Dynabeads™ Oligo(dT)₂₅

Citations & References (5)

Invitrogen™

Dynabeads™ Oligo(dT)₂₅

Name: Dynabeads™ Oligo(dT) 25
SKU: 61005
Price: 6671.00 HKD

Dynabeads™ Oligo(dT)25 mRNA isolation beads specifically target and capture mRNA molecules from virtually any crude sample and eliminate the needRead more

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Catalog Number	Quantity
61005	5 mL
61002	2 mL

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Catalog number 61005

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6,671.00

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Ends: 31-Dec-2025

8,517.00

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Quantity:

5 mL

Price (HKD)

6,671.00

온라인 행사

Ends: 31-Dec-2025

8,517.00

Save 1,846.00 (22%)

Each

Add to cart

Dynabeads™ Oligo(dT)₂₅ mRNA isolation beads specifically target and capture mRNA molecules from virtually any crude sample and eliminate the need to purify total RNA when the desired information-bearing nucleic acid is mRNA. Since mRNA comprises only about 1–5% ot total cellular RNA, the isolation of total RNA is not the most efficient way to isolate mRNA. Other technologies designed to purify total RNA yield ∼80% ribosomal RNA and force mRNA to compete with ribosomal RNA, transfer RNA, micro RNA, small nucleolar RNA, and small cytoplasmic RNA for membrane binding. Advantages of Dynabeads™ Oligo(dT)₂₅ beads:

• Fast and gentle procedure yields pure intact mRNA
• Extremely pure mRNA isolation, best choice upstream of cDNA synthesis
• Exquisitely sensitive mRNA isolation enables cDNA synthesis and cDNA library construction from ultra-small starting samples (enables cDNA library construction from a single cell)

How the beads work
The oligo(dT)₂₅-coated Dynabeads™ specifically target and capture the mRNA transcriptome from an extremely wide variety of crude starting samples. Ribosomal RNA, DNA, proteins, and small RNA molecules (such as transfer RNA, micro RNA, and small nucleolar RNA) do not bind to the beads and are discarded. Only polyadenylated RNA species (mRNA) are captured. Isolated mRNA is pure, eliminating the need for ribosomal RNA subtraction or a post-extraction DNase treatment. This column-free system ensures the highest transcriptome recovery:

• Physical mRNA capture on mobile magnetic beads
• Rapid and gentle magnetic handling procedures
• No mRNA lost during high g-force spins
• No mRNA trapped in column membranes during elution

Applications
mRNA is suitable for all downstream molecular applications, including gene cloning, cDNA synthesis, cDNA library construction, RT-PCR, quantitative RT-PCR, RPA (Ribonuclease Protection Assay), subtractive hybridization, primer extension, SAGE, RACE, and others. The Dynabeads™ Oligo(dT)₂₅ mRNA isolation beads are the ideal mRNA purification method prior to cDNA library construction. Use of these beads ensures the highest recovery and enrichment of the transcriptome. These beads capture more of the transcriptome than is possible with methods that integrate a total RNA isolation step upstream of mRNA isolation.

Verastile elution options
Elution can be performed in any volume down to 5 μL. mRNA elution is optional because enzymatic reactions in downstream procedures are not inhibited by presence of Dynabeads™. Additionally, one can perform cDNA synthesis directly on the beads to create a reusable solid-phase cDNA library.

For Research Use Only. Not for use in diagnostic procedures.

Specifications

Elution Volume10–20 μL

Final Product TypemRNA

For Use With (Application)qPCR

High-throughput CompatibilityHigh-throughput Compatible

Ligand TypeOligo-dT

Purification Time15 min.

Quantity5 mL

Shipping ConditionRoom Temperature

Starting Material AmountCells: ≤10⁶
Plant: ≤100 mg
Tissue: ≤50 mg
Total RNA: ≤75 μg

Yield10 μg mRNA per 1 mL of beads (Binding capacity)

Isolation TechnologyMagnetic Bead

Unit SizeEach

Contents & Storage

5 mL Dynabeads; 4°C

Frequently asked questions (FAQs)

I am getting DNA contamination after mRNA isolation using Dynabeads magnetic beads. Why is this?

There are several reasons why DNA contamination may occur:

- Incomplete DNA shearing.
- Incomplete removal of sample lysate after the hybridization step.
- Insufficient washing and/or removal of wash buffers.
- The ratio of sample to beads was too high.

I am getting rRNA contamination after mRNA isolation using Dynabeads magnetic beads. What should I do?

Ribosomal RNA is effectively eliminated by reextracting the mRNA from the eluate. Reuse the same Dynabeads Oligo(dT)25 beads that were used for the original isolation. Wash the beads twice in Washing Buffer B. Dilute the eluted mRNA with 4 times its volume of Lysis/Binding Buffer, then add the beads. Incubate with mixing at room temperature for 3-5 minutes, then continue with the Direct mRNA Isolation Protocol.

How long can I leave the isolated mRNA on Dynabeads Oligo(dT)25 magnetic beads?

We recommend immediate use of Dynabeads magnetic beads-mRNA complex or eluted mRNA for cDNA synthesis, in RT-PCR, or for other downstream applications. If storage is needed, we recommend you elute the mRNA from the beads using 10 mM Tris-HCl buffer (pH 7.5) and freeze it(-80°C). It is very important that all equipment and samples are RNase free.

My Dynabeads magnetic beads are not pelleting well with the magnet. Do you have any suggestions for me?

Please review the following possibilities for why your Dynabeads magnetic beads are not pelleting:

- The solution is too viscous.
- The beads have formed aggregates because of protein-protein interaction.

Try these suggestions: - Increase separation time (leave tub on magnet for 2-5 minutes)
- Add DNase I to the lysate (~0.01 mg/mL)
- Increase the Tween 20 concentration to ~0.05% of the binding and/or washing buffer.
- Add up to 20 mM beta-merecaptoethanol to the binding and/or wash buffers.

Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.

Can I use Dynabeads Oligo(dT)25 magnetic beads in real-time PCR?

Dynabeads magnetic beads are compatible with TaqMan real-time PCR chemistry and non-capillary real-time PRC instruments. However, Dynabeads magnetic beads exhibit a low level of autofluorescence that can increase the intensity of the fluorescent signal to some degree. This can be compensated for by using a Dynabeads magnetic beads and water background in the instrument. Then background signal intensity can be subtracted from the sample signal intensity in all subsequent real-time PCR experiments containing Dynabeads magnetic beads. Alternatively, when using the standard curve method of analysis, an appropriate amount of Dynabeads magnetic beads can be added to each sample used to construct the standard curve.

View all Dynabeads™ Oligo(dT)₂₅, 5 mL FAQs

Citations & References (5)

Citations & References

Abstract

Purification of mRNA directly from crude plant tissues in 15 minutes using magnetic oligo dT microspheres.

Authors:Jakobsen KS, Breivold E, Hornes E

Journal:Nucleic Acids Res

PubMed ID:2362831

Induction of nitric oxide synthase mRNA in coronary resistance arteries isolated from exercise-trained pigs.

Authors:Woodman CR, Muller JM, Laughlin MH, Price EM

Journal:Am J Physiol

PubMed ID:9435589

The purpose of this study was to develop a method by which endothelial cell nitric oxide synthase (ecNOS) mRNA expression could be measured in single coronary resistance arteries and to test the hypothesis that ecNOS gene expression is upregulated by exercise training. Yucatan miniature swine were randomly assigned to exercise-trained ... More

Disruption of imprinted gene methylation and expression in cloned preimplantation stage mouse embryos.

Authors:Mann MR, Chung YG, Nolen LD, Verona RI, Latham KE, Bartolomei MS

Journal:Biol Reprod

PubMed ID:12748125

Cloning by somatic cell nuclear transfer requires that epigenetic information possessed by the donor nucleus be reprogrammed to an embryonic state. Little is known, however, about this remodeling process, including when it occurs, its efficiency, and how well epigenetic markings characteristic of normal development are maintained. Examining the fate of ... More

Selective loss of imprinting in the placenta following preimplantation development in culture.

Authors:Mann MR, Lee SS, Doherty AS, Verona RI, Nolen LD, Schultz RM, Bartolomei MS

Journal:Development

PubMed ID:15240554

Preimplantation development is a period of dynamic epigenetic change that begins with remodeling of egg and sperm genomes, and ends with implantation. During this time, parental-specific imprinting marks are maintained to direct appropriate imprinted gene expression. We previously demonstrated that H19 imprinting could be lost during preimplantation development under certain ... More

In vitro characterization of somatostatin receptors in the human thymus and effects of somatostatin and octreotide on cultured thymic epithelial cells.

Authors:Ferone D, van Hagen PM, van Koetsveld PM, Zuijderwijk J, Mooy DM, Lichtenauer-Kaligis EG, Colao A, Bogers AJ, Lombardi G, Lamberts SW, Hofland LJ

Journal:Endocrinology

PubMed ID:9886848

Somatostatin (SS) and its analogs exert inhibitory effects on secretive and proliferative processes of various cells via high affinity SS receptors (SS-R). SS analogs bind with different affinity to the five cloned SS-R subtypes. Octreotide, an octapeptide SS analog, binds with high affinity to the SS-R subtype 2 (sst2). SS-R ... More