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Team:HKU Hong Kong - 2012</title>

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<li class="topfirst"><a href="https://2012.igem.org/Team:HKU_HongKong" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Home&nbsp;&nbsp;</a></li>

<li class="topmenu"><a href="#" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Team&nbsp;&nbsp;</a>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Team/About_Us.html">

About Us</a></li></font>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Team/Profiles.html">

Profiles</a></li></font>

     <li class="topmenu"><a href="#" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Project&nbsp;&nbsp;</a>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Project/Background.html">

Background</a></li></font>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Project/Future_Implications.html">

Future Implications</a></li></font>

     <li class="topmenu"><a href="#" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Data&nbsp;&nbsp;</a>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/Weekly_Notebook.html">

Weekly Notebook</a></li></font>

       <li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/Bio_Bricks.html">

Bio Bricks</a></li></font>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/Results.html">

Results</a></li></font>

     <li class="topmenu"><a href="#" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Protocols&nbsp;&nbsp;</a>

     <li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/Mol_Protocols.html">

&nbsp;Molecular Cloning&nbsp;</a></li></font>

<li><font size="10"><a href="https://2012.igem.org/Team:HKU_HongKong/Data/pvdQ_Protocols.html">

&nbsp;pvdQ Expression Analysis&nbsp;</a></li></font>

<li class="topmenu"><a href="https://2012.igem.org/Team:HKU_HongKong/Safety.html" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Safety&nbsp;&nbsp;</a></li>     

     <li class="toplast"><a href="https://2012.igem.org/Team:HKU_HongKong/Human_Practice.html" style="height:26px;line-height:26px;">

&nbsp;&nbsp;Human Practice&nbsp;&nbsp;</a></li>

<p style="text-align: justify">&nbsp;</p><h2 style="font-variant: normal; vertical-align: baseline; clear: left; font-family: Gentium Basic; letter-spacing: normal; orphans: 2; text-align: justify; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; padding: 0px; margin-left:0px; margin-right:0px"><span style="font-weight: 400"><font face="Trebuchet MS" size="6"><u>Molecular Cloning Protocols</font></u></span></h2>

<td height="2664">

<p style="font-variant: normal; vertical-align: baseline; clear: left; color: #232323; font-family: Gentium Basic; letter-spacing: normal; orphans: 2; text-align: justify; text-indent: 0px; text-transform: none; white-space: normal; widows: 2; -webkit-text-size-adjust: auto; -webkit-text-stroke-width: 0px; border: 0px none; padding: 0px; margin-left:0px; margin-right:0px">

  <span style="font-family: Trebuchet MS; font-weight: 400; text-decoration: underline">

      <i><font size="4" color="#000000" id="Transforming_Ecoli">

          Transforming Competent E.coli with the  

          Plasmid:</b> </a> <br>

      <br>

      </font></i></span><font color="#000000"></b><font size="2" face="Tahoma">We chose the biobrick  

        K137076 to ligate to the pvdQ gene for the following reasons: </font></font>

  </font></p>

        <ul>

          <li><font face="Tahoma" size="2" color="#000000">Take out the competent E-coli  

            cells from the -80 freezer. (Keep all tubes on ice).</font></li>

          <li><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">Add 1uL  

            of the plasmid DNA in 100uL competent cells (if from Kit). For  

            transformation of ligated product, add 10uL of the ligated plasmid DNA in  

            100uL competent cells.</span></font></li>

          <li>

            <font color="#000000">

            <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

            Incubate on ice for 10 min. </span></font></li>

          <li><font color="#000000">

            <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">Place  

            in water bath at 42°C for 90s.</span></font></li>

          <li><font color="#000000">

            <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">Place  

            immediately back on ice for at least 2 min.</span></font></li>

          <li><font color="#000000">

            <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">Add  

            800uL LB </span></font><font size="2" color="#000000">

            <span style="font-family: Tahoma; font-weight: 400">broth. Incubate for 1hr  

            at 37°C shaker</span></font><font color="#000000"><span style="font-size:11.0pt;font-family:&quot;Times New Roman&quot;,&quot;serif&quot;">.</span></font></li>

          <li><font size="2" color="#000000" face="Tahoma">Centrifuge at 130rpm for 5min  

            to remove supernatant. Re-suspend the pellet in about 10uL of supernatant.</font></li>

          <li><font face="Tahoma" size="2" color="#000000">Spread the entire re-suspended  

            pellet on ampicillin agar dishes.</font></li>

          <li><font face="Tahoma" size="2" color="#000000">Incubate for 12-16 hours at 37

            </font><font color="#000000">

            <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">°C.</span></font></li>

        </ul>

      Notes:</span></b></font></p>

<font color="#000000">

<span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

Colonies grown on plate were selected for colony PCR screening.</span></font><br>

<font color="#000000">

<span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">-  

Correct colonies were then cultured in 5 mL LB Broth with 0.5uL  

ampicillin for subsequent screening or mass culturing. </span>

<br>

</font><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">-  

      Mass culturing involved adding 200uL of the culture into 35mL LB Broth  

      with 35uL ampicillin. </span></font></p>

<p class="MsoNormal" style="text-autospace: none; text-align: left"><font color="#000000" size="4"><b>

  <u>

      <span style="font-family: Trebuchet MS; "><i>

<a name="Miniprep_to_Extract_the_Plasmid_from_E.coli_(QIAprep_Spin_Miniprep_Kit):__">

Miniprep to Extract the Plasmid from E.coli (QIAprep Spin Miniprep Kit):

</a> </i></span>

      </u></b></font></p>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Transfer some of the 5mL bacterial culture into a microcentrifuge  

        tube. Pellet by centrifugation at 13,500 rpm for 1 min. Repeat till  

        all the culture has been pelleted. </font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Resuspend the pellet in 250uL Buffer P1. </font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Add 250uL Buffer P2 (Lysis Buffer). Mix thoroughly by inverting the  

        tube 4-6 times. Do not allow prolonged lysis.</font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Immediately add 350uL Buffer N3 (Neutralization Buffer). Mix  

        immediately by inverting the tube. </font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Centrifuge for 10 minutes at 13,500 rpm. </font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Apply the resulting supernatant to the QIAprep spin column by  

        pipetting. Centrifuge for 1 minute at 13,500 rpm. </font></span>

      </li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Wash the QIAprep spin column by applying 0.75mL Buffer PE.  

        Centrifuge for 1 minute at 13,500 rpm.</font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Centrifuge for an additional 1 minute to remove residual ethanol.

        </font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Place the QIAprep spin column in microcentrifuge tube. Elute DNA by  

        adding 50uL warm H₂O. </font></span></li>

  <li>

    <span style="font-family: Tahoma; font-weight: 400">

        <font size="2" color="#000000">

        Centrifuge for 1 minute at 13,500 rpm.</font></span></li>

  </ul>

<p style="text-autospace: none; text-align: left; "><font color="#000000"><u><span style="font-size: 14pt; font-family: Trebuchet MS; font-style: italic">

<a name="Midiprep_for_Large_Volumes_of_Culture_(QIAGEN_Plasmid_Midi_Kit):_">Midiprep for Large Volumes of Culture (QIAGEN Plasmid Midi Kit):

</a> </span>

  </u></font></p>

<p class="MsoNormal" style="text-autospace: none; text-align: left; ">

  <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      Refer to the QIAGEN website for the protocol. </span></font></p>

<p class="MsoNormal" style="text-autospace: none; text-align: left; ">

  <font color="#000000"><u>

      <span style="font-size: 14pt; font-family: Trebuchet MS; font-style: italic">

      <a name="PCR_Amplification_of_Gene_from_Bacterial_Genome/Standard_Biobrick_Parts_">PCR Amplification of Gene from Bacterial Genome/Standard Biobrick Parts

      </span></u></font></p>

<p class="MsoNormal" style="text-autospace: none; text-align: left; "><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

  37.5μL &nbsp;&nbsp;ddH2O</span></font><br>

  <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      5.0μL&nbsp;&nbsp;&nbsp;&nbsp; 10x PCR Buffer</span></font><br>

      <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      2.5μL &nbsp;&nbsp;&nbsp;&nbsp;dNTPs</span></font><br>

      <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      1.0μL&nbsp;&nbsp;&nbsp;&nbsp; Forward Primer (Prefix)</span></font><br>

      <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      1.0μL &nbsp;&nbsp;&nbsp;&nbsp;Reverse Primer (Suffix)</span></font><br>

      <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      1.0μL &nbsp;&nbsp;&nbsp;&nbsp;Template DNA<br>

      </span></font><font color="#000000"><u><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">1.0  

    μL &nbsp;&nbsp;&nbsp;RTaq DNA Polymerase</span></u></font><br>

    <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

    50.0μL Total</span></font> </p>

        <font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400"><u>Note: </u><br>

after which gel purification needs to be carried out. </span><br>

        </font><font size="2" color="#000000"><span style="font-family: Tahoma">-<span style="font-weight: 400">

        </span></span></font><font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">The  

        volume of DNA used in the second PCR reaction depends on the  

          concentration of the DNA after the PCR Clean-up. </span></font>

<p class="MsoNormal" style="text-autospace: none; text-align: left"><font color="#000000"><i><u><span style="font-size: 14pt; font-family: Trebuchet MS">

<a name="PCR_Clean-Up_–_Qiagen_QIAquick_PCR_Purification:_">PCR Clean-Up –  

Qiagen QIAquick PCR Purification: </a> </span></u></i></font>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Add 5 volumes of Buffer PB to 1 volume of PCR mix. </span></font>

      </li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Place this mix within the QIAquick column. Centrifuge at 13,500 rpm  

        for 1 minute. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Discard flow through and centrifuge again to allow all the sample to  

        pass through.</span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Wash with 750uL Buffer PE. Centrifuge at 13,500 rpm for 1 minute.

        </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Discard flow through and centrifuge again to remove all residual  

        buffer. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Place the column in a micro centrifuge tube. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Apply 50uL of pre-warmed distilled H2O to the column. Stand for at  

        least 2 minutes.</span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Centrifuge at 13,500 rpm for 1 minute. </span></font></li>

  </ul>

<p class="MsoNormal" style="text-autospace: none; text-align: left"><font color="#000000"><u>

<a name="Colony_PCR_"><i><font face="Trebuchet MS"><span style="font-size: 10pt">Colony PCR</span></font></i></a></u><a name="Colony_PCR_">

          </font>

  <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

  <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

2.0μL &nbsp;&nbsp;&nbsp;&nbsp;10x PCR Buffer</span></font><br>

<font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      1.6μL &nbsp;&nbsp;&nbsp;&nbsp;dNTPs</span></font><br>

      <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      0.4μL &nbsp;&nbsp;&nbsp;&nbsp;Forward Primer (Prefix)</span></font><br>

      0.4μL &nbsp;&nbsp;&nbsp;&nbsp;Reverse Primer (Suffix)</span></font><br>

      <font color="#000000"><u>

      20.0μL Total</span></font></p>

  &nbsp;<font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400"><u>Notes</u>: </span></font>      

  <font size="2" color="#000000"><span style="font-family: Tahoma">-<span style="font-weight: 400">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">The

materials were kept on ice</span></font><br>

<font size="2" color="#000000"><span style="font-family: Tahoma">-<span style="font-weight: 400">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">PCR  

      Reaction: 95°C - 10 min</span></font></p>

  <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;  

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;95°C - 30 sec</span></font><br>

      <font color="#000000">

  <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;  

&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;57°C - 30 sec (appropriate annealing temperature for prefix and  

suffix)</span></font><br>

<font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;  

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;72°C - 30 sec </span>

      </font><br>

      <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;  

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;(<i>28 cycles all together)</i></span></font><br>

      <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;  

      &nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;&nbsp;72°C - 5 min </span>

      </font></p>

<p class="MsoNormal" style="text-autospace: none; text-align: left"><font color="#000000"><u>

<a name="Agarose_Gel_Electrophoresis_"><span style="font-size: 12pt; font-family: Trebuchet MS; font-style: italic">Agarose Gel Electrophoresis</span></a></u></font><a name="Agarose_Gel_Electrophoresis_">

</a>      

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Prepare a 2% or 1% Agarose Gel (amount in grams depending on volume  

        of TAE buffer used). Add 0.1% Ethidium Bromide of the total volume.

        </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Place the gel in the Electrophoresis Apparatus with the wells facing  

        the Negative Electrode. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Fill the apparatus with 1% TAE Buffer to fully submerge the wells.

        </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Load 5µL of 1kb Ladder for each Run </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Add 0.1% of 10% Loading Dye to the respective volume of sample. Mix  

        well and spin down. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Pipette the samples into the wells and run at 106 Volts. </span>

        </font></li>

  </ul>

<p class="MsoNormal" style="text-autospace: none; text-align: left; ">

  <font color="#000000"><u><font size="3">

          <span style="font-family: Trebuchet MS; font-style: italic">

<a name="Gel_Purification_of_DNA_(Qiagen_QIAquick_Gel_Extraction_Kit)">Gel  

          Purification of DNA (Qiagen QIAquick Gel Extraction Kit)</a></span></font></u></font></p>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Exercise the DNA fragment from the Agarose Gel using a scalpel.  

        Minimize the extra peripheral gel slice. </span></font></li>

  <li>

    <font face="Tahoma" size="2" color="#000000">Weigh the </font>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        gel slice (0.1g = 100uL) and add 3 Volumes of Buffer QG to every 1  

        Volume of Gel. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Incubate in 50°C water bath for 10 minutes to completely dissolve  

        the gel slice.</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Add 1 Volume of  

        Isopropanol to the sample. Mix well</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Apply the sample  

        to the QIAquick column. Centrifuge at 13,500 rpm for 1 minute.  

        [Repeat till the total volume of the sample has sieved through the  

        column]. Discard the flow through</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Apply </span>

        </font><font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

            0.5mL Buffer QG to the QIAquick column. Centrifuge at 13,500 rpm for  

            1 minute.</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Discard the flow  

        through</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Wash the column  

        with 0.75mL Buffer PE. Centrifuge at 13,500 rpm for 1 minute.</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Discard the flow  

        through and Centrifuge at 13,500 rpm for an additional 1 minute to  

        eliminate any residual ethanol.</span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Place the QIAquick column into a 1.5mL Eppendorf tube.</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-family: Tahoma; font-weight: 400">Apply the </span>

        </font><font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

            30uL warm H₂O to the column. Let the column stand for at  

            least 1 minute.</span></font></li>

  <li>

    <font size="2" color="#000000">

        <span style="font-weight: 400; font-family: Tahoma">Centrifuge at  

        13,500 rpm for 1 minute.<br>

        &nbsp;</span></font></li>

  </ul>

<p class="MsoNormal" style="text-autospace: none; text-align: left; margin-left: 0pt; margin-right: 10.0pt; ">

  <font color="#000000"><u>

      <span style="font-size: 12pt; font-family: Trebuchet MS; font-style: italic">

      <a name="Determining_DNA_Concentration_Using_NanoDrop_Spectrophotometry">Determining DNA Concentration Using NanoDrop Spectrophotometry</a></span></u></font></p>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Choose the Nucleic Acid Measurement option in the programme. </span>

        </font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Initialize the NanoDrop by adding 1uL clean H₂O. Clean  

        the sensor gently with tissue. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Set Blank by adding an additional 1uL of clean H₂O. Wipe  

        off. </span></font></li>

  <li>

    <font color="#000000">

        <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

        Add 1uL of the DNA sample to be measured. Wipe off after each run.

        </span></font> </li>

<p class="MsoNormal" style="text-autospace: none; text-align: left; margin-left: 0pt; margin-right: 10.0pt; ">

  <font color="#000000"><u>

      <span style="font-size: 12pt; font-family: Trebuchet MS; font-style: italic">

      <a name="DNA_Digestion_">DNA Digestion </a> </span></u></font></p>

<font color="#000000">

__μL &nbsp;&nbsp;ddH2O (to a total of 40uL)</span></font><br>

<font color="#000000">

4μL&nbsp;&nbsp;&nbsp;&nbsp; 10X NEBuffer</span></font><br>

      0.4μL&nbsp; 100X BSA</span></font><br>

          fact that 5 units of enzyme digest 1ug DNA.</span></font></p>

  <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">&nbsp;</span><span style="font-size: 12pt; font-family: Trebuchet MS; font-style: italic"><u>Dephosphorylation of 5&#39; Ends of Vector Backbone</u></span></a></font></p>

            - In</span></font><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">cubate at 37°C for 30 minutes</span></font><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">&nbsp;</span></font></p>

      <a name="Vector-Insert_Ligation">Vector-Insert Ligation</a></span></u></font></p>

<font color="#000000">

Autoclaved ddH2O (to a total of 20uL)</span></font><br>

<font color="#000000">

2μL&nbsp;&nbsp;&nbsp; T4 Ligase Buffer</span></font><br>

      20μL &nbsp;Total</span></font></p>

  <font color="#000000"><u>

      <span style="text-decoration: none; font-size: 10pt; font-family: Tahoma; font-weight: 400">

      &nbsp;</span></u></font><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400; text-decoration: underline">Notes:</span></font></p>

<p class="MsoNormal" style="text-autospace: none; text-align: left; ">

  <font size="2" color="#000000"><span style="font-family: Tahoma">-<span style="font-weight: 400">

      </span></span></font><font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

          Insert and Vector must be in a 3:1 ratio. The amount of each depends on  

          their concentration (ng/uL) and legnth (bp). </span></font><br>

          <font size="2" color="#000000"><span style="font-family: Tahoma">-<span style="font-weight: 400">  

I</span></span></font><font color="#000000"><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">ncubate  

<p class="MsoNormal" style="text-autospace: none; text-align: left; "><font color="#000000">

  <span style="font-size: 12pt; font-family: Trebuchet MS; font-style: italic; text-decoration: underline">

      <a name="PCR_Deletion_(Site-Directed_Mutagenesis)_Reaction">PCR Deletion (Site-Directed Mutagenesis) Reaction</a></span></font></p>

  <font color="#000000"><u>

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      Note</span></u><span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">:  

          Keep everything on ice and add all volumes in a PCR tube.</span></font></p>

<font color="#000000">

50µL)</span></font><br>

<font color="#000000">

5.0μL 10x PfuUltra buffer</span></font><br>

<font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      1.0μL dNTPs</span></font><br>

      <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">?  

      uL forward primer = 125ng fwd primer ÷ fwd primer concentration (ng/µL)</span></font><br>

      <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">?  

      uL reverse primer = 125ng rvs primer ÷ rvs primer concentration (ng/µL)</span></font><br>

      <font color="#000000">

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">?  

      µL dsDNA= 20ng insert ÷ insert concentration (ng/µL)</span></font><br>

      <font color="#000000"><u>

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      1.0μL </span></u>

      <span style="font-size: 10pt; font-family: Tahoma; font-weight: 400">

      PfuUltra<u> high-fidelity DNA polymerase</u></span></font><br>

      <font color="#000000">