DIG Gel Shift Kit, 2nd generation
ROCHE/03353591910 - storage temp.:-20°C (-15°C to -25°C)
Product Type: Chemical
Detection of digoxigenin-labeled oligonucleotides.
12 Principles of Green Chemistry: Principle 4—Designing Safer Chemicals
Chemical products should be designed to affect their desired function while minimizing their toxicity.
Chemical products should be designed to affect their desired function while minimizing their toxicity.
| description | New formulation containing Terminal Transferase, recombinant. |
| greener alternative category |  , Aligned |
| greener alternative product characteristics | Designing Safer Chemicals Learn more about the Principles of Green Chemistry . |
| manufacturer/tradename | Roche |
| Quality Level | 100 |
| shipped in | dry ice |
| storage temp. | −20°C (−15°C to −25°C) |
| sustainability | Greener Alternative Product |
| Application: | DIG Gel Shift Kit, 2nd generation has been used for nonradioactive detection of sequence-specific DNA binding proteins. The DIG Gel Shift Kit is used to prepare nonradioactive, 3′-end labeled oligonucleotide probes to detect DNA-protein complexes in a "gel mobility shift assay". |
| Features and Benefits: | The electrophoresis assay works best with shorter (30 to 100bp) DNA fragments, since these are less likely to have sequences that are outside the specific binding site, but can interact nonspecifically with target proteins. • Convenient, since the technique does not require special equipment or technology. • Reproducible, since DIG-labeled probes are stable indefinitely. • Safe, because the assay is nonradioactive. • Reliable, because the kit provides DIG-labeled control oligonucleotides to establish that the assay is working. • Function-tested with the controls provided in the kit (See "Quality"). • Sensitive, since the kit can detect as little as 20fmol of the control oligonucleotide (after it is labeled according to the kit protocol). |
| General description: | DIG Gel Shift Kit, 2nd generation contains reagents for nonradioactive 3′-end labeling of oligonucleotides, to be used in a "gel mobility shift" assay. It also contains offers, electrophoresis reagents and an enzyme-labeled antibody to facilitate the detection of DNA-protein complexes. DIG Gel Shift Kit employs recombinant terminal transferase and digoxigenin (DIG)-11- dideoxyuridine triphosphate (ddUTP) makes the labeling reaction very flexible. It can be used to label the 3′ ends of any oligonucleotide (whether it has a 5′- overhanging end, a 3′-overhanging end, or blunt ends). Both single- and double-stranded DNA can be labeled. |
| General description: | We are committed to bringing you Greener Alternative Products, which adhere to one or more of The 12 Principles of Greener Chemistry. This product is designed as a safer chemical. The DIG System was established as a sensitive and cost-effective alternative to radioactivity for the labeling and detection of nucleic acids. There are many available publications that prove the versatility of the DIG System, so use of radio-labeling is no longer the only option for labeling of DNA for hybridization. |
| Other Notes: | For life science research only. Not for use in diagnostic procedures. |
| Packaging: | 1 kit containing 16 components. 1 kit for up to 20 Oligonucleotide 3-end labeling reactions with DIG-11-ddUTP, 200 binding reactions, chemiluminescent detection reaction for up to 20 blots, DNA binding protein and oligonucleotide for up to 20 control reactions |
| Physical form: | Chlorophenol red-β-D-galactopyranoside |
| Preparation Note: | The study of DNA-protein interactions has been greatly facilitated in recent years by the rapid and simple "gel retardation" or "gel mobility shift" assay. Because free DNA and DNA-protein complexes migrate differently during gel electrophoresis, they can be separated and detected on native (nondenaturing) polyacrylamide or agarose gels. Sample Amount: 3.85pmol or 100ng Type: Oligonucleotides with 5′-overhanging ends, 3′-overhanging ends, or blunt ends; single- or double-stranded DNA fragments (30 - 200bp) Note: Ideally, fragments to be labeled should be between 30 and 100bp. Time required Oligonucleotide annealing and labeling: 10minutes Formation of oligonucleotide-protein complexes: 25minutes Electrophoresis: 1 hour to overnight, depending on electrophoresis system Blotting: 1 - 2 hours Immunological detection: 2hours Exposure to X-ray film or imager: 15 - 40minutes |
| Symbol |    GHS07,GHS08,GHS09 |
| Signal word | Danger |
| Hazard statements | H302 + H332 - H350i - H360F - H411 |
| Precautionary statements | P201 - P261 - P273 - P280 - P308 + P313 - P391 |
| RIDADR | UN 3316 9 |
| WGK Germany | WGK 3 |
| Flash Point(F) | Not applicable |
| Flash Point(C) | Not applicable |
| Storage Temp. | −20°C (−15°C to −25°C) |
| UNSPSC | 12352200 |
| Components | Labeling Buffer 5x concentrated; CoCl<SUB>2</SUB> Solution 25 mM; DIG-ddUTP Solution, 1 mM Digoxigenin-11-ddUTP; Recombinant Terminal Transferase 400 U/μl; Binding Buffer 5x concentrated; Control Oligonucletide ds 39mer, unlabeled 0.1 μg/μl, 3.85 pmol/μl; DIG-labeled Control Oligonucleotide ds 39mer 0.4 ng/μl, 15.54 fmol/μl; Control Factor Oct2A 25-75 ng/μl; Poly [d(I-C)] 0.1 μg/μl; Poly [d(A-T)] 0.1 μg/μl; Poly L-lysine 0.1 μg/μl; Loading Buffer without bromophenol blue; Loading Buffer with bromophenol blue; Anti-Digoxigenin-AP 750 U/ml; CSPD 10 mg/ml; Blocking Reagent |