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Test samples were previously extracted.

  1. Make sample spreadsheet and plate test samples by adding 30uL of sample to the corresponding well.

  2. Quantify samples on Synergy HTX.

  3. Normalize samples to 10ng/uL.

  4. Choose 4 plant and 4 stool to run PCR test.

  5. Make 1 step PCR MMX and plate in the template format below (Replace P1, P2, …. and S1, S2… with actual sample names):

PCR MasterMix

ul/rxn

Reagent

# of rxns

ul needed

3

5X Kapa HiFi Buffer

110

330

0.45

10M dNTPs

110

49.5

0.3

Kapa HiFi HotStart DNA Pol

110

33

7.25

HPLC H2O

110

797.5

11

Total Volume

110

1210

  • 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.

  • Primers: _______________ (fill in when primers arrive).

Template Format:

1

2

3

4

5

6

7

8

9

10

11

12

A

P1

P2

P3

P4

S1

S2

S3

S4

B

P1

P2

P3

P4

S1

S2

S3

S4

C

P1

P2

P3

P4

S1

S2

S3

S4

D

P1

P2

P3

P4

S1

S2

S3

S4

E

P1

P2

P3

P4

S1

S2

S3

S4

F

P1

P2

P3

P4

S1

S2

S3

S4

G

P1

P2

P3

P4

S1

S2

S3

S4

H

P1

P2

P3

P4

S1

S2

S3

S4

Run on thermocycler program TRNL_T*:

Step

Temp C

Cycles

Time

Denature

95

1X

10:00

Annealing

95

35X

0:30

Annealing** (Row E)

50

35X

0:30

Extension/Elongation

72

35X

2:00

Hold

4

1X

0:00

*TRNL_T program will test the efficiency of the PCR/annealing temperature by running it on a temperature gradient for each row. The table below shows the annealing temperature for each row.

**

Row

Annealing Temperature

A

60

B

57

C

55

D

53

E

50

F

48

G

46

H

44

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 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)

qPCR TRNL_Test

  • Make 1:1000 dilutions of column 1,2,3 and 6,7,8 from the PCR plates by adding 1 ul to 999 ul TE in a deep well plate: (Will fill in with proper sample names.)

 

1

2

3

4

5

6

7

8

9

10

11

12

A

P1_A

P2_A

P3_A

P4_A

S1_A

S2_A

S3_A

S4_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

P1_A

P2_A

P3_A

P4_A

S1_A

S2_A

S3_A

S4_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

 

 

 

 

Results:

Average results

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