Neogreen qPCR Master Mix (2x)

Description

qPCR Green Master Mix (2x) NB-60-0003-01 is a Defined reaction mixture for real-time PCR.
It is highly efficient and optimized for optimal performance.
The mix includes a hot-start enzyme control mechanism, enhancing detection sensitivity.
Incorporates the latest advancements in PCR enhancer technology, such as buffer chemistry and robustly engineered enzymes.
Engineered to deliver precise and dependable results for accurate analysis.

Storage temperature

Store qPCR Green Master Mix (2x) at -30 to -15 °C in a constant temperature freezer. Minimize freeze-thaw cycles by storing in working aliquots. Protect from light.

Compatible real-time PCR instruments

Bio-Rad: CFX96™, CFX384™, Opticon™, Opticon™ 2
Qiagen (Corbett): Rotor-Gene™ 3000, 6000 & Q
Roche: Lightcycler® 96, 480 & Nano
Applied Biosystems (with optional ROX addition or ROX OFF): 7000, 7300, 7700, 7900, 7900HT, 7900HT FAST, StepOne™ & StepOne™plus, 7500, 7500 FAST, QuantStudio™ 5, 6, 7, 12k Flex & ViiA7™

Quality control assays

Genomic DNA contamination:

qPCR Green Master Mix is screened for the presence of bacterial genomic DNA. Trace amounts of E. coli gDNA may be detected through a highly sensitive real-time PCR assay using primers specific for the E. coli 16S rRNA gene. Acceptable limits are established according to the quantity of DNA contaminant to an amount not enough to originate a positive signal.

Nuclease assays:

To test for DNase contamination, 0.2-0.3 μg of pNZY28 plasmid DNA are incubated with the master mix for 14-16 h at 37 °C. To test for RNase contamination, 1 μg of RNA is incubated with the master mix for 1 h at 37 °C. Following incubation, the nucleic acids are visualized on a GreenSafestained agarose gel. There must be no visible nicking or cutting of the nucleic acids.

Functional assay :

qPCR Green Master Mixes are extensively tested for activity, processivity, efficiency, sensitivity and heat activation.