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PR1MA Taq Plus

  • Higher fidelity for long PCR amplicons, up to 35 kb
  • Ideal for problematic templates
  • Better sensitivity and higher activity for low-copy and long PCR
  • Enzyme of choice for TA cloning


PR1MA Taq Plus, an optimized blend of our Hot Start Taq and a proofreading polymerase, provides 5X better fidelity than wild-type Taq and increased enzyme activity. It is the perfect choice for GC and AT rich templates, low copy number, and long PCR.

The 3' -5' exonuclease activity of the proofreading enzyme produces fragments suitable for TA cloning. PR1MA Taq Plus is provided with a 5X buffer with dNTPs or in a convenient one-tube 2X Master Mix.

PR1MA Taq Start Taq DNA Polymerase 

ItemDescriptionVolume
PR1000-TP-SPR1MA Taq Start Taq DNA Polymerase50 Units (Sample)
PR1000-TP-250PR1MA Taq Start Taq DNA Polymerase250 Units (5 U/p1)
PR1000-TP-500PR1MA Taq Start Taq DNA Polymerase1,000 Units (5 U/p1)

 

PR1MA™ Taq Plus Master Mix, 2X Concentration

  

ItemDescriptionVolume
PR1001-TP-SPR1MA Taq Plus Master Mix, 2X Concentration20 Reactions (Sample)
PR1001-TP-200PR1MA Taq Plus Master Mix, 2X Concentration200 x 50 uL Reactions
PR1001-TP-1000PR1MA Taq Plus Master Mix, 2X Concentration1,000 x 50 uL Reactions


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PR1MA qMAX Probe qPCR Mix

  • Same high efficiency for multiplex and singleplex reactions
  • Includes PR1MA Hot Start Taq Polymerase for greater specificity and accuracy
  • Compatible with popular hydrolysis and beacon probes
  • Ready to use 2X mastermix
  • Early Ct values and detection across a broad dynamic range 

Optimized for use with TaqMan, Scorpions® and molecular beacon probes, qMax Probe qPCR Mix is a ready-to-use formulation for real-time quantitative assays. qMax Probe utilizes PR1MA Hot Start Taq Polymerase or robust PCR with a variety of templates. A specially formulated buffer provides optimal conditions for both superior polymerase function and probe detection, resulting in earlier Ct values and a broad detection range. Complicated, multiplex reactions can be performed without any loss in performance or decrease in detection. The 2X mix requires little, if any optimization and can be used with both fast and standard protocols.

 

PR1MA qMax Probe qPCR Mix can be used to detect any DNA template, including genomic DNA and cDNA. Available in high, low and no ROX formulations, qMax Probe is compatible with most qPCR instruments.

*Please note these products ship on dry ice. Appropriate shipping charges apply unless otherwise noted on a quote.

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PR1MA
One-Step RT-PCR Kit

  • Convenient cDNA synthesis and PCR in a single tube from 1 pg total RNA
  • Formulated for highly specific and sensitive RT-PCR from any RNA templates
  • Incorporates thermostable reverse transcriptase and Hot-Start Taq for preparation at room temperature

The PR1MA One-Step RT-PCR Kit has been formulated for cDNA synthesis and subsequent PCR in a single tube for end-point analysis. This latest generation RT-PCR Kit consists of an MMLV-derived, thermostable Reverse Transcriptase (45°C to 55°C), an advanced RNase Inhibitor and PR1MA Hot Start Taq for ultra-sensitive one-step RT-PCR from as little as 1pg total RNA starting material.

The optimized buffer chemistry allows for efficient reverse transcription and PCR of problematic sequences with significant secondary structure (such as GC-rich targets). The PR1MA One-Step RT-PCR Kit is ideal for determining the presence or absence of RNA templates and quantifying expression through qualitative analysis of RNA transcription levels. The kit also efficiently synthesizes double-stranded cDNA for subsequent gene expression analysis.

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Item PR2110-100 has been discontinued by the manufacturer;
however, we will be continuing to supply the other quantities.

 

In place of item PR2110-100, please order items PR2110-50 or PR2110-200


PR1MA
qMAX
 cDNA Synthesis Kits

PR1MA now offers two cDNA Synthesis Kits, to meet a range of requirements.
 

The original cDNA Synthesis Kit is a 2-tube format for easy reaction setup and is ideal for 4 pg to 0.5 µg of input RNA. One tube includes our exceptionally stable Reverse Transcriptase combined with a potent RNAse inhibitor, and the other tube contains a 5X reaction buffer with an optimal mixture of anchored oligo (dT) primers and random hexamers to produce a non-biased population of cDNA. 
 

The 1st Strand cDNA Synthesis Flex Kit includes four components: a high-capacity Reverse Transcriptase, an optimized 5X buffer, separate solutions of oligo (dT) primers, and random hexamer primers. This multi-component format is ideal for 10 pg to 2.0 µg of input RNA and allows for greater flexibility in assay design.

 
PR1MA™ qMax cDNA Synthesis Kits
 
 
ItemDescriptionVolume (20 µL)
PR2100-C-SPR1MA™ qMax™ cDNA Synthesis Kit10 Reactions (Sample)
PR2100-C-25PR1MA™ qMax™ cDNA Synthesis Kit25 Reactions
PR2100-C-100PR1MA™ qMax™ cDNA Synthesis Kit100 Reactions
PR2100-C-250PR1MA™ qMax™ cDNA Synthesis Kit250 Reactions
 

PR1MA™ qMax First Strand cDNA Synthesis Flex Kits  
 
ItemDescriptionVolume (20 µL)
PR2110-SPR1MA™ qMax™ First Strand cDNA Synthesis Flex Kit10 Reactions (Sample)
PR2110-50PR1MA™ qMax™ First Strand cDNA Synthesis Flex Kit50 Reactions
PR2110-100PR1MA™ qMax™ First Strand cDNA Synthesis Flex Kit100 Reactions
PR2110-200PR1MA™ qMax™ First Strand cDNA Synthesis Flex Kit200 Reactions

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PR1MA dNTPs

  • Supplied as a ready-to-use 40 mM mix or a set of 4 separate 100 mM solutions
  • Free of impurities and inhibitors that reduce sensitivity and yield
  • No nuclease, protease or nickase activity
  • >99% pure, purified by HPLC
  • 24-month shelf life

PR1MA dNTP's are purified by HPLC in a strict process that results in greater than 99% purity. The stringent purification process eliminates PCR inhibitors such as tetraphosphates and pyrophosphates that can interfere with the sensitivity of your PCR and reduce yields.
The 40 mM dNTP Mix is a single tube that contains premixed dNTPs at a concentration of 10 mM each. The 100 mM dNTP Set contains four individual tubes, one each of dATP, dCTP, dGTP and dTTP. The nucleotides are supplied in ultra-pure water as an ammonium salt. Both the set and mix are stable for 24 months when stored at -20ºC.

Extensive quality control testing is performed to ensure the dNTPs are free of nuclease, protease and nickase activity. Each lot is performance tested in standard PCR, long PCR and qPCR reactions to assess reproducibility and sensitivity.

PR1MA dNTP Mix

ItemDescriptionVolume
PR3040-M-1PR1MA 40 mM dNTP Mix, Ready-to-use0.5 mL
PR3040-M-2PR1MA 40 mM dNTP Mix, Ready-to-use1 mL
PR3040-M-4PR1MA 40 mM dNTP Mix, Ready-to-use2 mL
PR3040-M-8PR1MA 40 mM dNTP Mix, Ready-to-use4 mL

PR1MA™ dNTP Set  

ItemDescriptionVolume
PR3101-S-1PR1MA 100 mM dNTP Set, dATP, dCTP, dGTP, dTTP250 uL / 25 umol each
PR3101-S-4PR1MA 100 mM dNTP Set, dATP, dCTP, dGTP, dTTP1 mL / 100 umol each
PR3101-S-20PR1MA 100 mM dNTP Set, dATP, dCTP, dGTP, dTTP20 x 250 uL / 25 umol each
 

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 PR1MA Hot Start Taq

  • Exceptional sensitivity for low-copy PCR
  • Ideal for multiplex PCR and amplification of GC-rich DNA
  • Same enhanced features as PR1MA Taq Polymerase
  • Buffer optimized for fast cycling and reproducibility 

Engineered for controlled polymerase activity, PR1MA Hot Start Taq is bound with a monoclonal antibody that blocks enzyme activity. This allows reactions to be set up at room temperature without the risk of non-specific amplification.

 

When samples are ready, the reaction mixture is heated to 95°C to denature the antibody and initiate the reaction. Similar to the standard PR1MA Taq, Hot Start Taq is provided with a 5X buffer, or in a ready-to-use 2X Master Mix. The Master Mix can be ordered with or without an incorporated red gel loading dye. The Red Dye Master Mix incorporates a red-loading dye that allows amplified samples to be loaded directly on an agarose gel.  The red color aids in visualization during pipetting, and higher density of the buffer ensures that the samples will drop into the gel wells.


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PR1MA High Fidelity Polymerase

  • 50X higher fidelity than Taq DNA polymerase
  • Works with crude DNA sample
  • Ideal for cloning, mutagenesis and microarrays
  • Produces blunt end products, to clone directly into blunt end vectors
  • Optimized buffer system with unique PCR enhancers 

For applications requiring highly accurate amplification, choose PR1MA High Fidelity DNA polymerase. Modified for better solubility and higher activity across a broad range of ionic conditions, this polymerase will amplify a wide range of targets, including those that are GC or AT rich as well as crude samples.

 

A 3'-5' proofreading exonuclease activity and an error rate of 4.55×10-7 makes PR1MA High Fidelity DNA Polymerase the perfect partner for cloning applications. The supplied 5X buffer with dNTPs is optimized for compatibility with a variety of targets.

Specifications

Item DescriptionVolume
PR1000-HF-SPR1MA High Fidelity DNA Polymerase20 Units (Sample)
PR1000-HF-200PR1MA High Fidelity DNA Polymerase200 Units (2 U/p1)
PR1000-HF-500PR1MA High Fidelity DNA Polymerase500 Units (2 U/p1)
PR1000-HF-1000PR1MA High Fidelity DNA Polymerase1,000 Units (2 U/p1)


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PR1MA High Fidelity Hot Start Master Mix

  • Leaves an A-overhang for TA cloning
  • Ideal for difficult, high GC content sequences
  • 10x fidelity of native Taq
  • Ideal for long PCR, up to 10kb targets 

PR1MA High Fidelity Hot Start Mix is a hot start 2x formulation which provides excellent sensitivity in low-copy number assays with 10x higher fidelity than Taq polymerase. The 2x master mix contains proprietary enhancers, an antibody-mediated hot-start mechanism, and a proofreading component for trouble-free PCR reaction assembly and performance.

 

The pre-optimized Hot Start Master Mix is supplied in a single tube, reducing the number of pipetting steps while improving throughput and reproducibility. The highly efficient buffer formulation and hot-start blend provide the ideal conditions for high-performance PCR and inactivity at room temperature thereby eliminating non-specific amplification.


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PR1MA  High Fidelity Master Mix

  • Leaves a blunt end
  • Rapid extension: up to 1 kb per 15 seconds
  • 100x fidelity of native Taq
  • Ideal for shorter, less complex targets

A 2x formulation which provides extreme sensitivity in low copy number assays with 100x the fidelity of native Taq, PR1MA High Fidelity Master Mix is perfect for shorter, less complex targets. The 2x master-mix contains proprietary enhancers and a proof-reading component for trouble-free PCR reaction assembly and performance. High Fidelity Master Mix delivers a unique balance of PCR sensitivity, high fidelity, versatility, and tolerance to inhibitors.

The pre-optimized Master Mix is supplied in a single tube, reducing the number of pipetting steps while improving throughput and reproducibility. The highly efficient buffer formulation provides the ideal conditions for high-performance PCR.

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PR1MA qMAX One-Step RT-qPCR Kits

  • RNA to cDNA to qPCR in one tube
  • High purity enzyme formulation for enhanced stability and performance
  • PR1MA Hot-Start Taq allows for preparation at room-temperature
  • Compatible with all qPCR instruments
  • Available for green fluorescence or probe detection
PR1MA qMAX One Step Kits allow for highly sensitive real time RT-qPCR assays to be performed directly from RNA templates.  Workflows are simplified with optimized formulations of ready-to-use 2X qPCR master mix and reverse transcriptase. Optimized buffer includes powerful RNase inhibitors and an extremely thermostable MMLV-derived reverse transcriptase enables robust first strand cDNA synthesis.  PR1MA Hot Start Taq uses an antibody mediated hot start mechanism allowing for sample preparation at room temperature.  Only after an initial incubation at 95°C will the Taq become active, so non-specific amplification is greatly reduced.  An inert blue dye is included in the Taq master mix to help simplify pipetting and reduce errors.

Both One-Step Kits are compatible with standard and fast cycling protocols and provide increased sensitivity, speed and reproducibility for a broad range of samples and targets.  The polymerase mix is available with different levels of ROX reference dye for compatibility with all qPCR instruments.

Two versions of our One-Step qPCR Kits are available:

PR1MA qMAX Green One-Step Kits incorporate our proprietary intercalating dye which exhibits higher fluorescent and lower PCR inhibition than other popular dyes such as SYBR.

PR1MA™ qMAX Probe One-Step Kits are optimized for use with popular TaqMan, Scorpions, and molecular beacon probes.

*Please note these products ship on dry ice.  Appropriate shipping charges apply unless otherwise noted on a quote.

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PR1MA SmartCheck DNA Ladders

  • Ready-to-use formulation includes loading buffer and tracking dye
  • 500 µL suitable for 100 lanes (5 µL per lane)
  • Higher intensity reference bands
  • Ultra pure production allows economical ambient shipping 

Technical Details
 

Protocol: Briefly vortex the tube and use 5 µL per lane. Additional loading buffer is not required.

Concentration: 0.1 mg / mL

Tracking dye: bromophenol blue and xylene cyanol

Buffer formulation: 10mM Tris-HCl (pH 8.0), 5 mM EDTA, 12.5% glycerol, 0.008% bromophenol blue, 0.008% xylene cyanol

Shipping and Storage: SmartCheck™ DNA Ladders are shipped at ambient temperature. On arrival, store at -20°C for optimum stability and long-term storage up to 15 months.

Production: SmartCheck™ ladders are produced from proprietary plasmids, digested to completion. A multistep chromatography method is used to ensure purity and DNA quality.

Quality Control: Each lot of SmartCheck™ DNA Ladders is tested with a spectrophotometer to confirm DNA concentration, as well as agarose electrophoresis to confirm band sharpness.

Specifications 

ItemDescriptionVolume
PR4005-100PR1MA™ SmartCheck™ 50bp DNA Ladder500 uL / 100 Lanes
PR4005-500PR1MA™ SmartCheck™ 50bp DNA Ladder5 x 500 uL / 500 Lanes
PR4010-100PR1MA™ SmartCheck™ 100bp DNA Ladder500 uL / 100 Lanes
PR4010-500PR1MA™ SmartCheck™ 100bp DNA Ladder5 x 500 uL / 500 Lanes
PR4100-100PR1MA™ SmartCheck™ 1kb DNA Ladder500 uL / 100 Lanes
PR4100-500PR1MA™ SmartCheck™ 1kb DNA Ladder5 x 500 uL / 500 Lanes
  

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PR1MA Mammalian Genotyping Kit

  • DNA extraction and amplification in 1 hour
  • Proprietary lysis buffer optimized for ear punches, tail snips and other mammalian tissues
  • Single tube - no organic solvents or clean up procedures
  • Enhanced PR1MA Hot Start Polymerase included

Traditionally, mammalian genotyping protocols have involved Proteinase K digestion, neutralization, organic extraction and lots of hands on time to get PCR-ready DNA.

The PR1MA Mammalian Genotyping Kit is quick and easy to use - add sample to the proprietary lysis buffer and incubate for 5-10 minutes, then add the deactivation buffer and incubate for 10 minutes. The crude lysate can then be amplified using fast PCR PR1MA Hot Start Taq Master Mix with red loading dye (included). The kit contains everything needed - just add sample and primers. 
 

PR1MA 1 Hour Mammalian Genotyping Kit 

Item

Description

Volume

PR1300-MG-S

PR1MA 1 Hour Mammalian Genotyping Kit

8 Reactions (Sample)

PR1300-MG-80

PR1MA 1 Hour Mammalian Genotyping Kit

80 Reactions

PR1300-MG-400

PR1MA 1 Hour Mammalian Genotyping Kit

400 Reactions

PR1300-MG-800

PR1MA™ 1 Hour Mammalian Genotyping Kit

800 Reactions

 PR1MA Genotyping Hot Start Master Mix, 2X Concentration with Red Dye

Item

Description

Volume

PR1301-HSR-400

PR1MA Genotyping Hot Start Master Mix, 2X Conc., Red Dye

400 Reactions


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