Robust real-time PCR master mix for amplification directly from blood, swabs or tissue
2 x conc. master mix
| Cat. No. | Amount | Price (EUR) | Buy / Note |
|---|---|---|---|
| PCR-396S | 2 x 1,25 ml (250 reactions x 20 μl) | 173,70 | Add to Basket/Quote Add to Notepad |
| PCR-396L | 10 x 1,25 ml (1.250 reactions x 20 μl) | 694,80 | Add to Basket/Quote Add to Notepad |
| PCR-396-100ML | 100 ml (10.000 reactions x 20 μl) | Ask for Quotation |
For general laboratory use.
Shipping: shipped on gel packs
Storage Conditions: store at -20 °C
avoid freeze/thaw cycles,
stable at 4 °C for up to 4 weeks
Shelf Life: 12 months
Form: liquid
Concentration: 2x
Description:
Direct qPCR ProbesMaster is designed for quantitative real-time analysis of target DNA directly from blood, swabs and animal- or plant tissue. The mix allows robust amplification avoiding the requirement of any prior DNA purification procedures.
The mix is recommended for use with dual-labeled fluorescent probes, e.g. TaqMan®, Molecular Beacon or Scorpion probes. It provides a powerful tool for multiplex-quantification of sample DNA in a broad dynamic range with exceptional sensitivity and precision.
The mix contains all reagents required for qPCR (except template, primer and labeled fluorescent probe) in a premixed 2 x concentrated ready-to-use solution. High robustness, reliability and sensitivity of the mix are based on a an antibody-blocked hot start polymerase in combination with an optimized and well-balanced buffer system.
The mix ensures fast and easy preparation with a minimum of pipetting steps and is specially recommended for:
Interference of remaining components from sample matrix
Due to the fast and easy but relatively rough sample preparation remaining components from the sample matrix may be co-transferred into the PCR assay. These remains are mostly blocked by a combination of specially optimized additives. If inhibition of the PCR reaction occurs with higher volumes of transferred sample volume, please reduce the sample volumes or use a dilution of the sample in 1x Direct Extraction Buffer or water.
Remaining components of the sample matrix may also show fluorescence signals specially in the yellow and red spectral range. If using this fluorescence range for multiplex PCR assays or if using ROX, please take special attention that there is no interference between fluorescence from remaining matrix material and the used fluorescence channels for amplicon detection.
ROX Reference Dye
The mix can also be used in combination with ROX reference dye (#PCR-351) in PCR instruments that are compatible with the evaluation of the ROX signal.
Content:
Direct qPCR ProbesMaster (red cap)
2x conc. mix of antibody-blocked Hot Start polymerase, dNTPs, reaction buffer, additives and stabilizers
Direct Extraction Buffer (yellow cap)
10x conc.
Please handle with care and wear personal protective equipment!
PCR-grade Water (white cap)
Procedure
Before starting, take reagents out from fridge and allow to thaw completely. Vortex all reagents briefly and spin down the liquids.
1. Sample preparation
1.a Blood Samples / Liquid Samples
1.b Samples from nasal or throat swabs
1.c Samples from Animal or Plant Tissue
| Sample size (diameter) | 1-2 mm | 3-4 mm | 5-8 mm |
| 1x Direct Extraction Buffer | 50 μl | 100 μl | 200 μl |
2. Preparation of the PCR Assay
Preparation of a master mix is crucial in quantitative PCR reactions to reduce pipetting errors. Prepare a master mix of all components except template as specified below. A reaction volume of 20-50 μl is recommended for most real-time instruments. Pipet with sterile filter tips and minimize the exposure of the labeled DNA probe to light. Perform the setup in an area separate from DNA preparation or analysis. No-template controls should be included in all amplifications.
| component | stock conc. | final conc. | 20 μl assay | 50 μl assay |
| Direct qPCR ProbesMaster | 2x | 1x | 10 μl | 25 μl |
| Extracted Sample | - | - | 1-2 μl | 2-5 μl |
| Forward Primer 11) | 10 μM | 300 nM | 0.6 μl | 1.5 μl |
| Reverse Primer 11) | 10 μM | 300 nM | 0.6 μl | 1.5 μl |
| TaqMan® / Dual Labeled Probe 11) | 10 μM | 200 nM | 0.4 μl | 1 μl |
| Forward Primer 22) | 10 μM | 300 nM | 0.6 μl | 1.5 μl |
| Reverse Primer 22) | 10 μM | 300 nM | 0.6 μl | 1.5 μl |
| TaqMan® / Dual Labeled Probe 22) | 10 μM | 200 nM | 0.4 μl | 1 μl |
| ROX Reference Dye #PCR-351 3) | 25 μM | 500 nM | 0.4 μl | 1 μl |
| PCR-grade water | - | - | fill up to 20 μl | fill up to 50 μl |
Mix the tubes briefly and spin down to remove bubbles.
3. PCR Cycling
Switch on the real-time PCR cycler and set all cycling parameters as recommended in the table below. Place the vials into the instrument and start the program.
| Initial denaturation | 95 °C | 2 min | 1x |
| Denaturation Annealing and elongation | 95 °C 60-65 °C 4) | 15 sec 30-60 sec5) | 35-45x |
To obtain optimal specificity and amplification results an individual optimization of the recommended parameters is recommended for each particular sample/primer pair.
4. Data Analysis
BIOZ Product Citations:
Direct Extraction Buffer
Signal word: Danger
Hazard statements:
Precautionary statements:
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