I'm probably going to write something wrong, but if you had to perform several lanes/runs/experiments for one single exome, that means that you could not get sufficient coverage across all the exome in one single lane/run/experiment. So if you merge the bams your coverage will not be that large. As I understand it, coverage for one bam will be "randomly" dispersed, so merging the different bams will only make your coverage homogeneous and will cover the exome completely.

HTH

please define ridiculous size. for whole-genome sequencing of human samples you can easily end up with alignments >100Gb.

Beyond merging the same sample from multiple lanes/experiments...

I was playing around with the idea of quickly/efficiently creating a "baseline" bam file, so that the coverage present represents the average coverage across all files.

For instance, say I wanted to merge every exome.bam for CEO population samples of the 1000G data set into a single file. I could not think of a way to merge all of those files while averaging read depth or coverage instead of combining it.

In the end though I think I wanted to use this created file in a way that would not be good science.