| Field | Specification |
|---|---|
| Alternative Names | Magnetic particles, streptavidin functionalized |
| Concentration | |
| Form | liquid |
| Product Type | |
| Relative Density | |
| Shipping | |
| Storage |
Overview
SuperMag Streptavidin Beads are streptavidin conjugated magnetic beads. Streptavidin is covalently coupled to their surface and makes most of the biotin binding sites sterically available for binding of biotinylated nucleic acids, antibodies, or other biotinylated ligands and targets. With large surface area, excellent colloidal stability and unique surface coating, SuperMag Streptavidin Beads exhibit high binding capacity, low non-specific binding and fast magnetic separation.
Key Features
- High binding capacity
- Significantly low non-specific binding
- Fast magnetic separation
Applications
- Cell separation
- Immunoprecipitation
- Immunoassay
Physical & Chemical Properties
- Surface Functional Group: Streptavidin
- pH: 6.0 - 8.0 at 25 °C (77 °F)
- Water Solubility: Completely miscible
- Magnetic Content: ~80%
- Chemical Stability: Stable under recommended storage conditions.
- Appearance / Color: brown/black
SuperMag Streptavidin Beads are hydrophilic superparamagnetic beads (50 nm, 100 nm, 150 nm, 200 nm) with streptavidin covalently coupled to their surface. Their smaller nano-scale size provides a larger collective surface area per mg compared to micron-sized beads, supporting high biotin-capture capacity in liquid-phase assays.
They are used for nucleic acid capture (via biotinylated probes), ELISA, immunoprecipitation, cell separation, and magnetic bead-based diagnostic assay development. The nanoscale particle size reduces steric hindrance for larger target molecules.
Smaller sizes (50 nm, 100 nm) remain in suspension longer, maximizing contact time with targets — useful for low-abundance capture. Larger sizes (150 nm, 200 nm) have a higher iron content per particle and settle faster with a magnet, reducing separation time.
Store at 2–8°C. Do not freeze — freezing causes irreversible aggregation. Vortex or bath-sonicate before use to ensure complete resuspension. Check the specification sheet for recommended working concentrations.
SuperMag beads are brown/black in suspension due to their iron oxide content. They are not suitable for flow cytometry applications that rely on optical scatter or fluorescence from the bead itself. For fluorescent detection, consider Quantum Dots or Fluorescent Nanoparticle conjugation approaches.
The following customization and add-on services are available for this product through the supplier. For inquiries and pricing, contact support@biohippo.com.
Customization Options
- Custom Particle Sizes: Magnetic beads in sizes beyond the standard catalog range, with narrow size distribution from nanometers to micrometers, can be manufactured for specific assay geometries and separation requirements.
- Custom Surface Functionalization: Customized surface coatings and functional group densities are available to optimize binding capacity, non-specific binding profiles, and colloidal stability for specific applications.
- Custom Conjugation Service: Pre-conjugated magnetic bead–antibody, bead–protein, or bead–streptavidin conjugates prepared using your supplied biomolecule are available. The supplier specializes in bioconjugation chemistry across magnetic beads, iron oxide nanoparticles, quantum dots, and latex beads.
- Assay Development Services: Support for magnetic bead-based chemiluminescent assay, lateral flow immunoassay, and custom immunoassay platform development is available.
- Bulk & OEM Manufacturing: OEM magnetic beads for chemiluminescent assay, lateral flow immunoassay, CTC (circulating tumor cell) isolation for liquid biopsy, and T-cell isolation and activation for immunotherapy are available at production scale.
To inquire about customization options, request a quote, or discuss OEM manufacturing, contact support@biohippo.com.
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- Guo L et al. (2026). Thread-Designed Vascular Scaffold with Magneto-Optical Probes Capture and Elimination of Circulating Tumor Cells In Vivo. Adv Mater. DOI: 10.1002/adma.202516675 PMID: 41546398
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- Zeng T et al. (2025). Integrated Biomimetic Platform for Enhancing the Efficient Capture and Visual Identification of Circulating Tumor Cells. Anal Chem. DOI: 10.1021/acs.analchem.5c06259 PMID: 41384307
- Liu X et al. (2026). Interacting proteins of AMPK studied using TurboID proximity labeling technology. Exp Ther Med. DOI: 10.3892/etm.2026.13144 PMID: 42022757
- Faresjö M (2026). A Useful Guide for Analysis of Biomarkers in Cancer by Fluorochrome (Luminex) Technique. Methods Mol Biol. DOI: 10.1007/978-1-0716-4901-5_1 PMID: 41478962
- Elejaga-Jimeno A et al. (2024). Tuning the properties of peptide imprinted nanoparticles for protein immunoprecipitation using magnetic streptavidin beads. Mikrochim Acta. DOI: 10.1007/s00604-024-06782-7 PMID: 39470840
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