Luna® Universal Probe qPCR Master Mix Protocol (M3004)

  • Prepare DNA or cDNA of interest using desired DNA extraction and purification method.
  • Make dilutions of DNA or cDNA to be used for the standard curve. These should be prepared fresh before each experiment and can be diluted in either water or TE.

Reaction Setup: For best results, we recommend running each DNA standard and sample in triplicate.

 COMPONENT  20 µl REACTION
 FINAL CONCENTRATION
 Luna Universal Probe qPCR Master Mix
 10 µl
 1X
 Forward primer (10 µM)
 0.8 µl
 0.4 µM
 Reverse primer (10 µM)
 0.8 µl
 0.4 µM
 Probe (10 µM)
 0.4 µl
 0.2 µM
 Template DNA
 variable  < 100 ng
 Nuclease-free Water
 to 20 µl
 

  1. Thaw Luna Universal Probe qPCR Master Mix and other reaction components at room temperature, then place on ice. After thawing completely, briefly mix each component by inversion, pipetting or gentle vortexing.
  2. Determine the total volume for the appropriate number of reactions, plus 10% overage and prepare assay mix of all components except DNA template accordingly. Mix thoroughly but gently by pipetting or vortexing. Collect liquid to the bottom of the tube by brief centrifugation.
  3. Aliquot assay mix into qPCR tubes or plate. For best results, ensure accurate and consistent pipetting volumes and minimize bubbles.
  4. Add DNA templates to qPCR tubes or plate. Seal tubes with flat, optically transparent caps; seal plates with optically transparent film. Care should be taken to properly seal plate edges and corners to prevent artifacts caused by evaporation.
  5. Spin tubes or plates briefly to remove bubbles and collect liquid (1 minute at 2,500–3,000 rpm).
  6. Program real-time instrument with indicated thermocycling protocol (see table below). Ensure a plate read is included at the end of the extension step.

Confirm the appropriate detection channel is selected for the fluorophore used in the assay.
 
We recommend using the “Fast” cycling profile where applicable (e.g., Applied Biosystems StepOnePlus®, QuantStudio®, 7500 Fast instruments).

 CYCLE STEP
TEMPERATURE
 TIME  CYCLES
 Initial Denaturation
 95°C  60 seconds
 1
 Denaturation

 Extension
 95°C

 60°C
 15 seconds

 30 seconds (+plate read)

 40-45