1TYM Sage Grouse

Samples arrived Samples checked in against list .

Extractions

Freeze dry samples
Extract using MN Nucleospin 96 Stool kits following spin speeds from MN Nucleospin 96 Soil kits
Transfer DNAs to plate
Transfer 30 ul as working aliquot
Normalize to 5 ng/ul

Dilute and Array fullITS Primers

Primers arrived 100uM in 50 ul

Add 575 to get primers to 8 uM with Integra Pipette using Pipette/Mix setting

Add 87.5 ul TE to new Primer plates

Use Nimbus to array first twelve plates using FULLITS_Primer_Prep_Adjustable 

TRNL PCR MasterMix

ul/rxn

Reagent

# of rxns

ul needed

ul/rxn

Reagent

# of rxns

ul needed

3

5X Kapa HiFi Buffer

450

1350

0.45

10M dNTPs

450

202.5

0.3

Kapa HiFi HotStart DNA Pol

450

135

7.25

HPLC H2O

450

3263

11

Total Volume

450

4950

  • Add 11 ul to each well of a hard shell, full skirt plate. Add 2 uL of primers and 2uL of template to each well.

fullITS PCR MasterMix

ul/rxn

Reagent

# of rxns

ul needed

 

ul/rxn

Reagent

# of rxns

ul needed

 

3

5X Kapa HiFi Buffer

450

1350

600

0.45

10M dNTPs

450

202.5

90

0.3

Kapa HiFi HotStart DNA Pol

450

135

60

8.25

HPLC H2O

450

3713

1650

12

Total Volume

450

5400

2400

 

Plate

TRNL Primers

fullITS Primers

Plate

TRNL Primers

fullITS Primers

1TYM1

TRNL19

fullITS05

TRNL20

fullITS06

1TYM2

TRNL17

fullITS07

TRNL18

fullITS08

1TYM3

TRNL21

fullITS09

TRNL22

fullITS10

1TYM4

TRNL23

fullITS11

TRNL24

fullITS12

1TYM5

TRNL16

fullITS02

Template Format:

Run TRNL plates on thermocycler program TRNL_T*:

Step

Temp C

Cycles

Time

Step

Temp C

Cycles

Time

Denature

95

1X

10:00

Denature

95

35X

0:30

Annealing

55

35X

0:30

Extension/Elongation

72

35X

0:30

Hold

4

1X

0:00

Run fullITS plates on thermocycler program fullITS:

Step

Temp C

Cycles

Time

Step

Temp C

Cycles

Time

Denature

95

1X

10:00

Denature

94

35X

0:30

Annealing** (Row C)

55

35X

0:40

Extension/Elongation

72

35X

1:00

Final Extension

72

1X

10:00

Hold

4

1X

0:00

MagBead Cleanup:

  • Equilibrate Beads to room Temperature

  • Add 15uL of ultra pure water to each well.

  • Add 24 ul of MagBeads to each well.

  • Pipette mix up and down 10 times.

  • Incubate at RT for 5 minutes

  • Secure plate on magnet plate; incubate at RT for 5 minutes (until wells are clear)

  • Remove 65 ul from each well; keep tips to left or right depending on the column to avoid bead pellet.

  • Add 100 ul Fresh 80% EtOH to each well. Incubate 30 seconds. Remove 100 ul from each well

  • Add 100 ul Fresh 80% EtOH to each well. Incubate 30 seconds. Remove 100 ul from each well

  • Reaspirate from each well to assure maximum EtOH removal

  • Allow plate to air dry for 7 minutes.

  • Remove sample plate from magnet plate.

  • Add 40 ul TE; pipette mix 10+ times. Incubate 2 minutes at RT.

  • Place sample plate back on magnet for 5 minutes or until all wells are cleared.

  • Transfer 40 ul to labeled transparent plate (Plate name_PCR_MIDs)

Normalize to 5 ng/ul

qPCR

 

Sequencing

Pool 2 parts TRNL with 2 parts fullITS and 1 part Baldwin CO1-Lark.

TRNL starting 2.77

FI starting 1.62

BALD starting 3.23

1 nM 1TYM_TRNL: 36 ul pool with 64 ul RSB

1 nM 1TYM_FI: 62 ul pool with 38 ul RSB

1 nM 1BALD_CO1: 31 ul pool with 69 ul RSB

 

Load Pool:

18 ul 1nM 1Bald

36 ul 1nM 1TYM_FI

36 ul 1nM 1TYM_TRNL

9 ul 1 nM PhiX

1 ul RSB