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IconStart® TopTaq DNA Polymerase is an engineered version of Taq DNA Polymerase combined with IconStart® technique. One binding protein binds to double-strand DNA template, preventing polymerase activity at room temperature. Other two binding proteins bind primers, preventing primer-dimer formation. Blocking proteins are released from primers and templates during the initial denaturation. This double blocking method has higher efficiency than antibody based, or chemically modified hot start PCR.
• Compared with IconStart® Taq DNA Polymerase, IconStart® TopTaq DNA Polymerase has higher amplification efficiency, specificity and sensitivity.
• IconStart® TopTaq DNA Polymerase offers 18-fold fidelity as compared to IconTaq® DNA Polymerase.
• The specificity is higher than antibody based or chemically modified hot start DNA polymerases.
• Template-independent “A” can be generated at the 3’ end of the PCR product. PCR products can be directly cloned into pIcon®-T vectors.
• Reduced nonspecific amplification and primer dimer formation.
• Different from Taq antibody, no risk of contamination from mammalian DNA.
• Different from chemical modification, long denaturing step is not needed.
• Amplification of genomic DNA fragment up to 15 kb.
Applications
• Complex templates
• GC/AT-rich templates
• Multiplex PCR
• High yield PCR
Storage
at -20 ? for two years
Shipping
Dry ice (-70 ?)
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