Team:Cornell/Week 9
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==Friday, August 5== | ==Friday, August 5== | ||
- | Lab work done by: Youjin Cho | + | Lab work done by: Youjin Cho, Claire Paduano |
- | + | ||
:'''Objective''' | :'''Objective''' | ||
- | ::Transform ligation of GFP/RFP/ | + | ::Transform ligation of GFP/RFP/VioE + AviTagged backbone |
- | + | ||
:#Desalted overnight ligation | :#Desalted overnight ligation | ||
:#Transformed the samples into DH5α electrocompetent cells | :#Transformed the samples into DH5α electrocompetent cells | ||
- | |||
- | |||
- | |||
:'''Group Meeting''' | :'''Group Meeting''' | ||
- | ::*Just finished transforming GFP/RFP/ | + | ::*Just finished transforming GFP/RFP/VioE + AviTag + pZE12 backbone |
- | ::*If the | + | ::*If the VioE gene successfully inserts and ligates with the AviTagged backbone, then we can ligate in VioA and VioB this weekend |
- | ::*Goal: to treat PDMS devices to coat with streptavidin and bind | + | ::*Goal: to treat PDMS devices to coat with streptavidin and bind AviTagged GFP and RFP to device |
==Saturday, August 6== | ==Saturday, August 6== | ||
Lab work done by: Youjin Cho, Charlie Chung | Lab work done by: Youjin Cho, Charlie Chung | ||
- | *Miniprepped 5mL cultures of transformed DH5α electrocompetent bacteria (standard Qiagen Miniprep protocol) | + | :*Miniprepped 5mL cultures of transformed DH5α electrocompetent bacteria (standard Qiagen Miniprep protocol) |
- | :NOTE: White masses were floating in bacteria culture -- potential contamination? | + | ::<u>NOTE</u>: White masses were floating in bacteria culture -- potential contamination? |
- | *NanoDrop spectrophotometry to determine DNA concentration of 50µL elution product | + | :*NanoDrop spectrophotometry to determine DNA concentration of 50µL elution product |
- | ::RFP (Colony 1) + | + | ::RFP (Colony 1) + AviTagged pZE12 vector backbone = 53.2ng/µL |
- | ::RFP (Colony 2) + | + | ::RFP (Colony 2) + AviTagged pZE12 vector backbone = 63.4ng/µL |
- | ::RFP (Colony 3) + | + | ::RFP (Colony 3) + AviTagged pZE12 vector backbone = 76.6ng/µL |
- | ::GFP (Colony 1) + | + | ::GFP (Colony 1) + AviTagged pZE12 vector backbone = 65.7ng/µL |
- | ::GFP (Colony 2) + | + | ::GFP (Colony 2) + AviTagged pZE12 vector backbone = 65.5ng/µL |
- | ::GFP (Colony 3) + | + | ::GFP (Colony 3) + AviTagged pZE12 vector backbone = 46.6ng/µL |
- | :: | + | ::VioE (Colony 1) did not grow in its culture tube |
- | :: | + | ::VioE (Colony 2) + AviTagged pZE12 vector backbone = 53.8ng/µL |
- | ::DNA from | + | ::DNA from VioE (Colony 3) was accidentally discarded...Charlie is extremely ashamed. |
Latest revision as of 17:23, 18 September 2011
Week 1 | Week 2 - 5 | Week 6 | Week 7 | Week 8 | Week 9 | Week 10 | Week 11 | Week 12 | Week 13 | Week 14 | Week 15 | Week 16 | Week 17 | Week 18 | Week 19 | Week 20 | Week 21 |
July 31st - August 6th
Sunday, July 31
Monday, August 1
Lab work done by: Jim Mathew
- Sent VioE and AviTag + backbone in for sequencing
Tuesday, August 2
Microfluidics work done by: Jim Mathew, Nick Kramer, Dan Levine, Claire Paduano, Youjin Cho, Bill Jo
- Microfluidics
- Dr. Archer showed us how to use the clean room
- Made a SU-8 master of our device
- Poured PDMS and baked overnight at 60°C
- Followed protocol that is used by Biomedical Engineering lab class and is provided by Dr. Archer
Wednesday, August 3
Microfluidics work done by: Jim Mathew, Nick Kramer, Dan Levine, Claire Paduano, Youjin Cho, Bill Jo
- Microfluidics
- Dr. Archer showed us how to cut out PDMS devices and seal to clean glass slides using plasma cleaner
- Tested chips for blockages in flow
- - Three working devices, one with complete blockage in the channel
- Poured more PDMS and baked overnight at 60°C
- Followed protocol used in Biomedical Engineering lab class and provided by Dr. Archer
Thursday, August 4
Morning lab work done by: Jim Mathew
- Objective
- Prepare Avi-Tagged pZE12 vector backbone for GFP, RFP, and VioE gene inserts
- Digestion Setup in Duplicate
- 32.6μL H2O
- 9.9μL AviTagged pZE12 vector backbone (2μg)
- 5μL 10x NEBuffer 4
- 0.5μL 100x BSA
- 1μL KpnI-HF (HF = high fidelity)
- 1μL SphI-HF
- 50μL Total
- Incubate in 37°C water bath for 2 hours
- Dephosphorylation of 5' Ends of Vector Backbone
- Add 1μL of Calf Intestine Alkaline Phosphatase (CIAP) to digested vector backbone in order to prevent self-ligation without gene insert included
- Incubate at 50°C for 5 minutes
- Run vector backbone through agarose gel electrophoresis
- Gel Extraction and Purification of Digested Backbone
- Followed standard Qiagen Gel Extraction protocol for pZE12 vector backbone that is now AviTagged and digested with KpnI and SphI
- NanoDrop spectrophotometry on the duplicate samples reported 12.7ng/μL and 14.2ng/μL
Afternoon lab work done by: Claire Paduano, Charlie Chung
- Objective
- Ligation of GFP, RFP, and VioE genes with AviTagged pZE12 backbone
- Ligation
- GFP + AviTagged Backbone
- 10.6μL AviTagged pZE12 vector backbone
- 3.6μL GFP
- 2.8μL H2O
- 2.0μL T4 DNA ligase buffer
- 1.0μL T4 DNA ligase
- 20μL Total
- RFP + AviTagged Backbone
- 10.3μL AviTagged pZE12 vector backbone
- 6.7μL RFP
- 2.0μL T4 DNA ligase buffer
- 1.0μL T4 DNA ligase
- 20μL Total
- VioE + AviTagged Backbone
- 10.6μL AviTagged pZE12 vector backbone
- 4.1μL VioE
- 2.3μL H2O
- 2.0μL T4 DNA ligase buffer
- 1.0μL T4 DNA ligase
- 20μL Total
- In all above reactions, volume of plasmid vector added corresponds with 100ng backbone
- Prepare control ligation reactions (inserts replaced with H2O) for each of the above constructs
- Same volume of vector backbone, buffer, ligase
- Volumes of all inserts (i.e. gene) go toward volume of H2O
- After ligation setup, incubate in 16°C water bath overnight
- Ligation reaction volumes were calculated using a formulated spreadsheet (see Protocol page) that is based on 100ng of vector backbone and a 3:1 molar ratio of insert:vector
- Reference for Inserts and Vector Backbone
- RFP gene - 678bp
- GFP gene - 717bp
- vioE gene - 576bp
- pZE12 vector - 2340bp
Friday, August 5
Lab work done by: Youjin Cho, Claire Paduano
- Objective
- Transform ligation of GFP/RFP/VioE + AviTagged backbone
- Desalted overnight ligation
- Transformed the samples into DH5α electrocompetent cells
- Group Meeting
- Just finished transforming GFP/RFP/VioE + AviTag + pZE12 backbone
- If the VioE gene successfully inserts and ligates with the AviTagged backbone, then we can ligate in VioA and VioB this weekend
- Goal: to treat PDMS devices to coat with streptavidin and bind AviTagged GFP and RFP to device
Saturday, August 6
Lab work done by: Youjin Cho, Charlie Chung
- Miniprepped 5mL cultures of transformed DH5α electrocompetent bacteria (standard Qiagen Miniprep protocol)
- NOTE: White masses were floating in bacteria culture -- potential contamination?
- NanoDrop spectrophotometry to determine DNA concentration of 50µL elution product
- RFP (Colony 1) + AviTagged pZE12 vector backbone = 53.2ng/µL
- RFP (Colony 2) + AviTagged pZE12 vector backbone = 63.4ng/µL
- RFP (Colony 3) + AviTagged pZE12 vector backbone = 76.6ng/µL
- GFP (Colony 1) + AviTagged pZE12 vector backbone = 65.7ng/µL
- GFP (Colony 2) + AviTagged pZE12 vector backbone = 65.5ng/µL
- GFP (Colony 3) + AviTagged pZE12 vector backbone = 46.6ng/µL
- VioE (Colony 1) did not grow in its culture tube
- VioE (Colony 2) + AviTagged pZE12 vector backbone = 53.8ng/µL
- DNA from VioE (Colony 3) was accidentally discarded...Charlie is extremely ashamed.