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Kit Contents
Dynabeads® Oligo (dT)25 * 1 × 2 ml
Binding Buffer 4 ml
Washing Buffer B 4ml
Elution Buffer 4 ml
*Approximately 5 mg/ml, supplied in PBS pH 7.4, containing 0.02% NaN3 as a preservative
Product Description
This product has been designed for rapid isolation of highly purified and intact mRNA from total RNA.
Principle of Isolation
The isolation protocol relies on base pairing between the poly A residues at the 3’ end of most mRNA and the oligo (dT)25 residues covalently coupled to the surface of the Dynabeads® . Other RNA species lacking a poly A tail will not hybridize to the beads and are readily washed away. 1 mg of beads (200 µl) will isolate up to µg of mRNA, depending on the sample. A typical mammalian cell contains about 10-30 pg of total RNA, from which 1-5% is mRNA.
Physical Characteristics of Dynabeads® Oligo (dT)25
Diameter: 2.8 µm ± 0.2 µm
(C.V. max 5%)
Surface area: 3–7 m² /g
Density: approx. 1.6 g/cm³
Magnetic mass susceptibility: 20 ± 25 × 10–6 m³/kg
Buffers
Binding Buffer 4 ml
20 mM Tris-HCl (pH 7.5)
1.0 M LiCl
2 mM EDTA
Washing Buffer B 4 ml
10 mM Tris-HCl (pH 7.5)
0.15 M LiCl
1 mM EDTA
10 mM Tris-HCl (pH 7.5) 4 ml
Additional Material Required
Technical Advice
Purification of mRNA from total RNA
The protocol below describes mRNA isolation from 75 μg of total RNA as starting material.
Preparation of RNA
Preparation of Dynabeads®
Isolation of mRNA
Regeneration and Reuse of Dynabeads® Oligo (dT)25
The oligo (dT)25 sequences are covalently attached to the bead surface. Whilst this enables a single step hybridization, the covalent nature of the binding also allows regeneration of the Dynabeads® Oligo (dT)25. The beads may be reused a total of four times without loss of yield. The reusable properties of these Dynabeads® provides a cost effective choice for the user. When mRNA is to be isolated from the same crude extract, the Dynabeads® Oligo (dT)25 can be reused without regeneration. By reusing the Dynabeads® on the same sample (without regeneration), large amounts of mRNA can be isolated. Simply follow the mRNA isolation procedure. After elution of the mRNA, wash the Dynabeads® once in Binding Buffer before adding the sample and a new capture of mRNA is performed. This can be repeated several times until no mRNA is left in the sample.
Note: The buffers in this kit is not sufficient for re-use of the Dynabeads® , and they will have to be made. The Binding Buffer in this kit is supplied as a 2 × concentrate. This is to obtain optimal hybridization condition when mixing 1:1 with the sample. When used to wash the Dynabeads® for reuse, adjust the Binding Buffer to 1 × concentration by adding an equal volume of DEPC-treated water.
Note: Buffers such as Tris cannot be DEPC treated as Tris inactivates DEPC. Solutions should be DEPC treated and autoclaved before adding Tris. Subsequently after adding Tris, autoclave the solution again. DEPC is a suspected carcinogen – handle with care. Wear gloves.
Regeneration Protocol
Use this protocol if you need to avoid cross contamination of mRNA between samples.
Buffers for regeneration(not supplied):
Reconditioning Solution:
0.1 M NaOH
Storage Buffer Oligo (dT)25:
250 mM Tris-HCl (pH 7.5)
20 mM EDTA
0.1% Tween20
0.02% Sodium azide (NaN3)
Note: Do not mix regenerated Dynabeads® Oligo (dT)25 with original stock suspension.
Invitrogen Dynal® AS complies with the Quality System Standards ISO 9001:2000 and ISO 13485:2003.
Storage/Stability
This product is stable until the expiry date stated on the label, when stored unopened at 2–8°C. Store opened vials at 2–8°C and avoid bacterial contamination. Do not store the Dynabeads® Oligo (dT)25 in distilled water.
Technical Support
Certificate of Analysis/Compliance is available upon request. The latest revision of the package insert/instruction for use is available on www.lifetechnologies.com.
Warnings and Limitations
The Dynabeads® mRNA Purification Kit is for research use only. The product is not for use in human diagnostic or therapeutic procedures. The Dynabeads® Oligo (dT)25 contains 0.02% sodium azide (NaN3) as a preservative. Sodium azide may react with lead and copper plumbing to form highly explosive metal azides. When disposing through plumbing drains, flush with large volumes of water to prevent azide build-up. Preservatives such as sodium azide are toxic if ingested. Avoid pipetting by mouth. Standard methods for preventing contamination by RNases during the preparation of mRNA must be taken. Take precautions to prevent RNase contamination of opened vials. Material Safety Data Sheet is available from www.lifetechnologies.com.