in silico characterization and expression analysis of the RNA helicase gene family in chickpea (C. arietinum L.)

Sheel Yadav; Yashwant K Yadava; Deshika Kohli; Shashi Meena; Gopal Kalwan; C Bharadwaj; Kishor Gaikwad; Ajay Arora; P K Jain

doi:10.1038/s41598-022-13823-9

Genome-wide identification, in silico characterization and expression analysis of the RNA helicase gene family in chickpea (C. arietinum L.)

Sci Rep. 2022 Jun 13;12(1):9778. doi: 10.1038/s41598-022-13823-9.

Authors

Sheel Yadav¹, Yashwant K Yadava¹, Deshika Kohli¹, Shashi Meena², Gopal Kalwan¹, C Bharadwaj³, Kishor Gaikwad¹, Ajay Arora², P K Jain⁴

Affiliations

¹ ICAR-National Institute for Plant Biotechnology, New Delhi, 110012, India.
² Division of Plant Physiology, ICAR-Indian Agricultural Research Institute, New Delhi, 110012, India.
³ Division of Genetics, ICAR-Indian Agricultural Research Institute, New Delhi, 110012, India.
⁴ ICAR-National Institute for Plant Biotechnology, New Delhi, 110012, India. jainpmb@gmail.com.

Abstract

The RNA helicases are an important class of enzymes which are known to influence almost every aspect of RNA metabolism. The majority of RNA helicases belong to the SF2 (superfamily 2) superfamily, members of which are further categorized into three separate subfamilies i.e., the DEAD, DEAH and DExD/H-box subfamilies. In chickpea, these RNA helicases have not been characterized until now. A genome-wide analysis across the chickpea genome led to the identification of a total of 150 RNA helicase genes which included 50 DEAD, 33 DEAH and 67 DExD/H-box genes. These were distributed across all the eight chromosomes, with highest number on chromosome 4 (26) and least on chromosome 8 (8). Gene duplication analysis resulted in identification of 15 paralogous gene pairs with Ka/Ks values < 1, indicating towards the genes being under purifying selection during the course of evolution. The promoter regions of the RNA helicase genes were enriched in cis-acting elements like the light and ABA-responsive elements. The drought responsiveness of the genes was analysed by studying the expression profiles of few of these genes, in two different genotypes, the cultivated variety ICC 8261 (kabuli, C. arietinum) and the wild accession ILWC 292 (C. reticulatum), through qRT-PCR. These genotypes were selected based on their drought responsiveness in a field experiment, where it was observed that the percentage (%) reduction in relative water content (RWC) and membrane stability index (MSI) for the drought stressed plants after withholding water for 24 days, over the control or well-watered plants, was least for both the genotypes. The genes CaDEAD50 and CaDExD/H66 were identified as drought-responsive RNA helicase genes in chickpea. The protein encoded by the CaDExD/H66 gene shares a high degree of homology with one of the CLSY (CLASSY) proteins of A. thaliana. We hypothesize that this gene could possibly be involved in regulation of DNA methylation levels in chickpea by regulating siRNA production, in conjunction with other proteins like the Argonaute, RNA dependent RNA polymerases and Dicer-like proteins.

MeSH terms

Cicer* / metabolism
Droughts
Gene Duplication
Gene Expression Regulation, Plant
RNA / metabolism
Water / metabolism

Substances

Water
RNA