Team:Lethbridge/Notebook/Lab Work/August

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(Aug 16, 2010 Evening)
 
(54 intermediate revisions not shown)
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<b>Method:</b> Used [[Team:Lethbridge/Notebook/Protocols|Restriction of Plasmid DNA]] protocol.
<b>Method:</b> Used [[Team:Lethbridge/Notebook/Protocols|Restriction of Plasmid DNA]] protocol.
-
* A front verctor was made made in sRBS ,mRBS, dT plasmids using EcoRI and Xbal enzymes
+
* A front vector was made made in sRBS ,mRBS, dT plasmids using EcoRI and Xbal enzymes
* pDNA that was cut out of plasmid for a front vector was pBAD, TetR, dT and pLacI using EcoRI and SpeI enzymes
* pDNA that was cut out of plasmid for a front vector was pBAD, TetR, dT and pLacI using EcoRI and SpeI enzymes
* A back vector was made in sRBS and mRBS plasmids with PstI and SpeI
* A back vector was made in sRBS and mRBS plasmids with PstI and SpeI
Line 252: Line 252:
</table>
</table>
*Added 48.8 &micro;L of Master Mix to each PCR reaction<br><br><br>
*Added 48.8 &micro;L of Master Mix to each PCR reaction<br><br><br>
 +
 +
<b>Objective:</b> Complete maxipreps of Lumazine (K249002), EYFP (E0030), and ECFP (E0020) and run on 1% agarose gel.<br>
<b>Objective:</b> Complete maxipreps of Lumazine (K249002), EYFP (E0030), and ECFP (E0020) and run on 1% agarose gel.<br>
<b>Method:</b><br>
<b>Method:</b><br>
Line 262: Line 264:
</table>
</table>
*Ran at 100V for 42 minutes. Stained in EtBr for 15 minutes.<br>  
*Ran at 100V for 42 minutes. Stained in EtBr for 15 minutes.<br>  
-
<b>Results:</b> <font color ="red">AGAROSE GEL PICTURE</font><br><br><br>
+
<b>Results:</b> [[image:Lethbridge_100803JV Maxiprep.JPG|50px]]<br><br><br>
 +
 
 +
 
<b>Objective:</b> Ligate dT into pSB1C3.<br>
<b>Objective:</b> Ligate dT into pSB1C3.<br>
<b>Method:</b><br>
<b>Method:</b><br>
Line 331: Line 335:
<tr><td>20<td>pLacI PCR product<td> good
<tr><td>20<td>pLacI PCR product<td> good
</table><br>
</table><br>
 +
 +
[[image:Lethbridge_100803AS.JPG|200px]]
----
----
<b>Objective:</b> To ligate: pBAD-sRBS/mRBS, sRBS/mRBS-TetR, TetR-dT, dT-pTet, pLacI-sRBS/mRBS, Mms6-ptet28(a), dT-PSB1C3<br>
<b>Objective:</b> To ligate: pBAD-sRBS/mRBS, sRBS/mRBS-TetR, TetR-dT, dT-pTet, pLacI-sRBS/mRBS, Mms6-ptet28(a), dT-PSB1C3<br>
-
<b>Method:</b> [[Team:Lethbridge/Notebook/Protocols|Ligation of Plasmid DNA]]
+
<b>Method:</b> [[Team:Lethbridge/Notebook/Protocols|Ligation of Plasmid DNA]]<br>
-
15 (&micro;L) pDNA in plasmid, and 15 (&micro;L) of pDNA biobrick)<br>
+
15&micro;L pDNA in plasmid, and 15 &micro;L of pDNA biobrick
==<font color="white">August 4, 2010==
==<font color="white">August 4, 2010==
Line 392: Line 398:
*Ran at 100V for 70 minutes.
*Ran at 100V for 70 minutes.
-
<b>Results:</b> <font color ="red">AGAROSE GEL PICTURE</font><br><br><br>
+
<b>Results:</b>[[image:Lethbridge_100804 JV Ligation PCR AS.JPG|200px]] <br><br><br>
 +
 
 +
 
 +
 
<b>Objective:</b> Transform the successful ligations<br>
<b>Objective:</b> Transform the successful ligations<br>
Line 454: Line 463:
Gel ran for 60 minutes at 100 V.  Small & faint band was slightly visible.
Gel ran for 60 minutes at 100 V.  Small & faint band was slightly visible.
-
Gel extraction was carried out using QIAGEN method.  Eluted to 12 (&micro;L).
+
Gel extraction was carried out using QIAGEN method.  Eluted to 12 (&micro;L).<br>
 +
[[image:Lethbridge_100809 JV Mms6 Gel Extract BW.jpg|200px]]
==<font color="white">August 6, 2010 Evening==
==<font color="white">August 6, 2010 Evening==
Line 522: Line 532:
<tr><td>7<td>lumazine(justin's)<td>5(&micro;L) sample, 1(&micro;L)dye
<tr><td>7<td>lumazine(justin's)<td>5(&micro;L) sample, 1(&micro;L)dye
</table><br>
</table><br>
 +
[[image:Lethbridge_100806ADSPCR.JPG|200px]]
Repeat gel with template controls
Repeat gel with template controls
Line 537: Line 548:
<tr><td>1<td>1Kb ladder<td>0.5(&micro;L) ladder, 2(&micro;L) dye, 9.5(&micro;L) H<sub>2</sub>0
<tr><td>1<td>1Kb ladder<td>0.5(&micro;L) ladder, 2(&micro;L) dye, 9.5(&micro;L) H<sub>2</sub>0
</table><br>
</table><br>
 +
[[image:Lethbridge_100809AS-PCR.jpg|200px]]
*ran at 100V for 75 minutes
*ran at 100V for 75 minutes
Line 570: Line 582:
</table><br>
</table><br>
-
Ran at 100 V for 45 minutes.  mRBS-xylE did not amplify while lumazine did amplify.   
+
Ran at 100 V for 45 minutes.  mRBS-xylE did not amplify while lumazine did amplify.  <br>
-
GEL PICTURE! 
+
<b>Results:</b> Ligation of mRBS-xylE NOT confirmed<br>
 +
[[image:Lethbridge_100809 HB xylE Lum PCR BW.jpg|50px]]
 +
 
----
----
Line 656: Line 670:
<tr><td>20<td>pLacI-sRBS 3 URD
<tr><td>20<td>pLacI-sRBS 3 URD
</table><br>
</table><br>
 +
[[image:Lethbridge_100809AVKG Top.jpg|200px]]
<table border ="3">
<table border ="3">
Line 681: Line 696:
</table><br>
</table><br>
-
GEL PICTURE!
+
[[image:Lethbridge_100809AVKG Bottom.jpg|200px]]
----
----
Line 690: Line 705:
<b>Method:</b><br>
<b>Method:</b><br>
-
<ul>
+
 
-
<li><u>Restrictions</u><br>
+
<u>Restrictions</u><br>
*Restrict Lumazine wit EcoRI and SpeI (Red Buffer)<br>
*Restrict Lumazine wit EcoRI and SpeI (Red Buffer)<br>
*Restrict the dT with XbaI and EcoRI (Orange Buffer)<br>
*Restrict the dT with XbaI and EcoRI (Orange Buffer)<br>
Line 706: Line 721:
Incubated reactions for 60 minutes at 37<sup>o</sup>C<br>
Incubated reactions for 60 minutes at 37<sup>o</sup>C<br>
-
<li><u>Ligation</u><br>
+
<u>Ligation</u><br>
Reaction set up as follows:
Reaction set up as follows:
*T4 DNA ligase - 0.25&micro;L<br>
*T4 DNA ligase - 0.25&micro;L<br>
Line 771: Line 786:
</table><br>
</table><br>
-
GEL PICTURE!
+
[[image:Lethbridge_100810ReRunRestrictionDigers.JPG|200px]]
----
----
Line 814: Line 829:
</table><br>
</table><br>
-
Controls:  sRBS, pTET & mRBS - will PCR these to compare size using same conditions as above.
+
Controls:  sRBS, pTET & mRBS - will PCR these to compare size using same conditions as above. <br>
-
 
+
[[image:Lethbridge_100810MassiveColonyPCR JV AS.JPG|200px]]<br>
-
GEL PICTURE!
+
[[image:Lethbridge_100810MassiveColonyPCR Large Gel JV AS.JPG|200px]]
==<font color="white">Aug 10, 2010 Evening==
==<font color="white">Aug 10, 2010 Evening==
Line 847: Line 862:
</table><br>
</table><br>
   
   
-
Ran samples on 1.5% agarose gel (1X TAE) for 60 minutes at 100V.  
+
Ran samples on 1.5% agarose gel (1X TAE) for 60 minutes at 100V. <br>
-
GEL PICTURE!
+
<b>Results:</b><br>
 +
[[image:Lethbridge_100810xylE PCR AS.JPG|100px]]
==<font color="white">Aug 11, 2010==
==<font color="white">Aug 11, 2010==
Line 907: Line 923:
<b>Results:</b>  Lanes 2, 3, 4 and 8 showed PCR amplification.  Colonies chosen don't show the correct insert size. <br>
<b>Results:</b>  Lanes 2, 3, 4 and 8 showed PCR amplification.  Colonies chosen don't show the correct insert size. <br>
 +
[[image:Lethbridge_100812 JV AS Colony PCR Pfu.JPG|200px]]
----
----
Line 935: Line 952:
</table><br>
</table><br>
-
Added 18&micro;L Master Mix to each reaction tube.
+
Added 18&micro;L Master Mix to each reaction tube.<br>
-
Analyzed PCR products on 2.5% TAE gel.
+
Analyzed PCR products on 2.5% TAE gel.<br>
-
GEL PICTURE!!!
+
<b>Results:</b><br>
 +
[[image:Lethbridge_100812ASJVMassColonyPCRLargeGel (1).JPG|200px]]<br><br>
 +
[[image:Lethbridge_100812ASJVMassColonyPCRSmallGel.JPG|200px]]
----
----
Line 966: Line 985:
</table><br>
</table><br>
-
Added 18&micro;L Master Mix to each reaction tube.
+
Added 18&micro;L Master Mix to each reaction tube.<br>
-
Analyzed PCR products on 2.5% TAE gel run at 100 V for 35 minutes.
+
Analyzed PCR products on 2.5% TAE gel run at 100 V for 35 minutes.<br>
-
GEL PICTURE!!!
+
[[image:Lethbridge_100813ADS Awesome PCR.JPG|200px]]
==<font color="white">Aug 13, 2010==
==<font color="white">Aug 13, 2010==
Line 988: Line 1,007:
</table><br>
</table><br>
-
Added 49&micro;L Master Mix to each reaction tube.
+
Added 49&micro;L Master Mix to each reaction tube.<br>
 +
 
----
----
Line 1,015: Line 1,035:
(36 cycles)
(36 cycles)
-
Added 19.5&micro;L Master Mix to each reaction tube.
+
Added 19.5&micro;L Master Mix to each reaction tube.<br>
-
Analyzed products on 1% TAE agarose gel which ran for 60 minutes at 100 V.   
+
Analyzed products on 1% TAE agarose gel which ran for 60 minutes at 100 V.<br>  
-
GEL PICTURE!
+
<b>Results:</b><br>
 +
[[image:Lethbridge_100814PlasmidBackbones.JPG|100px]]
==<font color="white">Aug 14, 2010==
==<font color="white">Aug 14, 2010==
Line 1,047: Line 1,068:
<tr><td>19<td>MT
<tr><td>19<td>MT
<tr><td>20<td>MT
<tr><td>20<td>MT
-
<tr><td>21<td>No Lanes
 
-
<tr><td>22<td>No Lanes
 
-
<tr><td>23<td>No Lanes
 
-
<tr><td>24<td>No Lanes
 
-
<tr><td>25<td>No Lanes
 
-
<tr><td>26<td>No Lanes
 
-
<tr><td>27<td>No Lanes
 
</table>
</table>
Line 1,087: Line 1,101:
</table>
</table>
-
GEL PICTURE!
+
[[image:Lethbridge_100815MiniprepPCR.JPG|200px]]
----
----
Line 1,119: Line 1,133:
Incubated at 37<sup>o</sup>C.
Incubated at 37<sup>o</sup>C.
-
Analyzed results on 2.5% TAE agarose gel which ran at 100 V for 50 minutes.
+
Analyzed results on 2.5% TAE agarose gel which ran at 100 V for 50 minutes.<br>
-
GEL PICTURE!!!
+
[[image:Lethbridge_100814ColonyPCRRetryandStartofassembly.JPG|200px]]
<b>Results:</b>  Lost all the DNA in the column clean-up step and will have to re-do.<br>
<b>Results:</b>  Lost all the DNA in the column clean-up step and will have to re-do.<br>
Line 1,130: Line 1,144:
<b>Objective:</b> Assemble mms6-dT and lumazine-dT using three antibiotic assembly. <br>
<b>Objective:</b> Assemble mms6-dT and lumazine-dT using three antibiotic assembly. <br>
-
<b>Method:</b>  1.  PCR amplify BioBricks (Prefix/Suffix)  2.  Restrict BioBricks  3.  Ligate BioBricks into psB1C3  4. Confirm ligation by PCR analysis (VF2/VR)  5.  Transform ligation mixes  6.  Screen colonies with Colony PCR  <br>
+
<b>Method:</b>   
 +
#PCR amplify BioBricks (Prefix/Suffix)   
 +
#Restrict BioBricks   
 +
#Ligate BioBricks into psB1C3   
 +
#Confirm ligation by PCR analysis (VF2/VR)   
 +
#Transform ligation mixes   
 +
#Screen colonies with Colony PCR   
<u>PCR:</u> Thermocycler set to iGEM program 11<br>
<u>PCR:</u> Thermocycler set to iGEM program 11<br>
Line 1,170: Line 1,190:
</table>
</table>
-
For psB1C3 -  
+
For pSB1C3 -  
<table><table border ="3">
<table><table border ="3">
<tr><td><b>Ingredient</b><td><b>Reaction Mix(&micro;L)</b>
<tr><td><b>Ingredient</b><td><b>Reaction Mix(&micro;L)</b>
Line 1,258: Line 1,278:
</table><br>
</table><br>
    
    
-
Added 15 (&micro;L) MM to each tube.
+
Added 15 (&micro;L) MM to each tube.<br>
 +
<b>Results:</b><br>
==<font color="white">Aug 15, 2010==
==<font color="white">Aug 15, 2010==
Line 1,363: Line 1,384:
Added 45 (&micro;L) MM to each tube.
Added 45 (&micro;L) MM to each tube.
-
Analyzed PCR products of BioBrick standard assembly; 3 part (or 3 antibiotic) assembly; and 3 part (3AB) Intermediate/2 part assembly on a 2% TAE agarose gel.   
+
Analyzed PCR products of BioBrick standard assembly; 3 part (or 3 antibiotic) assembly; and 3 part (3AB) Intermediate/2 part assembly on a 2% TAE agarose gel.  <br>
 +
<b>Results:</b><br>
 +
[[image:Lethbridge_100815PCRAssembly.JPG|200px]]
-
GEL PICTURE!
+
 
 +
----
 +
(In Lab: ADS)<br>
 +
 
 +
<b>Objective:</b> Produce large quantities of pSB1A3, pSB1C3 and pSB1T3.<br>
 +
 
 +
<b>Method:</b><br>
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x3.2)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>75<td>240
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>10<td>32
 +
<tr><td>dNTPs<td>5<td>16
 +
<tr><td>Primer (SB-prep-2Ea)<td>3.5<td>11.2
 +
<tr><td>Primer (SB-prep-3P)<td>3.5<td>11.2
 +
<tr><td>Template DNA<td>2<td>
 +
<tr><td>Pfu polymerase<td>1<td>3.2
 +
</table><br>
 +
 
 +
Added 98(&micro;L) to each tube.  Used PLASRB PCR Protocol from Aug. 13, 2010.
==<font color="white">Aug 16, 2010 ==
==<font color="white">Aug 16, 2010 ==
Line 1,412: Line 1,453:
</table><br>
</table><br>
-
Analyzed PCR products of overnight BioBrick standard assembly; 3 part (or 3 antibiotic) assembly; and 3 part (3AB) Intermediate/2 part assembly on a 2% TAE agarose gel.  
+
Analyzed PCR products of overnight BioBrick standard assembly; 3 part (or 3 antibiotic) assembly; and 3 part (3AB) Intermediate/2 part assembly on a 2% TAE agarose gel. <br>
-
 
+
<b>Results:</b><br>
-
GEL PICTURE!
+
[[image:Lethbridge_100816PostLigationPCRScreen.JPG|200px]]
==<font color="white">Aug 16, 2010 Evening ==
==<font color="white">Aug 16, 2010 Evening ==
Line 1,452: Line 1,493:
<b>Objective:</b> Transformations of insertions of mms6 or lumazine into pET28a. <br>
<b>Objective:</b> Transformations of insertions of mms6 or lumazine into pET28a. <br>
-
<b>Method:</b> Transformation of competent cells protocol.<br>
+
<b>Method:</b> used [[Team:Lethbridge/Notebook/Protocols|Competent Cell Transformation]] protocol
 +
* changes:
 +
**used 50&micro;L aliquottes of DH5&alpha
 +
**did not pipette up and down once, the cells were just swirled 3 times
 +
**added 400&micro;L SOC media, shoock at 37<sup>0</sup>C for 90 min
 +
**platted 250&micro;L and 150&micro;L<br>
-
With the following changes:
+
<table border ="3">
-
1.  50(&micro;L) aliquots of DH5alpha.
+
<td><b>results</b>
-
2.  Added 400(&micro;L) SOC media and put in shaker for 90 minutes at 37<sup>o</sup>C. 
+
<tr><td>contents<td><b>&250&micro;L</b><td><b>150&micro;L</b>
-
3.  Plated 150(&micro;L) and 250(&micro;L).
+
<tr><td>+ control(pUC19)<td>good<td>good
-
 
+
<tr><td>mms6<td>good<td>good
-
<b>Results:</b> .<br>
+
<tr><td>mms6-2<td>good<td>good
 +
<tr><td>mms6<td>good<td>x
 +
<tr><td>Lumazine<td>good<td>x
 +
<tr><td>Lumazine<td>good<td>x
 +
</table><br>
==<font color="white">Aug 17, 2010 ==
==<font color="white">Aug 17, 2010 ==
Line 1,481: Line 1,531:
</table><br>
</table><br>
-
Ran a 2% Agarose gel in 1X TAE buffer for 65 minutes at 100V.
+
Ran a 2% Agarose gel in 1X TAE buffer for 65 minutes at 100V.<br>
-
 
+
[[image:Lethbridge_100817PostLigationPCRTest.JPG|100px]]
-
GEL PICTURE!
+
==<font color="white">Aug 17, 2010 Evening ==
==<font color="white">Aug 17, 2010 Evening ==
Line 1,548: Line 1,597:
Added 45(&micro;L) MM to each rxn tube.
Added 45(&micro;L) MM to each rxn tube.
 +
----
 +
<b>Objective:</b> Analyze tendency of PstI to be heat killed.  <br>
 +
<b>Hypothesis:</b> Ligation will be counteracted by PstI digestion even following 20 minute heat kill at 80<sup>o</sup>C .<br>
 +
<b>Method:</b> Restrict plasmid DNA with PstI (and EcoRI control).  Reactions stopped by heat killing.  Plasmids re-ligated with T4 DNA Ligase.  Ligation confirmed with PCR.  If PCR product is present then enzyme heat killed but if there is no PCR Product then enzyme was not heat killed.  <br>
 +
 +
<u>Restriction Reactions:</u>
 +
<table><table border ="3">
 +
<tr><td><b>Ingredient</b><td><b>1X(&micro;L)</b>
 +
<tr><td>MilliQ H<sub>2</sub>0 Water</td><td>12.8
 +
<tr><td>Orange Buffer (10x)</td><td>2
 +
<tr><td>pDNA (dT)</td><td>5
 +
<tr><td>PstI</td><td>0.2
 +
<tr><td>EcoRI (control only)</td><td>0.2
 +
</table>
 +
 +
Incubated at 37<sup>o</sup>C  for 1.5 hours.  Heat killed enzymes for 20 minutes at 80<sup>o</sup>C.
 +
 +
<u>Ligation Reactions:</u>
 +
<table><table border ="3">
 +
<tr><td><b>Ingredient</b><td><b>1X(&micro;L)</b>
 +
<tr><td>MilliQ H<sub>2</sub>0 Water</td><td>15.8
 +
<tr><td>T4 Ligase Buffer (10x)</td><td>2
 +
<tr><td>Restriction Mix</td><td>2
 +
<tr><td>T4 DNA Ligase</td><td>0.2
 +
</table>
 +
 +
Incubated at room temperature overnight. 
 +
 +
PCR to confirm Ligation
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x2.2)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>33.8<td>74.36
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>5<td>11
 +
<tr><td>dNTPs<td>2<td>4.4
 +
<tr><td>Forward VF2 Primer<td>2<td>4.4
 +
<tr><td>Reverse VR Primer<td>2<td>4.4
 +
<tr><td>Template DNA<td>5<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>0.44
 +
</table><br>
 +
 +
Added 45(&micro;L) to each reaction tube.
 +
 +
==<font color="white">Aug 18, 2010 ==
 +
 +
(In Lab: JV)<br>
 +
<b>Objective:</b> Confirmation of ADS' analysis of PstI's tendency to be heat killed. <br>
 +
<b>Method:</b> Will PCR ligation reactions from different assembly methods and EcoRI and PstI controls. <br>
 +
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>33.8
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>5
 +
<tr><td>dNTPs<td>2
 +
<tr><td>Forward VF2 Primer<td>2
 +
<tr><td>Reverse VR Primer<td>2
 +
<tr><td>Template DNA<td>5
 +
<tr><td>Pfu polymerase<td>0.2
 +
</table><br>
 +
Ran on cycle 4 of thermocycler.
 +
 +
Viewed PCRs on 2% TAE agarose gel that ran at 110 V for 30 minutes.<br>
 +
[[image:Lethbridge_100818AssemblyandHeatKillPCR.JPG|200px]]
 +
----
 +
(In Lab: HB)<br>
 +
<b>Objective:</b> Analyze tendency of PstI to be heat killed. <br>
 +
<b>Method:</b> Restrict plasmid DNA with PstI (and EcoRI control).  Reactions stopped by heat killing.  Plasmids re-ligated with T4 DNA Ligase.  Ligation confirmed with PCR.  If PCR product is present then enzyme heat killed but if there is no PCR Product then enzyme was not heat killed.  <br>
 +
 +
<u>Restriction Reactions:</u>
 +
<table><table border ="3">
 +
<tr><td><b>Ingredient</b><td><b>1X(&micro;L)</b>
 +
<tr><td>MilliQ H<sub>2</sub>0 Water</td><td>12.8
 +
<tr><td>Orange Buffer (10x)</td><td>2
 +
<tr><td>pDNA (dT)</td><td>5
 +
<tr><td>PstI</td><td>0.2
 +
<tr><td>EcoRI (control only)</td><td>0.2
 +
</table>
 +
 +
Incubated at 37<sup>o</sup>C  for 1.5 hours.  Heat killed enzymes for 20 minutes at 80<sup>o</sup>C.
 +
 +
<u>Ligation Reactions:</u>
 +
<table><table border ="3">
 +
<tr><td><b>Ingredient</b><td><b>1X(&micro;L)</b>
 +
<tr><td>MilliQ H<sub>2</sub>0 Water</td><td>15.8
 +
<tr><td>T4 Ligase Buffer (10x)</td><td>2
 +
<tr><td>Restriction Mix</td><td>2
 +
<tr><td>T4 DNA Ligase</td><td>0.2
 +
</table>
 +
 +
Incubated at room temperature overnight. 
 +
 +
PCR to Confirm Ligation
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x6.5)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>33.8<td>219.7
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>5<td>32.5
 +
<tr><td>dNTPs<td>2<td>13
 +
<tr><td>Forward VF2 Primer<td>2<td>13
 +
<tr><td>Reverse VR Primer<td>2<td>13
 +
<tr><td>Template DNA<td>5<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>1.3
 +
</table><br>
 +
 +
Added 45(&micro;L) to each reaction tube.
 +
Used thermocycler iGEM Program 4. 
 +
 +
3 different treatments:  1.  Restricted, heat killed and ligated.  2.  Restricted and heat killed.  3. Restricted and not heat killed.
==<font color="white">Aug 19, 2010 ==
==<font color="white">Aug 19, 2010 ==
Line 1,596: Line 1,751:
Samples were run on a 2% agarose gel in 1X TAE Buffer.   
Samples were run on a 2% agarose gel in 1X TAE Buffer.   
-
GEL PICTURE!
+
----
 +
(In Lab: HB)<br>
 +
 
 +
<b>Objective:</b> Run a PCR testing VF2/Suffix and Prefix/VR.  A colony PCR of lumazine and mms6 in pET28a.  A PCR of 15 ligation tests. <br>
 +
(In Lab: JV)<br>
 +
<b>Objective:</b> Screen for colonies with the correct insert from Aug. 4, 2010 transformations.  <br>
 +
 
 +
<b>Method:</b>  Colony PCR.  Changes - Used pipette tip instead of toothpick.  Put colony in 20(&micro;L) autoclaved Milli-Q water. <br>
 +
 
 +
<u>PCR:</u> Thermocycler set to iGEM Program 4<br> 
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>9.8
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2
 +
<tr><td>dNTPs<td>2
 +
<tr><td>Forward Primer (VF2)<td>2
 +
<tr><td>Reverse Primer (VR)<td>2
 +
<tr><td>Template DNA (Cell Lysate)<td>2
 +
<tr><td>Pfu polymerase<td>0.2
 +
</table><br>
 +
 
 +
Added 18&micro;L Master Mix to each reaction tube.
 +
 
 +
<b>Method:</b>  Control test of primer combinations. <br>
 +
 
 +
Combination 1 - VF2/Suffix
 +
Combination 2 - Prefix/VR
 +
Combination 3 - Prefix/Suffix
 +
dT maxiprep used as known template DNA source.
 +
 
 +
<u>PCR Combination 1:</u><br> 
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>9.8
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2
 +
<tr><td>dNTPs<td>2
 +
<tr><td>Forward Primer (Prefix)<td>2
 +
<tr><td>Reverse Primer (Suffix)<td>2
 +
<tr><td>Template DNA (dT)<td>2
 +
<tr><td>Pfu polymerase<td>0.2
 +
</table><br>
 +
 
 +
<u>PCR Combination 2:</u><br> 
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>9.8
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2
 +
<tr><td>dNTPs<td>2
 +
<tr><td>Forward Primer (Prefix)<td>2
 +
<tr><td>Reverse Primer (VR)<td>2
 +
<tr><td>Template DNA (dT)<td>2
 +
<tr><td>Pfu polymerase<td>0.2
 +
</table><br>
 +
 
 +
<u>PCR Combination 3:</u><br> 
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>9.8
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2
 +
<tr><td>dNTPs<td>2
 +
<tr><td>Forward Primer (VF2)<td>2
 +
<tr><td>Reverse Primer (suffix)<td>2
 +
<tr><td>Template DNA (dT)<td>2
 +
<tr><td>Pfu polymerase<td>0.2
 +
</table><br>
 +
 
 +
<b>Method:</b>  PCR of 15 ligation tests. <br>
 +
 
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x19.5)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>9.8<td>191.1
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2<td>39
 +
<tr><td>dNTPs<td>2<td>39
 +
<tr><td>Forward VF2 Primer<td>2<td>39
 +
<tr><td>Reverse VR Primer<td>2<td>39
 +
<tr><td>Template DNA<td>2<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>3.9
 +
</table><br>
 +
 
 +
Added 18(&micro;L) to each tube. 
 +
----
 +
(In Lab: JV)<br>
 +
Analyzed HB's PCR products on 2% TAE gel which ran for 60 minutes at 100 V.<br>
 +
[[image:Lethbridge_100819PCRMania.JPG|200px]]
==<font color="white">Aug 20, 2010==
==<font color="white">Aug 20, 2010==
Line 1,608: Line 1,846:
<b>Results:</b> DNA concentration was good, however there was no evidence of an insert into pET-28(A). <br>
<b>Results:</b> DNA concentration was good, however there was no evidence of an insert into pET-28(A). <br>
-
GEL PICTURE!!!
+
[[image:Lethbridge_100819pET28aTransformScreenGel1.JPG|200px]]<br><br>
 +
[[image:Lethbridge_100819pET28aTransformScreenGel2.JPG|200px]]<br><br>
 +
[[image:Lethbridge_100819pET28aTransformScreenGel3.JPG|200px]]<br><br>
 +
[[image:Lethbridge_100819pET28aTransformScreenGel4.JPG|200px]]<br><br>
==<font color="white">Aug 23, 2010==
==<font color="white">Aug 23, 2010==
Line 1,644: Line 1,885:
</table>
</table>
-
15(&micro;L) added to each rxn tube.
+
15(&micro;L) added to each rxn tube.<br>
-
Incubated at 37<sup>o</sup>C  for 1.5 hours.  
+
Incubated at 37<sup>o</sup>C  for 1.5 hours. <br>
-
GEL PICTURE!
+
[[image:Lethbridge_100823HBMaxipreps.jpg|200px]]
 +
----
 +
(In Lab: AV)<br>
 +
<b>Objective:</b> To PCR amplify pSB1T3, pSB1C3, pSB1A3 and run on 1% agarose gel. <br>
 +
 
 +
<b>Method:</b><br>
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x6.5)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>14.9<td>96.85
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2<td>13
 +
<tr><td>dNTPs<td>1<td>6.5
 +
<tr><td>SB-prep-2 Primer<td>0.7<td>4.55
 +
<tr><td>SB-prep-3p Primer<td>0.7<td>4.55
 +
<tr><td>Template DNA<td>0.5<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>1.3
 +
</table><br>
 +
 
 +
Added 19.5(&micro;L) to each tube. 
 +
Ran on program 6 of thermocycler.
 +
 
 +
<b>Results:</b> Nothing visible on gel, therefore will have to try loading a larger volume of PCR product.<br>
 +
[[image:Lethbridge_100823AVBackbonePCR.jpg|100px]]
 +
 
 +
==<font color="white">Aug 24, 2010==
 +
 
 +
(In Lab: AV)<br>
 +
<b>Objective:</b> To re-run a 1% agarose gel of PCR products from Aug 23, 2010. <br>
 +
<b>Results:</b> Nothing appeared on gel, therefore the PCR was unsuccessful. <br>
 +
 
 +
==<font color="white">Aug 25, 2010==
 +
 
 +
(In Lab: JV)<br>
 +
<b>Objective:</b> Create amounts of pSB1C3. <br>
 +
 
 +
<b>Method:</b><br>
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x6.5)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>14.9<td>96.85
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2<td>13
 +
<tr><td>dNTPs<td>1<td>6.5
 +
<tr><td>SB-prep-2 Primer<td>0.7<td>4.55
 +
<tr><td>SB-prep-3p Primer<td>0.7<td>4.55
 +
<tr><td>Template DNA<td>0.5<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>1.3
 +
</table><br>
 +
 
 +
Added 19.5(&micro;L) to each tube.
 +
 
 +
PCR- Conditions:
 +
1.  95<sup>o</sup>C for 5 min
 +
2.  94<sup>o</sup>C for 30 sec
 +
3.  55<sup>o</sup>C for 30 sec
 +
4.  68<sup>o</sup>C for 4 min
 +
5.  68<sup>o</sup>C for 10 min
 +
6.  4<sup>o</sup>C  infinitely
 +
(36 cycles)
 +
 
 +
==<font color="white">Aug 25, 2010==
 +
(In Lab: FM)<br>
 +
<b>Objective:</b> Gradient PCR of xylE. <br>
 +
 
 +
<b>Method:</b><br>
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x10)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>5.8<td>58
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>1<td>10
 +
<tr><td>dNTPs<td>1<td>10
 +
<tr><td>Standard Prefix or Fusion Prefix Primer<td>0.5<td>5
 +
<tr><td>Standard Suffix or Fusion Suffix Primer<td>0.5<td>5
 +
<tr><td>Template DNA<td>1<td>10
 +
<tr><td>Pfu polymerase<td>0.2<td>2
 +
</table><br>
 +
 
 +
Gradient Temperatures:
 +
58.5<sup>o</sup>C, 60.5<sup>o</sup>C, 62.3<sup>o</sup>C, 64.1<sup>o</sup>C, 65.9<sup>o</sup>C, 67.7<sup>o</sup>C, 69.4<sup>o</sup>C, 71.1<sup>o</sup>C
 +
-----
 +
(In Lab: JS)<br>
 +
<b>Objective:</b> Run a 2% agarose gel of gradient PCR of xylE. <br>
 +
 
 +
[[image:Lethbridge_100826 xylE PCR Fix.jpg|200px]]
 +
 
 +
==<font color="white">Aug 26, 2010==
 +
(In Lab: KG)<br>
 +
<b>Objective:</b> Do PCR from Aug 25, 2010 to compare PCR of part from registry and our pSB1C3. <br>
 +
 
 +
<b>Method:</b><br>
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x2)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>14.9<td>29.8
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2<td>4
 +
<tr><td>dNTPs<td>1<td>2
 +
<tr><td>SB-prep-26 Primer<td>0.7<td>1.4
 +
<tr><td>SB-prep-3P Primer<td>0.7<td>1.4
 +
<tr><td>Template DNA<td>0.5<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>
 +
</table><br>
 +
 
 +
PCR- Conditions:
 +
1.  95<sup>o</sup>C for 5 min
 +
2.  94<sup>o</sup>C for 30 sec
 +
3.  55<sup>o</sup>C for 30 sec
 +
4.  68<sup>o</sup>C for 4 min
 +
5.  68<sup>o</sup>C for 10 min
 +
6.  4<sup>o</sup>C  infinitely
 +
(36 cycles)
 +
 
 +
Ran a 1% agarose gel of gradient PCR of xylE.
 +
Was stained in ethidium bromide for too long.
 +
 
 +
==<font color="white">Aug 31, 2010==
 +
(In Lab: DM)<br>
 +
<b>Objective:</b> Overexpression test of xylE part (BBa_K118021) in DH5alpha cells in m9 minimal media. <br>
 +
<b>Method:</b> [[Team:Lethbridge/Notebook/Protocols|Overexpression]]
 +
 
 +
0.5 M Catechol was made, to allow for the addition of 1(&micro;L) of this stock solution to be added to the samples taken during the overexpression.
 +
Upon addition of catechol, the solutions turned yellow!
 +
1 mL samples were taken for SDS-PAGE analysis. 
 +
Optical density readings at 600 nm and absorbance readings at 375 and 275 nm were recorded for flasks containing either glucose or sucrose.
 +
----
 +
(In Lab: ADS)<br>
 +
<b>Objective:</b> PCR amplify plasmid backbones (pSB1C3, pSB1A3 and pSB1T3). <br>
 +
<b>Method:</b> Use PCR product from Aug 13, 2010 as template DNA.
 +
 
 +
<table border ="3">
 +
<tr><td><b>Component</b><td><b>1X(&micro;L)</b><td><b>Master Mix(x3.5)(&micro;L)</b>
 +
<tr><td>Milli-Q H<sub>2</sub>O<td>14.4<td>52.4
 +
<tr><td>10x Pfu Buffer with MgSO<sub>4</sub><td>2<td>7
 +
<tr><td>dNTPs<td>1<td>3.5
 +
<tr><td>SB-prep-26 Primer<td>0.7<td>2.45
 +
<tr><td>SB-prep-3P Primer<td>0.7<td>2.45
 +
<tr><td>Template DNA<td>1<td>
 +
<tr><td>Pfu polymerase<td>0.2<td>0.7
 +
</table><br>
 +
 
 +
Added 19(&micro:L) to each tube.
 +
Phusion polymerase was used and apparently in the other previously unsuccessful PCRs, instead of Pfu polymerase.   
 +
 
 +
PCR- Conditions:
 +
1.  95<sup>o</sup>C for 5 min
 +
2.  94<sup>o</sup>C for 30 sec
 +
3.  55<sup>o</sup>C for 30 sec
 +
4.  68<sup>o</sup>C for 4 min
 +
5.  68<sup>o</sup>C for 10 min
 +
6.  4<sup>o</sup>C  infinitely
 +
(36 cycles)
 +
 
 +
Analyzed PCR on 1% TAE agarose gel which ran for 60 min at 100 V. 
 +
----
 +
<b>Objective:</b> Obtain new sources of pSB1T3, pSB1C3 and pSB1A3 plasmid backbone.  Backbone from registry used up. <br>
 +
 
 +
<b>Method:</b> pSB1A3 can be obtained from anything team already possesses.  pSB1C3 can be obtained from BBa_J04450 (RFP) in kit.  Don't have tetracycline plates so cannot obtain pSB1T3.  Used competent cell transformation protocol. <br>
 +
 
 +
<b>Method:</b> pSB1A3 can be obtained from anything team already possesses.  pSB1C3 can be obtained from BBa_J04450 (RFP) in kit.  Don't have tetracycline plates so cannot obtain pSB1T3.  Used [[Team:Lethbridge/Notebook/Protocols|Competent Cell Transformation]] protocol.  <br>
 +
 
 +
* changes:
 +
**used 50&micro;L aliquottes of DH5&alpha
 +
**did not pipette up and down once, the cells were just swirled 3 times
 +
**added 500&micro;L SOC media, shoock at 37<sup>0</sup>C for 90 min
 +
**platted 250&micro;L and 150&micro;L<br>
 +
 
 +
<table border ="3">
 +
<td><b>Results</b>
 +
<tr><td>contents<td><b>&250&micro;L</b><td><b>150&micro;L</b>
 +
<tr><td>+ control(pUC19)<td>good<td>good
 +
<tr><td>J04450<td>X (TMTC)<td>X(TMTC)
 +
</table><br>
 +
 
 +
Prepared overnight cultures for minipreps.  Added 5(&micro;L) of 35 mg/mL Chloramphenicl to 5 mL of LB Media.  Inoculated media with cells from single colony picked from transformation plate.  Incubated overnight at  37<sup>o</sup>C with shaking.
 +
<br><br>

Latest revision as of 19:17, 27 October 2010




Feel free to look around our notebook!


Here you can check out the work we have done in the lab, click on a month to take a look!


Contents

August

August 3, 2010

(in Lab: HB, AV, JV)

Objective: To restrict pBAD, sRBS, mRBS, TetR, dT and pTet for the assembly of pBAD-sRBS-TetR-dT-pTet

Method: Used Restriction of Plasmid DNA protocol.

  • A front vector was made made in sRBS ,mRBS, dT plasmids using EcoRI and Xbal enzymes
  • pDNA that was cut out of plasmid for a front vector was pBAD, TetR, dT and pLacI using EcoRI and SpeI enzymes
  • A back vector was made in sRBS and mRBS plasmids with PstI and SpeI
  • pDNA that was cut out of plasmid for a back vector was TeTR and it was restricted with XbaI and PstI
ConstructpDNAbufferEnzymes
pBAD-sRBS/mRBSpBADRedEcoRI and SpeI
pBAD-sRBS/mRBSsRBSOrangeXbaI and EcoRI
pBAD-sRBS/mRBSmRBSOrangeXbaI and EcoRII
sRBS/mRBS-TetRsRBSRedPstI and SpeI
sRBS/mRBS-TetRmRBSRedPstI and SpeI
sRBS/mRBS-TetRTetRTangoXbaI and PstI
TetR-dTTetRRedEcoRI and SpeI
TetR-dTdTOrangeXbaI and EcoRI
dT-pTetdTRedEcoRI and SpeI
dT-pTetpTetOrangeXbaI and EcoRI
pLAcI-sRBS/mRBSpLacIRedEcoRI and SpeI
pLAcI-sRBS/mRBSsRBSOrangeXbaI and EcoRI
pLAcI-sRBS/mRBSmRBSOrangeXbaI and EcoRI
Mms6-PET28(a)PET28(a)OrangeNotI
  • For all reactions
    • 158 (µL) Milli-Q H2O
    • 10 (µL) Buffer
    • 0.5(µL) of each enzyme
    • 10 (µL) pDNA

Restriction was incubated for 1 hour at 37oC


Objective: Run PCR of pBAD, TetR, dT, pLacI, and mms6.
Method: Used PCR thermocycler iGEM program 7

ComponentVolume per tube (µL)Master Mix (x6)
MilliQ H2O41.8250.8
10x Pfu Buffer with MgSO4530
dNTPs16
Forward Primer0.53
Reverse Primer0.53
Template DNA1-
Pfu DNA polymerase0.2-
Total50292.8
  • Added 48.8 µL of Master Mix to each PCR reaction



Objective: Complete maxipreps of Lumazine (K249002), EYFP (E0030), and ECFP (E0020) and run on 1% agarose gel.
Method:

LaneSampleComponents (µL)
11 kb ladder2 loading dye (5x) + 0.5 ladder + 3.5 MilliQ H2O
2ECFP2 DNA + 2 loading dye (5x) + 2 MilliQ H2O
3EYFP2 DNA + 2 loading dye (5x) + 2 MilliQ H2O
4Lumazine2 DNA + 2 loading dye (5x) + 2 MilliQ H2O
  • Ran at 100V for 42 minutes. Stained in EtBr for 15 minutes.

Results: Lethbridge 100803JV Maxiprep.JPG



Objective: Ligate dT into pSB1C3.
Method:

  • PCR amplify and purify both pSB1C3 and dT
  • Restrict both with EcoRI and PstI
  • Restrict pSB1C3 with DpnI
  • Ligate pSB1C3 and dT

Restriction:

RestrictionMilliQ H2O (µL)Buffer Orange (µL)pDNA (µL)Enzyme (µL)
pSB1C379.2510100.25 EcoRI + 0.25 PstI + 0.25 DpnI
pSB1C3 control801010-
dT79.5010100.25 EcoRI + 0.25 PstI
dT control801010-
  • Restriction were incubated at 37oC for 90 minutes.
  • Enzymes were heat killed for 20 minutes at 80oC.

August 3, 2010 Evening

(in lab: KG, JS)

Objective: To run 1.5% agarose of restrictions: pBAD, sRBS, mRBS, TetR, dT and pTet for the assembly of pBAD-sRBS-TetR-dT-pTet

Method: Used a 1.5% agarose gel with 2 (µL) of loading dye and 10 (µL) of pDNA.

LaneContentsResult
11kb ladder
2pTet (XbaI, EcoRI)good
3pTet (orange buffer)---
4dT (XbaI, EcoR)no good
5dT (orange buffer)---
6mRBS (SpeI, PstI) good
7mRBS (red buffer)---
8sRBS (SpeI, PstI) good
9sRBS (red buffer)---
10mRBS (XbaI, EcoRI) good
11mRBS (orange buffer)---
12sRBS (XbaI, EcoRl) good
13sRBS (orange buffer)---
14pet28(a) good
15100 bp ladder
16PSB1C3 not good
17PSB1C3 restriction digest---

LaneContentsResult
1TetR (EcorI, SpeI) good
2TetR (red buffer)---
3pLacI (EcoRI, SpeI) good
4pLacI (red buffer)---
5Mms6can not tell
6Mms6 control---
7TetR (Xbal, PstI) good
8TetR (tango buffer)---
9pBAD (EcoRI, SpeI)good
10pBAD (red buffer)---
11dT (EcoRI, SpeI)good
12dT (red buffer)---
13pLacI (2)?
14dT control not good
15dT restriction
16100 bp ladder
17dT PCR product good
18Mms6 PCR product good
19pBAD PCR product good
20pLacI PCR product good

Lethbridge 100803AS.JPG


Objective: To ligate: pBAD-sRBS/mRBS, sRBS/mRBS-TetR, TetR-dT, dT-pTet, pLacI-sRBS/mRBS, Mms6-ptet28(a), dT-PSB1C3

Method: Ligation of Plasmid DNA
15µL pDNA in plasmid, and 15 µL of pDNA biobrick

August 4, 2010

(in lab: JV)

Objective: PCR analysis of ligation product of August 3, 2010

  • Ligations
    • pBAD-mRBS
    • pBAD-SRBS
    • SRBS-tetR
    • mRBS-TetR
    • dt-pTet
    • mms6-pET-28a
    • dt-pSBIC3
    • pLacI-SRBS
  • Controls
    • pBAD
    • TetR
    • TetR
    • pLacI
    • mms6

Method:
PCR: Thermocycler set to iGEM program 7

Component1X(µL)Master Mix(x16)(µL)
Milli-Q H2O41.8668.6
10x Pfu Buffer with MgSO4580
dNTPs116
Forward Primer0.58
Reverse Primers0.58
Template DNA116
Pfu polymerase0.23.2

2.5% agarose gel(1x TAE)

lanecontentsSuccessful Ligation ?
150bp ladder---
2dt pSBIC3---
3dt pTetx
4dt control---
5sRBS-TetRx
6mRBS-TetR?
7TetR control---
8pLacI-mRBSx
9pLacI-sRBS?
10pLacI control---
11Mms6 pET-28ano band
12Mms6 control---
13pBad-SRBSx
14pBad-mRBSx
15pBad control---
  • Ran at 100V for 70 minutes.

Results:Lethbridge 100804 JV Ligation PCR AS.JPG



Objective: Transform the successful ligations

Method: used Competent Cell Transformation protocol

  • changes:
    • used 50µL aliquottes of DH5&alpha
    • did not pipette up and down once, the cells were just swirled 3 times
    • added 400µL SOC media, shoock at 370C for 90 min
    • platted 250µL and 150µL

Incubated from 12:00AM to 4;00 PM

results
contents&250µL150µL
dt-pTetgoodx
- controlxx
mms6-pET-28agoodgood
dt-pSBIC3xx
mRBS-TetRgoodgood
pLacI-mRBSgoodgood
SRBS-TetRxx
pBAD-SRBSgoodgood
+ contolgoodgood

August 6, 2010

In Lab: JV

Objective: Put lumazine synthase gene and mms6 into pET-28(A) for future overexpression.

Method: Restrict mms6 from Mr. Gene with NotI. Large quantities of DNA can be used so a gel extraction of the part can be done. PCR lumazine synthase out of its backbone. Restrict off the extra DNA fragments from the PCR with NotI. Restrict pET-28A with notI. Ligate.

Restriction:

RestrictionMilliQ H2O (µL)Buffer Orange (µL)pDNA (µL)Enzyme (µL)
mms6799.51001001 NotI

PCR:

Component1X(µL)
Milli-Q H2O41.85
10x Pfu Buffer with MgSO45
dNTPs1
Forward Primer (VF2)0.5
Reverse Primers (VR)0.5
Template DNA (Lumazine Synthase)1
Pfu polymerase0.2

2% Agarose Gel for Gel Extraction of mms6:

lanesampleloaded
1mms6 restricted with NotI1 mL sample
2mms6 unrestricted control10(µL) sample, 2(µL)dye
350bp ladder2(µL) ladder, 2(µL) dye, 8(µL) H20
31 kb ladder2(µL) ladder, 2(µL) dye, 8(µL) H20

Gel ran for 60 minutes at 100 V. Small & faint band was slightly visible. Gel extraction was carried out using QIAGEN method. Eluted to 12 (µL).
Lethbridge 100809 JV Mms6 Gel Extract BW.jpg

August 6, 2010 Evening

Objective: Attempt colony pcr for rapid screening

Method: Followed two protocols from openwet

  • Knight Protocol
    • place 20(µL) sterile H2O in 0.6mL sterile tube
    • with P10 pipette set to 3(µL) dip tip into colony
    • place pipette tip into water and pipette up and down 20 times(this can be stored at 40C for inoculation of overnight 5mL cultures)
  • Endy Protocol
    • place 50(µL) sterile H2O in 0.6mL sterile tube
    • with PLO pipette (set 3(µL)) dip sterile tip into colony
    • place pipette tip into water and pipette up and down 20 times
Knight cont'dEndy cont'd
setup 20(µL) reactionsetup 20(µL) reaction
1(µL) colony suspension2(µL) colony suspension
2(µL) 10x p.fu (+Mg SO42(µL) 10x p.fu (+Mg SO4
2(µL) dNTP2(µL) dNTP
1.25(µL)VF2 Primer (10(µM)0.75(µL)VF2 Primer (10(µM)
1.25(µL)VF Primer (10(µM)0.75(µL)VF Primer (10(µM)
0.2(µL) Pfu polymerase0.2(µL) Pfu polymerase
11.8 Milli-Q H2O12.6 Milli-Q H2O

  • as control for each rxn used equal volume of mRBS maxiprep
Knight cont'dEndy cont'd
cycling conditionscycling conditions
950C for 15 minutes950C for 6 minutes
*940C for 30 seconds**950C for 30 seconds
*560C for 30 seconds**560C for 30 seconds
*680C for 1 minutes**700C for 1 minutes
680C for 20 minutes700C for 10 minutes

(*) were run 39 times
(**) were run 35 times

Made the following program (called COLONYY) Lid preheat 980C

  • 980C for 15 minutes
  • 980C for 30 seconds
  • 560C for 30 seconds
  • 68-700C gradient for 1 minute
  • 68-700C gradient for 20 minute
  • 40C indefinte

bold selections were cycled 39 times

Objective: Analyzed PCR products on 2.5% TAE Agarose gel.

lanesampleloaded
150bp ladder1(µL) ladder, 1(µL) dye, 4(µL) H20
2Knight control5(µL) sample, 1(µL)dye
3Knight colony5(µL) sample, 1(µL)dye
4Endy control5(µL) sample, 1(µL)dye
5Endy colony5(µL) sample, 1(µL)dye
650bp ladder1(µL) ladder, 1(µL) dye, 4(µL) H20
7lumazine(justin's)5(µL) sample, 1(µL)dye

Lethbridge 100806ADSPCR.JPG

Repeat gel with template controls

lanesampleloaded
150bp ladder0.5(µL) ladder, 2(µL) dye, 9.5(µL) H20
2Endy Template5(µL) colony suspension, 1(µL)dye, 4(µL) H20
3Endy mRBS Control (PLR)5(µL) sample, 1(µL)dye
4Endy mRBS-TetR colony(PCR)5(µL) sample, 1(µL)dye
4mRBS template0.5(µL) sample, 1(µL)dye, 4(µL) H20
5Knight Template0.25(µL) colony suspension, 1(µL)dye, 4(µL) H20
6Knight mRBS control5(µL) ladder, 1(µL) dye
7Knight-mRBS-TetR colony5(µL) sample, 1(µL)dye
11Kb ladder0.5(µL) ladder, 2(µL) dye, 9.5(µL) H20

Lethbridge 100809AS-PCR.jpg

  • ran at 100V for 75 minutes

Aug 9, 2010

(In Lab: HB)

Objective: Run PCR of mRBS-xylE I1 and I2 and lumazine.

Method:
PCR: Thermocycler set to iGEM program 7

Component1X(µL)Master Mix(x4)(µL)
Milli-Q H2O41.8167.2
10x Pfu Buffer with MgSO4520
dNTPs14
Forward Primer (VF2)0.52
Reverse Primers (VR)0.52
Template DNA1
Pfu polymerase0.2

Added 48.8µL Master Mix to each reaction tube.

Objective: Run 2% agarose gel to confirm PCR of mRBS-xylE I1 and I2 and lumazine worked.

lanesampleloaded
150bp ladder0.5(µL) ladder, 1(µL) dye, 6.5(µL) H20
2mRBS-xylE I15(µL) sample, 2(µL)dye
3mRBS-xylE I25(µL) sample, 2(µL)dye
4Lumazine5(µL) sample, 2(µL)dye

Ran at 100 V for 45 minutes. mRBS-xylE did not amplify while lumazine did amplify.

Results: Ligation of mRBS-xylE NOT confirmed
Lethbridge 100809 HB xylE Lum PCR BW.jpg



(In Lab: AV)

Objective: Prepared glycerol stocks & Miniprepped the following using the Qiagen Protocol.

pLacI-mRBS Colony 1
pLacI-mRBS Colony 2
pLacI-sRBS Colony 2
pLacI-sRBS Colony 3
pBAD-mRBS Colony 1
pBAD-mRBS Colony 2
pBAD-sRBS Colony 1
pBAD-sRBS Colony 2
dT-pTet Colony 1
dT-pTet Colony 3
mRBS-TetR Colony 1
mRBS-TetR Colony 3


Objective: To determine which of the previous ligations worked.

Method: Restricted with single cutter and double cutter.


Restriction Reaction (SINGLE)

IngredientVolume(µL)
MilliQ H20 Water15.75
Orange Buffer (10x)2
pDNA2
EcoRI0.25


Restriction Reaction (DOUBLE)

IngredientVolume(µL)
MilliQ H20 Water15.50
Orange Buffer (10x)2
pDNA2
EcoRI0.25
PstI0.25


Unrestricted Control

IngredientVolume(µL)
MilliQ H20 Water16
Orange Buffer (10x)2
pDNA 2

DNA was restricted for 1 hour at 37oC.

Analyzed results on a 2% agarose gel with 2 (µL) of loading dye and 10 (µL) of pDNA. Load order as follows:

LaneContents
11kb ladder
250 bp ladder
3dT-pTet 1 DRD
4dT-pTet 1 SRD
5dT-pTet 1 URD
6dT-pTet 3 DRD
7dT-pTet 3 SRD
8dT-pTet 3 URD
9pLacI-mRBS 1 DRD
10pLacI-mRBS 1 SRD
11pLacI-mRBS 1 URD
12pLacI-mRBS 2 DRD
13pLacI-mRBS 2 SRD
14pLacI-mRBS 2 URD
15pLacI-sRBS 1 DRD
16pLacI-sRBS 1 SRD
17pLacI-sRBS 1 URD
18pLacI-sRBS 3 DRD
19pLacI-sRBS 3 SRD
20pLacI-sRBS 3 URD

Lethbridge 100809AVKG Top.jpg

LaneContents
11 kb ladder
250 bp ladder
3pBAD-mRBS 1 DRD
4pBAD-mRBS 1 SRD
5pBAD-mRBS 1 URD
6pBAD-mRBS 2 DRD
7pBAD-mRBS 2 SRD
8pBAD-mRBS 2 URD
9pBAD-sRBS 1 DRD
10pBAD-sRBS 1 SRD
11pBAD-sRBS 1 URD
12pBAD-sRBS 2DRD
13pBAD-sRBS 2 SRD
14pBAD-sRBS 2 URD
15mRBS-TetR 1 DRD
16mRBS-TetR 1 SRD
17mRBS-TetR 1 URD
18mRBS-TetR 3 DRD
19mRBS-TetR 3 SRD
20mRBS-TetR 3 URD

Lethbridge 100809AVKG Bottom.jpg


Aug 9,2010 Evening

(In Lab: JV, AS)

Objective: To ligate: lumazine into vector upstream of dT. Lumazine and mms6 into pET28a.

Method:

Restrictions

  • Restrict Lumazine wit EcoRI and SpeI (Red Buffer)
  • Restrict the dT with XbaI and EcoRI (Orange Buffer)
  • Restrict Lumazine Synthase with NotI (Red Buffer)

Set up reactions as follows:

ComponentVolume (µL)
MilliQ H2O15.6 or 15.8
Buffer2
pDNA2
Enzyme0.20 + 0.20

Incubated reactions for 60 minutes at 37oC

Ligation
Reaction set up as follows:

  • T4 DNA ligase - 0.25µL
  • DNA 1 - 8µL
  • DNA 2 - 8µL
  • 10x Ligation Buffer - 2µL
  • MilliQ H2O - 1.75µL

Incubated reactions overnight at room temperature.

Aug 10, 2010

(In Lab: JV)

Objective: Reran large gel from Aug 9/2010.

Load order was as follows:

LaneContents
150 bp ladder
2pBAD-mRBS 2 URD
3pBAD-mRBS 2 SRD
4pBAD-mRBS 2 DRD
5pLacI-sRBS 3 URD
6pLacI-sRBS 3 SRD
7pLacI-sRBS 3 DRD
8pLacI-mRBS 2 URD
9pLacI-mRBS 2 SRD
10pLacI-mRBS 1 DRD
11dT-pTet 3 URD
12dT-pTet 3 SRD
13dT-pTet 3 DRD
14pBAD-mRBS 1 URD
15pBAD-mRBS 1 SRD
16pBAD-mRBS 1 DRD
17pLacI-sRBS 2 URD
18pLacI-sRBS 2 SRD
19pLacI-sRBS 2 DRD
201 kb ladder

LaneContents
150 bp ladder
2pLacI-mRBS 1 URD
3pLacI-mRBS 1 SRD
4pLacI-mRBS 1 DRD
5dT-pTet 1 URD
6dT-pTet 1 SRD
7dT-pTet 1 DRD
8mRBS-TetR 3 URD
9mRBS-TetR 3 SRD
10mRBS-TetR 3 DRD
11mRBS-TetR 1 URD
12mRBS-TetR 1 SRD
13mRBS-TetR 1 DRD
14pBAD-sRBS 2 URD
15pBAD-sRBS 2 SRD
16pBAD-sRBS 2 DRD
17pBAD-sRBS 1 URD
18pBAD-sRBS 1 SRD
19pBAD-sRBS 1 DRD
201 kb ladder

Lethbridge 100810ReRunRestrictionDigers.JPG


(In Lab: JV)

Objective: Determine which ligations/transformations worked from 08/04/10.

Method: Colony PCR.

A: dT-pTet (1-10) B: pBAD-sRBS (1-10) C: pLacI-sRBS (1-10) D: pBAD-mRBS (1-10) E: mRBS-TetR (1-10) F: pLacI-mRBS (1-10)

Pick colony with pipette set at 3(µL) Pipette colony up and dow in 20(µL) sterile Milli-Q water. Will use 96 well plate.

PCR- Conditions: 1. 95oC for 15 min 2. 98oC for 20 sec 3. 55oC for 40 sec 4. 72oC for 2 min 5. 72oC for 20 min 6. 4oC infinitely

Reaction Mixture -

Method:
PCR: Thermocycler set to iGEM program 7

Component1X(µL)Master Mix(x65)(µL)
Milli-Q H2O10.9708.5
5X Phusion HF Buffer4260
dNTPs165
Forward Primer (VF2)165
Reverse Primers (VR)165
Colony Template2
Phusion polymerase0.1711.05

Controls: sRBS, pTET & mRBS - will PCR these to compare size using same conditions as above.
Lethbridge 100810MassiveColonyPCR JV AS.JPG
Lethbridge 100810MassiveColonyPCR Large Gel JV AS.JPG

Aug 10, 2010 Evening

(In Lab: ADS)

Objective: PCR amplify xylE from mRBS-xylE for creation of xylE BioBrick

Method: 20µL reactions

PCR- Conditions: 1. Initial Denaturation 98oC for 30 sec 2. Denaturation 98oC for 10 sec 3. Anneal (51oC, 55oC,59.8oC, 64.6oC, 69.1oC, 71oC) for 30 sec 4. Extend 72oC for 30 sec 5. Final Extend 72oC for 10 min 6. Held 4oC for 30 hours

6 tubes in gradient PCR.

Component1X(µL)Master Mix(x6.5)(µL)
Milli-Q H2O8.857.2
5X Phusion HF Buffer426
dNTPs213
Forward Primer 213
Reverse Primer213
Template DNA16.5
Polymerase0.21.3

Ran samples on 1.5% agarose gel (1X TAE) for 60 minutes at 100V.

Results:
Lethbridge 100810xylE PCR AS.JPG

Aug 11, 2010

(In Lab: AS, JV, TF)

Objective: Determine what transformations have the correct insert from Aug. 4, 2010.
Method: Colony PCR. Changes - Used pipette tip instead of toothpick.
PCR: Thermocycler set to iGEM PFUTEST

1. pLacI-mRBS: 4 (A - E) 50(µL) 2. pBAD-mRBS: 5 (A - E) 20(µL) 3. mRBS-TetR: 6 (A -E) 20(µL) Controls - mRBS

Component1X(µL)Master Mix(x7.5)(µL)
Milli-Q H2O9.873.5
10x Pfu Buffer with MgSO4215
dNTPs215
Forward Primer (VF2)215
Reverse Primer (VR)215
Template DNA2
Pfu polymerase0.21.5

Added 18µL Master Mix to each reaction tube.


(In Lab: ADS)

Objective: Transform mRBS-xylE BioBrick into DH5alpha.

Transformation -

A) Thawed 50(µL) Sub-Cloning Efficiency DH5alpha Competent Cells on ice. B) Gently mixed cells and then aliquoted 100(µL) into chilled polypropylene tubes. C) Added 2(µL) of BioBrick to cells. Added 5(µL) of pUC19 DNA to 100(µL) cells to determine efficiency. D) Incubated cells on ice for 30 minutes. E) Heat shocked cells for 45 seconds in a 42oC water bath. F) Placed on ice for 5 minutes. G) Added 0.4 mL of room temperature SOC medium. H) Shook at 225 rpm for 1 hour. I) Diluted control cells 1:100 with SOC medium. J) Spread 100(µL) of this dilution on LB-Amp agar plates K) Spread 50 and 250(µL) of experimental cells on LB-Cam agar plates. L) Incubated overnight at 37oC

Aug 12, 2010

(In Lab: JV)

Objective: Determine if Adam's colony PCRs' from Aug. 11, 2010 worked.
Method: Samples were run on a 2.5% agarose gel (1X TAE) for 1 hour at 100V.

GEL PICTURE!

Results: Lanes 2, 3, 4 and 8 showed PCR amplification. Colonies chosen don't show the correct insert size.
Lethbridge 100812 JV AS Colony PCR Pfu.JPG


(In Lab: JV)
Objective: Screen for colonies with the correct insert from Aug. 4, 2010 transformations.

Method: Colony PCR. Changes - Used pipette tip instead of toothpick. Put colony in 20(µL) autoclaved Milli-Q water.
PCR: Thermocycler set to iGEM PFUTEST

1. pLacI-sRBS: A (11 - 17) 2. pBAD-sRBS: B (11 - 17) 3. dT-pTet: C (11 - 17) 4. pLacI-mRBS: D (11-17) 5. pBAD-mRBS: E (11-17) 6. mRBS-TetR: F (11-17)

Controls - mRBS, pTet, sRBS

Component1X(µL)Master Mix(x47)(µL)
Milli-Q H2O9.8460.6
10x Pfu Buffer with MgSO4294
dNTPs294
Forward Primer (VF2)294
Reverse Primer (VR)294
Template DNA (Cell Lysate)294
Pfu polymerase0.29.4

Added 18µL Master Mix to each reaction tube.
Analyzed PCR products on 2.5% TAE gel.
Results:
Lethbridge 100812ASJVMassColonyPCRLargeGel (1).JPG

Lethbridge 100812ASJVMassColonyPCRSmallGel.JPG


(In Lab: ADS, KG)
Objective: Perform PCR on lumazine, mms6, xylE plasmids with prefix and suffix primers (these will tell us exact size without subtracting VF2/VR regions). If right will ligate into pET28a plasmids.

Method: Plasmids used included: 6 mms6 maxipreps. 4 lumazine maxipreps. 5 xylE maxipreps. 1 mRBS maxiprep
PCR: Thermocycler set to iGEM Program #11 PFU - P/S

PCR- Conditions: 1. Initial Denaturation 95oC for 3 min 2. Denaturation 95oC for 30 sec 3. Anneal (54oC) for 30 sec 4. Extend 72oC for 3 min 5. Final Extend 72oC for 15 min 6. Held 4oC infinitely (25 cycles)

Component1X(µL)Master Mix(x16.5)(µL)
Milli-Q H2O9.8161.7
10x Pfu Buffer with MgSO4233
dNTPs233
Forward Primer (Prefix)233
Reverse Primer (Suffix Antisense)233
Template DNA (Cell Lysate)2
Pfu polymerase0.23.3

Added 18µL Master Mix to each reaction tube.
Analyzed PCR products on 2.5% TAE gel run at 100 V for 35 minutes.
Lethbridge 100813ADS Awesome PCR.JPG

Aug 13, 2010

(In Lab: AS)

Objective: PCR amplify minipreps prepared on Aug 9/2010 to screen for properly assembled BioBricks.


Component1X(µL)Master Mix(x12.5)(µL)
Milli-Q H2O41.85523.1
10x Pfu Buffer with MgSO4562.5
dNTPs112.5
Forward Primer (VF2)0.56.25
Reverse Primer (VR)0.56.25
Template DNA1
Pfu polymerase0.151.888

Added 49µL Master Mix to each reaction tube.



(In Lab: AS)

Objective: PCR amplify pSB1A3, pSB1T3 and pSB1C3 for use in future 3 part assembly and subsequent growth for glycerol stock.

Component1X(µL)Master Mix(x13.5)(µL)
Milli-Q H2O14.952.15
10x Pfu Buffer with MgSO427
dNTPs13.5
Forward Primer (SB-prep-2)0.72.45
Reverse Primer (SB-prep-3p)0.72.45
Template DNA0.5
Pfu polymerase0.20.7

PCR- Conditions: 1. 94oC for 30 sec 2. 94oC for 30 sec 3. 55oC for 30 sec 4. 68oC for 3 min 5. 68oC for 10 min 6. 4oC infinitely (36 cycles)

Added 19.5µL Master Mix to each reaction tube.
Analyzed products on 1% TAE agarose gel which ran for 60 minutes at 100 V.

Results:
Lethbridge 100814PlasmidBackbones.JPG

Aug 14, 2010

(In Lab: AS)

2.5% agarose gel(1x TAE)

lanecontents
1pBAD-mRBS 1
2pBAD-mRBS 2
3pBAD-sRBS 1
4pBAD-sRBS 2
5mRBS-TetR 1
6mRBS-TetR 3
750 bp Ladder
8dT-pTet 1
9dT-pTet 3
10pLacI-mRBS 1
11pLacI-mRBS 2
12pLacI-sRBS 2
13pLacI-sRBS 3
14MT
15MT
16MT
17MT
18MT
19MT
20MT
lanecontents
1K249001
2K249004
3K249005
4K249006
5MT
6K249008
7K249008 (Qiagen)
8K249014
9K249017
1050 bp Ladder
111
122
133
144
155
16xylE-dT
17Lumazine-dT
18pLacI-sRBS
19MT
20MT
21MT
22MT
23MT
24MT
25MT
26MT
27MT

Lethbridge 100815MiniprepPCR.JPG


(In Lab: AS)

Objective: Insert mms6 and lumazine into pET28a using NotI restriction site.

Method: 1. Reserve 1(µL) of dirty PCR product for analysis. 2. Clean up PCR products using Qiagen prep. 3. Restrict 4 mms6 maxipreps and 4 lumazine maxipreps.

Restriction Reactions:

For lumazine and mms6 -

Ingredient1X(µL)Master Mix(x8.5)(µL)
MilliQ H20 Water7.866.30
Orange Buffer (10x)217
pDNA10
NotI0.21.7

Added 10 (µL) to each tube.

For pET28a -

IngredientReaction Mix(µL)
MilliQ H20 Water4.8
Orange Buffer (10x)5
pDNA40
NotI0.2

Incubated at 37oC. Analyzed results on 2.5% TAE agarose gel which ran at 100 V for 50 minutes.
Lethbridge 100814ColonyPCRRetryandStartofassembly.JPG

Results: Lost all the DNA in the column clean-up step and will have to re-do.

Aug 14, 2010 Evening

(In Lab: AS)

Objective: Assemble mms6-dT and lumazine-dT using three antibiotic assembly.

Method:

  1. PCR amplify BioBricks (Prefix/Suffix)
  2. Restrict BioBricks
  3. Ligate BioBricks into psB1C3
  4. Confirm ligation by PCR analysis (VF2/VR)
  5. Transform ligation mixes
  6. Screen colonies with Colony PCR

PCR: Thermocycler set to iGEM program 11

Component1X(µL)Master Mix(x10.5)(µL)
Milli-Q H2O10.8113.4
10x Pfu Buffer with MgSO4221
dNTPs221
Forward Primer (Prefix)221
Reverse Primers (Suffix Antisense)221
Template DNA1
Pfu polymerase0.22.1

Added 19 (µL) to each tube.

Restriction Reactions:

For lumazine and mms6 -

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water11.663.8
Red Buffer (10x)211
pDNA6
EcoRI0.21.1
SpeI0.21.1

Added 14 (µL) to each tube.

For dT -

IngredientReaction Mix(µL)
MilliQ H20 Water58
Tango Buffer (10x)10
pDNA30
XbaI1
PstI1

For pSB1C3 -

IngredientReaction Mix(µL)
MilliQ H20 Water70
Orange Buffer (10x)10
pDNA30
EcoRI1
PstI1
DpnI1

Also cut lumazine, mms6 and dT with one enzyme for two part, PCR amplification and subsequent ligation into pSB1X3.

For lumazine and mms6, CUT with SpeI -

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water15.886.9
Tango Buffer (10x)211
pDNA2
SpeI0.21.1

Added 18 (µL) to each reaction.

For dT, CUT with XbaI-

IngredientReaction Mix(µL)
MilliQ H20 Water79
Tango Buffer (10x)10
pDNA10
XbaI1

Incubated at 37oC for 1.5 hours. Heat killed enzymes for 20 minutes at 80oC.

Ligation Reactions:

3 Part: Lumazine/mms6 + dT + psB1C3

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water11.064.9
T4 Ligase Buffer (10x)211
Plasmid (psB1C3)211
Part 1 (Lumazine/mms6)2
Part 2 (dT)211
T4 DNA Ligase0.21.1

2 Part: Lumazine/mms6 + dT

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water13.875.9
T4 Ligase Buffer (10x)211
Part 1 (Lumazine/mms6)2
Part 2 (dT)211
T4 DNA Ligase0.21.1

Added 18(µL) to each rxn tube. Incubated 1 hour and overnight at room temperature ( 25oC).


Screening via PCR amplification : Thermocycler set to iGEM program 11
3 Part: Lum/mms6 + dT + pSB1C3

Component1X(µL)Master Mix(x5.5)(µL)
Milli-Q H2O33.8185.9
10x Pfu Buffer with MgSO4527.5
dNTPs211
VF2 Primer211
VR Primer211
Template DNA5
Pfu polymerase0.21.1

Added 45 (µL) MM to each tube.

2 Part: Lum/mms6 + dT

Component1X(µL)Master Mix(x5.5)(µL)
Milli-Q H2O6.837.4
10x Pfu Buffer with MgSO4211
dNTPs211
Prefix Primer211
Suffix Antisense Primer211
Template DNA5
Pfu polymerase0.21.1

Added 15 (µL) MM to each tube.
Results:

Aug 15, 2010

(In Lab: ADS)

Objective: Insert mms6 and lumazine into pET28a using NotI restriction site.

Method: 1. Reserve 1(µL) of dirty PCR product for analysis. 2. Clean up PCR products using Qiagen prep. 3. Restrict 3 mms6 maxipreps and 2 lumazine maxipreps.

Restriction Reactions:

For lumazine and mms6 -

Ingredient1X(µL)Master Mix(x10.5)(µL)
MilliQ H20 Water11.8123.9
Orange Buffer (10x)221
pDNA6
NotI0.22.1

Added 14 (µL) to each tube.

For pET28a -

IngredientReaction Mix(µL)
MilliQ H20 Water4.8
Orange Buffer (10x)5
pDNA40
NotI0.2

Incubated at 37oC for 1.5 hours. Heat killed enzymes at 80oC for 20 minutes.

Ligation Reactions:

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water13.975.9
T4 Ligase Buffer (10x)211
Plasmid (pET28a)211
Cut out part (Lumazine/mms6)2
T4 DNA Ligase0.21.1

Added 18(µL) to each tube. Incubated 1 hour and overnight at room temperature.

Aug 15, 2010 Evening

(In Lab: AS)

Objective: Assemble Lum-dT & mms6-dT using BioBrick standard assembly.

Method: Obtain plasmid DNA from maxipreps.

Restriction Reactions:

For lumazine and mms6 -

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water7.641.8
Red Buffer (10x)211
pDNA10
EcoRI0.21.1
SpeI0.21.1

For dT -

IngredientReaction Mix(µL)
MilliQ H20 Water38
Orange Buffer (10x)10
pDNA50
XbaI1
EcoRI1

Incubated at 37oC for 1.5 hours. Heat killed enzymes for 20 minutes at 80oC.

Ligation Reactions:

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water13.875.9
T4 Ligase Buffer (10x)211
Plasmid (dT)211
Cut out part (Lumazine/mms6)2
T4 DNA Ligase0.21.1

Added 18(µL) MM to each rxn tube. Incubated at one hour and overnight at room temperature.

Screening via PCR amplification : Thermocycler set to iGEM program 11

Component1X(µL)Master Mix(x5.5)(µL)
Milli-Q H2O36.8185.9
10x Pfu Buffer with MgSO4527.5
dNTPs211
VF2 Primer211
VR Primer211
Template DNA2
Pfu polymerase0.21.1

Added 45 (µL) MM to each tube.

Analyzed PCR products of BioBrick standard assembly; 3 part (or 3 antibiotic) assembly; and 3 part (3AB) Intermediate/2 part assembly on a 2% TAE agarose gel.
Results:
Lethbridge 100815PCRAssembly.JPG



(In Lab: ADS)

Objective: Produce large quantities of pSB1A3, pSB1C3 and pSB1T3.

Method:

Component1X(µL)Master Mix(x3.2)(µL)
Milli-Q H2O75240
10x Pfu Buffer with MgSO41032
dNTPs516
Primer (SB-prep-2Ea)3.511.2
Primer (SB-prep-3P)3.511.2
Template DNA2
Pfu polymerase13.2

Added 98(µL) to each tube. Used PLASRB PCR Protocol from Aug. 13, 2010.

Aug 16, 2010

(In Lab: KG)

Objective: Confirm overnight ligations done on August 15, 2010.

Method:

Screening via PCR amplification : Thermocycler set to iGEM program 4

Component1X(µL)
Milli-Q H2O33.8
10x Pfu Buffer with MgSO45
dNTPs2
VF2 Primer2
VR Primer2
Template DNA5
Pfu polymerase0.2

3AB Master Mix

ComponentMaster Mix(x5.5)(µL)
Milli-Q H2O185.9
10x Pfu Buffer with MgSO427.5
dNTPs11
Prefix Primer11
Suffix Primer11
Template DNA2
Pfu polymerase1.1

BBS/pSB1C3 Master Mix

ComponentMaster Mix(x11)(µL)
Milli-Q H2O371.8
10x Pfu Buffer with MgSO455
dNTPs22
VF2 Primer22
VR Primer22
Template DNA
Pfu polymerase2.2

Analyzed PCR products of overnight BioBrick standard assembly; 3 part (or 3 antibiotic) assembly; and 3 part (3AB) Intermediate/2 part assembly on a 2% TAE agarose gel.
Results:
Lethbridge 100816PostLigationPCRScreen.JPG

Aug 16, 2010 Evening

(In Lab: KG, AS)

Objective: Restriction of PCR Products (mms6-dT, lumazine-dT). Restriction is necessary for ligation into plasmid backbone pSB1C3

Method:

Restriction Reactions:

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water7.641.8
Orange Buffer (10x)211
pDNA10
PstI0.21.1
SpeI0.21.1

Incubated at 37oC for 1.5 hours. Heat killed enzymes for 2 minutes at 80oC.

Ligation Reactions:

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water13.875.9
T4 Ligase Buffer (10x)211
Plasmid Backbone (pSB1C3)211
pDNA2
T4 DNA Ligase0.21.1

(In Lab: KG)

Objective: Transformations of insertions of mms6 or lumazine into pET28a.

Method: used Competent Cell Transformation protocol

  • changes:
    • used 50µL aliquottes of DH5&alpha
    • did not pipette up and down once, the cells were just swirled 3 times
    • added 400µL SOC media, shoock at 370C for 90 min
    • platted 250µL and 150µL
results
contents&250µL150µL
+ control(pUC19)goodgood
mms6goodgood
mms6-2goodgood
mms6goodx
Lumazinegoodx
Lumazinegoodx

Aug 17, 2010

(In Lab: JV)

Objective: Confirm ligations done on August 16, 2010.

Method:
Screening via PCR amplification : Thermocycler set to iGEM program 4

Component1X(µL)Master Mix(x5.5)(µL)
Milli-Q H2O12.870.4
10x Pfu Buffer with MgSO4211
dNTPs15.5
VF2 Primer15.5
VR Primer15.5
Template DNA2
Pfu polymerase0.21.1

Ran a 2% Agarose gel in 1X TAE buffer for 65 minutes at 100V.
Lethbridge 100817PostLigationPCRTest.JPG

Aug 17, 2010 Evening

(In Lab: AS)

Objective: Repeat ligation of mms6-dT and lumazine-dT to pSB1C3.
Method: Use already restricted mms6-dT and lumazine-dT. Restrict pSB1C3 PCR product with EcoRI and PstI.

Restriction Reactions:

Ingredient1X(µL)
MilliQ H20 Water28.6
Orange Buffer (10x)6
pDNA (pSB1C3)25
PstI0.2
EcoRI0.2

Incubated at 37oC for 1.5 hours. Heat killed enzymes for 20 minutes at 80oC.

Ligation Reactions:

Ingredient1X(µL)Master Mix(x5.5)(µL)
MilliQ H20 Water13.875.9
T4 Ligase Buffer (10x)211
Part 2 (pSB1C3)211
Part 1 (mms6-dT/Lum-dT)2
T4 DNA Ligase0.21.1

Added 18(µL) MM to each rxn tube. Incubated overnight at room temperature.


Objective: Ligation confirmation by PCR. 2 different PCR reaction conditions were utilized. Believe PstI is not being heat inactivated.

Method:
PCR 1 - Show complete insertion of mms6-dT, lumazine-dT into pSB1C3. Both EcoRI and PstI ligations occurred.

Component1X(µL)Master Mix(x11)(µL)
Milli-Q H2O33.8371.8
10x Pfu Buffer with MgSO4555
dNTPs222
Forward VF2 Primer222
Reverse VR Primer222
Template DNA5
Pfu polymerase0.22.2

Added 45(µL) MM to each rxn tube.

PCR 2 - Show PstI is not heat killed and only EcoRI ligation occurred.

Component1X(µL)Master Mix(x16)(µL)
Milli-Q H2O33.8540.8
10x Pfu Buffer with MgSO4580
dNTPs232
Forward VF2 Primer232
Reverse VR Primer232
Template DNA5
Pfu polymerase0.23.2

Added 45(µL) MM to each rxn tube.


Objective: Analyze tendency of PstI to be heat killed.
Hypothesis: Ligation will be counteracted by PstI digestion even following 20 minute heat kill at 80oC .
Method: Restrict plasmid DNA with PstI (and EcoRI control). Reactions stopped by heat killing. Plasmids re-ligated with T4 DNA Ligase. Ligation confirmed with PCR. If PCR product is present then enzyme heat killed but if there is no PCR Product then enzyme was not heat killed.

Restriction Reactions:

Ingredient1X(µL)
MilliQ H20 Water12.8
Orange Buffer (10x)2
pDNA (dT)5
PstI0.2
EcoRI (control only)0.2

Incubated at 37oC for 1.5 hours. Heat killed enzymes for 20 minutes at 80oC.

Ligation Reactions:

Ingredient1X(µL)
MilliQ H20 Water15.8
T4 Ligase Buffer (10x)2
Restriction Mix2
T4 DNA Ligase0.2

Incubated at room temperature overnight.

PCR to confirm Ligation

Component1X(µL)Master Mix(x2.2)(µL)
Milli-Q H2O33.874.36
10x Pfu Buffer with MgSO4511
dNTPs24.4
Forward VF2 Primer24.4
Reverse VR Primer24.4
Template DNA5
Pfu polymerase0.20.44

Added 45(µL) to each reaction tube.

Aug 18, 2010

(In Lab: JV)
Objective: Confirmation of ADS' analysis of PstI's tendency to be heat killed.
Method: Will PCR ligation reactions from different assembly methods and EcoRI and PstI controls.

Component1X(µL)
Milli-Q H2O33.8
10x Pfu Buffer with MgSO45
dNTPs2
Forward VF2 Primer2
Reverse VR Primer2
Template DNA5
Pfu polymerase0.2

Ran on cycle 4 of thermocycler.

Viewed PCRs on 2% TAE agarose gel that ran at 110 V for 30 minutes.
Lethbridge 100818AssemblyandHeatKillPCR.JPG


(In Lab: HB)
Objective: Analyze tendency of PstI to be heat killed.
Method: Restrict plasmid DNA with PstI (and EcoRI control). Reactions stopped by heat killing. Plasmids re-ligated with T4 DNA Ligase. Ligation confirmed with PCR. If PCR product is present then enzyme heat killed but if there is no PCR Product then enzyme was not heat killed.

Restriction Reactions:

Ingredient1X(µL)
MilliQ H20 Water12.8
Orange Buffer (10x)2
pDNA (dT)5
PstI0.2
EcoRI (control only)0.2

Incubated at 37oC for 1.5 hours. Heat killed enzymes for 20 minutes at 80oC.

Ligation Reactions:

Ingredient1X(µL)
MilliQ H20 Water15.8
T4 Ligase Buffer (10x)2
Restriction Mix2
T4 DNA Ligase0.2

Incubated at room temperature overnight.

PCR to Confirm Ligation

Component1X(µL)Master Mix(x6.5)(µL)
Milli-Q H2O33.8219.7
10x Pfu Buffer with MgSO4532.5
dNTPs213
Forward VF2 Primer213
Reverse VR Primer213
Template DNA5
Pfu polymerase0.21.3

Added 45(µL) to each reaction tube. Used thermocycler iGEM Program 4.

3 different treatments: 1. Restricted, heat killed and ligated. 2. Restricted and heat killed. 3. Restricted and not heat killed.

Aug 19, 2010

(In Lab: JV)

Objective: Determine if any transformations from Aug 16, 2010 have the correct insert.
Method: Pick colonies and incubate at 37oC in LB Media with Kan overnight. Use QIAGEN method to extract plasmid DNA. Restrict plasmid DNA to determine if mms6 or lumazine has correctly ligated into pET-28(A).

Restriction Reactions:

mms6 RESTRICTED -

Ingredient1X(µL)Master Mix(x31)(µL)
MilliQ H20 Water15.75488.25
Red Buffer (10x)262
Template DNA
Enzyme (EcoRV)0.257.75

mms6 UNRESTRICTED -

Ingredient1X(µL)Master Mix(x31)(µL)
MilliQ H20 Water16496
Red Buffer (10x)262
Template DNA

lumazine RESTRICTED -

Ingredient1X(µL)Master Mix(x31)(µL)
MilliQ H20 Water15.75488.25
Tango Buffer (10x)262
Template DNA
Enzyme (EcoRV).257.75

lumazine UNRESTRICTED -

Ingredient1X(µL)Master Mix(x31)(µL)
MilliQ H20 Water16496
Tango Buffer (10x)262
Template DNA

Added 18(µL) to each restriction digest reaction. Incubated at 37oC for 1.5 hours. Heat killed enzymes for 20 minutes at 80oC.

Samples were run on a 2% agarose gel in 1X TAE Buffer.


(In Lab: HB)

Objective: Run a PCR testing VF2/Suffix and Prefix/VR. A colony PCR of lumazine and mms6 in pET28a. A PCR of 15 ligation tests.
(In Lab: JV)
Objective: Screen for colonies with the correct insert from Aug. 4, 2010 transformations.

Method: Colony PCR. Changes - Used pipette tip instead of toothpick. Put colony in 20(µL) autoclaved Milli-Q water.

PCR: Thermocycler set to iGEM Program 4

Component1X(µL)
Milli-Q H2O9.8
10x Pfu Buffer with MgSO42
dNTPs2
Forward Primer (VF2)2
Reverse Primer (VR)2
Template DNA (Cell Lysate)2
Pfu polymerase0.2

Added 18µL Master Mix to each reaction tube.

Method: Control test of primer combinations.

Combination 1 - VF2/Suffix Combination 2 - Prefix/VR Combination 3 - Prefix/Suffix dT maxiprep used as known template DNA source.

PCR Combination 1:

Component1X(µL)
Milli-Q H2O9.8
10x Pfu Buffer with MgSO42
dNTPs2
Forward Primer (Prefix)2
Reverse Primer (Suffix)2
Template DNA (dT)2
Pfu polymerase0.2

PCR Combination 2:

Component1X(µL)
Milli-Q H2O9.8
10x Pfu Buffer with MgSO42
dNTPs2
Forward Primer (Prefix)2
Reverse Primer (VR)2
Template DNA (dT)2
Pfu polymerase0.2

PCR Combination 3:

Component1X(µL)
Milli-Q H2O9.8
10x Pfu Buffer with MgSO42
dNTPs2
Forward Primer (VF2)2
Reverse Primer (suffix)2
Template DNA (dT)2
Pfu polymerase0.2

Method: PCR of 15 ligation tests.

Component1X(µL)Master Mix(x19.5)(µL)
Milli-Q H2O9.8191.1
10x Pfu Buffer with MgSO4239
dNTPs239
Forward VF2 Primer239
Reverse VR Primer239
Template DNA2
Pfu polymerase0.23.9

Added 18(µL) to each tube.


(In Lab: JV)
Analyzed HB's PCR products on 2% TAE gel which ran for 60 minutes at 100 V.
Lethbridge 100819PCRMania.JPG

Aug 20, 2010

(In Lab: JV)

Objective: Determine if attempts to PCR amplify plasmid backbone were successful.

Method: Ran samples on 1% agarose gel with 1X TAE buffer for 50 minutes at 100 V.

Results: DNA concentration was good, however there was no evidence of an insert into pET-28(A).

Lethbridge 100819pET28aTransformScreenGel1.JPG

Lethbridge 100819pET28aTransformScreenGel2.JPG

Lethbridge 100819pET28aTransformScreenGel3.JPG

Lethbridge 100819pET28aTransformScreenGel4.JPG

Aug 23, 2010

(In Lab: JV)

Objective: Obtained part <partinfo>BBa_K118021</partinfo> and <partinfo>BBa_I716462</partinfo>.

Method: Used competent cell transformation protocol.


(In Lab: HB)

Objective: Restrict 18 maxiprepped parts to quantify DNA.

Method: Restrict all 18 parts and run on a 1% agarose gel with unrestricted parts.

Restriction Reactions:

Restriction Mix -

Ingredient1X(µL)Master Mix(x19)(µL)
MilliQ H20 Water12.8243.2
Orange Buffer (10x)238
Template DNA5
EcoRI0.23.8

Unrestricted Mix -

Ingredient1X(µL)Master Mix(x19)(µL)
MilliQ H20 Water13247
Orange Buffer (10x)238
Template DNA5

15(µL) added to each rxn tube.
Incubated at 37oC for 1.5 hours.

Lethbridge 100823HBMaxipreps.jpg


(In Lab: AV)
Objective: To PCR amplify pSB1T3, pSB1C3, pSB1A3 and run on 1% agarose gel.

Method:

Component1X(µL)Master Mix(x6.5)(µL)
Milli-Q H2O14.996.85
10x Pfu Buffer with MgSO4213
dNTPs16.5
SB-prep-2 Primer0.74.55
SB-prep-3p Primer0.74.55
Template DNA0.5
Pfu polymerase0.21.3

Added 19.5(µL) to each tube. Ran on program 6 of thermocycler.

Results: Nothing visible on gel, therefore will have to try loading a larger volume of PCR product.
Lethbridge 100823AVBackbonePCR.jpg

Aug 24, 2010

(In Lab: AV)
Objective: To re-run a 1% agarose gel of PCR products from Aug 23, 2010.
Results: Nothing appeared on gel, therefore the PCR was unsuccessful.

Aug 25, 2010

(In Lab: JV)
Objective: Create amounts of pSB1C3.

Method:

Component1X(µL)Master Mix(x6.5)(µL)
Milli-Q H2O14.996.85
10x Pfu Buffer with MgSO4213
dNTPs16.5
SB-prep-2 Primer0.74.55
SB-prep-3p Primer0.74.55
Template DNA0.5
Pfu polymerase0.21.3

Added 19.5(µL) to each tube.

PCR- Conditions: 1. 95oC for 5 min 2. 94oC for 30 sec 3. 55oC for 30 sec 4. 68oC for 4 min 5. 68oC for 10 min 6. 4oC infinitely (36 cycles)

Aug 25, 2010

(In Lab: FM)
Objective: Gradient PCR of xylE.

Method:

Component1X(µL)Master Mix(x10)(µL)
Milli-Q H2O5.858
10x Pfu Buffer with MgSO4110
dNTPs110
Standard Prefix or Fusion Prefix Primer0.55
Standard Suffix or Fusion Suffix Primer0.55
Template DNA110
Pfu polymerase0.22

Gradient Temperatures: 58.5oC, 60.5oC, 62.3oC, 64.1oC, 65.9oC, 67.7oC, 69.4oC, 71.1oC


(In Lab: JS)
Objective: Run a 2% agarose gel of gradient PCR of xylE.

Lethbridge 100826 xylE PCR Fix.jpg

Aug 26, 2010

(In Lab: KG)
Objective: Do PCR from Aug 25, 2010 to compare PCR of part from registry and our pSB1C3.

Method:

Component1X(µL)Master Mix(x2)(µL)
Milli-Q H2O14.929.8
10x Pfu Buffer with MgSO424
dNTPs12
SB-prep-26 Primer0.71.4
SB-prep-3P Primer0.71.4
Template DNA0.5
Pfu polymerase0.2

PCR- Conditions: 1. 95oC for 5 min 2. 94oC for 30 sec 3. 55oC for 30 sec 4. 68oC for 4 min 5. 68oC for 10 min 6. 4oC infinitely (36 cycles)

Ran a 1% agarose gel of gradient PCR of xylE. Was stained in ethidium bromide for too long.

Aug 31, 2010

(In Lab: DM)
Objective: Overexpression test of xylE part (BBa_K118021) in DH5alpha cells in m9 minimal media.
Method: Overexpression

0.5 M Catechol was made, to allow for the addition of 1(µL) of this stock solution to be added to the samples taken during the overexpression. Upon addition of catechol, the solutions turned yellow! 1 mL samples were taken for SDS-PAGE analysis. Optical density readings at 600 nm and absorbance readings at 375 and 275 nm were recorded for flasks containing either glucose or sucrose.


(In Lab: ADS)
Objective: PCR amplify plasmid backbones (pSB1C3, pSB1A3 and pSB1T3).
Method: Use PCR product from Aug 13, 2010 as template DNA.

Component1X(µL)Master Mix(x3.5)(µL)
Milli-Q H2O14.452.4
10x Pfu Buffer with MgSO427
dNTPs13.5
SB-prep-26 Primer0.72.45
SB-prep-3P Primer0.72.45
Template DNA1
Pfu polymerase0.20.7

Added 19(&micro:L) to each tube. Phusion polymerase was used and apparently in the other previously unsuccessful PCRs, instead of Pfu polymerase.

PCR- Conditions: 1. 95oC for 5 min 2. 94oC for 30 sec 3. 55oC for 30 sec 4. 68oC for 4 min 5. 68oC for 10 min 6. 4oC infinitely (36 cycles)

Analyzed PCR on 1% TAE agarose gel which ran for 60 min at 100 V.


Objective: Obtain new sources of pSB1T3, pSB1C3 and pSB1A3 plasmid backbone. Backbone from registry used up.

Method: pSB1A3 can be obtained from anything team already possesses. pSB1C3 can be obtained from BBa_J04450 (RFP) in kit. Don't have tetracycline plates so cannot obtain pSB1T3. Used competent cell transformation protocol.

Method: pSB1A3 can be obtained from anything team already possesses. pSB1C3 can be obtained from BBa_J04450 (RFP) in kit. Don't have tetracycline plates so cannot obtain pSB1T3. Used Competent Cell Transformation protocol.

  • changes:
    • used 50µL aliquottes of DH5&alpha
    • did not pipette up and down once, the cells were just swirled 3 times
    • added 500µL SOC media, shoock at 370C for 90 min
    • platted 250µL and 150µL
Results
contents&250µL150µL
+ control(pUC19)goodgood
J04450X (TMTC)X(TMTC)

Prepared overnight cultures for minipreps. Added 5(µL) of 35 mg/mL Chloramphenicl to 5 mL of LB Media. Inoculated media with cells from single colony picked from transformation plate. Incubated overnight at 37oC with shaking.