Thursday, July 21st
Tasks:
Jordan
- Transformed J04550 RFP part to amplify for gRNA construct
- Resuspended Kit Plate 4, well 2H in 10 uL of water, transformed 2 uL of that into 50 uL comp cells
- Plated 50 and 100 uL
- Transformed competent cell test
- 7 test conditions: 50, 20, 10, 5, and .5 pg/uL of RFP plasmid (part J04550) and 1.11 ng/ul and 8.9 ng/ul of pSB1C3 + tet plasmid
- Transformed 1 ul of each
- Did two replicate plates of each
Michelle
- PCR INP part out of the iGEM registry
- 10 uL dH2O, pipet up and down, sit 5 min
- Transformed INP biobrick
- Transformed using 1 uL of diluted DNA from plate
- Followed bootcamp protocol except:
- 50 mL competent cells instead of 100 mL
- 450 uL SOC instead of 900 uL
- Used 108.3 ng/uL DNA straight from the iGEM plate
- Plated 100 uL
- Ran gel on PCR product
Paul
- Planned gRNA assembly procedure
- Selected storage plasmids for use in Golden Gate
- Transformed mRFP device:
- Transformed using 1 uL of diluted DNA from plate
- Followed bootcamp protocol except:
- 50 mL competent cells instead of 100 mL
- 450 uL SOC instead of 900 uL
- Used 108.3 ng/uL DNA straight from the iGEM plate
- Plated 100 uL
Sam
- Went to the products showcase thing to ask for free stuff
- Found more antibiotic experts
Sara
- Nanodropped the Gibson Tet Cas9 product - 1730 ng/uL
- Diluted the Gibson product to 50 ng/uL
- 1.16 uL Gibson product
- 38.84 uL NF water
- 40 uL in total
- Restriction digestion of Gibson
- 5 uL 10X NE buffer 4
- 1 uL EcoRi HF
- 20 uL 50 ng/uL Diluted Gibson (1 ug)
- 25 uL water
- 50 uL in total
- Ran a gel of the restriction digest with Shu
- 8 uL ladder
- 6 uL DNA
- 2.5 uL restricted DNA (50 ng)
- 2.5 uL NF water
- 1 uL loading dye
Shu
- Ran a gel of the restriction digest with Sara
- Sorting out the things we received from IDT today
- Read Golden Gate papers
- Looked into the traveling grant
Tasfia
- PCR’ed INP and ran a gel for product
- 2.5 uL 10X PCR buffer
- 0.5 uL 10 mM dNTPs
- 0.5 uL INP-fwd at 10 uM
- 0.5 uL INP-rev at 10 uM
- 0.5 uL template (BB part, 2.4 kb, so 2 min 24s of elongation)
- 1 hr at 50oC Total of 20 uL
- Transformed INP
- Transformed using 1 uL of diluted DNA from plate
- Followed bootcamp protocol except:
- 50 mL competent cells instead of 100 mL
- 450 uL SOC instead of 900 uL
- Used 108.3 ng/uL DNA straight from the iGEM plate
- Plated 100 uL
- Worked on presentation slideshow
Jordan
- Transformed J04550 RFP part to amplify for gRNA construct
- Resuspended Kit Plate 4, well 2H in 10 uL of water, transformed 2 uL of that into 50 uL comp cells
- Plated 50 and 100 uL
- Transformed competent cell test
- 7 test conditions: 50, 20, 10, 5, and .5 pg/uL of RFP plasmid (part J04550) and 1.11 ng/ul and 8.9 ng/ul of pSB1C3 + tet plasmid
- Transformed 1 ul of each
- Did two replicate plates of each
Michelle
- PCR INP part out of the iGEM registry
- 10 uL dH2O, pipet up and down, sit 5 min
- Transformed INP biobrick
- Transformed using 1 uL of diluted DNA from plate
- Followed bootcamp protocol except:
- 50 mL competent cells instead of 100 mL
- 450 uL SOC instead of 900 uL
- Used 108.3 ng/uL DNA straight from the iGEM plate
- Plated 100 uL
- Ran gel on PCR product
Paul
- Planned gRNA assembly procedure
- Selected storage plasmids for use in Golden Gate
- Transformed mRFP device:
- Transformed using 1 uL of diluted DNA from plate
- Followed bootcamp protocol except:
- 50 mL competent cells instead of 100 mL
- 450 uL SOC instead of 900 uL
- Used 108.3 ng/uL DNA straight from the iGEM plate
- Plated 100 uL
Sam
- Went to the products showcase thing to ask for free stuff
- Found more antibiotic experts
Sara
- Nanodropped the Gibson Tet Cas9 product - 1730 ng/uL
- Diluted the Gibson product to 50 ng/uL
- 1.16 uL Gibson product
- 38.84 uL NF water
- 40 uL in total
- Restriction digestion of Gibson
- 5 uL 10X NE buffer 4
- 1 uL EcoRi HF
- 20 uL 50 ng/uL Diluted Gibson (1 ug)
- 25 uL water
- 50 uL in total
- Ran a gel of the restriction digest with Shu
- 8 uL ladder
- 6 uL DNA
- 2.5 uL restricted DNA (50 ng)
- 2.5 uL NF water
- 1 uL loading dye
Shu
- Ran a gel of the restriction digest with Sara
- Sorting out the things we received from IDT today
- Read Golden Gate papers
- Looked into the traveling grant
Tasfia
- PCR’ed INP and ran a gel for product
- 2.5 uL 10X PCR buffer
- 0.5 uL 10 mM dNTPs
- 0.5 uL INP-fwd at 10 uM
- 0.5 uL INP-rev at 10 uM
- 0.5 uL template (BB part, 2.4 kb, so 2 min 24s of elongation)
- 1 hr at 50oC Total of 20 uL
- Transformed INP
- Transformed using 1 uL of diluted DNA from plate
- Followed bootcamp protocol except:
- 50 mL competent cells instead of 100 mL
- 450 uL SOC instead of 900 uL
- Used 108.3 ng/uL DNA straight from the iGEM plate
- Plated 100 uL
- Worked on presentation slideshow
