Description
The StableLink RT-qPCR Kit (with UDG) is a two-component, probe-based RT-qPCR master mix comprising Buffer Mix and Enzyme Mix. It is designed for sensitive fluorescent quantitative PCR detection in single or multiplex RNA targets. Optimized for performance, the buffer system is uniquely formulated to support both Taq DNA polymerase and reverse transcriptase activity, ensuring broad target compatibility and exceptional reaction stability. This kit incorporates a dUTP/thermolabile UDG carryover prevention system, enabling rapid degradation of uracil-containing contaminants at room temperature. Applications: Qualitative/quantitative PCR, multiplex PCR.Product Component TableU1492587Component100T1000T10000TStorageU1492587AStableLink RT-PCR Buffer Mix1.25 mL12.5 mL125 mL-20℃U1492587BStableLink RT-PCR Enzyme Mix100 µL1 mL10 mL-20℃ ProtocolReaction Setup Preparation:1. Thaw all required reagents at room temperature or 4°C. Mix thoroughly before use.2. Prepare the PCR Reaction Mixture according to the table below:Component Volume for 25 µL SystemFinal ConcentrationStableLink RT-PCR Buffer Mix12.5 µL1×StableLink RT-PCR Enzyme Mix1 µL1×Primer/Probe Mix1 µL/Template5 µL/ddH2OTo 25 µL/Total Volume25 µLNote: "1x" indicates the working concentration of the enzyme mix as provided.The amounts of primers, probes, and template can be adjusted according to experimental requirements.Adjust the volumes of primers, probes, and template as needed for your specific assay; use RNase-Free ddH₂O to bring the reaction to the final volume.To prepare reaction volumes other than 25 µL (e.g., 50 µL), scale the reagent volumes proportionally (e.g., double the volumes for a 50 µL reaction).3. Mixing and Setup:After preparing the reaction mixture, mix gently by pipetting or brief vortexing. Centrifuge briefly to collect the contents at the bottom of the tube. Proceed to PCR amplification.Standard Thermal Cycling Protocol:StepTemperatureTimeCirculation150℃10min1295℃2min1395℃15s45460℃40s (Acquire Fluorescence)45