Team:Slovenia/Notebook

From 2012.igem.org

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</p>
</p>
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<h2> Cloning </h2>
<h2> Cloning </h2>
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<li>The purity and concentration of the isolated DNA was analysed using NanoDrop. </li>
<li>The purity and concentration of the isolated DNA was analysed using NanoDrop. </li>
</ol>
</ol>
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<h3>Fragment DNA isolation from agarose gel</h3>
<h3>Fragment DNA isolation from agarose gel</h3>
<p><b>AGAROSE ELECTROPHORESIS</b></p>
<p><b>AGAROSE ELECTROPHORESIS</b></p>
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<li>Purity and amount of DNA was determined using NanoDrop. </li>
<li>Purity and amount of DNA was determined using NanoDrop. </li>
</ol>
</ol>
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<h3>RESTRICTION DIGEST</h3>
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<br/>
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<h3>Restriction digest</h3>
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<ol>
<ol>
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<li>Set up a restriction mixture:
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<li>To digest the desired DNA restriction reactions were prepared as follows: </li>
<ul style="margin-left:15px;"> <b>for analysis of cloned DNA</b>
<ul style="margin-left:15px;"> <b>for analysis of cloned DNA</b>
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           <li>1X optimized Restriction buffer (10X)</li>
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           <li>2µl of the appropriate restriction buffer (10X)</li>
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           <li>0.5 µL restriction enzyme (10 U/µL)</li>
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           <li>0.5 µL restriction enzyme</li>
           <li>Bring volume to 20 µL with nuclease-free water.</li>
           <li>Bring volume to 20 µL with nuclease-free water.</li>
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<i>or</i>
<i>or</i>
<ul style="margin-left:15px;"> <b>for isolation of specific DNA</b>
<ul style="margin-left:15px;"> <b>for isolation of specific DNA</b>
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           <li>1X optimized Restriction buffer 10X</li>
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           <li>2µl of the appropriate restriction buffer (10X)</li>
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           <li>up to 2 µL restriction enzyme 10 U/µL</li>
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           <li>up to 2 µL restriction enzyme </li>
           <li>Bring volume to 50 µL with nuclease-free water.</li>
           <li>Bring volume to 50 µL with nuclease-free water.</li>
</ul>
</ul>
</li>
</li>
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<li>The sample was incubated at optimal temperature for the restriction enzyme(s)</li>
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<li>The sample was incubated at optimal temperature for the restriction enzymes.</li>
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<li> Analysis of fragmented DNA was done by gel electrophoreses (loading dye was added to the samples before loaded on a agarose gel)</li>
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<li>Analysis of fragmented DNA was done by gel electrophoreses. </li>
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<li>Results were documented with</li>
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<li></li>
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<li>Desired DNA fragment was excised and purified using suitable DNA purification kit.</li>
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<li>Desired DNA fragment was excised and purified using suitable DNA purification kit. </li>
</ol>
</ol>
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<br/>
<br/>

Revision as of 18:05, 26 September 2012