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View additional product information for Dynabeads™ Co-Immunoprecipitation Kit - FAQs (14321D)
33 product FAQs found
Please review the following possibilities for why your Dynabeads magnetic beads are not pelleting:
- The solution is too viscous.
- The beads have formed aggregates because of protein-protein interaction.
Try these suggestions:
- Increase separation time (leave tub on magnet for 2-5 minutes)
- Add DNase I to the lysate (~0.01 mg/mL)
- Increase the Tween 20 concentration to ~0.05% of the binding and/or washing buffer.
- Add up to 20 mM beta-merecaptoethanol to the binding and/or wash buffers.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
For biotin-labeled DNA that is less than 1 kb, we recommend you use Dynabeads M270 Streptavidin (Cat. No. 65305) and MyOne C1 magnetic beads (Cat. No. 65001). We recommend our Dynabeads KilobaseBINDER Kit (Cat. No. 60101), which is designed to immobilize long (>1 kb) double-stranded DNA molecules. The KilobaseBINDER reagent consists of M-280 Streptavidin-coupled Dynabeads magnetic beads along with a patented immobilization activator in the binding solution to bind to long, biotinylated DNA molecules for isolation. Please see the following link (https://www.thermofisher.com/us/en/home/life-science/dna-rna-purification-analysis/napamisc/capture-of-biotinylated-targets/immobilisation-of-long-biotinylated-dna-fragments.html) for more information in regards to long biotinylated DNA fragment isolation.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
Yes, Dynabeads magnetic beads can be used to isolate single-stranded DNA. Streptavidin Dynabeads magnetic beads can be used to target biotinylated DNA fragments, followed by denaturation of the double-stranded DNA and removal of the non-biotinylated strand. The streptavidin-coupled Dynabeads magnetic beads will not inhibit any enzymatic activity. This enables further handling and manipulation of the bead-bound DNA directly on the solid phase. Please see the following link (https://www.thermofisher.com/us/en/home/life-science/dna-rna-purification-analysis/napamisc/capture-of-biotinylated-targets/preparing-single-stranded-dna-templates.html) for more information in regards to single-stranded DNA capture.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
Magnetic susceptibility is a measure of how quickly the beads will migrate to the magnet. This will depend on the iron content and the character of the iron oxide. The magnetic susceptibility given for the Dynabeads magnetic beads is the mass susceptibility, given either as cgs units/g or m^3/kg (the latter being an SI unit). For ferri- and ferromagnetic substances, the magnetic mass susceptibility is dependent upon the magnetic field strength (H), as the magnetization of such substances is not a linear function of H but approaches a saturation value with increasing field. For that reason, the magnetic mass susceptibility of the Dynabeads magnetic beads is determined by a standardized procedure under fixed conditions. The magnetic mass susceptibility given in our catalog is thus the SI unit. Conversion from Gaussian (cgs, emu) units into SI units for magnetic mass susceptibility is achieved by multiplying the Gaussian factor (emu/g or cgs/g) by 4 pi x 10^-3. The resulting unit is also called the rationalized magnetic mass susceptibility, which should be distinguished from the (SI) dimensionless magnetic susceptibility unit. In general, magnetic mass susceptibility is a measure of the force (Fz) influencing an object positioned in a nonhomogenous magnetic field. The magnetic mass susceptibility of the Dynabeads magnetic beads is measured by weighing a sample, and then subjecting the sample to a magnetic field of known strength. The weight (F1) is then measured, and compared to the weight of the sample when the magnetic field is turned off (F0). The susceptibility is then calculated as K x 10^-3 = [(F1-F0) x m x 0.335 x 10^6], where K is the mass susceptibility of the sample of mass m. The susceptibility is then converted to SI units.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
There are different methods to check binding of ligands to the beads, including optical density (OD) measurement, fluorescent labeling, and radioactive labeling.
For OD measurement, you would measure the OD of the ligand before immobilization to the beads and compare it with the ligand concentration that is left in the supernatant after coating. This gives a crude measurement of how much protein has bound to the beads.
Protocol:
1.Set spectrophotometer to the right wavelength. As a blank, use the Coupling Buffer.
2.Measure the absorbance of the Pre-Coupling Solution. A further dilution may be necessary to read the absorbance, depending upon the amount of ligand added.
3.Measure the absorbance of the Post-Coupling Solution. A dilution may be necessary to read the absorbance.
4.Calculate the coupling efficiency, expressed as the % protein uptake, as follows. [(Pre-Coupling Solution x D) - (Post-Coupling Solution x D)] x 100/(Pre-Coupling Solution x D) where D = dilution factor.
For fluorescent labeling, we suggest negatively quantifying the amount of ligand bound by measuring ligand remaining in the coupling supernatant (compared to the original sample), rather than directly measuring the ligands on the beads. Add labeled ligand to the beads, and measure how much ligand is left in the supernatant (not bound to the beads). By comparing this with the total amount added in the first place, you can then calculate how much of the ligand that has been bound to the beads. Keep in mind that the Dynabeads magnetic beads are also autofluorescent, which is why direct measuring of fluorescence of the bead-bound ligands is not recommended, but rather this indirect approach. The label could be, for example, FITC/PE. Some researchers perform a direct approach with success (using a flow cytometer).
Radioactive labeling is the most sensitive method of the three, but it is also the most difficult one. It involves radioactively labeling a portion of the ligand. We use radiolabeled I-125 in tracer amounts and mix it with "cold" ligands in a known ratio before coupling. The absolute quantities for the ligand on the beads should be obtained by measuring the beads in a scintillation (gamma) counter and comparing the cpm with a standard.
Protocol:
1.Take out an appropriate amount of beads and wash the beads in 1 mL of binding buffer.
2.Pipette out desired amount of human IgG in a separate tube.
3.Mix the human IgG with I-125-labeled human IgG (30,000 - 100,000 cpm).
4.Dilute the mixture of human IgG and I-125-labeled human IgG to 100 mL in binding buffer.
5.Incubate for 30 minutes at room temperature and measure the cpm in a scintillation counter.
6.Wash the beads (with coating) four times, and measure cpm again.
The % binding is calculated by using the equation : (cpm after washing/cpm before washing)x100%.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
Dynabeads magnetic beads come in three sizes: 4.5 µm (M-450), 2.8 µm (M-270/M-280), and 1 µm (MyOne beads). The largest of the Dynabeads magnetic beads is ideal for big targets like cells. The 2.8 µm beads are recommended for proteomics and molecular applications. The smallest of the beads, 1 µm, are ideal for automated handling.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
In general, short sonication is a good way to reduce aggregation of the beads and ensure optimal homogenous conditions at the time of ligand addition when coating the beads. When target is bound to the beads, more care is needed, as the binding might break. The streptavidin beads themselves should tolerate sonication. We have not tested sonication for long periods, but 5 minutes is fine. We do not have information about the streptavidin-biotin interaction being broken by such treatment.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
If desired, the uncoated epoxy or tosylactivated beads can be sterilized by washing with 70% ethanol. Coated beads cannot be sterilized.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center.
Dynabeads magnetic beads are uniform, non-porous, superparamagnetic, monodispersed and highly cross-linked polystyrene microspheres consisting of an even dispersion of magnetic material throughout the bead. The magnetic material within the Dynabeads magnetic beads consists of a mixture of maghemite (gamma-Fe2O3) and magnetite (Fe3O4). The iron content (Fe) of the beads is 12% by weight in Dynabeads magnetic beads M-280 and 20% by weight in Dynabeads magnetic beads M-450. The Dynabeads magnetic beads are coated with a thin polystyrene shell which encases the magnetic material, and prevents any leakage from the beads or trapping of ligands in the bead interior. The shell also protects the target from exposure to iron while providing a defined surface area for the adsorption or coupling of various molecules.
Uniformity of bead size and shape provides consistent physical and chemical properties. These uniform physical characteristics lead to high-quality, reproducible results.
The Dynabeads magnetic beads are available in three different sizes: 4.5 µm (M-450 beads), 2.8 µm (M-270/M-280 beads) and 1 µm (MyOne beads).
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
The lysis buffer in the kit will not lyse nuclei.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
The amount of beads required would depend on the downstream analysis you will be performing. As stated in the package insert, using 1.5 mg coated beads with 0.05-1.0 g of total cell extract is recommended if you are Western blotting. For mass spectrometry, more beads are required (typically 7.5 mg beads for 1.0-15.0 g of total cell extract). In cases where the target is purified, you would probably need less. It might also depend on whether total depletion of the main protein is required.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
The Dynabeads Co-Immunoprecipitation Kit (Cat. No. 14321D) was developed to mimic the intracellular conditions while providing customized stringency for different protein complexes in a cell solution. It offers the opportunity to optimize and fine tune weak and transient interactions between short amino acid sequences in different proteins.
The beads and buffers provided in the Dynabeads Co-Immunoprecipitation Kit will enable you to:
(1) Covalently immobilize antibodies of your choice onto the surface of Dynabeads M270 epoxy magnetic beads
(2) Use the antibody coated beads for co-immunoprecipitation
Benefits:
-Freedom to use any antibody
-No release of antibody in the eluate
-Co-IP buffer system
-Easy optimization
-Qualitative reproducibility
The most optimal antibody concentration for coupling is below 10 µg/mg Dynabeads magnetic beads and provides efficient coupling and functionality of the coupled antibody. Presence of 0.1% NaN3 and/or 0.1% BSA does not reduce coupling efficiency and functionality of the antibodies.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
There are two main ways of coupling antibodies to the beads (with several different options within the two groups): Covalent coupling and Noncovalent coupling.
For covalent coupling, there are several choices including:
Dynabeads M-280 Tosylactivated magnetic beads (Cat. No. 14203)
Dynabeads M-270 Epoxy magnetic beads (Cat. No. 14301)
Dynabeads Antibody Coupling Kit (Cat. No. 14311D, Dynabeads M-270 Epoxy and buffers for covalent coupling)
For co-immunoprecipitation, Dynabeads Co-Immunoprecipitation Kit (Cat. No. 143-21D, Dynabeads M-270 Epoxy magnetic beads, buffers for covalent coupling, and buffers optimized for co-immunoprecipitation; see Alber F et al. (2007) Determining the architectures of macromolecular assemblies. Nature 450, 683-694).
Dynabeads magnetic beads can also be used for immunoprecipitation, which relies on noncovalent binding of antibodies. The most common products used for noncovalent binding of antibodies to Dynabeads magnetic beads are:
Dynabeads Protein A magnetic beads (Cat. No. 10001D)
Dynabeads Protein G magnetic beads (Cat. No. 10003D)
Immunoprecipitation Kit - Dynabeads Protein A magnetic beads (Cat. No. 10006, containing Dynabeads magnetic beads and optimized buffers for immunoprecipitation)
Immunoprecipitation Kit - Dynabeads Protein G magnetic beads (Cat. No. 10007, Dynabeads magnetic beads and optimized buffers for immunoprecipitation)
Dynabeads magnetic beads coated with secondary antibodies. (Dynabeads Pan Mouse IgG magnetic beads (Cat. No. 11041) are 4.5 µm beads developed for cell separation that have increased capacity per volume when using Dynabeads M-280 Sheep Anti-Mouse IgG magnetic beads.
Thus, there are several products that can be considered for performing immunoprecipitation depending on preferences. If the target is the same as heavy or light chain antibody, we recommend covalently binding the antibody to the bead surface. This can be done either by cross-linking the antibody to beads coated with Protein A or G or with secondary antibody or by using one of the surface-activated Dynabeads products. As your primary antibody can be used in combination with Dynabeads Protein G magnetic beads (Cat. No. 100-03D) or Immunoprecipitation Kit - Dynabeads Protein G magnetic beads (Cat. No. 100-07D, contains immunoprecipitation buffers as well) or Dynabeads Sheep Anti-Mouse IgG magnetic beads, using a cross-linker will ensure covalent binding of your primary antibody. Depending on the antibody, the functionality of the antibody can be affected. The other option would be the surface-activated Dynabeads products. This is an easy but more time-consuming approach, since the coupling takes an overnight incubation, but it ensures functional antibodies that are not eluted off during elution. For this approach, we recommend the Dynabeads Antibody Coupling Kit (Cat. No. 14311D, contains both surface-activated beads and optimized buffers for covalent coupling).
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Storage should be at 2-8 degrees C. Freezing Dynabeads magnetic beads is not recommended. Provided the Dynabeads magnetic beads are stored correctly, quality is guaranteed until the expiration date stated on the label.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Dynabeads magnetic beads coated with antibody/ligand may be stored at 2-8 degrees C without loss of antigen binding capacity. For long-term storage, a final concentration of 0.02% NaN3 may be added to the antibody-coupled beads in a physiological buffer. Please note that not all coupled antibodies retain their function in long term storage. Verify your coupled antibody stability by testing in small scale. After storage, coated Dynabeads magnetic beads should be washed once in PBS/BSA for 5 min before use.
Find additional tips, troubleshooting help, and resources within our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Standard elution methods are used to dissociate the isolated protein from Dynabeads magnetic beads. The most suitable elution method depends on the characteristics of the isolated protein and the desired downstream application of the eluted protein. In many cases, Dynabeads magnetic beads can be recovered for reuse after elution. Some standard elution methods are listed below.
-pH change: elution can be achieved by reducing pH (for example, by using 0.1 M citrate (pH 2-3) as the elution buffer). Dynabeads magnetic beads are stable between pH 4-13. If the Dynabeads magnetic beads are exposed for a prolonged period of time to pH below 4, the beads may be adversely affected.
-Change of ionic strength: high-salt concentration buffers (e.g., NaI, KI, MgCl, KCl) can be used to elute isolated proteins. Optimization is required, by step-wise elution starting at 1 M and increasing to 3 M.
-Affinity elution: with this method, the eluting agent competes for the binding of the protein or the binding of the ligand e.g., elution of glycoproteins from a lectin coupled to Dynabeads magnetic beads may be achieved by the addition of the free sugar.
-Denaturing eluents: as a last resort, denaturing eluents such as chaotropic salts may be used to alter the structure of the protein. The proteins on the bead surface and the eluted proteins will be denatured.
-Polarity reducing agents : substances that reduce the polarity of the buffer often disrupt the hydrophobic interactions between antibody and protein. Dioxane or ethylene glycol may be used to reduce the polarity of the eluent.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
This kit is not recommended for use with antibodies that have been stabilized in glycerol. The antibody function may be severely affected. Consider dialyzing the IgG to remove the glycerol and then repeat the coupling process.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
The binding sites of your antibody have likely been altered by the crosslinking. When this occurs, your antibody will show reduced affinity or no affinity to its target antigen. Another consequence of crosslinking can also be increased affinity for unintended (nonspecific) targets. This is always a high risk with crosslinking, and it is a problem easily avoided by choosing another path to covalent antibody coupling. You can try using the Dynabeads Antibody Coupling Kit. This kit is a far superior solution for covalent antibody coupling to Dynabeads magnetic beads (compared to crosslinking with Dynabeads Protein A or G magnetic beads). The Dynabeads Antibody Coupling Kit is compatible with almost any antibody. It is designed specifically for covalent antibody coupling to Dynabeads magnetic beads. Unlike crosslinking, the Dynabeads Antibody Coupling Kit will not alter antibody specificity or affinity.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
The M stands for magnetic. M-280 refers to hydrophobic 2.8 micron beads, while M-270 refers to hydrophilic 2.8 micron beads. MyOne refers to 1 micron beads.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Answering this question is not straightforward. It will depend on the detection method. When using HRP (horseradish peroxidase)-based detection system or radioactivity in combination with a good antibody, very little target is required. More target is required when using an AP (alkaline phosphatase)-based detection system. When a sensitive detection system is used, detection will most likely be in the nanogram range. In some cases, pictograms of target can be detected.
Find additional tips, troubleshooting help, and resources within our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
The Dynabeads Co-immunoprecipitation Kit is specially designed for protein complex pulldown only, not for simple IP. These beads are the Dynabeads M270 Epoxy (Cat. No. 14301) beads and are used for covalent binding of the antibody so it will not be co-eluted off with the target complex during mild elution. The kit also contains a buffer system that should make it easier to optimize for recovering the complex.
With the Dynabeads Protein A or G magnetic beads, there is only a non-covalent binding between the Protein G on the beads and the antibody. Thus, the antibody will be co-eluted with the target protein unless you crosslink it to the beads beforehand. In general, we recommend the Dynabeads Co-immunoprecipitation Kit for complex pulldown, especially if you are working with large, labile complexes or if your downstream application is mass spectrometry.
Secondary coated Dynabeads magnetic beads (like the Dynabeads anti-mouse IgG beads) can also be used for IP, but, the drawback when compared to Dynabeads Protein A or G magnetic beads, is that they will only work with an antibody from 1 species. However, the binding between the primary antibody and the secondary antibody might be a bit stronger than between Protein A or G and the antibody. Hence, you can apply more stringent washing conditions. That being said, Dynabeads Protein A and G magnetic beads should give a very low background.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
Within practical limits, the elution volume can be scaled up or down to suit your experiment. However, volumes less than 10 µL become more difficult to work with. In addition, the amount of target is important. If you have a lot of beads with a lot of bound target in a small elution volume, your elution may not be very efficient. Typically, 15-100 µL of beads may be eluted in 30 µL. For efficient recovery of the antigen and/or binding partners, the elution volume should at minimum equal the volume of the beads.
Find additional tips, troubleshooting help, and resources within our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
There are several methods to quantify the amount of antibody bound to the beads. The crudest method is to measure the concentration of antibody in the coupling reaction before and after antibody attachment. Either fluorescence measurements or absorbance at 280 nm can be used. Alternatively, you could measure the amount of antibody bound to the beads by fluorescence, chemiluminescence, or radiolabeling detection methods.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Incubation time will depend on the immunogenicity of the primary antibody and its binding affinity with the specific antigens. For a good primary antibody, 30-40 minutes incubation should work well. If you are working with a poor antibody or a very low-abundance protein, you could try to increase binding by incubating overnight. However, this also increases the chance of background protein binding.
Find additional tips, troubleshooting help, and resources within our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
If the target protein has the same molecular weight as the heavy or light chain antibody, we would recommend covalently binding the antibody to the bead surface. This can be done by either crosslinking the antibody to the Dynabeads Protein A or G magnetic beads, or secondary coated beads, or by using one of the surface-activated Dynabeads magnetic beads.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
The Dynabeads Antibody Coupling kit includes buffers, beads, and the protocol for covalent antibody coupling to beads. The Dynabeads Co-Immunoprecipitation kit includes the complete Antibody Coupling Kit, plus the additional buffers and protocol required for successful co-immunoprecipitation.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
The lysis buffer in the Dynabeads Co-immunoprecipitation Kit will not lyse the nuclei; however, the IP Lysis Buffer in the Pierce IP and Co-IP Kits (Agarose and Magnetic) will lyse both the cell membrane and the nuclear membrane.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
The Dynabeads Co-Immunoprecipitation Kit contains Dynabeads M-270 Epoxy beads and proprietary buffers for co- immunoprecipitation.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
Using Dynabeads magnetic beads for protein isolation provides several advantages:
-Rapid binding kinetics: since the number of beads per volume for Dynabeads is approximately 1,000 times higher than for the same volume of a Sepharose slurry, the probability for Dynabeads magnetic beads to hit the target is far greater.
-Incubation time: due to the rapid binding kinetics, the protocol is usually very short.
-Low background: due to the rapid binding kinetics and the short incubation time, the background is also very low.
-Trapping of impurities: the beads offer no internal volume for binding or trapping of impurities.
-Low antibody consumption: this is because Dynabeads magnetic beads are nonporous, uniform superparamagnetic, monodispersed, highly crosslinked polystyrene microspheres consisting of an even dispersion of magnetic material throughout the bead. The beads are coated with a thin layer of a highly crosslinked polystyrene shell that encases the magnetic material and prevents any leakage from the beads or trapping of ligands in the bead interior. The outer layer also provides a defined surface area for the adsorption or coupling of various molecules such as antibodies. Uniformity of bead size and shape provide consistent physical and chemical properties. These uniform physical characteristics lead to high-quality, reproducible results.
-Reproducibility: due to easier practical handling, such as pipetting. No centrifugation steps or preclearing are required.
Find additional tips, troubleshooting help, and resources within ourProtein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
No. Not only is dithionite a reducing agent, but the strong affinity of the dithionite ion for bivalent and trivalent metal cations (M2+, M3+) allows it to enhance the solubility of iron, making it a chelating agent. As a result, the iron in the Dynabeads magnetic beads is reduced and pulled out when they are exposed to dithionite. The same is observed if Dynabeads magnetic beads are exposed to DTT and EDTA. With EDTA, we highly recommend checking the minimal amount of EDTA that your specific molecules would tolerate for binding to the Dynabeads, and if it will affect your specific application. For some applications, low concentrations of EDTA can be tolerated by Dynabeads. On the other hand, using 10 mM EDTA with heating affects the binding of biotin molecules to Dynabeads streptavidin.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Yes, they are compatible with 6-8 M Urea when used during post-coupling steps.
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.
Dynabeads magnetic beads, being magnetic in nature are really not designed to be centrifuged. That being said, the beads themselves are compact, as the pores in the polymer matrix are filled with magnetic material and coated with a final outer polymer shell that will further add to the rigidity of the beads. Hence, pressure should theoretically not be a problem for the beads themselves, but the force exerted by the beads on surrounding cells in the pellet may be detrimental to the cells.
Find additional tips, troubleshooting help, and resources within our Dynabeads Nucleic Acid Purification Support Center as well as our Protein Immunoprecipitation (IP), Co-Immunoprecipitation (Co-IP), and Pulldown Support Center.
Magnetic beads, unlike agarose beads, are solid and spherical, and antibody binding is limited to the surface of each bead. While magnetic beads do not have the advantage of a porous center to increase the binding capacity, they are significantly smaller than agarose beads (1 to 4 µm), which collectively gives them adequate surface area-to-volume ratios for optimum antibody binding.
High-power magnets are used to localize magnetic beads to the side of the incubation tube and out of the way to enable cell lysate aspiration without the risk of also aspirating immune complexes bound to the beads. Magnetic separation avoids centrifugation, which can break weak antibody-antigen binding and cause loss of target protein.
However, an issue with the use of magnetic beads is that bead size variations may prevent all beads from localizing to the magnet. Additionally, while immunoprecipitation using agarose beads only requires standard laboratory equipment, the use of magnetic beads for immunoprecipitation applications requires high-power magnetic equipment that can be cost-prohibitive. Read more about our Magnetic Immunoprecipitation Products (https://www.thermofisher.com/us/en/home/life-science/protein-biology/protein-assays-analysis/immunoprecipitation.html#products).
Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.