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Technique / Proteomics and protein biochemistry / Western blot assay


Western blot



Western blot

A typical western blot procedure includes following steps:

1. Protein lysate preparation from cells and tissues.
2. Protein assay for determination of protein concentration in lysate.
3. Denaturing and reduction of protein complexes before loading onto gel.
4. Protein electrophoresis to separate proteins according to their molecular weight (size).
5. Transfer of separated proteins onto appropriate membrane (nylone, nitrocellulose or PVDF etc).
6. Blocking the membrane with appropriate blocking reagents.
7. Incubation with primary antibody against the protein of your interests.
8. Incubation with enzyme-conjugated secondary antibody recognizing the primary antibody.
9. Western blot signal developing.
10. Storage of membrane or strip and re-probe with another antibody.

Useful links for western blot:

How to do a western blot (western blot protocol and general procedure)
A step by step protocol on western blot with detailed description on reagent preparation, sample lysis, protein quantitation, gel casting, transfer, blot and stripping. (Jonathan Flint lab)

Western blot introduction (Wikipedia)
A western blot (alternately, immunoblot) is a method in molecular biology/biochemistry/immunogenetics to detect protein in a given sample of tissue homogenate or extract. It uses gel electrophoresis to separate native proteins by shape and size. The proteins are then transferred out of the gel and onto a membrane (typically nitrocellulose or PVDF), where they are "probed" using antibodies specific to the protein. As a result, researchers can examine the size, processing, or amount of protein in a given sample and compare several groups.

Last update 15-Jan-2005, Rating Good of 9 votes.


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