Detecting multiple proteins by Western blotting using same-species primary antibodies, precomplexed serum, and hydrogen peroxide

Ritika Upadhaya; Wataru Mizunoya; Judy E. Anderson

doi:10.1016/j.ab.2011.08.014

Detecting multiple proteins by Western blotting using same-species primary antibodies, precomplexed serum, and hydrogen peroxide

Ritika Upadhaya, Wataru Mizunoya, Judy E. Anderson

Animal and Marine Bioresource Sciences

Research output: Contribution to journal › Article › peer-review

16 Citations (Scopus)

Abstract

Western blot detection of multiple proteins is challenged by the need to use antibodies from the same species and the harsh stripping methods that can remove protein or reduce protein antigenicity. Quenching using 27% hydrogen peroxide was developed as an alternative to stripping to inhibit horseradish peroxidase used to detect secondary antibodies. To detect two epitopes with same-species primary antibodies, quenching was followed by incubation in a precomplexed mixture of primary and secondary antibodies for the second epitope plus serum from that species. Both methods will be valuable in specific detection of multiple proteins by Western blotting, and will save time, valuable samples, and reagents.

Original language	English
Pages (from-to)	342-344
Number of pages	3
Journal	Analytical Biochemistry
Volume	419
Issue number	2
DOIs	https://doi.org/10.1016/j.ab.2011.08.014
Publication status	Published - Dec 15 2011

All Science Journal Classification (ASJC) codes

Biophysics
Biochemistry
Molecular Biology
Cell Biology

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10.1016/j.ab.2011.08.014

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abstract = "Western blot detection of multiple proteins is challenged by the need to use antibodies from the same species and the harsh stripping methods that can remove protein or reduce protein antigenicity. Quenching using 27% hydrogen peroxide was developed as an alternative to stripping to inhibit horseradish peroxidase used to detect secondary antibodies. To detect two epitopes with same-species primary antibodies, quenching was followed by incubation in a precomplexed mixture of primary and secondary antibodies for the second epitope plus serum from that species. Both methods will be valuable in specific detection of multiple proteins by Western blotting, and will save time, valuable samples, and reagents.",

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note = "Funding Information: The authors acknowledge funding by the Canadian Space Agency (9F007-052237/001/SR) and the Natural Sciences and Engineering Research Foundation, a postdoctoral fellowship from Foreign Affairs and International Trade Canada (W.M.), and assistance from W. Snow and S. Lakhi. ",

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AB - Western blot detection of multiple proteins is challenged by the need to use antibodies from the same species and the harsh stripping methods that can remove protein or reduce protein antigenicity. Quenching using 27% hydrogen peroxide was developed as an alternative to stripping to inhibit horseradish peroxidase used to detect secondary antibodies. To detect two epitopes with same-species primary antibodies, quenching was followed by incubation in a precomplexed mixture of primary and secondary antibodies for the second epitope plus serum from that species. Both methods will be valuable in specific detection of multiple proteins by Western blotting, and will save time, valuable samples, and reagents.

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Detecting multiple proteins by Western blotting using same-species primary antibodies, precomplexed serum, and hydrogen peroxide

Abstract

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