The sequencing people in house told us that the library fragments range from 200-500 bp with a major band at ~280bp, so for tophat setting, how could we set up -r? we have 100 cycles for read1 and 100 cycles for read2.
tophat -r 80 index/index_mm9 R1.fastq R2.fastq
thanks!
(previously, the sequencing results from Illumina just informed us 75bp for paired end reads, and total fragments are 300bp, so we set up -r as 150)
tophat -r 80 index/index_mm9 R1.fastq R2.fastq
thanks!
(previously, the sequencing results from Illumina just informed us 75bp for paired end reads, and total fragments are 300bp, so we set up -r as 150)
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