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Illumina DNA Prep

Measure DNA concentration via Synergy HTX
- If samples are above 16 ng/ul, normalize that sample between 4 and 16 ng/ul.
  - If more than 5 samples per plate, use Nimbus to normalize to 10 ng/ul
Add 30 ul of each sample to hard shell 96 well plate
Bring BLT and TB1 to RT
Add 20 ul Tagmentation Master Mix after vortexing:

...

Place plate on magnetic stand and allow to clear 3 minutes
Remove and discard supernatant
Remove plate from magnets
Slowly add 100 ul TWB directly to beads, pipette slowly until resuspended
Place plate on magnetic stand and allow to clear 3 minutes
Remove and discard supernatant
Remove plate from magnets
Slowly add 100 ul TWB directly to beads, pipette slowly until resuspended
Place plate on magnetic stand and allow to clear at least 3 minutes, leave until ready next MM is ready to add:

ul per Rxn	Reagent	Thaw notes	Rxns	ul Needed
22	EPM	On ice, invert to mix, quick spin
22	H2O	At RT, vortex, quick spin

Remove Supernatant
Remove fro from magnet
Add 40 ul MM from above and pipette to resuspend
Seal and quick spin
10 ul pre paired i7 and i5 index adapters
Pipette 40 ul up and down to mix
Run on Cycler Program:

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Spot Check preps via qPCR and/or bioanalyzer

MyBaits:

1st Hybridization

Pool 4+ libraries together in equal volumes
Prepare Hybridization MM:

ul per Rxn	Reagent	Thaw notes
9.25	Hyb N	After RT thaw, heat @60C to dissolve precipitate
3.5	Hyb D
0.5	Hyb S	After RT thaw, heat @60C to dissolve precipitate
1.25	Hyb R
1.1	H2O
4.4	Baits

Incubate Hyb MM at 60C for 10 min
Incubate at RT for 5 min
Add 18.5 ul Hyb MM to Hyb rxn tubes, HYB (0.2 ml)
Add 5 ul Blockers Mix to separate LIB tube:

ul per Rxn	Reagent	Thaw notes	Rxns	ul Needed
	Block O
	Block C
	Block X

Add 7 ul of a library pool to each Blocker Mix (LIB) and mix by pipette
Add LIBs to Cycler running:

Temp	Time (mm:ss)	Cycles
95 C	5:00
60 C*	5:00
60 C	0:00

Once Cycler reaches temp for step 2, add HYBs to cycler
After step 2 completes, transfer 18 ul from HYBs to each LIB
Incubate overnight 16 - 24 hours

Wash

Make and Heat Wash Buffer X at 60 C for >30 minutes:

ul per Rxn	Reagent	Thaw notes	Rxns	ul Needed
5.88	Hyb S
147	Wash Buffer
582.35	H2O

Aliquot 30 ul beads per rxn to 0.2 ul strip tubes
Place on magnet for 1-2 minutes
Discard supernatant
Add 200 ul Binding Buffer, vortex to resuspend, and quick spin
Place on magnet for 1-2 minutes
Discard Supernatant and return to step 4 twice more
Resuspend in 70 ul Binding Buffer
Heat Bead Aliquots to 60C for 2 minutes
Transfer 30 ul LIBs to Heated Beads, pipette to mix
Incubate for 5 minutes, agitate after 2.5 minutes
Transfer Tubes to magnet and allow to clear
Add 180 ul warmed Wash Buffer X, incubate at 60 C for 15 s, vortex and spin
Incubate for 5 minutes at 60 C, agitate at 2.5
Place on Magnet until solution clears
Discard supernatant
Return to step 12 for 4 total washes
Discard residual supernatant
Add 30 ul Buffer E And thoroughly resuspend off magnet
Incubate at 95 C for 5 minutes
Place on Magnet until solution clears and transfer 15 ul of supernatant to 2 tubes with PCR MM:

ul per Rxn	Reagent	Thaw notes
10	5X KAPA HF Buffer
1.5	10M dNTPs
1	Kapa HiFi HotStart DNA Pol	Thaw on ice, flick to mix
1	F and R FlowCell Primers
21.5	H2O

Run on Cycler Program:

Temp C	Cycles	Time
95*	1X	3:00
98	14X	0:20
60	14X	0:30
72	14X	0:45
72	1X	5:00
8	1X	0:00

2nd Hybridization

Pool 4+ libraries together in equal volumes
Prepare Hybridization MM:

ul per Rxn	Reagent	Thaw notes
9.25	Hyb N	After RT thaw, heat @60C to dissolve precipitate
3.5	Hyb D
0.5	Hyb S	After RT thaw, heat @60C to dissolve precipitate
1.25	Hyb R
4.4	H2O
1.1	Baits

Incubate Hyb MM at 60C for 10 min
Incubate at RT for 5 min
Add 18.5 ul Hyb MM to Hyb rxn tubes, HYB (0.2 ml)
Add 5 ul Blockers Mix to separate LIB tube:

ul per Rxn	Reagent	Thaw notes	Rxns	ul Needed
	Block O
	Block C
	Block X

Add 7 ul of a library pool to each Blocker Mix (LIB) and mix by pipette
Add LIBs to Cycler running:

Temp	Time (mm:ss)	Cycles
95 C	5:00
60 C*	5:00
60 C	0:00

Once Cycler reaches temp for step 2, add HYBs to cycler
After step 2 completes, transfer 18 ul from HYBs to each LIB
Incubate overnight 16 - 24 hours

Wash

Make and Heat Wash Buffer X at 60 C for >30 minutes:

ul per Rxn	Reagent	Thaw notes	Rxns	ul Needed
5.88	Hyb S
147	Wash Buffer
582.35	H2O

Aliquot 30 ul beads per rxn to 0.2 ul strip tubes
Place on magnet for 1-2 minutes
Discard supernatant
Add 200 ul Binding Buffer, vortex to resuspend, and quick spin
Place on magnet for 1-2 minutes
Discard Supernatant and return to step 4 twice more
Resuspend in 70 ul Binding Buffer
Heat Bead Aliquots to 60C for 2 minutes
Transfer 30 ul LIBs to Heated Beads, pipette to mix
Incubate for 5 minutes, agitate after 2.5 minutes
Transfer Tubes to magnet and allow to clear
Add 180 ul warmed Wash Buffer X, incubate at 60 C for 15 s, vortex and spin
Incubate for 5 minutes at 60 C, agitate at 2.5
Place on Magnet until solution clears
Discard supernatant
Return to step 12 for 4 total washes
Discard residual supernatant
Add 30 ul Buffer E And thoroughly resuspend off magnet
Incubate at 95 C for 5 minutes
Place on Magnet until solution clears and transfer 15 ul of supernatant to 1 tubes with PCR MM and 1 without:

ul per Rxn	Reagent	Thaw notes
10	5X KAPA HF Buffer
1.5	10M dNTPs
1	Kapa HiFi HotStart DNA Pol	Thaw on ice, flick to mix
1	F and R FlowCell Primers
21.5	H2O

Run on Cycler Program:

Temp C	Cycles	Time
95*	1X	3:00
98	8X	0:20
60	8X	0:30
72	8X	0:45
72	1X	5:00
8	1X	0:00

Version	Old Version 2	New Version 3
Changes made by	Gregg Randolph	Gregg Randolph
Saved on	Aug 17, 2021	Aug 18, 2021

Versions Compared

Key

Illumina DNA Prep

Spot Check preps via qPCR and/or bioanalyzer

MyBaits:

1st Hybridization

Wash

2nd Hybridization

Wash