Can I use single and paired end fastq data from same species to generate single transcriptomic assembly in rnaSPADES? #1172
-
|
Dear Spades community. I am using rnaSpades to generate transcriptomics assembly from my species of interest. I have a total of 45 RNAseq datasets - 42 (of 45) are single-end FASTQ files whereas 3 (of 45) are paired-end FASTQ files. I would like to use all 45 FASTQ files to generate a single assembly. Therefore, I would like to know if is it acceptable (as well as correct) to use both paired and single-end FASTQ files in a single rnaSPADES command. Please see below the example: rnaspades.py --pe1-1 File1_1.fq.gz --pe1-2 File1_2.fq.gz --pe1-1 File2_1.fq.gz --pe1-2 File2_2.fq.gz --pe1-1 File3_1.fq.gz --pe1-2 File3_2.fq.gz --s1 File1.fq.gz --s1 File2.fq.gz --s1 FileN.fq.gz --threads 20 -o OUTPUT I would highly appreciate any suggestions on this. Thank you, |
Beta Was this translation helpful? Give feedback.
Replies: 1 comment 1 reply
-
|
Yes, you can provide unlimited number of input files to rnaSPAdes |
Beta Was this translation helpful? Give feedback.
-
|
Thank you @asl. I appreciate your response. |
Beta Was this translation helpful? Give feedback.
Yes, you can provide unlimited number of input files to rnaSPAdes