Difference between revisions of "Team:Uppsala/Transcriptomics/cDNA Conversion"

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<h4>Set up:</h4>  
 
<h4>Set up:</h4>  
<p>This troubleshooting experiment had three major parts: i) optimizing the protocol for the use of RNase Cocktail using longer incubation time and/or larger quantity, ii) use of RNAse H for digestion and iii) clean-up step with purification beads to determine whether the beads have affinity for RNA.<br><br>
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<p>This troubleshooting experiment had three major parts: i) optimizing the protocol for the use of RNase Cocktail using longer incubation time and/or larger quantity, ii) use of RNAse H for digestion and iii) clean-up step with purification beads to determine whether the beads have affinity for RNA.</p><br>
<b>i)</b> Total of 8 samples with 125 ng of RNA were prepared (from previous cDNA samples that shown RNA contamination, eg. there was DNA present in the samples as well). The experiment was optimized for time and amount of RNase Cocktail. <br><br>
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<h5><b>1.</b></h5>
<b>ii)</b> RNA ladder was digested using both RNase H, RNAse Cocktail or both. Also each of the tests was prepared in either RNase-free water or buffer solution used during the cDNA synthesis. Digested DNA was visualised on a gel. <br><br>
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<p>Total of 8 samples with 125 ng of RNA were prepared (from previous cDNA samples that shown RNA contamination, eg. there was DNA present in the samples as well). The experiment was optimized for time and amount of RNase Cocktail.</p> <br>
<b>iii)</b> 1000 ng of RNA ladder were purified using AMX beads and shown on a gel.</p>
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<h5><b>2.</b></h5> 
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<p>RNA ladder was digested using both RNase H, RNAse Cocktail or both. Also each of the tests was prepared in either RNase-free water or buffer solution used during the cDNA synthesis. Digested DNA was visualised on a gel. </p><br>
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<h5><b>3.</b></h5> 
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<p>1000 ng of RNA ladder were purified using AMX beads and shown on a gel.</p>
  
 
<h4>Results:</h4>  
 
<h4>Results:</h4>  

Revision as of 09:41, 15 October 2018