Publication | Open Access
Use of a protein-blotting procedure and a specific DNA probe to identify nuclear proteins that recognize the promoter region of the transferrin receptor gene.
288
Citations
29
References
1985
Year
GeneticsDna AnalysisMolecular BiologyMolecular GeneticsTransferrin Receptor GeneSpecific Dna ProbeProteomicsCrude Nuclear ExtractsBiochemistryMolecular Biological MethodReceptor (Biochemistry)Dna ReplicationOligonucleotideNuclear OrganizationGene ExpressionCell BiologyPromoter RegionReporter Gene AssayNatural SciencesProtein EngineeringMedicine
We describe a procedure for detecting high-affinity, sequence-specific DNA-binding proteins from crude nuclear extracts. The technique utilizes electrophoretic transfer of NaDodSO4/PAGE-fractionated proteins onto nitrocellulose filters. Incubation of the filters with a 5% (wt/vol) solution of nonfat dry milk effectively blocks nonspecific and low-affinity DNA-binding sites. Incubation of the blocked filters with radiolabeled DNA under optimal binding conditions and subsequent autoradiography reveals high-affinity DNA-protein interactions. We have used this procedure to identify proteins that bind specifically to the promoter region of the transferrin receptor gene.
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