How to Optimize qPCR using SYBR Green Assays - Ask TaqMan #38
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- Опубликовано: 24 июл 2024
- Learn More: www.thermofisher.com/sybr
Are you new to using SYBR Green Assays for qPCR or having trouble getting accurate results? Today, let’s discuss how you can design and optimize qPCR using SYBR Green assays as the detection method.
First, beware of reverse transcription (RT) bias when converting RNA to cDNA. Nearly all RT enzymes have the potential to introduce RT bias. When this happens the amount of cDNA won’t align with the amount in RNA samples. Learn More about RT Methods in this video: • What is the Right RT M...
You can test for RT bias by reverse transcribing two-fold dilutions of a known amount of RNA. Then run a qPCR standard curve for each assay and endogenous control. The standard cure should be linear with a target slope of -3.323.”
Once the cDNA is generated make sure to use the right primers for the qPCR.
You will need to use some bioinformatics to design your primers, such as a tool like SNPMasker.
In general, primers should be 20 nucleotides in length with a GC content in the 30-70% range. The last 5 nucleotides at the 3’ end should include no more than two G or C bases to avoid specificity issues. Finally, amplicons should be short -- generally between 50 - 150 base pairs.
The next step is primer validation. The objective is to find the right concentration of forward and reverse primers that will yield the most robust assay without non-specific amplification or primer dimers.
This is accomplished by running multiple qPCRs with 3 different concentrations of forward and reverse primers in a matrix format. The appropriate range of primer concentration is determined by the master mix.
For instance, Applied Biosystems PowerUp SYBR Green Master Mix works best with primer concentrations in the range of 300 - 800 nM.
Getting back to our experiments to optimize primer concentrations, the next step is to evaluate the Ct and run a melting curve also known as a dissociation curve for each primer concentration combination.
If dissociation curve shows primer-dimers, there are two options:
A. Start over and redesign the primers.
B. Alter cycling temperatures to remove primer-dimers.
The last step in ensuring that your primer set is going to yield usable, reproducible data is to ensure the PCR efficiency is within 90 - 110%. You can do this by simply running a standard curve with at least 5 logs of input DNA and using the software on your instrument to calculate PCR efficiency.
If this all seems too complicated, you can use pre-designed TaqMan assays instead, which removes the primer design variable and ensures the best possible primer set
Once the primers are designed, experimental analysis can begin.
Here’s a tip! For measuring relative gene expression levels of two different samples, most researchers use what’s known as the ΔΔCt (ddCt) method. This analysis generates relative changes form one state to the next, much like a disease state versus treatments
For more information about SYBR Green experiments, TaqMan assays or related reagents, please visit www.thermofisher.com/qpcr or www.thermofisher.com/sybr
And If you have more questions concerning SYBR green assays, ΔΔCt analysis or any other qPCR questions, remember to Ask TaqMan and submit your questions on our website www.thermofisher.com/ask
Thanks for watching! 
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Thank you
You're welcome, we are glad the video was helpful.
Thank you so much, I am just learning how to use the ThermoFisher thermo cycle with Sybr and next week with taqman
This was very helpman, thanks TaqMan!
Thanks for watching!
Hey, I couldn't find a proper animation video for the explanation of whole concept and working pf Real time PCR using Cyber green.. I think there is a need of good animation videos of the same.
"The 3' end should contain no more than 2 G or C bases to avoid specificity issues." Is this correct? I think the 3' end should have MORE G or C bases to form GC clamps that increase specificity.
how to optimize primers ?
Thank you .excellent.
Should I run temperature gradients?
Thanks Joshua for your question.
If you are uncertain of what temperature to use for your annealing temperature, a temperature gradient is a great way to test what optimal annealing temperature to use. However, if you already know what annealing temperature to use, a temperature gradient is not necessary.
For additional technical support, please contact us at thermofisher.com/askaquestion. Thank you!
Nice drawings
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ryan reynolds?