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June

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Safety Instructions

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Introduction to centrifuges and autoclaves

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Finished mandatory training

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Media Preparation

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Amplification and Purification of non-synthetic parts

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July

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Augusti

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@@ Line 18: / Line 18: @@
 		#calendar>table {
 			margin: 2em;
-			border-spacing: 10px;
+			border-spacing: 5px;
 			border-collapse: separate;
 		}
+		#calendar table tr td {
+			width: 130px;
+			height: 80px;
+		}
 		.date {
 			background-color: #f4f4f4;
@@ Line 39: / Line 44: @@
              margin-left: 1em;
          }
+		.prev-month, .next-month {
+			background-color: #7d7d7d;
+		}
          #contentDialog {
              min-height: 100px;
@@ Line 53: / Line 62: @@
              height: 75%;
              padding: 16px;
-             border: 16px solid #ED6D22;
+             border: 16px solid #ed6d22;
              background-color: white;
              z-index:1002;
@@ Line 311: / Line 320: @@
                      <h1>26</h1>
                      <ul class="titles">
-                         <li>Plasmid Purification</li>
+                         <li>Title one</li>
-                         <li>Amplification and purification of parts</li>
+                         <li>Title two</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-						<h2>Plasmid Purification</h2>
-						<p> Performed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416, p2055 and a plasmid containig our Cas9 sequence
-						(pTPG1-dCas9-UPGP)via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by
-						water on the last step. <br>
-						<h2>Amplification and purification of parts</h2>
-						<p>Performed a PCR amplification of the non-synthetic parts that failed on the day before and on the dCas9 sequence and the three fluorescent proteins
-						-Yellow, Cyano and Red (YFP, CFP and RFP, respectively). <br>
-						<p>The PCR was done using the Phusion High-Fidelity DNA Polymerase (see protocol here) and the program used was: <br>
-							<ol>
-							<li>3 min at 98ºC </li>
-							<li>10s at 98ºC </li>
-							<li>Gradient from 50 to 55ºC for 30s </li>
-							<li>30s at 60ºC </li>
-							<li>2min 15s at 72ºC </li>
-							<li>Go to step 2 (repeat 39 times) </li>
-							<li>10 min at 72ºC. </li>
-							</ol>
-						<p>A diagnostic gel was performed and the result is as follows: <br>
-						[[File: Bio-Rad 2014-06-26 17hr 53min.jpg|frameless|300px]] <br>
-						</span>
                  </td>
@@ Line 340: / Line 329: @@
                      <h1>27</h1>
                      <ul class="titles">
-                         <li>Gel extraction</li>
+                         <li>Title one</li>
-						<li>PCR amplification and merging</li>
+                        <li>Title two</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-					<h2>Gel extraction</h2>
-						<p>Extracted the fluorecent proteins amplified on the day before with a GeneJet gel extraction kit.The manufacter's
-						instructions were followed, except the elution buffer was subtituted by water on the last step.
-					<h2>PCR amplification and merging</h2>
-						<p>Performed a PCR to fuse 	the pDSE4, pHO and dCas9 parts together.<br>
-						<p>The PCR was done using the Phusion High-Fidelity DNA Polymerase (see protocol here) and the program used was: <br>
-						<ol>
-							<li>3 min at 98ºC </li>
-							<li>10s at 98ºC</li>
-							<li>Gradient from 50 to 55ºC for 30s</li>
-							<li>30s at 60ºC</li>
-							<li>2min 15s at 72ºC</li>
-							<li>Go to step 2 (repeat 39 times)</li>
-							<li>10 min at 72ºC.</li>
-						</ol>
-						<p>A diagnostic gel was performed and the result is as follows: <br>
-						[[File: Bio-Rad 2014-06-27 15hr 07min-2.jpg|frameless|300px]] <br>
-						<p>The bands did not seem correct, so this PCR was repeated on the next day.<br>
-					</span>
                  </td>
@@ Line 368: / Line 338: @@
                      <h1>28</h1>
                      <ul class="titles">
-                         <li>PCR amplification and merging</li>
+                         <li>Title one</li>
-                         <li>Plasmid restriction</li>
+                         <li>Title two</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-					<h2>PCR amplification and merging</h2>
-						<p>Repeated the PCR to fuse the pDSE4, pHO and dCas9 parts together.<br>
-						<p>The PCR was done using the Phusion High-Fidelity DNA Polymerase (see protocol here) and the program used was: <br>
-						<ol>
-							<li>3 min at 98ºC </li>
-							<li>10s at 98ºC</li>
-							<li>50ºC for 30s</li>
-							<li>58ºC for 30s</li>
-							<li>2min 15s at 72ºC</li>
-							<li>Go to step 2 (repeat 39 times)</li>
-							<li>10 min at 72ºC.</li>
-						</ol>
-					<p>A diagnostic gel was performed and the result is as follows: <br>
-					[File: Bio-Rad 2014-06-30 15hr 24min.jpg|frameless|300px]] <br>
-					<p>This did not seemed to work either.
-					<h2>Plasmid restriction</h2>
-						<p>Cleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. <br>
-						<p>Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
-						(alkaline phosphatase) and up to 20 UL of deionized sterile water.<br>
-						<p>This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC.<br>
-				</span>
                  </td>
@@ Line 398: / Line 347: @@
                      <h1>29</h1>
                      <ul class="titles">
+                        <li>Title one</li>
+                        <li>Title two</li>
                      </ul>
-                     <span class="hidden"></span>
+                     <span class="hidden">This is where all the information goes!</span>
                  </td>
              </tr>
@@ Line 407: / Line 358: @@
                      <h1>30</h1>
                      <ul class="titles">
-                         <li>PCR amplification and merging</li>
+                         <li>Title one</li>
+                        <li>Title two</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-					<h2>PCR amplification and merging</h2>
-						Repeated the PCR to fuse the pDSE4, pHO and dCas9 parts together.<br>
-						<p>The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br>
-						<ol>
-							<li>3 min at 98ºC </li>
-							<li>10s at 98ºC</li>
-							<li>50ºC for 30s</li>
-							<li>58ºC for 30s</li>
-							<li>2min 30s at 72ºC</li>
-							<li>Go to step 2 (repeat 40 times)</li>
-							<li>10 min at 72ºC.</li>
-						</ol>
-						<p> A diagnostic gel was performed, however the sizes of the resulting fragments did not match the expected.
-					<h2>Plasmid restriction</h2>
-						<p>Cleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. <br>
-						<p>Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
-						(alkaline phosphatase) and up to 20 UL of deionized sterile water.<br>
-						<p>This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC.<br>
-						<p>Samples were loaded into a gelGreen, that showed p413, p415 and p416 approximately in the 5000bp size band, while p414 presented two bands, one around 4000bp and another at 2000bp.<br>
-						<p> this indicates that the 5000bp band corresponds to the uncut plasmid, while the 4000bp and 2000bp are probably contaminations.<br>
-					</span>
                  </td>
-                 <td id="2014-07-01" class="date next-month">
+                 <td id="2014-07-01" class="date next-month"> <!-- My birthday -->
                      <h1>1</h1>
                      <ul class="titles">
-                       <li>Plasmid restriction</li>
+                        <li>Title one</li>
-                         <li>PCR amplification</li>
+                         <li>Title two</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-					<h2>Plasmid restriction</h2>
-						<p>Cleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. <br>
-						<p>Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
-						(alkaline phosphatase) and up to 20 UL of deionized sterile water.<br>
-						<p>This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC.<br>
-					<h2>PCR amplification</h2>
-					<p>Amplified the parts pDSE4, cas9 and pHO. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br>
-						<ol>
-							<li>3 min at 98ºC </li>
-							<li>10s at 98ºC</li>
-							<li>50ºC for 30s</li>
-							<li>58ºC for 30s</li>
-							<li>2min 15s at 72ºC</li>
-							<li>Go to step 2 (repeat 40 times)</li>
-							<li>10 min at 72ºC.</li>
-					<p>	A diagnostic gel was performed, however the sizes of the resulting fragments did not match the expected.
-					</span>
                  </td>
@@ Line 464: / Line 376: @@
                      <h1>2</h1>
                      <ul class="titles">
-                         <li>PCR amplification</li>
+                         <li>Title one</li>
-						<li>Gel extraction</li>
+                         <li>Title two</li>
-                         <li>Concentration determination</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-					<h2>PCR amplification</h2>
-					<p>Repeated the amplification of the parts pDSE4, cas9 and pHO. The PCR was done using the Phusion High-Fidelity DNA Polymerase and the program used was: <br>
-						<ol>
-							<li>3 min at 98ºC </li>
-							<li>10s at 98ºC</li>
-							<li>50ºC for 30s</li>
-							<li>58ºC for 30s</li>
-							<li>2min 15s at 72ºC</li>
-							<li>Go to step 2 (repeat 40 times)</li>
-							<li>10 min at 72ºC.</li>
-					<p>	A diagnostic gel was performed and the sizes of the fragments matched for the pDSE4 and pHO, but not for the Cas9.<br>
-					<h2>Gel extraction</h2>
-						<p>Extracted the DNA fragments previously amplified with a GeneJet gel extraction kit.The manufacter's
-						instructions were followed, except the elution buffer was subtituted by water on the last step.
-					<h2>Concentration determination</h2>
-					<p>The concentration of all the fragments obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 8.5 ng of DNA per UL to 42ng/UL.<br>
-					</span>
                  </td>
@@ Line 491: / Line 385: @@
                      <h1>3</h1>
                      <ul class="titles">
-                     </ul>
+                        <li>Title one</li>
-                     <span class="hidden"></span>
+                        <li>Title two</li>
+                    </ul>
+                     <span class="hidden">This is where all the information goes!</span>
                  </td>
@@ Line 498: / Line 394: @@
                      <h1>4</h1>
                      <ul class="titles">
-                         <li>Plasmid Purification</li>
+                         <li>Title one</li>
-                         <li>Plasmid restriction</li>
+                         <li>Title two</li>
-						<li>Gel extraction</li>
-						 <li>Concentration determination</li>
                      </ul>
-                     <span class="hidden">
+                     <span class="hidden">This is where all the information goes!</span>
-					<h2>Plasmid purification</h2>
-					<p>Performed plasmid purification on E. coli cells containing plasmids p413, p414, p415, p416 and p2055 via a GenJet Plasmid Purification Kit. The manufacter's instructions were followed, except the elution buffer was subtituted by
-						water on the last step. Each plasmid was purified in duplicates.
-					<h2>Plasmid restriction</h2>
-						<p>Cleaved the plasmids p413TEF, p414TEF, p415TEF and p416TEF by using the enzymes SacI and XbaI. <br>
-						<p>Approximately 500ng of each plasmid was mixed with o.5UL of SacI, 0.5UL of XbaI, 2UL of FastDigest buffer, 1UL of FastAP
-						(alkaline phosphatase) and up to 20 UL of deionized sterile water. Control tubes containing just one of the enzymes each were also prepared.<br>
-						<p>This reaction mixture was incubated at in a water bath at 37ºC for 10 minutes and then enzymatic inactivation was performed for 5min in a heating block at 60ºC.<br>
-						<p> A diagnostic gelGreen was performed and showed that the cleavage of plasmids p413, p415 and p416 was successful.<br>
-					<h2>Gel extraction</h2>
-						<p>Extracted the cleaved plasmids with a GeneJet gel extraction kit.The manufacter's instructions were followed, except the elution buffer was subtituted by water on the last step.
-					<h2>Concentration determination</h2>
-					<p>The concentration of the circular and linear plasmids obtained was measured via a NanoDrop. The samples were measured in duplicates. The results ranged from 6.55 ng of DNA per UL to 543.4ng/UL.<br>
-					</span>
                  </td>
@@ Line 524: / Line 403: @@
                      <h1>5</h1>
                      <ul class="titles">
+                        <li>Title one</li>
+                        <li>Title two</li>
                      </ul>
-                     <span class="hidden"></span>
+                     <span class="hidden">This is where all the information goes!</span>
                  </td>
@@ Line 532: / Line 412: @@
                      <h1>6</h1>
                      <ul class="titles">
+                        <li>Title one</li>
+                        <li>Title two</li>
                      </ul>
-                     <span class="hidden"></span>
+                     <span class="hidden">This is where all the information goes!</span>
                  </td>
              </tr>

Team:Gothenburg/Calendar

From 2014.igem.org

Revision as of 21:40, 5 October 2014

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