ProPrime Taq DNA Polymerase

Cat. No.: FP1508914
AVAILABLE TO ORDER
GRADE & PURITY Suitable for molecular biology ? Molecular-biology grade — free of nucleases and contaminants that degrade DNA/RNA. Use in cloning, PCR, and nucleic-acid work needing clean reagents. EnzymoPure™ ? EnzymoPure™ — Aladdin's line of high-quality enzymatic solutions. Use when enzyme purity and defined activity drive assay or process performance. for DNA and RNA applications ? For nucleic-acid (DNA & RNA) applications — nuclease-controlled across both. Use in workflows handling DNA and RNA together where degradation is a risk. 5 U/μL
 ·  off list, applied to all prices below.
Size
Status
Price
Qty
250U
FP1508914-250U
8-12 wks(?) Production requires sourcing of materials. We appreciate your patience and understanding.
$79.90
2.5KU
FP1508914-2.5KU
8-12 wks(?) Production requires sourcing of materials. We appreciate your patience and understanding.
$499.90
25KU
FP1508914-25KU
8-12 wks(?) Production requires sourcing of materials. We appreciate your patience and understanding.
$3,499.90
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Why this grade

Suitable for molecular biology,EnzymoPure™,for DNA and RNA applications,5 U/μL for DNA and RNA applications,Suitable for molecular biology,EnzymoPure™ for sensitive chromatographic and analytical workflows requiring minimal baseline interference.

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Storage & shipping

Store at -20°C,Avoid repeated freezing and thawing Ships Ice chest + Ice pads Check lot-specific COA for exact specifications.

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Quality documents

SDS, COA, datasheet, and spec sheet available for download. Lot-specific COA accessible via lot number lookup.

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Literature proof

Cited in 0 peer-reviewed publications across chromatography, organic synthesis, and cross-coupling reactions.

Overview

  ProPrime Taq DNA Polymerase is a mutant enzyme obtained by site-directed mutagenesis of wild-type Taq enzyme using genetic engineering techniques. Compared with the wild-type, this enzyme has higher affinity for templates and stronger resistance to inhibitors. It exhibits high tolerance to endogenous and exogenous interferents in clinical samples, enabling direct amplification of whole blood, crude extracts from fecal samples, and crude extracts from plant samples, which effectively reduces steps such as sample pretreatment and DNA extraction.This enzyme has a fast amplification rate, making it suitable for rapid PCR; it also has high detection sensitivity, which is applicable for low-template detection.

  It can be used in probe-based quantitative real-time PCR (qPCR) detection assays.

  This antibody-modified enzyme is modified with three monoclonal antibodies, which simultaneously block the 5’-3’ polymerase activity and 5’-3’ exonuclease activity of Taq enzyme. Before high-temperature heating, the blocking effect of the antibodies on the polymerase activity can effectively inhibit non-specific amplification caused by non-specific annealing of primers or primer dimers under low-temperature conditions, thereby improving the specificity and efficiency of amplification. The blocking effect of the antibodies on the exonuclease activity can reduce the cleavage of fluorescent probes under low-temperature conditions, ensuring a stable baseline in qPCR and obtaining a good S-shaped amplification curve.

  When the amplification reaction system is heated to 95°C for 2.5 minutes, the modified antibodies denature and dissociate, releasing the polymerase activity and exonuclease activity of Taq enzyme. Therefore, no special inactivation treatment is required, and the enzyme can be used under conventional PCR reaction conditions.

When used with the improved amplification buffer, it can be quickly thermally activated, effectively increasing the amount of reaction products and improving the sensitivity, specificity, and anti-interference ability of the PCR reaction.

Scope of Application

  Hot-start qPCR amplification, direct whole blood amplification, anti-interference amplification, rapid PCR, and ARMS (Amplification Refractory Mutation System)

Precautions

  1. For most amplification reactions, the initial denaturation time can be set at 95°C for 2.5 minutes. If the template is complex, the denaturation time can be adjusted appropriately.
  2. The extension time should be determined according to the length of the PCR product. For example, when amplifying a 2kb fragment of human genomic DNA, the extension time can be as fast as 15 seconds. If it is a complex template (such as using whole blood as a template for amplification), the extension time can be appropriately prolonged.

Other Precautions

  1. When performing PCR amplification using whole blood as a template, the volume of whole blood added is recommended to be controlled within 20% (v/v) of the reaction system volume.
  2. When used for quantitative real-time PCR (qPCR), the volume of whole blood added is recommended to be ≤ 5% (v/v) of the reaction volume; excessive addition of blood samples will affect the collection of fluorescent signals.

Usage Method

Preparation before Reaction System Configuration

1.1 Dissolve and mix all solutions required for the reaction at room temperature or 4°C, then place them on an ice bath or in an ice box. It is recommended to aliquot the reaction solutions for use to avoid repeated freezing and thawing.

1.2 The volume of the reaction system can be adjusted proportionally according to the project requirements, as long as the final concentration of each component remains consistent.

1.3 Refer to the table below to set up the quantitative real-time PCR (qPCR) reaction system. It is recommended that the preparation of the qPCR reaction system be carried out on an ice bath or in an ice box:

ComponentVolume AddedFinal Concentration
5×GN Buffer (without Mg²⁺)10 μL
dNTPs (25 mM each)0.4 μL0.2 mM
Template DNA5 - 10 μL
Forward Primer (10 μM)1 μL0.2 μM
Reverse Primer (10 μM)1 μL0.2 μM
Probe (10 μM)0.5 μL0.1 μM
ProPrime Taq DNA Polymerase (5U/μL)0.5 μL2.5 U/50 μL
MgCl₂ (100 mM)1 μL2 mM
ddH₂OTo 50 μL
Total Volume50 μL

*Recommended amounts of different types of templates in a 50 μL reaction volume are as follows:

Mammalian genomic DNA: 0.1 - 1 μg

E. coli genomic DNA: 10 - 100 ng

Plasmid DNA: 0.1 - 10 ng

1.4 The recommended amount of Mg²⁺ is 2 mM - 6 mM.

1.5 Vigorous shaking should be avoided during the preparation process. Mix the solution by gently pipetting up and down or slightly vortexing, then centrifuge at room temperature for a few seconds.

Reaction Procedure

1. Conventional Qualitative PCR (taking the amplification of a 1 kb fragment as an example)

Step NameTemperatureTimeNumber of Cycles
Heat Shock95°C2min30s1
Denaturation95°C20s30 - 35
Annealing55°C20s30 - 35
Extension72°C40s30 - 35
Extension72°C7min1
Storage12°C1

2. Fluorescent Quantitative PCR

Step NameTemperatureTimeNumber of Cycles
Heat Shock95°C2min30s1
Denaturation95°C15s35 - 40
Annealing + Extension55°C40s35 - 40

a. The settings of the PCR reaction (including temperature, time, number of cycles, etc.) need to be adjusted according to factors such as the template, primers, length of the PCR product, and GC content.

b. The extension time should be set based on the length of the PCR product. Generally, the fastest extension time for each 1 kb of product is 15 seconds. For example, if the length of the PCR product is 1 kb, the extension time can be set to 15 seconds; if the length of the PCR product is 2 kb, the extension time can be set to 30 seconds. If the amplification effect is not ideal, the extension time can be appropriately extended to 45 seconds, and so on for fragments of other lengths.

Experimental Examples

1. In direct whole blood amplification, the tolerance to whole blood of two competing products and Aladdin Taq DNA Polymerase was compared. The results showed that Aladdin Taq DNA Polymerase had stronger tolerance to whole blood: it could tolerate 10% whole blood in qPCR projects and 20% whole blood in PCR projects.

2. Using λDNA as the template to amplify a 1 kb target fragment, Aladdin antibody-modified enzyme exhibits higher amplification sensitivity, and its amplification efficiency with low template is significantly better than that of two competing products.

3.Using human genomic DNA as the template to amplify a 2 kb target fragment, the Aladdin antibody-modified enzyme can amplify the target fragment in a shorter extension time, with an average extension rate of 7.5 seconds per kilobase (s/kb), making it suitable for rapid PCR.

Specifications

Unit definition
One unit (U) of activity is defined as the activity that catalyzes the incorporation of 10 nanomoles (nmol) of total nucleotides into acid-insoluble substances within 30 minutes at 74°C, using activated salmon sperm DNA as the template/primer.
Bioactivity
5 U/μL
Storage and Shipping
Storage
Store at -20°C,Avoid repeated freezing and thawing
Shipped In
Ice chest + Ice pads
Stability And Storage
Store at -20℃ long term. Upon receipt, it is recommended to aliquot. Avoid freeze/thaw cycle.
Contents & Storage

FP1508914

Components

250U

2.5KU

25KU

Storage

FP1508914A

ProPrime Taq DNA Polymerase (5U/μL)

50 μL

500 μL

5 mL

-20℃

FP1508914B

5×GN Buffer(Without Mg²⁺)

1.0 mL

10×1.0 mL

100 mL

-20℃

FP1508914C

100 mM Mg²⁺

100 μL

1.0 mL

10 mL

-20℃

Documentation

📋 Safety Data Sheet (SDS)

Comprehensive hazard, handling, storage, and regulatory compliance document.

Download SDS →

✅ Certificate of Analysis (COA)

Lot-specific quality data. Enter your lot number to retrieve the exact COA.

Look up COA →

📊 Datasheet

Quick-reference summary of product specifications and applications.

View datasheet →

🔬 Specification Sheet

Full quality attributes and acceptance criteria for this grade.

View spec sheet →

Advanced Data

Certificates(CoA,COO,BSE/TSE and Analysis Chart)
C of A & Other Certificates(BSE/TSE, COO):
Analytical Chart:

Find and download the COA for your product by matching the lot number on the packaging.

2 results found

Lot NumberCertificate TypeDateItem
ZJ26F0333690Certificate of AnalysisMar 31, 2026 FP1508914
ZJ26F0333689Certificate of AnalysisMar 31, 2026 FP1508914
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