Team:Penn/Notebook

From 2012.igem.org

(Difference between revisions)

Revision as of 10:37, 15 September 2012

Penn 2012 iGEM Wiki

June 2012 Notebook

Week 1

June 6th

Set up some lab equipment
Autoclaved for a while
Organized biobrick stuff
Called Vinoo about DNA planning

June 7th

Transformed Cph8, pLsr, and LuxS
Placed order with Vinoo
Developed idea using PGY/PCN system to activate a gene

Week 2

June 11th

Wet Lab

PCR'd mCherry from NAS157
Ran 1% Gel and purified product

Dry Lab

Designed primers for LsR promoter
Meeting with Dr. Sarkar

June 12th

Wet Lab

Digested mCherry PCR product with BamHI and NotI
Column purified mCherry and ligated into NAS152 backbone
Transformed NAS152-mCherry into DH5alpha
Poured 25 LB-Kan plates

Dry Lab

Research more information about bacterial drug delivery system
More research into biofilm project

June 14th

Wet Lab

Fill in later....

Dry Lab

Met with Dr. Goulian, obtained pDawn and pDusk
Identified inaK as a surface display gene we can use

Week 3

June 18th

Wet Lab

Miniprep pDawn and pDusk
Test cut pDawn and pDusk with XmaI, analytical gel was correct
Prep cut pDawn and pDusk with BamHI and NotI, gel purified

Dry Lab

Ordered and picked up PCR purification kit from cell center
Additional orders through cell center
Designed primers for one of Peter's components (forgot which)

June 20

Wet Lab

Picked 2 colonies of pDawn-mCherry, innoculated in 5 mL of LB and 50 ug/mL of Kan
PCR purified fragments (Peter), then ran gel?

@@ Line 212: / Line 212: @@
 <li>Finalized synthesis order (minus linker)</li>
 </ul>
+			</div>
+<h2 class="accordion-header">Week 4</h2>
+			<div class="accordion-content">
 			</div>
 </div>
+<p style="text-align:center">July 2012 Notebook</p>
 <div id="accordion-container">
-			<h2 class="accordion-header">Week 1</h2>
+			<h2 class="accordion-header">Week 5</h2>
 			<div class="accordion-content">
-				<p><b>June 6th</b></p>
-                                                 <ul>
-                                                  <li>Set up some lab equipment</li>
-                                                  <li>Autoclaved for a while</li>
- <li>Organized biobrick stuff</li>
-                                                  <li>Called Vinoo about DNA planning</li>
-                                                </ul>
-<br>
-<p><b>June 7th</b></p>
-                                                 <ul>
-                                                  <li>Transformed Cph8, pLsr, and LuxS</li>
-                                                  <li>Placed order with Vinoo</li>
- <li>Developed idea using PGY/PCN system to activate a gene</li>
-                                                </ul>
 			</div>
-			<h2 class="accordion-header">Week 2</h2>
+			<h2 class="accordion-header">Week 6</h2>
 			<div class="accordion-content">
-<p><b>June 11th</b></p>
-                             &nbsp;&nbsp;<p>Wet Lab</p>
-                                                 <ul>
-                                                  <li>PCR'd mCherry from NAS157</li>
-                                                  <li>Ran 1% Gel and purified product</li>
-                                                </ul>
-&nbsp;&nbsp;<p>Dry Lab</p>
-<ul>
-<li>Designed primers for LsR promoter</li>
-<li>Meeting with Dr. Sarkar</li>
-</ul>
-<br>
-<p><b>June 12th</b></p>
-                             &nbsp;&nbsp;<p>Wet Lab</p>
-                                                 <ul>
-                                                  <li>Digested mCherry PCR product with BamHI and NotI</li>
-                                                  <li>Column purified mCherry and ligated into NAS152 backbone</li>
-<li>Transformed NAS152-mCherry into DH5alpha</li>
-<li>Poured 25 LB-Kan plates</li>
-                                                </ul>
-&nbsp;&nbsp;<p>Dry Lab</p>
-<ul>
-<li>Research more information about bacterial drug delivery system</li>
-<li>More research into biofilm project</li>
-</ul>
-<br>
-	<p><b>June 14th</b></p>
-&nbsp;&nbsp;<p>Wet Lab</p>
-                                                 <ul>
-                                                  <li>Fill in later....</li>
-                                                </ul>
-&nbsp;&nbsp;<p>Dry Lab</p>
-<ul>
-<li>Met with Dr. Goulian, obtained pDawn and pDusk</li>
-<li>Identified inaK as a surface display gene we can use</li>
-</ul>
 			</div>
-			<h2 class="accordion-header">Week 3</h2>
+			<h2 class="accordion-header">Week 7</h2>
 			<div class="accordion-content">
+			</div>
+<h2 class="accordion-header">Week 8</h2>
-<p>June 18th</p>
+			<div class="accordion-content">
-&nbsp;&nbsp;<p>Wet Lab</p>
-<ul>
-<li>Miniprep pDawn and pDusk</li>
-<li>Test cut pDawn and pDusk with XmaI, analytical gel was correct</li>
-<li>Prep cut pDawn and pDusk with BamHI and NotI, gel purified</li>
-</ul>
-&nbsp;&nbsp;<p>Dry Lab</p>
-<ul>
-<li>Ordered and picked up PCR purification kit from cell center</li>
-<li>Additional orders through cell center</li>
-<li>Designed primers for one of Peter's components (forgot which)</li>
-</ul>
-<br>
-<p>June 20</p>
-&nbsp;&nbsp;<p>Wet Lab</p>
-<ul>
-<li>Picked 2 colonies of pDawn-mCherry, innoculated in 5 mL of LB and 50 ug/mL of Kan</li>
-<li>PCR purified fragments (Peter), then ran gel?</li>
-</ul>
-&nbsp;&nbsp;<p>Dry Lab</p>
-<ul>
-<li>Researched DARPin binding domains and linkers</li>
-<li>Finalized some biobrick orders</li>
-<li>Finalized synthesis order (minus linker)</li>
-</ul>
 			</div>