Hello,
I want to ask you what is the best way for visualizing big file (Bam), I am going to sort bam file with samtools sort at first, then convert it to bedgraph by this command: bedtools genomecov -ibam *.bam -bg -scale 10.0, and visualize it by IGV. this way is right and certain in your idea or what else?
thanks in advance
If you want to be able to see content regardless of the zoom level then make a bigWig files (e.g., with bamCoverage from deepTools or from the bedGraph file bedtools genomecov produces). But if you're going to zoom in and look at smaller regions (<20kb) anyway then just stick with the indexed and sorted BAM file. BAM will still be slower to render than bigWig data, but it otherwise works fine.
You can direcly open your sorted and indexed bam file in IGV. It's not required to convert it to bedgraph.
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What is the aim of your visualisation? Are you specifically interested in a single gene or locus?