Hytrophobic magnetic beads protocol

Protocol

PEI Magnetic Beads

Products

1 μm BcMag™ PEI Magnetic Beads
Cat. No.  DA101

Unit Size  5 ml
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1 μm BcMag™ PEI Magnetic Beads
Cat. No.  DA102

Unit Size  10 ml
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5 μm BcMag™ PEI Magnetic Beads
Cat. No.  DA103

Unit Size  5 ml
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5 μm BcMag™ PEI Magnetic Beads
Cat. No.  DA104

Unit Size  10 ml
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Cat. No.

DA101

DA102

DA103

DA104

Product Name

1 μm BcMag™ PEI Magnetic Beads

1 μm BcMag™ PEI Magnetic Beads

5 μm BcMag™ PEI Magnetic Beads

5 μm BcMag™ PEI Magnetic Beads

Unit Size

5 ml

10 ml

5 ml

10 ml

Specification

Composition

Magnetic beads grafted with branched polyethylenimine groups.

Magnetization

~45 EMU/g

Type of Magnetization

Superparamagnetic

Effective Density

2.0 g/ml

Stability

Most organic solvents

Strong Anion Exchange beads

1 μm beads: ~3 mg BSA/ ml of Beads

5 μm beads: ~2 mg BSA/ ml of Beads

Storage

Store at 4°C upon receipt.

Introduction

In the biological research field, isolating and purifying specific molecules is vital. Traditional chromatography methods can be time-consuming and require significant expertise. Magnetic beads, coupled with adsorbent technology, offer a faster and more efficient alternative. BcMag™ PEI Magnetic Beads are uniform magnetic resins with a high density of branched polyethyleneimine (PEI) groups. PEI’s unique structure allows it to trap protons, resulting in efficient fractionation of biological molecules.

PEI Structure

Strong anion exchange beads feature and benefits

Fast and simple – PEI magnetic beads-based format eliminates columns or filters or a laborious repeat of pipetting or centrifugation.

Convenient and expandable – PEI magnetic format enables high-throughput processing of multiple samples in parallel with many different automated liquid handling systems.

Robust – PEI magnetic beads do not crack or run dry.

Low bed volume – Working with small magnetic bead volumes allows for minimal buffer volumes, resulting in concentrated elution fractions.

Strong anion exchange beads Applications

Protein pre-fractionation in cell lysates

Optimizing purification conditions for new protein preparation protocols

Protein purification and concentration

Antibody purification from serum, ascites, or tissue culture supernatant

Preparation of samples before 1D or 2D PAGE

Phosphopeptide purification before MS analysis

PROTOCOL

Note: The following protocol is an example of fractionating a protein or peptide sample with BcMag™ PEI magnetic beads. Users are encouraged to choose alternative binding, washing, or elution buffers to get the best results and determine the optimal working conditions based on the protocol and suggestions described in the troubleshooting section. It is critical to match the amount of the beads to the amount of protein in the starting material in all protein purification experiments. It is not only for financial reasons but also because insufficient Strong Anion Exchange resin results in inadequate protein binding in the solution. Too many affinity binding sites will result in the binding of other proteins, making the purification less selective and requiring extra purification steps to achieve pure protein. We recommend performing a titration to optimize the beads used for each application. It is necessary to optimize volumes of elution to avoid unnecessary sample dilution.

Note: Select the appropriate buffer

Based on the protein’s pI, empirically calculate the appropriate buffer (pH and salt concentration) for purifying and eluting the protein of interest. In a buffered solution above the protein’s pI, the protein becomes negatively charged (deprotonated) and binds to the positively charged functional groups of an anion exchange resin. To choose the correct buffer for a selected pH, the following is a general rule for selecting a buffer pH:

Anion exchanger — 0.5–1.5 pH units higher than the protein’s pI of interest.

Cation exchanger — 0.5–1.5 pH units lower than the protein’s pI of interest.

Principle of Ion exchange chromatography

A. Equipment

Magnetic Rack (for manual operation)

Based on sample volume, the user can choose one of the following Magnetic Racks:

– BcMag™ Magnetic Rack-2 for holding two individual 1.5 ml centrifuge tubes (Cat. No. MS-01);

– BcMag™ Magnetic Rack-6 for holding six individual 1.5 ml centrifuge tubes (Cat. No. MS-02);

– BcMag™ Magnetic Rack-24 for holding twenty-four individual 1.5-2.0 ml centrifuge tubes (Cat. No. MS-03);

– BcMag™ Magnetic Rack-50 for holding one 50 ml centrifuge tube, one 15 ml centrifuge tube, and four individual 1.5 ml centrifuge tubes (Cat. No. MS-04);

– BcMag™ Magnetic Rack-96 for holding a 96 ELISA plate or PCR plate (Cat. No. MS-05).

For larger scale purification, Ceramic Magnets Block for large scale purification (6 in x 4 in x 1 in block ferrite magnet, Applied Magnets, Cat. No. CERAMIC-B8).

Corning 430825 cell culture flask for large-scale purification (Cole-Parmer, Cat. No. EW-01936-22)

Mini BlotBoy 3D Rocker, fixed speed, small 10″ x 7.5″ platform w/ flat mat (Benchmark Scientific, Inc. Cat. No. B3D1008) or compatible

B. Buffer

Binding/Wash Buffer: 25 mM Tris•HCl, pH 8.0. The pH of the Binding/Wash Buffer should be at least one pH unit away from the pI of the target protein or peptide. (Note: For best results, the salt should be ≤ 25mM in the sample).

Elution Buffer: 25 mM Tris-HCl pH 8.0. To elute the target protein or peptide from the magnetic beads, the user should optimize elution conditions for individual application by stepwise elution using solutions with increasing salt concentration, i. e., increase stepwise to a final salt concentration of 2.5 M).

General Protocol for using the Strong Anion Exchange Magnetic Beads –

a.

BcMag™ PEI magnetic beads preparation

1.

Vigorously shake the bottle until the magnetic resins become homogeneous and transfer an appropriate volume of the magnetic resins from the bottle to a new tube or flask.

Note:

Optimize the number of resins used for each application. Insufficient resins will lead to lower yields. Too many beads will cause higher background.

Do not allow the resins to sit for more than 3 minutes before dispensing. Resuspend the magnetic beads every 3 minutes.

2.

Place the tube on the magnetic rack for 1-3 minutes. Remove the supernatant while the tube remains on the rack. Add ten bead-bed volumes of dH2O and mix the beads by pipetting or vortex. Again, place the tube on the magnetic rack for 1-3 minutes and remove the supernatant while the tube remains on the rack.

3.

Repeat step (2) one more time.

4.

Equilibrate the beads by adding ten bead-bed volumes of Binding/Washing buffer and shake it to mix them. Incubate at room temperature with continuous rotation for 2 minutes. Place the tube on the magnetic rack for 1-3 minutes. Remove the supernatant while the tube remains on the rack. The resins are ready for purification.

b.

Purification

1.

Add the equilibrated beads (Step a (4)) to the sample and incubate on Mini BlotBoy 3D Rocker with continuous rotation for 5-10 minutes.

2.

Place the tube on the magnetic rack for 1-3 minutes. Remove the supernatant while the tube remains on the rack. Add ten bead-bed volumes of Binding/Washing buffer and shake it ten times to wash the beads. Again, place the tube on the magnetic rack for 1-3 minutes and remove the supernatant while the tube remains on the rack.

3.

Repeat step (2) six times.

Note:

This step is critical to get high pure protein. It may be necessary to wash the beads more than six times for some proteins to reduce the nonspecific binding.

Optimize the washing buffer (pH and salt concentration)

Elute protein with an appropriate volume of elution buffer by pipetting up and down 10-15 times or vortex mixer for 5 minutes.

Note:

Determine the optimum elution buffers (pH and salt concentration) and eluting the protein 2-3 times may be necessary.

4.

Elute protein with an appropriate volume of elution buffer by pipetting up and down 10-15 times or vortex mixer for 5 minutes.

Note:

Determine the optimum elution buffers (pH and salt concentration) and eluting the protein 2-3 times may be necessary.

5.

Collect and transfer the supernatant to a new tube.

C. Troubleshooting

Problem

Low yield

Probable Cause

The sample’s ionic strength is high.

Suggestion

  • The sample should be dialyzed, desalted, or diluted in a salt ≤25 mM purification buffer.

Problem

Low yield

Probable Cause

The sample contains interfering detergents.

Suggestion

  • Remove the detergents.

Problem

The protein failed to elute.

Probable Cause

Ionic interaction is too strong.

Suggestion

  • Increase the NaCl concentration.
  • Decrease pH of the Elution Buffer.
  • Using Weak Anion Exchange Magnetic Beads

Problem

Poor separation

Probable Cause

Carry-over between eluted fractions

Suggestion

  • Add more wash steps between each elution step

Problem

Poor separation

Probable Cause

Proteins or peptides with similar pI to the target protein

Suggestion

  • Optimize NaCl concentration and/or pH of the Elution Buffer

Problem

Probable Cause

Suggestions

Low yield

The sample’s ionic strength is high.

  • The sample should be dialyzed, desalted, or diluted in a salt ≤25 mM purification buffer.

The sample contains interfering detergents.

  • Remove the detergents.

The protein failed to elute.

Ionic interaction is too strong.

  • Increase the NaCl concentration.
  • Decrease pH of the Elution Buffer.
  • Using Weak Anion Exchange Magnetic Beads

Poor separation

Carry-over between eluted fractions

  • Add more wash steps between each elution step

Proteins or peptides with similar pI to the target protein

  • Optimize NaCl concentration and/or pH of the Elution Buffer

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