Real Time PCR From Cell Culture

Real Time qPCR

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 5 uM mixture of fwd and rev and then make a working solution of 0.4 uL + 4.6 uL water per reaction)
Generate primers using http://pga.mgh.harvard.edu/primerbank/index.html

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

Book PCR Machine for 2h
Thaw, mix and quickly spin RNA, dNTP mix, random hexamers, 10X RT buffer, 25 mM MgCl2 water
Combine the following:
1. 8 uL RNA
2. 1 uL dNTP mix
3. 1 uL Random Hexamers
Put in PCR machine and run program RT 65C (takes 5 min)
In a separate tube add in the following order (for 10 reactions):
1. 20 uL 10X RT buffer
2. 40 uL 25 mM MgCl2
3. 20 uL 0.1M DTT
4. 10 uL RNAse Out
Add 9 uL of the reaction mix to each primer/RNA mixture from previous step, mix and quickly centrifuge
Sit on the bench for 2 min
Add 1 uL SuperScript II RT to each tube
Put in PCR machine and run program RT Reaction. After run (75 min) place on ice.
Add 1 uL RNase H and put in PCR machine and run program RT 37. Takes 20 min.
Store cDNA at -20 until use.

Book 3h on qPCR machine at http://felix2.lsi.umich.edu/ORS
Prepare primer mix from 5 uM primer pair stocks. Per reaction add 0.4 uL primers + 4.6 uL water.
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.
Add 10 uL per row into 8 wells of a PCR strip plus an extra 10-20 uL
Using a multichannel pipettor, add 10 uL Master mix to each well
Start qPCR Machine using the machine in the Lin Lab or the Saltiel Lab machine