Identification of a novel and plant height-independent QTL for coleoptile length in barley and validation of its effect using near isogenic lines

Author:

Gao Shang1,Su Zhouyang1,Ma Jun2,Ma Jian3,Liu Chunji1,Li Huihui4,Zheng Zhi5ORCID

Affiliation:

1. CSIRO Queensland Bioscience Precinct

2. China Agricultural University College of Agronomy and Biotechnology

3. Sichuan Agricultural University

4. Chinese Academy of Agricultural Sciences Institute of Crop Sciences

5. CSIRO Queensland Bioscience Precinct Agriculture and Food Unit

Abstract

Abstract Coleoptile length (CL) is one of the most important agronomic traits in cereal crops due to its direct influence on the optimal depth for seed sowing which facilitates better seedling establishment. Varieties with longer coleoptiles are preferred in drought-prone areas where less moisture maintains at the top layer of the soil. Compared to wheat, genetic study on coleoptile length is limited in barley. Here, we reported a study on detecting the genomic regions associated with CL in barley by assessing a population consisting of 201 recombinant inbred lines (RILs). Four putative QTL conferring CL were consistently identified on chromosomes 1H, 5H, 6H, and 7H in each of the trials conducted. Of these QTL, the two located on chromosomes 5H and 6H (designated as Qcl.caf-5H and Qcl.caf-6H) are likely novel and Qcl.caf-5Hshowed the most significant effect explaining up to 30.9% of phenotypic variance with a LOD value of 15.1. To further validate the effect of this putative QTL, five pairs of near isogenic lines (NILs) were then developed and assessed. Analysis of the NILs showed an average difference of 21.0% in CL between the two isolines. Notably, none of the other assessed morphological characteristics showed consistent differences between the two isolines for each pair of the NILs. Candidate genes underlying the Qcl.caf-5H locus were also predicted by employing orthologous analysis and comparing the genome assemblies for both parental genotypes of the mapping population in the present study. Taken together, these findings expand our understanding on genetic basis of CL and will be indicative for further gene cloning and functional analysis underly this locus in barley.

Publisher

Research Square Platform LLC

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