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Latest revision as of 11:12, 27 October 2013

Notebook: March

20.03.2013

Transformation

Investigator: Christian

Aim: Preparation of BioBrick templates → Transformation into E. coli DH5α.

Transformation of 1 µl pPha-NR, 1 µl pPha-T1 and 1 µl pCAT (diluted 1:3 with bidest. H2O) in E. coli DH5α (30 min ice, 90 sec 42°C, 1 min ice, 45 min 37°C + 1 ml LB), plated on LB_amp, overnight at 37°C.

21.03.2013

Inoculation

Investigator: Christian

Aim: Preparation of BioBrick templates → Inoculation of transformants for miniprep.

2 colonies of pPha-NR and pPha-T1 inoculated in 5 ml LB_amp, overnight at 37°C.

pCAT is a cosmid, transformation failed.

22.03.2013

Miniprep

Investigator: Christian

Aim: Preparation of BioBrick templates → Miniprep of the template-plasmids.

Miniprep of the liquid cultures (QIAprep Spin Miniprep Kit (Qiagen)), eluted in 25 µl bidest. H2O.

Digest

Investigator: Christian

Aim: Preparation of BioBrick templates → Control digestion of the template plasmids.

3 µl DNA template
1 µl enzyme 1
1 µl enzyme 2
4 µl buffer 2
31 µl bidest. H2O

Samples:

Digestion of pPha-NR with EcoRI and NcoI.

Digestion of pPha-T1 with EcoRI and NdeI.

The samples were incubated for 1 h at 37 °C.

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe per 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Lane		Content		Expectations
2+3		pPha-NR		2868 bp + 992 bp
4+5		pPha-T1		3554 bp + 541 bp

All positive.

PCR

Investigator: Christian

Aim: Construction of BioBricks → Deletion of restriction sites in iBB3, iBB4 and iBB5 via mutagenesis PCR.

Mutagenesis PCR of Pf_cpB (iBB3), P_NR (iBB4), and T_fcpA (iBB5).

Volume	Reagent	Temp (°C)	Time
1 µl	Phusion polymerase	95	3 min
1 µl	Primer fw (100 pmol/µl)	95	30 sec
1 µl	Primer rv (100 pmol/µl)	65	45 sec	x19
1 µl	Template pPha-NR (diluted 1:100)	72	4:10 min
1 µl	dNTPs	72	6 min
5 µl	10x buffer	4	Hold
35 µl	bidest. H2O

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe in 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Lane		Content
2		P_fcpB
3		P_NR
4		P_fcpA
5		P_fcpB
6		P_NR
7		P_fcpA

Digest

Investigator: Christian

Aim: Construction of BioBricks → Digestion of the template plasmid.

Digestion of the template with 1 µl DppI.

Transformation

Investigator: Christian

Aim: Construction of BioBricks → Transformation of mutagenised plasmids.

Transformation of 1 µl PCR-product into E. coli DH5α (30 min ice, 60 sec 42°C, 1 min ice, 30 min 37°C + 1 ml LB), plated on LB_amp, overnight at 37°C.

26.03.2013

Inoculation

Investigator: Christian

Aim: Construction of BioBricks → Inoculation of transformants for miniprep.

Transformation of iBB5 failed, new mutagenesis primers ordered.

3 colonies of iBB3 and iBB4 inoculated in 5 ml LB_amp, overnight at 37°C.

Inoculation

Investigator: Christian

Aim: Production of chemo-competent E. coli cells → Inoculation of E. coli DH5α pre-culture.

Inoculation of Ca-competent E. coli DH5α in 2x5 ml LB, overnight at 37°C.

Inoculation

Investigator: Christian

Aim: Preparation of BioBrick templates → Inoculation for glycerol stocks.

PPha-NR and pPha-T1 were inoculated in 5 ml LB, overnight at 37°C (for glycerol stocks).

27.03.2013

Miniprep

Investigator: Christian

Aim: Construction of BioBricks → Miniprep of transformants.

Miniprep of of iBB3 and iBB4 (QIAprep Spin Miniprep Kit (Qiagen)), eluted in 30 µl bidest. H2O.

Inoculation

Investigator: Christian

Aim: Production of chemo-competent E. coli cells → Inoculation of E. coli DH5α pre-culture.

3 ml E. coli DH5α pre-culture inoculated in 100 ml LB.

PCR

Investigator: Christian

Aim: Construction of BioBricks → Amplification of iBB2 via PCR.

PCR on CAT-cassette (iBB2):

Volume	Reagent	Temp (°C)	Time
1 µl	Q5 Polymerase	95	3 min
1 µl	Primer fw (1pmol/µl)	95	30 sec
1 µl	Primer rv (1pmol/µl)	65	30 sec	x26
1 µl	Template	72	1 min
1 µl	dNTPs	72	7 min
10 µl	5x Q5-buffer	4	Hold
36 µl	bidest. H2O

The PCR was cleaned via 1% agarose gel: Relevant fragments were cut from the gel and then purified via QIAgen Gel Extraction Kit (Qiagen). Elution into 20 µl elution buffer.

Transformation

Investigator: Christian

Aim: Production of chemo-competent E. coli → Control of cells.

Competent cells are harvested and frozen.

Controlled with several Transformations:

on LB
on LB_amp
on LB_amp with 1 µl pPha-T1
cells from AG Bange as control

30 min ice, 60 sec 42°C, 60 sec ice, 60 min 37°C + 1 ml LB; plated, overnight at 37°C.

Digest

Investigator: Christian

Aim: Construction of BioBricks → Control digestion of mutations.

3 µl DNA template
1 µl enzyme 1
1 µl enzyme 2
1 µl buffer
5 µl bidest. H2O

Samples:

Digestion of iBB3 (P_fcpB) with PvuII.

Digestion of IBB4 (P_NR) with PstI.

The samples were incubated for 1 h at 37 °C.

Gel electrophoresis

Gel substances

1% Agarose gel
10 µl RedSafe in 50 ml gel
6 µl GeneRuler™ 1kb plus DNA Ladder (Thermo Scientific)
6x loading buffer (for samples)

Lane	Content	Comment
2	P_fcpB 1	no cut, vector in different forms
3	P_fcpB 2
4	P_fcpB 3
5	P_NR 1	1 cut → linearized plasmid
6	P_NR 2
7	P_NR 3

28.03.2013

Sequencing

Investigator: Christian

Aim: Construction of BioBricks → Sequencing.

IBB3 and iBB4 with point mutations prepared for sequencing:

AGBOOOK 128: iBB4 1
AGBOOOK 129: iBB4 2
AGBOOOK 130: iBB4 3
AGBOOOK 131: iBB3 1
AGBOOOK 132: iBB3 2
AGBOOOK 133: iBB3 3

@@ Line 1: / Line 1: @@
 {{:Team:Marburg/Template:Header}}
-{{:Team:Marburg/Template:ContentTitle}}
+{{:Team:Marburg/Template:ContentTitleNav}}
-Notebook: March
+Notebook: March <html><a href="https://2013.igem.org/Team:Marburg/Notebook:April"><img src="https://static.igem.org/mediawiki/2013/7/71/Mr-igem-next-arrow.png" style="float:right;margin-left:5px !important;" alt="Next"></a>&nbsp;<a href="https://2013.igem.org/Team:Marburg/Notebook:Ptricornutum"><img src="https://static.igem.org/mediawiki/2013/1/13/Mr-igem-previous-arrow.png" alt="Previous" style="float:right;"></a></html>
-{{:Team:Marburg/Template:ContentStart}}
+{{:Team:Marburg/Template:ContentStartNav}}<html>
-<html>
@@ Line 21: / Line 19: @@
      <div class="aim">
 		<span class="aim">Aim:</span>
-		<span class="aim-desc">Preparation of BioBrick-templates &rarr; Transformation into <i>E. coli</i> DH5&alpha;.</span>
+		<span class="aim-desc">Preparation of BioBrick templates &rarr; Transformation into <i>E. coli</i> DH5&alpha;.</span>
 	</div>
 	<div class="exp-content">
-		<p>Transformation of 1 µl pPha-NR, 1 µl pPha-T1 and 1 µl pCAT (diluted 1:3 with H2O) in <i>E. coli</i> DH5&alpha; (30 min ice, 90 sec 42°C, 1 min ice, 45 min 37°C + 1 ml LB), plated on LB<sub>amp</sub>, oN 37°C.</p>
+		<p>Transformation of 1 µl pPha-NR, 1 µl pPha-T1 and 1 µl pCAT (diluted 1:3 with bidest. H2O) in <i>E. coli</i> DH5&alpha; (30 min ice, 90 sec 42°C, 1 min ice, 45 min 37°C + 1 ml LB), plated on LB<sub>amp</sub>, overnight at 37°C.</p>
 	</div>
 </fieldset>
@@ Line 45: / Line 43: @@
      <div class="aim">
 		<span class="aim">Aim:</span>
-		<span class="aim-desc">Preparation of BioBrick-templates &rarr; Inoculation of transformants for miniprep.</span>
+		<span class="aim-desc">Preparation of BioBrick templates &rarr; Inoculation of transformants for miniprep.</span>
 	</div>
 	<div class="exp-content">
-		<p>2 colonies of pPha-NR and pPha-T1 inoculated in 5 ml LB<sub>amp</sub>, oN 37°C.</p>
+		<p>2 colonies of pPha-NR and pPha-T1 inoculated in 5 ml LB<sub>amp</sub>, overnight at 37°C.</p>
-		<p>pCAT is a Cosmid, transformation failed.</p>
+		<p>pCAT is a cosmid, transformation failed.</p>
 	</div>
 </fieldset>
@@ Line 70: / Line 68: @@
      <div class="aim">
 		<span class="aim">Aim:</span>
-		<span class="aim-desc">Preparation of BioBrick-templates &rarr; Miniprep of the template-plasmids.</span>
+		<span class="aim-desc">Preparation of BioBrick templates &rarr; Miniprep of the template-plasmids.</span>
 	</div>
 	<div class="exp-content">
-		<p>Miniprep of the liquid cultures (“QIAprep Spin Miniprep Kit” (Qiagen, Düsseldorf)), eluted in 25 µl H2O.</p>
+		<p>Miniprep of the liquid cultures (QIAprep Spin Miniprep Kit (Qiagen)), eluted in 25 µl bidest. H2O.</p>
 	</div>
 </fieldset>
@@ Line 86: / Line 84: @@
      <div class="aim">
 		<span class="aim">Aim:</span>
-		<span class="aim-desc">Preparation of BioBrick-templates &rarr; Control digestion of the template plasmids.</span>
+		<span class="aim-desc">Preparation of BioBrick templates &rarr; Control digestion of the template plasmids.</span>
 	</div>
 	<div class="exp-content">
@@ Line 94: / Line 92: @@
 			<li>1 µl enzyme 2</li>
 			<li>4 µl buffer 2</li>
-			<li>31 µl H2O</li>
+			<li>31 µl bidest. H2O</li>
 		</ul>
 		<p>Samples:</p>
 		<p>Digestion of pPha-NR with <i>EcoR</i>I and <i>Nco</i>I.</p>
 		<p>Digestion of pPha-T1 with <i>EcoR</i>I and <i>Nde</i>I.</p>
-		<p>The samples were incubated for 1 h at 37° C.</p>
+		<p>The samples were incubated for 1 h at 37 °C.</p>
 		<table class="gel digest">
 			<colgroup>
@@ Line 113: / Line 111: @@
 			<tr>
 				<td>
-					<img src="beispiel.png" width="50%" alt="gel-electrophoresis-image" />
+					<img src="https://static.igem.org/mediawiki/2013/d/d9/Gel_2013-03-22.png" width="100%" alt="gel-electrophoresis-image" />
 				</td>
 				<td>
@@ Line 126: / Line 124: @@
 					</p>
 					<p>
-						<span class="exp">Expectations</span>
+							<table class="gel">
-						<ul class="exp">
+								<colgroup>
-							<li>pPha-NR: 2868 bp + 992 bp</li>
+									<col width="10%" />
-							<li>pPha-T1: 3554 bp + 541 bp</li>
+									<col width="2%" />
-						</ul>
+									<col width="50%" />
+									<col width="5%" />
+									<col width="33%" />
+								</colgroup>
+								<thead>
+									<th>Lane</th>
+									<th>&nbsp;</th>
+									<th>Content</th>
+									<th>&nbsp;</th>
+									<th>Expectations</th>
+								</thead>
+								<tr>
+									<td>2+3</td>
+									<th>&nbsp;</th>
+									<td>pPha-NR</td>
+									<th>&nbsp;</th>
+									<td>2868 bp + 992 bp</td>
+								</tr>
+								<tr>
+									<td>4+5</td>
+									<th>&nbsp;</th>
+									<td>pPha-T1</td>
+									<th>&nbsp;</th>
+									<td>3554 bp + 541 bp</td>
+								</tr>
+							</table>
 					</p>
 					<p>All positive.</p>
@@ Line 171: / Line 194: @@
 			<tr>
 				<td>1 µl</td>
-				<td>Phusion Polymerase</td>
+				<td>Phusion polymerase</td>
 				<td>&nbsp;</td>
 				<td>95</td>
@@ Line 178: / Line 201: @@
 			<tr>
 				<td>1 µl</td>
-				<td>Primer 1 (100pmol/µl)</td>
+				<td>Primer fw (100 pmol/µl)</td>
 				<td>&nbsp;</td>
 				<td>95</td>
@@ Line 185: / Line 208: @@
 			<tr>
 				<td>1 µl</td>
-				<td>Primer 2 (100pmol/µl) </td>
+				<td>Primer rv (100 pmol/µl) </td>
 				<td>&nbsp;</td>
 				<td>65</td>
@@ Line 214: / Line 237: @@
 			<tr>
 				<td>35 µl</td>
-				<td>ddH20</td>
+				<td>bidest. H2O</td>
 				<td>&nbsp;</td>
 			</tr>
@@ Line 233: / Line 256: @@
 			<tr>
 				<td>
-					<img src="beispiel.png" width="50%" alt="gel-electrophoresis-image" />
+					<img src="https://static.igem.org/mediawiki/2013/e/e6/Gel_2013-03-25.png" width="100%" alt="gel-electrophoresis-image" />
 				</td>
 				<td>
@@ Line 244: / Line 267: @@
 						<li>6x loading buffer (for samples)</li>
 					</ul>
+					</p>
+					<p>
+							<table class="gel">
+								<colgroup>
+									<col width="10%" />
+									<col width="2%" />
+									<col width="50%" />
+									<col width="5%" />
+									<col width="33%" />
+								</colgroup>
+								<thead>
+									<th>Lane</th>
+									<th>&nbsp;</th>
+									<th>Content</th>
+									<th>&nbsp;</th>
+									<th>&nbsp;</th>
+								</thead>
+								<tr>
+									<td>2</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpB</sub></td>
+									<th>&nbsp;</th>
+									<td>&nbsp;</td>
+								</tr>
+								<tr>
+									<td>3</td>
+									<th>&nbsp;</th>
+									<td>P<sub>NR</sub></td>
+									<th>&nbsp;</th>
+									<td>&nbsp;</td>
+								</tr>
+								<tr>
+									<td>4</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpA</sub></td>
+									<th>&nbsp;</th>
+									<td>&nbsp;</td>
+								</tr>
+								<tr>
+									<td>5</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpB</sub></td>
+									<th>&nbsp;</th>
+									<td>&nbsp;</td>
+								</tr>
+								<tr>
+									<td>6</td>
+									<th>&nbsp;</th>
+									<td>P<sub>NR</sub></td>
+									<th>&nbsp;</th>
+									<td>&nbsp;</td>
+								</tr>
+								<tr>
+									<td>7</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpA</sub></td>
+									<th>&nbsp;</th>
+									<td>&nbsp;</td>
+								</tr>
+							</table>
 					</p>
 				</td>
@@ Line 263: / Line 346: @@
 		<span class="aim-desc">Construction of BioBricks &rarr; Digestion of the template plasmid.</span>
 	</div>
+	<div class="exp-content">
 		<p>Digestion of the template with 1 µl <i>Dpp</i>I.</p>
-		<table class="gel digest">
-			<colgroup>
-				<col width="50%" />
-				<col width="50%" />
-			</colgroup>
-		<thead>
-			<tr>
-				<th colspan="2" class="title">Gel electrophoresis</th>
-			</tr>
-		</thead>
-		<tbody>
-			<tr>
-				<td>
-					<img src="beispiel.png" width="50%" alt="gel-electrophoresis-image" />
-				</td>
-				<td>
-					<p>
-					<span class="gel-elc">Gel substances</span>
-					<ul class="gel-sub">
-						<li>1% Agarose gel</li>
-						<li>10 µl RedSafe per 50 ml gel</li>
-						<li>6 µl GeneRuler&trade; 1kb plus DNA Ladder (Thermo Scientific)</li>
-						<li>6x loading buffer (for samples)</li>
-					</ul>
-					</p>
-				</td>
-			</tr>
-		</tbody>
-		</table>
 	</div>
 </fieldset>
@@ Line 308: / Line 363: @@
 	</div>
 	<div class="exp-content">
-		<p>Transformation of 1 µl PCR-product into <i>E. coli</i> DH5&alpha; (30 min ice, 60 sec 42°C, 1 min ice, 30 min 37°C + 1 ml LB), plated on LB<sub>amp</sub>, oN 37°C.</p>
+		<p>Transformation of 1 µl PCR-product into <i>E. coli</i> DH5&alpha; (30 min ice, 60 sec 42°C, 1 min ice, 30 min 37°C + 1 ml LB), plated on LB<sub>amp</sub>, overnight at 37°C.</p>
 	</div>
 </fieldset>
@@ Line 333: / Line 388: @@
 	<div class="exp-content">
 		<p>Transformation of iBB5 failed, new mutagenesis primers ordered.</p>
-		<p>3 colonies of iBB3 and iBB4 inoculated in 5 ml LB<sub>amp</sub>, oN 37°C.</p>
+		<p>3 colonies of iBB3 and iBB4 inoculated in 5 ml LB<sub>amp</sub>, overnight at 37°C.</p>
 	</div>
 </fieldset>
@@ Line 349: / Line 404: @@
 	</div>
 	<div class="exp-content">
-		<p>Inoculation of Ca-competent <i>E. coli</i> DH5&alpha; in 2x5 ml LB, oN 37°C.</p>
+		<p>Inoculation of Ca-competent <i>E. coli</i> DH5&alpha; in 2x5 ml LB, overnight at 37°C.</p>
 	</div>
 </fieldset>
@@ Line 362: / Line 417: @@
      <div class="aim">
 		<span class="aim">Aim:</span>
-		<span class="aim-desc">Preparation of BioBrick-templates &rarr; Inoculation for glycerol stocks.</span>
+		<span class="aim-desc">Preparation of BioBrick templates &rarr; Inoculation for glycerol stocks.</span>
 	</div>
 	<div class="exp-content">
-		<p>PPha-NR and pPha-T1 were inoculated in 5 ml LB, oN 37°C (for glycerol stocks).</p>
+		<p>PPha-NR and pPha-T1 were inoculated in 5 ml LB, overnight at 37°C (for glycerol stocks).</p>
 	</div>
 </fieldset>
@@ Line 389: / Line 444: @@
 	</div>
 	<div class="exp-content">
-		<p>Miniprep of of iBB3 and iBB4 (“QIAprep Spin Miniprep Kit” (Qiagen, Düsseldorf)), eluted in 30 µl H2O.</p>
+		<p>Miniprep of of iBB3 and iBB4 (QIAprep Spin Miniprep Kit (Qiagen)), eluted in 30 µl bidest. H2O.</p>
 	</div>
 </fieldset>
@@ Line 447: / Line 502: @@
 			<tr>
 				<td>1 µl</td>
-				<td>Primer 1 (1pmol/µl)</td>
+				<td>Primer fw (1pmol/µl)</td>
 				<td>&nbsp;</td>
 				<td>95</td>
@@ Line 454: / Line 509: @@
 			<tr>
 				<td>1 µl</td>
-				<td>Primer 2 (1pmol/µl) </td>
+				<td>Primer rv (1pmol/µl) </td>
 				<td>&nbsp;</td>
 				<td>65</td>
@@ Line 483: / Line 538: @@
 			<tr>
 				<td>36 µl</td>
-				<td>ddH20</td>
+				<td>bidest. H2O</td>
 				<td>&nbsp;</td>
 			</tr>
 		</table>
-		<br />
+		<p>The PCR was cleaned via 1% agarose gel: Relevant fragments were cut from the gel and then purified via QIAgen Gel Extraction Kit (Qiagen). Elution into 20 µl elution buffer.</p>
-		<!-- Gel-Bild-->
-		<table class="gel pcr">
-			<colgroup>
-				<col width="50%" />
-				<col width="50%" />
-			</colgroup>
-		<thead>
-			<tr>
-				<th colspan="2" class="title">Gel electrophoresis</th>
-			</tr>
-		</thead>
-		<tbody>
-			<tr>
-				<td>
-					<img src="beispiel.png" width="50%" alt="gel-electrophoresis-image" />
-				</td>
-				<td>
-					<p>
-					<span class="gel-elc">Gel substances</span>
-					<ul class="gel-sub">
-						<li>1% Agarose gel</li>
-						<li>10 µl RedSafe in 50 ml gel</li>
-						<li>6 µl GeneRuler&trade; 1kb plus DNA Ladder (Thermo Scientific)</li>
-						<li>6x loading buffer (for samples)</li>
-					</ul>
-					</p>
-					<p>The relevant fragments were cut from the gel and then purified via “Qiagen Gel Extraction Kit” (Qiagen, Düsseldorf). Elution into 20 µl elution buffer.</p>
-				</td>
-			</tr>
-		</tbody>
-		</table>
 	</div>
 </fieldset>
@@ Line 531: / Line 555: @@
      <div class="aim">
 		<span class="aim">Aim:</span>
-		<span class="aim-desc">: Production of chemo-competent <i>E. coli</i> &rarr; Control of cells.</span>
+		<span class="aim-desc">Production of chemo-competent <i>E. coli</i> &rarr; Control of cells.</span>
 	</div>
 	<div class="exp-content">
-		<p>Competent cells harvested and frozen.</p>
+		<p>Competent cells are harvested and frozen.</p>
 		<p>Controlled with several Transformations:</p>
 			<ul class="justalist">
@@ Line 542: / Line 566: @@
 				<li>cells from AG Bange as control</li>
 			</ul>
-		<p>30 min ice, 60 sec 42°C, 60 sec ice, 60 min 37°C + 1 ml LB; plated, oN 37°C.</p>
+		<p>30 min ice, 60 sec 42°C, 60 sec ice, 60 min 37°C + 1 ml LB; plated, overnight at 37°C.</p>
 	</div>
 </fieldset>
@@ Line 563: / Line 587: @@
 			<li>1 µl enzyme 2</li>
 			<li>1 µl buffer</li>
-			<li>5 µl H2O</li>
+			<li>5 µl bidest. H2O</li>
 		</ul>
 		<p>Samples:</p>
-		<p>Digestion of iBB3 with <i>Pvu</i>II.</p>
+		<p>Digestion of iBB3 (P<sub>fcpB</sub>) with <i>Pvu</i>II.</p>
-		<p>Digestion of IBB4 with <i>Pst</i>I.</p>
+		<p>Digestion of IBB4 (P<sub>NR</sub>) with <i>Pst</i>I.</p>
-		<p>The samples were incubated for 1 h at 37° C.</p>
+		<p>The samples were incubated for 1 h at 37 °C.</p>
+		<!-- Gel-Bild-->
 		<table class="gel digest">
 			<colgroup>
@@ Line 582: / Line 607: @@
 			<tr>
 				<td>
-					<img src="beispiel.png" width="50%" alt="gel-electrophoresis-image" />
+					<img src="https://static.igem.org/mediawiki/2013/3/3d/Gel_2013-03-27.png" width="100%" alt="gel-electrophoresis-image" />
 				</td>
 				<td>
@@ Line 589: / Line 614: @@
 					<ul class="gel-sub">
 						<li>1% Agarose gel</li>
-						<li>10 µl RedSafe per 50 ml gel</li>
+						<li>10 µl RedSafe in 50 ml gel</li>
 						<li>6 µl GeneRuler&trade; 1kb plus DNA Ladder (Thermo Scientific)</li>
 						<li>6x loading buffer (for samples)</li>
@@ Line 595: / Line 620: @@
 					</p>
 					<p>
-						<span class="exp">Expectations</span>
+							<table class="gel">
-						<ul class="exp">
+								<colgroup>
-							<li>iBB3: no cut, vector in different forms</li>
+									<col width="10%" />
-							<li>iBB4: 1 cut, linearized plasmid</li>
+									<col width="2%" />
-						</ul>
+									<col width="50%" />
+									<col width="5%" />
+									<col width="33%" />
+								</colgroup>
+								<thead>
+									<th>Lane</th>
+									<th>&nbsp;</th>
+									<th>Content</th>
+									<th>&nbsp;</th>
+									<th>Comment</th>
+								</thead>
+								<tr>
+									<td>2</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpB</sub> 1</td>
+									<th>&nbsp;</th>
+									<td rowspan="3">no cut, vector in different forms</td>
+								</tr>
+								<tr>
+									<td>3</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpB</sub> 2</td>
+									<th>&nbsp;</th>
+								</tr>
+								<tr>
+									<td>4</td>
+									<th>&nbsp;</th>
+									<td>P<sub>fcpB</sub> 3</td>
+									<th>&nbsp;</th>
+								</tr>
+								<tr>
+									<td>5</td>
+									<th>&nbsp;</th>
+									<td>P<sub>NR</sub> 1</td>
+									<th>&nbsp;</th>
+									<td rowspan="3">1 cut &rarr; linearized plasmid</td>
+								</tr>
+								<tr>
+									<td>6</td>
+									<th>&nbsp;</th>
+									<td>P<sub>NR</sub> 2</td>
+									<th>&nbsp;</th>
+								</tr>
+								<tr>
+									<td>7</td>
+									<th>&nbsp;</th>
+									<td>P<sub>NR</sub> 3</td>
+									<th>&nbsp;</th>
+								</tr>
+							</table>
 					</p>
-					<p>All positive.</p>
 				</td>
 			</tr>
@@ Line 646: / Line 719: @@
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-{{:Team:Marburg/Template:ContentEnd}}
+{{:Team:Marburg/Template:ContentEndNav}}
 {{:Team:Marburg/Template:Footer}}

Team:Marburg/Notebook:March

From 2013.igem.org

Latest revision as of 11:12, 27 October 2013

Notebook: March

20.03.2013

21.03.2013

22.03.2013

26.03.2013

27.03.2013

28.03.2013