RapiDxFire Hot Start Taq DNA Polymerase
Product information
RapiDxFire Hot Start Taq DNA Polymerase is recombinant Taq DNA Polymerase from Thermus aquaticus
bound to select blockers, which prevents unwanted, nonspecific
amplification during reaction set up at temperatures less than 60 °C.
Enzyme activity is restored after a short 15 second burst at 94 °C,
enabling fast detection of low abundance target DNA. The Taq polymerase
possesses 5′→3’ polymerase activity (amplicons up to 5 Kb) and dsDNA
specific 5→3’ exonuclease activity, ideal for use with hydrolysis probes
in qPCR reactions. The glycerol-free (GF), Triton®-free, and high-
concentration formulation- is compatible with downstream lyophilisation
methods and provides robust enzyme stability in liquid form (>28 days
at 37 °C). These features provide flexible preparation and storage
methods for qPCR master mixes (and detection assays) in addition to
enabling benchtop reaction setups in warmer environments. Whether you
are developing automated diagnostic tests or producing amplicons for
downstream applications, RapiDxFire Hot Start Taq DNA Polymerase is your
perfect choice for both demanding and routine PCR applications.
RapiDxFire Hot Start Taq is provided with 10x Reaction Buffer and a separate tube of 25 mM MgCl2. RapiDxFire Hot Start Taq GF enzyme storage buffer is free of glycerol (Item ID. 30043-1 and 30044-1). All reagents are free of Triton X-100.
Applications
- Food borne pathogen detection
- Diagnostic test development
- Biomarker discovery and monitoring
- Gene expression analysis
- SNP genotyping
- Copy number variation (CNV) analysis
- Cloning
Figure 1. RapiDxFire Hot Start Taq DNA Polymerase
performs better than three market-leading hot start Taq polymerases. The
comparison was conducted using a E. coli gene-specific assay that
produces a melt peak at ~89°C. PCR cycling conditions included a 90
minute pre-incubation at 35°C to induce non-specific amplification. Each
polymerase was tested using 1.25 Units of Taq and supplier-recommended
buffer in a 25 µL reaction using SYBR green detection. All three
competitors exhibit non-specific amplification as seen by the second
melt peak.
Figure 2. Effect of RapiDxFire Hot Start Taq DNA
Polymerase activation time on assay sensitivity. Target detection and
PCR efficiency were compared when using a short 15-second hot start Taq
activation time (green) versus a standard 2-minute activation time (red)
at 94 °C prior to PCR cycling. RapiDxFire Hot Start Taq polymerase was
tested using 0, 100, 1000, 10,000 copies of purified human DNA using a
gene specific assay. Real-time detection of PCR products was performed
using BHQplus™ probes and BioRad CFX C1000 Touch™ thermocycler.
Figure 3. Stability of RapiDxFire Hot Start Taq
polymerase in glycerol-free enzyme storage buffer. Hot Start Taq enzyme
was subjected to -20 °C, 4 °C, 20-25 °C, and 37 °C for 28 days prior to
performing real time PCR using an E. coli gene specific assay
against template DNA and No Template Control (NTC) in a glycerol-free
reaction buffer. Detection of PCR products (2.4 kb) was performed in
real time using an intercalating dye and BioRad CFX C1000 Touch™.
Concentration: 5 U/µL (Cat No. 30042-1, 30043-1) or 50 U/µL (Cat. No. 30044-1).
Storage: Store at -20 °C.
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