Hi!

I performed a smart-seq2 experiment on B-cells. After some minor changes in the protocol I got a satisfying amplification with no primer dimers and a 3 to 15 ng of cDNA (see attached bioanalyzer result).

- Biotinylated primers (TSO, oligo-dTNV, ISPCR) and reducing the amount of TSO by 5 and ISPCR by 2.
- SPRI beads 0.6x instead of ampurebeads 1x.

http://www.hostingpics.net/viewer.ph...6Sanstitre.png

Unfortunately I am only interested in a subpopulation of B-cells which are expressing a given transcript (poly-adenylated, ranging from 600 to 2000 bp) and my only option currently is to detect it after performing the amplification. Those cells can't be sorted before the smart-seq2 procedure.
I tried to detect it by qPCR and got systematic amplification in my 10 cells and 100 cells controls. Unfortunately in the 1-cells wells only a small fraction of my cells were positive while I was expecting almost all of them. Given the results I have the impression that this transcript is sometimes retrotranscribed sometimes not.

I have several questions related to this issue:

1. Do you have any recommandation on how to improve the retrotranscription of relatively rare transcripts?
2. Do you think that adding a transcript specific primer during the retrotranscription could help?
   I was thinking to use add an oligo:
   
   ISPCR sequence - linker - specific primer
   
   at the RNA denaturation step in addition of the oligo-dTNV.
3. What is the minimal length of transcript which can be retrotranscribed with smart-seq2 (and why)? I see clearly that 500 bp seems like the limit but could not find a good explaination for it.

Thanks in advance for your answers!