4.7 Article

A chromosomal assembly of the soybean cyst nematode genome

期刊

MOLECULAR ECOLOGY RESOURCES
卷 21, 期 7, 页码 2407-2422

出版社

WILEY
DOI: 10.1111/1755-0998.13432

关键词

effectors; genome; nematode; parasite; plant; soybean

资金

  1. North Central Soybean Research Program [00071398]

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The soybean cyst nematode is a sedentary plant parasite that causes significant yield losses in soybean crops, exacerbated by limited natural resistance and ineffective treatment options. By studying the genome assembly and annotation, insights into the molecular mechanisms of nematode infection in soybeans can be gained, leading to the development of novel control strategies.
The soybean cyst nematode (Heterodera glycines) is a sedentary plant parasite that exceeds billion USD annually in yield losses. This problem is exacerbated by H. glycines populations overcoming the limited sources of natural resistance in soybean and by the lack of effective and safe alternative treatments. Although there are genetic determinants that render soybeans resistant to nematode genotypes, resistant soybeans are increasingly ineffective because their multiyear usage has selected for virulent H. glycines populations. Successful H. glycines infection relies on the comprehensive re-engineering of soybean root cells into a syncytium, as well as the long-term suppression of host defences to ensure syncytial viability. At the forefront of these complex molecular interactions are effectors, the proteins secreted by H. glycines into host root tissues. The mechanisms that control genomic effector acquisition, diversification, and selection are important insights needed for the development of essential novel control strategies. As a foundation to obtain this understanding, we created a nine-scaffold, 158 Mb pseudomolecule assembly of the H. glycines genome using PacBio, Chicago, and Hi-C sequencing. A Mikado consensus gene prediction produced an annotation of 22,465 genes using short- and long-read expression data. To evaluate assembly and annotation quality, we cross-examined synteny among H. glycines assemblies, and compared BUSCO across related species. To describe the predicted proteins involved in H. glycines' secretory pathway, we contrasted expression between preparasitic and parasitic stages with functional gene information. Here, we present the results from our assembly and annotation of the H. glycines genome and contribute this resource to the scientific community.

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