Electroblotting is a method in molecular biology/biochemistry/immunogenetics to transfer proteins or nucleic acids onto a membrane by using PVDF or nitrocellulose, after gel electrophoresis. The protein or nucleic acid can then be further analyzed using probes such as specific antibodies, ligands like lectins, or stains. This method can be used with all polyacrylamide and agarose gels. An alternative technique for transferring proteins from a gel is capillary blotting.
This technique was patented in 1989 by William J. Littlehales under the title "Electroblotting technique for transferring specimens from a polyacrylamide electrophoresis or like gel onto a membrane.
This technique relies upon current and a transfer buffer solution to drive proteins or nucleic acids onto a membrane. Following electrophoresis, a standard tank or semi-dry blotting transfer system is set up. A stack is put together in the following order from cathode to anode: sponge | three sheets of filter paper soaked in transfer buffer | gel | PVDF or nitrocellulose membrane | three sheets of filter paper soaked in transfer buffer | sponge. It is a necessity that the membrane is located between the gel and the positively charged anode, as the current and sample will be moving in that direction. Once the stack is prepared, it is placed in the transfer system, and a current of suitable magnitude is applied for a suitable period of time according to the materials being used.
Typically the electrophoresis gel is stained with Coomassie brilliant blue following the transfer to ensure that a sufficient quantity of material has been transferred. Because the proteins may retain or regain part of their structure during blotting they may react with specific antibodies giving rise to the term immunoblotting. Alternatively the proteins may react with ligands like lectins giving rise to the term affinity blotting.
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Le transfert de protéines, en anglais western blot (également appelé buvardage de western ou encore technique des immuno-empreintes), est une méthode de biologie moléculaire permettant la détection et l'identification de protéines spécifiques dans un échantillon biologique (sérum ou autre extrait ou homogénat tissulaire) à l'aide d'anticorps dirigés contre ces protéines que l'on souhaite détecter. Le western blot permet ainsi de visualiser des protéines particulières dans un mélange complexe.
alt=Appareil à électrophorèse sur gel d'agarose|vignette|Appareil pour électrophorèse d'ADN en gel d'agarose. Le gel est horizontal baigne dans le tampon qui remplit la cuve. L'ADN est déposé dans des puits à une extrémité du gel. L'alimentation en arrière-plan fournit la tension électrique continue qui permet la migration des fragments d'ADN dans le gel. L'électrophorèse sur gel est une variante de l'électrophorèse de zones.
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