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You are here : PCR / DNA Amplification » Polymerases » p-Taq Polymerase

p-Taq Polymerase

p- Taq Polymerase is developed to enhance the specificity and yield of DNA amplification. The polymerase provides a convenient setting up at room temperature because of blocking the the enzyme with optimized mix of inhibitors

Cat.-no Description Amount Price € Shop
 S108  p- Taq Polymerase (qPCR)     200 units     65.00  add 
 S109  p- Taq Polymerase (qPCR)  5x200 units  259.00  add 

p- Taq Polymerase: Order/request by E-mail
p- Taq Polymerase: Datasheet
p- Taq Polymerase: Deutsche Beschreibung

Features: p- Taq Polymerase for qPCR is designed for Real Time PCR. Polyclonal antibodies inhibit the reaction at room temperature until after the first denaturation step. This prevents primer-dimers and other artefacts. Using the enzyme there is no need to adjust the existing standard PCR protocol in your lab.

Applications for Taq Polymerase:
- Hot Start and real time PCR
- Multiplex PCR
- Amplification of complex genomic and cDNA templates
- no primer-dimers and other artefacts; inactive at room temperature
- short activation time
- enhanced PCR sensitivity

Description:
Maximo p- Taq Polymerase is an optimized mixture of a high processive Taq Polymerase and polyclonal antibodies to Taq Polymerase. The enzyme is a thermostable DNA polymerase that possesses a 5´→3´ polymerase activity and a double-strand specific 5´→3´ exonuclease activity. The enzyme consists of a single polypeptide with a molecular weight of 94kDa.
 
Concentration: 5 u/µl

Unit definition:
One unit incorporates 10 nmol of deoxyribonucleotide into acid-precipitation material in 30 min at 72°C degree

Storage Buffer: 
50 mM Tris-HCl, pH 8.2, 0.1 mM EDTA, 0.1% Tween 20, 0.1% NP40, 1 mM DTT, 50% Glycerol

Reaction Buffer:
10X Buffer: 100mM KCl, 80mM (NH4)2SO4, 100mM Tris-HCl, pH9.0, 0.5% Nonident P40, 15 mM MgSO4

Quality control for Taq Poymerase:
Activity and performance test, SDS-PAGE purity, absence of endonucleases/nickases and exonucleases test
 
Usage:  
Use your existing and optimized protocol. In contrast to chemically modified Taq DNA pol. where the first denaturation step needs up to 15 min, Maximo p-Superhot Taq does not need a prolonged heating or denaturation time.

Components Volume per reaction
 10X reaction buffer  5 µl
 Mg+  optional
 dNTP-Mix (40mM)  1.0 µl
 Up-stream primer (10 µM stock)  0,5-2.5 µl
 Down-stream primer (10µM stock)   0.5-2,5 µl
 Template DNA  0.1-15 ng/ml plasmid DNA
 1-10 µg/ml genomic DNA
 Maximo p Taq Polymerase (5 u/µl)   0.2 - 1.0 µl  
 Sterile dest. Water (molecular bio. grade)  up to 50 µl total reaction volume

Note: 
- vortex all solutions carefully before using
- add the enzyme after Template DNA
- may you have to optimize the MgCl2 concentration for best result

General Thermo-Cycler protocol:
 Step  Time  Temperature
 Initial denaturation  4-5 min  94-95°C
 
25-30 Cycles:
 Denaturation
 Annealing
 Extension
 		  10-25 sec
 10-25 sec
 60 sec
 94-95°C
 55-65°C
 72°C per 1kb
 
 Final extension    5 min  72°C

Note: 
- In case of low amount of DNA template, additionally cycles may be used 

Transportation: on blue ice

Storage: Taq Polymerase can be stored at -20°C for 24 months

Related products:


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Overview Polymerases:
DFS-Taq Polymerase DNA-free
Taq Polymerase (DNA free) is a highly purified polymerase (DNA-free) especially for PCR reactions where freedom from endogenous template (i.e., E. coli DNA) is essential
Taq Polymerase
Maximo Taq Polymerase is a highly purified polymerase for routine amplification
Taq Polymerase 2X-preMix
Maximo Taq as 2X-preMix includes all components (Taq DNA polymerase, dNTPs, MgCl2, and reaction buffer) in an optimal concentration for routine PCR
Taq  Polymerase blue ready-to-load
Maximo Tag-Blue is a highly purified polymerase for routine amplification. The enzyme is ready-to-load. No extra dye or loading buffer is needed!
m-Superhot Taq DNA pol.
M-Superhot Taq Polymerase is developed to enhance the specificity, sensitivity and yield of DNA amplification. The enzyme provides a convenient setting up at room temperature
m-Anti-Taq
Mouse Monoclonal Antibody - Enhancer for Polymerase reactions
p-Superhot Taq DNA pol.
p-Superhot Taq Polymerase is developed to enhance the specificity and yield of DNA amplification. The polymerase provides a convenient setting up at room temperature because of blocking the the enzyme with optimized mix of inhibitors
Pfu/Psp DNA Polymerase
Pfu DNA polymerase generated PCR fragments exhibits the lowest error rate of any thermostable DNA polymerases. The fragments are blunt-ended for direct ligation
Pfu/Psp red DNA Polymerase RTL
Pfu DNA polymerase (RTU=READY-TO-LOAD) is a convenient Mixture of proof-reading Enzyme, red dye and loading buffer. It generated PCR fragments exhibits the lowest error rate of any thermostable DNA polymerases. The fragements are blunt-ended for direct ligation
Pfu/Psp DNA Polymerase 2X-preMix
Pfu DNA polymerase 2X-preMix is a convenient Mixture of proof-reading Enzyme, reaction buffer dNTP´s and MgCl2. It generated PCR fragments exhibits the lowest error rate of any thermostable DNA polymerases. The fragements are blunt-ended for direct ligation
Tth DNA Polymerase
Tth DNA Polymerase Maximo is used to reverse-transcribe RNA efficiently in the presence of manganese. PCR can be performed in the same tube using the intrinsic DNA polymerase activity simply by chelation of manganese cation and the addition of magnesium.


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