S1 Fig. Experimental set-up and differentially expressed genes (DEGs)
2023
Pedro-Jové, Roger de | Corral, Jordi | Rocafort, Mercedes | Puigvert, Marina | Azam, Fàtima Latif | Vandecaveye, Agustina | Macho, Alberto P. | Balsalobre, Carlos | Coll, Núria S. | Orellano, Elena G. | Valls, Marc
A) RNA sampling conditions from environmental (soil and mineral water) and previously obtained samples (rich B medium reference and three in planta conditions). B) Transcriptomic data analysis pipeline. First, raw RNA-seq data quality was evaluated with FastQC (v.0.11.5), trimmed with trimGalore (v.0.6.1) and potential rRNA contaminants were filtered out with the SortMeRNA software (v.4.2.0). Reads were mapped with Bowtie2 (v. 2.4.4) and alignments quantified with FADU v. 1.8. The R. solanacearum UY031 genome GCF_001299555.1_ASM129955v1 was used. DEG analyses were performed with Deseq2 (v. 1.34.0). Genes with |log2(fold-change)|>1.5 and adjusted p-value <0.01 were considered as differentially expressed (DEG) when compared to the reference medium. The UpsetR package (v. 1.4.0) (90) was used to detect unique DEG and intersections among the in the different conditions. Deseq2 transformed counts normalized for sample size were used for principal component analysis. C) DEGs in the different conditions. Bars show the total number of up- (yellow) and downregulated (blue) genes for each condition compared to the reference Rich B medium. The line graph and the right Y axis indicate the percentage of DEGs. Drawings created with BioRender.
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اظهر المزيد [+] اقل [-]الكلمات المفتاحية الخاصة بالمكنز الزراعي (أجروفوك)
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تم تزويد هذا السجل من قبل Consorcio CSIC-IRTA-UAB Centro de Investigación Agrogenómica (CRAG)