Team:Lethbridge/Notebook/Lab Work/May
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- | == | + | <br> |
- | ===May 5/2010=== | + | |
+ | <align="centre"> | ||
+ | <table border="0" width="100%" style="background-color:#000000"> | ||
+ | |||
+ | <tr> | ||
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+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Safety"> | ||
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+ | <font color="white">Feel free to look around our notebook! | ||
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+ | |||
+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Protocols"> | ||
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+ | <font color="white">Here you can check out the work we have done in the lab, click on a month to take a look! | ||
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+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/April"> | ||
+ | <img src="https://static.igem.org/mediawiki/2010/8/8a/UofLapril.jpg" width="60"/> | ||
+ | </a> | ||
+ | </th> | ||
+ | |||
+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/May"> | ||
+ | <img src="https://static.igem.org/mediawiki/2010/7/7b/UofLmaybutton.jpg" width="80"/> | ||
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+ | |||
+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/June"> | ||
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+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/July"> | ||
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+ | |||
+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/August"> | ||
+ | <img src="https://static.igem.org/mediawiki/2010/1/15/UofLaugustbutton.jpg" width="60"/> | ||
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+ | </th> | ||
+ | |||
+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/September"> | ||
+ | <img src="https://static.igem.org/mediawiki/2010/4/4d/UofLseptemberbutton.jpg" width="60"/> | ||
+ | </a> | ||
+ | </th> | ||
+ | |||
+ | <th><a href="https://2010.igem.org/Team:Lethbridge/Notebook/Lab_Work/October"> | ||
+ | <img src="https://static.igem.org/mediawiki/2010/4/4e/UofLoctoberbutton.jpg" width="60"/> | ||
+ | </a> | ||
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+ | |||
+ | |||
+ | <tr> | ||
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+ | <hr> | ||
+ | |||
+ | <BLOCKQUOTE> | ||
+ | |||
+ | =<font color="white">May= | ||
+ | ==<font color="white">May 5/2010== | ||
(in the lab: JV)<br> | (in the lab: JV)<br> | ||
<b>Objective:</b> Test Restriction Endonucleases for activity (take 2)<br> | <b>Objective:</b> Test Restriction Endonucleases for activity (take 2)<br> | ||
Line 56: | Line 211: | ||
Reactions will be assembled as follows:<br> | Reactions will be assembled as follows:<br> | ||
<table><table border="3"> | <table><table border="3"> | ||
- | <tr><td><b>Enzyme<td>Buffer<td>Volume MM(µL)<td>Volume Enzyme(µL)</b> | + | <tr><td><b>Enzyme</b></td><td><b>Buffer</b></td><td><b>Volume MM(µL)</b></td><td><b>Volume Enzyme(µL)</b></td></tr> |
- | <tr><td>PstI</td><td>Red</td><td>19.75</td><td>.25</td></tr> | + | <tr><td>PstI</td><td>Red</td><td>19.75</td><td>0.25</td></tr> |
- | <tr><td>XbaI</td><td>Tango</td><td>19.75</td><td>.25</td></tr> | + | <tr><td>XbaI</td><td>Tango</td><td>19.75</td><td>0.25</td></tr> |
- | <tr><td>SpeI</td><td>Tango</td><td>19.75</td><td>.25</td></tr> | + | <tr><td>SpeI</td><td>Tango</td><td>19.75</td><td>0.25</td></tr> |
- | <tr><td>EcoRI</td><td>Red</td><td>19.75</td><td>.25</td></tr> | + | <tr><td>EcoRI</td><td>Red</td><td>19.75</td><td>0.25</td></tr> |
- | <tr><td>EcoRI/SpeI</td><td>Red</td><td>19.5</td><td>.25+.25</td></tr> | + | <tr><td>EcoRI/SpeI</td><td>Red</td><td>19.5</td><td>0.25 + 0.25</td></tr> |
- | <tr><td>XbaI/SpeI</td><td>Tango</td><td>19.5</td><td>.25+.25</td></tr> | + | <tr><td>XbaI/SpeI</td><td>Tango</td><td>19.5</td><td>0.25 + 0.25</td></tr> |
- | <tr><td>EcoRI/PstI</td><td>Red</td><td>19.5</td><td>.25+.25</td></tr> | + | <tr><td>EcoRI/PstI</td><td>Red</td><td>19.5</td><td>0.25 + 0.25</td></tr> |
- | <tr><td>XbaI/PstI</td><td>Tango</td><td>19.5</td><td>.25+.25</td></tr> | + | <tr><td>XbaI/PstI</td><td>Tango</td><td>19.5</td><td>0.25 + 0.25</td></tr> |
</table><br> | </table><br> | ||
Make up Master Mixes as follows:<br> | Make up Master Mixes as follows:<br> | ||
Line 106: | Line 261: | ||
<b>Conclusion:</b> Test other source of SpeI to see if it has any activity.<br><br> | <b>Conclusion:</b> Test other source of SpeI to see if it has any activity.<br><br> | ||
- | ===May 6/2010 | + | ==<font color="white">May 6/2010== |
- | (in the lab:KG, AS)<br> | + | (in the lab: KG, AS)<br> |
<b>Objective:</b> To check if the old SpeI enzyme (exp date: March 2011) will cleave plasmid DNA, since we believe the newer SpeI enzyme (exp date: 2012) does not.<br> | <b>Objective:</b> To check if the old SpeI enzyme (exp date: March 2011) will cleave plasmid DNA, since we believe the newer SpeI enzyme (exp date: 2012) does not.<br> | ||
<b>Method:</b><br> | <b>Method:</b><br> | ||
Line 141: | Line 296: | ||
S(N); SpeI(N)<br> | S(N); SpeI(N)<br> | ||
S(O); SpeI(O)<br><br> | S(O); SpeI(O)<br><br> | ||
- | Placed in -20<sup>o</sup>C freezer of later analysis by agarose electrophoresis<br> | + | Placed in -20<sup>o</sup>C freezer of later analysis by agarose electrophoresis<br> |
- | + | ||
- | ===May 10/2010 | + | ==<font color="white">May 10/2010== |
(in the lab:JV)<br> | (in the lab:JV)<br> | ||
<b>Objective:</b> To analyze the restriction test done by KG and AS on May 6/2010 by agarose electrophoresis<br><br> | <b>Objective:</b> To analyze the restriction test done by KG and AS on May 6/2010 by agarose electrophoresis<br><br> | ||
Line 176: | Line 330: | ||
Add 500µL of stock ampicillin to 500mL of media<br><br> | Add 500µL of stock ampicillin to 500mL of media<br><br> | ||
- | ===May 11/2010 Evening | + | ==<font color="white">May 11/2010 Evening== |
- | (in the lab: KG, AV, MC, TF, JV, JS)< | + | (in the lab: KG, AV, MC, TF, JV, JS)<br> |
<b>Objective:</b> To transform the following plasmids into DH5α <i>E.coli</i> cells. | <b>Objective:</b> To transform the following plasmids into DH5α <i>E.coli</i> cells. | ||
<table><table border="3"> | <table><table border="3"> | ||
Line 216: | Line 370: | ||
<li>pTet</li></ul><br> | <li>pTet</li></ul><br> | ||
- | ===May 12/2010 | + | ==<font color="white">May 12/2010== |
(in the lab: JV)<br> | (in the lab: JV)<br> | ||
<b>Objective: Miniprep of plasmid DNA from transformed cells</b>(JV, AV, HB)<br> | <b>Objective: Miniprep of plasmid DNA from transformed cells</b>(JV, AV, HB)<br> | ||
Line 336: | Line 490: | ||
Start overnight cultures of cells that grew for plasmid prep and sequencing.<br><br> | Start overnight cultures of cells that grew for plasmid prep and sequencing.<br><br> | ||
- | ===May 14/2010 | + | ==<font color="white">May 14/2010== |
(in the lab: JV)<br> | (in the lab: JV)<br> | ||
<b>Objective:</b> Quantify pDNA concentration in order to ensure sufficient material for sequence analysis.<br> | <b>Objective:</b> Quantify pDNA concentration in order to ensure sufficient material for sequence analysis.<br> | ||
Line 408: | Line 562: | ||
There is plasmid DNA in each sample which, when cut with both the prefix and suffix enzyme, yields a band approximately 2000bp (size of pSB1A3 is 2157bp).<br><br> | There is plasmid DNA in each sample which, when cut with both the prefix and suffix enzyme, yields a band approximately 2000bp (size of pSB1A3 is 2157bp).<br><br> | ||
- | ===May 17/2010 | + | ==<font color="white">May 17/2010== |
(in the lab: JV, AV)<br> | (in the lab: JV, AV)<br> | ||
Make agar plates with 100µg/mL of ampicillin<br> | Make agar plates with 100µg/mL of ampicillin<br> | ||
Line 414: | Line 568: | ||
Make 13 x 5mL sterile liquid LB broth<br><br> | Make 13 x 5mL sterile liquid LB broth<br><br> | ||
- | ===May 17/2010 Evening | + | ==<font color="white">May 17/2010 Evening== |
(in the lab: TF, AS)<br> | (in the lab: TF, AS)<br> | ||
<b>Objective:</b> To grow cells for future use<br> | <b>Objective:</b> To grow cells for future use<br> | ||
Line 447: | Line 601: | ||
Only sRBS (D5) and pBad-TetR cells (from transformation plates) grew.<br> | Only sRBS (D5) and pBad-TetR cells (from transformation plates) grew.<br> | ||
- | ===May 18/2010 | + | ==<font color="white">May 18/2010== |
(in the lab: JV, AV, HB)<br> | (in the lab: JV, AV, HB)<br> | ||
<b>NOTE:</b> Cells from liquid cultures grown last night (May 17/2010) were made into glycerol stocks and placed into the [[Team:Lethbridge/Notebook/Working_Glycerol_Stocks|working glycerol stock box]] as follows:<br> | <b>NOTE:</b> Cells from liquid cultures grown last night (May 17/2010) were made into glycerol stocks and placed into the [[Team:Lethbridge/Notebook/Working_Glycerol_Stocks|working glycerol stock box]] as follows:<br> | ||
Line 540: | Line 694: | ||
<li>xylE (C4-2007 Box)</li></ul><br> | <li>xylE (C4-2007 Box)</li></ul><br> | ||
- | ===May 18/2010 Evening | + | ==<font color="white">May 18/2010 Evening== |
(in the lab: KG)<br> | (in the lab: KG)<br> | ||
<b>Objective:</b> Restrict pLacI, sRNS, sRBS-Lumazine Synthase-dt out of plasmid then ligase pLacI and sRBS also pLacI sRBS-Lumazine Synthase-dt.<br> | <b>Objective:</b> Restrict pLacI, sRNS, sRBS-Lumazine Synthase-dt out of plasmid then ligase pLacI and sRBS also pLacI sRBS-Lumazine Synthase-dt.<br> | ||
Line 603: | Line 757: | ||
<tr><tr>sRBS-Lumazine Synthase-dt</table><br> | <tr><tr>sRBS-Lumazine Synthase-dt</table><br> | ||
Begin room temperature incubation at 8:25pm. | Begin room temperature incubation at 8:25pm. | ||
- | ===May 19/2010 | + | |
+ | ==<font color="white">May 19/2010== | ||
(in the lab:JV)<br> | (in the lab:JV)<br> | ||
Line 637: | Line 792: | ||
Reactions ran for 1 hour at 37<sup>o</sup>C.<br> | Reactions ran for 1 hour at 37<sup>o</sup>C.<br> | ||
- | ===May 20/2010 | + | ==<font color="white">May 20/2010== |
(in the lab:JV, AV)<br> | (in the lab:JV, AV)<br> | ||
Line 674: | Line 829: | ||
[[image:100520AV.JV-Plasmid Check.JPG|200px|none]] | [[image:100520AV.JV-Plasmid Check.JPG|200px|none]] | ||
- | ===May 20/2010 Evening | + | ==<font color="white">May 20/2010 Evening== |
(in the lab:JS, AS)<br> | (in the lab:JS, AS)<br> | ||
Line 712: | Line 867: | ||
[[image:100520JS1.JPG|200px|none]] | [[image:100520JS1.JPG|200px|none]] | ||
- | ===May 25/2010 | + | ==<font color="white">May 25/2010== |
(in the lab:JV, HB, AV)<br> | (in the lab:JV, HB, AV)<br> | ||
Line 726: | Line 881: | ||
<b>NOTE</b> (June 1/2010; AS): Likely that the problem here was the method used to heat shock the cells. Cells were heat shocked in a heat plate, with incomplete contact of the heating surface, causing inefficient transfer of heat to cells for shock and movement of DNA into competent cells. | <b>NOTE</b> (June 1/2010; AS): Likely that the problem here was the method used to heat shock the cells. Cells were heat shocked in a heat plate, with incomplete contact of the heating surface, causing inefficient transfer of heat to cells for shock and movement of DNA into competent cells. | ||
- | ===May 25/2010 Evening | + | ==<font color="white">May 25/2010 Evening== |
(in the lab: AV, KG)<br> | (in the lab: AV, KG)<br> | ||
Line 865: | Line 1,020: | ||
Removed at 9:30pm<br> | Removed at 9:30pm<br> | ||
- | ===May 26/2010 | + | ==<font color="white">May 26/2010== |
(In the lab: JV)<br> | (In the lab: JV)<br> | ||
<b>Objective:</b> Purify plasmid DNA (via mini-prep) of the cells grown last night.<br> | <b>Objective:</b> Purify plasmid DNA (via mini-prep) of the cells grown last night.<br> | ||
Line 886: | Line 1,041: | ||
<b>Results:</b> Will restrict and run agarose gels tomorrow.<br> | <b>Results:</b> Will restrict and run agarose gels tomorrow.<br> | ||
- | ===May 27/2010 | + | ==<font color="white">May 27/2010== |
(In the lab: JV, AV)<br> | (In the lab: JV, AV)<br> | ||
Line 953: | Line 1,108: | ||
† Also added 8µL of water to this mix<br><br> | † Also added 8µL of water to this mix<br><br> | ||
Ran both gels at 100V for 2 hours.<br> | Ran both gels at 100V for 2 hours.<br> | ||
+ | <b>Results:</b><br> | ||
+ | Gel 1<br> | ||
+ | [[image:100527 AV Plasmid Test 1.jpg|200px|none]]<br> | ||
+ | Gel 2<br> | ||
+ | [[image:100527 JV Plasmid Test 1.jpg|200px|none]]<br> | ||
+ | <b>Conclusion:</b> To be concluded....<br><br> | ||
+ | |||
+ | <b>Objective:</b> Transform DH5α cells with plasmids containing ligation products from May 25/2010.<br> | ||
+ | <b>Method:</b> | ||
+ | Transform, using the [[Team:Lethbridge/Notebook/Protocols|competent cell transformation]] protocol, the ligation products with the most intense banding from each of the following ligation reactions:<br> | ||
+ | *mms6 + dT (B6 + A6)<br> | ||
+ | *xylE + dT (B4 + C4)<br> | ||
+ | Incubate at 37<sup>o</sup>C overnight.<br> | ||
+ | <b>Results:</b><br> | ||
+ | No colonies grew, even on positive control plate.<br> | ||
+ | ===May 31/2010=== | ||
+ | <b>Objective:</b> Transform part BBa_J33204 (Ribosomal Binding Site + xylE gene) into DH5α cells.<br> | ||
+ | <b>Method:</b><br> | ||
+ | Obtained part BBa_J33204 from 2010 iGEM Spring Distribution Kit Plate 1, well 7P.<br> | ||
+ | Transformed using [[Team:Lethbridge/Notebook/Protocols|competent cell transformation]] protocol, along with negative control (milliQ H<sub>2</sub>O water) and positive control (pUC19 plasmid). | ||
+ | Plated 100µL and 50µL on separate pre-warmed LB agar plates containing 100µg/mL ampicillin.<br> | ||
+ | Added 250µL of SOC media and incubated for <u>90 minutes</u> at 37<sup>o</sup>. <br> | ||
+ | <b>Results:</b><br> | ||
+ | Obtained the following number of colonies on each plate: | ||
+ | *BBa_J33204 50µL - 13 colonies<br> | ||
+ | *BBa_J33204 100µL - 18 colonies<br> | ||
+ | *pUC19 - 9 colonies<br> | ||
+ | <b>Other lab activities:</b><br> | ||
+ | *Inoculated 5mL of LB liquid broth (Amp<sup>+</sup> with cells containing Bba_J33204 picked from colony off transformation plate and incubated at 37<sup>o</sup>C with shaking overnight.<br><br> | ||
+ | AV quantified each pDNA stock in the [[Team:Lethbridge/Notebook/Working_Plasmids|working plasmids box]] by measuring the A<sub>260</sub> of a 1:100 dilution of the pDNA samples in a UV cuvette. Results are posted on the [[Team:Lethbridge/Notebook/Working_Plasmids|working plasmids]] page.<br> | ||
+ | |||
+ | ==<font color="white">May 31/2010 - Evening== | ||
+ | <b>Objective:</b> Transform recent ligation reactions that didn't work the first time around.<br> | ||
+ | <b>Method:</b> Use [[Team:Lethbridge/Notebook/Protocols|competent cell transformation]] protocol to transform the following ligation products:<br> | ||
+ | *pLacI + sRBS<br> | ||
+ | *pLacI + sRBS-Lum-dT (times 2)<br> | ||
+ | *mms6 (B6) + dT<br> | ||
+ | *mms6 (A6) + dT<br> | ||
+ | *xylE (C4) + dT<br> | ||
+ | *xylE (B4) + dT<br> | ||
+ | Plated all cells; spun down media so cells were pelleted and removed 200uL of cell-free media. Re-suspended pelleted cells in remaining media, and plated onto ampicillin plates.<br> | ||
+ | <b>Results:</b><br> | ||
+ | No growth on plates EXCEPT: | ||
+ | *Positive control (pUC19) - 9 colonies <br> | ||
+ | *mms6 (B6) + dT - 1 colonies <br><br> | ||
+ | <br> |