Team:Freiburg/Project/toolkit

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Revision as of 19:11, 29 September 2013

The uniCAS toolkit - Customize your experiments!

You want to have a maximum of activation or repression of your genes by a minimal effort? Then you have to use the uniCAS toolkit provided by the iGEM team Freiburg 2013. All you have to do is:

Click yourself through the routine below
Order the appropriate plasmids and oligos
Conduct a minimal of cloning
Start your personalized experiment

By the end of the routine you will get a personal manual. All you need to use the uniCAS toolkit will be described there. Best of all: The uniCAS toolkit is all open source!

Activation

Repression

Non inducible uniCAS Activator (Cas9-VP16 device)

You have chosen to activate a gene using a non inducible Cas9-VP16 device. Therefore you have to order the following plasmids from the iGEM parts registry . After receiving our plasmids, you will have to clone your target sequence into our crRNA plasmid (protocol see below).

No.	Biobrick	Device	Order	GeneBank File
1	BBa_K1150017	CMV-HA-NLS-Cas9-NLS-BGH	order	genebank
2	BBa_K1150020	CMV-HA-NLS-Cas9-L3-VP16-NLS-BGH	order	genebank
3	BBa_K1150034	crRNA - plasmid	order	genebank

Note:
All plasmids are optimized for expression in mammalian systems. The devices are also available containing an SV40 instead of an CMV promotor (have a look at our parts side). This system was tested mainly in CHO-K1, HEK-293T and HeLa cells.

Design of the crRNA plasmid:

Use our crRNA design tool to design the crRNAs that are needed to target your gene of interest. It will generate possible target sites and the appropriate oligos. Order the oligos by the company of your choice. We recommend to test several different loci to target your gene of interest because the efficiency of different crRNA-loci can differ.

Oligo annealing: Anneal forward and reverse oligo to get the desired crRNA. Therefore mix 10 µl of 100 µM forward Oligo, 10 µl of 100 µM reverse Oligo and 80 µl of ddH2O. Heat the solution to 95° C for 5 minutes. Then turn off the heat block and let the solution cool down.
Digest plasmid BBa_K1150034 with Bbs1: The restriction enzyme Bbs1 should always be stored at -80° C. Mix about 500 ng of BBa_K1150034 with 1 µl of Bbs1, appropriate amount of buffer and fill up to 50 µl with ddH2O. Digest for exact 3 hours at 37° C.
Ligate crRNAs (step 1) into Bbs1 cut backbone: The insert (crRNAs) should be ligated into the backbone in 3 molar insert excess. Therefore use this formular: Required Volume of Insert = 3 x Volume(Backbone) x length(Insert) x concentration (Backbone) / [ length(Backbone) x concentration(Insert) ]. Use about 50 ng Bacbbone. The length of insert is always 30 basepairs. The length of the backbone is 2900 basepairs. You have to mix the appropriate amount of Backbone and the appropriate amount of Insert with 1 µl of T4 Ligase and 2 µl of 10xT4 ligase buffer. Then fill up to 20 µl with ddH2O. This mix should incubate for 30 minutes at room temperature.
Transform 3-5 µl of the mix following standard protocol. Pick clones, miniprep the plasmids and sequence it with pSB1C3 reverse sequencing primer (sequence: CGCCTTTGAGTGAGCTGATACCGC).

Now that you have created the desired crRNA plasmids it is possible to use them indiviually or fuse different crRNA loci together into one crRNA plasmid (recommended).

Design of a multiple target crRNA plasmid:

It is shown that multiple targeting of one gene of interest increases the efficiency of regulation. If you want to fuse different crRNA loci together into one plasmid use the following protocol:

Digest first crRNA plasmid with XXX and XXX. This is your backbone. Therefore mix about 500 ng Backbone with 1 µl Enzyme 1 and 1 µl Enzyme 2, add an appropriate amount of compatible buffer and fill up to approximate 30-50 µl. Incubate mix at 37° C for 2 hours.
Digest second crRNA plasmid with XXX and XXX. This is your insert (procedure see above).
Ligate the insert in 3 molar excess into the backbone (formular see paragraph above).
Transform 3-5 µl of the mix following standard protocol. Pick clones, miniprep the plasmids and sequence it with pSB1C3 forward sequencing primer (sequence: GAGTGCCACCTGACGTCTAAGAAAC) and pSB1C3 reverse sequencing primer (sequence: CGCCTTTGAGTGAGCTGATACCGC).

Experimental design (recommendation for mammalian cell culture):

Transfect BBa_K1150020 with all desired crRNA plasmids (seperate crRNA plasmid and/or multiple crRNAs plasmid)
Non-effector control: Transfect the appropriate crRNA - plasmid togehter with BBa_K1150017 that has no effector.
Off target control: Transfect BBa_K1150020 without any crRNA plasmid.

@@ Line 588: / Line 588: @@
 functional tests of the different activation effectors. </p>
-<label><input id="rdb4" type="radio" name="toggler_two" value="3" onClick="pageScroll()"/>VP16
+<label><input id="rdb4" type="radio" name="toggler_two" value="3" onClick="pageScroll()"/>VP16 (recommended) </label>
+<!-- <label><input id="rdb5" type="radio" name="toggler_two" value="4" onClick="pageScroll()"/> ?????? </label> -->
-(recommended) </label>
-<!-- <label><input id="rdb5" type="radio" name="toggler_two" value="4" onClick="pageScroll()"/>
-?????? </label> -->
 </div>
@@ Line 599: / Line 595: @@
 <img src="https://static.igem.org/mediawiki/2013/d/da/Repression.png">
 <p> Effectively repress your genes using KRAB or G9a as functional effector. </p>
-<label><input id="rdb4" type="radio" name="toggler_two" value="5" onClick="pageScroll()"/>KRAB
+<label><input id="rdb4" type="radio" name="toggler_two" value="5" onClick="pageScroll()"/>KRAB </label>
+<label><input id="rdb5" type="radio" name="toggler_two" value="6" onClick="pageScroll()"/> G9A </label>
-</label>
-<label><input id="rdb5" type="radio" name="toggler_two" value="6" onClick="pageScroll()"/> G9A
-</label>
 </div>
@@ Line 616: / Line 608: @@
 <img src="https://static.igem.org/mediawiki/2013/6/6e/Activation.png"> <img src="">
 <p> Effectively activate your genes using VP16 as functional effector. </p>
-<label><input id="rdb4" type="radio" name="toggler_three" value="7" onClick="pageScroll()"/> No
+<label><input id="rdb4" type="radio" name="toggler_three" value="7" onClick="pageScroll()"/> No Induction </label>
+<label><input id="rdb5" type="radio" name="toggler_three" value="8" onClick="pageScroll()"/> Red light induction </label>
-Induction </label>
+<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="9" onClick="pageScroll()"/> Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="8" onClick="pageScroll()"/> Red
+<label><input id="rdb5" type="radio" name="toggler_three" value="10" onClick="pageScroll()"/> UV light induction </label>
-light induction </label>
-<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="9" onClick="pageScroll()"/>
-Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="10" onClick="pageScroll()"/> UV
-light induction </label>
 </div>
@@ Line 633: / Line 617: @@
 <img src="https://static.igem.org/mediawiki/2013/6/6e/Activation.png"> <img src="">
 <p> Effectively repress your genes using KRAB as functional effector. </p>
-<label><input id="rdb4" type="radio" name="toggler_three" value="11" onClick="pageScroll()"/> No
+<label><input id="rdb4" type="radio" name="toggler_three" value="11" onClick="pageScroll()"/> No Induction </label>
+<label><input id="rdb5" type="radio" name="toggler_three" value="12" onClick="pageScroll()"/> Red light induction </label>
-Induction </label>
+<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="13" onClick="pageScroll()"/> Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="12" onClick="pageScroll()"/> Red
+<label><input id="rdb5" type="radio" name="toggler_three" value="14" onClick="pageScroll()"/> UV light induction </label>
-light induction </label>
-<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="13" onClick="pageScroll()"/>
-Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="14" onClick="pageScroll()"/> UV
-light induction </label>
 </div>
@@ Line 650: / Line 626: @@
 <img src="https://static.igem.org/mediawiki/2013/6/6e/Activation.png"> <img src="">
 <p> Effectively repress your genes using KRAB as functional effector. </p>
-<label><input id="rdb4" type="radio" name="toggler_three" value="15" onClick="pageScroll()"/> No
+<label><input id="rdb4" type="radio" name="toggler_three" value="15" onClick="pageScroll()"/> No Induction </label>
+<label><input id="rdb5" type="radio" name="toggler_three" value="16" onClick="pageScroll()"/> Red light induction </label>
-Induction </label>
+<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="17" onClick="pageScroll()"/> Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="16" onClick="pageScroll()"/> Red
+<label><input id="rdb5" type="radio" name="toggler_three" value="18" onClick="pageScroll()"/> UV light induction </label>
-light induction </label>
-<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="17" onClick="pageScroll()"/>
-Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="18" onClick="pageScroll()"/> UV
-light induction </label>
 </div>
@@ Line 667: / Line 635: @@
 <img src="https://static.igem.org/mediawiki/2013/6/6e/Activation.png"> <img src="">
 <p> Effectively repress your genes using G9a as functional effector. </p>
-<label><input id="rdb4" type="radio" name="toggler_three" value="19" onClick="pageScroll()"/> No
+<label><input id="rdb4" type="radio" name="toggler_three" value="19" onClick="pageScroll()"/> No Induction </label>
+<label><input id="rdb5" type="radio" name="toggler_three" value="20" onClick="pageScroll()"/> Red light induction </label>
-Induction </label>
+<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="21" onClick="pageScroll()"/> Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="20" onClick="pageScroll()"/> Red
+<label><input id="rdb5" type="radio" name="toggler_three" value="22" onClick="pageScroll()"/> UV light induction </label>
-light induction </label>
-<!-- <label><input id="rdb5" type="radio" name="toggler_three" value="21" onClick="pageScroll()"/>
-Blue light induction </label> -->
-<label><input id="rdb5" type="radio" name="toggler_three" value="22" onClick="pageScroll()"/> UV
-light induction </label>
 </div>
@@ Line 699: / Line 659: @@
 			<p>
-			You have chosen to activate a gene using a non inducible Cas9-VP16 device.
+			You have chosen to activate a gene using a non inducible Cas9-VP16 device. Therefore you have to order the following plasmids from the <a id="link" href="http://parts.igem.org/Main_Page"> iGEM parts registry </a>. After receiving our plasmids, you will have to clone your target sequence into our crRNA plasmid (protocol see below).
-Therefore you have to order the following plasmids from the <a id="link" href="http://parts.igem.org/Main_Page"> iGEM parts registry </a>. After receiving our plasmids, you will have to clone your target sequence into our crRNA plasmid (protocol see below).
 			</p>
@@ Line 716: / Line 674: @@
 					<td> BBa_K1150017 </td>
 					<td> CMV-HA-NLS-Cas9-NLS-BGH </td>
-					<td> <a id="link"
+					<td> <a id="link" href="http://parts.igem.org/partsdb/get_part.cgi?part=BBa_K1150017"> order </a> </td>
-href="http://parts.igem.org/partsdb/get_part.cgi?part=BBa_K1150017"> order </a> </td>
 					<td> <a id="link" href=""> genebank </a> </td>
 				</tr>
@@ Line 725: / Line 681: @@
 					<td> BBa_K1150020 </td>
 					<td> CMV-HA-NLS-Cas9-L3-VP16-NLS-BGH </td>
-					<td> <a id="link"
+					<td> <a id="link" href="http://parts.igem.org/partsdb/get_part.cgi?part=BBa_K1150020"> order </a> </td>
-href="http://parts.igem.org/partsdb/get_part.cgi?part=BBa_K1150020"> order </a> </td>
 					<td> <a id="link" href=""> genebank </a> </td>
 				</tr>
@@ Line 734: / Line 688: @@
 					<td> BBa_K1150034 </td>
 					<td> crRNA - plasmid </td>
-					<td> <a id="link"
+					<td> <a id="link" href="http://parts.igem.org/partsdb/get_part.cgi?part=BBa_K1150034"> order </a> </td>
-href="http://parts.igem.org/partsdb/get_part.cgi?part=BBa_K1150034"> order </a> </td>
 					<td> <a id="link" href=""> genebank </a> </td>
 				</tr>
@@ Line 746: / Line 698: @@
 			<p>
 			Note: <br>
-			All plasmids are optimized for expression in mammalian systems. The devices are also available
+			All plasmids are optimized for expression in mammalian systems. The devices are also available containing an SV40 instead of an CMV promotor (have a look at our <a id="link" href="https://2013.igem.org/Team:Freiburg/parts"> parts </a> side). This system was tested mainly in CHO-K1, HEK-293T and HeLa cells.
-containing an SV40 instead of an CMV promotor (have a look at our <a id="link" href="https://2013.igem.org/Team:Freiburg/parts"> parts </a> side). This system was tested mainly in CHO-K1, HEK-293T and HeLa cells.
 			</p>
@@ Line 760: / Line 711: @@
 			<ol>
-				<li> <b>Oligo annealing:</b> Anneal forward and reverse oligo to get the
+				<li> <b>Oligo annealing:</b> Anneal forward and reverse oligo to get the desired crRNA. Therefore mix 10 µl of 100 µM forward Oligo, 10 µl of 100 µM reverse Oligo and 80 µl of ddH2O. Heat the solution to 95° C for 5 minutes. Then turn off the heat block and let the solution cool down.</li>
+				<li> <b>Digest plasmid BBa_K1150034 with Bbs1:</b> The restriction enzyme Bbs1 should always be stored at -80° C. Mix about 500 ng of BBa_K1150034 with 1 µl of Bbs1, appropriate amount of buffer and fill up to 50 µl with ddH2O. Digest for exact 3 hours at 37° C.
-desired crRNA. Therefore mix 10 µl of 100 µM forward Oligo, 10 µl of 100 µM reverse Oligo and 80
-µl of ddH2O. Heat the solution to 95° C for 5 minutes. Then turn off the heat block and let the
-solution cool down.</li>
-				<li> <b>Digest plasmid BBa_K1150034 with Bbs1:</b> The restriction enzyme
-Bbs1 should always be stored at -80° C. Mix about 500 ng of BBa_K1150034 with 1 µl of Bbs1,
-appropriate amount of buffer and fill up to 50 µl with ddH2O. Digest for exact 3 hours at 37° C.
 </li>
-				<li> <b>Ligate crRNAs (step 1) into Bbs1 cut backbone:</b> The insert
+				<li> <b>Ligate crRNAs (step 1) into Bbs1 cut backbone:</b> The insert (crRNAs) should be ligated into the backbone in 3 molar insert excess. Therefore use this formular: Required Volume of Insert = 3 x Volume(Backbone) x length(Insert) x concentration (Backbone) / [ length(Backbone)  x concentration(Insert) ]. Use about 50 ng Bacbbone. The length of insert is always 30 basepairs. The length of the backbone is 2900 basepairs. You have to mix the appropriate amount of Backbone and the appropriate amount of Insert with 1 µl of T4 Ligase and 2 µl of 10xT4 ligase buffer. Then fill up to 20 µl with ddH2O. This mix should incubate for 30 minutes at room temperature.</li>
+				<li> <b>Transform</b> 3-5 µl of the mix following standard protocol. Pick clones, miniprep the plasmids and sequence it with pSB1C3 reverse sequencing primer (sequence: CGCCTTTGAGTGAGCTGATACCGC).</li>
-(crRNAs) should be ligated into the backbone in 3 molar insert excess. Therefore use this
-formular: Required Volume of Insert = 3 x Volume(Backbone) x length(Insert) x concentration
-(Backbone) / [ length(Backbone)  x concentration(Insert) ]. Use about 50 ng Bacbbone. The length
-of insert is always 30 basepairs. The length of the backbone is 2900 basepairs. You have to mix
-the appropriate amount of Backbone and the appropriate amount of Insert with 1 µl of T4 Ligase and
-µl of 10xT4 ligase buffer. Then fill up to 20 µl with ddH2O. This mix should incubate for 30
-minutes at room temperature.</li>
-				<li> <b>Transform</b> 3-5 µl of the mix following standard protocol. Pick
-clones, miniprep the plasmids and sequence it with pSB1C3 reverse sequencing primer (sequence:
-CGCCTTTGAGTGAGCTGATACCGC).</li>
 			</ol>
 			<p>
-			Now that you have created the desired crRNA plasmids it is possible to use
+			Now that you have created the desired crRNA plasmids it is possible to use them indiviually or fuse different crRNA loci together into one crRNA plasmid (recommended).
-them indiviually or fuse different crRNA loci together into one crRNA plasmid (recommended).
@@ Line 808: / Line 729: @@
 			</p>
-			<p>It is shown that multiple targeting of one gene of interest <a
+			<p>It is shown that multiple targeting of one gene of interest <a id="link" href="https://2013.igem.org/Team:Freiburg/Project/crrna#multiple_targeting">increases the efficiency of regulation</a>. If you want to fuse different crRNA loci together into one plasmid use the following protocol:
-id="link" href="https://2013.igem.org/Team:Freiburg/Project/crrna#multiple_targeting">increases the
-efficiency of regulation</a>. If you want to fuse different crRNA loci together into one plasmid
-use the following protocol:
 			</p>
 			<ol>
-				<li> <b>Digest first crRNA plasmid</b> with XXX and XXX. This is your
+				<li> <b>Digest first crRNA plasmid</b> with XXX and XXX. This is your backbone. Therefore mix about 500 ng Backbone with 1 µl Enzyme 1 and 1 µl Enzyme 2, add an appropriate amount of compatible buffer and fill up to approximate 30-50 µl. Incubate mix at 37° C for 2 hours. </li>
+				<li> <b>Digest second crRNA plasmid</b> with XXX and XXX. This is your insert (procedure see above).</li>
-backbone. Therefore mix about 500 ng Backbone with 1 µl Enzyme 1 and 1 µl Enzyme 2, add an
+				<li> <b>Ligate</b> the insert in 3 molar excess into the backbone (formular see paragraph above).
+				<li> <b>Transform</b> 3-5 µl of the mix following standard protocol. Pick clones, miniprep the plasmids and sequence it with pSB1C3 forward sequencing primer (sequence: GAGTGCCACCTGACGTCTAAGAAAC) and pSB1C3 reverse sequencing primer (sequence: CGCCTTTGAGTGAGCTGATACCGC).</li>
-appropriate amount of compatible buffer and fill up to approximate 30-50 µl. Incubate mix at 37° C
-for 2 hours. </li>
-				<li> <b>Digest second crRNA plasmid</b> with XXX and XXX. This is your
-insert (procedure see above).</li>
-				<li> <b>Ligate</b> the insert in 3 molar excess into the backbone
-(formular see paragraph above).
-				<li> <b>Transform</b> 3-5 µl of the mix following standard protocol. Pick
-clones, miniprep the plasmids and sequence it with pSB1C3 forward sequencing primer (sequence:
-GAGTGCCACCTGACGTCTAAGAAAC) and pSB1C3 reverse sequencing primer (sequence:
-CGCCTTTGAGTGAGCTGATACCGC).</li>
 			</ol>
 			</div>
@@ Line 843: / Line 742: @@
 			</p>
 			<ol>
-				<li> <b>Transfect</b> BBa_K1150020 with all desired crRNA plasmids
+				<li> <b>Transfect</b> BBa_K1150020 with all desired crRNA plasmids (seperate crRNA plasmid and/or multiple crRNAs plasmid) </li>
+				<li> <b>Non-effector control:</b> Transfect the appropriate crRNA - plasmid togehter with BBa_K1150017 that has no effector.</li>
-(seperate crRNA plasmid and/or multiple crRNAs plasmid) </li>
+				<li> <b>Off target control:</b> Transfect BBa_K1150020 without any crRNA plasmid.</li>
-				<li> <b>Non-effector control:</b> Transfect the appropriate crRNA -
-plasmid togehter with BBa_K1150017 that has no effector.</li>
-				<li> <b>Off target control:</b> Transfect BBa_K1150020 without any crRNA
-plasmid.</li>
@@ Line 859: / Line 752: @@
 	</div>
-	<img src="https://static.igem.org/mediawiki/2013/6/62/Toolbox_back_bottom_freiburg_13.png"
+	<img src="https://static.igem.org/mediawiki/2013/6/62/Toolbox_back_bottom_freiburg_13.png" style="width:850px; margin-top:-2px;">
-style="width:850px; margin-top:-2px;">
 </div>
@@ Line 874: / Line 765: @@
 <div id="check-10" class="toHide3" style="display:none">
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