Team:Toronto/Notebook

From 2014.igem.org

(Difference between revisions)

Latest revision as of 01:47, 18 October 2014

Week 1
- picked single MG1655 and pTRC99A strains into liquid culture, incubated overnight (pTRC99A in LB+Amp)
- prepped DNA for transformation – pCas9 and RFP reporter
- made MG1655 electrocompetent – electroporate and plated transformants, incubated overnight
Week 2
- transformation of RFP, pCas9, GFP, fmt into NEB5alpha
- overnight culture of MG1655 and pTRC99A
- Miniprepped RFP and pTRC99A
- O/N cultures of RFP, pCas9, GFP from transformation
- miniprep of O/N cultures of transformants and pTRC99A
Week 3
- miniprep again, greater volume (3mL) for RFP, GFP, Cas9, pTRC99A + nanodrop
- O/N culture from plate of extra biobrick, RFP, MG1655
- start RFP and MG1655 liquid cultures for the RFP spectrum measurements in the afternoon
- digest 8 samples from yesterday’s miniprep of 8 biobrick cultures, load and run gel of digest
- oligos and gblocks arrived
- did PCR of pCas9 and pTRC99A chunks
- Started MG1655 liquid culture for making chemically competent
Week 4
- miniprepped pCas9 + pTRC99A (w 7mL of cells)
- did gel extraction – cut out pCas9 + pTRC digests – PCR both as well as nanodrop
- Mon/Tues = PCR w mastermix, Wed = make comp MG1655 and heatshock RFP, Thurs/Fri = confirm RFP and Marafini protocol/golden-gate assembly
Week 5
- Wed. minipreps were good (however possibly from just high free nucleotides), gel extraction failed (no DNA at the end and a lot of salt contamination) – so just PCR from miniprepped plasmids
- digest and run gel of digest at the same time!
- if PCR worked, digest PCR product w DpnI – got nothing for pCas9 though on the gel (to be re-PCR-ed), but bright bands for pTRC
- competent MG1655 also done
- PCR of miniprep C1 #1 of cas9… did 10 x 10uL reaction using gradient temps in 58-68 range
- heat shock transformation for MG1655 w RFP plasmid but very few colonies on CM plate
Week 6
- PCR product (???) run on gel, pick most successful PCR
- DpnI digest following protocol in NEB Gibson manual Transform RFP & MG1655, O/N cultures
- pCas9PCR product visible on gel
- DpnI digest + PCR cleanup of digest (ended up not having enough DNA)
- plating of transformed RFP into DH5a
- processed PCR – ran on gel, DpnI digest also ran on gel, PCR cleanup, nanodrop (worked well)
- needed to transform pCas9+spacer plasmid & RFP DH5a
Week 7/8
- transform RFP & BL21(DE3)
- PCR of pCas9, pTRC99A
- Gibson – pick 8 colonies, make O/N colonies, try to PCR form reaction to get 4-fragment superchunk
- Maraffini – use Anderson high for 4 fragment (phosphorylation + annealing of spacers if we get a lot of DNA), otherwise using Aug 18 miniprep do a BsaI digest
- 3 things in parallel:
- look at plates from transformation, run E+P digests on gel – if the digests look wrong size, do colony PCR on rest of Gibson colonies on plates
- try a gel-extraction protocol…
Week 9
- Main thing – GIBSON ASSEMBLY
- screened 8 colonies – miniprepped, EcoRI + PstI digest & wrong product, non-specific assembly
- did digests of plasmids w one restriction enzyme instead of double digest + run gel (for less confusing results) – used miniprep #1-4
- made O/N cultures from first Gibson reaction #9-15 – miniprepped and streak out plates
- minipreps #5-8 from earlier digested w EcoRI and PstO (separately), run on gel
- take 2 minipreps, do 3 reactions on each – EcoRI only, PstI only, both EcoRI + PstI
Week 10
- miniprep out RFP plasmid to be used for putting biobricks into pSB1C3, will want to screen for non-red colonies at the end of the process
- unable to do digest because nanoprep of all 3 minipreps was too low
- primers arrived – ran PCR w new primers
- ran the original gblocks w extended gblocks – not enough of original gblocks to show up on gel
- combined PCR reactions of tracr gblocks into one, same with Anderson High PCR products
- glycerol stocked 3 tubes of colonies from first Gibson attempt (#3, 4, 7)
- transformed Gibson in NEB5alpha, ½ of each reaction tube into a total of 4 NEB5alpha – 4 tubes plated onto 2 plates each = total 8 plates incubated
- on Friday, found colonies from the Gibson assembly and did colony PCR
- colony PCR primers were designed to cover the seams where the 4 chunks joined
- mixed the template DNA and biobrick primers for the Cas9-array chunk, but did not add the master mix yet (done later)
Week 11
- ran Gibson colony PCR on gel – colonies #3 + 6 have correct bands, started O/N cultures of them w cell suspensions from colony PCR
- miniprep and glycerol stock them (low copy plasmid – do 3uL miniprep)
- PCR of cas9 chunk – run on gel, see if band is at 4595
- using RFP miniprep from earlier, digest w EcoRI and PstI
- nothing on gel at correct size…. only used 1uL of DNA for gel though
- digest ~1000ng of Gibson miniprep from 2 colonies w EcoRI and PstI, run on gel
- run 5uL of tube labelled C6*
- cas9-array chunk biobrick extension PCR barely worked – not enough DNA after PCR purification but tracr chunk biobrick PCR worked
- transformed ligation into NEB5alpha – after 2 hour (actual = 10 min) incubation in SOB, pipetted into 2mL LB Cm and grew overnight
- miniprepped to see if it grew and packed it up for shipping!

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+{{Templates/head}}
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+<div id="bg"></div>
+<div id="splash-wrapper">
+	<section id="splash" style="position:absolute;">
+		<div class="container">
+			<!--<h1><span>Biocontainment: a novel approach</span></h1>-->
+		</div>
+	</section>
+	<nav>
+		<div class="container" style="position:relative;">
+			<ul id="navbar">
+                                <div id="tabs" style="display:inline-block; width:80%; position:absolute; bottom:0;">
+				<li id="home">
+					<a href='https://2014.igem.org/Team:Toronto#navbar' scroll-on-click><i class="fa fa-home"></i>Home</a>
+				</li>
+				<li id="team">
+					<a href='https://2014.igem.org/Team:Toronto/Team#navbar' scroll-on-click><i class="fa fa-users"></i> Team</a>
+				</li>
+				<li id="project">
+					<a href='https://2014.igem.org/Team:Toronto/Project#navbar' scroll-on-click><i class="fa fa-gears"></i> Project</a>
+				</li>
+				<li id="parts">
+					<a href='https://2014.igem.org/Team:Toronto/Parts#navbar' scroll-on-click><i class="fa fa-wrench"></i> Parts</a>
+				</li>
+				<li id="modeling">
+					<a href='https://2014.igem.org/Team:Toronto/Modeling#navbar' scroll-on-click>
+<i class="fa fa-bar-chart"></i> Modeling</a>
+				</li>
+				<li class="active" id="notebook">
+					<a href='https://2014.igem.org/Team:Toronto/Notebook#navbar' scroll-on-click><i class="fa fa-book"></i> Notebook</a>
+				</li>
+                                 <li id="humanpractices">
+					<a href='https://2014.igem.org/Team:Toronto/HumanPractices#navbar' scroll-on-click><i class="fa fa-child"></i> Human Practices</a>
+				</li>
+				<li id="safety">
+					<a href='https://2014.igem.org/Team:Toronto/Safety#navbar' scroll-on-click><i class="fa fa-exclamation-triangle"></i> Safety</a>
+				</li>
+				<li id="attributions">
+					<a href='https://2014.igem.org/Team:Toronto/Attributions#navbar' scroll-on-click><i class="fa fa-asterisk"></i> Attributions</a>
+				</li>
+                                <div style="clear:both;"></div>
+                                </div>
+			        <div id="igemlogo" style="display:inline-block; float:right;">
+                            <a href="2014.igem.org"><img style="height:100px;" src="https://static.igem.org/mediawiki/2014/8/84/Igemlogo_300px2.png"> </a>
+                        </div>
+                             </ul>
+		</div>
+	</nav>
+</div>
-<!--main content -->
+<section id="main">
-<table width="70%" align="center">
+	<div id="main-inner">
+		<div id="view" ng-view data-autoscroll="true">
+<div class="first container-wrapper">
-<!--welcome box -->
+	<div class="container">
-<tr>
+		<ul>
-<td style="border:1px solid black;" colspan="3" align="center" height="150px" bgColor=#FF404B>
+	<li class="week">
-<h1 >WELCOME TO iGEM 2014! </h1>
+		<h2><span>Week 1</span></h2>
-<p>Your team has been approved and you are ready to start the iGEM season!
+		<ul class="thingsdone">
-<br>On this page you can document your project, introduce your team members, document your progress <br> and share your iGEM experience with the rest of the world! </p>
+			<li>
-<br>
+				picked single MG1655 and pTRC99A strains into liquid culture,
-<p style="color:#E7E7E7"> <a href="https://2014.igem.org/wiki/index.php?title=Team:Toronto/Notebook&action=edit"style="color:#FFFFFF"> Click here  to edit this page!</a> </p>
+				incubated overnight (pTRC99A in LB+Amp)
-</td>
+			</li>
-</tr>
+				<ul>
+				<li>
-<tr> <td colspan="3"  height="5px"> </td></tr>
+					miniprepped pTRC, O/N culture of MG1655
-<!-- end welcome box -->
+				</li>
-<tr>
+				<li>
+					MG1655 did not grow on antibiotic plates, so stocks are good!
-<!--navigation menu -->
+				</li>
-<td align="center" colspan="3">
+				</ul>
+			<li>
-<table  width="100%">
+				prepped DNA for transformation – pCas9 and RFP reporter
-<tr heigth="15px"></tr>
+			</li>
-<tr heigth="75px">
+			<li>
+				made MG1655 electrocompetent –
+				electroporate and plated transformants, incubated overnight
-<td style="border:1px solid black;" align="center" height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+			</li>
-<a href="https://2014.igem.org/Team:Toronto"style="color:#000000">Home </a> </td>
+		</ul>
+	</li>
-<td style="border:1px solid black;" align="center" height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+	<li class="week">
-<a href="https://2014.igem.org/Team:Toronto/Team"style="color:#000000"> Team </a> </td>
+		<h2><span>Week 2</span></h2>
+		<ul class="thingsdone">
-<td style="border:1px solid black;" align="center"  height ="45px"  onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+			<li>
-<a href="https://igem.org/Team.cgi?year=2014&team_name=Toronto"style="color:#000000"> Official Team Profile </a></td>
+				transformation of RFP, pCas9, GFP, fmt into NEB5alpha
+			</li>
-<td style="border:1px solid black" align="center"  height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+				<ul>
-<a href="https://2014.igem.org/Team:Toronto/Project"style="color:#000000"> Project</a></td>
+					<li>
+						transformants plated and incubated overnight
-<td style="border:1px solid black;" align="center"  height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+					</li>
-<a href="https://2014.igem.org/Team:Toronto/Parts"style="color:#000000"> Parts</a></td>
+					<li>
+						then inoculated into liquid culture, incubated overnight
-<td style="border:1px solid black;" align="center" height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+					</li>
-<a href="https://2014.igem.org/Team:Toronto/Modeling"style="color:#000000"> Modeling</a></td>
+				</ul>
+			<li>
-<td style="border:1px solid black;" align="center" height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+				overnight culture of MG1655 and pTRC99A
-<a href="https://2014.igem.org/Team:Toronto/Notebook"style="color:#000000"> Notebook</a></td>
+			</li>
+			<li>
-<td style="border:1px solid black;" align="center"  height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+				Miniprepped RFP and pTRC99A
-<a href="https://2014.igem.org/Team:Toronto/Safety"style=" color:#000000"> Safety </a></td>
+			</li>
+				<ul>
-<td style="border:1px solid black;" align="center"  height ="45px" onMouseOver="this.bgColor='#d3d3d3'" onMouseOut="this.bgColor='#e7e7e7'" bgColor=#e7e7e7>
+					<li>tested restriction enzymes EcoRI, Xbal, SpeI, Pstl
-<a href="https://2014.igem.org/Team:Toronto/Attributions"style="color:#000000"> Attributions </a></td>
+						on miniprep and ran on gel w/ uncut as control
+					</li>
+					<li>
-<td align ="center"> <a href="https://2014.igem.org/Main_Page"> <img src="https://static.igem.org/mediawiki/igem.org/6/60/Igemlogo_300px.png" width="55px"></a> </td>
+						cut plasmids were too faint to see – need more
-</tr>
+						concentrated DNA in preps!
-</table>
+					</li>
+				</ul>
+			<li>
-</tr>
+				O/N cultures of RFP, pCas9, GFP from transformation
+			</li>
+			<li>
-</tr>
+				miniprep of O/N cultures of transformants and pTRC99A
+			</li>
+		</ul>
+	<li class="week">
+		<h2><span>Week 3</span></h2>
+		<ul class="thingsdone">
-</td>
+			<li>
+				miniprep again, greater volume (3mL)
-<tr> <td colspan="3"  height="15px"> </td></tr>
+				for RFP, GFP, Cas9, pTRC99A + nanodrop
-<tr><td bgColor="#e7e7e7" colspan="3" height="1px"> </tr>
+			</li>
-<tr> <td colspan="3"  height="5px"> </td></tr>
+				<ul>
+					<li>
+						digest product (w SpeI, EcoRI, cutsmart) and run on gel
-<!--requirements section -->
+					</li>
-<tr><td colspan="3"> <h3>Notebook</h3></td></tr>
+				</ul>
-</tr>
+			<li>
+				O/N culture from plate of extra biobrick, RFP, MG1655
+			</li>
-<tr>
+			<li>
-<td width="45%"  valign="top">
+				start RFP and MG1655 liquid cultures for the RFP
-<p>You should make use of the calendar feature on the wiki and start a lab notebook. This may be looked at by the judges to see how your work progressed throughout the summer. It is a very useful organizational tool as well. </p>
+				spectrum measurements in the afternoon
-</td>
+			</li>
+				<ul>
-<td></td>
+					<li>
-<td></td>
+						RFP grew slowly and was transformed into NEB5alpha instead of MG1655
-</tr>
+					</li>
+				</ul>
+			<li>
+				digest 8 samples from yesterday’s miniprep of 8 biobrick cultures,
+				load and run gel of digest
+			</li>
+			<li>
+				oligos and gblocks arrived
+			</li>
+			<li>
+				did PCR of pCas9 and pTRC99A chunks
+			</li>
+			<li>
+				Started MG1655 liquid culture for making chemically competent
+			</li>
+				<ul>
+					<li>
+						make chemically competent cells, transform RFP into them,
+						PCR purification, run on gel
+					</li>
+				</ul>
+			</ul>
+<li class="week">
+		<h2><span>Week 4</span></h2>
+		<ul class="thingsdone">
+			<li>
+				miniprepped pCas9 + pTRC99A (w 7mL of cells)
+			</li>
+			<li>
+				did gel extraction – cut out pCas9 + pTRC digests –
+				PCR both as well as nanodrop
+			</li>
+			<li>
+				Mon/Tues = PCR w mastermix,
+				Wed = make comp MG1655 and heatshock RFP,
+				Thurs/Fri = confirm RFP and Marafini protocol/golden-gate assembly
+			</li>
+				<ul>
+					<li>
+						PCR from the Friday before did not work
+					</li>
+					<li>
+						so do lots of minipreps from 10mL cultures and start over, use larger volumes for digests
+					</li>
+						DNA eluted into collection tube but saw salt contamination when nanodropped therefore redo miniprep…
+					</li>
+					<li>
+						miniprepped pTRC and pCas9 and then nanodropped –
+						results were good so created gel for next day, as well as a digestion
+					</li>
+					<li>
+						digested/ran the gel/extracted, will nanodrop gel extraction – if worked, try PCR again
+					</li>
+				</ul>
+			</ul>
+<li class="week">
+		<h2><span>Week 5</span></h2>
+		<ul class="thingsdone">
+			<li>
+				Wed. minipreps were good (however possibly from just high free nucleotides), gel extraction failed (no DNA at the end and a lot of salt contamination) – so just PCR from miniprepped plasmids
+			</li>
+			<li>
+				digest and run gel of digest at the same time!
+			</li>
+				<ul>
+					<li>
+						PCR of pTRC and pCas9 – have also been digested
+					</li>
+					<li>
+						ran gel! 5 part sample, 1 part loading dye
+					</li>
+				</ul>
+			<li>
+				if PCR worked, digest PCR product w DpnI – got nothing for pCas9 though on the gel (to be re-PCR-ed), but bright bands for pTRC
+			</li>
+			<li>
+				competent MG1655 also done
+			</li>
+			<li>
+				PCR of miniprep C1 #1 of cas9… did 10 x 10uL reaction using gradient temps in 58-68 range
+			</li>
+				<ul>
+					<li>
+						run on gel to see if PCR worked
+					</li>
+					<li>
+						PCR gel showed 2 weak bands – either not enough DNA or PCR failed
+					</li>
+				</ul>
+			<li>
+				heat shock transformation for MG1655 w RFP
+				plasmid but very few colonies on CM plate
+			</li>
+		</ul>
+<li class="week">
+		<h2><span>Week 6</span></h2>
+		<ul class="thingsdone">
+			<li>
+				PCR product (???) run on gel, pick most successful PCR
+			</li>
+			<li>
+				DpnI digest following protocol in NEB Gibson manual
+				Transform RFP & MG1655, O/N cultures
+			</li>
+			<li>
+				pCas9PCR product visible on gel
+			</li>
+			<li>
+				DpnI digest + PCR cleanup of digest (ended up not having enough DNA)
+			</li>
+			<li>
+				plating of transformed RFP into DH5a
+			</li>
+			<li>
+				processed PCR – ran on gel, DpnI digest also ran on gel, PCR cleanup, nanodrop (worked well)
+			</li>
+			<li>
+				needed to transform pCas9+spacer plasmid & RFP DH5a
+			</li>
+		</ul>
+<li class="week">
+		<h2><span>Week 7/8</span></h2>
+		<ul class="thingsdone">
+			<li>
+				transform RFP & BL21(DE3)
+			</li>
+			<li>
+				PCR of pCas9, pTRC99A
+			</li>
+			<li>
+				Gibson – pick 8 colonies, make O/N colonies, try to PCR form reaction to get 4-fragment superchunk
+			</li>
+			<li>
+				Maraffini – use Anderson high for 4 fragment
+				(phosphorylation + annealing of spacers if we get a lot of DNA), otherwise using Aug 18 miniprep do a BsaI digest
+			</li>
+				<ul>
+					<li>
+						got colonies from Gibson
+					</li>
+				</ul>
+			<li>
+things in parallel:
+			</li>
+				<ul>
+					<li>
+						miniprepped plasmids from Gibson transformants from O/N liquid cultures (need to be sent for sequencing)
+						, plasmids digested w E+P and to be run on gel
+					</li>
+					<li>
+						making competent MG1655 – transform RFP into it
+					</li>
+					<li>
+						tried BsaI digestion and gel extraction on Stanford-brown pCas9 (for Marafini/Golden-gate),
+						does not seem to work even w large volumes
+					</li>
+				</ul>
+			<li>
+				look at plates from transformation, run E+P digests on gel – if the digests look wrong size, do colony PCR on rest of Gibson colonies on plates
+			</li>
+				<ul>
+					<li>
+						use fwd/rev primers for cas9 and p!TRC chunks
+					</li>
+					<li>
+						if correct, also PCR the 3-fragment superchunk from the miniprep plasmid by using Cas9 fwd with p!TRC rev primers
+					</li>
+				</ul>
+			<li>
+				try a gel-extraction protocol…
+			</li>
+		</ul>
+<li class="week">
+		<h2><span>Week 9</span></h2>
+		<ul class="thingsdone">
+			<li>
+				Main thing – <b>GIBSON ASSEMBLY</b>
+			</li>
+			<li>
+				screened 8 colonies – miniprepped, EcoRI + PstI digest & wrong product, non-specific assembly
+			</li>
+				<ul>
+					<li>
+						extend gblocks (Anderson high + tracr) so more overlap, try Gibson again
+					</li>
+				</ul>
+			<li>
+				did digests of plasmids w one restriction enzyme instead of double digest + run gel (for less confusing results) – used miniprep #1-4
+			</li>
+			<li>
+				made O/N cultures from first Gibson reaction #9-15 – miniprepped and streak out plates
+			</li>
+			<li>
+				minipreps #5-8 from earlier digested w EcoRI and PstO (separately), run on gel
+			</li>
+			<li>
+				take 2 minipreps, do 3 reactions on each – EcoRI only, PstI only, both EcoRI + PstI
+			</li>
+		</ul>
+<li class="week">
+		<h2><span>Week 10</span></h2>
+		<ul class="thingsdone">
+			<li>
+				miniprep out RFP plasmid to be used for putting biobricks into pSB1C3, will want to screen for non-red colonies at the end of the process
+			</li>
+			<li>
+				unable to do digest because nanoprep of all 3 minipreps was too low
+			</li>
+			<li>
+				primers arrived – ran PCR  w new primers
+			</li>
+				<ul>
+					<li>
+						also digested RPF
+					</li>
+					<li>
+						run digests on gel (1/2 thickness)
+					</li>
+				</ul>
+			<li>
+				ran the original gblocks w extended gblocks –
+				not enough of original gblocks to show up on gel
+			</li>
+			<li>
+				combined PCR reactions of tracr gblocks into one,
+				same with Anderson High PCR products
+			</li>
+				<ul>
+					<li>
+						purified both
+					</li>
+					<li>
+						PCR purified Cas9 array from a PCR in August
+					</li>
+					<li>
+						purified p!TRC chunk found
+					</li>
+					<li>
+						all 4 to be used for Gibson assembly!
+					</li>
+				</ul>
+			<li>
+				glycerol stocked 3 tubes of colonies from first
+				Gibson attempt (#3, 4, 7)
+			</li>
+			<li>
+				transformed Gibson in NEB5alpha, ½ of each reaction
+				tube into a total of 4 NEB5alpha – 4 tubes plated
+				onto 2 plates each = total 8 plates incubated
+			</li>
+			<li>
+				on Friday, found colonies from the Gibson assembly and
+				did colony PCR
+			</li>
+			<li>
+				colony PCR primers were designed to cover the seams
+				where the 4 chunks joined
+			</li>
+			<li>
+				mixed the template DNA and biobrick primers for the
+				Cas9-array chunk, but did not add the master mix yet
+				(done later)
+			</li>
+		</ul>
+<li class="week">
+		<h2><span>Week 11</span></h2>
+		<ul class="thingsdone">
+			<li>
+				ran Gibson colony PCR on gel – colonies #3 + 6 have correct bands, started O/N cultures of them w cell suspensions from colony PCR
+			</li>
+			<li>
+				miniprep and glycerol stock them (low copy plasmid – do 3uL miniprep)
+			</li>
+			<li>
+				PCR of cas9 chunk – run on gel, see if band is at 4595
+			</li>
+			<li>
+				using RFP miniprep from earlier, digest w EcoRI and PstI
+			</li>
+				<ul>
+					<li>
+						linearised plasmid digested same way (if DNA dissolved – was left sitting overnight to dissolve)
+					</li>
+				</ul>
+			<li>
+				nothing on gel at correct size…. only used 1uL of DNA for gel though
+			</li>
+			<li>
+				digest ~1000ng of Gibson miniprep from 2 colonies w EcoRI and PstI, run on gel
+			</li>
+			<li>
+				run 5uL of tube labelled C6*
+			</li>
+			<li>
+				cas9-array chunk biobrick extension PCR barely worked – not enough DNA after PCR purification
+				but tracr chunk biobrick PCR worked
+			</li>
+				<ul>
+					<li>
+						digested/ligated into pSB1C3, transformed into competent cells
+					</li>
+					<li>
+						Gibson colonly #3 didn’t assemble correctly, only produced 1 band from E+P digestion
+					</li>
+				</ul>
+			<li>
+				transformed ligation into NEB5alpha – after 2 hour (actual = 10 min) incubation in SOB, pipetted into 2mL LB Cm and grew overnight
+			</li>
+			<li>
+				miniprepped to see if it grew and packed it up for shipping!
-</table>
+	</li>
+</ul>
+	</div>
+</div>
+</div>
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+University of Toronto iGEM
+                                                        <a href="https://igem.org/Team.cgi?year=2014&team_name=Toronto"> Official Team Profile </a>
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