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

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                     <p>The resuts from our runs unfortunately did not produce as good results as seen above. Due to the major issues with sequencing and actually generating enough data, it can be seen in <b>figure 6</b> what kind of effects it had. Judging by the adjusted p-values it is clear that even though the genes can indeed be identified the statistical significance is extremely uncertain (the minimal accepted threshold is an adjusted p-value of <= 0.05). Any up-or down regulation of fold-change of interest was not able to be identified either. Looking at these errors it can be assumed that no major change in fold-change as well as low significancy is due to simply not enough data being generated from the prior sequencing step. Because of these facts no gene could be identified as a possible candidate for our reporter system.</p>
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                     <p>The resuts from our runs unfortunately did not produce as good results as seen above. Due to the major issues with sequencing and actually generating enough data, it can be seen in <b>figure 6</b> what kind of effects it had. Judging by the adjusted p-values it is clear that even though the genes can indeed be identified as seen in <b>Table 1</b> the statistical significance is extremely uncertain (the minimal accepted threshold is an adjusted p-value of <= 0.05). Any up-or down regulation of fold-change of interest was not able to be identified either. Looking at these errors it can be assumed that no major change in fold-change as well as low significancy is due to simply not enough data being generated from the prior sequencing step. Because of these facts no gene could be identified as a possible candidate for our reporter system.</p>
 
                      
 
                      
 
                     <h1>References</h1>
 
                     <h1>References</h1>

Revision as of 19:39, 17 October 2018





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