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I am trying to align a miRNA-seq FASTQ file using the mapper.pl from miRDeep2 but I am not having any luck.
The reads in the FASTQ file are ~50bp.
I am not sure where my mistake is as I get 46380 reads mapped (less than 1.6% of total reads). This is my code
I think my mistake is with the adapter sequence. The adapter for this sample is ATCACGA (it is in the sample name too). I looked at this website illumina-adapter-and-primer-sequences/ and my samples (I do have more) follow the TruSeq™ DNA Sample Prep Kit v2 but if I try to put a longer adapter (TruSeq Adapter, Index 1) I just get +- 10000 mapped reads.
I am not sure how to proceed. Any help would be appreciated.
The reads in the FASTQ file are ~50bp.
I am not sure where my mistake is as I get 46380 reads mapped (less than 1.6% of total reads). This is my code
Code:
mapper.pl /mnt/d/work/NNNN_1_SAMPLE1_ATCACGA_S2_L001_R1_001.fastq -e -h -j -k ATCACGA -l 16 -m -p GRCh38_primary_assembly_genome -s /mnt/d/work/tools/mirdeep2/test/2.collapsed_reads.fa - t /mnt/d/work/tools/mirdeep2/test/2.grch38.arf -n -v
I am not sure how to proceed. Any help would be appreciated.
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