After confirming that the DNA available for this project looked good, I performed bisulfite treatment on the following gDNA samples:
1NF11
1NF15
1NF16
1NF17
2NF5
2NF6
2NF7
2NF8
NF2_6
NF2_18
M2
M3
Sample names breakdown like this:
1NF#
1 = Fidalgo Bay outplants
NF = Fidalgo Bay broodstock origination
= Sample number
2NF#
Same as above, but:
2 = Oyster Bay outplants
NF2_# (Oysters grown in Oyster Bay; DNA provided by Katherine Silliman)
NF2 = Fidalgo Bay broodstock origination, family #2
= Sample number
M2/M3 = C.gigas from Katie Lotterhos
Followed the guidelines of the [TruSeq DNA Methylation Library Prep Guide (Illumina)(https://github.com/sr320/LabDocs/blob/master/protocols/Commercial_Protocols/Illumina_truseq-dna-methylation-library-prep-guide-15066014-a.pdf).
Used the [EZ DNA Methylation-Gold Kit (ZymoResearch)(https://github.com/sr320/LabDocs/blob/master/protocols/Commercial_Protocols/ZymoResearch_EZ_DNA_Methylation-Gold_Kit_d5005i.pdf) according to the manufacturer’s protocol with the following changes/notes:
Used 100ng DNA (per Illumina recs; Zymo recommends at least 200ng for “optimal results”).
Thermal cycling was performed in 0.5mL thin-wall tubes in a PTC-200 (MJ Research) using a heated lid
Centrifugations were performed at 13,000g
Desulphonation incubation for 20mins.
DNA quantity calculations are here (Google Sheet): 20151218_oly_bisulfite_calcs
Samples were stored @ -20C. Will check samples via Bioanalyzer before proceeding to library construction.