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Master Mixes used with links to QC pages

10-20-22_AmpliconMM : QC

PCR

  • Pull Out 5FB1_Norm and allow to thaw; wash hands before proceeding.

  • Pull Out 4 hard shell, full skirt plates and label them 7-5FB1_16S1, 7-5FB1_16S2, 7-5FB1_ITS1, and 7-5FB1_ITS2

  • Pull Out 10-20-22_AmpliconMM_1 and allow to thaw

  • Pull Out long16S0C1, long16S0D1, longITS0C1, and longITS0D1 and vortex and spin down

  • Add 11 ul MM to each well of the 4 hard shell, full skirt plates. Save MM remainder in a clean 2 ml tube. Transfer label.

  • Add 2 ul 5FB1 Norm to each plate

  • Add 2 ul from one of the primer plates to each plate. Seal, vortex, and spin.

Run on Thermocycler Program GSAF36:

Temp C

Cycles

Time

95*

1X

3:00*

98

36X

0:30

62

36X

0:30

72

36X

0:30

72

1X

5:00

4

1X

0:00

  • Remember to save any remaining MM in a 2 ml tube, transfer label from 5 ml, and return to -20 for possible future retesting.

MagBead Cleanup:

Some plates were cleaned up using the Nimbus platform protocol “AxyPrep MagBead PCR1 No MM”

Manually, it was done:

  • Equilibrate Beads to room Temperature

  • Add 24 ul of MagBeads to each well and 15 ul of replicate to same well of replicate

  • 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)

  • Store in -20 until ready to qPCR

qPCR NovaSeq5_ConTest1

  • Make 1:1000 dilutions of column 8 from the PCR plates by adding 1 ul to 999 ul TE in a deep well plate:

 

1

2

3

4

5

6

7

8

9

10

11

12

A

NTC

NTC

NTC

B

0.0002 pM Std

0.0002 pM Std

0.0002 pM Std

C

0.002 pM Std

0.002 pM Std

0.002 pM Std

D

0.02 pM Std

0.02 pM Std

0.02 pM Std

E

0.2 pM Std

0.2 pM Std

0.2 pM Std

F

2 pM Std

2 pM Std

2 pM Std

G

20 pM Std

20 pM Std

20 pM Std

H

 

 

 

  • Add 16 ul of Illumina Library Quantification MasterMix to each well:

ul/rxn

Reagent

# of rxns

ul needed

10 ul

KAPA SYBR FAST qPCR MM (2X)

110

1100

2 ul

Primer Premix (10X)

110

220

4 ul

Ultra Pure Water

110

440

16 ul

Total Volume

110

1760

  • Add 4 ul of template, pool, or standards to each well:

 

1

2

3

4

5

6

7

8

9

10

11

12

A

20 pM Std

20 pM Std

20 pM Std

B

2 pM Std

2 pM Std

2 pM Std

C

0.2 pM Std

0.2 pM Std

0.2 pM Std

D

0.02 pM Std

0.02 pM Std

0.02 pM Std

E

0.002 pM Std

0.002 pM Std

0.002 pM Std

F

0.0002 pM Std

0.0002 pM Std

0.0002 pM Std

G

NTC

NTC

NTC

H

NTC

NTC

NTC

Results:

Plate Name

Average Result (nanomoles)

Full qPCR results below:

 Sequencing Test:

Dilute to 1 nM based off qPCR results. qPCR results are in pM, but 1:1000 dilution used. The results are effectively in nM for pool.

  • 1000/Results = ul of Pool to Add

100/8.4 = 12uL of Pool to Add

  • 100 - uL of Pool to Add = ul of “10 mM Tris 8.5” to Add

100- 12 = 82 uL of 10mM Tris 8.5

Dilute 1 nM full pool to loading concentration of 60 pM:

  • Add 6 ul 1 nM Pool to 82 ul “10 mM Tris 8.5” and 12 ul 50 pM PhiX

  • Remove iSeq 100 i1 Flow Cell from refrigerator 5’s crisper drawer and open white foil pack and allow to equilibrate to RT for 10-15 minutes.

  • Open “iSeq 100 i1 Reagent Cartridge v2”. Turn on iSeq100

  • Click on “Sequence”. Watch Video. Do what video tells you to do. Follow on screen instructions until run starts.

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