Difference between revisions of "Team:Uppsala/Transcriptomics/PolyA Tailing"

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As you might already know no work is done for free, and that is the case for the poly(A) polymerase. Thereby ATP is added, which is an energy molecule that activates the poly(A) polymerase. The mRNA is then analyzed with gel-electrophoresis to confirm that the poly(A) tail attachment was a success. It can be noted that we had some difficulties in acquiring good results initially from this step, which included degradation and apparent non-existing tailing of the samples. After several attempts however, and a complete change in Poly(A)-tailing reagents, the procedure started to work properly.</p>
 
As you might already know no work is done for free, and that is the case for the poly(A) polymerase. Thereby ATP is added, which is an energy molecule that activates the poly(A) polymerase. The mRNA is then analyzed with gel-electrophoresis to confirm that the poly(A) tail attachment was a success. It can be noted that we had some difficulties in acquiring good results initially from this step, which included degradation and apparent non-existing tailing of the samples. After several attempts however, and a complete change in Poly(A)-tailing reagents, the procedure started to work properly.</p>
 
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<h2 id="Resu">Result</h2>
 
 
  
 
 
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    <p>A successful poly(A) tailed mRNA has a complete chain of adenosines connected to the 3’UTR of the mRNA strand. Initially, the adition of polyA has been very inefficient due to among other reasons low enzyme concentrations. Using double the recommended amount of enzyme, we managed to successfully attach of polyA tail to RNA. To be able to clearly illustrate the polyadenylation, we have added polyA tails to RNA ladder as can be seen in <b>Figure 1 </b>. The shift in size is especially well visible for the lowest 200 bp band.</p><br><br>
 
 
    <p>Equal enzyme concentrations as those used in the RNA ladder polyadenylation were used to attach polyA tails to the isolated mRNA. The increase in polyA polymerase concentration has resulted in significantly higher cDNA yields, as decribed <a href="https://2018.igem.org/Team:Uppsala/Transcriptomics/cDNA_Conversion">here</a></p><br><br>
 
 
                    
 
                    
 
                            
 
                            
 
                          
 
                          
 
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                        <h2 id="Resu">Result</h2>
  
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                                <p>A successful poly(A) tailed mRNA has a complete chain of adenosines connected to the 3’UTR of the mRNA strand. Initially, the adition of polyA has been very inefficient due to among other reasons low enzyme concentrations. Using double the recommended amount of enzyme, we managed to successfully attach of polyA tail to RNA. To be able to clearly illustrate the polyadenylation, we have added polyA tails to RNA ladder as can be seen in <b>Figure 1 </b>. The shift in size is especially well visible for the lowest 200 bp band.</p><br><br>
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    <p>Equal enzyme concentrations as those used in the RNA ladder polyadenylation were used to attach polyA tails to the isolated mRNA. The increase in polyA polymerase concentration has resulted in significantly higher cDNA yields, as decribed <a href="https://2018.igem.org/Team:Uppsala/Transcriptomics/cDNA_Conversion">here</a></p><br><br>
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  <p><b>Figure 1.</b> A successful poly(A) tail attachment onto RiboRuler High Range RNA Ladder (Thermo Fisher Scientific). The polyadnenylation is clearly visible on the bottom 200 bp band.</p>
 
  <p><b>Figure 1.</b> A successful poly(A) tail attachment onto RiboRuler High Range RNA Ladder (Thermo Fisher Scientific). The polyadnenylation is clearly visible on the bottom 200 bp band.</p>
 
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Revision as of 00:14, 18 October 2018