Team:Michigan/Quorum Sensing
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__NOTOC__ | __NOTOC__ | ||
{{Michigan Header}} | {{Michigan Header}} | ||
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{|style="color:#1c2bf2;background-color:#fafa19;font-size:9pt;text-align:center" cellpadding="5" cellspacing="0" border="1" bordercolor="#fff" width="62%" | {|style="color:#1c2bf2;background-color:#fafa19;font-size:9pt;text-align:center" cellpadding="5" cellspacing="0" border="1" bordercolor="#fff" width="62%" | ||
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| [[Team:Michigan/Quorum_Sensing#7/25/2010|7/25/2010]] | | [[Team:Michigan/Quorum_Sensing#7/25/2010|7/25/2010]] | ||
| [[Team:Michigan/Quorum_Sensing#7/26/2010|7/26/2010]] | | [[Team:Michigan/Quorum_Sensing#7/26/2010|7/26/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#7/27/2010|7/27/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#7/28/2010|7/28/2010]] | ||
| - | | - | ||
+ | | [[Team:Michigan/Quorum_Sensing#7/30/2010|7/30/2010]] | ||
| - | | - | ||
+ | |- | ||
+ | !Week 6 | ||
| - | | - | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/2/2010|8/2/2010]] | ||
| - | | - | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/4/2010|8/4/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/5/2010|8/5/2010]] | ||
| - | | - | ||
+ | | - | ||
+ | |- | ||
+ | !Week 7 | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | |- | ||
+ | !Week 8 | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | | - | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/19/2010|8/19/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/20/2010|8/20/2010]] | ||
+ | | - | ||
+ | |- | ||
+ | !Week 9 | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/22/2010|8/22/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/23/2010|8/23/2010]] | ||
+ | | - | ||
+ | | - | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/26/2010|8/26/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/27/2010|8/27/2010]] | ||
+ | | [[Team:Michigan/Quorum_Sensing#8/28/2010|8/28/2010]] | ||
+ | |- | ||
|} | |} | ||
+ | |||
+ | {|cellspacing=0 style="background: transparent" | ||
+ | |-valign="top" | ||
+ | |width="700px" | | ||
+ | |||
=Quorum Sensing Team= | =Quorum Sensing Team= | ||
Members include [[User:Infekt|Alex Pyden]], [[User:Chillywings|Marcus Lehr]], [[User:Jejihong|Jennifer Hong]], [[User:Ericrayn|Eric Raynal]], [[User:Katemisk|Katie Miskovich]], and [[User:Audraw|Audra Williams]] | Members include [[User:Infekt|Alex Pyden]], [[User:Chillywings|Marcus Lehr]], [[User:Jejihong|Jennifer Hong]], [[User:Ericrayn|Eric Raynal]], [[User:Katemisk|Katie Miskovich]], and [[User:Audraw|Audra Williams]] | ||
- | ==7/7/ | + | ==7/7/2010== |
''Jennifer and Alex - in Lin Lab'' | ''Jennifer and Alex - in Lin Lab'' | ||
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~1.5 hrs | ~1.5 hrs | ||
- | == 7/8/ | + | == 7/8/2010 == |
''Alex, Jennifer and Eric - in ERB'' | ''Alex, Jennifer and Eric - in ERB'' | ||
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4 hrs of work | 4 hrs of work | ||
- | == 7/17/ | + | == 7/17/2010 == |
''Alex & Jennifer - in ERB'' | ''Alex & Jennifer - in ERB'' | ||
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**AI-2 reporter & LuxS null mutant (''E. coli'', does not produce AI-2, amp and kan-resistant) | **AI-2 reporter & LuxS null mutant (''E. coli'', does not produce AI-2, amp and kan-resistant) | ||
Removed these strains from 4°C -- they are stored in soft agar stab cultures | Removed these strains from 4°C -- they are stored in soft agar stab cultures | ||
+ | |||
Made one streak plate on LB+amp for each strain from stabs | Made one streak plate on LB+amp for each strain from stabs | ||
- | *placed in | + | *placed in 37°C (rm. 1239) |
Made one 2mL LB+amp broth cultures in a 15mL tube for each strain from stabs | Made one 2mL LB+amp broth cultures in a 15mL tube for each strain from stabs | ||
*placed in 30°C, 200 rpm shaking (rm. 1230) | *placed in 30°C, 200 rpm shaking (rm. 1230) | ||
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Created protocol/plan for experiment. [[Media:Quorum+Sensing+Tables-1-.pdf|Testing AI-2 Response]] | Created protocol/plan for experiment. [[Media:Quorum+Sensing+Tables-1-.pdf|Testing AI-2 Response]] | ||
- | == 7/19/ | + | == 7/19/2010 == |
''Alex and Marcus'' | ''Alex and Marcus'' | ||
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~6 hrs | ~6 hrs | ||
- | == 7/21/ | + | == 7/21/2010 == |
''Alex, Eric and Jeremy'' | ''Alex, Eric and Jeremy'' | ||
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*stored in iGEM box -- -80°C Lin Lab | *stored in iGEM box -- -80°C Lin Lab | ||
Plated LuxS<sup>-</sup> and MarC<sup>-</sup> mutants and ''Pseudomonas'' strains on LB | Plated LuxS<sup>-</sup> and MarC<sup>-</sup> mutants and ''Pseudomonas'' strains on LB | ||
+ | |||
Plated W3110 and MDAI2 on LB+amp+kan | Plated W3110 and MDAI2 on LB+amp+kan | ||
*placed all six plates in 37°C ERB 1239 | *placed all six plates in 37°C ERB 1239 | ||
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~1.5 hrs | ~1.5 hrs | ||
- | == 7/22/ | + | == 7/22/2010 == |
''Alex'' | ''Alex'' | ||
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- | == 7/23/ | + | == 7/23/2010 == |
''Alex'' | ''Alex'' | ||
Updated Strain Database | Updated Strain Database | ||
- | == 7/25/ | + | == 7/25/2010 == |
''Alex and Eric'' | ''Alex and Eric'' | ||
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Left stuff in autoclave | Left stuff in autoclave | ||
- | == 7/26/ | + | == 7/26/2010 == |
''Alex and Marcus'' | ''Alex and Marcus'' | ||
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*each 5 mL LB + 50μg/mL kan + 100μg/mL amp in a 15mL tube (added 5 μL each of a 1000X stock of each antibiotic) | *each 5 mL LB + 50μg/mL kan + 100μg/mL amp in a 15mL tube (added 5 μL each of a 1000X stock of each antibiotic) | ||
*incubated 30°C, 200 rpm shaking -- '''6:30 pm''' | *incubated 30°C, 200 rpm shaking -- '''6:30 pm''' | ||
- | |||
- | == 7/27/ | + | == 7/27/2010 == |
''Alex, Eric and Marcus'' | ''Alex, Eric and Marcus'' | ||
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**100 - 2.34 - 2 = '''95.66''' | **100 - 2.34 - 2 = '''95.66''' | ||
*placed both cultures in 37°C, 225 rpm shaking - ERB 1230, '''11:50am''' | *placed both cultures in 37°C, 225 rpm shaking - ERB 1230, '''11:50am''' | ||
- | |||
---- | ---- | ||
''Marcus and Eric'' | ''Marcus and Eric'' | ||
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*both seem to fluoresce at GFP equally | *both seem to fluoresce at GFP equally | ||
**''This is probably not right; MDAI2 should not have GFP. Will check on a fluorospectrometer tonight'' | **''This is probably not right; MDAI2 should not have GFP. Will check on a fluorospectrometer tonight'' | ||
- | |||
---- | ---- | ||
''Alex'' | ''Alex'' | ||
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**Many ''Acinetobacter'' controls were run - all at 0 or 1 | **Many ''Acinetobacter'' controls were run - all at 0 or 1 | ||
**''This is bad -- MDAI2 is clearly producing GFP, meaning it produces AI-2. Need to contact Tsao authors.'' | **''This is bad -- MDAI2 is clearly producing GFP, meaning it produces AI-2. Need to contact Tsao authors.'' | ||
- | |||
- | == 7/28/ | + | == 7/28/2010 == |
''Alex'' | ''Alex'' | ||
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*for Ann; will deliver tomorrow | *for Ann; will deliver tomorrow | ||
- | |||
- | == 7/30/ | + | == 7/30/2010 == |
''Alex and Marcus - w/ Charlie and Prae'' | ''Alex and Marcus - w/ Charlie and Prae'' | ||
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*placed all plates in 37°C | *placed all plates in 37°C | ||
*excess electroporation culture stored in 4°C | *excess electroporation culture stored in 4°C | ||
- | |||
- | == 8/2/ | + | == 8/2/2010 == |
''Alex and Eric'' | ''Alex and Eric'' | ||
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**W3110: '''204.86''' | **W3110: '''204.86''' | ||
**MDAI2: '''198.34''' | **MDAI2: '''198.34''' | ||
- | ''OK, | + | ''OK, I don't know if these have GFP or what. At any rate, if they do, the MDAI2 is too close to W3110. We'll probably have to work with the YFP biobrick instead.'' |
Got ''C. vulgaris'' from Bobby Levine | Got ''C. vulgaris'' from Bobby Levine | ||
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Autoclaved waste flasks | Autoclaved waste flasks | ||
*55 min (30 sterilize) | *55 min (30 sterilize) | ||
- | * | + | *25°C |
- | + | ||
- | == 8/ | + | == 8/3/2010 == |
+ | ''Alex and Marcus'' | ||
+ | |||
+ | Took yesterday's overnights to Alex's (Xi) lab since the Lin lab fluorospectrophotometer was in use. | ||
+ | *Excitation Frequency: 485 | ||
+ | *Emission Frequency: 545 | ||
+ | *Sensitivity: 50 | ||
+ | [[Image:LuxS- test.jpg]] | ||
+ | |||
+ | Fluorescence/OD600: | ||
+ | *LuxS<sup>-</sup>: 2263 | ||
+ | *DH5α + pLsr-YFP: 2078 | ||
+ | *LuxS<sup>-</sup> + pLsr-YFP: 1456 | ||
+ | |||
+ | Very confusing results, LuxS<sup>-</sup> was supposed to be the negative control, and shows the highest fluorescence per OD. Some factor must be confounding our assay. | ||
+ | |||
+ | Also, made 10 mL overnights of LuxS<sup>-</sup> (pLsr-YFP) and MDAI2 (pET6 + pET-GFP) in 50 mL tubes at 7 pm in LB+Amp+Kan. Put in shaker at 30°C. | ||
+ | |||
+ | == 8/4/2010 == | ||
''Alex and Marcus'' | ''Alex and Marcus'' | ||
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Updated QS experimental [[Media:QS_Procedures-1-.pdf|protocol]] | Updated QS experimental [[Media:QS_Procedures-1-.pdf|protocol]] | ||
- | |||
- | == 8/5/ | + | == 8/5/2010 == |
''Alex'' | ''Alex'' | ||
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made presentation for tomorrow | made presentation for tomorrow | ||
+ | |||
+ | Finished exp by protocol | ||
+ | *processed [[Media:QS_experiment_8-5-10(1).pdf|data]] and uploaded it | ||
+ | *discarded 15mL tubes | ||
+ | *discarded both 24-well plates | ||
+ | |||
+ | <!--Alex, please stop adding your timestamp. Thanks.--> | ||
+ | |||
+ | == 8/19/2010 == | ||
+ | ''Alex'' | ||
+ | |||
+ | Acquired new strains (soft agar stabs from Tsao Lab) | ||
+ | *W3110 + pTC6 + pET-GFP | ||
+ | *MDAI2 + pTC6 + pET-GFP | ||
+ | *BL21 + pTC5 + pET-GFP | ||
+ | **produces more AI-2 than W3110 | ||
+ | *moved all to ERB 4°C | ||
+ | Made broth cultures of MDAI2 and BL21 from stab cultures | ||
+ | *each 2 mL LB in a 15mL tube | ||
+ | *37°C, 200 rpm shaking | ||
+ | *placed in incubator at 8pm | ||
+ | |||
+ | Added [[Team:Michigan/Project|Quorum Sensing project description]] to Wiki | ||
+ | |||
+ | == 8/20/2010 == | ||
+ | ''Alex'' | ||
+ | |||
+ | [Earlier, Marcus cryostored BL21 and MDAI2 in Lin -80°C and made a spread plate of new MDAI2 strain.] | ||
+ | |||
+ | Made streak plate of BL21 | ||
+ | *placed in 35°C incubator | ||
+ | Made frozen stock of BL21 and MDAI2 | ||
+ | *each 500 μL culture + 500 μL 50% glycerol | ||
+ | *stored in ERB -20°C | ||
+ | Updated strain database | ||
+ | |||
+ | == 8/22/2010 == | ||
+ | ''Alex'' | ||
+ | |||
+ | Moved MDAI2 spread plate and BL21 streak plate from 37°C to 4°C | ||
+ | |||
+ | ---- | ||
+ | Made BL21 broth culture | ||
+ | *10 mL LB+100μg/mL amp+50μg/mL kan in a 50mL tube | ||
+ | *37°C, 200 rpm shaking | ||
+ | *8:00pm | ||
+ | |||
+ | == 8/23/2010 == | ||
+ | ''Marcus'' | ||
+ | |||
+ | Measured OD600 of overnight in Gulari Lab spectrophotometer. | ||
+ | -Used LB+ Amp(100μg/mL)+ Kan(50μg/mL) blank | ||
+ | -OD was 1.55 | ||
+ | |||
+ | Made dilution to OD 0.02 into 50 mL flask using [[Media:OD600 Cell Dilution Protocol.pdf|OD600 Cell Dilution Protocol]]. | ||
+ | -48.3 mL LB | ||
+ | -1 mL 40% glucose solution | ||
+ | -0.645 mL overnight culture | ||
+ | |||
+ | Put in 37°C shaker for 4 hours and then collected supernatant according to [[Media:QS_Procedures-1-.pdf|Lsr Circuit Test Protocols]]. Supernatant was labeled and stored in the ERB -20°C. | ||
+ | |||
+ | == 8/26/2010 == | ||
+ | ''Alex and Marcus'' | ||
+ | |||
+ | Made cultures of MDAI2 + pTC6 + pET-GFP (new) and LuxS<sup>-</sup> + pLsrA-YFP | ||
+ | *each 2 mL LB + 100μg/mL amp + 50μg/mL kan in each of four 15mL tubes (8 tubes total) | ||
+ | *incubated 30°C, 200 rpm shaking, 9:15pm | ||
+ | |||
+ | == 8/27/2010 == | ||
+ | ''Alex'' | ||
+ | |||
+ | Obtained cultures and supernatants from ERB -- 1:15pm (16 hrs); transfered to Xi Lab, SPH | ||
+ | |||
+ | Began Quorum Sensing experiment again, following [[Media:QS_Procedures-1-.pdf|posted protocol]] | ||
+ | *Used BL21 supernatant instead of MDAI2 | ||
+ | *had to wait until 6:45pm to run exp; cells were overgrown and started to die/pellet | ||
+ | **therefore, took only broth, avoiding pellet, for OD and spin | ||
+ | *spun at 5000rpm instead of 4200 | ||
+ | *plate template: | ||
+ | {| | ||
+ | !well | ||
+ | !pellet | ||
+ | !supernatant | ||
+ | |- | ||
+ | |A1 | ||
+ | |MDAI2 | ||
+ | |LB | ||
+ | |- | ||
+ | |A2 | ||
+ | |MDAI2 | ||
+ | |W3110 | ||
+ | |- | ||
+ | |A3 | ||
+ | |MDAI2 | ||
+ | |BL21 | ||
+ | |- | ||
+ | |A4 | ||
+ | |MDAI2 | ||
+ | |''C. vulgaris'' | ||
+ | |- | ||
+ | |B1 | ||
+ | |LuxS<sup>-</sup>+pLsrA-YFP | ||
+ | |LB | ||
+ | |- | ||
+ | |B2 | ||
+ | |LuxS<sup>-</sup>+pLsrA-YFP | ||
+ | |W3110 | ||
+ | |- | ||
+ | |B3 | ||
+ | |LuxS<sup>-</sup>+pLsrA-YFP | ||
+ | |BL21 | ||
+ | |- | ||
+ | |B4 | ||
+ | |LuxS<sup>-</sup>+pLsrA-YFP | ||
+ | |''C. vulgaris'' | ||
+ | |- | ||
+ | |C1 | ||
+ | |[blank] | ||
+ | |LB | ||
+ | |- | ||
+ | |C2 | ||
+ | |[blank] | ||
+ | |MDAI2 | ||
+ | |- | ||
+ | |C3 | ||
+ | |[blank] | ||
+ | |W3110 | ||
+ | |- | ||
+ | |C4 | ||
+ | |[blank] | ||
+ | |''C. vulgaris'' | ||
+ | |} | ||
+ | |||
+ | *ran growth curve for 16 hrs (overnight) instead of 6, drawing from Singapore protocol | ||
+ | Returned supernatants to ERB -20°C | ||
+ | |||
+ | == 8/28/2010 == | ||
+ | ''Alex'' | ||
+ | |||
+ | Obtained data from QS main experiment | ||
+ | *uploaded [[media:QS_exp_2.xls|here]] | ||
+ | |||
+ | Only the wells with LB added to pellet had a significant increase in fluorescence over time. | ||
+ | *This doesn't make sense, but seems to replicate earlier results. | ||
+ | It seems that the LB blank well was contaminated slightly. This shouldn't really matter, unless the contamination was also in the other two LB wells, in which case maybe co-culture was what cause the increase in fluorescence. However, OD also only increased significantly for the LB wells, so this is probably why the fluorescence also increased. | ||
+ | This does present another experiment idea, however: maybe we can try to culture MDAI2 alone, and then in co-culture with K12 to see if there it a difference in GFP. | ||
+ | At any rate, I'm not sure it's feasible to co-culture with algae, so quorum sensing project is probably done. | ||
+ | |||
+ | |width="250px" style="background: transparent"| | ||
+ | |||
+ | ==='''In the Lab'''=== | ||
+ | |||
+ | [[Image:QS01.jpg|middle|250px]] | ||
+ | |||
+ | [[Image:QS02.jpg|middle|250px]] | ||
+ | |||
+ | [[Image:QS03.jpg|middle|250px]] | ||
+ | |||
+ | [[Image:QS04.jpg|middle|250px]] | ||
+ | |||
+ | [[Image:QS05.jpg|middle|250px]] | ||
+ | |||
+ | [[Image:QS06.jpg|middle|250px]] | ||
+ | |||
+ | [[Image:QS07.jpg|middle|250px]] |
Latest revision as of 01:14, 27 October 2010