Wagner Fish RFS Project 1 (Trout1)

Owned by Gregg Randolph
Last updated: Dec 08, 2021
2 min read

As of 12-08-2021:

3700 fish DNA samples expected for Restriction Fragment Sequencing library prep. 2-3 plates will be pooled for PCR and sequencing. The first 12 may arrive by 12-13-21.

The below tables will need to be adjusted once we settle on how many we are doing at a time.

 

Setup Notes

~40 plates of trout to be prepared via the MseI and EcoRI GBS library prep protocol with some slight modifications:

  • Only 2-3 plates will be included in each pool

  • Pooling of samples for PCR will either only be done in groups of three or handled by half plates in sets of 4

  • Each Pool will be run by itself on an SP 1x100 NovaSeq

Check In Samples Against List from Will Rosenthal

 

Load Submission Data into MISO

 

Quantify DNA samples and normalize if any are higher than 150 ng/ul.

Restriction Digestion

(Keep MM and reaction plates on ice)

Set Incubator to 37 C

Add 3 ul Digestion MM to 11 plates using the 8 channel

Reagent

ul/rxn

rxns

ul needed (1.5x)

10x T4 Buffer

1.15

3700

6387

5M NaCl

0.12

3700

666

1 mg/ml BSA

0.6

3700

3332

H2O

0.73

3700

4056

MseI (enzyme)

0.12

3700

666

EcoR1 (enzyme)

0.28

3700

1555

Total

3

3700

16662

Add 6 ul template to each plate with Benchsmart. Cover and seal each plate, vortex, centrifuge and incubate at 37C for 8 hours. Followed by 65C in EcoBGC oven for 1 hour.

Adaptor Ligation

Spin down plates and add 1.4 ul Ligation MM to each well with 8 channel.

Reagent

ul/rxn

rxns

ul needed (1.6x)

Reagent

ul/rxn

rxns

ul needed (1.6x)

MseI oligo

1

3700

5920

H2O

0.112

3700

663.8

10x T4 Buffer

0.1

3700

592

5M NaCl

0.01

3700

59.2

1 mg/ml BSA

0.05

3700

296

T4 DNA ligase

0.1675

3700

991

Total

1.4

3700

8462

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

Template

EcoR1 MID plate

Pool

Template

EcoR1 MID plate

Pool

 

 

1

 

 

1

 

 

1

 

 

1

 

 

1

 

 

1

 

 

2

 

 

2

 

 

2

 

 

2

 

 

2

Label reaction plates with MID plate used.

Cover, vortex, and spin plates. Incubate plates at RT for 2 hours on benchtop.

Add 120 ul of low EDTA TE store at 4C for a month or -20C for longer.

PCR Amplification

Create working pools. For Pool A combine ligated plates matching well to well. For pool B combine ligated plates with even plates flipped upside down (H12 in A1). C1 and C2 will be recombining Plate 5 column wise. Combine columns 1-3, 4-6, 7-9 and 10-12 into columns 1-3 of a new plate. Then, to columns 7-9 of the same plate, add columns 1-3 and 7-9. Flip Plate 5 around and then pipette 6-4 and 12-10 into columns 7-9 of the pool plate. Mix together 20 ul from each well of each plate for pooled plate using the Benchsmart. After pooling all samples, vortex and spin down plates then use 4 ul from the pooled plates for PCR templates.

Pool

Plate1

Plate2

Plate3

Plate4

Pool

Plate1

Plate2

Plate3

Plate4

1A

 

 

 

 

Pool

Plate1

Plate2

Plate3

Plate4

Pool

Plate1

Plate2

Plate3

Plate4

1B

 

 

 

 

 

Pool

Plate5 Col 1-6

Plate5 Col 7-12

Plate6 Col 1-6

Plate6 Col 7-12

Pool

Plate5 Col 1-6

Plate5 Col 7-12

Plate6 Col 1-6

Plate6 Col 7-12

1C

 

 

 

 

 

Pool

Plate5 Col 1-6

Plate5 Col 12-7

Plate6 Col 1-6

Plate6 Col 12-7

Pool

Plate5 Col 1-6

Plate5 Col 12-7

Plate6 Col 1-6

Plate6 Col 12-7

1D

 

 

 

 

 

Pool

Plate7

Plate8

Plate9

Plate10

Pool

Plate7

Plate8

Plate9

Plate10

2A

 

 

 

 

Pool

Plate7

Plate8

Plate9

Plate10

Pool

Plate7

Plate8

Plate9

Plate10

2B

 

 

 

 

 

Pool

Plate11 Col 1-3

Plate11 Col 4-6

Plate11 Col 7-9

Plate11 Col 10-12

Pool

Plate11 Col 1-3

Plate11 Col 4-6

Plate11 Col 7-9

Plate11 Col 10-12

2C

 

 

 

 

 

Pool

Plate11 Col 1-3

Plate11 Col 6-4

Plate11 Col 7-9

Plate11 Col 12-10

Pool

Plate11 Col 1-3

Plate11 Col 6-4

Plate11 Col 7-9

Plate11 Col 12-10

2D

 

 

 

 

PCR1:

Make MM1 in a 15 ml tube:

Reagent

ul/rxn

rxns

ul needed (x1.4)

Reagent

ul/rxn

rxns

ul needed (x1.4)

H2O

9.52

1850

24658

5x iProof buffer

4

1850

10360

10 mM dNTPs

0.4

1850

1036

50 mM MgCl2

0.4

1850

1036

5 uM Illumina Primers

1.33

1850

3444

iProof TAQ

0.2

1850

518

DMSO

0.15

1850

388

total

16

1850

41440

Add 16 ul of PCR1 MM to each well of four new hard shell PCR plates with 8 channel

Add 4uL of template from pooled plates with Benchsmart

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

Temp C

Cycles

Time

Temp C

Cycles

Time

95*

1X

3:00

98

30X

0:30

60

30X

0:30

72

30X

0:40

72

1X

10:00

4*

1X*

0:00*

*pause step

Extra PCR

Add 2.125 ul of the MM directly to the previous PCR

Reagent

ul/rxn

rxns

ul needed (x 1.6)

5x Iproof buffer

0.425

1850

1258

10 mM dNTPs

0.4

1850

1184

Primers

1.33

1850

3936.8

Total

2.155

1850

6378.8

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

Temp C

Cycles

Time

Temp C

Cycles

Time

98

1X

3:00

60

1X

2:00

72

1X

10:00

4

1X

0:00

Pippin Prep Size Select (350-450 bp select):

 

Run Final Product on qPCR for check

Result from qPCR check:

 

Â