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FAQ.md

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Q. Is my BAM file sorted? A. Run samtools view -H <file> | grep SO:. If sorted, should indicate the sort order otherwise say unsorted. Further, the bam index files generated from the unsorted files are of smaller size (hence look fishy).

Q. Is my data paired-end or single-end sequenced? A. Run samtools flagstat <file>; should indicate the number of reads in paired-end mode along with total number of reads.

Q. What are the blacklist regions across species? A. See here: https://sites.google.com/site/anshulkundaje/projects/blacklists

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