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Magnetic bead protein extraction, as a cutting-edge and excellent protein purification technology, is unique in the fields of biological research and biotechnology with its unparalleled efficiency and specificity. It utilizes the interaction between special ligands on the surface of magnetic beads and target proteins to achieve precise capture and efficient separation of proteins in complex biological matrices.
1. Principle of protein extraction using magnetic beads
Magnetic beads usually consist of a magnetic core made of magnetite and different materials covering its surface (such as agarose, polyethylene, silica, etc.). These surface materials can bind to specific affinity ligands (such as nickel-NTA ligands) and then interact with proteins with specific tags (such as His tag, Strep tag, etc.). Under the influence of a magnetic field, the magnetic beads bound to proteins can be quickly separated from the mixture to achieve protein purification.
2. Steps of protein extraction using magnetic beads
1. Magnetic bead pretreatment: Fully suspend the magnetic beads, place an appropriate amount of magnetic beads in a centrifuge tube, add binding/washing buffer and wash to remove impurities and non-specific binders on the surface of the magnetic beads.
2. Sample preparation: Select appropriate biological samples (such as cell lysates, tissue extracts, etc.) according to experimental needs, and perform appropriate processing to release the target protein.
3. Binding of magnetic beads to proteins: Add the pretreated magnetic beads to the sample, and incubate the ligands on the surface of the magnetic beads to bind to the target protein. In this step, conditions such as incubation time and temperature need to be optimized according to the specific conditions of the experiment.
4. Magnetic separation: Under the action of a magnetic field, the magnetic beads bound to the protein are adsorbed to the magnetic stand and separated from unbound impurities. At this point, the supernatant can be discarded and the magnetic bead-protein complex retained.
5. Washing: Use washing buffer to wash the magnetic bead-protein complex multiple times to remove non-specific binding impurities.
6. Elution: Use an appropriate elution buffer (such as low pH buffer, SDS buffer, etc.) to elute the target protein from the magnetic beads. At this time, the eluate is collected and the purified protein can be obtained.
3. Advantages of protein extraction using magnetic beads
1. Strong specificity: The interaction between the ligand on the surface of the magnetic beads and the target protein is highly specific, which can ensure the accuracy of the purification process.
2. Easy operation: The magnetic separation process is fast and simple, without complicated centrifugation or filtration steps, which can greatly improve the purification efficiency.
3. Small sample loss: Since the particle size of magnetic beads is small and easy to control, sample loss can be minimized during the purification process.
4. Good compatibility: The magnetic bead method is compatible with a variety of expression systems and sample types, and is suitable for protein purification needs of different scales and types.
4. Precautions
1. Low temperature operation should be maintained during the entire extraction process to prevent protein denaturation or degradation.
2. The amount of magnetic beads and incubation conditions need to be optimized according to the specific conditions of the experiment to obtain the best purification effect.
3. Washing and elution steps should be carried out fully to ensure the purity and recovery of the purified protein.
With the continuous advancement and cross-fusion of science and technology, the magnetic bead protein extraction technology continues to be iterated and optimized. The introduction of new materials, innovation in surface modification technology and the development of automated equipment have injected new vitality and possibilities into this technology.
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