Difference between revisions of "Team:UParis BME/Wetlab"

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<p class="textContent">We used a medium based on DMEM +10% of FBS for cell culture and phosphate buffered saline (PBS) to wash the cells and remove the dead ones. Due to the cell adhesion on the interior surface of the flask we used the trypsin to detach them and later resuspended them in the medium. This technique is used to grow the targeted cell line until we reach a good confluency (between 80-90%). Cells were regularly tested negative for mycoplasma contamination, and no contamination was detected. </p>
 
<p class="textContent">We used a medium based on DMEM +10% of FBS for cell culture and phosphate buffered saline (PBS) to wash the cells and remove the dead ones. Due to the cell adhesion on the interior surface of the flask we used the trypsin to detach them and later resuspended them in the medium. This technique is used to grow the targeted cell line until we reach a good confluency (between 80-90%). Cells were regularly tested negative for mycoplasma contamination, and no contamination was detected. </p>
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<p class="textContent"><a href="https://static.igem.org/mediawiki/2021/f/f4/T--UParis_BME--cellculture.pdf">Protocol Adherent Cell culture</a></p>
  
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<h4>Exosome Extraction and miRNAs isolation</h4>
  
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<p class="textContent"> to completed </p>
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<p class="textContent"><a href="https://static.igem.org/mediawiki/2021/7/7a/T--UParis_BME--exosome_extraction.pdf">Protocol Exosome extraction</a></p>
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<p class="textContent"> to completed </p>
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<p class="textContent"><a href="https://static.igem.org/mediawiki/2021/9/90/T--UParis_BME--WB_miRextraction.pdf">Protocol Western Blot - miRNAs isolation</a></p>
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<h4>exosomal miRNAs quantification using RT qPCR</h4>
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<p class="textContent"> to be completed </p>
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<p class="textContent"><a href="https://static.igem.org/mediawiki/2021/6/6e/T--UParis_BME--miRqPCR.pdf">Protocol miRNAs quantification using qPCR</a></p>
  
  

Revision as of 17:33, 20 October 2021