Difference between revisions of "Team:Uppsala/Transcriptomics/Bioinformatics"

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                             <p><b>Figure 1:</b>Running demultiplexing and barcode trimming from the terminal. The programme first separates the reads according to barcode and then searches for available possible barcodes to be trimmed off.</p>
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                             <p><b>Figure 1:</b> Running demultiplexing and barcode trimming from the terminal. The programme first separates the reads according to barcode and then searches for available possible barcodes to be trimmed off.</p>
 
                              
 
                              
  
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                             <p><b>Figure 2:</b>Results of a differential gene expression analysis using Deseq2 on test files. The genes (shown with their gene ID) as well as their mean base length and several statistical results can be seen..</p>
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                             <p><b>Figure 2:</b> Results of a differential gene expression analysis using Deseq2 on test files. The genes (shown with their gene ID) as well as their mean base length and several statistical results can be seen..</p>
 
                              
 
                              
  
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<p>After the differential gene expression analysis is done the data was filtered twice, one time for the best adjusted P-value and subsequently for the highest (meaning the most significant) fold changes. Left were a couple of candidate genes which could be easily identified by their gene ID through various databases such as NCBI.</p>
  
 
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Revision as of 17:40, 15 October 2018