To study the impact of wheat streak mosaic virus on global gene expression in wheat curl mite, we generated a de novo transcriptome assembly using 50 x 50 paired end reads from the Illumina HiSeq 2500. Reads were assembled using Trinity (version 2.0.6) and contigs greater than 200 nt were retained. All assembled transcripts were annotated using the Trinotate pipeline using blastp searches against the Swiss-prot/Uni-Prot database, blastx searches against the Swiss-prot/Uni-Prot databases, HMM searches against the Pfam-A database, blastp searches against the non-redundant protein database, and signalP and tmHMM predictions. To reduce noise from low abundance transcripts not well supported by the data, we filtered the assembly to retain only those transcripts with TPM values >=0.5.
- TXTRaw Trinity Assembly
- xlbTrinotate annotations for raw Trinity assembly
- TXTBlastp results versus non-redundant protein database
- TXTProtein predictions for raw trinity transcriptome assembly (wheat curl mite)
- TXTFinal trinity transcriptome assembly for wheat curl mite
- TXTNucleotide coding regions for final transcriptome assembly for wheat curl mite
- TXTProtein predictions for final transcriptome assembly (wheat curl mite)
- xlbTrinotate annotations for final Trinity assembly (wheat curl mite)