I was wondering if anyone had an empirical evidence in the comparison between the TruSeq and Nexterra protocols? We have been considering switching over to the Epicentre products exclusively but lack any definitive evidence of performance. Does anyone have an argument either way?
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First, Epicentre now is owned by Illumina, so no difference there.
Second, "Nextera" is a mixture of several component methodologies:
(1) "Tagmentation" (in vitro transposase action) is used instead of sonication or other methods of mechanical fragmentation.
(2) Dual indexes (one in each adapter) are deployed rather than the single indexes of TruSeq.
(3) At least for NexteraXT, "normalization" beads are used equalize all the libraries to be included in a single pool.
(4) The lower concentration of resulting library pools is compensated for by using a heat denaturation, rather than a base denaturation prior to clustering. This may be possible because the products come off the normalization beads as ssDNA.
We have not yet run any Nextera libraries. But the process does look streamlined -- especially for handling library construction for large numbers of samples (eg 96).
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Phillip
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shearing differences
I'm told (but have no direct experience) that the "tagmentation" step, which uses enzymatic fragmentation via an engineered transposase, has some non-randomness that could potentially result in reduced coverage in certain areas. The transposase has some sequence specificity that you'd have to look up. But the sample prep sure is easy!
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