Hey, you posted this in the Illumina forum. You want the Solid forum. (Maybe a moderator would be so kind as to move this thread to the solid forum?)

We actually use 3 different nick translation times, then pool them before the gel isolation step. We are hoping that will reduce systematic bias a little. That is, if there are sequence contexts where the nick translating polymerase is very slow or very fast, they might be missed with one time point because the resulting libraries will be too larger or too small, respectively. But by using 3 time points we might move the too slow or too fast pools into the correct size window.

We just re-made a library from a species that we knew had DNA that was a slow nick-translator. 10, 12 and 14 minutes were what we used for it. That gave us a smear from about 150-350 bp on the gel. We took stuff above 250 bp.

Any particular reason you are going for 400 bp instead of the recommended 300 bp?

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Phillip