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Hi All
I used tophat to map my 100 million base paired illumina reads after trimming with average length of 86 bp. In the bam output file generated by tophat I only find around 55 million read mapped and around 42 million reads unmapped. Can any one tell me that is it a feasible number in case of mammals.
Also what can be the reason on so much of unmapped reads since I have already cleaned the data with q value 30 and removed the adapters and primers.
In this paper http://www.plosone.org/article/info%...l.pone.0046415 I see that the comparison of topaht with GSNAP where tophat has very low mapping reads
Regards
I used tophat to map my 100 million base paired illumina reads after trimming with average length of 86 bp. In the bam output file generated by tophat I only find around 55 million read mapped and around 42 million reads unmapped. Can any one tell me that is it a feasible number in case of mammals.
Also what can be the reason on so much of unmapped reads since I have already cleaned the data with q value 30 and removed the adapters and primers.
In this paper http://www.plosone.org/article/info%...l.pone.0046415 I see that the comparison of topaht with GSNAP where tophat has very low mapping reads
Regards
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