Elimination of keratin artifact bands from western blots by using low concentrations of reducing agents

T. F. Lee; T. W. McNellis

doi:10.1016/j.ab.2008.07.035

Elimination of keratin artifact bands from western blots by using low concentrations of reducing agents

T. F. Lee, T. W. McNellis

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

7 Scopus citations

Abstract

We encountered β-mercaptoethanol-dependent artifact signals in western blot analyses using polyclonal antisera. Replacing β-mercaptoethanol with dithiothreitol in the loading buffer did not eliminate the artifact signals. However, lowering the concentration of either dithiothreitol or β-mercaptoethanol eliminated the background problems and allowed specific detection of the target protein. These results are consistent with the background signal being caused by anti-keratin antibodies in the antisera and keratin contamination of reagents. This study highlights the importance of testing a range of reducing agent concentrations when trying to eliminate artifact bands from western blots. However, this method may not be applicable when target proteins have disulfide bridges.

Original language	English (US)
Pages (from-to)	141-143
Number of pages	3
Journal	Analytical Biochemistry
Volume	382
Issue number	2
DOIs	https://doi.org/10.1016/j.ab.2008.07.035
State	Published - Nov 15 2008

All Science Journal Classification (ASJC) codes

Biophysics
Biochemistry
Molecular Biology
Cell Biology

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10.1016/j.ab.2008.07.035

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title = "Elimination of keratin artifact bands from western blots by using low concentrations of reducing agents",

abstract = "We encountered β-mercaptoethanol-dependent artifact signals in western blot analyses using polyclonal antisera. Replacing β-mercaptoethanol with dithiothreitol in the loading buffer did not eliminate the artifact signals. However, lowering the concentration of either dithiothreitol or β-mercaptoethanol eliminated the background problems and allowed specific detection of the target protein. These results are consistent with the background signal being caused by anti-keratin antibodies in the antisera and keratin contamination of reagents. This study highlights the importance of testing a range of reducing agent concentrations when trying to eliminate artifact bands from western blots. However, this method may not be applicable when target proteins have disulfide bridges.",

author = "Lee, {T. F.} and McNellis, {T. W.}",

note = "Funding Information: This work was supported, in part, by a United States Department of Agriculture Cooperative State Research, Education, and Extension Service grant program (USDA-CSREES grant no. 2002-35319-11561 to T.W. M.), by the Department of Plant Pathology at the Pennsylvania State University, and by the Intercollege Graduate Program in Plant Biology at the Pennsylvania State University.",

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doi = "10.1016/j.ab.2008.07.035",

language = "English (US)",

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journal = "Analytical Biochemistry",

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AU - McNellis, T. W.

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N2 - We encountered β-mercaptoethanol-dependent artifact signals in western blot analyses using polyclonal antisera. Replacing β-mercaptoethanol with dithiothreitol in the loading buffer did not eliminate the artifact signals. However, lowering the concentration of either dithiothreitol or β-mercaptoethanol eliminated the background problems and allowed specific detection of the target protein. These results are consistent with the background signal being caused by anti-keratin antibodies in the antisera and keratin contamination of reagents. This study highlights the importance of testing a range of reducing agent concentrations when trying to eliminate artifact bands from western blots. However, this method may not be applicable when target proteins have disulfide bridges.

AB - We encountered β-mercaptoethanol-dependent artifact signals in western blot analyses using polyclonal antisera. Replacing β-mercaptoethanol with dithiothreitol in the loading buffer did not eliminate the artifact signals. However, lowering the concentration of either dithiothreitol or β-mercaptoethanol eliminated the background problems and allowed specific detection of the target protein. These results are consistent with the background signal being caused by anti-keratin antibodies in the antisera and keratin contamination of reagents. This study highlights the importance of testing a range of reducing agent concentrations when trying to eliminate artifact bands from western blots. However, this method may not be applicable when target proteins have disulfide bridges.

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ER -

Elimination of keratin artifact bands from western blots by using low concentrations of reducing agents

Abstract

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