A genome-scale integrated approach aids in genetic dissection of complex flowering time trait in chickpea

Hari D Upadhyaya; Deepak Bajaj; Shouvik Das; Maneesha S Saxena; Saurabh Badoni; Vinod Kumar; Shailesh Tripathi; C L L Gowda; Shivali Sharma; Akhilesh K Tyagi; Swarup K Parida

doi:10.1007/s11103-015-0377-z

A genome-scale integrated approach aids in genetic dissection of complex flowering time trait in chickpea

Plant Mol Biol. 2015 Nov;89(4-5):403-20. doi: 10.1007/s11103-015-0377-z. Epub 2015 Sep 22.

Authors

Affiliations

¹ International Crops Research Institute for the Semi-Arid Tropics (ICRISAT), Patancheru, Telangana, 502324, India.
² National Institute of Plant Genome Research (NIPGR), Aruna Asaf Ali Marg, New Delhi, 110067, India.
³ National Research Centre on Plant Biotechnology (NRCPB), New Delhi, 110012, India.
⁴ Division of Genetics, Indian Agricultural Research Institute (IARI), New Delhi, 110012, India.
⁵ National Institute of Plant Genome Research (NIPGR), Aruna Asaf Ali Marg, New Delhi, 110067, India. swarup@nipgr.ac.in.

PMID: 26394865
DOI: 10.1007/s11103-015-0377-z

Abstract

A combinatorial approach of candidate gene-based association analysis and genome-wide association study (GWAS) integrated with QTL mapping, differential gene expression profiling and molecular haplotyping was deployed in the present study for quantitative dissection of complex flowering time trait in chickpea. Candidate gene-based association mapping in a flowering time association panel (92 diverse desi and kabuli accessions) was performed by employing the genotyping information of 5724 SNPs discovered from 82 known flowering chickpea gene orthologs of Arabidopsis and legumes as well as 832 gene-encoding transcripts that are differentially expressed during flower development in chickpea. GWAS using both genome-wide GBS- and candidate gene-based genotyping data of 30,129 SNPs in a structured population of 92 sequenced accessions (with 200-250 kb LD decay) detected eight maximum effect genomic SNP loci (genes) associated (34% combined PVE) with flowering time. Six flowering time-associated major genomic loci harbouring five robust QTLs mapped on a high-resolution intra-specific genetic linkage map were validated (11.6-27.3% PVE at 5.4-11.7 LOD) further by traditional QTL mapping. The flower-specific expression, including differential up- and down-regulation (>three folds) of eight flowering time-associated genes (including six genes validated by QTL mapping) especially in early flowering than late flowering contrasting chickpea accessions/mapping individuals during flower development was evident. The gene haplotype-based LD mapping discovered diverse novel natural allelic variants and haplotypes in eight genes with high trait association potential (41% combined PVE) for flowering time differentiation in cultivated and wild chickpea. Taken together, eight potential known/candidate flowering time-regulating genes [efl1 (early flowering 1), FLD (Flowering locus D), GI (GIGANTEA), Myb (Myeloblastosis), SFH3 (SEC14-like 3), bZIP (basic-leucine zipper), bHLH (basic helix-loop-helix) and SBP (SQUAMOSA promoter binding protein)], including novel markers, QTLs, alleles and haplotypes delineated by aforesaid genome-wide integrated approach have potential for marker-assisted genetic improvement and unravelling the domestication pattern of flowering time in chickpea.

Keywords: Chickpea; Flowering time; GBS; GWAS; QTL; SNP.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Chromosome Mapping
Cicer / genetics*
Cicer / growth & development*
Flowers / genetics
Flowers / growth & development
Gene Expression Profiling
Genome, Plant*
Genome-Wide Association Study
Genotype
Haplotypes
Linkage Disequilibrium
Phenotype
Polymorphism, Single Nucleotide
Quantitative Trait Loci
Time Factors