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Team:Cornell/Week 15
From 2011.igem.org
(Difference between revisions)
(→Tuesday, September 13) |
(→Thursday, September 15) |
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| Line 54: | Line 54: | ||
::::1.0μL diluted reverse primer (125ng) | ::::1.0μL diluted reverse primer (125ng) | ||
::::0.3μL dsDNA (20ng) | ::::0.3μL dsDNA (20ng) | ||
| - | ::::<u>1.0μL PfuUltra</u> | + | ::::<u>1.0μL PfuUltra High-Fidelity DNA polymerase</u> |
::::50.0μL Total | ::::50.0μL Total | ||
| - | ::::* | + | ::::*1µL fwd primer diluted in 5.3µL ddH2O before adding 1µl to reaction mixture |
| - | ::::* | + | ::::*1µL rvs primer diluted in 5.6µL ddH2O before adding 1µl to reaction mixture |
::'''Avi-Tagged VioB''' | ::'''Avi-Tagged VioB''' | ||
| Line 66: | Line 66: | ||
::::1.0μL diluted reverse primer (125ng) | ::::1.0μL diluted reverse primer (125ng) | ||
::::0.4μL dsDNA (20ng) | ::::0.4μL dsDNA (20ng) | ||
| - | ::::<u>1.0μL PfuUltra</u> | + | ::::<u>1.0μL PfuUltra Hi-Fi DNA polymerase</u> |
::::50.0μL Total | ::::50.0μL Total | ||
| - | ::::* | + | ::::*1µL fwd primer diluted in 7.6µL ddH2O before adding 1µl to reaction mixture |
| - | ::::* | + | ::::*1µL rvs primer diluted in 7.7µL ddH2O before adding 1µl to reaction mixture |
::'''Avi-Tagged VioE''' | ::'''Avi-Tagged VioE''' | ||
| Line 78: | Line 78: | ||
::::1.0μL diluted reverse primer (125ng) | ::::1.0μL diluted reverse primer (125ng) | ||
::::0.2μL dsDNA (20ng) | ::::0.2μL dsDNA (20ng) | ||
| - | ::::<u>1.0μL PfuUltra</u> | + | ::::<u>1.0μL PfuUltra Hi-Fi DNA polymerase</u> |
::::50.0μL Total | ::::50.0μL Total | ||
| - | ::::* | + | ::::*1µL fwd primer diluted in 6.2µL ddH2O before adding 1µl to reaction mixture |
| - | ::::* | + | ::::*1µL rvs primer diluted in 5.6µL ddH2O before adding 1µl to reaction mixture |
:::Run PCR protocol as listed under 'PCR Deletion' in protocols sections | :::Run PCR protocol as listed under 'PCR Deletion' in protocols sections | ||
:::Note: fwd and rvs primer dilution calculations based on our particular primer MWs and stock elution volumes | :::Note: fwd and rvs primer dilution calculations based on our particular primer MWs and stock elution volumes | ||
:*'''Transformation via Electroporation''' | :*'''Transformation via Electroporation''' | ||
| - | ::*Add 1. | + | ::*Add 1.0µL dPN1 to each PCR reaction |
| - | ::*Incubate in thermocycler at | + | ::*Incubate in thermocycler at 37°C for 1 hour |
::*After incubation, transform PCR product into electrocompetent cells | ::*After incubation, transform PCR product into electrocompetent cells | ||
| - | :::- (VioA+Avi-Tag) into DH5α | + | :::- (VioA + Avi-Tag) into DH5α |
| - | :::- (VioB+Avi-Tag) into DH5α | + | :::- (VioB + Avi-Tag) into DH5α |
| - | :::- (VioE+Avi-Tag) into DH5α | + | :::- (VioE + Avi-Tag) into DH5α |
---- | ---- | ||
Afternoon lab work done by: Youjin Cho, Charlie Chung | Afternoon lab work done by: Youjin Cho, Charlie Chung | ||
| - | :*Gel purification of digested light-lysis gene insert | + | :*'''Gel purification of digested light-lysis gene insert''' |
::- After NanoDrop DNA quantification, 26ng/µL | ::- After NanoDrop DNA quantification, 26ng/µL | ||
| - | :*Ligation of light-lysis gene insert with pSB1C3 iGEM backbone | + | :*'''Ligation of light-lysis gene insert with pSB1C3 iGEM backbone''' |
::9µL light-lysis (insert) DNA | ::9µL light-lysis (insert) DNA | ||
::8µL pSB1C3 backbone | ::8µL pSB1C3 backbone | ||
| Line 103: | Line 103: | ||
::<u>1µL T4 DNA ligase</u> | ::<u>1µL T4 DNA ligase</u> | ||
::20µL Total | ::20µL Total | ||
| - | :*Control Ligation Setup | + | :*'''Control Ligation Setup''' |
::9µL ddH2O | ::9µL ddH2O | ||
::8µL pSB1C3 backbone | ::8µL pSB1C3 backbone | ||
| Line 109: | Line 109: | ||
::<u>1µL T4 DNA ligase</u> | ::<u>1µL T4 DNA ligase</u> | ||
::20µL Total | ::20µL Total | ||
| - | :*Plated | + | :*Plated transformed products of PCR deletion technique on VioA, VioB, and VioE using ampicillin-treated agar plates |
Afternoon microfluidics work done by: Maneesh Gupta | Afternoon microfluidics work done by: Maneesh Gupta | ||
:*Tested effect of fluorescein with lysate on streptavidin-biotin binding to see if lysate interferes with their affinity | :*Tested effect of fluorescein with lysate on streptavidin-biotin binding to see if lysate interferes with their affinity | ||
Revision as of 01:00, 16 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 |
September 11th - September 17th
Sunday, September 11
~God bless America -- never forget~
Monday, September 12
Afternoon lab work done by: Nancy Li, Charlie Chung
- Prepared ten 3mL LB cultures (with 3µL carbenicillin) of colonies picked from plates dated Sept 3
- - RFP + Avi-Tagged pZE12 in DH5α
- - vioA + Avi-Tagged pZE12 in DH5α
- - vioB + Avi-Tagged pZE12 in DH5α
- - vioE + Avi-Tagged pZE12 in DH5α
- - RFP + Avi-Tagged pZE12 in MC4100
- - vioA + Avi-Tagged pZE12 in MC4100
- - vioB + Avi-Tagged pZE12 in MC4100
- - vioE + Avi-Tagged pZE12 in MC4100
- - Control tube is just a colony with pZE12 (no insert gene)
- - LB with carbenicillin (no inoculation with bacteria)
- Incubating at 37°C in the shaker at Weill Hall
- Cultures are to be lysed for release of natively biotinylated RFP and vio enzymes in characterizing streptavidin-coated microfluidics chips
- Did not extensively search for L-tryptophan (starting substrate in the synthesis of prodeoxyviolacein) in the reagents shelf of our Weill Lab space, but does not appear to be in plain view (may be tucked away in an obscure corner?)
Tuesday, September 13
Afternoon lab work done by: Charlie Chung
- Objective: Transfer yesterday's 3mL starter culture into today's larger scale culture (20mL LB + 20µL ampicillin)
- Autoclaved two 1L LB at 1:30pm (~1.5 hour cycle)
- Claire's batch of five autoclaved 250mL flasks are ready for use
- Prepared stock solution of 1000x ampicillin (100mg/mL)
- - Weigh out 1g ampicillin sodium salt (Sigma)
- - Dissolve in 10mL ddH2O
- - Syringe filter (0.22µm membrane) the ampicillin solution
- Stored in the bottom shelf of Weill Lab refrigerator (it's in a 15mL conical -- will later aliquot into Eppendorfs)
Evening lab work done by: Claire Paduano
- Prepared cultures of Avi-Tagged VioA, VioB, VioE and RFP in 20mL LB with 20µL ampicillin
- Left in 37°C shaker to culture
Wednesday, September 14
Thursday, September 15
Morning lab work done by: Claire Paduano and Jim Mathew
- DpnI Digestion of PCR Reaction Product
- - Retried the PCR deletion method on Avi-Tagged VioA, VioB, and VioE
- Avi-Tagged VioA
- 40.7μL ddH2O
- 5.0μL 10x PfuUltra buffer
- 1.0μL dNTPs
- 1.0μL diluted forward primer (125ng)
- 1.0μL diluted reverse primer (125ng)
- 0.3μL dsDNA (20ng)
- 1.0μL PfuUltra High-Fidelity DNA polymerase
- 50.0μL Total
- 1µL fwd primer diluted in 5.3µL ddH2O before adding 1µl to reaction mixture
- 1µL rvs primer diluted in 5.6µL ddH2O before adding 1µl to reaction mixture
- Avi-Tagged VioB
- 40.6μL ddH2O
- 5.0μL 10x PfuUltra buffer
- 1.0μL dNTPs
- 1.0μL diluted forward primer (125ng)
- 1.0μL diluted reverse primer (125ng)
- 0.4μL dsDNA (20ng)
- 1.0μL PfuUltra Hi-Fi DNA polymerase
- 50.0μL Total
- 1µL fwd primer diluted in 7.6µL ddH2O before adding 1µl to reaction mixture
- 1µL rvs primer diluted in 7.7µL ddH2O before adding 1µl to reaction mixture
- Avi-Tagged VioB
- Avi-Tagged VioE
- 40.8μL ddH2O
- 5.0μL 10x PfuUltra buffer
- 1.0μL dNTPs
- 1.0μL diluted forward primer (125ng)
- 1.0μL diluted reverse primer (125ng)
- 0.2μL dsDNA (20ng)
- 1.0μL PfuUltra Hi-Fi DNA polymerase
- 50.0μL Total
- 1µL fwd primer diluted in 6.2µL ddH2O before adding 1µl to reaction mixture
- 1µL rvs primer diluted in 5.6µL ddH2O before adding 1µl to reaction mixture
- Run PCR protocol as listed under 'PCR Deletion' in protocols sections
- Note: fwd and rvs primer dilution calculations based on our particular primer MWs and stock elution volumes
- Transformation via Electroporation
- Add 1.0µL dPN1 to each PCR reaction
- Incubate in thermocycler at 37°C for 1 hour
- After incubation, transform PCR product into electrocompetent cells
- - (VioA + Avi-Tag) into DH5α
- - (VioB + Avi-Tag) into DH5α
- - (VioE + Avi-Tag) into DH5α
- Avi-Tagged VioE
Afternoon lab work done by: Youjin Cho, Charlie Chung
- Gel purification of digested light-lysis gene insert
- - After NanoDrop DNA quantification, 26ng/µL
- Ligation of light-lysis gene insert with pSB1C3 iGEM backbone
- 9µL light-lysis (insert) DNA
- 8µL pSB1C3 backbone
- 2µL 10x T4 DNA ligase buffer
- 1µL T4 DNA ligase
- 20µL Total
- Control Ligation Setup
- 9µL ddH2O
- 8µL pSB1C3 backbone
- 2µL 10x T4 DNA ligase buffer
- 1µL T4 DNA ligase
- 20µL Total
- Plated transformed products of PCR deletion technique on VioA, VioB, and VioE using ampicillin-treated agar plates
Afternoon microfluidics work done by: Maneesh Gupta
- Tested effect of fluorescein with lysate on streptavidin-biotin binding to see if lysate interferes with their affinity
- - Used 5:1 ratio of lysate to fluorescein
- - Chips used in the experiment were coated yesterday (streptavidin is 1 day old)
- - Flow rate = 1µL/min for 50 minutes
- - Tested chips "Aaaaahhh" and "Chippy". Test chip was "Aaaahhh" which contained lysate + fluorescein. "Chippy" :: contained lysate. Stored both chips in fridge with DI water. Pictures taken with chips filled in air.
- Tested chip "stardust" with fluorescein two days after it was coated with streptavidin. Stored in DIwater in fridge.
- - Flow rate = 5µl/min for 20min. pics taken in air.
