PR1MA Taq provides superior results for routine applications. Modified to improve DNA-binding, this polymerase offers higher solubility and greater template affinity, resulting in consistently superior performance. PR1MA Taq Polymerase exhibits a 5' to 3' nuclease activity, but no 3' to 5' (proofreading) activity and works well with a wide range of DNA templates including GC-rich sequences.
The polymerase is supplied with a 5X buffer containing MgCl2 and proprietary mix of enhancers (dNTP's not included). For convenience, PR1MA Taq is also available in a ready to use 2X Master Mix - just add primers and template DNA. Our "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.
PR1MA™ SmartStain™ PS (Pre-Stain) can be used as a direct replacement for Ethidium Bromide in agarose and polyacrylamide gel electrophoresis. The stain emits green fluorescence when bound to dsDNA or ssDNA and emits red fluorescence when bound to RNA. PR1MA™ SmartStain™ PS exhibits excitation peaks at 290 nm and 490 nm, allowing it to be used with UV and blue light.
Supplied as a ready-to-use 2X master mix, PR1MA qMax Green has been engineered for high sensitivity, fact cycling and excellent reproducibility. PR1MA Hot Start Polymerase provides accurate PCR of a variety of templates including low copy number and difficult sequences, while the proprietary qMax Green intercalating dye exhibits higher fluorescence and lower PCR inhibition than other popular green dyes.
These two components are supported by a specially formulated buffer with an exacting combination of salts, PCR enhancers, stabilizers and pH that results in earlier Ct values and a high specificity across a broad dynamic range.*Please note these products ship on dry ice. Appropriate shipping charges apply unless otherwise noted on a quote.
PR1MA Taq Plus
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
Item
Description
Volume
PR1000-TP-S
50 Units (Sample)
PR1000-TP-250
250 Units (5 U/p1)
PR1000-TP-500
1,000 Units (5 U/p1)
PR1MA Taq Plus Master Mix, 2X Concentration
PR1001-TP-S
20 Reactions (Sample)
PR1001-TP-200
200 x 50 µL Reactions
PR1001-TP-1000
1,000 x 50 µL Reactions
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.
Successful PCR requires careful control of many variables. Pipetting errors, poor performing polymerases, dNTP concentrations, are just a few of the variables that can all contribute to reaction problems. PR1MA has developed their new qMAX™ Gold to control these variables and help you achieve the best possible amplification performance. To reduce the chance of pipetting errors, qMAX™ Gold includes an inert yellow dye so small volumes are easy to visualize in PCR plates. qMAX™ Gold is a ready to use, 2X mastermix of PR1MA Hot Start Taq enzyme, dNTPs, a sensitive fluorescent intercalating dye, and optimized reaction buffer. The Hot Start Taq allows reaction set up at room temperature while the temperature stable formulation guarantees optimal performance even if the mix is left at room temperature for extended periods.Just add primers and DNA targets to the mix, and then proceed to amplification. qMAX™ Gold is compatible with all real time thermal cyclers and exhibits high sensitivity with normal or fast 2-step cycling protocols. *Please note these products ship on dry ice. Appropriate shipping charges apply unless otherwise noted on a quote.
PR1MA One-Step RT-PCR Kit
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.
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 set up 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, and separate solutions of oligo (dT) primers, and random hexamer primers. This multi-component format is ideal for 10pg to 2.0µg of input RNA and allows for greater flexibility in assay design. PR1MA qMax cDNA Synthesis Kits
Volume (20 µL)
PR2100-C-S
PR1MA qMax cDNA Synthesis Kit
10 Reactions (Sample)
PR2100-C-25
25 Reactions
PR2100-C-100
100 Reactions
PR2100-C-250
250 Reactions
PR1MA qMax First Strand cDNA Synthesis Flex Kits
PR2110-S
PR1MA qMAX First Strand cDNA Synthesis Flex Kit
PR2110-50
50 Reactions
PR2110-100
PR2110-200
200 Reactions
PR1MA dNTPs
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.
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.
The 40mM dNTP Mix is a single tube that contains premixed dNTPs at a concentration of 10mM each. The 100mM 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. PR1MA dNTP Mix
PR3040-M-1
PR1MA 40 mM dNTP Mix, Ready-to-use
0.5 mL
PR3040-M-2
1 mL
PR3040-M-4
2 mL
PR3040-M-8
4 mL
PR1MA dNTP Set
PR3101-S-1
PR1MA 100 mM dNTP Set, dATP, dCTP, dGTP, dTTP
250 µL/25 µmol each
PR3101-S-4
1 mL/100 µmol each
PR3101-S-20
20 x 250 µL/25 µmol each
PR1MA Hot Start Taq
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.
PR1MA High Fidelity Polymerase
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.
PR1000-HF-S
PR1MA High Fidelity DNA Polymerase
20 Units (Sample)
PR1000-HF-200
200 Units (2 U/p1)
PR1000-HF-500
500 Units (2 U/p1)
PR1000-HF-1000
1,000 Units (2 U/p1)
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 proof-reading 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.
