For security reasons, you will be logged out in 4 minutesThis video has been hidden to respect your third-party cookie preferences.Authorise YouTube cookies when viewing videos presenting our products or services.
• Optimized mixture of thermostable DNA polymerases Taq (Thermus aquaticus), Pfu (Pyrococcus furiosus) and a polymerization activator • Ultrapure recombinant polymerases, thermostable and hot start. Pfu proofreading • The hot start property of the polymerases makes them inactive at room temperature allowing the preparation of the reaction mix at room temperature • Unique composition of the reaction buffer promoting pH stability at high temperature and ensuring high efficiency for long sequence amplifications • Amplification of genomic DNA sequences from 3 to 25 kb and episomal DNA sequences up to 40 kb • Particularly suitable for the amplification of eukaryotic genomes • Ideal for genome mapping and sequencing of long fragments • Supplied with a 10X reaction buffer • Available in 100 and 500 unit formats
• For demanding PCR applications in which high specificity are essential • Reduces nonspecific priming • Kit Contents: Tris-HCl, KCl, MgCl₂, dNTPs, Taq DNA Polymerase, Hot Start Activator protein, additional MgCl₂ tube
The RTG (Ready-To-Go) is to provide the mix necessary for the reaction as preformulated, premixed, predispensed beads
• Increased reproducibility • Minimized pipetting steps • Reduced the potential for contamination • Long-term ambient-temperature stable (> 12 months)
Illustra Hot Start Mix RTG beads: for PCR requiring high amplification specificity. The only reagents to be added are water, the DNA to amplify and the primers.
Polymerase Chain Reaction (PCR) is covered by patents held by Roche Molecular Systems and F Hoffmann-La Roche Ltd.
• For the stabilization of DNA, RNA or circulating, cell-free DNA (ccfDNA) depending on Cat.No. • Secure and standardized sampling • CE/IVD certified • Compatible with sensitive applications: RT-qPCR, NGS, methylation...
• DNA polymerase hot start at an initial concentration of 2.5 U/µl • Increases PCR specificity, sensitivity and throughput by reducing the risk of mismatch and primer-dimer formation • Activated during the initial 10 min denaturation step at 95 °C • Conserved 5'-'3' exonuclease activity and absence of 3'-'5' exonuclease activity • Adds a free adenine to the 3' end of the amplicon (monoadenylation) • Kit with 3 different 10X reaction buffers: without MgCl₂ (A), with MgCl₂ (B), with 2 inert dyes for direct deposit (C) • Kit supplied with dNTPs (separate tube)
• Fast qPCR mix with SYBR Green I dye for use with most real-time thermal cyclers • Contains Perpetual Taq hot start DNA polymerase, optimised buffer, dNTPs (dTTP partially replaced by dUTP) and SYBR Green I dye • Uracile N-glycosylase (UNG) heat-labile provided to limit the risk of cross-contamination (optional use) • Available with ROX dye (separate tube) for standardisation
• Fast qPCR mix with hydrolysis probes for use with most real-time thermal cyclers • Contains Perpetual Taq hot start DNA polymerase, optimised buffer, dNTPs (dTTP partially replaced by dUTP) and SYBR Green I dye • Uracile N-glycosylase (UNG) heat-labile provided to limit the risk of cross-contamination (optional use) • Available with ROX dye (separate tube) for standardisation
• Mix designed for high resolution melting curve (HRM) analysis of DNA samples • Allows detection of gene mutations and single polymorphisms (SNPs) including class III and IV • Contains onTaq hot start DNA polymerase, optimised buffer, dNTPs and fluorescent dye • OnTaq polymerase activated during the initial denaturation step of the PCR at 95 °C for 15 min