https://bridgeslab.sph.umich.edu/protocols/index.php?action=history&feed=atom&title=TaqmanTaqman - Revision history2026-05-10T02:09:50ZRevision history for this page on the wikiMediaWiki 1.45.1https://bridgeslab.sph.umich.edu/protocols/index.php?title=Taqman&diff=1243&oldid=prevMjwils: Created page with "<big>'''Taqman Real-Time qPCR ''' </big> '''Materials''' • cDNA: see First Strand cDNA Synthesis (AB Kit) for details • Thermo Scientific ASsolute Blue qPCR Mix Plus R..."2017-05-10T15:16:44Z<p>Created page with "<big>'''Taqman Real-Time qPCR ''' </big> '''Materials''' • cDNA: see First Strand cDNA Synthesis (AB Kit) for details • Thermo Scientific ASsolute Blue qPCR Mix Plus R..."</p>
<p><b>New page</b></p><div><big>'''Taqman Real-Time qPCR<br />
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'''Materials'''<br />
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• cDNA: see First Strand cDNA Synthesis (AB Kit) for details<br />
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• Thermo Scientific ASsolute Blue qPCR Mix Plus ROX Vial (#AB-4136/B)<br />
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• 384 well qPCR plate (ThermoFisher Catalog # 4309849) and covers (Catalog # 4360954)<br />
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• Taqman Gene Expression Assay Primers stored at -20<br />
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'''Plate Preparation<br />
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1. Book 2h on qPCR machine by signing up on the sheet in room 6041<br />
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2. Prepare cDNA and dilute in water in a 96 well plate. Typically, a 20x dilution of cDNA leaves enough to be detected.<br />
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3. Get optically clear 384 well plate and keep on paper towel. Do not touch bottom of plate.<br />
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4. Sketch out plate in your notes. Typically, rows are different primers while columns are different cDNA.<br />
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5. Calculate how many samples x how many replicates per sample (start with 3 or 4 until you are consistent enough technically to decrease). This will be the number of wells needed for each primer.<br />
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6. Prepare master mix. For a 10 uL reaction, you will need 5 uL of Absolute Blue mix, 0.5 uL of Taqman primer, and 2.5 uL of RNase Free Water. Mix components into 1.5 mL tube. Be sure to make 10-20% extra for volume loss. <br />
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7. Using the repeater multichannel pipetter, put on 2 or 3 tips (depending on plate arrangement) and set pipette to the amount of samples needed. Dispense 8 uL per well. <br />
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8. Using multichannel pipetter, add 2 uL of prepared cDNA into each designated well. Be sure to dispense to the bottom of the well.<br />
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9. Once plate is complete, put optically clear cover on it using plastic square to ensure the edges are sealed. Do not leave fingerprints on the seal.<br />
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10. You can prep the plate ~3 hours beforehand, keeping at 4C until the machine is ready.<br />
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11. Immediately before the run spin the plate briefly (2 minutes at 4000 RPM) in the swinging bucket centrifuge.<br />
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'''Run Protocol<br />
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• Set up run using Thermo Cloud/QuantStudio or Roche LightCycler</div>Mjwils