what is the % reads on target including +/-100bp? if this metric shows >90% reads on target then i suspect your coverage issue can be resolved by narrowing the gDNA insert size based on your preferred read length. (i.e. ~200bp insert for 2x100bp reads)

Hi!

I used the "Tiled Region" provided by NimbleGen as .bed file for my calculations.
(http://www.nimblegen.com/products/se...tml#annotation)

When I understand you correctly, it might happen that I have reads with one end of the read on target and the other end off target. In my calculations, such an overlapping paired-end read is counted as one sequence on target and one sequence off target. I will extend the Tiled Region by 300bp and recalculated the % on target. Maybe this will increase the % on target to ~ 80%.

However, I wonder why I obtained the advertised 60% with the version 1 library, even though I used the same strict method to calculate the % on target.

Regards,
Ulli

could be the probes used to target additional loci in v2 are less stringent, or a difference in sample prep

My numbers are consistently better than those Nimblegen quotes.

My experience:

At 80M reads, >97% of tiled regions were covered at 10X or higher, and nearly 100% of tiled bases are covered at least once.

Randomly extracting 20M reads from that, >83% of tiled regions are covered at 10X or higher, and almost 97% of tiled regions are covered at least once.

Edit:

Sorry, I think I misunderstood. It looks like your confusion is regarding "off-target" enrichment, not coverage of the tiled intervals. Expect a very large number of alignments to regions immediately adjacent to the tiles. We expect >90% (the number currently quoted by Nimblegen as far as I know) of the tiles to have reads covering them at 10X or higher generally. However, I also find significantly higher coverage outside the tiled intervals than Nimblegen claims. That said, it doesn't negatively impact the exome enrichment and simultaneously yields extra in the introns/UTRs, so I don't see it as a bad thing.