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5X UniFi™ 1-Step qRT-PCR Probe Master Mix

Features

  • Best-in-class performance for both single and multiplex detection
  • Convenient all-in-one master mix
  • High specificity and sensitivity across a wide range of sample sources

Applications

  • One-step qRT-PCR from mRNA, total RNA and viral RNA targets
  • For use with standard and fast qPCR platforms
  • Single and multiplex qRT-PCR reactions

Purchase 5X UniFi™ 1-Step qRT-PCR Probe Master Mix

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

Catalog # Size Package Content Price* Qty
BR0504601 250 reactions of 20 µl 1 × 1 ml 5X UniFi™ 1-Step qRT-PCR Probe Master Mix
€227.00
BR0504602 1000 reactions of 20 µl 5 × 1 ml 5X UniFi™ 1-Step qRT-PCR Probe Master Mix
€785.00

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

OR

biotechrabbit™ UniFi™ 1-Step qRT-PCR Probe Master Mix provides outstanding performance for real-time PCR quantification of RNA templates, including mRNA, total RNA and viral RNA from a wide range of targets. The master mix ensures high specificity and sensitivity in single and multiplex detection, making it the ideal choice for extremely low-copy-number targets in pathogen detection.

The mix is provided as a 5X concentrated master mix, offering flexibility in pipetting schemes and template input for various PCR applications. UniFi™ 1-Step qRT-PCR Probe Master Mix uses proprietary reverse transcriptase technology and buffer chemistry for efficient cDNA synthesis and qPCR in a single tube.

 

Component

Composition

UniFi™ 1-Step qRT-PCR Probe Master Mix

5X concentrated formulation of a UniFi™ 1-Step qRT-PCR Probe Master Mix

 

Storage

Store at −20 °C until expiry date.



Handling
Prevention of reaction contamination

RNase contamination is a particular concern when working with RNA. RNase A, which poses a major threat to RNA integrity, is a highly stable laboratory contaminant. To prevent RNA degradation and minimize the risk of contamination in one-step RT-PCR, follow the guidelines below:

  • Use separate clean areas for preparation of samples and reaction mixtures.
  • Use DEPC-treated tubes and pipette tips or certified nuclease-free labware with aerosol filters.
  • Wear fresh gloves when handling RNA and all reagents.
  • Assess RNA integrity before RT-PCR using denaturing agarose gel electrophoresis.
  • Use only water and reagents that are free of DNA, DNases and RNases.
  • With every one-step RT-PCR setup, perform a contamination control reaction without template RNA.
Basic Protocol
  • Keep the master mix protected from light until use.
  • Aliquot the master mix to minimize freeze-thaw cycles and light exposure.
  • Thaw all reagents on ice and mix thoroughly. 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 RNA) and negative controls (water or buffer).
  • First pipette the primer mixture, then add the template, and add the Master Mix last.
  • Before preparing mixes, calculate the required volume based on the number of reactions plus one additional reaction.
  • For better correlation, run the reactions in triplicate.

Component

Volume

Final concentration

Primer Mix (Reverse and Forward)

Variable

100–400 nM

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

Specific Probe

Variable

200 nM

Template RNA

Variable

0.01 pg–1 µg

Use 1 pg–1 µg total RNA or more than 0.01 pg mRNA.

5X UniFi™ 1-Step qRT-PCR Probe Master Mix

4 µl

Nuclease-free water

Variable

 

Total volume

20 µl

 

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

Step

Temperature

Time

Cycles

Reverse Transcription

50 °C

10 min

1

Initial activation

95 °C

3 min

1

Denaturation

95 °C

10 s

40–45

Annealing/Extension*

60–68 °C*

30 s

*The recommended annealing/extension temperature is primer Tm +2 °C. Use gradient PCR to optimize the annealing temperature. Do not use annealing temperatures below 60 °C. For melt analysis, refer to the instrument instructions.

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