Calgary/constructing wetlab

From 2007.igem.org

< Calgary(Difference between revisions)
 
(10 intermediate revisions not shown)
Line 1: Line 1:
<html>
<html>
 +
<!--
 +
  E. coLisa Construction Plan
 +
  This page describes the approachs and techniques used to construct the logic circut
 +
  Also this page describes the work done with the light sensing system developed by Austin Texas
 +
  The logic circut construction plan was written and provided by Dave Curran
 +
  The light sensor work was written and provided by Patrick King
 +
-->
<head>
<head>
-
<meta http-equiv="Content-Type" content="text/html; charset=utf-8" />
+
<!--
-
<title>Protocols</title>
+
  Cascading Style Sheet (CSS) component
 +
  in plain html style sheets are completely independent of the HTML page but are included in this page to simplify design within a wiki script environment.
 +
  This section describes the layout, colors and images displayed on the page
 +
-->
<style>
<style>
 +
 +
.ideasList{
 +
margin-bottom:30px
 +
}
 +
ul#sub {
ul#sub {
margin:0px;
margin:0px;
Line 43: Line 58:
font-size:13px;
font-size:13px;
color:#FFFFFF;
color:#FFFFFF;
 +
}
 +
 +
a.mainLinks:hover {
 +
text-decoration:none;
 +
background-color:#006633;
}
}
Line 57: Line 77:
</head>
</head>
<body>
<body>
 +
<!--
 +
  E.coLisa Title
 +
  The title and and top level navigation links
 +
-->
<table class="header">
<table class="header">
   <tr>
   <tr>
     <td><a href="https://2007.igem.org/Calgary"><img style="border:none" src="https://static.igem.org/mediawiki/2007/3/34/BackToHome.gif" alt="back to U of C Homepage"></a></td>
     <td><a href="https://2007.igem.org/Calgary"><img style="border:none" src="https://static.igem.org/mediawiki/2007/3/34/BackToHome.gif" alt="back to U of C Homepage"></a></td>
     <td><a name="top"> <img src="https://static.igem.org/mediawiki/2007/f/fe/EcoLisaHeader2.gif" /></a></td>
     <td><a name="top"> <img src="https://static.igem.org/mediawiki/2007/f/fe/EcoLisaHeader2.gif" /></a></td>
-
     <td align="right"><a href=""><img img style="border:none" src="https://static.igem.org/mediawiki/2007/2/29/CheckOutevoGEM.gif" alt="Check out evoGEM"></a></td>
+
     <td align="right"><a href="https://2007.igem.org/Calgary/evoGEM_introduction"><img img style="border:none" src="https://static.igem.org/mediawiki/2007/2/29/CheckOutevoGEM.gif" alt="Check out evoGEM"></a></td>
   </tr>
   </tr>
</table>
</table>
-
 
+
<!--
 +
  E.coLisa main menu
 +
  The navigation menu for the E.co Lisa section of the site
 +
-->
<table class="links" >
<table class="links" >
   <tr>
   <tr>
-
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/choosing_our_project" title="choosing our project" >Projects</a> </td>
+
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/choosing_our_project" title="choosing our project" >Projects</a> </td>
-
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/design" title="designing our project">Project Design: Wet Lab</a> </td>
+
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/design" title="designing our project - wetlab">Design: Wet Lab</a> </td>
-
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/constructing_printer" title="constructing our project - printer and software" >Project Design: Printer and Software</a> </td>  
+
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/constructing_printer" title="designing our project - printer" >Design: Printer</a> </td>
-
     <td align="center"><a class="mainLinks" href="https://2007.igem.org/Calgary/testing" title="testing our parts and primers" >Testing</a> </td>
+
    <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/software" title="designing our project - printer" >Design: Software</a> </td>
-
     <td align="center"><a class="mainLinks" href="https://2007.igem.org/Calgary/constructing_wetlab" title="constructing our project" >Constructing our Project: The Wetlab</a> </td>
+
     <td align="center" ><a class="mainLinks" href="https://2007.igem.org/Calgary/testing" title="testing our parts and primers" >Testing</a> </td>
-
     <td align="center" bgcolor="#006633" valign="top"><a class="mainLinks" href="https://2007.igem.org/Calgary/protocols" title="protocols" >Protocols</a> </td>
+
     <td align="center" bgcolor="#006633"><a class="mainLinks" href="https://2007.igem.org/Calgary/constructing_wetlab" title="constructing our project" >Construction: The Wetlab</a> </td>
 +
     <td align="center" valign="top"><a class="mainLinks" href="https://2007.igem.org/Calgary/protocols" title="protocols" >Protocols</a> </td>
     <td align="center"><a class="mainLinks" href="https://2007.igem.org/Calgary/final_result" title="final results" >Final Result of E.co Lisa</a> </td>
     <td align="center"><a class="mainLinks" href="https://2007.igem.org/Calgary/final_result" title="final results" >Final Result of E.co Lisa</a> </td>
   </tr>
   </tr>
</table>
</table>
-
<table width="100%" style="margin-bottom:30px;">
+
 
-
  <tr>
+
<!--
-
    <td valign="top"><ul id="sub">
+
  Construction of the logic circut
-
        <li><a href="#transformation" title="Bacterial Transformation Protocol"> Bacterial Transformation </a></li>
+
  Plan provided by Dave Curran
-
        <li><a href="#rehydration" title="Protocol for rehydrating cells from registery"> Rehydration </a></li>
+
-->
-
        <li><a href="#pcr" title="Protocol for pcr"> Taq PCR </a></li>
+
<p style="font-size:20px;">The Logic Circut </p>
-
      </ul></td>
+
<p style="font-size:14px"><b> The application below shows the schematics of both the complex and simple systems. Hovering over a part with the mouse will highlight its corresponding description in the table. Clicking on a part in the diagram will open the registry's page that desribes the part.</b> </p>
-
    <td valign="top"><ul id ="sub">
+
<p><em>NOTE: if you are viewing this page with internet explorer you will have to click on the application once before you can use it</em></p>
-
        <li><a href="#ct" title="Construction Technique"> Construction Technique</a></li>
+
<!--
-
        <li><a href="#pp" title="Plasmid Prep"> Plasmid Prep </a></li>
+
  Interactive Logic Circut
-
        <li><a href="#ap" title="Antarctic Phosphatase"> Vector Dephosphorylation </a></li>
+
  This application allows the user to see a schematic of the registry provided parts used to design our circut. Hovering over an icon will highlight its description in the corresponding table. Clicking on an icon will link to the iGEM registry's description of the part.
-
      </ul></td>
+
  The application was designed by Paul Adamiak
-
    <td valign="top"><ul id="sub">
+
  Note: The application uploaded to the iGEM server is a .swf file and cannot be edited in anyway. To obtain the original .fla file please email Paul Adamiak at pjadamia@ucalgary.ca
-
        <li><a href="#platePrep" title="Antarctic Phosphatase"> LB - Agar Plate </a></li>
+
-->
-
        <li><a href="#overnight" title="overnight"> Over Night Growth </a></li>
+
<div style="margin-top:1.5em; margin-bottom:30px;">
-
        <li><a href="#gsp" title="Glycerol Stock"> Glycerol Stock Preparation </a></li>
+
   <object classid="clsid:D27CDB6E-AE6D-11cf-96B8-444553540000" codebase="http://download.macromedia.com/pub/shockwave/cabs/flash/swflash.cab#version=6,0,29,0" id="flash" width="900px" height="650px">
-
      </ul></td>
+
    <param name="movie" value="https://static.igem.org/mediawiki/2007/7/73/IgemDesign.swf" />
-
    <td valign="top"><ul id="sub">
+
     <param name="quality" value="high" />
-
        <li><a href="#age" title="Agarose Gel Electrophoresis"> Agarose Gel Electrophoresis </a></li>
+
     <param name="menu" value="false" />
-
        <li><a href="#rd" title="Restriction Digest"> Restriction Digest </a></li>
+
     <param name="wmode" value="transparent" />
-
        <li><a href="#lp" title="Ligation"> Ligation </a></li>
+
     <param name="loop" value="false" />
-
      </ul></td>
+
     <param name="play" value="false" />
-
  </tr>
+
     <param name="salign" value="t" />
-
</table>
+
     <embed src="https://static.igem.org/mediawiki/2007/7/73/IgemDesign.swf" wmode="" quality="high" menu="false" pluginspage="http://www.macromedia.com/go/getflashplayer" type="application/x-shockwave-flash" width="900px" height="650px"></embed>
-
<div style="margin-bottom:60px">
+
   </object>
-
  <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="transformation"> Bacterial Transformation</a></p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <ul>
+
-
    <li> Thaw 100 ul of competen cells (per transformation) on ice just before they are needed</li>
+
-
    <li> Add DNA (max 20ul) thawed cells and mix by flicking the side of the tube. Leave on ice for 30 minutes</li>
+
-
    <li> Heat shock for 2 minutes at 42 degrees Celsius or 5 minutes at 37 degrees Celsius</li>
+
-
    <li> Place on Ice for 5 minutes </li>
+
-
    <li> Add 250ul SOC medium to each tube</li>
+
-
    <li> Incubate for 30 to 60 minutes with shaking at 37 degrees Celsius. (Note that for Kanamycin containing plasmides always use one hour)</li>
+
-
    <li> Spin down to remove all supernatant except approximately 100 ul</li>
+
-
    <li> Plate approximately 30 ul on each of two antibiotic plates </li>
+
-
    <li> Grow overnight at 37 degrees Celsius </li>
+
-
  </ul>
+
-
  <p> For this protocol we used three controls
+
-
  <ul>
+
-
    <li> <b> Positive Control </b> - pBluescript in TOP10 cells on amp resistant plates </li>
+
-
    <li> <b> Negative Control </b> - TOP10 cells grown on amp resistant plates </li>
+
-
    <li> <b> Negative Control </b> - DB31 cells on amp resistant plates </li>
+
-
  </ul>
+
-
  </p>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td width="85%"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="rehydration"> Rehydration </a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <p> Biobrick parts are shipped from the registry in a dehydrated from. As such they must be rehydrated before they can be used. </p>
+
-
  <ul>
+
-
    <li> Puncture a hole through the foil with a pipette tip into the well that corresponds to the Biobrick - standard part that you want</li>
+
-
    <li> Add 15 ul of diH20 (deionized water)</li>
+
-
    <li>Take 1 ul DNA and transform into your desired competent cells, plate out onto a plate with the correct antibiotic and grow overnight. Your goal here is to obtain single colonies</li>
+
-
  </ul>
+
-
  <p> For this protocol we used three controls
+
-
  <ul>
+
-
    <li> <b> Positive Control </b> - pBluescript in TOP10 cells on amp resistant plates </li>
+
-
    <li> <b> Negative Control </b> - TOP10 cells grown on amp resistant plates </li>
+
-
    <li> <b> Negative Control </b> - DB31 cells on amp resistant plates </li>
+
-
  </ul>
+
-
  </p>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td width="85%"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="pcr">Taq PCR Protocol </a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <table width="90%" border="1px" style="margin-bottom:15px;">
+
-
    <tr>
+
-
      <td><b>Reagent</b></td>
+
-
      <td><b>Volume ( 1x )</b></td>
+
-
      <td><b>Volume ( 3x )</b></td>
+
-
      <td><b>Volume ( 5x )</b></td>
+
-
      <td><b>Volume ( 15x )</b></td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>Sterile H2O</td>
+
-
      <td>36 ul</td>
+
-
      <td>108 ul</td>
+
-
      <td>180 ul</td>
+
-
      <td>540 ul</td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>10X Taq Buffer</td>
+
-
      <td>5 ul</td>
+
-
      <td>15 ul</td>
+
-
      <td>25 ul</td>
+
-
      <td>75 ul</td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>2mM dNTPs</td>
+
-
      <td>5 ul</td>
+
-
      <td>15 ul</td>
+
-
      <td>25 ul</td>
+
-
      <td>75 ul</td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>Forward Primer (100 ug/ul) </td>
+
-
      <td>1 ul</td>
+
-
      <td>3 ul</td>
+
-
      <td>5 ul</td>
+
-
      <td>15 ul</td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>Reverse Primer (100 ug/ul) </td>
+
-
      <td>1 ul</td>
+
-
      <td>3 ul</td>
+
-
      <td>5 ul</td>
+
-
      <td>15 ul</td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>50mM MgCl2</td>
+
-
      <td>1.5 ul</td>
+
-
      <td>4.5 ul</td>
+
-
      <td>7.5 ul</td>
+
-
      <td>22.5 ul</td>
+
-
    </tr>
+
-
    <tr>
+
-
      <td>Taq Polymerase (50 ug/ul)</td>
+
-
      <td>0.5 ul</td>
+
-
      <td>1.5 ul</td>
+
-
      <td>2.5 ul</td>
+
-
      <td>7.5 ul</td>
+
-
    </tr>
+
-
  </table>
+
-
  <p><b> Thermocycler Conditions </b></p>
+
-
  <ul>
+
-
    <li> 1 Cycle - 6 minutes at 95 degrees Celsius </li>
+
-
    <li> 36 cycles
+
-
      <ul>
+
-
        <li> 1 minute at 95 degrees Celsius </li>
+
-
        <li> 1 minute at 58 degrees Celsius ( this step done at 65 degrees Celsius for higher GC content ) </li>
+
-
        <li> 1 minute at 72 degrees Celsius </li>
+
-
      </ul>
+
-
    </li>
+
-
    <li> 1 Cycle - 10 minutes at 72 degrees Celsius then HOLD at 4 degrees Celsius </li>
+
-
  </ul>
+
-
  <p> Conditions were varied as needed. For example in cases of longer products all 1 minute times were increased to 1.5 to 3 minutes</p>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="pp"> Plasmid Preparation Protocol - from GenElute Plasmid Miniprep Kit </a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <ul>
+
-
    <li><em>Harvest Cells</em>
+
-
      <ul>
+
-
        <li>pellet 1-5 ml of an overnight culture.</li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em> Resuspend Cells </em>
+
-
      <ul>
+
-
        <li>Completely resuspend the bacterial pellet with 200ul of resuspension solution. Vortex or pipette up and down to throroughly resuspend cells until homogenous. Incomplete suspensions will result in poor recovery. </li>
+
-
        <li> Another rapid way to resuspend the cell pelles is to scrape teh bottoms of the microcentrifuge tubes back and forth five times across the surface of a polpropylene microcentrifuge tube storage rack with 5 X 16 holes </li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em>Lyse Cells</em>
+
-
      <ul>
+
-
        <li> Lyse resuspended cells by adding 200 ul of the lysis solution. Immediately mix the contents by gentle inversion (6-8 times) until the mixture becomes clear and viscous. <b> Do Not Vortex </b>. </li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em>Neutralize</em>
+
-
      <ul>
+
-
        <li> Precipitate the cell debris by adding 350 ul of the Neutralization/Binding solution. Gently invert the tube 4-6 times. Pellet the cell debris by centrifuging at maximum speed for 10 minutes.</li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em> Prepare Column </em>
+
-
      <ul>
+
-
        <li> Insert a GenElute Miniprep Binding Column into a provided microcentrifuge tube, if not already assembled. add 500 ul of the Column Preparation Solution to each miniprep column and centrifuge at Max speed for 30 to 60 seconds. Discard the flow through liquid.</li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em>Load Cleared Lysate</em>
+
-
      <ul>
+
-
        <li> Transfer the cleared lysate from step 4 to the column prepared in step 5 and centrifuge at Max speed for 30 to 60 seconds. Discard the flow through</li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em>Wash Column</em>
+
-
      <ul>
+
-
        <li>Add 750 ul of the diluted Wash Solution to the column. Centrifuge at Max speed for 30 to 60 seconds. The column wash step removes residual salt and other contaminants introduced during the column load. Discard the flow through liquid and centrifuge again at maximum speed for 1 to 2 minutes without any additional wash solution to remove excess alcohol</li>
+
-
      </ul>
+
-
    </li>
+
-
    <li><em>Elute DNA </em>
+
-
      <ul>
+
-
        <li>Transfer the column to a fresh collection tube. Add 100ul of Elution Solution or molecular biology reagent water to the column. For DNA sequencing and other enzymatic applications, use water or 5mM tris-HCL, pH 8.0, as an eluant. Centrifuge at Max speed for 1 minute. DNA is now present in the eluate and is ready for immediate use or storage at -20 degrees Celsius. </li>
+
-
      </ul>
+
-
    </li>
+
-
  </ul>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="ct"> Construction Technique</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <p> Determine the order of the two parts you will be putting together; the one in front will be referred to as the insert, while the one behind will be referred to as the vector.  Both the vector and the insert need to have their own separate tube, at least in the beginning. </p>
+
-
  <p><em> Restriction Digest Protocol</em></p>
+
-
  <p> In the Insert Tube...
+
-
  <ul>
+
-
    <li>600ng of DNA (To figure out the volume, the calculation is 600 / concentration of plasmid. This gives you volume in μL).</li>
+
-
    <li>Water, so that the volume of DNA and water in the tube is 35 μL</li>
+
-
    <li>4 μL of React 1 Buffer </li>
+
-
    <li>0.5 μL of EcoR1 </li>
+
-
    <li>0.5 μL of Spe1</li>
+
-
  </ul>
+
-
  </p>
+
-
  <p> In the vector Tube...
+
-
  <ul>
+
-
    <li>250ng of DNA (To figure out the volume, the calculation is 250 / concentration of plasmid.  This gives you volume in μL).</li>
+
-
    <li>Water, so that the volume of DNA and water in the tube is 35 μL </li>
+
-
    <li>4 μL of React 2 Buffer</li>
+
-
    <li>0.5 μL of EcoR1</li>
+
-
    <li>0.5 μL of Xba1</li>
+
-
  </ul>
+
-
  </p>
+
-
  <p> Put both tubes into the 37°C water bath for one hour.  After, place them into the 65°C heating block for 10 minutes.  This destroys any enzymes in the tube (which is ok, because by now they’ve done all they need to).
+
-
    Take the insert out, and put it in a -20°C freezer. </p>
+
-
  <p><em> Antarctic Phosphatase Protocol</em></p>
+
-
  <p> To the vector tube, add 5 μL of 10x Antarctic Phosphatase Buffer, 4 μL of water, and 1 μL of Antarctic Phosphatase.  We do this to prevent the vector from closing up again without any insert.
+
-
    Put the tube into the 37°C water bath for 30 mins.  After, place it in the 65°C heating block for 10 minutes. </p>
+
-
  <p><em> Ligation Protocol </em></p>
+
-
  <p>Take the insert out of the freezer, and add 5 μL of insert and 5 μL of vector to a new tube. Label the rest of each tube as Unligated, put the date on the tube, and stick it in the -20°C freezer incase your transformation doesn’t work. To the single tube of 10μL mix, add 10 μL of 2x Quick Ligase Buffer, and 1 μL of Quick Ligase. Let this sit at room temperature for 5 minutes. </p>
+
-
  <p> You are now done.  If you are going to transform this construction product, add all 21μL to a tube of whatever bacteria you're using. </p>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="ap"> Vector Dephosphorylation with Antarctic Phosphatase</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <p> Vector Dephosphorylation with Atlantic Phosphotase Protocol </p>
+
-
  <p> Ensure that restriction enzyme has been heat inactivated by heating tube in 37°C water bath for one hour. Then place into a 65°C heating block for 10 minutes. This destroys any remaining enzymes in the tube.</p>
+
-
  <p>
+
-
  <ul>
+
-
    <li>Add 1/10 volume of 10x Antarctic Phosphatase Reaction Buffer to 1 ug of DNA cut with any restriction endonuclease in any buffer.</li>
+
-
    <li>Add 1 μl of Antarctic Phosphatase (5 units) and mix. </li>
+
-
    <li>Incubate for 15 minutes at 37°C for 5´ extensions or bluntends, 60 minutes for 3´ extensions. <em>Note: for typical iGEM restriction digests use one hour.</em></li>
+
-
    <li>Heat inactivate for 5 minutes at 65°C (or as required to inactivate the restriction enzyme).</li>
+
-
  </ul>
+
-
  </p>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
   <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="platePrep"> LB - Agar Plate Preparation Protocol</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <ul>
+
-
    <li>Weigh 35g of LB-Agar powder mix per litre of media desired. One litre makes 40-50 plates</li>
+
-
    <li>Select an appropriate flask; the lab autoclave will cause flasks half full and above to boil over! Use a 2L flasks for up to .5 L of media, a 4 litre flask for up to 1.5L, etc</li>
+
-
    <li>Disolve LB-Agar, using water from one of the wall mounted nanopure filters. Add a stir bar and use a magnetic stirrer to speed things up </li>
+
-
    <li>Cover the flask with aluminum foil, and secure the foil with autoclave tape. The foil should be somewhat loose (to avoid building pressure in the flask while sterilizing and blowing the foil off), but not so loose that lots of liquid can escape </li>
+
-
    <li>Put the flask in a plastic autoclave tray, load into the autoclave, and sterilize using the 20 minute liquid program</li>
+
-
    <li>Once the autoclave finishes venting (which can take twice as long as the sterilization proper), check that the foil covering is still in place. If it is not, the media is contaminated! Unload using the insulated oven gloves</li>
+
-
    <li>Allow the media to cool until it can be handled without the oven mits. The cold room can be used to speed this up. Alternatively, if a large batch of media is prepared flasks may be kept hot in the prep lab water bath, to avoid all of them cooling at once. Agar polymerization cannot be reversed once it starts (and if it begins to set in the flask you're in trouble!), but media can be kept from setting further by keeping it hot.</li>
+
-
    <li>Once media is cool, add other desired ingredients. Use the magnetic stirrer to mix, but do NOT add a stir bar now, or the media will be contaminated. (If one wasn't added before, you must do without.) Common additions include:
+
-
      <ul>
+
-
        <li>ampicillin (stock 100mg/ml, final 100ug/ml)</li>
+
-
        <li>kanamycin (stock 50mg/ml, final 50ug/ml)</li>
+
-
        <li>chloramphenicol (stock 50mg/ml, final 30ug/ml)</li>
+
-
        <li>x-gal (stock 40mg/ml, final 40ug/ml)</li>
+
-
        <li>To achieve final concentrations, add 1mL of stock per 1L of media, except for chloramphenicol, where 0.6mL per 1L of media is added instead</li>
+
-
      </ul>
+
-
    </li>
+
-
    <li>Pour directly from the flask into sterile petri plates. Use a quick pass with a bunsen burner flame to snuff out bubbles that form during pouring. Do not subject the plate to continuous heat or the plate will melt, and the heat sensitive ingredients added in the previous step will be destroyed. Bubbles can allow cells to access nutrients without being exposed to the plate's antibiotic, and should be blown out immediately before the gel can set. It's a good idea for one person to pour while another flames bubbles. </li>
+
-
    <li>Allow the plates to stand right side up overnight, or until the gel sets if they are needed sooner. Plates should be stored upside down to keep condensation from falling on the media. Store petri plates in the plastic bags they ship in, in the 4 degree cold room. </li>
+
-
  </ul>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="overnight"> Over Night Growth</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <p> <em> Adapted from Butanerds Protocols from the University of Alberta iGEM Protocols pdf</em></p>
+
-
  <p> What you will need
+
-
  <ul>
+
-
    <li> 10mL culture tube. Use 16mm x 160mm or 16mm x 125mm</li>
+
-
    <li> 5 mL LB</li>
+
-
    <li> 5 uL 1000X antibiotiecs</li>
+
-
    <li> Single colonies on a plate (best not to start an over night from a glycerol stock)</li>
+
-
  </ul>
+
-
  </p>
+
-
  <p> Protocol </p>
+
-
  <ul>
+
-
    <li> Pipet 5uL 1000X antibiotic into culture tube </li>
+
-
    <li> Add 5mL non-contaminated LB. Do this first. Then add antibiotic</li>
+
-
     <li> Select a single colony using a sterile toothpick or flamed loop that has been cooled </li>
+
-
    <li> Place toothpick or loop in culture tube and stir </li>
+
-
    <li> Remove toothpick or loop and place culture tube in incubator at 37 C overnight shaking vigorously (250 RPM)</li>
+
-
  </ul>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
     <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="gsp"> Glycerol Stock Preparation</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
     </tr>
+
-
  </table>
+
-
  <p> <em> Adapted from Butanerds Protocols from the University of Alberta iGEM Protocols pdf</em></p>
+
-
  <p> What you will need </p>
+
-
  <ul>
+
-
    <li> Overnight bacterial growth </li>
+
-
    <li> screw captubes </li>
+
-
    <li> glycerol </li>
+
-
  </ul>
+
-
  <p> Protocol </p>
+
-
  <ul>
+
-
    <li> Pipet 0.5mL of 50% glycerol into 3 1.5 screw cap tubes</li>
+
-
    <li> Add 0.5mL of overnight culture to each tube </li>
+
-
    <li> Pipet up and down to gently mix</li>
+
-
    <li> Flash freeze  in liquid N2 or dry ice/ethanol bath </li>
+
-
    <li> Place in -80 C freezer when frozen </li>
+
-
  </ul>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
     <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="age"> Agarose Gel Electrophoresis Protocol</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
     </tr>
+
-
  </table>
+
-
  <p> <em> Adapted from Butanerds Protocols from the University of Alberta iGEM Protocols pdf</em></p>
+
-
  <p> What you will need </p>
+
-
  <ul>
+
-
    <li> 1X TAE </li>
+
-
    <li> Graduated Cylinder</li>
+
-
    <li> 125 mL flask </li>
+
-
    <li> Agarose </li>
+
-
    <li> Gel Pouring Tray </li>
+
-
    <li> Tape </li>
+
-
    <li> Gel rig </li>
+
-
    <li> Ethidium Bromide </li>
+
-
  </ul>
+
-
  <p> Protocol </p>
+
-
  <ul>
+
-
    <li> Measure out 120mL of buffer </li>
+
-
    <li> Transfer buffer to 125 mL flask </li>
+
-
    <li> Weigh out enough agarose to make a 1% gel (in our case 1.2 g of agarose was the right amount)</li>
+
-
    <li> Transfer agarose to 125mL flask</li>
+
-
    <li> Melt agarose in microwave until solution is almose boiling, stirring every 15-20 seconds (should be around 2 minutes)</li>
+
-
    <li> Allow agarose to cool (do not let it cool to the point where it is hard)</li>
+
-
    <li> Add 3 uL of Ethidium Bromide to the cooling agarose</li>
+
-
    <li> Assemble the gel pouring apparatus by inserting gate into slots. Use a pastuer pipet to run a bead of molton agarose along the edges of the gates to seal the box and prevent leaks</li>
+
-
    <li> Allow gel to cool until flask can be handled comfortabley</li>
+
-
    <li> Place comb in the gel rig</li>
+
-
    <li> Pour agarose into gel tray</li>
+
-
    <li> Allow to solidify. While the gel is solidifying prepare the samples. Add your sample and 1 uL 10x Loading Dye, 4 uL of DNA and 5 uL of water</li>
+
-
    <li> Pour 1X TBE over gel so that gel is covered by a 3-5mm buffer</li>
+
-
    <li> Load samples into lane (Don't forget to load a 1kb+ ladder into one of the lanes)</li>
+
-
    <li> Hook electrodes to gel apparatus</li>
+
-
    <li> Run the apparatus at 100V for 30 - 45 minutes (make sure to watch that the dye does not run off the gel)</li>
+
-
    <li> Visualize the gel and record the results</li>
+
-
  </ul>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
     <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="rd"> Restriction Digest</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
     </tr>
+
-
  </table>
+
-
  <p> This protocol is also described as a part of our <a href="#ct" title="construction technique"> Construction Technique</a>. Start by selecting the order of the two parts you will be putting together; the one in front will be referred to as the insert, while the one behind will be referred to as the vector.  Both the vector and the insert need to have their own separate tube, at least in the beginning. This is important because it allows for clean addition new parts to a the circut </p>
+
-
  <p> In the Insert Tube...
+
-
  <ul>
+
-
    <li>600ng of DNA (To figure out the volume, the calculation is 600 / concentration of plasmid.  This gives you volume in μL).</li>
+
-
    <li>Water, so that the volume of DNA and water in the tube is 35 μL</li>
+
-
    <li>4 μL of React 1 Buffer </li>
+
-
    <li>0.5 μL of EcoR1 </li>
+
-
    <li>0.5 μL of Spe1</li>
+
-
  </ul>
+
-
  </p>
+
-
  <p> In the vector Tube...
+
-
  <ul>
+
-
    <li>250ng of DNA (To figure out the volume, the calculation is 250 / concentration of plasmid.  This gives you volume in μL).</li>
+
-
    <li>Water, so that the volume of DNA and water in the tube is 35 μL </li>
+
-
    <li>4 μL of React 2 Buffer</li>
+
-
    <li>0.5 μL of EcoR1</li>
+
-
    <li>0.5 μL of Xba1</li>
+
-
  </ul>
+
-
  </p>
+
-
  <p> Put both tubes into the 37°C water bath for one hour.  After, place them into the 65°C heating block for 10 minutes.  This destroys any enzymes in the tube (which is ok, because by now they’ve done all they need to).
+
-
    Take the insert out, and put it in a -20°C freezer. </p>
+
-
</div>
+
-
<div style="margin-bottom:60px">
+
-
  <table width="100%">
+
-
    <tr>
+
-
      <td style="width:85%;"><p style="font-size:14px; font-weight:bold"><a style="text-decoration:none" name="lp"> Ligation Protocol</a> </p></td>
+
-
      <td width="15%"><a style="float:right;" href="#top" title="return to top">return to top</a> </td>
+
-
    </tr>
+
-
  </table>
+
-
  <p> This protocol is also described as a part of our <a href="#ct" title="construction technique"> Construction Technique</a>. Start by selecting the order of the two parts you will be putting together; the one in front will be referred to as the insert, while the one behind will be referred to as the vector.  Both the vector and the insert need to have their own separate tube, at least in the beginning. This is important because it allows for clean addition new parts to a the circut </p>
+
-
  <ul>
+
-
    <li>Take insert out of the freezer and ad 5 uL of insert and 5 uL f vector to a new tube </li>
+
-
    <li>Clearly label the remaining tubes of each (insert and vector) as Unligated, put the date on the tube and place in -20 C freezer in case the transformation does not work</li>
+
-
    <li>To the single tube containing both insert and vector add 10 uL of 2x Quick Ligase Buffer and 1 uL of Quick Ligase.</li>
+
-
    <li>Let this sit at room temperature for 5 minutes</li>
+
-
   </ul>
+
</div>
</div>
 +
<p> We planned to build the simple system diagrammed above in order to eventually express agarase through laser activation of <em>E. coli</em>. Since we had many of the parts already in composite form, the goal was to attach together the 5 composite parts above. </p>
 +
<br />
 +
<p><b><em>Construction Outline </em></b></p>
 +
<p>When constructing a composite part, the two pieces can be classified as an insert and a vector.  One piece is entirely cut out of its plasmid (the insert), while in the other plasmid (the vector) an opening is made just in from of the coding region itself (this is backwards in a reverse construction, which we did not use).  After the ligation step in the construction, there are several different plasmids in the mix.  First, you may have original parent plasmid that was never cut, from both plasmids.  The probability of having parent vector plasmid is quite small though, due to the phosphatase treatment in the construction.  You may also have insert plasmid that has had the actual insert cut out.  Both this and parent insert plasmid will confer a certain antibiotic resistance to any bacteria that will uptake it, and as a result, you will have no way of knowing which bacteria have uncut insert plasmid, cut-out insert plasmid, or your desired construction product.  This problem is why it is important that the two parts you are joining together have different resistance markers in their plasmids, or at least that the vector plasmid has a resistance the insert does not.  Looking at the four composite parts above that we were planning to use, all of them have only ampicillin resistance.  Because of this, before we could start any constructions, we had to confer a new resistance to two of the above composites, and this required a plasmid switch.  These involve two items: a plasmid with the required resistance and containing the cell death gene <em>ccdB</em>, and the part you wish to switch.  All you need do then is mix the two parent plasmids together, insert the appropriate enzymes to cut out both <em>ccdB</em> your gene, and then ligate.  There will be four possible products from this procedure.  If <em>ccdB</em> ends up in either its original plasmid or in your old plasmid, any cell that uptakes it will die.  If your part ends up in its old plasmid, it will be killed, as it will not have the resistance genes of the new plasmid.  Therefore, the only cells that survive will be the ones containing your part in the new plasmid.  Plasmid switches were done with parts and I13504 and A340620, moving them into plasmids containing ampicillin and chloramphenicol resistances, as these were to be the vectors in the subsequent construction techniques.</p>
 +
<p>With our two newly modified parts ready, the first step was to attach together R0084 with A340620, and S01414 with I13504.  Once the construction of these two composites was complete, overnight cultures were made, and the plasmids isolated.  The plan was to then attach together these two composites, but again they both had the same resistance markers.  To overcome this problem, we again did a plasmid switch, moving the new composite S01414 + I13504 into a plasmid containing ampicillin and kanamycin.  We were then able to attach together our two composites into our final logic circuit.</p>
 +
<br />
 +
<p><em> When designing this system, there were some possible problems noted with a pivotal part in our system, <em>ompF</em> (R0084), the promoter controlled by the light-sensing system. </em></p>
 +
<p>There were some contradictions in the literature about what this part did, and exactly how it would respond to light.  Also, this is not the part that the Texas team used in their project; they used the opposing part <em>ompC</em>.  We decided to go ahead and begin testing OmpC, and to begin putting it together with other parts, just in case we had to use it.  So every step noted above was done with <em>ompC</em> in place of <em>ompF</em> at the same time.  And since <em>ompC</em> exists in two forms in the registry, (R0083 and R0082), both parts were used simultaneously.  To test <em>ompC</em>, the part was put onto a GFP test construct, I13504 AC, to check the functioning and reliability of the promoter in both TOP10 and CP919 (the knockout strain needed for functionality of the light sensing system).  After both of these new parts were made, they had to be transformed into both CP919 and TOP10.  It was expected to glow in TOP10, though not too brightly, and to glow perhaps a little brighter in CP919.</p>
 +
<br />
 +
<p><b><em>RNA Lock and Keys</em></b></p>
 +
<p> One of the parts we were interested in using (for our off-switch) is an RNA lock and key to control translation.  The lock first needed to be tested, to see how tight its control really is.  To do this, was attached to a GFP testing part I13401 AC, with a constitutive promoter placed in front.  Since there should be no way to unlock the RBS in front of the GFP, the cells were not expected to glow at all, and this was indeed the case when we tested the construct out.  At the same time the lock test was being constructed, the relevant key was attached to a constitutive promoter, and then this construct attached to the locked GFP.  When transformed into <em>E. coli</em>, this construct was expected to glow quite strongly, alas the key proved difficult to work with, and this test has not yet been carried out.  Each of these testing procedures was done in parallel, as there were two sets of lock/keys to test out. </p>
 +
<p> Any crosstalk between the two sets of lock/keys also was to be tested.  To do this, the key construct 1 would be attached to lock construct 3, and as well 3 onto lock 1.  There should be no expression of GFP in either of these crosstalk experiments, or at least no more then the cells containing only a lock construct. </p>
 +
<p> Finally, the rate of control needs to be characterized for the RNA lock/keys.  To do this, an inducible promoter was to trigger expression of an RNA key, and for this we were going to use the AHL-induced promoter R0062.  First though, we were in need of a standard control, made by attaching R0062 to the GFP testing construct I13504 AC.  After that, a constitutive promoter was put in front of S01414 (which is necessary for functioning of the AHL promoter), and the two pieces put together.  This construct should not glow in TOP10, until AHL is added, and the speed of this expression should be characterized. </p>
 +
<p> During construction of the lock pieces, another part was made by putting S01414 (RBS and <em>luxR</em>) behind the locked GFP, and before the terminators.  This construct should not glow on its own, but should after addition of AHL. </p>
 +
<!--
 +
  Light Sensor Work
 +
  Information provided by Patrick King
 +
-->
 +
<p><b>Work With The Light Sensor</b></p>
 +
<p> The popularity of the light sensing biobrick parts since their release by the '05 Austin iGEM team is the best evidence of how useful a light induced system could be. Light can be easily and accurately applied with the right instruments, and could offer much more precise induction compared with the chemical inducers used today. However, just as the promise of the light sensor has spread, so has it's reputation as a tricky system to work with. Our project plan incorporated the light sensor controlling agarase expression, but most of our efforts on it were spent just trying to duplicate the functionality seen in the '05 Nature brief communication by Levskaya et al. </p>
 +
<p> <em>1) The Biobrick Light Sensor</em> </p>
 +
<p> On our first attempt to use the light sensor we used the Biobrick part M30109, which contains the three genes that code for the light sensor encoded in Biobrick format. M30109 was omitted from the iGEM'07 registry plate distribution by accident, so we made a special request for it from the registry.<br />
 +
  The M30109-pSB1AC3 plasmid proved extremely difficult to work with, however. Routine restriction digests and PCR amplifications known to work with the pSB1AC3 plasmid backbone failed completely. CP919 is the light sensor chassis E.coli strain, and experiments with light to test the sensor in CP919 also failed. Ultimately, M30109 was set aside and a different source material for the light sensor was sought. However, before abandoning this part one last PCR probe was done using primers for each of the three light sensor coding regions (biobrick parts I15008, I15009 and I15010). The gel is included below, and it indicates that these three regions are intact in M30109. Why exactly M30109 fails remains a mystery, but given that our primers anneal at the restriction sites flanking Biobrick parts, and that restriction digests of M30109 didn't succeed, the current hypothesis is that a restriction site has mutated or is damaged. Given more time, we might have returned to M30109 to find out what's going on with it. </p>
 +
<img src = "https://static.igem.org/mediawiki/2007/6/66/Aug2_2007_M_subgenes.gif" alt="Gel from August 2nd 2007" />
 +
<p><em>2) The Original Two Plasmid Light Sensor</em></p>
 +
<p> After difficulties with the biobrick light sensor we moved on to the original version of the system: the one developped by Levskaya et al. Jeff Tabor, a former Austin iGEM team member, was kind enough to send us the plasmids pPL-PCB and pCPH8. Colony PCR of the pPL-PCB pCPH8 double transformant we made, using the proven light sensor coding region primers, revealed that the three genes were present, and that double transformation worked. </p>
 +
<img src="https://static.igem.org/mediawiki/2007/3/3b/Sept4_double_transformant_labeled.gif" alt="gel from September 4th 2007 - shows double transformation">
 +
<p> The next hurdle was to demonstrate that the system itself could work. CP919 transformed with both plasmids was incubated in light and dark, in the hope of seeing a light sensitive response but none was observed. On a tip from Jeff Tabor that the pPL-PCB plasmid may be unstable, we switched to using only freshly transformed cells in our experiments but this made no difference. Most recently, we acquired a red bandpass filer. A bandpass filter is a lens that allows only light of a certain wavelength to pass through it, our filter was selected to transmit only frequencies that the light sensor will respond to. Apparently, the sensor can be inactivated by infrared light, which the filter should block. </p>
 +
<p> At the time of this writing our strategy is two fold: to experiment with more powerful light sources than the lamp we currently use, and to conduct more rigorous verification of the light sensor plasmids' integrity. </p>
 +
<p> <em>3) Biobrick Light Sensor Subparts (I15008, I15009, I15010, S03321, S03322, S03410, S03417, S03422)</em>
 +
<p> While working with (and having trouble with) the full Biobrick light sensor M30109, we also entertained constructing a new copy of it from its subparts (listed). Many of these components proved to be just as unstable as M30109 itself, producing erratic PCR and digest results. Work on these subparts was dropped, but recently we returned to these parts as alternatives to one or the other of the original two plasmids. Construction had begun with biobrick parts S03410 and S03422, which contain between them the same genes as the pPL-PCB plasmid. Unfortunately this procedure was incomplete as of the end of the iGEM'07 work period, . </p>
 +
<img src="https://static.igem.org/mediawiki/2007/8/81/Aug7_M30109_source_parts.jpg" alt="August 7 m30109 source parts" />
</body>
</body>
</html>
</html>

Latest revision as of 06:43, 19 December 2007

back to U of C Homepage Check out evoGEM

The Logic Circut

The application below shows the schematics of both the complex and simple systems. Hovering over a part with the mouse will highlight its corresponding description in the table. Clicking on a part in the diagram will open the registry's page that desribes the part.

NOTE: if you are viewing this page with internet explorer you will have to click on the application once before you can use it

We planned to build the simple system diagrammed above in order to eventually express agarase through laser activation of E. coli. Since we had many of the parts already in composite form, the goal was to attach together the 5 composite parts above.


Construction Outline

When constructing a composite part, the two pieces can be classified as an insert and a vector. One piece is entirely cut out of its plasmid (the insert), while in the other plasmid (the vector) an opening is made just in from of the coding region itself (this is backwards in a reverse construction, which we did not use). After the ligation step in the construction, there are several different plasmids in the mix. First, you may have original parent plasmid that was never cut, from both plasmids. The probability of having parent vector plasmid is quite small though, due to the phosphatase treatment in the construction. You may also have insert plasmid that has had the actual insert cut out. Both this and parent insert plasmid will confer a certain antibiotic resistance to any bacteria that will uptake it, and as a result, you will have no way of knowing which bacteria have uncut insert plasmid, cut-out insert plasmid, or your desired construction product. This problem is why it is important that the two parts you are joining together have different resistance markers in their plasmids, or at least that the vector plasmid has a resistance the insert does not. Looking at the four composite parts above that we were planning to use, all of them have only ampicillin resistance. Because of this, before we could start any constructions, we had to confer a new resistance to two of the above composites, and this required a plasmid switch. These involve two items: a plasmid with the required resistance and containing the cell death gene ccdB, and the part you wish to switch. All you need do then is mix the two parent plasmids together, insert the appropriate enzymes to cut out both ccdB your gene, and then ligate. There will be four possible products from this procedure. If ccdB ends up in either its original plasmid or in your old plasmid, any cell that uptakes it will die. If your part ends up in its old plasmid, it will be killed, as it will not have the resistance genes of the new plasmid. Therefore, the only cells that survive will be the ones containing your part in the new plasmid. Plasmid switches were done with parts and I13504 and A340620, moving them into plasmids containing ampicillin and chloramphenicol resistances, as these were to be the vectors in the subsequent construction techniques.

With our two newly modified parts ready, the first step was to attach together R0084 with A340620, and S01414 with I13504. Once the construction of these two composites was complete, overnight cultures were made, and the plasmids isolated. The plan was to then attach together these two composites, but again they both had the same resistance markers. To overcome this problem, we again did a plasmid switch, moving the new composite S01414 + I13504 into a plasmid containing ampicillin and kanamycin. We were then able to attach together our two composites into our final logic circuit.


When designing this system, there were some possible problems noted with a pivotal part in our system, ompF (R0084), the promoter controlled by the light-sensing system.

There were some contradictions in the literature about what this part did, and exactly how it would respond to light. Also, this is not the part that the Texas team used in their project; they used the opposing part ompC. We decided to go ahead and begin testing OmpC, and to begin putting it together with other parts, just in case we had to use it. So every step noted above was done with ompC in place of ompF at the same time. And since ompC exists in two forms in the registry, (R0083 and R0082), both parts were used simultaneously. To test ompC, the part was put onto a GFP test construct, I13504 AC, to check the functioning and reliability of the promoter in both TOP10 and CP919 (the knockout strain needed for functionality of the light sensing system). After both of these new parts were made, they had to be transformed into both CP919 and TOP10. It was expected to glow in TOP10, though not too brightly, and to glow perhaps a little brighter in CP919.


RNA Lock and Keys

One of the parts we were interested in using (for our off-switch) is an RNA lock and key to control translation. The lock first needed to be tested, to see how tight its control really is. To do this, was attached to a GFP testing part I13401 AC, with a constitutive promoter placed in front. Since there should be no way to unlock the RBS in front of the GFP, the cells were not expected to glow at all, and this was indeed the case when we tested the construct out. At the same time the lock test was being constructed, the relevant key was attached to a constitutive promoter, and then this construct attached to the locked GFP. When transformed into E. coli, this construct was expected to glow quite strongly, alas the key proved difficult to work with, and this test has not yet been carried out. Each of these testing procedures was done in parallel, as there were two sets of lock/keys to test out.

Any crosstalk between the two sets of lock/keys also was to be tested. To do this, the key construct 1 would be attached to lock construct 3, and as well 3 onto lock 1. There should be no expression of GFP in either of these crosstalk experiments, or at least no more then the cells containing only a lock construct.

Finally, the rate of control needs to be characterized for the RNA lock/keys. To do this, an inducible promoter was to trigger expression of an RNA key, and for this we were going to use the AHL-induced promoter R0062. First though, we were in need of a standard control, made by attaching R0062 to the GFP testing construct I13504 AC. After that, a constitutive promoter was put in front of S01414 (which is necessary for functioning of the AHL promoter), and the two pieces put together. This construct should not glow in TOP10, until AHL is added, and the speed of this expression should be characterized.

During construction of the lock pieces, another part was made by putting S01414 (RBS and luxR) behind the locked GFP, and before the terminators. This construct should not glow on its own, but should after addition of AHL.

Work With The Light Sensor

The popularity of the light sensing biobrick parts since their release by the '05 Austin iGEM team is the best evidence of how useful a light induced system could be. Light can be easily and accurately applied with the right instruments, and could offer much more precise induction compared with the chemical inducers used today. However, just as the promise of the light sensor has spread, so has it's reputation as a tricky system to work with. Our project plan incorporated the light sensor controlling agarase expression, but most of our efforts on it were spent just trying to duplicate the functionality seen in the '05 Nature brief communication by Levskaya et al.

1) The Biobrick Light Sensor

On our first attempt to use the light sensor we used the Biobrick part M30109, which contains the three genes that code for the light sensor encoded in Biobrick format. M30109 was omitted from the iGEM'07 registry plate distribution by accident, so we made a special request for it from the registry.
The M30109-pSB1AC3 plasmid proved extremely difficult to work with, however. Routine restriction digests and PCR amplifications known to work with the pSB1AC3 plasmid backbone failed completely. CP919 is the light sensor chassis E.coli strain, and experiments with light to test the sensor in CP919 also failed. Ultimately, M30109 was set aside and a different source material for the light sensor was sought. However, before abandoning this part one last PCR probe was done using primers for each of the three light sensor coding regions (biobrick parts I15008, I15009 and I15010). The gel is included below, and it indicates that these three regions are intact in M30109. Why exactly M30109 fails remains a mystery, but given that our primers anneal at the restriction sites flanking Biobrick parts, and that restriction digests of M30109 didn't succeed, the current hypothesis is that a restriction site has mutated or is damaged. Given more time, we might have returned to M30109 to find out what's going on with it.

Gel from August 2nd 2007

2) The Original Two Plasmid Light Sensor

After difficulties with the biobrick light sensor we moved on to the original version of the system: the one developped by Levskaya et al. Jeff Tabor, a former Austin iGEM team member, was kind enough to send us the plasmids pPL-PCB and pCPH8. Colony PCR of the pPL-PCB pCPH8 double transformant we made, using the proven light sensor coding region primers, revealed that the three genes were present, and that double transformation worked.

gel from September 4th 2007 - shows double transformation

The next hurdle was to demonstrate that the system itself could work. CP919 transformed with both plasmids was incubated in light and dark, in the hope of seeing a light sensitive response but none was observed. On a tip from Jeff Tabor that the pPL-PCB plasmid may be unstable, we switched to using only freshly transformed cells in our experiments but this made no difference. Most recently, we acquired a red bandpass filer. A bandpass filter is a lens that allows only light of a certain wavelength to pass through it, our filter was selected to transmit only frequencies that the light sensor will respond to. Apparently, the sensor can be inactivated by infrared light, which the filter should block.

At the time of this writing our strategy is two fold: to experiment with more powerful light sources than the lamp we currently use, and to conduct more rigorous verification of the light sensor plasmids' integrity.

3) Biobrick Light Sensor Subparts (I15008, I15009, I15010, S03321, S03322, S03410, S03417, S03422)

While working with (and having trouble with) the full Biobrick light sensor M30109, we also entertained constructing a new copy of it from its subparts (listed). Many of these components proved to be just as unstable as M30109 itself, producing erratic PCR and digest results. Work on these subparts was dropped, but recently we returned to these parts as alternatives to one or the other of the original two plasmids. Construction had begun with biobrick parts S03410 and S03422, which contain between them the same genes as the pPL-PCB plasmid. Unfortunately this procedure was incomplete as of the end of the iGEM'07 work period, .

August 7 m30109 source parts