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4X CAPITAL™ qPCR Probe Master Mix Plus

Features

  • Best-in-class performance for both single and multiplex detection
  • Convenient master mix for low-copy number pathogen detection
  • Highly sensitive for low-abundance DNA targets
  • Minimized risk of carryover contamination

Applications

  • Standard and fast cycling qPCR with rapid extension rate for early Ct values
  • For use on a wide range of probe technologies including Taqman®, Molecular Beacons® and Scorpion® probes

Purchase 4X CAPITAL™ qPCR Probe Master Mix Plus

Availability: In stock Bulk requests please inquire at oem@biotechrabbit.com

Catalog # Size Package Content Price* Qty
BR0503101 200 reactions of 20 µl 1 × 1 ml 4X CAPITAL™ qPCR Probe Master Mix UDG
€155.00
BR0503102 1000 reactions of 20 µl 5 × 1 ml 4X CAPITAL™ qPCR Probe Master Mix UDG
€490.00
BR0503103 4000 reactions of 20 µl 20 × 1 ml 4X CAPITAL™ qPCR Probe Master Mix UDG
€1,760.00

*Does not include applicable tax, shipping & handling, or other charges.

OR

biotechrabbit™ CAPITAL™ qPCR Probe Master Mix Plus is a high-performance solution designed for quantitative PCR (qPCR) applications that require utmost precision and reliability. This ready-to-use mix combines a robust Taq DNA polymerase, UDG (Uracil-DNA Glycosylase), and dUTP to provide enhanced protection against carryover contamination, ensuring the accuracy and reproducibility of your qPCR results.

The UDG enzyme is incorporated to degrade uracil-containing DNA, a common byproduct of PCR carryover, while the inclusion of dUTP ensures that any contaminating DNA from previous PCRs is not amplified. This system not only improves the reliability of qPCR assays but also simplifies the workflow by preventing false positives.

 

Component

Composition

4X CAPITAL™ qPCR Probe Master Mix UDG

Optimized 4X qPCR Probe Master Mix with UDG for prevention of carryover contamination.

 

Storage

Store at −20 °C until expiry date.



Handling
Prevention of PCR contamination

When assembling the amplification reactions, care should be taken to eliminate the possibility of contamination with undesired DNA.

  • Use separate clean areas for preparation of samples and reaction mixtures and for cycling.
  • Wear fresh gloves. Use sterile tubes and pipette tips with aerosol filters for PCR setup.
  • Use only water and reagents that are free of DNA and nucleases.
  • With every PCR setup, perform a contamination control reaction that does not include template DNA.
Basic Protocol
  • Aliquot the master mix to minimize freeze-thaw cycles and light exposure.
  • Thaw on ice and mix all reagents very well. Assemble and keep all reactions on ice.
  • Use only high-quality, optically clear reaction plates and seals designed for fluorescence applications.
  • Do not use corner wells, or use a more robust seal.
  • Reserve plate positions for positive controls (control DNA) and negative controls (water or buffer).
  • First pipette the primer-probe mixture, then add the template, and add the Master Mix last.
  • Before preparing mixes, calculate the volume needed according to the number of reactions plus one extra reaction.
  • For better correlation, run the reactions in triplicate.

Component

Volume

Final concentration

Primer Mix (Reverse and Forward)

Variable

100–400 nM

Too high primer concentrations result in unspecific amplification and should be avoided.

Specific Probe

Variable

200 nM

Template DNA

Variable

10 pg–100 ng

Use diluted or undiluted cDNA from less than 1 µg RNA.

CAPITAL™ qPCR Probe Mix, 4×

5 µl

Nuclease-free water

Variable

 

Total volume

20 µl

 

  • Gently mix the reactions without creating bubbles. Do not vortex. Bubbles will interfere with fluorescence detection.
  • Place the reaction into the PCR cycler.
Cycling program

Step

Temperature

Time

Cycles

Initial activation

95 °C

2–3 min

1

Denaturation

95 °C

10–15 s

40–45

Annealing/Extension*

60–68 °C

30 s

*Recommended annealing temperature is 2 °C above primer Tm. Use gradient PCR to optimize the annealing temperature. Do not use temperatures below 60 °C.

Do not exceed 30 seconds. For melt analysis, refer to the instrument instructions.

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