CTR:Notebook/Migrant/2017/06/14: Difference between revisions

Latest revision as of 02:19, 27 September 2017

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BestRAD Library Prep - COLO Plate 1 and COYE Plate 2

96 well plate of 100ng of DNA in 10uL volume

Digestion (2017-06-14)
- Mix and add to each well:
  - 0.68 uL water
  - 1.20 uL NEBuffer 4
  - 0.12 uL SbfI-HF
- Incubation:
  - COLO P1, RAPDIG on TONY
  - COLO P2, BEDIG on SORK
- 37 degrees for 60 minutes
- 80 degrees for 20 minutes

BestRAD SbfI adapter ligation (2017-06-14)
- Add 2 uL annealed BestRAD SbfI adapters (50nM) to each well, using newly diluted plate of adaptors sent from UC Berkeley June 2016
- Mix and add to each well:
  - 1.28 uL water
  - 0.40 uL NEBuffer 4
  - 0.16 uL ATP
  - 0.16 uL T4 Ligase
- Incubation:
  - COLO P1, RAPLIG on TONY
  - COLO P2, BESTLIG on SORK
- 20 degrees for overnight (16 hours)
- 65 degrees for 20 minutes

1st Clean up (2017-06-15)
- Take 8 uL from each well and combine to 1.7 mL tube, split entire volume into 2 separate tubes
- AMPure bead clean up:
  - Used 380 uL beads to DNA (1:1), per tube
  - 2 washes of 800 uL 80% EtOH each
  - Elute in 105 uL Low TE per tube

Sonication (2017-06-15)
- BioRuptor NGS: 10 cycles of 15 seconds on, 90 seconds off, High Power
- Combined both tubes of sheared DNA and ran on a gel

1) 2uL COLO P1 sheared DNA 2) 2uL 100bp low scale ladder, 3) 2uL COLO P2 sheared DNA

Bind Ligated fragments to Dynabeads(2017-06-15)
- Transfer 200 μL of prepared Dynabeads to the tube of sonicated DNA (~200 μL)
- 3 washes of 150 μL 1X B+W Buffer
- 2 washes with 150 μL 56°C 1X B+W Buffer

Liberate DNA from Dynabeads(2017-06-15)
- 2 washes of 100ul 1X NEB Buffer 4
- Resuspend beads in 40 μL of 1X NEB Buffer 4
- Add 2 μL of SbfI-HF
- Incubate tube at 37°C for 60 min.(LIBDNA on JOHN, Block B)

2nd Clean up (2017-06-19)
- Take 45 uL of supernatant
- AMPure bead clean up:
  - Used 45 uL beads to DNA (1:1)
  - 2 washes of 200 uL 80% EtOH
  - Elute in 56 uL LowTE

Blunt End Repair (2017-06-19)
- Mix:
  - 55.5 uL fragmented DNA
  - 3.0 uL End Prep Enzyme Mix
  - 6.5 uL End Repair Reaction Buffer
- Incubation (NEBENDRP on JOHN Block B):
  - 20 degrees for 30 minutes
  - 65 degrees for 30 minutes

NEBNext adapter ligation (2017-06-19)
- Add to mix:
  - 15.0 uL Blunt/TA Ligase Master Mix
  - 2.5 uL NEBNext adaptor for Illumina (1.5 uM)
  - 1.0 uL Ligation Enhancer
- Incubation (NEBLIGAT on JOHN Block B):
  - 20°C for 15 minutes
- Added 3 μL of USER enzyme to ligation mixture.
- Incubation (USERENZ on JOHN Block B)
  - 37°C for 15 minutes

Size selection (2017-06-19)
- Add 16.5 uL water for a total of 100 uL
- AMPure bead size selection:
  - 45 uL beads to remove large fragments
  - 25 uL beads to remove small fragments
  - 3 washes of 200 uL 80% EtOH
  - Elute in 20 uL LowTE

First Test PCR amplification (2017-06-19)
- Mix:
  - 5 uL DNA
  - 25 uL NEBNext Q5 Hot Start HiFi PCR Master Mix
  - 10 uL H₂Owater
  - 5 uL Index 1 Primer (10 uM)
  - 5 uL Universal PCR Primer (10 uM)
- PCR cycle (BestRAD TestPCR on SORK Lab's Thermocycler):
  - 98°C for 30 seconds
  - 15 cycles of:
    - 98°C for 10 seconds
    - 65°C for 75 seconds
  - 65°C for 5 minutes

1) 5uL COLO P1 PCR Product 2) 2uL 100bp low scale ladder, 3) 5uL COLO P2 PCR Product

Final PCR amplification (2017-06-19)
- Mix:
  - 15 uL DNA
  - 25 uL NEBNext Q5 Hot Start HiFi PCR Master Mix
  - 5 uL Index 1 Primer (10 uM)
  - 5 uL Universal PCR Primer (10 uM)
- PCR cycle (BestRAD FinalPCR on SORK Lab's Thermocycler):
  - 98°C for 30 seconds
  - 10 cycles of:
    - 98°C for 10 seconds
    - 65°C for 75 seconds
  - 65°C for 5 minutes

1) 5uL COLO P1 PCR Product 2) 2uL 100bp low scale ladder, 3) 5uL COLO P2 PCR Product

Size Selection Bead Clean Up (2017-06-22)
- Add 55 uL low TE for a total of 100 uL
- AMPure bead size selection:
  - 45 uL beads to remove large fragments
  - 25 uL beads to remove small fragments
  - 3 washes of 200 uL 80% EtOH
  - Elute in 30 uL LowTE

Qubit:
- Plate 1: 2.2 ng/μL
- Plate 2: 2.04 ng/μL

Run 1μL on BioAnalyzer DNA High Sensitivity Chip (2017-06-23)

Plate 1:

Plate 2:

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+|style="background-color: #F2F2F2" align="center"|[[File:Report.png|frameless|link={{#sub:{{FULLPAGENAME}}|0|-11}}]][[{{#sub:{{FULLPAGENAME}}|0|-11}}|Main project page]]<br />{{#if:{{#lnpreventry:{{FULLPAGENAME}}}}|[[File:Resultset_previous.png|frameless|link={{#lnpreventry:{{FULLPAGENAME}}}}]][[{{#lnpreventry:{{FULLPAGENAME}}}}{{!}}Previous entry]]&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;}}{{#if:{{#lnnextentry:{{FULLPAGENAME}}}}|[[{{#lnnextentry:{{FULLPAGENAME}}}}{{!}}Next entry]][[File:Resultset_next.png|frameless|link={{#lnnextentry:{{FULLPAGENAME}}}}]]}}
 |-
 | colspan="2"|
@@ Line 138: / Line 138: @@
 *Qubit:
-**Plate 1:  ng/μL
+**Plate 1: 2.2 ng/μL
-**Plate 2:  ng/μL
+**Plate 2: 2.04 ng/μL
 *Run 1μL on BioAnalyzer DNA High Sensitivity Chip (2017-06-23)
 *Plate 1:
-[[CTR:500px|500px]]
+[[Image:COLO P1 Bioanalyzer.JPG|500px]]
 *Plate 2:
-[[CTR:500px|500px]]
+[[Image:COLO P2 Bioanalyzer.JPG|500px]]
-*[ Bioanalyzer Results]

CTR:Notebook/Migrant/2017/06/14: Difference between revisions

Latest revision as of 02:19, 27 September 2017

BestRAD Library Prep - COLO Plate 1 and COYE Plate 2

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