Team:Michigan/Oil Sands June July

From 2010.igem.org

(Difference between revisions)
(7/7/2010)
(7/30/2010)
 
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'''Biobrick Transformation''' with Marc, Katie and Audra according to the heat shock transformation protocol
'''Biobrick Transformation''' with Marc, Katie and Audra according to the heat shock transformation protocol
-
*Started culture for biobrick transformation from over night at 2:30
+
*Started culture for Biobrick transformation from overnight at 2:30.
-
*At 5:00pm the cultures had overgrown to an OD600 of 1.2
+
*At 5:00pm the cultures had overgrown to an OD600 of 1.2.
-
**A a 1:3 dilution of cells was performed and the cells were allowed to go through another doubling period of 20 minutes
+
**A 1:3 dilution of cells was performed and the cells were allowed to go through another doubling period of 20 minutes.
-
*The OD600 was measured again and found to be around 0.500
+
*The OD600 was measured again and found to be around 0.500.
-
*the cultures were placed on ice at 5:30 and allowed to chill for 20 minutes
+
*the cultures were placed on ice at 5:30 and allowed to chill for 20 minutes.
-
*The washings were performed and the comp cells were resuspended in the residual CaCl2 only
+
*The washings were performed and the comp cells were resuspended in the residual CaCl2 only.
-
*The OD600 of the comp cells without the glycerol was above 0.3 therefore the comp cells were concentrated enough
+
*The OD600 of the comp cells without the glycerol was above 0.3 therefore the comp cells were concentrated enough.
-
*The heat shock was performed for the following biobricks
+
*The heat shock was performed for the following biobricks:
**BBa_179015
**BBa_179015
**BBa_179005
**BBa_179005
Line 108: Line 108:
**BBa_117002
**BBa_117002
**BBa_103006
**BBa_103006
-
*The cultures were placed in the 30C shaker to grow up for an hour at 30C at 9:00pm
+
*The cultures were placed in the 30C shaker to grow up for an hour at 30C at 9:00pm.
-
*The cultures were plated at 10:00pm
+
*The cultures were plated at 10:00pm.
 +
 
==7/9/2010==
==7/9/2010==
''Ann''
''Ann''
'''Biobrick Transformation''' with Josh, Prae, Charlie according to the miniprep protocol
'''Biobrick Transformation''' with Josh, Prae, Charlie according to the miniprep protocol
-
*After 9 hours of growing at 37C, the plates did not have any colonies on them
+
*After 9 hours of growing at 37C, the plates did not have any colonies on them.
-
*After 22 hours of growth plates that had grown had clear colonies
+
*After 22 hours of growth plates that had grown had clear colonies.
-
**The positive and negative controls grew out accordingly
+
**The positive and negative controls grew out accordingly.
-
**Only BBa_179015 and BBa_179005 had colonies (both from plate 1 and none from plate 2...)
+
**Only BBa_179015 and BBa_179005 had colonies (both from plate 1 and none from plate 2...):
***BBa_179015 had over 100 colonies
***BBa_179015 had over 100 colonies
***BBa_179005 had 2 colonies
***BBa_179005 had 2 colonies
-
*5 mL overnight cultures were started with 100 mg/mL amp at 8pm from a single colony on each plate
+
*5 mL overnight cultures were started with 100 mg/mL AMP at 8pm from a single colony on each plate.
==7/10/2010==
==7/10/2010==
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Miniprep
Miniprep
-
*Made frozen stocks from overnight culture of miniprep  
+
*Made frozen stocks from overnight culture of miniprep.
-
*Performed miniprep on BBa_179015 and BBa_179005
+
*Performed miniprep on BBa_179015 and BBa_179005.
-
*Measured DNA concentration with the Nanodrop
+
*Measured DNA concentration with the Nanodrop:
**BBa_179015-11 ng/mL
**BBa_179015-11 ng/mL
**BBa_179005-40 ng/mL
**BBa_179005-40 ng/mL
Digest
Digest
-
*Ran according to the digest protocol in the protocol section
+
*Ran according to the digest protocol in the protocol section.
-
**Cut parts with EcoRI and PstI
+
**Cut parts with EcoRI and PstI.
-
*Digested at 37C for 30 minutes
+
*Digested at 37C for 30 minutes.
Gel
Gel
-
*Ran according to the protocol in the protocol section
+
*Ran according to the protocol in the protocol section.
-
*Used 8 well comb instead of 13 well comb so the samples were too dilute too see
+
*Used 8 well comb instead of 13 well comb; the samples were too dilute too see.
==7/12/2010==
==7/12/2010==
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*Reran gel from 7/10/2010
*Reran gel from 7/10/2010
**Lane 1-Invitrogen 1 kb plus ladder
**Lane 1-Invitrogen 1 kb plus ladder
-
**Lane 2-Digested Bba_179005
+
**Lane 2-Digested BBa_179005
-
***Ran out of undigested Bba_179005
+
***Ran out of undigested BBa_179005
-
**Lane 3-Digested Bba_179015
+
**Lane 3-Digested BBa_179015
-
**Lane 4-Uncut miniprep plasmid Bba_179015
+
**Lane 4-Uncut miniprep plasmid BBa_179015
-
We found that we successfully extracted BBa_179015, T7-GFP, because there were expected bands at 906 and 2079 as faintly seen in the gel picture above.  No appeared for biobrick Bba_179005, T7 promoter, so this biobrick will be transformed again.
+
We successfully extracted BBa_179015, T7-GFP; expected bands at 906 and 2079 were faintly seen in the gel picture above.  No bands appeared for Biobrick Bba_179005, T7 promoter; this biobrick will be transformed again.
'''Biobrick Transformation take 2''' with Jeremy
'''Biobrick Transformation take 2''' with Jeremy
-
Autoclaved DI water for transformation and autoclaved sterile containers
+
Autoclaved DI water for transformation and autoclaved sterile containers.
-
*to autoclave sterile containers fill with DI water and decant the water before you start the culture in the container
+
*To autoclave sterile containers fill with DI water and decant the water before you start the culture in the container.
==7/13/2010==
==7/13/2010==
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''Ann''
''Ann''
-
Performed according to the electroporation transformation  
+
This was performed according to the electroporation transformation.
*Started the culture at 9:05am
*Started the culture at 9:05am
*Removed the culture at 12:05pm with an OD600 of 0.809
*Removed the culture at 12:05pm with an OD600 of 0.809
Line 183: Line 184:
**Bba_K103006
**Bba_K103006
**Bba_I719005
**Bba_I719005
-
*The cultures were allowed to grow in the incubator from 2:15-4:00pm
+
*The cultures grew in the incubator from 2:15-4:00pm.
-
**The cultures started to clump after growing this time
+
**The cultures started to clump after growing this time.
-
*100 uL of cells were plated on 100 mg/mL AMP plates
+
*100 uL of cells were plated on 100 mg/mL AMP plates.
==7/14/2010==
==7/14/2010==
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Electroporation Transformation
Electroporation Transformation
-
All of the transformation plates grew out! (minus the negative control of course)
+
All of the transformation plates (minus the negative control) grew out!
-
This means we should do all transformations by electroporation from now on. Just check with the Lin Lab to make sure we can use the electroporation machine for a few hours before starting
+
We should do all transformations by electroporation from now on. Just check with the Lin Lab to make sure we can use the electroporation machine for a few hours before starting.
Miniprep
Miniprep
*Started overnight cultures in 5 mL of LB plus 100 mg/mL AMP
*Started overnight cultures in 5 mL of LB plus 100 mg/mL AMP
-
**The following biobricks were started from the transformation plate
+
**The following biobricks were started from the transformation plate:
***Bba_K117008
***Bba_K117008
***Bba_K117002
***Bba_K117002
Line 207: Line 208:
***Bba_K103006
***Bba_K103006
***Bba_I719005
***Bba_I719005
-
**The following biobricks were started from the frozen stock in the -80C freezer
+
**The following biobricks were started from the frozen stock in the -80°C freezer:
***BBa_K719015
***BBa_K719015
'''INPNC Biobrick part'''
'''INPNC Biobrick part'''
-
*We received the INPNC biobrick (Bba_K265008) from UC Davis 2009 team.  THANK YOU!!!
+
*We received the INPNC Biobrick (Bba_K265008) from UC Davis 2009 team.  THANK YOU!!!
-
*It was shipped on LB plates in a pMA-SK plasmid from Mr. Gene in ''E. coli'' DH5alpha
+
*It was shipped on LB plates in a pMA-SK plasmid from Mr. Gene in ''E. coli'' DH5α
-
*Since this plasmid has AMP antibiotic resistance I am pouring plates today with Marc and Kevin with 100 mg/mL AMP resistance to streak out the culture tomorrow with Josh
+
*Since this plasmid has AMP antibiotic resistance I am pouring plates today with Marc and Kevin using 100 mg/mL AMP resistance; the culture will be streaked out tomorrow with Josh.
==7/25/2010==
==7/25/2010==
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''Ann''
''Ann''
-
Tonight I started an 8mL culture of E. coli DH5alpha in LB broth and place in the 30C shaker to grow out overnight
+
An 8 mL culture of E. coli DH5α in LB broth was produced and placed in the 30°C shaker to grow overnight.
==7/26/2010==
==7/26/2010==
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Electroporation transformation
Electroporation transformation
-
Started larger culture for comp cell preparation in 40mL of LB in a 500 mL sterile container at 9:00am
+
Started larger culture for comp cell preparation in 40 mL of LB in a 500 mL sterile container at 9:00am.
-
At 11:30am the OD of the culture was 0.730 and the cultures were placed on ice
+
At 11:30am the OD600 of the culture was 0.730 and the cultures were placed on ice.
-
The transformation of the biobricks was performed for according to the electroporation transformation protocol listed under the protocol section
+
The transformation of the biobricks was performed according to the electroporation transformation protocol listed under the protocol section of this Wiki.
-
The biobricks removed from the registry are as follows
+
The biobricks removed from the registry are as follows:
*E0040 (GFP)
*E0040 (GFP)
*K157013 (linker)
*K157013 (linker)
*I0500 (pBAD)
*I0500 (pBAD)
-
The miniprep of I79015 was used as a positive control and a negitive control was also run
+
The miniprep of I79015 was used as a positive control and a negative control was also run
-
The OD600 of the comp cells were not measured
+
The OD600 of the comp cells was not measured.
-
All of the time constants for the transformation were above 5
+
All of the time constants for the transformation were above 5.
-
the GFP, linker parts and the positive and negitive control were plated on 100 mg/mL AMP plates.   The pBAD part and negitive control were plated on 50 mg/mL KAN
+
The GFP, linker parts and the positive and negative control were plated on 100 mg/mL AMP plates. The pBAD part and negative control were plated on 50 mg/mL KAN plates.
==7/27/2010==
==7/27/2010==
-
'''Biobrick Transformation of suface display and pBAD'''  
+
'''Biobrick Transformation of surface display and pBAD'''  
Transformation Results
Transformation Results
-
The GFP and linker transformation worked and many colonies grew out on the 100 mg/mL AMP plates
+
The GFP and linker transformation worked and many colonies grew out on the 100 mg/mL AMP plates.
-
The pBAD part did not grow out on the KAN plates.  Upon further inspection this plasmid needs to be grown with IPTG to switch the origin of replication to a high copy above 100 copies per cell.  Otherwise, another orgin of replication dominates that is less than 10 copies per cell and the antibiotic concentration of 50 mg/mL maybe too high.  This transformation will have to be tried again
+
The pBAD part did not grow out on the KAN plates.  Upon further inspection this plasmid needs to be grown with IPTG to switch the origin of replication to a higher copy above 100 copies per cell.  Otherwise, another origin of replication dominates that is less than 10 copies per cell. An antibiotic concentration of 50 mg/mL is probably too high; this transformation will have to be attempted a second time.
'''Miniprep of surface display'''
'''Miniprep of surface display'''
-
At 9:00am a 5 mL culture of the newly transformed GFP part, the newly transformed linker part, the ompA part transformed previously and the INP from the UC davis team were started for a miniprep in LB with 100 mg/mL AMP.  
+
At 9:00am a 5 mL culture of the newly transformed GFP part, the newly transformed linker part, the OmpA part transformed previously and the INP from the UC Davis team were started for a miniprep in LB with 100 mg/mL AMP.  
-
The modified miniprep protocol was used listed on the protocol section of the wiki to get a higher DNA concentration
+
The modified miniprep protocol was used listed on the protocol section of the wiki to get a higher DNA concentration.
-
At 9:00pm the GFP, linker and INP parts were miniprepped.  The ompA culture had not grown out (b/c not enough -80C freezer stock was added) and a new culture was restarted at 11:00pm in 5 mL of LB with 100 mg/mL AMP.   
+
At 9:00pm the GFP, linker and INP parts were miniprepped.  The OmpA culture had not grown out (not enough -80°C freezer stock was added) and a new culture was restarted at 11:00pm in 5 mL of LB with 100 mg/mL AMP.   
'''Pouring Plates'''
'''Pouring Plates'''
-
More LB with 100 mg/mL AMP plates and LB with 25 mg/mL KAN plates were poured
+
More LB with 100 mg/mL AMP plates and LB with 25 mg/mL KAN plates were poured.
==7/28/2010==
==7/28/2010==
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'''OmpA Miniprep'''
'''OmpA Miniprep'''
-
The OmpA culture grew out and was miniprepped according the the modified miniprep protocol at 11:30am
+
The OmpA culture grew out and was miniprepped according the modified miniprep protocol at 11:30am.
'''Nanodrop of surface display parts'''
'''Nanodrop of surface display parts'''
-
The minipreped cultures from yesterday were nanodropped to determine the DNA concentration according to the protocol in the protocol section of the wiki
+
The miniprepped cultures from yesterday were nanodropped to determine the DNA concentration according to the protocol in the protocol section of the wiki:
*GFP: 47.8 ng/uL
*GFP: 47.8 ng/uL
*linker: 33.2 ng/uL
*linker: 33.2 ng/uL
Line 288: Line 289:
'''Digest of surface display parts'''
'''Digest of surface display parts'''
-
The following biobricks were digested according to the protocol on the wiki with the enzymes listed below
+
The following biobricks were digested according to the protocol on the wiki with the enzymes listed below:
*GFP 1: XbaI and PstI
*GFP 1: XbaI and PstI
Line 301: Line 302:
'''Gel of Digest for surface display parts'''
'''Gel of Digest for surface display parts'''
-
A gel was run of the above digest with uncut plasmid as a control
+
A gel was run of the above digest with uncut plasmid as a control:
[[Image:7-28biobrickgel.jpg|300px]]
[[Image:7-28biobrickgel.jpg|300px]]
-
*Lane 1: invitrogen 1 kb plus ladder
+
*Lane 1: Invitrogen 1 kb Plus ladder
-
*Lane 2: GFP cut with XbaI and PstI (GFP: 720 bp Backbone: 2079 bp)
+
*Lane 2: GFP cut with XbaI and PstI (GFP: 720 bp; Backbone: 2079 bp)
*Lane 3: GFP cut with EcoRI and XbaI
*Lane 3: GFP cut with EcoRI and XbaI
*Lane 4: uncut GFP plamid
*Lane 4: uncut GFP plamid
-
*Lane 5:INP cut with EcoRI and SpeI (INP: 924 bp backbone: 2550 bp)
+
*Lane 5: INP cut with EcoRI and SpeI (INP: 924 bp; Backbone: 2550 bp)
-
*Lane 6:INP cut with SpeI and PstI
+
*Lane 6: INP cut with SpeI and PstI
-
*Lane 7:uncut INP plasmid
+
*Lane 7: uncut INP plasmid
-
*Lane 8:Linker cut with XbaI and SpeI (Linker: 45 bp backbone: 2428 bp)
+
*Lane 8: Linker cut with XbaI and SpeI (Linker: 45 bp; Backbone: 2428 bp)
-
*Lane 9:Linker cut with SpeI and PstI
+
*Lane 9: Linker cut with SpeI and PstI
*Lane 10: uncut Linker plasmid
*Lane 10: uncut Linker plasmid
-
*Lane 11: OmpA cut with EcoRI and SpeI (OmpA: 464 bp backbone: 2079 bp)
+
*Lane 11: OmpA cut with EcoRI and SpeI (OmpA: 464 bp; Backbone: 2079 bp)
*Lane 12: OmpA cut with SpeI and PstI
*Lane 12: OmpA cut with SpeI and PstI
-
*Lane 13:uncut OmpA plasmid
+
*Lane 13: uncut OmpA plasmid
==7/29/2010==
==7/29/2010==
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'''Biofilm Assay in LB media'''
'''Biofilm Assay in LB media'''
-
Started cultures of E. coli K12, P. putida (oilsands) and P. fluorescens (oilsands) in 2 mL of LB and grew in the 30C shaker overnight
+
Cultures of E.coli K12, P. Putida (oilsands) and P. fluorescens (oilsands) were made in 2 mL of LB and placed in the 30°C shaker to grow overnight.
==7/30/2010==
==7/30/2010==
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'''Biofilm Assay in LB media'''
'''Biofilm Assay in LB media'''
-
Today we carried out the following [[Media:7-28-2010_Biofilm_Formation_Experiment.pdf|biofilm assay protocol]]
+
Today the following was carried out: [[Media:7-28-2010_Biofilm_Formation_Experiment.pdf|Biofilm assay protocol]]
*@ 8:10am the cultures were started from the overnight
*@ 8:10am the cultures were started from the overnight
-
*@ 10:00am the OD600 of each culture was measured to be
+
*@ 10:00am the OD600 of each culture was measured to be:
**E. coli K12: 0.8
**E. coli K12: 0.8
**P. fluorescens: 1.2
**P. fluorescens: 1.2
**P. putida: 1.0
**P. putida: 1.0
-
***These cultures were overgrown but still used for the experiment
+
***These cultures were overgrown but still used for the experiment.
-
The results of this experiment are presented in the chart below
+
The results of this experiment are presented in the chart below:
[[Image:7-30-2010_Biofilm_formation_in_LB_media_jpeg.jpg|500px]]
[[Image:7-30-2010_Biofilm_formation_in_LB_media_jpeg.jpg|500px]]
-
There is a large error in the P. putida strain because there was the largest variation in the OD 600 of the liquid culture which also resulted in a large variation in the CV OD 600 reading
+
There is a large error in the P. putida strain because there was the largest variation in the OD600 of the liquid culture which also resulted in a large variation in the CV OD600 reading.
-
We need to find a reference to compare our biofilms to.  This could be either a strain that does not form biofilms or a strain that forms biofilms very well
+
We need to find a reference to compare our biofilms to.  This could be either a strain that does not form biofilms or a strain that forms biofilms very well.
'''Transformation of pBAD'''
'''Transformation of pBAD'''
-
Marcus and Alex tried the transformation of pBAD again according to the electroporation protocol with Ann's Notes
+
Marcus and Alex tried the transformation of pBAD again according to the electroporation protocol with Ann's Notes.
-
The recovery after electroporation was performed in 1 mL of LB with 1mM of IPTG added in order to have the pBAD part have a high copy number
+
The recovery after electroporation was performed in 1 mL of LB with 1mM of IPTG added in order to have the pBAD part have a high copy number.
-
30 uL of 1M IPTG solution was added to a 25 mg/mL KAN plate and spread with sterile beads in order to keep the high copy plasmid in the pBAD part while plating
+
30 uL of 1M IPTG solution was added to a 25 mg/mL KAN plate and spread with sterile beads in order to keep the high copy plasmid in the pBAD part while plating.
==7/30/2010==
==7/30/2010==
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'''Transformation of pBAD'''
'''Transformation of pBAD'''
-
The transformation was successful and there were about 30 colonies on the plate.  One colony was picked at 7:30 pm for a miniprep the next day and added to 5mL of LB + 25 mg/mL KAN + 1 mM IPTG and grown out in the 30C shaker
+
The transformation was successful; 30 colonies were observed on the plate.  One colony was picked at 7:30 pm for a miniprep the next day and added to 5mL of LB + 25 mg/mL KAN + 1 mM IPTG to grow out in the 30°C shaker.
-
Another culture was started of GFP from the -80C freezer stock in 5 mL of LB + 100 mg/mL AMP for a miniprep.  Both the ligations with GFP did not work, so as long as we are miniprepping and digesting we want to re-verify this part
+
Another culture was started of GFP from the -80°C freezer stock in 5 mL of LB + 100 mg/mL AMP for a miniprep.  Both the ligations with GFP did not work; as long as we are miniprepping and digesting we want to re-verify this part.

Latest revision as of 00:19, 27 October 2010


Michigan Header





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Week 1 - 6/28/2010 6/29/2010 6/30/2010 7/1/2010 7/2/2010 -
Week 2 - - - 7/7/2010 7/8/2010 7/9/2010 7/10/2010
Week 3 - 7/12/2010 7/13/2010 7/14/2010 - - -
Week 4 - - - - - - -
Week 5 7/25/2010 7/26/2010 7/27/2010 7/28/2010 7/29/2010 7/30/2010 7/31/2010

Back to Oil Sands Main Notebook

6/28/2010

Pseudomonas putida KT2440 Antibiotic Resistance

6/29/2010

Pseudomonas putida KT2440 Antibiotic Resistance

6/29/2010 and 6/30/2010

Pseudomonas putida KT2440 Antibiotic Resistance

7/1/2010

Literature Review Napthenic Acids Composition & HPLC Analysis

7/2/2010

Pseudomonas putida KT2440 Antibiotic Resistance

7/7/2010

Ann

Biobrick Transformation with Alex and Jennifer

  • Made CaCl2 solution and 100 mg/mL amphicilin stock solution according to the media section of the Wiki.
  • Started an overnight culture of DH5α according to the heat shock transformation protocol.
    • A 12 mL culture was started because the protocol was multiplied by 4.

7/8/2010

Ann

Biobrick Transformation with Marc, Katie and Audra according to the heat shock transformation protocol

  • Started culture for Biobrick transformation from overnight at 2:30.
  • At 5:00pm the cultures had overgrown to an OD600 of 1.2.
    • A 1:3 dilution of cells was performed and the cells were allowed to go through another doubling period of 20 minutes.
  • The OD600 was measured again and found to be around 0.500.
  • the cultures were placed on ice at 5:30 and allowed to chill for 20 minutes.
  • The washings were performed and the comp cells were resuspended in the residual CaCl2 only.
  • The OD600 of the comp cells without the glycerol was above 0.3 therefore the comp cells were concentrated enough.
  • The heat shock was performed for the following biobricks:
    • BBa_179015
    • BBa_179005
    • BBa_145001
    • BBa_117008
    • BBa_117002
    • BBa_103006
  • The cultures were placed in the 30C shaker to grow up for an hour at 30C at 9:00pm.
  • The cultures were plated at 10:00pm.

7/9/2010

Ann

Biobrick Transformation with Josh, Prae, Charlie according to the miniprep protocol

  • After 9 hours of growing at 37C, the plates did not have any colonies on them.
  • After 22 hours of growth plates that had grown had clear colonies.
    • The positive and negative controls grew out accordingly.
    • Only BBa_179015 and BBa_179005 had colonies (both from plate 1 and none from plate 2...):
      • BBa_179015 had over 100 colonies
      • BBa_179005 had 2 colonies
  • 5 mL overnight cultures were started with 100 mg/mL AMP at 8pm from a single colony on each plate.

7/10/2010

Ann

Biobrick Transformation with Marcus, Bryce, Kilho, Josh, Charlie, Jeremy

Miniprep

  • Made frozen stocks from overnight culture of miniprep.
  • Performed miniprep on BBa_179015 and BBa_179005.
  • Measured DNA concentration with the Nanodrop:
    • BBa_179015-11 ng/mL
    • BBa_179005-40 ng/mL

Digest

  • Ran according to the digest protocol in the protocol section.
    • Cut parts with EcoRI and PstI.
  • Digested at 37C for 30 minutes.

Gel

  • Ran according to the protocol in the protocol section.
  • Used 8 well comb instead of 13 well comb; the samples were too dilute too see.

7/12/2010

Ann

Biobrick Transformation with Jeremy

Gel

7-12-2010 T7 promoter and T7 gfp biobricks.JPG

  • Reran gel from 7/10/2010
    • Lane 1-Invitrogen 1 kb plus ladder
    • Lane 2-Digested BBa_179005
      • Ran out of undigested BBa_179005
    • Lane 3-Digested BBa_179015
    • Lane 4-Uncut miniprep plasmid BBa_179015

We successfully extracted BBa_179015, T7-GFP; expected bands at 906 and 2079 were faintly seen in the gel picture above. No bands appeared for Biobrick Bba_179005, T7 promoter; this biobrick will be transformed again.

Biobrick Transformation take 2 with Jeremy

Autoclaved DI water for transformation and autoclaved sterile containers.

  • To autoclave sterile containers fill with DI water and decant the water before you start the culture in the container.

7/13/2010

Biobrick Transformation take 2 with Jeremy, Marcus, Josh, Kevin, Audra, Katie

Ann

This was performed according to the electroporation transformation.

  • Started the culture at 9:05am
  • Removed the culture at 12:05pm with an OD600 of 0.809
  • The OD600 of the comp cells were 1.2 after washing
  • The time constant for all electroporation were between 5.6 and 5.8 for the following biobricks
    • Bba_K117008
    • Bba_K117008 #2 (from resuspending remaining part left in registry in 15 uL of ultra pure water)
    • Bba_K117002
    • Bba_K145001
    • Bba_K103006
    • Bba_I719005
  • The cultures grew in the incubator from 2:15-4:00pm.
    • The cultures started to clump after growing this time.
  • 100 uL of cells were plated on 100 mg/mL AMP plates.

7/14/2010

Biobrick Transformation take 2

Ann

Electroporation Transformation

All of the transformation plates (minus the negative control) grew out!

We should do all transformations by electroporation from now on. Just check with the Lin Lab to make sure we can use the electroporation machine for a few hours before starting.

Miniprep

  • Started overnight cultures in 5 mL of LB plus 100 mg/mL AMP
    • The following biobricks were started from the transformation plate:
      • Bba_K117008
      • Bba_K117002
      • Bba_K145001
      • Bba_K103006
      • Bba_I719005
    • The following biobricks were started from the frozen stock in the -80°C freezer:
      • BBa_K719015

INPNC Biobrick part

  • We received the INPNC Biobrick (Bba_K265008) from UC Davis 2009 team. THANK YOU!!!
  • It was shipped on LB plates in a pMA-SK plasmid from Mr. Gene in E. coli DH5α
  • Since this plasmid has AMP antibiotic resistance I am pouring plates today with Marc and Kevin using 100 mg/mL AMP resistance; the culture will be streaked out tomorrow with Josh.

7/25/2010

Biobrick Transformation of suface display and pBAD

Ann

An 8 mL culture of E. coli DH5α in LB broth was produced and placed in the 30°C shaker to grow overnight.

7/26/2010

Biobrick Transformation of suface display and pBAD

Ann

Electroporation transformation

Started larger culture for comp cell preparation in 40 mL of LB in a 500 mL sterile container at 9:00am.

At 11:30am the OD600 of the culture was 0.730 and the cultures were placed on ice.

The transformation of the biobricks was performed according to the electroporation transformation protocol listed under the protocol section of this Wiki.

The biobricks removed from the registry are as follows:

  • E0040 (GFP)
  • K157013 (linker)
  • I0500 (pBAD)

The miniprep of I79015 was used as a positive control and a negative control was also run

The OD600 of the comp cells was not measured.

All of the time constants for the transformation were above 5.

The GFP, linker parts and the positive and negative control were plated on 100 mg/mL AMP plates. The pBAD part and negative control were plated on 50 mg/mL KAN plates.

7/27/2010

Biobrick Transformation of surface display and pBAD

Transformation Results

The GFP and linker transformation worked and many colonies grew out on the 100 mg/mL AMP plates.

The pBAD part did not grow out on the KAN plates. Upon further inspection this plasmid needs to be grown with IPTG to switch the origin of replication to a higher copy above 100 copies per cell. Otherwise, another origin of replication dominates that is less than 10 copies per cell. An antibiotic concentration of 50 mg/mL is probably too high; this transformation will have to be attempted a second time.

Miniprep of surface display

At 9:00am a 5 mL culture of the newly transformed GFP part, the newly transformed linker part, the OmpA part transformed previously and the INP from the UC Davis team were started for a miniprep in LB with 100 mg/mL AMP.

The modified miniprep protocol was used listed on the protocol section of the wiki to get a higher DNA concentration.

At 9:00pm the GFP, linker and INP parts were miniprepped. The OmpA culture had not grown out (not enough -80°C freezer stock was added) and a new culture was restarted at 11:00pm in 5 mL of LB with 100 mg/mL AMP.

Pouring Plates

More LB with 100 mg/mL AMP plates and LB with 25 mg/mL KAN plates were poured.

7/28/2010

OmpA Miniprep

The OmpA culture grew out and was miniprepped according the modified miniprep protocol at 11:30am.

Nanodrop of surface display parts

The miniprepped cultures from yesterday were nanodropped to determine the DNA concentration according to the protocol in the protocol section of the wiki:

  • GFP: 47.8 ng/uL
  • linker: 33.2 ng/uL
  • INP: 41.8 ng/uL
  • OmpA: 49.3 ng/uL

Digest of surface display parts

The following biobricks were digested according to the protocol on the wiki with the enzymes listed below:

  • GFP 1: XbaI and PstI
  • GFP 2: EcoRI and XbaI
  • INP 1: EcoRI and SpeI
  • INP 2: SpeI and PstI
  • Linker 1: XbaI and PstI
  • Linker 2: SpeI and PstI
  • OmpA 1: EcoRI and SpeI
  • OmpA 2: SpeI and PstI

Gel of Digest for surface display parts

A gel was run of the above digest with uncut plasmid as a control:

7-28biobrickgel.jpg

  • Lane 1: Invitrogen 1 kb Plus ladder
  • Lane 2: GFP cut with XbaI and PstI (GFP: 720 bp; Backbone: 2079 bp)
  • Lane 3: GFP cut with EcoRI and XbaI
  • Lane 4: uncut GFP plamid
  • Lane 5: INP cut with EcoRI and SpeI (INP: 924 bp; Backbone: 2550 bp)
  • Lane 6: INP cut with SpeI and PstI
  • Lane 7: uncut INP plasmid
  • Lane 8: Linker cut with XbaI and SpeI (Linker: 45 bp; Backbone: 2428 bp)
  • Lane 9: Linker cut with SpeI and PstI
  • Lane 10: uncut Linker plasmid
  • Lane 11: OmpA cut with EcoRI and SpeI (OmpA: 464 bp; Backbone: 2079 bp)
  • Lane 12: OmpA cut with SpeI and PstI
  • Lane 13: uncut OmpA plasmid

7/29/2010

Biofilm Assay in LB media

Cultures of E.coli K12, P. Putida (oilsands) and P. fluorescens (oilsands) were made in 2 mL of LB and placed in the 30°C shaker to grow overnight.

7/30/2010

Biofilm Assay in LB media

Today the following was carried out: Biofilm assay protocol

  • @ 8:10am the cultures were started from the overnight
  • @ 10:00am the OD600 of each culture was measured to be:
    • E. coli K12: 0.8
    • P. fluorescens: 1.2
    • P. putida: 1.0
      • These cultures were overgrown but still used for the experiment.

The results of this experiment are presented in the chart below:

7-30-2010 Biofilm formation in LB media jpeg.jpg

There is a large error in the P. putida strain because there was the largest variation in the OD600 of the liquid culture which also resulted in a large variation in the CV OD600 reading.

We need to find a reference to compare our biofilms to. This could be either a strain that does not form biofilms or a strain that forms biofilms very well.

Transformation of pBAD

Marcus and Alex tried the transformation of pBAD again according to the electroporation protocol with Ann's Notes.

The recovery after electroporation was performed in 1 mL of LB with 1mM of IPTG added in order to have the pBAD part have a high copy number.

30 uL of 1M IPTG solution was added to a 25 mg/mL KAN plate and spread with sterile beads in order to keep the high copy plasmid in the pBAD part while plating.

7/30/2010

Transformation of pBAD

The transformation was successful; 30 colonies were observed on the plate. One colony was picked at 7:30 pm for a miniprep the next day and added to 5mL of LB + 25 mg/mL KAN + 1 mM IPTG to grow out in the 30°C shaker.

Another culture was started of GFP from the -80°C freezer stock in 5 mL of LB + 100 mg/mL AMP for a miniprep. Both the ligations with GFP did not work; as long as we are miniprepping and digesting we want to re-verify this part.

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