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Use iProof Polymerase for this. We can play around with KAPA afterwards to see if we don’t need 2 taqs in house

• Used this r-script to bind the Masterkey to the pool and mid plate map, this plate map, and the 2017 plate map to make this demux key

• QC from University of Colorado Genomics Core

Sequencing Reports Nov 2021

Lane Summary (Pools 1 and 2) AHNYYMDRXY

Lane Summary (Pools 3 and 4) BHNYW7DRXY

Sequencing Reports April 2021

Flowcell Summary (Pools 1 and 2)

Lane Summary (Pools 1 and 2)

Flowcell Summary (Pools 3 and 4)

Lane Summary (Pools 3 and 4)

Reagents and Ordering

•  EcoR1 (20,000 units/ml)
•  MseI (10,000 units/ml)
•  T4 DNA ligase buffer (400,000 units/ml)
•  DNA polymerase (BioRad iProof or KAPA HiFi)
•  BSA (1 mg/ml)-We have this in 20 mg/ul
•  1 M NaCl-We have this at 5M
•  DMSO
•  EcoR1 adaptors (We need 1 uM MIDed in plates)
•  Mse1 Adaptors (10 uM stock probably need to dilute from 100 uM)
•  IIllpcr2 (5 10 uM working)
•  Illpcr1 (5 10 uM working)
•  Pool of above 2 primers (2.5 uM working of each)

Original SOP

Normalize templates

Use plate reader to quantify templates

Normalize to between 20 ng/ul and 150 ng/ul

2017 alfalfa: Transfer to conical pcr plates. Normalize on nimbus to 100 ng/ul in 30 ul.

Illumina Primer Pooling

Add 900 ul std TE to 5 tubes

Add 50 ul of both Illpcr1 and Illpcr2 to each tube

Seal, vortex, and spin tubes. You will need 2 tubes for this prep.

MseI oligo Annealing

Only needs to be done after first making working stock.

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Heat to 95C for 5 minutes and allow to slowly cool to RT.

EcoRI plate 4 oligo Annealing

SpeedVac plates Stock Plate 7 and Stock Plate 8 to dry oligos

Resuspend plate 4a and 4b to 25 uM. We will have to calculate based off initial expected volume and concentration.with 20 ul H2O and 60 ul std TE to avoid over saturating with Tris and EDTA to create 25 uM stocks.

Combine 4 ul from each plate in a well to well fashion with 92 ul of TE to create a 1 uM working plate.

Label it “GBS Working Stock Plate 4” Seal, Vortex, and Spin down resulting plate.

Heat to 95C for 5 minutes and allow to slowly cool to RT

Restriction Digestion

(Keep MM and reaction plates on ice)

Add 3 ul Digestion MM to 22 16 plates using the Benchsmart

Use an 8 channel to divvy up 71 ul across a plate and then the Benchsmart to add 3 ul to 22 plates.

Add 6 ul template to each plate with 8 channel. Cover and seal each plate, vortex, centrifuge and incubate at 37C for 8 hours. Followed by 62C for 1 hour.

Adaptor Ligation

Spin down plates and add 1.4 ul Ligation MM to each well with Benchsmart.

Add 1 ul of EcoR1 Adaptors with 8-channel and Track which template plate gets which MID plate.

Label reaction plates with MID plate used.

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Add 189 ul of low EDTA TE store at 4C for a month or -20C for longer.

PCR Amplification

Pool ligated plates matching well to well in sets of 4 with one set of 2 avoiding combining the same MIDs together:

We are running duplicate PCRs for each template.

Add 16 ul of PCR1 MM to each well of plates

Add 4 ul of restriction/ligation products to each well

Seal, Vortex, Spin down, and then run on Thermocycler program: GBS1:

*pause step

Extra PCR

Add 2.125 ul of the MM directly to the previous PCR

Then continue with the last four unlisted steps for GBS1 from above:

Pooling

Size Selection

Blue Pippin?

Gel Extraction?We utilized the Pippin Prep machine on loan from the Ernest Lab, selecting for the range 300-450bp.