Tuesday, July 26th
Agenda:
- Troubleshoot uneven gel running
- Review constructs
- Human practices
- Find protocols for next steps
- Ligate GFP and mCherry parts into the storage vector
- Look into Weinberg and Provost travel grants
Tasks:
Jordan
- Reran sfGFP and mCherry PCR with Sara
- Procedure:
- 2.5 uL 10X PCR buffer
- 0.5 uL 10 mM dNTPs
- 0.5 uL of forward primer at 10 mM
- 0.5 uL of reverse primer at 10 mM
- 0.5 uL template (Shu's miniprep GFP and mCherry products)
- 0.25 Taq polymerase
- 20.25 uL H20
- PCR settings:
- Denature: 95°C, 7 s.
- Anneal: 51°C, 43 s.
- Elongate 72°C, 2 m
- Funds organization
- Reworked CLP letter
Michelle
- Made Kan Plates:
- 350 mL LB
- 1.75 mL Kanamycin (10 mg/mL) (to 50 ug/mL working concentration)
- Poured 1.25 sleeve’s worth of plates
- Made Tet Plates
- 300 mL LB
- 0.6 mL Tetracycline (5 mg/mL) (to 10 ug/mL working concentration)
- Poured 1 sleeve’s worth of plates
- Made LB Stock
- 10.03 g Tryptone
- 1 mL 1N NaOH
- 5.02 g Bacto Yeast extract
- 5.04 g NaCl
- Made 1X TAE
- 100 mL 10X TAE
- 900 mL dH20
Paul
- Sent Cas9 minipreps to sequencing
- Ran gels on GG PCR products (sfGFP & mCherry)
- Ran PCR on GFP&mCherry (Ta=56¯C)
- Sequencing Premix Protocol (use small 600 uL tubes)
- 1 template+1 primer per tube
- 450-600 ng of DNA template (~100-800)
- 1.2 uL of 10 uM primer
- Water to 15 uL
- Submit sequencing through Genesifter account
Sara
- Reran sfGFP and mCherry PCR with Sara
- Procedure:
- 2.5 uL 10X PCR buffer
- 0.5 uL 10 mM dNTPs
- 0.5 uL of forward primer at 10 mM
- 0.5 uL of reverse primer at 10 mM
- 0.5 uL template (Shu's miniprep GFP and mCherry products)
- 0.25 Taq polymerase
- 20.25 uL H20
- PCR settings:
- Denature: 95°C, 7 s.
- Anneal: 51°C, 43 s.
- Elongate 72°C, 2 m
- Loaded the samples into the gels with Paul
- Troubleshot too-concentrated primers in PCR reaction
Shu
- Transformation of mRFP in pSB1T3
- Sent Tyler Josh’s slides
Tasfia
- Cleaned up miniprepped INP PCR product (80.2 ng/uL final concentration)
- Autoclaved LB
- Poured Tet plates (see Michelle’s notes for details)
Tyler
- Sequencing Cas9 preparation
- Reviewed SS Primers, created more mRFP guides, sent to Kelly
- Began reviewing Josh’s modeling slides from Shu, emailed Joe about meeting time
Jordan
- Reran sfGFP and mCherry PCR with Sara
- Procedure:
- 2.5 uL 10X PCR buffer
- 0.5 uL 10 mM dNTPs
- 0.5 uL of forward primer at 10 mM
- 0.5 uL of reverse primer at 10 mM
- 0.5 uL template (Shu's miniprep GFP and mCherry products)
- 0.25 Taq polymerase
- 20.25 uL H20
- PCR settings:
- Denature: 95°C, 7 s.
- Anneal: 51°C, 43 s.
- Elongate 72°C, 2 m
- Procedure:
- Funds organization
- Reworked CLP letter
Michelle
- Made Kan Plates:
- 350 mL LB
- 1.75 mL Kanamycin (10 mg/mL) (to 50 ug/mL working concentration)
- Poured 1.25 sleeve’s worth of plates
- Made Tet Plates
- 300 mL LB
- 0.6 mL Tetracycline (5 mg/mL) (to 10 ug/mL working concentration)
- Poured 1 sleeve’s worth of plates
- Made LB Stock
- 10.03 g Tryptone
- 1 mL 1N NaOH
- 5.02 g Bacto Yeast extract
- 5.04 g NaCl
- Made 1X TAE
- 100 mL 10X TAE
- 900 mL dH20
Paul
- Sent Cas9 minipreps to sequencing
- Ran gels on GG PCR products (sfGFP & mCherry)
- Ran PCR on GFP&mCherry (Ta=56¯C)
- Sequencing Premix Protocol (use small 600 uL tubes)
- 1 template+1 primer per tube
- 450-600 ng of DNA template (~100-800)
- 1.2 uL of 10 uM primer
- Water to 15 uL
- 1 template+1 primer per tube
- Submit sequencing through Genesifter account
Sara
- Reran sfGFP and mCherry PCR with Sara
- Procedure:
- 2.5 uL 10X PCR buffer
- 0.5 uL 10 mM dNTPs
- 0.5 uL of forward primer at 10 mM
- 0.5 uL of reverse primer at 10 mM
- 0.5 uL template (Shu's miniprep GFP and mCherry products)
- 0.25 Taq polymerase
- 20.25 uL H20
- PCR settings:
- Denature: 95°C, 7 s.
- Anneal: 51°C, 43 s.
- Elongate 72°C, 2 m
- Procedure:
- Loaded the samples into the gels with Paul
- Troubleshot too-concentrated primers in PCR reaction
Shu
- Transformation of mRFP in pSB1T3
- Sent Tyler Josh’s slides
Tasfia
- Cleaned up miniprepped INP PCR product (80.2 ng/uL final concentration)
- Autoclaved LB
- Poured Tet plates (see Michelle’s notes for details)
Tyler
- Sequencing Cas9 preparation
- Reviewed SS Primers, created more mRFP guides, sent to Kelly
- Began reviewing Josh’s modeling slides from Shu, emailed Joe about meeting time
