Selection of functional EPHB2 genotypes from ENU mutated grass carp treated with GCRV

Meher un Nissa; Zhu-Xiang Jiang; Guo-Dong Zheng; Shu-Ming Zou

doi:10.1186/s12864-021-07858-x

BMC Genomics (Jul 2021)

Selection of functional EPHB2 genotypes from ENU mutated grass carp treated with GCRV

Meher un Nissa,
Zhu-Xiang Jiang,
Guo-Dong Zheng,
Shu-Ming Zou

Affiliations

Meher un Nissa: Genetics and Breeding Center for Blunt Snout Bream, Ministry of Agriculture
Zhu-Xiang Jiang: Genetics and Breeding Center for Blunt Snout Bream, Ministry of Agriculture
Guo-Dong Zheng: Genetics and Breeding Center for Blunt Snout Bream, Ministry of Agriculture
Shu-Ming Zou: Genetics and Breeding Center for Blunt Snout Bream, Ministry of Agriculture

DOI: https://doi.org/10.1186/s12864-021-07858-x
Journal volume & issue: Vol. 22, no. 1
pp. 1 – 14

Abstract

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Abstract Background N-ethyl-N-nitrosourea (ENU) mutagenesis is a useful method for the genetic engineering of plants, and the production of functional mutants in animal models including mice and zebrafish. Grass carp reovirus (GCRV) is a haemorrhagic disease of grass carp which has caused noteworthy losses in fingerlings over the last few years. To overcome this problem, we used ENU mutant grass carp in an attempt to identify functional resistance genes for future hereditary rearing projects in grass carp. Results This study used ENU-mutated grass carp to identify genetic markers associated with resistance to the haemorrhagic disease caused by GCRV. Bulked segregant analysis (BSA) was performed on two homozygous gynogenetic ENU grass carp groups who were susceptible or resistant to GCRV. This analysis identified 466,162 SNPs and 197,644 InDels within the genomes of these mixed pools with a total of 170 genes annotated in the associated region, including 49 genes with non-synonymous mutations at SNP sites and 25 genes with frame shift mutations at InDel sites. Of these 170 mutated genes, 5 randomly selected immune-related genes were shown to be more strongly expressed in the resistant group as compared to the susceptible animals. In addition, we found that one immune-related gene, EPHB2, presented with two heterozygous SNP mutations which altered the animal’s responded to GCRV disease. These SNPs were found in the intron region of EPHB2 at positions 5859 (5859G > A) and 5968 (5968G > A) and were significantly (p = 0.002, 0.003) associated with resistance to GCRV. These SNP sites were also shown to correlate with the GCRV-resistant phenotype in these ENU grass carp. We also evaluated the mortality of the different ENU fish genotypes in response to GCRV and the SNPs in EPHB2. The outcomes of these evaluations will be useful in future selections of GCRV-resistant genes for genetic breeding in grass carp. Conclusion Our results provide a proof of concept for the application of BSA-sequence analysis in detecting genes responsible for specific functional genotypes and may help to develop better methods for marker-assisted selection, especially for disease resistance in response to GCRV.

Published in BMC Genomics

ISSN: 1471-2164 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Technology: Chemical technology: Biotechnology; Science: Biology (General): Genetics
Website: http://bmcgenomics.biomedcentral.com

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