Tweet
Hello,
I am a PhD student, looking a human methylation patterns. I am planning to design a targeted amplicon bisulfite sequencing, using a modified 16S protocol https://support.illumina.com/documen...15044223-b.pdf
All together, we would like to sequence 8250 amplicons (50 people, 5 brain regions each, 33 amplicons per brain region). We will do multiplex sequencing, so we need 250 combinations of indexes (50 people and 5 brain regions).
According to our regional Illumina commercial service each of the 33 amplicons per region per person should be multiplied separately with overhang primers, and then all the 33 amplicons should be equimolarly merged into one sample and multiplied by one pair of Nextera forward and reverse indexes.
Now my main question would be will the second round of PCR work? Will there be sufficient amplification concentration at the end? Can you successfully amplify 33 different amplicons simultaneously in a single well? They will be approximately similar in length (around 300bp) but still. Any input is greatly appreciated.
The plan for library preparation is as follows:
1. DNA isolation
2. Bisulfite conversion
3. PCR round one using primers with 5’ overhang (8250 reactions)
4. Gel Electrophoresis / Agilent
5. Cleaning with magnetic beads
6. Measurement of DNA concentration (fluorescence)
7. Equimolar pooling of all 33 amplicons per per person for all five brain regions
8. PCR round two to add forward and reverse indexes to pools of amplicon - 250 samples, combined two Nextera XT kits (set A and D)
9. Gel Electrophoresis / Agilent
10. Cleaning with magnetic beads
11. Measurement of DNA concentration (fluorescence)
12. Equimolar combination of all 250 samples to generate a single library
I am a PhD student, looking a human methylation patterns. I am planning to design a targeted amplicon bisulfite sequencing, using a modified 16S protocol https://support.illumina.com/documen...15044223-b.pdf
All together, we would like to sequence 8250 amplicons (50 people, 5 brain regions each, 33 amplicons per brain region). We will do multiplex sequencing, so we need 250 combinations of indexes (50 people and 5 brain regions).
According to our regional Illumina commercial service each of the 33 amplicons per region per person should be multiplied separately with overhang primers, and then all the 33 amplicons should be equimolarly merged into one sample and multiplied by one pair of Nextera forward and reverse indexes.
Now my main question would be will the second round of PCR work? Will there be sufficient amplification concentration at the end? Can you successfully amplify 33 different amplicons simultaneously in a single well? They will be approximately similar in length (around 300bp) but still. Any input is greatly appreciated.
The plan for library preparation is as follows:
1. DNA isolation
2. Bisulfite conversion
3. PCR round one using primers with 5’ overhang (8250 reactions)
4. Gel Electrophoresis / Agilent
5. Cleaning with magnetic beads
6. Measurement of DNA concentration (fluorescence)
7. Equimolar pooling of all 33 amplicons per per person for all five brain regions
8. PCR round two to add forward and reverse indexes to pools of amplicon - 250 samples, combined two Nextera XT kits (set A and D)
9. Gel Electrophoresis / Agilent
10. Cleaning with magnetic beads
11. Measurement of DNA concentration (fluorescence)
12. Equimolar combination of all 250 samples to generate a single library
Comment