I have a problem using pybamview.
Opened this issue · 2 comments
Hi, My name is Kim Dong Seok who is the university student of South Korea. Nowadays I am studying RNA-Seq in my laboratory. I wanted to visualize my RNA mapping result, so I had searched some tools which can visualize the mapping result. Fortunately, I found the cool visualization tool, Pybamview! I really really want to use this tool.
Before, I use this tool, I prepared the data need to pybamview. I have a reference FASTA file and sequencing FASTQ files.
Before I start to use pybamview, I followed stages needed to use pybamview.
First, I aligned the RNA-Seq reads to reference FASTA file by using Tophat.
the command is;
tophat -p 10 Gracilariopsis_genome.fasta Gpch_RNA_1_Idx1_ATCACG_L008_R1_001.fastq ...(ellipsis)...I put all fastq in this command. Then, I followed your pybamview step.
And then, I got the results like this.
but when I run the result, I got abnormal result.
I don't know why the result is. I checked the result whether the data is mapped or not like this.
I think the mapping result is correct, but why the error message is happened, whenever I use pybamview --bam acceepted_hits.sorted,bam ???
I cannot understand the error message, ERROR: No samples found in BAM file.
plead help me..
My email address is dongseokkim6662@gmail.com
help me plz...
tophat -p 10 Gracilariopsis_genome.fasta ----> not fasta file, but index file.. (changed, it's my mistake)