StableScript™ One-Step RT-qPCR Mix

A highly efficient and sensitive RT-qPCR formulation for detection using hydrolysis probes with robust inhibitor resistance

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StableScript™ One Step RT-qPCR Mix (250 reactions)

Cat. No. / ID:   P7730L

For 250 reactions: 10X StableScript™ Enzyme Mix (0.5 ml) and 4X StableScript™ Reaction Buffer (2 x 1.5 mL)
£711.00
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The StableScript™ One-Step RT-qPCR Mix is intended for molecular biology applications. This product is not intended for the diagnosis, prevention, or treatment of a disease.
Need bulk, customized or optimized products for commercial purposes? We also offer support with logistics, compliance and more. Reach out to cooperate with QIAGEN Strategic Partnerships & OEM

Features

  • Able to multiplex while maintaining sensitivity and specificity
  • Formulated using StableScript™ Reverse Transcriptase with Improved thermostability, processivity and inhibitor resistance
  • Detects as little as 0.1pg of RNA in 4 plex assay
  • Excellent Lot-to-Lot consistency

Product Details

The StableScript™ One-Step RT-qPCR Mix is a highly efficient and sensitive RT-qPCR formulation for DNA and RNA detection using 
hydrolysis probes. The 10X enzyme mix contains a blend of a new RNAse H minus reverse transcriptase with higher 
thermostability and inhibitor resistance (StableScript™), a fast-activating hot start DNA polymerase (Phoenix™), and specific 
enhancers to increase sensitivity and inhibitor resistance. 


StableScript™ One-Step RT-qPCR Mix is supplied with 4X StableScript™ Reaction Buffer B7720L, containing dNTPs and 
Magnesium.

 

Performance

StableScript™ One-Step RT-qPCR Mix is a blend of StableScript™ Reverse Transcriptase and Phoenix™ Hot Start Taq DNA 
Polymerase enzymes. StableScript™ Reverse Transcriptase is engineered for increased thermostability. Increasing the temperature 
for cDNA synthesis can aid in overcoming challenging RNA targets because higher temperatures help unravel RNA structures, 
reducing the likelihood of hindering reverse transcription.


The Phoenix™ Polymerase is a recombinant, thermostable Taq DNA polymerase complexed with a thermolabile, neutralizing 
antibody. This fast-activating antibody-mediated hot-start capability enhances the overall specificity, sensitivity, and yield of the PCR 
reaction by reducing nonspecific amplification and primer-dimer formation prior to cycling. Together with StableScript™, Phoenix™ 
creates StableScript™ One-Step RT-qPCR Mix, an extremely sensitive RT-qPCR mix:

  • qPCR formulation for detection using hydrolysis probes
  • Robust inhibitor resistance
  • Able to multiplex while maintaining sensitivity and specificity
  • Detects as little as 0.1pg of RNA in 4 plex assay
  • Increased thermostability with optimal cDNA synthesis from 50ºC to 65ºC 
  • Stable on benchtop overnight
  • Excellent dynamic range on a variety of assay systems
  • Exceptional lot-to-lot consistency

Mix properties

  • Storage temperature: –25°C to –15°C

 

Procedure

StableScript™ One Step RT-qPCR reaction setup

General precautions against degradation of RNA template should be taken when setting up a reaction, including setting up the 
reaction with nuclease free water, RNase inhibitor, nuclease free PCR tubes and sterile pipette tips with filter, adding reverse 
transcriptase last, gentle pipetting, thorough mixing and a quick centrifugation. The following procedure can be used as a 
guideline. Reactions may need to be optimized individually.

  1. The 4X StableScript™ Reaction Buffer should be thaw completely and vortex for 3-5 seconds to mix thoroughly. Quickly 
    spin to collect contents.
  2. Prepare the primer/probe mix. A final concentration of 0.4-0.9μM for each primer and 0.1-0.5μM for the probe is
    recommended. However, the optimal concentration for primers/probes needs to be empirically determined for each assay.
  3. Determine the number of reactions to prepare, including No Template Controls (NTCs). Add 10% extra volume to 
    compensate for the pipetting loss.
  4. Follow the table below to set up the reaction mix. It is recommended to make a master mix to minimize variations and 
    potential errors.
    Components Volume/Rxn Final Concentration
    4X StableScript™ Reaction Buffer 5μL 1X
    Primer/Probe Mix XμL Variable
    10X StableScript™ Enzyme Mix 2μL 1X
    RNA Template Up to 2μL 1pg to 1µg total RNA
    Nuclease-Free Water To a final 20μL reaction volume -
  5. Seal the PCR plate and spin briefly to collect contents at the bottom.

     Thermal Cycling Conditions: 

     Program the cycling conditions are recommended as below. 

Standard Cycling Program* Steps Temperature  Time Cycles
Reverse Transcription 55°C 10 min 1
Taq Activation/Initial Denaturation 95°C 3 min 1
Denaturation 95°C 5-10 sec 40
Annealing/Extension* 60°C 30-60 sec

*Cycling parameters can be modified (especially the annealing/extension condition) to fit specific assays. 

Quality control analysis

The functionality of the RT-PCR Assay is evaluated by amplification of three mRNA transcripts in a one-step RT-qPCR assay. The 
amplification threshold (Ct) of the test lot is compared to a reference lot.

Notes: 

Enzyme components were tested prior to formulation of the master mix and found free of contaminating endonucleases and 
exonucleases. Enzyme purity was >99% as determined by SDS-PAGE, and negligible E. coli genomic DNA contamination was 
confirmed by qPCR. Specific activity was verified for each enzyme pre-formulation.

 

Applications

This product is available for molecular biology applications such as:

  • One-step RT-qPCR.
  • Gene expression analysis of RNA targets
  • DNA and RNA detection and quantification

Resources

Quick-Start Protocols (1)
Safety Data Sheets (1)
Certificates of Analysis (1)