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  • 36 total samples to be processed in 6 batches

    • Batch1: 2 sample batch

    • Batch2: 2 sample batch

    • Batch3: 16 samples

    • Batch4: 16 samples

Sample

Processing number

Batch

Index

1

1

2

1

3

2

4

2

5

3

6

3

7

3

8

3

9

3

10

3

11

3

12

3

13

3

14

3

15

3

16

3

17

3

18

3

19

3

20

3

21

4

22

4

23

4

24

4

25

4

26

4

27

4

28

4

29

4

30

4

31

4

32

4

33

4

34

4

35

4

36

4

1Cell Preparation

  • B1
  • B2
  • B3
  • B4
  • Thaw and stage capture and lysis materials
    • Thaw one PIP tube per sample and RNase Inhibitor on ice
    • Stage at RT Partitioning Reagent, Chemical Lysis Buffer 3
    • Stage Combination 1.5 ml/0.5 ml tube stand, P200 and P1000 wide and standard
    • Stage one 0.5 ml tube per sample
  • Warm Cell Suspension Buffer to 37 C and cell suspension if frozen for 60-90 seconds
    • decontaminate cell vial with 70% isopropyl alcohol
    • thaw remaining ice at RT 30-60 sec
    • Use a wide bore P1000 to gently mix and transfer to 15 ml conical tube
    • Slowly add 9 ml warmed thawing media (>30s)
  • Centrifuge cells at 200 xg for 5 minutes to pellet
  • Aspirate as much supernatant as possible without disturbing pellet
  • Add 1 ml prewarmed Cell Suspension Buffer, gently mix with wide bore P1000
    • Place remaining Cell Suspension Buffer on ice
  • Centrifuge at 200 x g for 3 min
  • Aspirate as much supernatant as possible
  • Use standard bore P100 to add 200-400 ul cold Cell Suspension Buffer and gently mix to resuspend 10-15 times
  • Measure cell count
  • Use wide bore P1000 to prepare 1,250 live cells/ul in Cell Suspension Buffer
  • Measure cell count, repeat 9 and 10 until cell count reached
    • place on ice

Capture and Lysis

  • Centrifuge Thawed PIP tubes for ~5 seconds and return to ice
  • Preheat Dry Bath with 0.5 ml block to 25 C (lid +5C or 30 C)
  • Use P200 wide bore to gently mix cell suspension 10x
  • Add 4 ul cell suspension directly into PIPs
  • Add 1-2 ul RNase Inhibitor directly into PIPs slowly
  • Mix PIP mix with standard bore low retention P200 at 25 ul (avoid bubbles) 10x
  • Add 280 ul Partitioning Reagent down the side of tube
  • Cap tubes and place in the yellow rotating vortex adapter in horizontal config
    • vortex 3000 rpm 15 sec
    • rotate adapter to vertical config and vortex 3000 rpm for 2 minutes
  • Place PIP tubes in 0.5 ml side of stand. Let stand 30 s
  • Place a P200 set at 115 ul toward bottom of tube and wait 5 s then slowly aspirate
  • Repeat above: P200 at bottom, 5 s, slowly aspirate
  • Check Chemical Lysis Buffer 3 for crystals, if present warm w dry bath, vortex 10s, centrifuge
  • Add 40 ul CLB 3 to each 0.5 ml tube with low retention P200
  • Add 120 ul Partitioning Reagent to each 0.5 ml tube
  • Vortex 0.5 ml tube 10s, then immediately pipette 160 ul to PIP
  • Mix PIPs by inversion >10x
  • Insert PIP tubes into dry bath and select skip and yes to run:

T2 PIP Cell Lysis

Preheat

25 C

0:00

Step 1

25 C

15:00

Step 2

37 C

45:00

Step 3

25 C

10:00

Step 4

20 C

0:00

HOLD POINT IN DRY BATH UP TO 96 HOURS

mRNA isolation

  • B1
  • B2
  • B3
  • B4
  • Thaw and stage materials
    • Thaw at RT Breaking Buffer for >20 m, DePartitioning Reagent
    • On ice Washing Buffer, RT Additive Mix V, one tube TSO per 2 samples
    • Stage and label per sample 1.5 ml Safe Locks, 1.5/0.5 ml stand, red PIPseq guide rack
      • Aliquot 1 ml Washing Buffer into 1.5 ml tubes and place in ice
    • 0.2 ml 8 tube strips and lids
  • Remove PIPtubes and place in blue stand, allow to settle for 30s if needed
  • Place P200 at bottom of tube slowly, wait 5 s, aspirate ~130ul slowly, wipe tip along side slowly
  • Add 200 ul Breaking Buffer to each PIP along side
  • Add 40 ul DePartitioning Reagent to each PIP along side
  • Invert to break emulsion 10-20x
  • Centrifuge for 10s
  • Ensure distinct interface between pink bottom and cloudy top
    • if not, add 4 ul DePartitioning and repeat inversion and centrifuge
  • Remove ALL pink and red layers with P200
  • Centrifuge 10 s
  • Remove ALL remaining pink with a P20, place 0.5 ml tubes on ice
  • Use P200 to slowly transfer 180 ul PIPs to chilled Wash in 1.5 ml tubes
  • Briefly centrifuge 0.5 ml tubes
  • Repeat transfer of another 180 ul to 1.5 ml tubes
  • Place tubes in blue stand and vortex horizontally for 3 s
  • Centrifuge 1 m, turn off for gradual slow
  • Gently Place tubes back in rack
  • Aspirate slowly and discard supernatant to the 4 or L mark on stand
  • Wash2
    • Add 1 ml Washing Buffer, vortex in stand horizontally 3 sec, centrifuge 1 m
    • Gently place in rack, Aspirate slowly and discard supernatant to the 4 or L mark on stand
  • Wash3
    • Add 1 ml Washing Buffer, vortex in stand horizontally 3 sec, centrifuge 1 m
    • Gently place in rack, Aspirate slowly and discard supernatant to the 4 or L mark on stand
  • Wash4
    • Add 1 ml Washing Buffer, vortex in stand horizontally 3 sec, centrifuge 1 m
    • Gently place in rack, Aspirate slowly and discard supernatant to the 4 or L mark on stand
  • Move ~100 ul (ALL) into 0.2 ml tube (PCR strip) cap
  • Spin 5 s at 2000 xg and place in red rack
  • Let settle >1 minute
  • Reduce Volume to guide wire, then place on ice

cDNA synthesis

  • Prep Reagents
    • Thaw RT Enzyme Mix on ice
    • Prepare 1:1 Washing Buffer, 600 ul per sample, keep on ice
    • stage ultra pure water
  • Prepare RT Master Mix:

Reagent

Volume per run

2.2

8.8

17.6

RT Additive Mix V

31.1

68.4

273.7

547.4

TSO

3.1

6.8

27.3

54.6

RT Enzyme Mix

4.8

10.6

42.2

84.5

Total

39

85.8

343.2

686.5

  • Mix well by pipetting, centrifuge briefly
  • Add 39 ul RT MM to each 0.2 ml well, mix well by pulse vortexing
  • Centrifuge <1 s
  • Thermocycle with lid at 105C:

Temp

Duration

25 C

30:00

42 C

90:00

85 C

10:00

4 C

0:00

HOLD POINT 4 C in Thermocycler overnight

  • B1
  • B2
  • B3
  • B4
  • Stage Reagents
    • Thaw on ice 4X PCR MM and WTA Primer
    • Stage two 1.5 ml tube and ultra pure water
  • Briefly centrifuge 0.2 ml tubes, then Add 120 ul 0.5X Wash Buffer, seal with new lid
  • Vortex mix for 5 s
  • Centrifuge 5 s, power off centrifuge to slow, and return to red rack
  • Tap guide rack 3 x on bench
  • Let settle 1 minute
  • Aspirate and discard 150 ul
  • Wash2
    • Add 150 ul 0.5 X Washing Buffer, vortex mix 5 s, centrifuge 5s
    • Tap 3 x, let settle 1 minute
    • Aspirate and discard 150 ul
  • Wash3
    • Add 150 ul 0.5 X Washing Buffer, vortex mix 5 s, centrifuge 5s
    • Tap 3 x, let settle 1 minute
    • Aspirate and discard 150 ul
  • Wash4
    • Add 150 ul 0.5 X Washing Buffer, vortex mix 5 s, centrifuge 5s
    • Tap 3 x, let settle 1 minute
    • Aspirate and discard 150 ul
  • Reduce Volume to rack guidewire and place on ice

cDNA Amplification

  • Pipette mix WTA Primer and centrifuge briefly
  • Make 1X WTA Primer (3 ul WTA and 27 ul H2O for the 2 and 2) or (6ul WTA and 54 ul H2O for 8 )
  • Make PCR MM using pipette mixing for reagents

Reagent

V per run

2.2x

8.8x

17.6

4X PCR MM

15

33

132

264

1X WTA Primer

6

13.2

52.8

105.6

Total

21

46.2

184.8

369.6

  • Add 21 ul MM into each PCR tube
    • Pulse vortex in black stand and quick spin down
  • Run on Thermocycler with 105 C lid:

Temp

Time

Cycles (60 ul)

95

3:00

1

98

0:15

5

69

10:00

5

72

5:00

1

4

0:00

1

HOLD POINT 4 C in Thermocycler overnight

Isolate cDNA from PIPs in Post PCR area

  • B1
  • B2
  • B3
  • B4
  • Stage QC reagents on ice
    • 4X PCR MM
    • WTA Primer (do not dilute)
    • Washing Buffer
  • Stage Reagents at RT
    • CE Buffer, low EDTA TE, ultra pure water
    • Illumina Purification Beads (limit light exposure) >20 minutes
    • 0.2 ml tubes or strip tubes and lids
    • Magnet rack
  • Add 40 ul CE Buffer to each WTA rxn and seal with new lids
  • Pulse vortex and spin down
  • Place in guide rack, tap on bench, and wait > 1 minute for PIPs to settle below guide
  • Transfer 60 ul supernatant into a NEW labeled 0.2 ml tube
  • Add another 60 ul CE Buffer to the original tubes
  • Pulse vortex, spin down 5s, load back into guide rack
  • Tap on bench and let settle >1 minute
  • Transfer 60 ul supernatant into tubes containing supernatant
  • Briefly centrifuge supernatant tubes.
  • If PIPs are present, transfer supernatant to new tubes
  • Save remaining PIP pellet at -80C as backup

MagBead Purification

  • Prepare at least 400 ul of fresh 85% Ethanol per rxn (340 ul EtOH and 60 ul ultra pure water)
  • Resuspend Illumina Purification beads via vortex <30s
  • Check Volumes of samples
  • Add 0.8x beads to each sample (96 ul beads for 120 ul sample or sampleX0.8 of beads)
  • Vortex until thoroughly mixed then pulse centrifuge to bring liquid to bottom
  • Incubate 5 min at RT
  • Place tubes in magnetic stand for 5 minutes or until liquid is clear
  • Remove supernatant <216 ul
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Pipette again to remove all EtOH
  • Air Dry for 2-5 minutes
  • Remove from magnet and Add 42 ul low EDTA TE to each sample
    • Pipette mix 10x or until beads are resuspended
  • Incubate 5 minutes at RT
  • Return tubes to magnet for 2 minutes
  • Remove and save 40 ul of supernatant in new tubes and place on ice

cDNA QC of remaining 2 ul

  • Add 9 ul ultra pure water to remaining 2 ul and mix without disturbing beads
  • Incubate 1 minute
  • Transfer 10 ul to new PCR tubes and place on ice
  • Prepare QC MM:

Reagent

V per rxn

2.2X

8.8X

17.6

4X PCR MM

6.25

13.8

55

110

WTA Primer

1

2.2

8.8

17.6

0.5X Washing Buffer

7.75

17

68.2

136.4

Total

15

33

132

264

  • Add 15 ul of QC MM to each 10 ul sample
  • Run on Thermocycler:

Temp

Time

Cycles (25 ul)

95

3:00

1

98

0:15

13

69

4:00

13

72

5:00

1

4

0:00

1

HOLD POINT 4 C in Thermocycler overnight

QC bead cleanup

  • B1
  • B2
  • B3
  • B4
  • Stage Reagents at RT
    • CE Buffer
    • Illumina Purification Beads >20 minutes
    • ultra pure water
    • low EDTA TE
    • tapestation supplies
  • Prepare at least 400 ul of fresh 85% Ethanol per rxn (340 ul EtOH and 60 ul ultra pure water)
  • Add 15 ul ultra pure water to each sample
  • Add 32 ul Illumina Purification Beads, Mix by pipette 15 times with 67 ul
  • Incubate 5 minutes RT
  • Place on Magnet, Incubate 5 minutes
  • Discard ~72 ul supernatant
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Pipette again to remove all EtOH
  • Air Dry for 2-5 minutes
  • Remove from magnet, Add 11 ul low EDTA TE, Mix by pipette >10X
  • Incubate 5 minutes RT
  • Return tubes to magnet for 2 minutes
  • Remove and save 10 ul supernatant for QC
  • Run samples on HS D5000 ScreenTape

Library Prep

  • Stage Reagents at RT
    • Illumina Purification Beads >20 minutes
    • ultra pure water
    • low EDTA TE
  • Thaw Reagents on ice
    • Library Prep Buffer
    • Library Prep Enzymes
    • Library Prep Mix A
    • Library Adapter Mix
    • 4 X PCR MM
    • UDI Library Index Mix Strip
  • Obtain the 40 ul of cDNA and place on ice
  • Pre-Chill Thermocycler
  • Add 10 ul MM to each tube:

Reagent

V per sample

2.2

8.8

17.6

Library Prep Buffer

4

8.8

35.2

70.4

Library Prep Enzymes

6

13.2

52.8

105.6

  • Vortex to mix 5-10s
  • Thermocycle with lid at 105C:

Temp

Time. (50ul)

4

0:00

30

6:00

65

30:00

4

0:00

  • Prepare Library Adapter Mix

Reagent

V per rxn

2.2

8.8

17.6

Library Adapter Mix

0.75

1.7

6.6

13.2

Ultra Pure Water

4.25

9.3

37.4

74.8

  • Add 5 ul to each rxn
  • Pipette mix Library Prep Mix A 15X at ~130 ul and place on ice
  • Add 20 ul to each sample (viscous)
  • Pipette Mix 10X at 40 ul, brief centrifuge to collect
  • Incubate 20 C for 20 minutes (no heated lid)
  • Prepare at least 400 ul 85% EtOH per sample
  • Resuspend Illumina Purification Beads by vortex < 30s
  • Remove ligation rxn from incubation
  • Add 60 ul Illumina Purification Beads to each sample, pipette mix
  • Incubate 5 minutes at RT
  • Place on magnet 5 minutes
  • Remove ~135 ul supernatant
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Pipette again to remove all EtOH
  • Air Dry for 2-5 minutes
  • Remove from magnet and add 34 ul ultra pure water, Pipette mix >10X at 32.5 ul
  • Incubate 5 minutes at RT
  • Return tubes to magnet for 2 minutes
  • Transfer 32.5 ul to new 0.2 ml tubes, store on ice
  • Thaw 4X PCR MM and UDI Index Mix strip
  • Add 5 ul Unique UDI Library Index Mix to each tube and record
  • Add 12.5 ul 4X PCR MM
  • Pipette Mix 10X at 32ul
  • Thermocycle with lid at 105C:

Temp

Time

Cycles

98

0:45

1

98

0:15

16

67

0:30

16

69

0:45

16

72

1:00

1

4

0:00

Hold

HOLD POINT 4 C in Thermocycler overnight

  • B1
  • B2
  • B3
  • B4
  • Stage Reagents
    • Illumina Purification Beads >20 minutes
  • Prepare at least 400 ul 85% EtOH per sample
  • Resuspend Beads by vortex
  • Add 45 ul to PCR rxns
  • Add 76 ul Illumina Purification Beads to each
  • Mix by pipette 15X at 160 ul
  • Incubate 5 minutes at RT
  • Place tubes on Magnet for 5 minutes
  • Discard ~172 ul supernatant
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Add 200 ul 85% EtOH, incubate 30 s, and discard
  • Pipette again to remove all EtOH
  • Air Dry for 2-5 minutes
  • Remove tube(s) from magnet, Add 21 ul low EDTA TE, Mix pipette 10X 20ul
  • Incubate 5 minutes at RT
  • Return tubes to magnet for 2 minutes
  • Transfer 20 ul supernatant to new tubes

HOLD POINT -20 C long term

  • B1
  • B2
  • B3
  • B4
  • Tape Station Each library
  • qPCR or Qubit each library
  • No labels