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

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c-11.3,9.2-25,13.9-41.1,13.9c-13.5,0-25.3-2.4-35.4-7.2l-0.6-1.3C1831.5,162.6,1832,153,1832.3,138z"/>
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c-11.3,9.2-25,13.9-41.1,13.9c-13.5,0-25.3-2.4-35.4-7.2l-0.6-1.3C1831.5,162.6,1832,153,1832.3,138z"/>
 
</g>
 
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<h1>cDNA Conversion</h1>
 
<h1>cDNA Conversion</h1>
 
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<p> cDNA stands for complementary DNA, and can be described as a double stranded DNA that is made with RNA as template. Our ultimate goal is the sequence the RNA that we have extracted - and with our sequencing method of choice, we need to turn the RNA back into DNA for it to be read properly. To do this, we use a technique known as reverse transcription to read and copy the RNA contents onto a newly made DNA strand, with no genetic information lost!
 
<p> cDNA stands for complementary DNA, and can be described as a double stranded DNA that is made with RNA as template. Our ultimate goal is the sequence the RNA that we have extracted - and with our sequencing method of choice, we need to turn the RNA back into DNA for it to be read properly. To do this, we use a technique known as reverse transcription to read and copy the RNA contents onto a newly made DNA strand, with no genetic information lost!
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<h2>Experiment</h2>
 
<h2>Experiment</h2>
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        <th style= “width: auto”>Sample</th>
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        <th style=“width: auto” >RNA [ng/µL]</th>
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<p><b>Table 1:</b> The average of measured values for each of the samples. Measuring RNA (or DNA) with corresponding Kit resulted in expected results eg. around 10 ng of RNA and very low amount of DNA. </p><br>
 
<p><b>Table 1:</b> The average of measured values for each of the samples. Measuring RNA (or DNA) with corresponding Kit resulted in expected results eg. around 10 ng of RNA and very low amount of DNA. </p><br>
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<h4>Conclusion</h4>
 
<h4>Conclusion</h4>
 
<p>The experiment only investigated interactions between dsDNA and ssRNA, which are not supposed to introduce any bias into the measurement as per manufacturer's information (Source). The remaining question is how would a RNA:DNA hybrid be treated by the dye. It is possible that RNA was not properly digested and therefore remains in the hybrid form. A hybrid could hypothetically be detected by both RNA and DNA specific kit. Unfortunately no proven hybrid sample was available and therefore this hypothesis could not be tested. <br><br>
 
<p>The experiment only investigated interactions between dsDNA and ssRNA, which are not supposed to introduce any bias into the measurement as per manufacturer's information (Source). The remaining question is how would a RNA:DNA hybrid be treated by the dye. It is possible that RNA was not properly digested and therefore remains in the hybrid form. A hybrid could hypothetically be detected by both RNA and DNA specific kit. Unfortunately no proven hybrid sample was available and therefore this hypothesis could not be tested. <br><br>
  
It was concluded that having DNA - RNA mixture does not influence the measurement in a significant way. RNA amount is moderately decreased after addition of DNA into the sample, which would not explain the presence of RNA in cDNA samples. What remains to be investigated is how would a RNA:DNA hybrid influence the measurement. We therefore conclude that the RNA measurement in our samples is accurate and there is RNA present, either as a ssRNA of RNA:DNA hybrid. </p><br><br>
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It was concluded that having DNA - RNA mixture does not influence the measurement in a significant way. RNA amount is moderately decreased after addition of DNA into the sample, which would not explain the presence of RNA in cDNA samples. What remains to be investigated is how would a RNA:DNA hybrid influence the measurement. We therefore conclude that the RNA measurement in our samples is accurate and there is RNA present, either as a ssRNA of RNA:DNA hybrid. </p><br><br>
  
 
<h3>Is RNA template properly digested? Is it carried over with the AMPure XP Beads?</h3>
 
<h3>Is RNA template properly digested? Is it carried over with the AMPure XP Beads?</h3>
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This corresponds with described ability of RNAseH to preferentially digest RNA:DNA hybrids.</p>
 
This corresponds with described ability of RNAseH to preferentially digest RNA:DNA hybrids.</p>
  
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<p><b>Figure 1:</b> Results after digestion with RNases.</p><br>
 
<p><b>Figure 1:</b> Results after digestion with RNases.</p><br>
  
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We have managed to successfully synthesize complementary DNA to our mRNA samples, which unfortunately did contain undigested RNA. A protocol needs to be developed that assures all of the RNA has been removed from the sample prior to the preparation of the library. Moreover, additional troubleshooting needs to be performed to determine why is the digestion not efficient. </p>
 
We have managed to successfully synthesize complementary DNA to our mRNA samples, which unfortunately did contain undigested RNA. A protocol needs to be developed that assures all of the RNA has been removed from the sample prior to the preparation of the library. Moreover, additional troubleshooting needs to be performed to determine why is the digestion not efficient. </p>
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Revision as of 13:33, 15 October 2018