Generation and Characterization of a Sugarbeet Transcriptome and Transcript-Based SSR Markers

The Plant Genome. 2014;7(2) DOI 10.3835/plantgenome2013.11.0038


Journal Homepage

Journal Title: The Plant Genome

ISSN: 1940-3372 (Online)

Publisher: Crop Science Society of America

LCC Subject Category: Agriculture: Plant culture | Science: Biology (General): Genetics

Country of publisher: United States

Language of fulltext: English

Full-text formats available: PDF, HTML



Karen Klotz Fugate

Diego Fajardo

Brandon Schlautman

Jocleita Peruzzo Ferrareze

Melvin D. Bolton

Larry G. Campbell

Eric Wiesman

Juan Zalapa


Blind peer review

Editorial Board

Instructions for authors

Time From Submission to Publication: 15 weeks


Abstract | Full Text

Sugarbeet is a major source of refined sucrose and increasingly grown for biofuel production. Demand for higher productivity for this crop requires greater knowledge of sugarbeet physiology, pathology, and genetics, which can be advanced by the development of new genomic resources. Towards this end, a sugarbeet transcriptome of expressed genes from leaf and root tissues at varying stages of development and production, and after elicitation with jasmonic acid (JA) or salicylic acid (SA), was constructed and used to generate simple sequence repeat (SSR) markers. The transcriptome was generated via paired-end RNA sequencing and contains 82,404 unigenes. A total of 37,207 unigenes were annotated, of which 9480 were functionally classified using clusters of orthologous groups (COG) annotations, 17,191 were classified into biological process, molecular function, or cellular component using gene ontology (GO) terms, and 17,409 were assigned to 126 metabolic pathways using Kyoto Encyclopedia of Genes and Genomes (KEGG) identifiers. A SSR search of the transcriptome identified 7680 SSRs, including 6577 perfect SSRs, of which 3834 were located in unigenes with ungapped sequence. Primer-pairs were designed for 288 SSR loci, and 72 of these primer-pairs were tested for their ability to detect polymorphisms. Forty-three primer-pairs detected single polymorphic loci and effectively distinguished diversity among eight genotypes. The transcriptome and SSR markers provide additional, public domain genomic resources for an important crop plant and can be used to increase understanding of the functional elements of the sugarbeet genome, aid in discovery of novel genes, facilitate RNA-sequencing based expression research, and provide new tools for sugarbeet genetic research and selective breeding.