Team:Cornell/Week 19

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Latest revision as of 19:07, 16 October 2011

Results | Protocol | Notebook | Parts Submitted

October 9th - October 15th

Sunday, October 9

iGEM 2011 Regionals Jamboree: Americas!

Monday, October 10

iGEM 2011 Regionals Jamboree: Americas Award Ceremony

Cornell brings home the Gold
Cornell advances to the iGEM 2011 World Jamboree!

Outreach

Attended meetings and added input for both AlumniGEM and Community Bricks.

Tuesday, October 11

Wednesday, October 12

Lab work done by: Charlie Chung

Picked Colonies: four (40mL LB + 40µL ampicillin) cultures shaking at 37°C

- AviTagged GFP

- AviTagged VioA from PCR deletion

- AviTagged VioB from PCR deletion

- AviTagged VioE from PCR deletion

Thursday, October 13

Lab work done by: Charlie Chung

Picking Colonies

(40mL LB + 40µL ampicillin) culture of empty pZE12 vector as a negative control shaking at 37°C

Miscellaneous

Freshly made 1000x ampicillin and 1M IPTG are in the DNA cryobox of Olin 301 (-20°C fridge)

Subculturing of AviTagged Vio Enzymes

20mL from 40mL cultures of VioA, B, E were transferred to (1L LB + 1mL ampicillin) flask for a 1:50 dilution

- Wanted OD to be between 0.05-0.08 after a 2-3hr incubation period, but accidentally let it grow over to 0.1xx

- Regardless, induced with 1mL 1M IPTG

(*EDIT*): Supposed to be a 0.1µM induction with IPTG, so should have added 100µL and not 1000µL to a 1000mL culture. Overinducing may lead to insoluble fractions.

- Shaking at room temp in Olin 301 for 20+ hours until 6pm on Friday (when we'll spin the cells down)

Subculturing of AviTagged GFP

two 10mL from 40mL culture of GFP were transferred to two (500mL LB + 500µL ampicillin) flasks for a 1:50 dilution

- Wanted OD to be 0.05-0.08 after a 2-3hr incubation period, but accidentally let it grow over to 0.1xx

- Regardless, induced with 500µL 1M IPTG

(*EDIT*): Supposed to be a 0.1µM induction with IPTG, so should have added 50µL and not 500µL to a 500mL culture. Overinducing may lead to insoluble fractions.

- Shaking at room temp in Olin 301 for 20+ hours until 6pm on Friday (when we'll spin the cells down)

Preparing Freezer Stocks

Took 500µL from remainder of the 40mL cultures and added 500µL of 30% glycerol to create freezer stocks of GFP and VioA, B, E

- In -80°C freezer of Olin 303

Preparation for Sequencing Confirmation of GFP and Vio Colonies

Miniprep purification of 5mL from remainder of the 40mL cultures. Eluted products are in -20°C fridge. To be submitted for sequencing

Friday, October 14

Lab work done by: Charlie Chung

Subculturing of Negative Control (empty pZE12 vector)

Transfer two 10mL samples from 40mL culture of empty pZE12 vector to two (500mL LB + 500µL ampicillin) flasks for a 1:50 dilution
Incubate overnight on 37°C shaker in Olin 304

Protein Extraction of GFP and VioA, B, E

Spin down 1L cultures into a pellet (10 min at 3200rpm)
Resuspend in 20mL autoclaved water
Transfer to 50mL conical tube and spin for 10 min at 3200rpm
Store in -80°C freezer

Western Blot Preparation

Centrifuge 1.5mL of GFP and VioA, B, E cultures for 10 min at 14,000rpm
BugBuster will be used for protein extraction

Saturday, October 15

Afternoon lab work done by: Charlie Chung

Preparation of Starter Cultures for pZE12 Vector and Vio Enzymes

Used freezer stocks to inoculate (5mL LB + 5µL ampicillin) cultures of empty pZE12 vector and VioA, B, E
Shaking in 37°C incubator of Olin 304

Lysate Extraction of E. coli with Empty pZE12 Vector -- Negative Control

Spin down 1L culture into pellets (10 min at 3200rpm; next time do longer and faster spin)
Stored in -20°C fridge of Olin 303

@@ Line 5: / Line 5: @@
 <br>
 <html>
-<font size="5"> <i> September 25th - October 1st </i></font>
+<font size="5"> <i> October 9th - October 15th </i></font>
 </html><br><br>
 ==Sunday, October 9==
-iGEM 2011 Regional Jamborees: Americas!
+'''iGEM 2011 Regionals Jamboree: Americas!'''
 ==Monday, October 10==
-iGME Americans Regional Jamboree Award Cereomoy
+:'''iGEM 2011 Regionals Jamboree: Americas Award Ceremony'''
+::*Cornell brings home the Gold
+::*Cornell advances to the iGEM 2011 World Jamboree!
+----
+:'''Outreach'''
+::*Attended meetings and added input for both AlumniGEM and Community Bricks.
 ==Tuesday, October 11==
@@ Line 17: / Line 23: @@
 ==Wednesday, October 12==
 Lab work done by: Charlie Chung
-:*'''Picked colonies''': five (40mL LB + 40µL ampicillin) cultures shaking at 37°C
+:'''Picked Colonies''': four (40mL LB + 40µL ampicillin) cultures shaking at 37°C
 ::- AviTagged GFP
-::- Dysfunctional RFP colony (negative control)
 ::- AviTagged VioA from PCR deletion
 ::- AviTagged VioB from PCR deletion
@@ Line 25: / Line 30: @@
 ==Thursday, October 13==
+Lab work done by: Charlie Chung
+:'''Picking Colonies'''
+::*(40mL LB + 40µL ampicillin) culture of empty pZE12 vector as a negative control shaking at 37°C
+:'''Miscellaneous'''
+::*Freshly made 1000x ampicillin and 1M IPTG are in the DNA cryobox of Olin 301 (-20°C fridge)
+:'''Subculturing of AviTagged Vio Enzymes'''
+::*20mL from 40mL cultures of VioA, B, E were transferred to (1L LB + 1mL ampicillin) flask for a 1:50 dilution
+:::- Wanted OD to be between 0.05-0.08 after a 2-3hr incubation period, but accidentally let it grow over to 0.1xx
+:::- Regardless, induced with 1mL 1M IPTG
+::::(<u>'''*EDIT*'''</u>): Supposed to be a 0.1µM induction with IPTG, so should have added 100µL and not 1000µL to a 1000mL culture. Overinducing may lead to insoluble fractions.
+:::- Shaking at room temp in Olin 301 for 20+ hours until 6pm on Friday (when we'll spin the cells down)
+:'''Subculturing of AviTagged GFP'''
+::*two 10mL from 40mL culture of GFP were transferred to two (500mL LB + 500µL ampicillin) flasks for a 1:50 dilution
+:::- Wanted OD to be 0.05-0.08 after a 2-3hr incubation period, but accidentally let it grow over to 0.1xx
+:::- Regardless, induced with 500µL 1M IPTG
+::::(<u>'''*EDIT*'''</u>): Supposed to be a 0.1µM induction with IPTG, so should have added 50µL and not 500µL to a 500mL culture. Overinducing may lead to insoluble fractions.
+:::- Shaking at room temp in Olin 301 for 20+ hours until 6pm on Friday (when we'll spin the cells down)
+:'''Preparing Freezer Stocks'''
+::*Took 500µL from remainder of the 40mL cultures and added 500µL of 30% glycerol to create freezer stocks of GFP and VioA, B, E
+:::- In -80°C freezer of Olin 303
+:'''Preparation for Sequencing Confirmation of GFP and Vio Colonies'''
+::*Miniprep purification of 5mL from remainder of the 40mL cultures. Eluted products are in -20°C fridge. To be submitted for sequencing
 ==Friday, October 14==
+Lab work done by: Charlie Chung
+:'''Subculturing of Negative Control''' ''(empty pZE12 vector)''
+::*Transfer two 10mL samples from 40mL culture of empty pZE12 vector to two (500mL LB + 500µL ampicillin) flasks for a 1:50 dilution
+::*Incubate overnight on 37°C shaker in Olin 304
+:'''Protein Extraction of GFP and VioA, B, E'''
+::*Spin down 1L cultures into a pellet (10 min at 3200rpm)
+::*Resuspend in 20mL autoclaved water
+::*Transfer to 50mL conical tube and spin for 10 min at 3200rpm
+::*Store in -80°C freezer
+:'''Western Blot Preparation'''
+::*Centrifuge 1.5mL of GFP and VioA, B, E cultures for 10 min at 14,000rpm
+::*BugBuster will be used for protein extraction
 ==Saturday, October 15==
+Afternoon lab work done by: Charlie Chung
+:'''Preparation of Starter Cultures for pZE12 Vector and Vio Enzymes'''
+::*Used freezer stocks to inoculate (5mL LB + 5µL ampicillin) cultures of empty pZE12 vector and VioA, B, E
+::*Shaking in 37°C incubator of Olin 304
+:'''Lysate Extraction of ''E. coli'' with Empty pZE12 Vector''' -- ''Negative Control''
+::*Spin down 1L culture into pellets (10 min at 3200rpm; next time do longer and faster spin)
+::*Stored in -20°C fridge of Olin 303