Transfer efficiency from polyacrylamide gels and binding to Immobilon P and CD were tested in different buffers with 125I-labelled proteins. With a derivatized poly(vinylidene difluoride) membrane, a pH 8 medium was found to be superior to a more alkaline solution, for both acidic and basicproteins. New staining protocols were tried on ImmobilonCD. Toluidine Blue and iodine vapour gave a negative and a positive stain, respectively, with a fair band-to-background contrast. Protein sequencing after both stains was not impaired by interfering peaks. Biuret solution stained the protein bands pale pink but, even after copper removal with a chelating agent, it completely prevented Edman degradation. The first two procedures compare favourably with a commercial kit for protein detection, Quick Stain, that provides comparable sensitivity but results in several spurious peaks on protein sequencing.

Basic proteins and basic membranes adjusting blotting and staining conditions to immobilon CD / E. Gianazza, P. Coari, M. Lovati, C. Manzoni, E. Ghibaudi, M. Salmona. - In: JOURNAL OF CHROMATOGRAPHY A. - ISSN 0021-9673. - 698:1-2(1995), pp. 351-359.

Basic proteins and basic membranes adjusting blotting and staining conditions to immobilon CD

E. Gianazza
Primo
;
M. Lovati;C. Manzoni;
1995

Abstract

Transfer efficiency from polyacrylamide gels and binding to Immobilon P and CD were tested in different buffers with 125I-labelled proteins. With a derivatized poly(vinylidene difluoride) membrane, a pH 8 medium was found to be superior to a more alkaline solution, for both acidic and basicproteins. New staining protocols were tried on ImmobilonCD. Toluidine Blue and iodine vapour gave a negative and a positive stain, respectively, with a fair band-to-background contrast. Protein sequencing after both stains was not impaired by interfering peaks. Biuret solution stained the protein bands pale pink but, even after copper removal with a chelating agent, it completely prevented Edman degradation. The first two procedures compare favourably with a commercial kit for protein detection, Quick Stain, that provides comparable sensitivity but results in several spurious peaks on protein sequencing.
Settore BIO/10 - Biochimica
1995
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/2434/180943
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