Genetic Diversity Analysis of Chickpea (Cicerarietinuml.) Genotypes Through Est -SSR Markers and Seed Protein Profiling
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Sardar Vallabh Bhai Patel University of Agriculture & Technology, Meerut
Abstract
Expressed sequence tags simple sequence repeats (EST-SSRs) are important sources
for investigation of genetic diversity and molecular marker development. Similar to genomic·
SSRs, the EST-SSRs are useful marker for many applications in genetics and plant breeding
such as genetic diversity analysis, molecular mapping and cross-transferability across related
species and genera. In spite of low polymorphism, these markers show variation in the
expressed part of the genome. In the present investigation EST -SSRs and total seed protein
profiling (SDS-PAGE) are used to determine the genetic diversity between twenty chickpea
genotypes. In this research, a total oftwenty pairs ofEST-SSRs primers were used to find out
the genetic diversity, out of twenty markers, only seventeen pairs of primers showed good
amplification over twenty chickpea genotype. Thirteen primer pairs (76.5%) were
monomorphic and four primer pairs (23.5%) were polymorphic in the chickpea genotypes.
The average polymorphism information content (PIC) values of the primers was ranged from
0.5 to 0.997 indicating a wide coverage across the genome and genetic similarity. SDS-PAGE
results revealed that seeds of chickpea genotypes are rich in storage proteins with a number of
stable bands in the gel. The major components of all the species were in the molecular
weight range from 95 to 11 kDa, with the variation in relative mobility values. The present
study suggests that with appropriate primer and reaction condition, EST-SSRs marker and
SDS-PAGE can be used effectively to establish genetic identity among chickpea at both
genus and species levels for polygenetic analysis.
