Jordan

Figure 1: Troubleshooting summary

• Ran periplasm fraction protocol on Cas9 culture in TetR
• Centrifuged 25 mL suspension for 20 minutes at 4000 rpm and 4C
• Discarded supernatant
• Resuspended in 6.25 mL of ice-cold sucrose cell fractioning buffer 1
• Incubated for 20 minutes, shook periodically
• Centrifuged for 30 minutes at 4000 rpm and 4 degrees
• Discarded supernatant
• Resuspended in 1.56 mL ice cold buffer 2 with no detergents, transferred to eppendorf tube
• Incubated for 20 minutes on ice
• Centrifuged for 15 minutes at 11000 rpm on tabletop centrifuge
• Saved supernatant, in fridge

Michelle

• Gel extracted Cas9 for SS and Cas9 for iGEM
• Nanodrop results:
• Cas9 lnrz for SS: 9.0 ng/uL, 260/280: 1.8, 260/230: 0.44
• Cas9 res.dig. for iGEM: 8.8 ng/uL, 260/280: 1.85, 260/230: 0.43

Paul

• Got sequencing back for gRNA assembled construct
• Results aligned under “Assembled Parts>pSB1T3…+gRNA”
• Few point mutations on mRFP and Terminator-likely not too bad
• Gibson assembly of YcdO (10 uL: *6:1 insert:bb, 1% DMSO, 4 hrs @50 C*)
• 4.4 uL of Cas9 lnrz for SS (from 9/1/16 PCR, gel extracted 9/6/16- 9 ng/uL)
• 0.5 uL of YcdO (from PCR products, 38 ng/uL)
• 0.1 uL DMSO
• 5 uL Gibson Assembly HiFi MasterMix
• Met w/ Joe (w/ Tyler) about modeling
• Detect potential off target cleavage sites of our gRNA in the gut microbiome
• Restriction digest linear pSB1C3 and linear Cas9 (EcoRI, SpeI)

Sam

• Sent Emma Nechamkin emails
• Grew up two cultures (25 mL to start, ~22 mL now exist)
• Both JC8031
• One has pClyA-GFP-His6 Cam
• Induced with 290 uL arabinose at about .5 absorbance (actual absorbance labelled)
• One is normal
• No antibiotic
• Overnight in the 37°C shaking incubator
• Found and watched antibiotics and CRISPR videos
• Started adding graphics to pamphlet

Tyler

• Mathematical modeling meeting w/Joe
• Transformation of ligated products + Gibson SS (Ycdo)
• 3µL Ligated Cas9 Product
• 5µL Gibson SS Product
• 1µL Transformation control (50pg mRFP control)
• 2µL Gibson (+) control