• Start Bioron International
• Hot-Start PCR
• PCR Products
• Devices
• Nucleotides
• DNA / Markers
• DNA-RNA Purification
• Other Enzymes
• Dialysis Membranes
• Plastic Consumables
Excellent Products from Bioron

• PCR Products
  • Overview Polymerases
  • DFS-Taq DNA Polymerase -- The "Cleaner" Taq (E-Coli-FREE ) ---
  • DFS-Gen-Taq Mastermix
  • Anti Taq
  • SuperHoTTaq "Hot-Start" DNA Pol.
  • Red SuperHoTTaq (Hot Start) DNA pol.
  • qPCR Mastermix
  • Dry SuperHoTTaq Mastermix-blue stain
  • DryHoTTaq Mastermix qPCR
  • GC-rich PCR
  • Tth DNA Polymerase
  • Pfu DNA Polymerase
  • UDG
  • AMV-RT
  • M-MuLV-RT
  • 1 Tube RT-PCR Kit "Hot-Start" for qPCR
  • RNase Inhibitor
  • Blunt-end cloning
  • PCR Theory & Protocols
  • Take It Easy PCR Kit
  • PCR-buffer I
  • PCR-buffer II
  • PCR-buffer III
  • dU-HOT Mastermix
  • Taq T DNA Pol.
  • Taq red DNA Pol.
  • Klein Taq DNA Pol.
  • Psp DNA Polymerase
• Real time PCR
• Devices
• Diagnostic Kits
• DNA Marker, DNA, Plasmid
• DNA-RNA Purification
• Protein Purification
• Nucleotides
• Dialysis Membranes
• Other Enzymes
• Mol-Bio Chemicals
• Restriction Enzymes
• Mutation Analysis
• Tubes, tips, Tissue culture
• Advertising 07/08
• Distribution

Download
Catalog 2007

Klein Taq

Datasheet: Klein Taq DNA Polymerase

Deutsches Datenblatt: Klein Taq DNA Polymerase

Description:
KleinTaq is a derivative of Taq DNA polymerase. It is a 5'-exo-minus N-terminally truncated Thermus aquaticus DNA polymerase. As expressed from a gene construct in E.coli, translation initiates at Met236, bypassing the 5'-3' exonuclease domain of the DNA polymerase-encoding gene.

The enzyme reveals a highly active and even more heat-stable DNA polymerase activity in comparison with Taq DNA polymerase. The optimal range of Mg²⁺ concentration for KleinTaq is broader than for the majority of thermostable polymerases. This feature allows to optimize reaction conditions easier then for other polymerases. Repeated exposure to 98°C does not diminish the enzyme activity. Significant activity remains even after exposure to 99°C.

The mutation rate during polymerization is twofold lower for KleinTaq in comparison with full-length Taq DNA polymerase. KleinTaq has a very low background ability to extend a mismatched 3'-oligonucleotide end making it suitable for mutation analysis with mutation-specific oligonucleotides.

Concentration:
5-10000 units/ml

Unit definition:
One unit is defined as the amount of enzyme that incorporates 10 nmoles of dNTPs into acid-insoluble form in 30 min at 72°C.

Storage buffer:
10 mM K-phosphate pH 7,0, 100 mM NaCl, 0,5 mM EDTA, 1 mM DTT, 0,01% Tween 20, 50% glycerol

Storage:
-20^oC

Reaction buffer 10x incomplete:
160 mM (NH₄)₂SO₄; 670 mM Tris-HCl pH (ph 8,8) ; 0,1% Tween-20

Reaction buffer 10x complete:
160 mM (NH₄)₂SO₄; 670 mM Tris-HCl pH (ph 8,8) ; 0,1% Tween-20, 25 mM MgCl₂

Reaction buffer 10x complete II KCl: 
500 mM KCl; 100 mM Tris-HCl pH (ph 8,8) ; 0,1% Tween-20, 15 mM MgCl₂

Plus one tube MgCl2 (100mM)

Quality control:
Activity, SDS-PAGE purity, absence of endonucleases/ nickases and exonucleases  

Klein Taq protocol for ~ 2000 bp amplification

for 50 µl volume:  

Thermocycling:
The number of cycles will depend on the amount of template DNA. In most cases 25 cycles are sufficient. For  low copy number genes or rare DNAs, 30-35 cycles is recommended. The amplification parameters will vary depending on the primers, amplicon size and the thermal cycler used. It may be necessary to optimize the system. For 5 - 10 kb amplicon increase the extension time to 6-10 min.

For example: Thermal Cycler 480 (Perkin-Elmer-Cetus); amplicon size 500 - 2000 bp, template 10 ng plasmid DNA .

The reaction proceeded in 25 cycles:

94°C             30 - 45 s
58 - 61°C            30  s
72°C                  100 s

Copyright © BIORON GmbH