QRT-PCR/Single tube: Difference between revisions
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== Starting Materials == | == Starting Materials == | ||
* Validated PCR primers that are efficient over the range of RNA that you are assaying. | * Validated PCR primers & probe that are efficient over the range of RNA that you are assaying. | ||
* PCR primers and probe for a house keeping gene (ie B-actin, GAPDH, RPL19) | |||
* Taq Polymerase, MuLV RT | * Taq Polymerase, MuLV RT | ||
* dNTPs, MgCl2, nuclease free water | * dNTPs, MgCl2, nuclease free water |
Revision as of 13:16, 26 March 2007
This protocol describes one-step real time quantitivie PCR to quantify relative levels of RNA in
Starting Materials
- Validated PCR primers & probe that are efficient over the range of RNA that you are assaying.
- PCR primers and probe for a house keeping gene (ie B-actin, GAPDH, RPL19)
- Taq Polymerase, MuLV RT
- dNTPs, MgCl2, nuclease free water
- PCR strip caps or 96-well plates with transpearant caps
- total RNA (~50ng per reaction, diluted to 10ng/ul)
Basic Principle
- Combine RT, Taq, dNTPs, primers, probe and RNA in a single tube.
- Reverse transcribe the RNA for ~ 30' to form a template for Taq-mediated PCR.
- Do 40 cycles of PCR. Measure the levels of template are quantified during each cycle with a real-time PCR machine.
- Analyze the results.
Protocol
Analysis
Delta-Delta Ct Method. See Livak KJ, Schmittgen. Methods 25 402-408 (2001)