hi,

I have searched for the answer but I still need more clear explanation to understand the concept.

we need to filter out exons that have extremely low coverage (median read depth across all samples less than 20, which mostly reflect capture failure).

As I know, the concept of coverage depth is different from read depth... coverage depth simply means how much each segmentation is covered by the sequencing platform. While read depth means how many times a segmentation has been read. (please correct me if I'm wrong).

now my question is how can "extremely low coverage" be defined as "median read depth across all samples less than 20"?

could someone give me a clear explanation of "median" read depth?

Thank you so much

1. Count the number of reads per region in each sample.
   • Be sure to filter out anything that's excluded by your variant caller.
2. Take the median per region across samples
3. Filter

For most people, coverage and read depth are the same. If a certain nucleotide has 10 reads overlapping it, then the coverage for it is 10X. A region of interest (a single exon or an entire exome) has multiple nucleotides. Each nucleotide has a specific coverage value. You can take a median of those to get the median coverage.

Also, you can use something like GATK DepthOfCoverage to do the calculation for you: https://www.broadinstitute.org/gatk/guide/tooldocs/org_broadinstitute_gatk_tools_walkers_coverage_DepthOfCoverage.php