Difference between revisions of "Team:Uppsala/Transcriptomics/Barcoding-Library Preparation"

(Undo revision 454669 by Mk3johnson (talk))
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Additional troubleshooting would need to be performed to adjust the protocols provided by Oxford Nanopore to our application, which was unfortunately not possible in the course of this project due to budgetary and time restrictions. </p>
 
Additional troubleshooting would need to be performed to adjust the protocols provided by Oxford Nanopore to our application, which was unfortunately not possible in the course of this project due to budgetary and time restrictions. </p>
  
<h2 >Conclusion</h2>
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<h2 id="Conc">Conclusion</h2>
  
 
<p>Most issues connected with low sequencing throughput link back to contamination of the library with RNA. If this issue was to be removed, sequencing in sufficient throughput and quality would be possible as shown on the example of sequencing lambda phage gDNA.<br></p>
 
<p>Most issues connected with low sequencing throughput link back to contamination of the library with RNA. If this issue was to be removed, sequencing in sufficient throughput and quality would be possible as shown on the example of sequencing lambda phage gDNA.<br></p>

Revision as of 21:43, 17 October 2018





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