Hi all
I have a project in which RNA Sequencing is necessary. Last year, I did a pilot project with 16 samples using an Illumina HiSeq 2500 instrument in Rapid Mode. I did the RNA extractions and quality control myself. Libraries were done at my institution's core facility, with the TruSeq Stranded mRNA protocol because I work with a non-model organism, and my samples were collected in the field. Reads were 100 nt long and SE. Reads per sample ranged from 7 to 22 million reads, and this has worked well for my preliminary analyses.
Now, I am planning to expand the sequencing, but I am concerned I may get strong batch effects if I keep processing my samples “bit by bit”. However, processing all samples (approx. 96) at the same time is very expensive, so I need to consider other alternatives. One possibility that is cost effective is to reduce the read length to SE50. Another possibility is to use a different instrument, like the HiSeq 4000 which yields more reads per lane. Some facilities offer the Kappa Stranded mRNA libraries prep protocol.
I would like to be as consistent as possible and I was wondering if the community has any advice/experience on reducing the number of reads, and/or changing the library prep, and/or changing the instrument in terms of technical variability and batch effects.
Thank you,
Ana
Please make your own seperate question instead of writing in another question.