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Merck
CN

LSKMAGL10

PureProteome Albumin Magnetic Beads

The PureProteome Albumin Magnetic Beads are conjugated to an antibody specific for human serum albumin.

Synonym(s):

Albumin Magnetic Beads, Protein Bead Kit

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About This Item

UNSPSC Code:
41116133
NACRES:
NA.56
eCl@ss:
32160405
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packaging

pkg of 10 mL

manufacturer/tradename

PureProteome

technique(s)

depletion: suitable (serum), protein purification: suitable

particle size

10 μm

shipped in

wet ice

storage temp.

2-8°C

General description

The PureProteome Albumin Magnetic Beads are conjugated to an antibody specific for human serum albumin. These magnetic beads provide a rapid, scalable, and reproducible means to deplete >98% of albumin from serum and plasma samples, facilitating the detection and analysis of proteins of interest. For efficient depletion, the PureProteome Magnetic Beads must be used with the PureProteome Magnetic Stand.

Analysis Note

Depletion: >98% depletion of Albumin


Storage Class

12 - Non Combustible Liquids

wgk

WGK 2

flash_point_f

Not applicable

flash_point_c

Not applicable



Certificates of Analysis (COA)

Search for Certificates of Analysis (COA) by entering the products Lot/Batch Number. Lot and Batch Numbers can be found on a product’s label following the words ‘Lot’ or ‘Batch’.

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Related Content

Biomarkers offer important information about homeostasis, disease, response to drug treatments, and environmental stimuli. Sera are rich sources of biomarkers (biological indicator proteins, peptides, small molecules, etc.) and are easier to sample than other tissues. However, the complexity of serum and the presence of highly abundant proteins like albumin and immunoglobulin can mask less abundant species, hindering biomarker detection. PureProteome albumin magnetic beads remove more than 98% of albumin from human serum. Here, we demonstrate that PureProteome albumin magnetic beads may also be used to remove albumin from mouse, guinea pig and rat sera. Depleted samples are often dilute, and may need concentration for downstream analyses. Therefore, we present a protocol for the convenient concentration of these samples using Amicon Ultra 2 mL centrifugal filters.

Purification of recombinant proteins expressed in E.coli requires many time-consuming steps. To liberate the protein of interest, traditional bacterial lysis relies on the addition of lysozyme and a combination of sonication and repeated freeze/thaw cycles to break the bacterial cell wall. Disruption of the cell is accompanied by an increase in the viscosity of the suspension, due to the release of DNA. An endonuclease is added to digest the DNA, thus reducing the viscosity of the lysate. Finally, to render the lysate compatible with traditional purification methods, insoluble cell debris must be removed by centrifugation.

Traditionally, protein purification from E. coli consists of four distinct phases: harvest, bacterial cell lysis, lysate clarification and protein purification. Bacterial lysis typically requires several time-consuming, hands-on steps, such as freeze/thaw cycles and sonication. These harsh lysis techniques may negatively impact protein quality and contribute to sample-to-sample variability. To maintain protein activity and integrity, detergent-based lysis buffers are routinely used to avoid mechanical protein extraction methods. Regardless of the lysis method used, centrifugation is traditionally required to pellet unwanted cell debris and permit recovery of the clarified lysate. The final step, purification, is frequently performed using affinity media specific for expressed epitope tags. Agarose-based media have typically been used, either as a slurry in microcentrifuge tubes or packed into gravity-driven or spin columns. While easier to manipulate, columns are greatly affected by lysate consistency and carryover of cell debris, which can lead to clogging of the column frits.

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Global Trade Item Number

SKUGTIN
LSKMAGL1004053252479274