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제품 설명
4X CAPITAL™ qPCR Green Master Mix
제품 번호
BR0501701 - 200 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix
BR0501702 - 1000 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix
BR0501703 - 4000 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix
BR0501801 - 200 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix LROX
BR0501802 - 1000 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix LROX
BR0501803 - 4000 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix LROX
BR0501901 - 200 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix HROX
BR0501902 - 1000 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix HROX
BR0501903 - 4000 reactions of 20 µl / 1 ml CAPITAL qPCR Green Master Mix HROX
제품 특징
Description
biotechrabbit CAPITAL qPCR Green Mix allows sensitive and specific amplification with an excellent signal to noise ratio and rapid extension rates. Extremely low-copy-number targets can be detected with high efficiency over several logs of template concentration, while primer-dimer formation is efficiently minimized.
CAPITAL qPCR Green Mix shows accurate and robust performance in wide range of applications, including gene expression and copy number variation analysis.
To enable the use of the kit on qPCR platforms with different reference dye concentration requirements, three kit formats are available: a kit containing no ROX, as well as LRox and HRox versions containing ROX in the corresponding concentrations.
Info: Recommended annealing temperature is 2°C above primer Tm (use gradient PCR to optimize the annealing temperature).
Other Information
Quality ControlFunctional assayMix tested functionally in qPCR. |
Protocols
When assembling the amplification reactions, care should be taken to eliminate the possibility of contamination with undesired DNA.
Component | Volume | Final concentration |
Primer Mix (Reverse and Forward) | Variable | 100–400 nM |
Too high primer concentrations result in unspecific amplification and should be avoided. | ||
Template DNA | Variable | 10 pg – 100 ng |
Use diluted or undiluted cDNA from less than 1 µg RNA | ||
CAPITAL qPCR Green Mix, 4× | 5 µl | 1× |
Nuclease free water | Variable |
|
Total volume | 20 µl |
|
Step | Temperature | Time | Cycles |
Initial activation | 95°C | 2-3 min | 1 |
Denaturation | 95°C | 10–15 s | 40–45 |
Annealing/Extension* | (60-68°C) | 30 s |
*Recommended annealing/extension temperature is primer Tm +2°C. Use gradient PCR to optimize the annealing temperature. Do not use temperatures below 60°C. Do not exceed 30 seconds.
For melt analysis refer to instrument instructions.
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