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Setup Notes

~6 plates of trout to be prepared via the MseI and EcoRI GBS library prep protocol with some slight modifications:

  • Cleanup each full pool via ultra purification

  • Size select for 300-366bp fragments size window via Pippin Prep

  • Send Out for Sequencing

  • 5% PhiX spike

Check In Samples Against List from Will Rosenthal

Load Submission Data into MISO

Quantify and normalize samples:

  • Normalize plate reader with Buffer AE for all plates

  • Quantify all plates

  • Normalize first 3 to 10 ng/ul and others to 30 ng/ul

Restriction Digestion

(Keep MM and reaction plates on ice)

Set Incubator to 37 C

Add 3 ul Digestion MM to 32 plates using the 8 channel

Reagent

ul/rxn

rxns

ul needed (1.5x)

10x T4 Buffer

1.15

800

690

5M NaCl

0.12

800

72

1 mg/ml BSA

0.6

800

360

H2O

0.73

800

438

MseI (enzyme)

0.12

800

72

EcoR1 (enzyme)

0.28

800

168

Total

3

800

1800

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)

MseI oligo

1

800

800

H2O

0.112

800

89.6

10x T4 Buffer

0.1

800

80

5M NaCl

0.01

800

8

1 mg/ml BSA

0.05

800

40

T4 DNA ligase

0.1675

800

134

Total

1.4

800

1120

Add 1 ul of EcoR1 Adaptors with 96-channel and Track which template plate gets which MID plate.

Template

GTL Plate

EcoR1 MID plate

Pool Plate

Library

YCT_library_22_6_3

3Trout1

1

3Trout_Pool1

1

Teton_Library_22_3_1

3Trout2

2

3Trout_Pool1

1

Teton_Library_Plate_22_3_2

3Trout3

3

3Trout_Pool2and4

1

Tetons_Library_Plate_22_5_4

3Trout4

4

3Trout_Pool2

2

YCT_Library_22_3_5

3Trout5

5

3Trout_Pool2

2

UMT_YCT_RBT_DNA to UWY

3Trout6

6

3Trout_Pool2and4

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

 PCR1:

Reagent

ul/rxn

rxns

ul needed (x1.4)

H2O

9.52

350

3332

5x iProof buffer

4

350

1400

10 mM dNTPs

0.4

350

140

50 mM MgCl2

0.4

350

140

5 uM Illumina Primers

1.33

350

465

iProof TAQ

0.2

350

70

DMSO

0.15

350

52.5

total

16

350

5600

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

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 2.155 ul of the MM directly to the previous PCR

Reagent

ul/rxn

rxns

ul needed (x 1.6)

5x Iproof buffer

0.425

360

153

10 mM dNTPs

0.4

360

144

Primers

1.33

360

479

Total

2.155

360

776

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

Temp C

Cycles

Time

98

1X

3:00

60

1X

2:00

72

1X

10:00

4

1X

0:00

Pool Using PCR Plates with Assist Plus

Organize plates by Library # above, vortex, and quick spin

Use 4GbsPoolx8

Use single channel to combine 48 ul from each well of a column into a separate labeled tube.

Pippin Prep Size Select (300-366 bp select):

 

Run Final Product on qPCR for check and quant

Result from qPCR check:

load =800 pM

dilute 1 nM PhiX to 500 pM

Run Final Products on Tapestation for size check

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