Michael,
Eh?

ABI uses the Ambion RNA library kit. It directly ligates RNA to double-stranded adapters with 5' or 3' five random nucleotide overhangs. It would not be compatible with T/A cloning.

Are you sure you (or your sequence provider) did not switch to "create cDNA then fragment and treat as a DNA library" to save money on library construction? Obviously this could result in a different sequence profile.

By the way, ABI really, really needs to drop their library kit prices to have any hope of competing with Illumina since the new TruSeq kits were released. The Ambion "SOLiD Total RNA Seq Kit" is directional, while the TruSeq RNA kit is not. But we are talking >$400 (if you count ribosomal depletion -- included in TruSeq, but not in Ambion kit) vs ~$70 for TruSeq in reagents so there is a big problem for ABI here if they don't respond soon.

--
Phillip

Sorry --- didn't supply you with enough information.

What I'm doing is using a single cell (or few cell) protocol for generating cDNA from total RNA -- been doing this for quite a while, works very well.

The cDNA is then sheared and a fragment library prepared from this material. The previous protocol (v3/v4) used a blunt ligation to add adapters and columns for each purification step. The new 5500 fragment library protocol uses T-tailed adapters, with bead-based purification. Much more efficient.

Michael