Hi everyone!
Present, I have two file *fastq (fastq_1 and fastq_2) of Illumina.
follow me known: file fastq_1 is seq from 3' - 5', and fastq_2 is seq form 5' - 3'. So when I want to align between two file. Need to reverse reads of fastq_2? or the seq of fastq_2 was reversed automatically by Illumina?
What should i do?
Thanks for help.
Present, I have two file *fastq (fastq_1 and fastq_2) of Illumina.
follow me known: file fastq_1 is seq from 3' - 5', and fastq_2 is seq form 5' - 3'. So when I want to align between two file. Need to reverse reads of fastq_2? or the seq of fastq_2 was reversed automatically by Illumina?
What should i do?
Thanks for help.
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