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PanProbes™ Universal qPCR MasterMix

The PanProbes™ Universal qPCR MasterMix is a ready-to-use, 2x concentrated master mix optimized for probe-based real-time PCR. Designed for compatibility with a wide range of commercial qPCR systems (both ROX-dependent and ROX-independent), this master mix ensures reliable and accurate results every time.

  • Enhanced Antibody-Mediated Hot-Start Taq DNA Polymerase: Ensures minimal non-specific amplification, increasing the specificity and efficiency of your reactions.
  • Optimized for Probe-Based Real-Time PCR: Achieve accurate quantification with high sensitivity.
  • Versatile Compatibility: Works with most commercially available qPCR systems, offering flexibility in your experimental setup.
  • Comprehensive Reaction Components: Contains dNTPs, MgCl2, stabilizers, and enhancers—everything you need for a successful PCR reaction.

This PanProbes™ Universal qPCR MasterMix simplifies the workflow while enhancing PCR performance, making it an essential tool for researchers seeking reproducibility and high-quality results.

Figure 1. Performance of PanProbes™ Universal qPCR MasterMix

                                      

 

  • Combine the assay Master Mix thoroughly to ensure consistency and equally dispense the solution into each qPCR tube or into the wells of a qPCR plate. Employ good pipetting practice to ensure assay precision and accuracy. 
  • Add DNA samples (and DNase-free H2O if needed) to the PCR tubes or wells containing assay Master Mix (Table 1), seal the tubes or wells with flat caps or optically transparent film. Note: to ensure thorough mixing of reaction components, vortex for approximately 30 seconds (or more). 
  • Spin the tubes or plate to remove any air bubbles and collect the reaction mixture in the vessel bottom.
  •  Setup the thermal cycling protocol on a real-time PCR instrument according to Table 2. Note: optimization may be needed for better performance. 
  •  Load the PCR tubes or plate into the real-time PCR instrument and commence the run. 
  •  Perform data analysis according to the instrument-specific instructions.

Note: Optimal conditions for amplification will vary depending on the primers and thermal cycler used. It may be necessary to optimize the system for individual primers, template, and thermal cycler.

Template 

  • Purified high quality DNA is needed for a success PCR reaction. 
  • The final concentration of DNA template please refer to table 1. 

Important notes 

  1. Shake gently before use to avoid foaming and low-speed centrifugation. 
  2. During operation, always wear a lab coat, disposable gloves, and protective equipment

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