Team:Freiburg/Notebook/lab gfp reporter

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Latest revision as of 05:13, 28 October 2013

GFP-reporter-plasmid Notebook

May

03. May 2013

Testdigest of pSB1C3 backbone

As a source plasmid to get the pSB1C3 backbone we used a biobrick called BBa_K515107

Approach of test digest:

µl
2	BBa_K515107
2	NEB Buffer 4 (10X)
0.5	EcoR1-HF
0.5	Pst1-HF
15	H2O

PCR 1

µl	type
25	Q5-HF Mastermix
20ng	DNA
2.5	Primer1
2,5	Primer2
Add to 50	H₂O

CMV-promotor

oIG6000
oIG6001
Temp.: eGFP-Plasmid

GFP

oIG6002
oIG 6003
Temp.: eGFP-Plasmid

Terminator

oIG6004
oIG6005
Temp.: eGFP-Plasmid

CFP

oIG6002
oIG6012
Temp.: CFP M4 Plasmid

Gel of PCR 1

expected length of the fragments: 1. CMV: 685bp 2. eGFP: 824bp 3.terminator: 350bp 4.CFP: 820bp bands were not expactly running as expected, but perhaps due to the marker. the marker bands are not separated clearly. So the bands were cut out and gel ex was performed. Nanodropping after the Gel ex: 1. CMV: 156ng/µl 2. eGFP: 143ng/µl 3. terminator: 163ng/µl 4. CFP: 85ng/µl

07. May 3013

Fusion PCR 7.5.13

µl	type
10	5x Q5 Buffer
4	DNTPs
0.5	Q5
1	CMV
1	eGFP
2.5	oIG600
2,5	oIG6003
Add to 50	H₂O

µl	type
10	5x Q5 Buffer
4	DNTPs
0.5	Q5
1	terminator
1.5	CFP
2.5	oIG602
2,5	oIG6005
Add to 50	H₂O

additionally a no template control was performed. the PCRs were run with Manus PCR programm. 1.30min elongation time.

preperation digest of pSB1C3

As a source plasmid to get the pSB1C3 backbone we used a biobrick called BBa_K515107

Approach of test digest:

µl
5	BBa_K515107
5	NEB Buffer 4 (10X)
1	Xba-HF
1	Pst1-HF
38	H2O

gelbild of fusion PCR and prep digest

08. May 3013

PCR: second try of the first one

µl	type
10	Q5-Buffer
4	DNTPs
2	DNA (1:10 diluted)
0,5	Q5
2.5	Primer fw
2,5	Primer rv
Add to 50	H₂O

the same results as in the first try were obtained and the bands were cut out and put in the freezer but a gel ex was never performed.

digest of pSB1C3 (Bba_K32305 and Bba_K32380)

µl	type
2	DNA
5	NEB-Buffer 4
1	Xba1
1	Pst1
Add to 50µl	H₂O

Temp.: 37°C
Incubation time: 2h

length of backbone: 2070bp. insert that is cut out: 1274bp (...80). Bands on gel as expected.

10.05.13

Fusion PCR

1. CMV+eGFP

µl	type
10	Q5-HF Reaction Buffer
1	CMV
1	eGFP
2,5	oIG6000
2,5	oIG6003
2.5	dNTPs
1	DMSO
Add to 50	H₂O

2. CFP+SV40 terminator

µl	type
10	Q5-HF Reaction Buffer
1	ecfp
1	termin
2,5	oIG6002
2,5	oIG6005
2.5	dNTPs
1	DMSO
Add to 50	H₂O

3. eGFP+ SV40 terminator

µl	type
10	Q5-HF Reaction Buffer
1	termin
1	eGFP
2,5	oIG6002
2,5	oIG6005
2.5	dNTPs
1	DMSO
Add to 50	H₂O

Annealing: 60°C
Extension:40s

June

5.6.13

PCR of construct 405 (Anne & Patrick) for CMV promotor

µl	type
10	Q5-HF Reaction Buffer
1	Template: 405
2,5	oIG6000
2,5	oIG6001
4	dNTPs
0,5	Q5-HF Polymerase
Add to 50	H₂O

Annealing: 60°C
Extension:

PCR of construct 405 (Anne & Patrick) for GFP

µl	type
10	Q5-HF Reaction Buffer
1	Template: 405
2,5	oIG6002
2,5	oIG6003
4	dNTPs
0.5	Q5-HF Polymerase
Add to 50	H₂O

Annealing: 60°C
Extension:

6.6.13

Gelelectrophoresis of PCR products (5.6.13)

Gelextraction

name	ng/µl
GFP (405)	88
CMV (405)	98
Terminator	36
pSB1C3 05 (old)	26,7

Gibson

µl	type
0,92	pSB1C3
0,9	GFP
0,66	CMV
0,47	Terminator
2,06	H₂O

1 h,50 °C
3 min. RT
3 min, 4 °C
4 µl Transformation

7.6.13

Testdigest:

µl	type
1 and 2	DNA
1	NEB-Buffer 4
0.5	EcoRI
0.5	BamHI
Add to 10 µl	H₂O

Temp.: 37°C
Incubation time: 1,5h

PCR of eCFP

µl	type
10	Q5-HF Reaction Buffer
1	Template: Pal113 (eCFP)
2,5	oIG6025
2,5	oIG6002
4	dNTPs
0,5	Q5-HF Polymerase
Add to 50	H₂O

Annealing: 60°C
Extension:

PCR of bgh Terminator

µl	type
10	Q5-HF Reaction Buffer
1	Template: pMH (bgh terminator)
2,5	oIG6022
2,5	oIG6023
4	dNTPs
0,5	Q5-HF Polymerase
Add to 50	H₂O

Annealing: 60°C
Extension:20sec

10.6.13

Repetition of PCR of eCFP

temperature gradient: 48°C - 60°C

µl	type
10	Q5-HF Reaction Buffer
1	Template: Pal113 (eCFP)
2,5	oIG6002
2,5	oIG6003
4	dNTPs
1,5	DMSO
0,5	Q5-HF Polymerase
Add to 50	H₂O

Tube	temperature [°C]
1	48
2	50
3	51,4
4	52,9
5	56,4
6	58,7
7	60

Sequencing of Minipreps of pIG6000 (1 & 2) (8.6.13)

Gibson: CMV, GFP (405), bgh (105) and pSB1C3

µl	type
0,92	pSB1C3
0,9	GFP
0,66	CMV
0,56	bgh Terminator
add to 5 µl	H₂O

1 h,50°C
3 min. RT
3 min,°C
4 µl Transformation

Gibson: CMV (405), eCFP (Pal113), bgh (105) and pSB1C3

µl	type
0,92	pSB1C3
1,36	eCFP
0,66	CMV
0,56	bgh Terminator
add to 5 µl	H₂O

1 h,50°C
3 min. RT
3 min, 4°C
4 µl Transformation

11.6.13

Gibson has worked: 6 colonies for minipreps

Testdigest: Gibson (6.6.13)

µl	type
1	DNA
1	NEB-Buffer 4
0.5	NdeI
0.5	XhoI
Add to 10 µl	H₂O

Temp.: 37°C
Incubation time: 1,5h

the testdigest showd as expected 3 bands (896bp, 389bp ans 2517bp) Bands of clone 8 seemed to be right and we sent it for sequenzing (primer: 17, 18)

12.6.13

Sequnecing of clone 8 containing CFP were unclear. to test if the two plasmid are functional they were transfected into CHO cells. therefore 750ng DNA of each mini-prep were transfected per well in a 48 well plate.

13.6.13

In parallel to the transfection test a testdigest of piG6000 and piG6001 was performed.

Testdigest: piG6000 and piG6001

µl	type
1	DNA
2	NEB-Buffer 4
0.5	NdeI
0.5	XhoI
Add to 10 µl	H₂O

Temp.: 37°C
Incubation time: 1,5h

clone 3 and 4 of piG6000 run as expected and they also show strong fluorescence in the CHO cells. Clone c,d,e and f of piG6001 run higher as expected but they do not show visible flourescence (this might be due to transfecting a mini-prep instead of a midi-prep) Clone 3 of piG6000 and clone e of piG6001 were sequenced

18.13

sequencing results of both constructs are positive.

18.13

midi-prep of pIG600 and retrafo of pIG6001

20.13

CMV min

Idea: making pIG6000 able to be activated by Cas9-VP16. therefore the constitutively active CMV promoter is exchanged by a CMV min. oligos will be designed to target PsB1C3 ao that VP16 can activate the minimal promoter and the cells start to show green fluorescence.

digest of pIG6000

µl	type
10	DNA
5	NEB-Buffer cut smart
2,5	NheI HF
12,5	SacII
Add to 50µl	H₂O

Temp.: 37°C
Incubation time: 1,5h

digest of plasmid of Patrick and Anne (600)

µl	type
10	DNA
5	NEB-Buffer cut smart
2,5	NheI HF
12,5	SacII
Add to 50µl	H₂O

Temp.: 37°C
Incubation time: 1,5h

Bands were as expected:
pIG6000: 631bp and 3154bp. here the higher band was cut out as it is the vector
pIGPanne: 109bo and 2683bp. here the lower, smaler band was cut out as it is the CMVmin prompter. Gel ex was performed

Ligation of pIG6002

µl	type
7	vector
5 ,5	Insert
2	T4 ligase Buffer
1	T4 ligase
Add to 50µl	H₂O

Temp.: 16°C
Incubation time: 1h

Then E.Coli were transformed with 4µl of the ligation.

22.6.13

Mini-preps of pIG6002 were performed

23.13

test digest of pIG6002

µl	type
4	DNA
52	NEB-Buffer cut smart
0,5	NheI HF
0,5	SacII
Add to 20µl	H₂O

Temp.: 37°C
Incubation time: 1,5h

all 6 digested mini showed the same positive result! therefore the CMVmin project is accomplished

@@ Line 1: / Line 1: @@
 {{:Template:Freiburg2013_Template1}}
+{{:Template:Freiburg2013_Template2}}
@@ Line 41: / Line 42: @@
 </p>
-<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/lab_effector"> Effector </a></p>
-<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/induction"> Induction </a> </p>
-<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/crrna"> Targeting </a></p>
-<p class="second_order"> <a id="link" href="https://2013.igem.org/Team:Freiburg/Notebook/lab_multiple_targeting"> Multiple targeting </a> </p>
+<p class="first_order"><a class="active" href="https://2013.igem.org/Team:Freiburg/Notebook/crrna"> Targeting </a></p>
-<p class="second_order"> <a id="link" href="https://2013.igem.org/Team:Freiburg/Notebook/lab_gfp_reporter"> GFP-Reporter-Plasmid </a> </p>
+<p class="second_order_note"> <a id="link" href="https://2013.igem.org/Team:Freiburg/Notebook/lab_multiple_targeting"> Multiple targeting </a> </p>
+<p class="second_order_note"> <a id="link" href="https://2013.igem.org/Team:Freiburg/Notebook/lab_crrna_plasmid"> crRNA-Plasmid </a> </p>
+<p class="second_order_note"> <a class="active" id="link" href="https://2013.igem.org/Team:Freiburg/Notebook/lab_gfp_reporter"> GFP-reporter-plasmid </a> </p>
-<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/method"> uniBAss </a></p>
+<p class="third_order"> <a href="#may"> May </a> </p>
+<p class="third_order"> <a href="#june" > June </a> </p>
+<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/lab_effector"> Effector </a></p>
+<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/induction"> Effector Control </a> </p>
 <p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/modeling"> Modeling </a></p>
-<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/standardisation"> Standardisation </a></p>
+<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/method"> uniBAss </a></p>
+<p class="first_order"><a href="https://2013.igem.org/Team:Freiburg/Notebook/standardisation"> Standardization </a></p>
+<p class="first_order"> <a id="link" href="https://2013.igem.org/Team:Freiburg/protocols"> Material and Methods </a> </p>
@@ Line 62: / Line 67: @@
 ********************************************** -->
-<div id="main_contant" style="height:500px;">
+<div id="main_contant_note">
@@ Line 69: / Line 74: @@
 </div>
+<div id="may">
+<p id="h2">
+May
+</p>
+</div>
+<div id="tag">
+	<h2> 03. May 2013 </h2>
+	<h3> Testdigest of pSB1C3 backbone </h3>
+	<p> As a source plasmid to get the pSB1C3 backbone we used a
+biobrick called BBa_K515107
+	</p>
+	<h4> Approach of test digest: </h4>
+	<table border="1">
+	<tbody>
+		<tr>
+			<th> &micro;l </th>
+		</tr>
+		<tr>
+			<td> 2 </td>
+			<td> BBa_K515107 </td>
+		</tr>
+		<tr>
+			<td> 2 </td>
+			<td> NEB Buffer 4 (10X) </td>
+		</tr>
+		<tr>
+			<td> 0.5 </td>
+			<td> EcoR1-HF </td>
+		</tr>
+		<tr>
+			<td> 0.5 </td>
+			<td> Pst1-HF </td>
+		</tr>
+		<tr>
+			<td> 15 </td>
+			<td> H2O </td>
+		</tr>
+  </tbody>
+</table>
+	<h3>PCR 1</h3>
+	<div id="floatleft">
+		<table id="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 25 </td>
+					<td> Q5-HF Mastermix </td>
+				</tr>
+				<tr>
+					<td> 20ng </td>
+					<td> DNA </td>
+				</tr>
+				<tr>
+					<td> 2.5 </td>
+					<td> Primer1 </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> Primer2 </td>
+				</tr>
+				<tr>
+					<td> Add to 50 </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+	<div id="floatright">
+	<ol>
+		<li> CMV-promotor </li>
+		<ul>
+			<li> oIG6000 </li>
+			<li> oIG6001 </li>
+			<li> Temp.: eGFP-Plasmid </li>
+		</ul>
+		<li> GFP </li>
+		<ul>
+			<li> oIG6002 </li>
+			<li> oIG 6003 </li>
+			<li> Temp.: eGFP-Plasmid </li>
+		</ul>
+		<li> Terminator </li>
+		<ul>
+			<li> oIG6004 </li>
+			<li> oIG6005 </li>
+			<li> Temp.: eGFP-Plasmid </li>
+		</ul>
+		<li> CFP </li>
+		<ul>
+			<li> oIG6002 </li>
+			<li> oIG6012 </li>
+			<li> Temp.: CFP M4 Plasmid </li>
+		</ul>
+	</ol>
+<h3>Gel of PCR 1</h3>
+<p>expected length of the fragments: 1. CMV: 685bp 2. eGFP: 824bp
+.terminator: 350bp 4.CFP: 820bp
+bands were not expactly running as expected, but perhaps due to the
+marker. the marker bands are not separated clearly. So the bands were
+cut out and gel ex was performed. Nanodropping after the Gel ex: 1.
+CMV: 156ng/&micro;l 2. eGFP: 143ng/&micro;l 3. terminator:
+ng/&micro;l 4. CFP: 85ng/&micro;l </p>
+</div>
+<div id="tag">
+	<h2> 07. May 3013 </h2>
+	<h3>Fusion PCR 7.5.13</h3>
+	<div id="floatleft">
+		<table id="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> 5x Q5 Buffer&nbsp;</td>
+				</tr>
+				<tr>
+					<td> 4 </td>
+					<td> DNTPs</td>
+				</tr>
+				<tr>
+					<td> 0.5 </td>
+					<td> Q5</td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> CMV </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> eGFP </td>
+				</tr>
+				<tr>
+					<td> 2.5 </td>
+				<td> oIG600 </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6003 </td>
+				</tr>
+				<tr>
+					<td> Add to 50 </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+	<div id="floatright">
+		<table id="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> 5x Q5 Buffer&nbsp;</td>
+				</tr>
+				<tr>
+					<td> 4 </td>
+					<td> DNTPs</td>
+				</tr>
+				<tr>
+					<td> 0.5 </td>
+					<td> Q5</td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> terminator </td>
+				</tr>
+				<tr>
+					<td> 1.5 </td>
+					<td> CFP </td>
+				</tr>
+				<tr>
+					<td> 2.5 </td>
+					<td> oIG602 </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6005 </td>
+				</tr>
+				<tr>
+					<td> Add to 50 </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		<table>
+	</div>
+		<p> additionally a no template control was performed. the PCRs
+were run with Manus PCR programm. 1.30min elongation time.
+		</p>
+		<h3> preperation digest of pSB1C3 </h3>
+		<p> As a source plasmid to get the pSB1C3 backbone we used a
+biobrick called BBa_K515107
+		</p>
+		<h4> Approach of test digest: </h4>
+		<div id="floatleft">
+			<table border="1">
+			<tbody>
+				<tr>
+				<th> &micro;l</th>
+				<th> </th>
+				</tr>
+				<tr>
+					<td> 5 </td>
+					<td> BBa_K515107 </td>
+				</tr>
+				<tr>
+					<td> 5 </td>
+					<td> NEB Buffer 4 (10X) </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> Xba-HF </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> Pst1-HF </td>
+				</tr>
+				<tr>
+					<td> 38 </td>
+					<td> H2O </td>
+				</tr>
+			</tbody>
+			</table>
+			<p>gelbild of fusion PCR and prep digest
+			</p>
+		</div>
+	</div>
+</div>
+<div id="tag">
+<h2> 08. May 3013 </h2>
+<h3>PCR: second try of the first one</h3>
+	<div id="floatleft">
+		<table id="tabelle">
+			<tbody>
+    <tr>
+      <th> &micro;l </th>
+      <th> type </th>
+    </tr>
+    <tr>
+      <td> 10 </td>
+      <td> Q5-Buffer </td>
+    </tr>
+    <tr>
+      <td> 4 </td>
+      <td> DNTPs </td>
+    </tr>
+    <tr>
+      <td> 2 </td>
+      <td> DNA (1:10 diluted) </td>
+    </tr>
+    <tr>
+      <td> 0,5 </td>
+      <td> Q5 </td>
+    </tr>
+    <tr>
+      <td> 2.5 </td>
+      <td> Primer fw </td>
+    </tr>
+    <tr>
+      <td> 2,5 </td>
+      <td> Primer rv </td>
+    </tr>
+    <tr>
+      <td> Add to 50 </td>
+      <td> H<sub>2</sub>O </td>
+    </tr>
+			</tbody>
+		</table>
+	</div>
+<p> the same results as in the first try were obtained and the
+bands were cut out and put in the freezer but a gel ex was never
+performed.
+</p>
+<h3>digest of pSB1C3 (Bba_K32305 and Bba_K32380)</h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+    <tr>
+      <th> &micro;l </th>
+      <th> type </th>
+    </tr>
+    <tr>
+      <td> 2 </td>
+      <td> DNA </td>
+    </tr>
+    <tr>
+      <td> 5 </td>
+      <td> NEB-Buffer 4 </td>
+    </tr>
+    <tr>
+      <td> 1 </td>
+      <td> Xba1 </td>
+    </tr>
+    <tr>
+      <td> 1 </td>
+      <td> Pst1 </td>
+    </tr>
+    <tr>
+      <td> Add to 50&micro;l </td>
+      <td> H<sub>2</sub>O </td>
+    </tr>
+			</tbody>
+		</table>
+	</div>
+	<div id="floatright">
+<ul>
+  <li> Temp.: 37&deg;C </li>
+  <li> Incubation time: 2h </li>
+</ul>
+	</div>
+<p> length of backbone: 2070bp. insert that is cut out: 1274bp
+(...80). Bands on gel as expected.
+</p>
+</div>
+<div id="tag">
+	<h2> 10.05.13 </h2>
+	<h3> Fusion PCR </h3>
+	<h4> 1. CMV+eGFP </h4>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> Q5-HF Reaction Buffer </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> CMV </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> eGFP </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6000 </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6003 </td>
+				</tr>
+				<tr>
+					<td> 2.5 </td>
+					<td> dNTPs </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> DMSO </td>
+				</tr>
+				<tr>
+					<td> Add to 50 </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+	<h4>2. CFP+SV40 terminator</h4>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> Q5-HF Reaction Buffer </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> ecfp </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> termin </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6002 </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6005 </td>
+				</tr>
+				<tr>
+					<td> 2.5 </td>
+					<td> dNTPs </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> DMSO </td>
+				</tr>
+				<tr>
+					<td> Add to 50 </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+	<h4>3. eGFP+ SV40 terminator</h4>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> Q5-HF Reaction Buffer </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> termin </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> eGFP </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6002 </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> oIG6005 </td>
+				</tr>
+				<tr>
+					<td> 2.5 </td>
+					<td> dNTPs </td>
+				</tr>
+				<tr>
+					<td> 1 </td>
+					<td> DMSO </td>
+				</tr>
+				<tr>
+					<td> Add to 50 </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+	<div id="floatright">
+		<ul>
+			<li> Annealing: 60&deg;C </li>
+			<li> Extension:40s </li>
+		</ul>
+</div>
+</div>
+<div id="tag">
+<div id="june" style="padding-top:200px">
+<p id="h2">
+June
+</p>
+</div>
+        <h2> 5.6.13 </h2>
+        <h3> PCR of construct 405 (Anne & Patrick) for CMV promotor </h3>
+	<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 10 </td>
+			<td> Q5-HF Reaction Buffer </td>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> Template: 405 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6000 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6001 </td>
+		</tr>
+		<tr>
+			<td> 4 </td>
+			<td> dNTPs </td>
+		</tr>
+		<tr>
+			<td> 0,5 </td>
+			<td> Q5-HF Polymerase </td>
+		</tr>
+		<tr>
+			<td> Add to 50 </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> Annealing: 60&deg;C </li>
+		<li> Extension: </li>
+	</ul>
+	</div>
+	<div>
+<h3> PCR of construct 405 (Anne & Patrick) for GFP </h3>
+	</div>
+		<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 10 </td>
+			<td> Q5-HF Reaction Buffer </td>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> Template: 405 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6002 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6003 </td>
+		</tr>
+		<tr>
+			<td> 4 </td>
+			<td> dNTPs </td>
+		</tr>
+		<tr>
+			<td> 0.5 </td>
+			<td> Q5-HF Polymerase </td>
+		</tr>
+		<tr>
+			<td> Add to 50 </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> Annealing: 60&deg;C </li>
+		<li> Extension: </li>
+	</ul>
+	</div>
+</div>
+<div id="tag">
+        <h2> 6.6.13 </h2>
+        <h3> Gelelectrophoresis of PCR products (5.6.13) </h3>
+<h3> Gelextraction </h3>
+	<table class="tabelle">
+		<tr>
+			<th> name </th>
+			<th> ng/&micro;l </th>
+		</tr>
+		<tr>
+			<td> GFP (405) </td>
+			<td> 88 </td>
+		</tr>
+			<tr>
+			<td> CMV (405) </td>
+			<td> 98 </td>
+		</tr>
+		<tr>
+			<td> Terminator </td>
+			<td> 36 </td>
+		</tr>
+		<tr>
+			<td> pSB1C3 05 (old) </td>
+			<td> 26,7 </td>
+		</tr>
+	</table>
+	<h3> Gibson </h3>
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 0,92 </td>
+			<td> pSB1C3 </td>
+		</tr>
+			<tr>
+			<td> 0,9 </td>
+			<td> GFP </td>
+		</tr>
+		<tr>
+			<td> 0,66 </td>
+			<td> CMV </td>
+		</tr>
+		<tr>
+			<td> 0,47 </td>
+			<td> Terminator </td>
+		</tr>
+		<tr>
+			<td> 2,06 </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	<div id="floatright">
+	<ul>
+		<li> 1 h,50 °C </li>
+		<li> 3 min. RT </li>
+		<li> 3 min, 4 °C </li>
+		<li> 4 µl Transformation </li>
+	</ul>
+	</div>
+	</div>
+<div id="tag">
+        <h2> 7.6.13 </h2>
+	<h3>  Testdigest: </h3>
+	<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 1 and 2 </td>
+			<td> DNA </td>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> NEB-Buffer 4 </td>
+		</tr>
+		<tr>
+			<td> 0.5 </td>
+			<td> EcoRI </td>
+		</tr>
+		<tr>
+			<td> 0.5 </td>
+			<td> BamHI </td>
+		</tr>
+		<tr>
+			<td> Add to 10 &micro;l </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> Temp.: 37&deg;C </li>
+		<li> Incubation time: 1,5h </li>
+	</ul>
+	</div>
+	<h3> PCR of eCFP </h3>
+	<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 10 </td>
+			<td> Q5-HF Reaction Buffer </td>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> Template: Pal113 (eCFP) </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6025 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6002 </td>
+		</tr>
+		<tr>
+			<td> 4 </td>
+			<td> dNTPs </td>
+		</tr>
+		<tr>
+			<td> 0,5 </td>
+			<td> Q5-HF Polymerase </td>
+		</tr>
+		<tr>
+			<td> Add to 50 </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> Annealing: 60&deg;C </li>
+		<li> Extension: </li>
+	</ul>
+	</div>
+	<h3> PCR of bgh Terminator </h3>
+	<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 10 </td>
+			<td> Q5-HF Reaction Buffer </td>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> Template: pMH (bgh terminator) </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6022 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6023 </td>
+		</tr>
+		<tr>
+			<td> 4 </td>
+			<td> dNTPs </td>
+		</tr>
+		<tr>
+			<td> 0,5 </td>
+			<td> Q5-HF Polymerase </td>
+		</tr>
+		<tr>
+			<td> Add to 50 </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> Annealing: 60&deg;C </li>
+		<li> Extension:20sec </li>
+	</ul>
+	</div>
+</div>
+<div id="tag">
+        <h2> 10.6.13 </h2>
+        <h3> Repetition of PCR of eCFP </h3>
+	<div id="floatright">
+	<ul>
+		<li> temperature gradient: 48&deg;C - 60&deg;C </li>
+	</ul>
+	</div>
+	<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 10 </td>
+			<td> Q5-HF Reaction Buffer </td>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> Template: Pal113 (eCFP) </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6002 </td>
+		</tr>
+		<tr>
+			<td> 2,5 </td>
+			<td> oIG6003 </td>
+		</tr>
+		<tr>
+			<td> 4 </td>
+			<td> dNTPs </td>
+		</tr>
+		<tr>
+			<td> 1,5 </td>
+			<td> DMSO </td>
+		</tr>
+		<tr>
+			<td> 0,5 </td>
+			<td> Q5-HF Polymerase </td>
+		</tr>
+		<tr>
+			<td> Add to 50 </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatleft">
+	<table class="tabelle">
+		<tr>
+			<th> Tube </th>
+			<th> temperature [&deg;C] </th>
+		</tr>
+		<tr>
+			<td> 1 </td>
+			<td> 48 </td>
+		</tr>
+		<tr>
+			<td> 2 </td>
+			<td> 50 </td>
+		</tr>
+		<tr>
+			<td> 3 </td>
+			<td> 51,4 </td>
+		</tr>
+		<tr>
+			<td> 4 </td>
+			<td> 52,9 </td>
+		</tr>
+		<tr>
+			<td> 5 </td>
+			<td> 56,4 </td>
+		</tr>
+		<tr>
+			<td> 6 </td>
+			<td> 58,7 </td>
+		</tr>
+		<tr>
+			<td> 7 </td>
+			<td> 60 </td>
+		</tr>
+	</table>
+	</div>
+	<p>Sequencing of Minipreps of pIG6000 (1 & 2) (8.6.13) </p>
+	<h3> Gibson: CMV, GFP (405), bgh (105) and pSB1C3</h3>
+	<div>
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 0,92 </td>
+			<td> pSB1C3 </td>
+		</tr>
+			<tr>
+			<td> 0,9 </td>
+			<td> GFP </td>
+		</tr>
+		<tr>
+			<td> 0,66 </td>
+			<td> CMV </td>
+		</tr>
+		<tr>
+			<td> 0,56 </td>
+			<td> bgh Terminator </td>
+		</tr>
+		<tr>
+			<td> add to 5 µl </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> 1 h,50&deg;C </li>
+		<li> 3 min. RT </li>
+		<li> 3 min,&deg;C </li>
+		<li> 4 µl Transformation </li>
+	</ul>
+	</div>
+	<h3> Gibson: CMV (405), eCFP (Pal113), bgh (105) and pSB1C3</h3>
+	<div>
+	<table class="tabelle">
+		<tr>
+			<th> &micro;l </th>
+			<th> type </th>
+		</tr>
+		<tr>
+			<td> 0,92 </td>
+			<td> pSB1C3 </td>
+		</tr>
+			<tr>
+			<td> 1,36 </td>
+			<td> eCFP </td>
+		</tr>
+		<tr>
+			<td> 0,66 </td>
+			<td> CMV </td>
+		</tr>
+		<tr>
+			<td> 0,56 </td>
+			<td> bgh Terminator </td>
+		</tr>
+		<tr>
+			<td> add to 5 µl </td>
+			<td> H<sub>2</sub>O </td>
+		</tr>
+	</table>
+	</div>
+	<div id="floatright">
+	<ul>
+		<li> 1 h,50&deg;C </li>
+		<li> 3 min. RT </li>
+		<li> 3 min, 4&deg;C </li>
+		<li> 4 µl Transformation </li>
+	</ul>
+	</div>
+</div>
+<div id="tag">
+        <h2> 11.6.13 </h2>
+        <p> Gibson has worked: 6 colonies for minipreps
+		</p>
+	<h3>  Testdigest: Gibson (6.6.13) </h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tr>
+				<th> &micro;l </th>
+				<th> type </th>
+			</tr>
+			<tr>
+				<td> 1  </td>
+				<td> DNA </td>
+			</tr>
+			<tr>
+				<td> 1 </td>
+				<td> NEB-Buffer 4 </td>
+			</tr>
+			<tr>
+				<td> 0.5 </td>
+				<td> NdeI </td>
+			</tr>
+			<tr>
+				<td> 0.5 </td>
+				<td> XhoI </td>
+			</tr>
+			<tr>
+				<td> Add to 10 &micro;l </td>
+				<td> H<sub>2</sub>O </td>
+			</tr>
+		</table>
+	</div>
+	<div id="floatright">
+		<ul>
+			<li> Temp.: 37&deg;C </li>
+			<li> Incubation time: 1,5h </li>
+		</ul>
+	</div>
+	<p> the testdigest showd as expected 3 bands (896bp, 389bp ans 2517bp) Bands of clone 8 seemed to be right and we sent it for sequenzing (primer: 17, 18) </p>
+</div>
+<div id="tag">
+	<h2> 12.6.13 </h2>
+	<p> Sequnecing of clone 8 containing CFP were unclear. to test if the two plasmid are functional they were transfected into CHO cells. therefore 750ng DNA of each mini-prep were transfected per well in a 48 well plate. </p>
+</div>
+<div id="tag">
+	<h2> 13.6.13 </h2>
+	<p> In parallel to the transfection test a testdigest of piG6000 and piG6001 was performed.</p>
+	<h3>  Testdigest: piG6000 and piG6001 </h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tr>
+				<th> &micro;l </th>
+				<th> type </th>
+			</tr>
+			<tr>
+				<td> 1  </td>
+				<td> DNA </td>
+			</tr>
+			<tr>
+				<td> 2</td>
+				<td> NEB-Buffer 4 </td>
+			</tr>
+			<tr>
+				<td> 0.5 </td>
+				<td> NdeI </td>
+			</tr>
+			<tr>
+				<td> 0.5 </td>
+				<td> XhoI </td>
+			</tr>
+			<tr>
+				<td> Add to 10 &micro;l </td>
+				<td> H<sub>2</sub>O </td>
+			</tr>
+		</table>
+	</div>
+	<div id="floatright">
+		<ul>
+			<li> Temp.: 37&deg;C </li>
+			<li> Incubation time: 1,5h </li>
+		</ul>
+	</div>
+	<p> clone 3 and 4 of piG6000 run as expected and they also show strong fluorescence in the CHO cells. Clone c,d,e and f of piG6001 run higher as expected but they do not show visible flourescence (this might be due to transfecting a mini-prep instead of a midi-prep)
+Clone 3 of piG6000 and clone e of piG6001 were sequenced </p>
+</div>
+<div id="tag">
+        <h2> 18.13 </h2>
+		<p>sequencing results of both constructs are positive.
+		</p>
+</div>
+<div id="tag">
+        <h2> 18.13 </h2>
+		<p>midi-prep of pIG600 and retrafo of pIG6001
+		</p>
+</div>
+<div id="tag">
+        <h2> 20.13 </h2>
+		<h3> CMV min </h3>
+		<p>Idea: making pIG6000 able to be activated by Cas9-VP16. therefore the constitutively active CMV promoter is exchanged by a CMV min. oligos will be designed to target PsB1C3 ao that VP16 can activate the minimal promoter and the cells start to show green fluorescence.
+		</p>
+		<h3>digest of pIG6000</h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> DNA </td>
+				</tr>
+				<tr>
+					<td> 5 </td>
+					<td> NEB-Buffer cut smart </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> NheI HF</td>
+				</tr>
+				<tr>
+					<td> 12,5</td>
+					<td> SacII  </td>
+				</tr>
+				<tr>
+					<td> Add to 50&micro;l </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+<ul>
+  <li> Temp.: 37&deg;C </li>
+  <li> Incubation time: 1,5h </li>
+</ul>
+<h3>digest of plasmid of Patrick and Anne (600)</h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 10 </td>
+					<td> DNA </td>
+				</tr>
+				<tr>
+					<td> 5 </td>
+					<td> NEB-Buffer cut smart </td>
+				</tr>
+				<tr>
+					<td> 2,5 </td>
+					<td> NheI HF</td>
+				</tr>
+				<tr>
+					<td> 12,5</td>
+					<td> SacII  </td>
+				</tr>
+				<tr>
+					<td> Add to 50&micro;l </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+<ul>
+  <li> Temp.: 37&deg;C </li>
+  <li> Incubation time: 1,5h </li>
+</ul>
+<p> Bands were as expected:<br>
+pIG6000: 631bp and 3154bp. here the higher band was cut out as it is the vector <br>
+pIGPanne: 109bo and 2683bp. here the lower, smaler band was cut out as it is the CMVmin prompter.
+Gel ex was performed
+<h3>Ligation of pIG6002</h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 7 </td>
+					<td> vector</td>
+				</tr>
+				<tr>
+					<td> 5 ,5</td>
+					<td> Insert </td>
+				</tr>
+				<tr>
+					<td> 2 </td>
+					<td> T4 ligase Buffer</td>
+				</tr>
+				<tr>
+					<td> 1</td>
+					<td> T4 ligase </td>
+				</tr>
+				<tr>
+					<td> Add to 50&micro;l </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+<ul>
+  <li> Temp.: 16&deg;C </li>
+  <li> Incubation time: 1h </li>
+</ul>
+<p>Then E.Coli were transformed with 4&micro;l  of the ligation. </p>
+</div>
+<div id="tag">
+        <h2> 22.6.13 </h2>
+		<p>Mini-preps of pIG6002 were performed
+		</p>
+</div>
+<div id="tag">
+        <h2> 23.13 </h2>
+		<h3>test digest of pIG6002</h3>
+	<div id="floatleft">
+		<table class="tabelle">
+			<tbody>
+				<tr>
+					<th> &micro;l </th>
+					<th> type </th>
+				</tr>
+				<tr>
+					<td> 4 </td>
+					<td> DNA </td>
+				</tr>
+				<tr>
+					<td> 52</td>
+					<td> NEB-Buffer cut smart </td>
+				</tr>
+				<tr>
+					<td> 0,5 </td>
+					<td> NheI HF</td>
+				</tr>
+				<tr>
+					<td> 0,5</td>
+					<td> SacII  </td>
+				</tr>
+				<tr>
+					<td> Add to 20&micro;l </td>
+					<td> H<sub>2</sub>O </td>
+				</tr>
+			</tbody>
+		</table>
+	</div>
+<ul>
+  <li> Temp.: 37&deg;C </li>
+  <li> Incubation time: 1,5h </li>
+</ul>
+<p> all 6 digested mini showed the same positive result! therefore the CMVmin project is accomplished
+</p>