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RNA-Seq analysis of grapevine induced resistance

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4TH STATSEQ WORKSHOP 18TH and 19TH April, 2012

Polo Zanotto - University of Verona (Italy)

36

RNA-Seq analysis of grapevine induced resistance

Perazzolli, M.1,*; Moretto, M.1; Fontana, P.1; Ferrarini, A.2; Velasco, R.1;

Delledonne, M.2; Pertot, I.1

1IASMA Research and Innovation Centre, Fondazione Edmund Mach, Via E. Mach 1,

38010 San Michele all’Adige (TN), Italy

2Università degli Studi di Verona, Dipartimento di Biotecnologie, Strada Le Grazie 15,

37134 Verona, Italy

*Presenting author: Michele Perazzolli (michele.perazzolli@fmach.it)

Induced systemic resistance (ISR) is a mechanism of the plant immune system. ISR is activated by selected strains of non-pathogenic microorganisms and provide protection against different types of pathogens in several plant species. In grapevine, treatment with the biocontrol agent Trichoderma harzianum T39 (T39) induces resistance against downy mildew caused by Plasmopara viticola. ISR seems to be a promising strategy for controlling crop diseases, but scarce information is available on the molecular mechanisms in non-model plants.

Transcriptional changes associated with T39 treatment and subsequent inoculation with P.

viticola were analyzed in grapevine by Illumina RNA-Seq method. Three biological replicates

were analyzed for each condition. Each biological replicate was sequenced twice on separate lane and paired-end reads 100 nucleotides in length were obtained. More than 15 million reads were obtained for each biological replicate, corresponding to a coverage of at least 32x the grapevine transcriptome. Filtered reads were mapped to the grapevine genome using TopHat tool, and the expression value of grapevine genes was calculated using Cufflinks tool. Whereas exons comprise the 9% of the genome, 77% of mapped reads showed matches to predicted genes. From one to nine isoforms were recognized for each gene, and more than 3500 new expressed regions were identified. Pearson correlations were greater than 0.97 and 0.95 between technical and biological replicates, respectively. Counts of technical replicates were summed to get better coverage, and 7024 genes resulted as differentially expressed in at least one comparison accordingly to DESeq statistical analysis. Functional annotation of differentially expressed genes by Argot2 tool highlighted a specific transcriptional reprogramming of T39-treated grapevines in response to pathogen inoculation.

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