Hi Eric!! I am very interested in your post because at our lab we are trying to implement the Access Array Fluidgm technology to amplify 20-30 nuclear loci in a wide set of samples (over 2000), but we would like first to prove if the methodology is appropriate for adequate genotype fragments between 100-200pb. I have made some quotations for the pilot experiment and the cost is around $130 per sample (assuming we are going to amplify 48 loci in 48 samples, and the cost does include primers and MID's) which I think is cheap but means a lot of money when we are talking just about an experiment. So I am curious about where did you develop your experiments with Acces Array?, here in Mexico is difficult to have access to these technologies. Also I would like to know how much would be the deep of sequencing for an adequate genotype of a nuclear loci using Illumina?, which coverage would you recommend? Any additional comments?

Thank you a lor for any help

Hi NJ, I am sorry to tell you that we ended up not using Access Array. I therefore have no pertinent information to give you. Best of luck!

Eric

Oh! I am sorry to read that, but I am curious, is there any methodological reason that you have to not work with Access Array? or was just a change of priorities? Thank you

We just changed our minds and continued to use the good old method of library prep since we never went to very high numbers of samples per lane. Cheers