Determine the necessary mass, volume, or concentration for preparing a solution.
BioReagent, endotoxin tested, 50% v/v BioReagent,Endotoxin tested for sensitive chromatographic and analytical workflows requiring minimal baseline interference.
Store at 2-8°C,Do not freeze Ships Wet ice,Do not freeze Check lot-specific COA for exact specifications.
SDS, COA, datasheet, and spec sheet available for download. Lot-specific COA accessible via lot number lookup.
Cited in 0 peer-reviewed publications across chromatography, organic synthesis, and cross-coupling reactions.
This product is an affinity chromatography separation medium formed by coupling D-biotin to agarose base beads. The affinity between D-biotin and streptavidin is extremely high, with a dissociation constant on the order of 10⁻¹⁴ mol/L, making it one of the strongest non-covalent interactions in nature. The binding between this product and streptavidin is highly stable and specific, requiring harsh conditions (e.g., 2% SDS denaturing buffer) for dissociation. Therefore, it is suitable for the immobilization of avidin, streptavidin, and their conjugates, with applications in diagnostic assays and protein purification. Additionally, some streptavidin mutants exhibit significantly reduced affinity for D-biotin, enabling reversible binding. This product can also be used to purify such streptavidin mutants.
Aladdin Biotin Agarose Resin is stored in 20% ethanol, with a settled gel to storage solution ratio of 1:1. The product specification refers to the actual volume of the settled gel.
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Notes:
① Over 90% of the beads fall within this size range.
② DBC₁₀% measured under: 10% breakthrough, 6 min residence time.
③ Maximum tested flow rate at 10 cm column height.
Protocol
1. Column Packing
The following procedure describes column packing when connected to a chromatography system:
(1) Equilibrate all materials to the operating temperature. Degas liquids if possible.
(2) Resin Quantity Calculation:
Settled resin volume = Column volume × Compression factor (1.15 for this resin).
(3) Resin Preparation: Resuspend the resin slurry thoroughly. Measure the required volume, remove storage solution by filtration, and wash 3 times with ~3 resin volumes of purified water.
(4) Packing Slurry Preparation: Transfer resin to a suitable container and add packing solution to achieve a 50–75% (v/v) slurry. Mix well before use.
(5) Pre-packing Setup: Fill the bottom of the clean column with packing solution to remove air from the bottom frit and outlet. Retain a small amount of liquid, tighten the bottom end fitting, and ensure the column is vertical.
(6) Packing: Pour the well-mixed slurry into the column in one slow, continuous motion (use a packing reservoir if needed). After adding all resin, fill the reservoir with packing solution, attach the top lid, and connect the column to the system.
(7) Compression: Allow the resin to settle naturally (or use a low flow rate of 50–150 cm/h). Apply a high flow rate (600 cm/h; ensure pressure ≤0.3 MPa) until the interface is stable. Mark the stable height, stop the pump, and lower the adapter to the position corresponding to the compression factor (1.15). Tighten the adapter and equilibrate the column at a high flow rate.
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2. Column Efficiency Testing
After packing, assess column efficiency using HETP (Height Equivalent to a Theoretical Plate) and As (Asymmetry Factor) with acetone or NaCl as tracers:
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Calculate HETP, N, and As using:
HETP = L / N
N = 5.54 × (Vʀ / Wₕ)²
As = a / b
HETP should be <3× the average particle diameter (HETP/D₅₀ < 3), and As should be 0.8–1.5.
3. Recommended Buffers
Binding Buffer: 20 mM Tris-HCl, 150 mM NaCl, 1 mM EDTA, pH 8.0
Elution Buffer: Binding Buffer + 10–50 mM D-biotin
Regeneration Buffer: 0.1 M NaOH
4. Sample Purification
(1) Equilibration: Equilibrate with 5 CV Binding Buffer at 100–150 cm/h.
(2) Loading: Load sample at 20–100 cm/h. Pre-treat sample (dialysis, ultrafiltration, or dilution) to match Binding Buffer. Filter through 0.45 μm or centrifuge to remove particulates.
(3) Wash: Wash with 5–10 CV Binding Buffer at 100–150 cm/h until baseline is stable.
(4) Elution: Elute with 6–10 CV Elution Buffer at 100–150 cm/h.
(5) Regeneration: Wash with 3–5 CV water, regenerate with 3–5 CV 0.1 M NaOH, rinse to neutral pH, and store in 20% ethanol or re-equilibrate with Binding Buffer.
5. Storage
Store in 20% ethanol at 2–8°C. Do not freeze.
Comprehensive hazard, handling, storage, and regulatory compliance document.
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