qPCRBIO SyGreen® Real time PCR Mixes

The error rate is approximately 1 in 200,000 nucleotides (1 x 10^-5).

No, it is a next-gen asymmetric cyanine dye that is non-inhibitory at high concentrations, providing more consistent melt curves.

Lo-ROX (112 nM), Hi-ROX (1.12 µM), and Separate-ROX (50 µM additive).

Yes, it is fully compatible with bisulfite-treated templates for methylation analysis.

The 3 mM final Magnesium Chloride (MgCl2) concentration in the mix is high enough to compensate for any minor chelation caused by 1x TE storage buffers.

While 2 minutes at 95°C is recommended for maximum stringency, the Hot-Start Taq can be activated in as little as 10 seconds for standard, low-complexity templates.

To stop DNA from sticking to polypropylene tubes, dilute your standards in a buffer of 10 mM Tris-HCl (pH 8.0) containing 0.05% Tween-20. Avoid freezing standards after dilution.

This is usually due to high enzymatic efficiency. To confirm it isn't non-specific amplification, check for a single peak in your melt analysis. If multiple peaks appear, increase your annealing temperature.

High background is often caused by an excess of template DNA. Diluting your samples 100x to 1000x typically resolves the issue by reducing the amount of non-target DNA the dye binds to.

Yes. The enzyme produces 3'-d(A)-overhangs. We recommend using a standard spin-column clean-up kit before ligation to remove the intercalating dye and buffer salts.