Difference between revisions of "Team:Uppsala/Transcriptomics/rRNA Depletion"

 
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<p>rRNA stands for ribosomal RNA and constitutes a large part of the cells ribosomes. In fact, about 90% of the total RNA content of the cell is rRNA, with the rest being microRNA, tRNA and mRNA. While the rRNA has been very useful for RNA quality control in the previous step of the pipeline, it actually holds no genetic information of value for us and can be removed to make the RNA sample clearer and lighter in preparation for the coming steps.</p>
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<p>rRNA stands for ribosomal RNA and constitutes a large part of the cells ribosomes. In fact, about 90% of the total RNA content of the cell is rRNA, with the rest being microRNA, tRNA and mRNA. While the rRNA has been very useful for RNA quality control in the previous step of the pipeline, it actually holds no genetic information of value for us and can be removed to make the RNA sample more clear and lighter in preparation for the coming steps.</p>
  
 
<h2 id="Exp">Experiment</h2>
 
<h2 id="Exp">Experiment</h2>
  
<p>We performed our rRNA depletions using Thermo Fishers MICROBexpress Bacterial mRNA Enrichment Kit. This kit utilizes magnetic beads which are primed to capture and bind the rRNA to them. These beads are added to the sample. Using a magnet, the beads can then be pulled to the side of the sample tube and the eluate can be pipetted, giving us an RNA sample free of rRNA[1]! A total of 10000ng of total RNA is used for each sample in the rRNA depletion step.<br><br>
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<p>We performed our rRNA depletions using Thermo Fishers MICROBExpress Bacterial mRNA Enrichment Kit. This kit utilizes magnetic beads which are primed to capture and bind the rRNA to them. These beads are added to the sample. Using a magnet, the beads can then be pulled to the side of the sample tube and the eluate can be pipetted, giving us an RNA sample free of rRNA [1]. A total of 10000ng of total RNA is used for each sample in the rRNA depletion step.<br><br>
  
 
As with more of the following steps of this pipeline, this procedure requires several chemicals and other reagents to function. These agents remain in the RNA sample after the depletion and can interfere with following steps of refining the RNA. They are removed by precipitation, which forces the RNA out of the solution and allows us to collect it by centrifugation[1, 2].<br><br>
 
As with more of the following steps of this pipeline, this procedure requires several chemicals and other reagents to function. These agents remain in the RNA sample after the depletion and can interfere with following steps of refining the RNA. They are removed by precipitation, which forces the RNA out of the solution and allows us to collect it by centrifugation[1, 2].<br><br>
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                             <p><b>Figure 1.</b> This figure shows a gel electrophoresis comparison between totalRNA and our two selected samples which have undergone rRNA depletion. S.1 is w16_2, while S.2 is c16_2. While both samples have clearly had rRNA removed from them, some still appear to remain in S.1 </p>   
 
                             <p><b>Figure 1.</b> This figure shows a gel electrophoresis comparison between totalRNA and our two selected samples which have undergone rRNA depletion. S.1 is w16_2, while S.2 is c16_2. While both samples have clearly had rRNA removed from them, some still appear to remain in S.1 </p>   
 
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<h2 id="Conc">Conclusion</h2>
 
<h2 id="Conc">Conclusion</h2>
<p>These results can generally be seen as acceptable and can be moved on to the next step of the process.<br><br>In many cases, a successful rRNA depletion results in a loss of up to 90% of the total nucleic acid contents of the cell [4]. A significantly smaller loss may raise suspicions of inadequate rRNA removal. This may be due to several reasons - such as poor dispersion of the magnetic beads throughout the sample, causing less of the beads to bind the the rRNA molecules. It can also be due to poor separation of the magnetic beads from the eluate (eg. not enough time on the magnet), or by overloading the sample by introducing too much input RNA [1]. We selected two out of the four samples to go forward with and verified the rRNA removal with gel electrophoresis. The results from the gel indicated rRNA removal in both samples, although not perfect results and not equal between the samples. From our experience, a total rRNA removal is very difficult to obtain using our method, and we deemed the two samples as good to go for the next step.</p>  
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<p>These results can generally be seen as acceptable and can be moved on to the next step of the process.<br><br>In many cases, a successful rRNA depletion results in a loss of up to 90% of the total nucleic acid contents of the cell [4]. A significantly smaller loss may raise suspicions of inadequate rRNA removal. This may be due to several reasons - such as poor dispersion of the magnetic beads throughout the sample, causing less of the beads to bind the rRNA molecules. It can also be due to poor separation of the magnetic beads from the eluate (eg. not enough time on the magnet), or by overloading the sample by introducing too much input RNA [1]. We selected two out of the four samples to go forward with and verified the rRNA removal with gel electrophoresis. The results from the gel indicated rRNA removal in both samples, although not perfect results and not equal between the samples. From our experience, a total rRNA removal is very difficult to obtain using our method, and we deemed the two samples as good to go for the next step.</p>  
  
 
<h3> Precipitation</h3>
 
<h3> Precipitation</h3>
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<b>Ethanol:</b> The ethanol on the other hand has the function of simplify the interaction between the nucleic acids and the salt. The salt in combination with the ethanol forces the nucleic acids to precipitate and can thereby be separated from the water with centrifugation.<br><br>
 
<b>Ethanol:</b> The ethanol on the other hand has the function of simplify the interaction between the nucleic acids and the salt. The salt in combination with the ethanol forces the nucleic acids to precipitate and can thereby be separated from the water with centrifugation.<br><br>
 
<b>Glycogen:</b> It is important that the visibility of the RNA pellet is good enough to avoid touching it when pipetting the supernatant. When adding the glycogen the pellet gets more visible due to the fact that glycogen is a polysaccharide and cannot be dissolved in alcohols. Thereby when the glycogen is added into the RNA sample, nucleic acids will get trapped and get precipitated with the glycogen.<br><br>
 
<b>Glycogen:</b> It is important that the visibility of the RNA pellet is good enough to avoid touching it when pipetting the supernatant. When adding the glycogen the pellet gets more visible due to the fact that glycogen is a polysaccharide and cannot be dissolved in alcohols. Thereby when the glycogen is added into the RNA sample, nucleic acids will get trapped and get precipitated with the glycogen.<br><br>
<b>Glycoblue:</b> Another complementary method to visualize the RNA pellet is to dye it. GlycoBlue is a blue dye that binds specific to glycogen, contributing of making the pellet even more visible. Thereby it will be easier for the user to pipette with less chance of touching the pellet.</p>
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<b>Glycoblue:</b> Another complementary method to visualize the RNA pellet is to dye it. GlycoBlue is a blue dye that binds specifically to glycogen, making the pellet even more visible. Thereby it will be easier for the user to pipette with less chance of touching the pellet.</p>
  
  
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<h2 id="References">References</h2>
 
<h2 id="References">References</h2>
<p><b>[1]</b> Thermo Fisher, 2018. MICROBExpress™ Kit Protocol (PN 1905 Rev C) <a href="https://assets.thermofisher.com/TFS-Assets/LSG/manuals/cms_057051.pdf">https://assets.thermofisher.com/TFS-Assets/LSG/manuals/cms_057051.pdf</a> Date of visit 2018-10-15</p><br>
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<p><b>[1]</b> Thermo Fisher, 2018. MICROBExpress™ Kit Protocol (PN 1905 Rev C) <a href="https://assets.thermofisher.com/TFS-Assets/LSG/manuals/cms_057051.pdf">https://assets.thermofisher.com/TFS-Assets/LSG/manuals/cms_057051.pdf</a> Date of visit 2018-10-15</p>
<p><b>[2]</b> Walker, SE, Lorsch J. 2013. Chapter Nineteen - RNA Purification - Precipitation Methods. Methods in Enzymology, 530. p.337-343.</p><br>
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<p><b>[2]</b> Walker, SE, Lorsch J. 2013. Chapter Nineteen - RNA Purification - Precipitation Methods. Methods in Enzymology, 530. p.337-343.</p>
<p><b>[3]</b> Thermo Fisher, 2018. Qubit Flourometric Quantitation. <a href="https://www.thermofisher.com/se/en/home/industrial/spectroscopy-elemental-isotope-analysis/molecular-spectroscopy/fluorometers/qubit.html">https://www.thermofisher.com/se/en/home/industrial/spectroscopy-elemental-isotope-analysis/molecular-spectroscopy/fluorometers/qubit.html</a> Date of visit 2018-10-15</p><br>
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<p><b>[3]</b> Thermo Fisher, 2018. Qubit Flourometric Quantitation. <a href="https://www.thermofisher.com/se/en/home/industrial/spectroscopy-elemental-isotope-analysis/molecular-spectroscopy/fluorometers/qubit.html">https://www.thermofisher.com/se/en/home/industrial/spectroscopy-elemental-isotope-analysis/molecular-spectroscopy/fluorometers/qubit.html</a> Date of visit 2018-10-15</p>
 
<p><b>[4]</b> Petrova OE, Garcia-Alcalde F, Zampaloni C, Sauer K. 2017. Comparative evaluation of rRNA depletion procedures for the improved analysis of bacterial biofilm and mixed pathogen culture transcriptomes. Scientific Reports 7, Article number: 41114.
 
<p><b>[4]</b> Petrova OE, Garcia-Alcalde F, Zampaloni C, Sauer K. 2017. Comparative evaluation of rRNA depletion procedures for the improved analysis of bacterial biofilm and mixed pathogen culture transcriptomes. Scientific Reports 7, Article number: 41114.
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Latest revision as of 09:57, 3 December 2018