Difference between revisions of "Real Time PCR From Cell Culture"
From Bridges Lab Protocols
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#Use Superscript RT-PCR kit from Invitrogen, following manufacturers instructions | #Use Superscript RT-PCR kit from Invitrogen, following manufacturers instructions | ||
#Store cDNA at -20 until use | #Store cDNA at -20 until use | ||
+ | #Typically dilute 5X in water (adjust for higher or lower expressing transcripts) | ||
===Plate Preparation=== | ===Plate Preparation=== |
Revision as of 18:51, 26 May 2009
Contents
Real Time qPCR
Materials
- cDNA for templates
- Qiashredder and RNEasy kits from Qiagen
- Superscript Kit from Invitrogen
- SyberGreen PCR Master Mix Applied Biosystems
- 96 well qPCR plate
- Primers (Dilute to 0.22 uM mixture of fwd and rev)
- Generate primers using http://pga.mgh.harvard.edu/primerbank/index.html
Protocol
RNA Extraction
- Use RNEasy kit with Qiashredder. see Harvesting RNA from Cells grown in monolayer. For a 12 well plate, use 350 uL of RLT (add 10 uL B-ME per 1 mL of RLT buffer).
- Scrape cells and pass through Qiashredder column. Do the optional DNAse step at step 5 using the RNAse free DNAse from Qiagen.
- Store at -20 until RT reaction
RT-PCR Reaction
- Use 8 uL of RNA per RT reaction.
- Use Superscript RT-PCR kit from Invitrogen, following manufacturers instructions
- Store cDNA at -20 until use
- Typically dilute 5X in water (adjust for higher or lower expressing transcripts)
Plate Preparation
- Book 3h on qPCR machine at http://felix2.lsi.umich.edu/ORS/index.php?UID=2fd952b00de25
- Prepare primer mix from 5 uM primer pair stocks by adding 0.4 uL primers + 4.6 uL water per reaction
- Get 96 well block and keep on rack. Do not touch bottom of plate.
- Add 5 uL template per well.
- Add 5 uL primer per well
- Using PCR strip and multichannel pipettor, add 10 uL Master mix to each well
References (Saltiel Lab)
<pubmed>18829989</pubmed> <pubmed>17008399</pubmed> <pubmed>17200717</pubmed> <pubmed>17192460</pubmed> <pubmed>16926380</pubmed>