Difference between revisions of "Team:CSU Fort Collins/NoteBook/JanThroughApr"

Latest revision as of 03:39, 19 October 2016

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January Through April

1/4/16:

Ligated b0034 and c0061

Transformed Ligated mixture

Ran PCR results on a 2% gel

1/5/16:

Digested LuxR with EcoRI and SpeI

Performed Colony PCR on transformation from the 4th

1/11/16:

slr0435 Excision from Synechocystis sp. PCC6803 with PCR using Phusion(size 276 bp).

Ran PCR results on a 2% gel

Digested I0462 and E0030 with EcoRI and SpeI, R0062 and B0015 with EcoRI and XbaI, B0034 with SPeI and PstI, and C0061 with XbaI and PstI.

1/12/16:

Digested slr0435 and resuspended pSB1C3 with EcoRI and PstI

Ligated pSB1C3 and slr0435

Transformed ligation mixture

1/13/16:

Colony PCR performed on slr0435+pSB1C3 transformed colonies

Ran PCR results on 1% gel

Digested I0462 and E0030 with EcoRI and SpeI, R0062 and B0015 with EcoRI and XbaI, B0034 with SPeI and PstI, and C0061 with XbaI and PstI.

Ran on 1% gel

1/21/16:

Digested I0462 and E0030 with EcoRI and SpeI, and C0061 with XbaI and PstI.

Ran on 1% gel

Phosphatase treatment

Use Antarctic Phosphatase with 10x buffer. Need 1uL to treat 1ug of DNA

Add 1uL phosphatase and 5uL 10x buffer to bring total rxn volume to 50uL

Incubate at 37C for 1 hour, and heat inactivate at 70C for 5 minutes

1/25/16:

Overnight ligated R0062 and I0462, B0034 and C0061, B0015 and E0030 at 16 C

1/25/16:

Transformed the overnight ligation mixtures

2/6/16:

PCRed out BBA_J23106 out of glycerol stock 19 using Q5 master mix 19rxns

2/9/16:

Transformed Bba_K325909 from parts kit into DH5a cels

2/11/16:

To confirm that Bba_K325909 are functioning we tried to induce expression using L-arabinose

No luminescence was produced

2/16/16:

Decided to order two gBlocks for quorum portion of the project

3/24/16:

Set up O/N cultures of K1033929, K592009 and E1010 in 5 mL of LB with 5 uL of Cm34 antibiotic

3/29/16:

Ran promoters Sll027, and LrtA in a 1% gel

Sll0027

LrtA

4/6/16:

Ran Cpcg2 on 1% gel

4/12/16:

Prepare pSB1C3 vector for Infusion
gBlocks (Quorum 1 and Quorum 2) have 15 bp homology with each other along with prefix and suffix at the entire block’s ends

Digesting the vector with XbaI will leave 16 bp homology with Quorum 1

Digesting the vector with SpeI will leave 20 bp homology with Quorum 2

Digested c0061 with SPeI and XbaI

Ran on 1% gel

4/12/16:

Reaction: PSB1C3 3.06 uL,Q1 2.5ul,Q2 1.78ul, 5x Infusion Mix 2ul, H20 .66ul

Transformation
Add 1 uL Infusion rxn to 50 uL Stellar Cells

Incubate 30 min on ice, 45 sec at 42C, 2 min on ice

Add 250 uL SOC media

1 hour outgrowth at 37C

Plate 50 uL on LB+Cam plates

37C overnight

4/18/16:

Colony PCR on 5 Qblock transformed colonies

4/19/16:

Ran PCR products from the 18th on a 1% gel

4/20/16:

Quorum Colony PCR Phusion

4/22/16:

Ran the PCR product from the 20th on a 1% gel

May >>

@@ Line 25: / Line 25: @@
 <div class = 'Days'><h5>1/4/16:</h5></div>
-<div class = 'Info'><p>Ligated b0034 and c0061 </p> <p>Transformed Ligated mixture</p>
+<div class = 'Info'><ul><li>Ligated b0034 and c0061 </li> <li>Transformed Ligated mixture</li>
-<p>Ran PCR results on a 2% gel</p>
+<li>Ran PCR results on a 2% gel</li>
+</ul>
 </div>
@@ Line 40: / Line 41: @@
 <div class = 'Days'><h5>1/11/16:</h5></div>
-<div class = 'Info'><p>slr0435 Excision from <i>Synechocystis sp. PCC6803</i> with PCR using Phusion(size 276 bp).</p>
+<div class = 'Info'><ul><li>slr0435 Excision from <i>Synechocystis sp. PCC6803</i> with PCR using Phusion(size 276 bp).</li>
-<p>Ran PCR results on a 2% gel</p>
+<li>Ran PCR results on a 2% gel</li>
 <img src = "https://static.igem.org/mediawiki/2016/e/ec/CSU_gJan152016.png">
-<p>Digested I0462 and  E0030 with EcoRI and  SpeI, R0062 and B0015 with EcoRI and XbaI, B0034 with SPeI and PstI, and C0061 with XbaI and PstI.</p>
+<li>Digested I0462 and  E0030 with EcoRI and  SpeI, R0062 and B0015 with EcoRI and XbaI, B0034 with SPeI and PstI, and C0061 with XbaI and PstI.</li>
+</ul>
 </div>
 <div class = 'Days'><h5>1/12/16:</h5></div>
-<div class = 'Info'><p>Digested slr0435 and resuspended pSB1C3 with EcoRI and PstI</p>
+<div class = 'Info'><ul><li>Digested slr0435 and resuspended pSB1C3 with EcoRI and PstI</li>
-<p>Ligated pSB1C3 and slr0435</p>
+<li>Ligated pSB1C3 and slr0435</li>
-<p>Transformed ligation mixture</p>
+<li>Transformed ligation mixture</li>
+</ul>
 </div>
 <div class = 'Days'><h5>1/13/16:</h5></div>
-<div class = 'Info'><p>Colony PCR performed on slr0435+pSB1C3 transformed colonies</p>
+<div class = 'Info'><ul><li>Colony PCR performed on slr0435+pSB1C3 transformed colonies</li>
-<p>Ran PCR results on 1% gel</p>
+<li>Ran PCR results on 1% gel</li>
 <img src = "https://static.igem.org/mediawiki/2016/c/c0/CSU_gJan16Slr0435.png">
+<li>Digested I0462 and  E0030 with EcoRI and  SpeI, R0062 and B0015 with EcoRI and XbaI, B0034 with SPeI and PstI, and C0061 with XbaI and PstI.</li>
+<li>Ran on 1% gel</li>
+<img src = "https://static.igem.org/mediawiki/2016/d/dd/CSU_g13Dig.png">
+</ul>
 </div>
+<div class = 'Days'><h5>1/21/16:</h5></div>
+<div class = 'Info'><ul><li>Digested I0462 and  E0030 with EcoRI and  SpeI,  and C0061 with XbaI and PstI.</li>
+<li>Ran on 1% gel</li>
+<img src = "https://static.igem.org/mediawiki/2016/e/ea/CSU_Gel12116.png">
+<li>Phosphatase treatment</li>
+<li>Use Antarctic Phosphatase with 10x buffer. Need 1uL to treat 1ug of DNA</li>
+<li>Add 1uL phosphatase and 5uL 10x buffer to bring total rxn volume to 50uL</li>
+<li>Incubate at 37C for 1 hour, and heat inactivate at 70C for 5 minutes</li>
+</ul>
+</div>
+<div class = 'Days'><h5>1/25/16:</h5></div>
+<div class = 'Info'><ul><li>Overnight ligated R0062 and I0462, B0034 and C0061, B0015 and E0030 at 16 C</li>
+</ul>
+</div>
+<div class = 'Days'><h5>1/25/16:</h5></div>
+<div class = 'Info'><ul><li>Transformed the overnight ligation mixtures</li>
+</ul>
+</div>
 <div class = 'Days'><h5>2/6/16:</h5></div>
-<div class = 'Info'><p>PCRed out BBA_J23106 out of glycerol stock 19 using Q5 master mix 19rxns</p>
+<div class = 'Info'><ul><li>PCRed out BBA_J23106 out of glycerol stock 19 using Q5 master mix 19rxns</li>
+</ul>
 </div>
 <div class = 'Days'><h5>2/9/16:</h5></div>
-<div class = 'Info'><p>Transformed Bba_K325909 from parts kit into DH5a cels</p>
+<div class = 'Info'><ul><li>Transformed Bba_K325909 from parts kit into DH5a cels</li>
+</ul>
 </div>
 <div class = 'Days'><h5>2/11/16:</h5></div>
-<div class = 'Info'><p>To confirm that Bba_K325909 are functioning we tried to induce expression using L-arabinose</p>
+<div class = 'Info'><ul><li>To confirm that Bba_K325909 are functioning we tried to induce expression using L-arabinose</li>
-<p>No luminescence was produced</p>
+<li>No luminescence was produced</li>
+</ul>
+</div>
+<div class = 'Days'><h5>2/16/16:</h5></div>
+<div class = 'Info'><ul><li>Decided to order two gBlocks for quorum portion of the project</li>
+</ul>
 </div>
 <div class = 'Days'><h5>3/24/16:</h5></div>
-<div class = 'Info'><p>Set up O/N cultures of K1033929, K592009 and E1010 in 5 mL of LB with 5 uL of Cm34 antibiotic </p>
+<div class = 'Info'><ul><li>Set up O/N cultures of K1033929, K592009 and E1010 in 5 mL of LB with 5 uL of Cm34 antibiotic </li>
+</ul>
 </div>
 <div class = 'Days'><h5>3/29/16:</h5></div>
-<div class = 'Info'><p>Ran promoters Sll027, and LrtA in a 1% gel</p>
+<div class = 'Info'><ul><li>Ran promoters Sll027, and LrtA in a 1% gel</li>
 <h6>Sll0027</h6>
 <img src = "https://static.igem.org/mediawiki/2016/0/0f/CSU_gSll02632416.png">
 <h6>LrtA</h6>
 <img src = "https://static.igem.org/mediawiki/2016/3/33/CSU_gLrta32416.png">
+</ul>
 </div>
 <div class = 'Days'><h5>4/6/16:</h5></div>
-<div class = 'Info'><p>Ran Cpcg2 on 1% gel</p>
+<div class = 'Info'><ul><li>Ran Cpcg2 on 1% gel</li>
 <img src = "https://static.igem.org/mediawiki/2016/f/f1/CSU_Cpcg224616.png">
+</ul>
 </div>
+<div class = 'Days'><h5>4/12/16:</h5></div>
+<div class = 'Info'><h6>Prepare pSB1C3 vector for Infusion</h6><ul><li>gBlocks (Quorum 1 and Quorum 2) have 15 bp homology with each other along with prefix and suffix at the entire block’s ends</li>
+<li>Digesting the vector with XbaI will leave 16 bp homology with Quorum 1</li>
+<li>Digesting the vector with SpeI will leave 20 bp homology with Quorum 2</li>
+<li>Digested c0061 with SPeI and XbaI</li>
+<li>Ran on 1% gel</li>
+<img src = "https://static.igem.org/mediawiki/2016/a/a8/CSU_g41216.png">
+</ul>
+</div>
+<div class = 'Days'><h5>4/12/16:</h5></div>
+<div class = 'Info'><h6></h6><ul><li> Reaction: PSB1C3 3.06 uL,Q1 2.5ul,Q2 1.78ul, 5x Infusion Mix 2ul, H20 .66ul</li>
+<h6>Transformation</h6><li>Add 1 uL Infusion rxn to 50 uL Stellar Cells</li>
+<li>Incubate 30 min on ice, 45 sec at 42C, 2 min on ice</li>
+<li>Add 250 uL SOC media</li>
+<li>1 hour outgrowth at 37C</li>
+<li>Plate 50 uL on LB+Cam plates</li>
+<li>37C overnight</li>
+</ul>
+</div>
+<div class = 'Days'><h5>4/18/16:</h5></div>
+<div class = 'Info'><ul><li>Colony PCR on 5 Qblock transformed colonies</li>
+</ul>
+</div>
+<div class = 'Days'><h5>4/19/16:</h5></div>
+<div class = 'Info'><ul><li>Ran PCR products from the 18th on a 1% gel</li>
+<img src = "https://static.igem.org/mediawiki/2016/f/f3/CSU_gQ41916.png">
+</ul>
+</div>
+<div class = 'Days'><h5>4/20/16:</h5></div>
+<div class = 'Info'><ul><li>Quorum Colony PCR Phusion</li>
+</ul>
+</div>
+<div class = 'Days'><h5>4/22/16:</h5></div>
+<div class = 'Info'><ul><li>Ran the PCR product from the 20th on a 1% gel</li>
+<img src = "https://static.igem.org/mediawiki/2016/b/b7/CSU_gQ42216.png">
+</ul>
+</div>
+<h2 align="right"><a href = "https://2016.igem.org/Team:CSU_Fort_Collins/NoteBook/May">May >></a>
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