-
Chemiluminescent Western blotting
- AdvanStain Iris
- WesternEaze-Chemi Kit
- AdvanStain Total Fluorescent Protein Staining Kits
- AdvanBlock-Chemi blocking solution
- FLASHBlot transfer buffer
- FLASHBlot-SD transfer buffer
- Development folders
- WesternBright ECL HRP substrate
- WesternBright ECL Spray
- WesternBright Quantum HRP substrate
- WesternBright Sirius HRP substrate
- HRP-conjugated secondary antibodies
- LucentBlue X-ray film
- Background Quenching Sheets
- WesternBright ChemiPen
- Transfer membranes
- Incubation trays
- AdvanWash washing solution
- Western Blot Strip-It Buffer
- Blotting sponge pads
- Blotting papers
- X-ray film cassette
-
Fluorescent Western blotting
- FLASHBlot transfer buffer
- AdvanBlock-Fluor blocking solution
- AdvanBlock-PF blocking solution
- AdvanStain Total Fluorescent Protein Staining Kits
- LightSaver™ Fluorescence Enhancing Solution
- FLASHBlot-SD transfer buffer
- WesternBright MCF
- SpectraDye Secondary Antibodies
- SpectraDye Antibody Labeling Kits
- Background Quenching Sheets
- Transfer membranes
- Development folders
- Incubation trays
- AdvanWash washing solution
- Fluorescent Western standardization blot
- Blotting papers
- ELISA
- Electrophoresis
- Antibodies and antibody labeling
- Sample preparation
- Purification
- Protein staining
-
Buffers and solutions
- FLASHBlot transfer buffer
- AdvanBlock-PF blocking solution
- Western Blot Strip-It Buffer
- AdvanBlock-Chemi blocking solution
- AdvanBlock-EIA blocking solution
- AdvanBlock-Fluor blocking solution
- Protein sample loading buffers
- FLASHBlot-SD transfer buffer
- AdvanWash washing solution
- 10X EIA Coating Buffer
- LightSaver™ Fluorescence Enhancing Solution
- Avant buffer pouches
- SARS-CoV-2
- Custom services
New special offers are available!
RapidClean
The fast and easy way to remove protein from RNA and DNA samples
- Complete removal of proteins from aqueous solutions of nucleic acids
- Protocol less than 5 minutes, start to finish
- Non-toxic alternative to phenol-chloroform extraction
- Nucleic acid recovery rates >95%
- Recovery of nucleic acids from 5 nucleotides to greater than 40 kb
- Suitable for DNA, RNA, cDNA, microRNA, oligonucleotides
Rapid clean resin arrives as a ready-to-use 10x slurry.
Kit includes:
RapidClean resin
Spin filters
| CAT # | PRODUCT | SIZE | PRICE | QUANTITY | |
|---|---|---|---|---|---|
| R-14011-250 | RapidClean Resin, 0.25 ml | 250ul |
$ 80.00 (USD) |
||
| R-14011-B10 | RapidClean Resin, 1 ml | 1ml |
$ 233.00 (USD) |
||
| K-01001-010 | RapidClean Protein Removal Kit, 10 rxns | 10 rxns |
$ 178.00 (USD) |
||
| K-01001-025 | RapidClean Protein Removal Kit, 25 rxns | 25 rxns |
$ 360.00 (USD) |
Description
In less than 5 minutes, completely remove protein from aqueous solutions of single- and double-stranded nucleic acids.
RapidClean is a novel affinity resin designed to remove all protein from aqueous solutions of nucleic acids, providing an alternative to hazardous and lengthy phenol-chloroform procedures. The RapidClean resin binds and removes protein in a 5-minute protocol that combines convenience, speed, and nucleic acid recovery rates in excess of 95%.
 |
Figure 1. RapidClean completely removes T4 DNA ligase. No detectable ligase activity remains in a reaction mix after exraction with RapidClean (lane 2). EcoRI digested λ-DNA (lane C, Control) was incubated for 16 hours at room temperature with T4 DNA ligase (lane 1) or with the same mixture extracted with RapidClean (lane 2). |
|
Figure 2. Extraction with RapidClean completely removes Exonuclease III. ϕX174/HaeIII DNA (Lane M) was digested by a 40 min incubation at 37 °C with 10 units of Exonuclease III (lane 1), but no digestion occured when the enzyme mix was extracted twice with RapidClean before addition of the ϕX174/HaeIII DNA target (lane 2).
|
 |
 |
Figure 3. RapidClean purifies plasmid DNA as efficiently as phenol-cholorform extractions.RapidClean purifies plasmid DNA as efficiently as phenol-cholorform extractions. Crude plasmid pellet containing pUC119 plasmid DNA was ethanol precipitated, suspended in TE buffer (lane 1), treated with RNase (lanes 2 and 5), and extracted with RapidClean once (lane 3) or twice (lane 4), or extracted with phenol-chloroform once (lane 6) or twice (lane 7). |
|
Figure 4. Extraction with RapidClean completely removes DNase I, Mung Bean Nuclease, and S1 nuclease activity.Extraction with RapidClean completely removes DNase I, Mung Bean Nuclease, and S1 nuclease activity. M12mp18 ssDNA (lane 1) is completely digested by 30 minute incubations at 37°C with DNase 1 (lane 2), Mung Bean Nuclease (lane 4) or S1 nuclease (lane 6), but no residual nicking activity is observed if the reactions are first extracted twice with RapidClean (lanes 3, 5, and 7). Lane M: 1 kb DNA ladder.
|
 |
Connect