PrimeTime™ qPCR Primer Assays

No signal or amplification can result from a number of causes ranging from problems with the experimental design to inadvertently leaving out a necessary component from the reaction.

Here are some recommendations:

• Check the sequences of the probes and primers to be sure the bases and fluorophore/quencher modifications are all correct.
• Run the failed qPCR on an agarose gel to check for the correct amplification product size.

• If you do not see an amplicon you can try adding more cDNA to the reaction mixture.
• If you do see an amplicon on the gel, check the real-time PCR instrument to make sure it is set at the correct wavelength to detect the right fluorophore and that it is set to monitor the fluorescence at the correct step of the PCR protocol which is after the elongation step.
• If your amplicon is very GC rich, you can also try adding up to 5% formamide to the reaction mixture. You can also increase the Mg²⁺ concentration (in increments of 0.5 mM, up to 7 mM) but increased Mg²⁺ concentration can also cause nonspecific priming.
• Check the master mix components; it is possible that one of the components (such as the polymerase or probe) were inadvertently left out. We recommend that you repeat a failed experiment once to make sure it was not due to a simple mistake in the first round.
• Check on the probe design. How long is the probe? What is the Tm of the probe? Probes must be around ~10°C higher than the primers so that the probe can hybridize before the primers.
• If the Tm of the probe is too low, it will not hybridize and no signal will be generated. In addition, try to avoid a probe with a G at the 5' end. The G can quench the fluorophore which may result in poor signal generation.

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For most qPCR assays, use 1 to 100 ng cDNA per 20 µL reaction.

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The cycle at which fluorescence from amplification exceeds the background fluorescence has been referred to as threshold cycle (C_t), crossing point (C_p), and take-off point (TOF) by different instrument manufacturers. But the term is now standardized by the MIQE guidelines as the quantification cycle( C_q). A lower C_q correlates with higher target expression in a sample.

Access the MIQE guidelines at:

Bustin SA, Benes V, et al. (2009) The MIQE Guidelines: minimum information for publication of quantitative real-time PCR experiments. Clin Chem, 55(4): 611−622. Updates: Bustin

SA, Beaulieu JF, et al. (2010) MIQE précis: Practical implementation of minimum standard guidelines for fluorescence-based quantitative real-time PCR experiments. BMC Mol Biol.11: 74–78, and Bustin SA, Benes V, et al. (2011) Primer sequence disclosure: A clarification of the MIQE Guidelines. Clin Chem, 57:919−921.

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PrimeTime One-Step RT-qPCR Master Mix performance in qPCR experiments is equal to or better than most other master mixes designed for one-step qPCR. Click here to view the representative data.

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The stability of PrimeTime Gene Expression Master Mix makes it ideal for overnight PCR runs and high throughput experiments using robotic liquid handling systems.

Reliable results have been obtained when the qPCR was run directly after setup or after the reactions were maintained at room temperature for up to 72 hr.

Download the white paper, Ambient shipping of PrimeTime Gene Expression Master Mix for more data.

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We provide a separate tube of reference dye so that you may use the PrimeTime Gene Expression Master Mix on reference dye-dependent or dye-independent instruments.

Also, the separate tube of reference dye provides a way to add a high or low dye concentration to the master mix, depending on the requirements of your instrument.

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Yes, it uses an antibody-mediated, hot-start polymerase. During the initial denaturation step of qPCR cycling, polymerase activity is unblocked when the polymerase is released from the antibody.

This hot-start polymerase enhances reaction precision of the qPCR by avoiding non-specific amplification of DNA and primer dimer formation. It is therefore critical to follow the cycling conditions provided in the PrimeTime Gene Expression Master Mix Protocol.

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Yes. The Primetime™ Gene Expression Master Mix has been successfully used in qPCR experiments run on the QuantStudio™ 7 Flex (Thermo Fisher Scientific), 7900HT (Thermo Fisher Scientific), 7500 (Thermo Fisher Scientific), the CFX384™ (BioRad), and the LightCycler® 480 (Roche) instruments. All such experiments used the cycling conditions provided in the PrimeTime Gene Expression Master Mix Protocol. 
 
Reference dye is provided in a separate tube, so you may add it to the master mix at the levels required by your real-time PCR instrument.

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The amount of reference dye that should be added to the PrimeTime Gene Expression Master Mix depends on which real-time PCR system you are using.

A table that details how much reference dye to add is provided in the PrimeTime Gene Expression Master Mix Protocol.

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IDT offers the SUN™ dye, which is our product offering for the VIC dye (Thermo Fisher Scientific).

More information about probes labeled with the SUN fluorophore can be found on the PrimeTime™ qPCR probes page or the SUN fluorophore Decoded™ article.

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When performing qPCR it is ideal to have your probe T_m about 5−10 degrees higher than your primer T_m. The annealing temperature should be set 3−5 degrees lower than the lowest primer T_m.

Use this as a general guideline, but note that optimization may still be necessary.

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We ship PrimeTime™ Gene Expression Master Mix, PrimeTime qPCR assays, and other oligonucleotide products at ambient temperature.

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Phosphorothioate bonds (PS bonds) increase oligonucleotide resistance to exonuclease degradation. For single-stranded oligos, nuclease-resistance is highest when every phosphodiester bond is changed to a PS bond.

In general, we recommend at least 3 PS bonds on both 5' and 3' ends of the oligo, though more PS bonds will give greater exonuclease resistance.

Note that PCR primers with PS bonds at both ends will still result in double-stranded (ds) PCR products with PS bonds only at the 5' ends of each product strand. While protected from 5' to 3' nuclease activity, because these dsDNAs lack PS bonds at the 3' strand ends, exonucleases with 3' to 5' activity will still be able to degrade them.

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Proofreading polymerases (Pfu, Diamond Taq®, etc) have been shown to remove 3' bases from PCR primers [1].

If you experience this problem, you can protect your primer from degradation by adding one or more phosphorothioate bonds to the 3' end of your primer.

Also make sure to add the enzyme last, after the addition of dNTPs, in your PCR to minimize the risk of this issue taking place.

Reference

1. Skerra A. Phosphorothioate primers improve the amplification of DNA sequences by DNA polymerases with proofreading activity. Nucleic Acids Res. 1992;20(14):3551-3554.

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To determine what dyes are compatible with your instrument, download our Real-time qPCR assay design guide or take a look at the PrimeTime™ Multiplex Dye Selection Tool.

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Currently, the IDT ZEN quencher is available with FAM, HEX, TET, Yakima Yellow^® (ELITech Group), JOE™ (Thermo Fisher Scientific), MAX™, and SUN™ fluorophores. Double-quenched probes have significantly lower background fluorescence, especially for longer probes.

The ZEN quencher is available on PrimeTime™ qPCR Probes and on the probes supplied with PrimeTime qPCR Probe Assays. For any special oligonucleotide requests that include the ZEN quencher but are not found on our website (non-catalog requests), please contact us.

For more information, see our DECODED™ article,  Double-quenched probes increase qPCR sensitivity and precision.

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5′ Cy dyes are attached to the 5' hydroxyl group of the sugar via a phosphodiester bond.

3' Cy dyes are attached to the 3' hydroxyl group of the sugar via a phosphodiester bond.

Internal Cy dyes are attached to the backbone via the phosphodiester bonds of the bases between which the dyes occur.

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IDT oligos have various estimated ship dates depending on product type and composition. Oligos added to the shopping cart will show an estimated ship date for each line item.

Once the order is placed, this estimated ship date can be found on the order confirmation email as well as in the order history of your web account. You can find the order history at idtdna.com/site/orderstatus/orderstatus.

Select the order number you wish to review, and the status and estimated ship date of each line item will be shown.

IDT will email you a confirmation when your order has been shipped. This shipping confirmation will include the tracking number of the package, which you can use to monitor the status of your shipment. If you have additional questions about your order, please contact us.

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It is good practice, but not necessary to thaw or keep reagents on ice. We see no difference in results between reaction mixes prepared with the PrimeTime™ Gene Expression Master Mix that were used directly after thawing vs. those kept at room temperature for up to 24 hours.

PrimeTime Gene Expression Master Mix also shows exceptional temperature stability, even after a heat stress test (up to 8 hr at 55°C). Review the data in our white paper, Ambient shipping of PrimeTime Gene Expression Master Mix.

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Standard desalting is the recommended purification for qPCR primers.

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