Taq DNA Polymerase

CAS: 9012-90-2 Cat. No.: FP1508912 Peso molecular: 94 kDa Número EC: 232-741-2
Disponible para pedir
GRADE & PURITY Recombinant ? Recombinant — produced via recombinant expression for defined sequence and consistency. Use for reproducible, animal-free proteins of known origin. 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
Estado
Price
Qty
1KU
FP1508912-1KU
8-12 wks(?) Production requires sourcing of materials. We appreciate your patience and understanding.
29,90US$
10KU
FP1508912-10KU
8-12 wks(?) Production requires sourcing of materials. We appreciate your patience and understanding.
189,90US$
Enter a quantity for the sizes you want to add.
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Why this grade

Recombinant,Suitable for molecular biology,EnzymoPure™,for DNA and RNA applications,5 U/μL for DNA and RNA applications,Recombinant,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.

📋

Quality documents

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

📚

Literature proof

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

Descripción general

Taq DNA Polymerase, abbreviated as Taq enzyme, is one of the most commonly used DNA polymerases. It is a highly thermostable DNA polymerase derived from the thermophilic bacterium Thermus aquaticus, with a molecular weight of 94 kDa. The enzyme is obtained through recombinant expression of the Thermus aquaticus DNA Polymerase gene, followed by separation and purification. PCR products amplified using this product have an additional "A" base at the 3’ end, allowing direct cloning into T-Vectors (the magnesium ion concentration in the buffer is 2 mM).

Component List

FP1508912

 

Components

1KU

10KU

Storage

FP1508912A

 

Taq DNA Polymerase (5U/μL)

200 μL

2×1.0 mL

-20℃

FP1508912B

 

5×Taq Buffer (Mg²⁺ Plus)

4×1.0 mL

40 mL

-20℃

Application Scope

PCR amplification using the hot-start method


Precautions

Primer Design (descriptions of key considerations for primer design)Examples:
  1. The last base at the 3' end of the primer is preferably G or C.
  2. The final 8 bases at the 3' end of the primer should avoid consecutive mismatches.
  3. The 3' end of the primer should avoid forming hairpin structures.
  4. The Tm values of the forward and reverse primers should preferably differ by no more than 1℃, and the optimal Tm value range is 55~65℃ (Primer Premier 5 is recommended for calculating primer Tm values).
  5. Additional sequences of the primer, i.e., sequences not paired with the template, should not be included in the Tm value calculation.
  6. The GC content of the primer should be controlled between 40% and 60%.
  7. The overall distribution of A, G, C, and T in the primer should be as uniform as possible, avoiding regions with high GC or AT content.
  8. Avoid complementary sequences of more than 5 bases within a single primer or between the two primers; complementary sequences of more than 3 bases at the 3' ends of the two primers should also be avoided.
  9. After primer design, use the NCBI BLAST tool to verify primer specificity to prevent non-specific amplification.

Usage Method

Preparation before reaction system preparation:
a. Thaw all required solutions at room temperature (20±5℃) or 2~8℃, mix thoroughly by inverting up and down, and place on an ice bath or in an ice box. It is recommended to aliquot the reaction solutions for use to avoid repeated freeze-thaw cycles.
b. Prepare the PCR reaction system with reference to the table below. The preparation of the PCR reaction system is recommended to be performed on an ice bath or in an ice box.
Component
Added Volume
Final Concentration
5×Taq Buffer (Mg²⁺ Plus)10 μL
dNTPs (2.5 mM each)0.4 μL0.2 mM
Forward Primer (10μM)1 μL0.2 μM
Reverse Primer (10μM)1 μL0.2 μM
Taq DNA Polymerase (5U/μl)0.5 μl2.5U/50μl
Template DNA*10 μl/
ddH₂OTo 50 μL/
Final  Volume
50 μL

*Recommended amounts of different types of templates in a 50µl 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;

c. Avoid vigorous shaking during preparation. Mix gently by pipetting up and down or slight vortexing, then centrifuge at room temperature for a few seconds.


Reaction Procedure

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

b. PCR reaction settings (including temperature, time, and number of cycles) should be adjusted according to different conditions such as template type, primers, length of PCR product, and GC content.

c. The time for STEP4 (Extension) should be set based on the length of the PCR product. Typically, the extension time is 1 min per kb of the product. For example, if the PCR product length is 1 kb, the extension time can be set to 1 min; if the product length is 2 kb, the extension time can be set to 2 min, and so on.

d. For the first-time PCR, set the number of cycles to 35 to maximize the chance of amplifying the expected PCR product. For semi-quantitative or quantitative PCR, the number of cycles must be properly optimized to ensure the reaction does not reach the plateau phase.

Specifications

Definición de unidad
The activity is defined as 1 unit (U) when 10 nmol of total nucleotides are incorporated into acid-insoluble substances within 30 minutes at 74℃, using activated chinook salmon sperm DNA as the template/primers.
Bioactividad
5 U/μL
Almacenamiento y envío
Condiciones de almacenamiento de almacenamiento
Store at -20°C,Avoid repeated freezing and thawing
Enviado en
Ice chest + Ice pads
Estabilidad y almacenamiento
Store at -20℃ long term. Upon receipt, it is recommended to aliquot. Avoid freeze/thaw cycle.
Contents & Storage

FP1508912

 

Components

1KU

10KU

Storage

FP1508912A

 

Taq DNA Polymerase (5U/μL)

200 μL

2×1.0 mL

-20℃

FP1508912B

 

5×Taq Buffer (Mg²⁺ Plus)

4×1.0 mL

40 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

Certificados (CoA, COO, BSE/TSE y tabla de análisis)
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 TypeFechaArticulo
ZJ26F0434220Certificate of AnalysisApr 14, 2026 FP1508912
ZJ26F0434221Certificate of AnalysisApr 14, 2026 FP1508912
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