Team:Michigan/Oil Sands June July
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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 | + | **Lane 2-Digested BBa_179005 |
- | ***Ran out of undigested | + | ***Ran out of undigested BBa_179005 |
- | **Lane 3-Digested | + | **Lane 3-Digested BBa_179015 |
- | **Lane 4-Uncut miniprep plasmid | + | **Lane 4-Uncut miniprep plasmid BBa_179015 |
- | We | + | 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. |
==7/13/2010== | ==7/13/2010== | ||
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''Ann'' | ''Ann'' | ||
- | + | 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 | ||
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**Bba_K103006 | **Bba_K103006 | ||
**Bba_I719005 | **Bba_I719005 | ||
- | *The cultures | + | *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 | + | 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 | 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 | ||
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***Bba_K103006 | ***Bba_K103006 | ||
***Bba_I719005 | ***Bba_I719005 | ||
- | **The following biobricks were started from the frozen stock in the - | + | **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 | + | *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'' | + | *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 | + | *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'' | ||
- | + | 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 | + | 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 | + | 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 | + | 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 | + | The miniprep of I79015 was used as a positive control and a negative control was also run |
- | The OD600 of the comp cells | + | 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 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 | + | '''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 | + | 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 | + | 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 | + | 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 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 | + | 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 | ||
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'''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 | ||
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'''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: | + | *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 | + | *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 | + | *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 | + | *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''' | ||
- | + | 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 | + | 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 | + | 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 | + | 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 - | + | 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