Determine the necessary mass, volume, or concentration for preparing a solution.
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.
UltraBio™ RNA Clean Magnetic Beads based on Solid Phase Reverse Immobilization (SPRI) technology, these beads utilize a novel nucleic acid purification medium coating combined with an optimized buffer system to purify RNA from diverse sources. They efficiently remove protein, salt ions, and other impurities, enhancing RNA purity—ideal for RNA purification in library construction workflows.
User-Supplied Reagents & Equipment
1. Reagents
80% Ethanol (prepared with Nuclease-free H₂O)
Nuclease-free H₂O
2. Equipment
Nucleic acid extraction instrument
Microcentrifuge tubes or deep-well plates
Vortex mixer
Pipettes
Thermostatic shaker
Manual Operation Protocol
1.Binding
Add 1.8× sample volume of RNA Purification Beads to the RNA solution.
Vortex-mix thoroughly and incubate at room temperature for 5 min.
Place the tube on a magnetic rack until the solution clears completely. Discard the supernatant.
2.Wash 1
Keep the tube on the magnetic rack.
Add 200 μL 80% ethanol (prepared with Nuclease-free H₂O).
Incubate for 1 min (do not resuspend beads).
Discard the supernatant (keep tube on the rack).
3.Wash 2
Repeat Step 2.
4.Ethanol Removal
Remove the tube from the magnetic rack.
Air-dry for 2–5 min at room temperature.
Critical: Avoid over-drying beads to maintain purification efficiency.
5.Elution
Add a user-defined volume of Nuclease-free H₂O.
Vortex-mix thoroughly and incubate at room temperature for 5 min.
6.RNA Recovery
Place the tube on the magnetic rack for 2–5 min until the solution clears.
Transfer the supernatant to a new Nuclease-free tube.
Automated Extraction: 16/32-Channel Instrument
1. Plate Setup (96-Well Plate)
| Sample Position | 1, 7 | 2, 8 | 3, 9 | 6, 12 |
| Reagent | Sample + 1.8× sample volume RNA Clean Magnetic Beads | 200 μL 80% ethanol | 200 μL 80% ethanol | Nuclease-free H₂O (volume adjusted as needed) |
2. Extraction Procedure
Load the prepared 96-well plate into the instrument.
Insert magnetic tip sets.
Select and execute the instrument-specific program.
3. Post-Run Processing
Transfer eluted RNA from columns 6 and 12 to clean Nuclease-free tubes.
Automated Extraction: 96-Channel Instrument
1. Plate Setup (96-Well Plate)
|
Note: Simultaneously processes 96 samples.
2. Extraction Procedure
Load the prepared plate into the instrument.
Insert magnetic tip sets.
Execute the instrument-specific program.
3. Post-Run Processing
Seal elution plates for immediate use or transfer RNA to Nuclease-free PCR plates.
Store at -20°C.
Precautions:
Bead Suspension Handling: This reagent is supplied as a bead suspension. DO NOT freeze or centrifuge. Vortex-mix thoroughly before use.
Nuclease-Free Practice: Use DNase/RNase-free consumables: Centrifuge tubes, Pipette tips, Microplates
Pre-Use Equilibration: Equilibrate beads to room temperature (RT) for ≥30 minutes prior to use.
Avoid Over-Drying: During ethanol removal (Step 4): Air-dry beads for ≤5 minutes. Over-drying significantly reduces RNA yield/recovery.
Comprehensive hazard, handling, storage, and regulatory compliance document.
Download SDS →Lot-specific quality data. Enter your lot number to retrieve the exact COA.
Look up COA →Full quality attributes and acceptance criteria for this grade.
View spec sheet →Find and download the COA for your product by matching the lot number on the packaging.
| Lot Number | Certificate Type | Fecha | Articulo |
|---|---|---|---|
| Certificate of Analysis | Jun 20, 2026 | R751581 | |
| Certificate of Analysis | Jun 20, 2026 | R751581 |