Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations: A Method to Maximize S-Nitrosylation Detection

Heaseung Sophia Chung; Christopher I. Murray; Vidya Venkatraman; Erin L. Crowgey; Peter P. Rainer; Robert N. Cole; Ryan D. Bomgarden; John C. Rogers; Wayne Balkan; Joshua M. Hare; David A. Kass; Jennifer E. Van Eyk

doi:10.1161/CIRCRESAHA.115.307336

Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations: A Method to Maximize S-Nitrosylation Detection

Heaseung Sophia Chung, Christopher I. Murray, Vidya Venkatraman, Erin L. Crowgey, Peter P. Rainer, Robert N. Cole, Ryan D. Bomgarden, John C. Rogers, Wayne Balkan, Joshua M. Hare, David A. Kass, Jennifer E. Van Eyk

School of Medicine

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

16 Scopus citations

Abstract

Rationale: S-nitrosylation (SNO), an oxidative post-translational modification of cysteine residues, responds to changes in the cardiac redox-environment. Classic biotin-switch assay and its derivatives are the most common methods used for detecting SNO. In this approach, the labile SNO group is selectively replaced with a single stable tag. To date, a variety of thiol-reactive tags have been introduced. However, these methods have not produced a consistent data set, which suggests an incomplete capture by a single tag and potentially the presence of different cysteine subpopulations. Objective: To investigate potential labeling bias in the existing methods with a single tag to detect SNO, explore if there are distinct cysteine subpopulations, and then, develop a strategy to maximize the coverage of SNO proteome. Methods and Results: We obtained SNO-modified cysteine data sets for wild-type and S-nitrosoglutathione reductase knockout mouse hearts (S-nitrosoglutathione reductase is a negative regulator of S-nitrosoglutathione production) and nitric oxide-induced human embryonic kidney cell using 2 labeling reagents: the cysteine-reactive pyridyldithiol and iodoacetyl based tandem mass tags. Comparison revealed that <30% of the SNO-modified residues were detected by both tags, whereas the remaining SNO sites were only labeled by 1 reagent. Characterization of the 2 distinct subpopulations of SNO residues indicated that pyridyldithiol reagent preferentially labels cysteine residues that are more basic and hydrophobic. On the basis of this observation, we proposed a parallel dual-labeling strategy followed by an optimized proteomics workflow. This enabled the profiling of 493 SNO sites in S-nitrosoglutathione reductase knockout hearts. Conclusions: Using a protocol comprising 2 tags for dual-labeling maximizes overall detection of SNO by reducing the previously unrecognized labeling bias derived from different cysteine subpopulations.

Original language	English (US)
Pages (from-to)	846-857
Number of pages	12
Journal	Circulation research
Volume	117
Issue number	10
DOIs	https://doi.org/10.1161/CIRCRESAHA.115.307336
State	Published - Oct 23 2015

Keywords

S-nitrosothiols
nitric oxide
oxidation-reduction
proteomics

ASJC Scopus subject areas

Physiology
Cardiology and Cardiovascular Medicine

Access to Document

10.1161/CIRCRESAHA.115.307336

Cite this

Chung, H. S., Murray, C. I., Venkatraman, V., Crowgey, E. L., Rainer, P. P., Cole, R. N., Bomgarden, R. D., Rogers, J. C., Balkan, W., Hare, J. M., Kass, D. A., & Van Eyk, J. E. (2015). Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations: A Method to Maximize S-Nitrosylation Detection. Circulation research, 117(10), 846-857. https://doi.org/10.1161/CIRCRESAHA.115.307336

Chung, HS, Murray, CI, Venkatraman, V, Crowgey, EL, Rainer, PP, Cole, RN, Bomgarden, RD, Rogers, JC, Balkan, W, Hare, JM, Kass, DA & Van Eyk, JE 2015, 'Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations: A Method to Maximize S-Nitrosylation Detection', Circulation research, vol. 117, no. 10, pp. 846-857. https://doi.org/10.1161/CIRCRESAHA.115.307336

@article{a051074b38a640e1a4e5dec381e43990,

title = "Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations: A Method to Maximize S-Nitrosylation Detection",

abstract = "Rationale: S-nitrosylation (SNO), an oxidative post-translational modification of cysteine residues, responds to changes in the cardiac redox-environment. Classic biotin-switch assay and its derivatives are the most common methods used for detecting SNO. In this approach, the labile SNO group is selectively replaced with a single stable tag. To date, a variety of thiol-reactive tags have been introduced. However, these methods have not produced a consistent data set, which suggests an incomplete capture by a single tag and potentially the presence of different cysteine subpopulations. Objective: To investigate potential labeling bias in the existing methods with a single tag to detect SNO, explore if there are distinct cysteine subpopulations, and then, develop a strategy to maximize the coverage of SNO proteome. Methods and Results: We obtained SNO-modified cysteine data sets for wild-type and S-nitrosoglutathione reductase knockout mouse hearts (S-nitrosoglutathione reductase is a negative regulator of S-nitrosoglutathione production) and nitric oxide-induced human embryonic kidney cell using 2 labeling reagents: the cysteine-reactive pyridyldithiol and iodoacetyl based tandem mass tags. Comparison revealed that <30% of the SNO-modified residues were detected by both tags, whereas the remaining SNO sites were only labeled by 1 reagent. Characterization of the 2 distinct subpopulations of SNO residues indicated that pyridyldithiol reagent preferentially labels cysteine residues that are more basic and hydrophobic. On the basis of this observation, we proposed a parallel dual-labeling strategy followed by an optimized proteomics workflow. This enabled the profiling of 493 SNO sites in S-nitrosoglutathione reductase knockout hearts. Conclusions: Using a protocol comprising 2 tags for dual-labeling maximizes overall detection of SNO by reducing the previously unrecognized labeling bias derived from different cysteine subpopulations.",

keywords = "S-nitrosothiols, nitric oxide, oxidation-reduction, proteomics",

author = "Chung, {Heaseung Sophia} and Murray, {Christopher I.} and Vidya Venkatraman and Crowgey, {Erin L.} and Rainer, {Peter P.} and Cole, {Robert N.} and Bomgarden, {Ryan D.} and Rogers, {John C.} and Wayne Balkan and Hare, {Joshua M.} and Kass, {David A.} and {Van Eyk}, {Jennifer E.}",

note = "Publisher Copyright: {\textcopyright} 2015 American Heart Association, Inc.",

year = "2015",

month = oct,

day = "23",

doi = "10.1161/CIRCRESAHA.115.307336",

language = "English (US)",

volume = "117",

pages = "846--857",

journal = "Circulation research",

issn = "0009-7330",

publisher = "Lippincott Williams and Wilkins",

number = "10",

}

TY - JOUR

T1 - Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations

T2 - A Method to Maximize S-Nitrosylation Detection

AU - Chung, Heaseung Sophia

AU - Murray, Christopher I.

AU - Venkatraman, Vidya

AU - Crowgey, Erin L.

AU - Rainer, Peter P.

AU - Cole, Robert N.

AU - Bomgarden, Ryan D.

AU - Rogers, John C.

AU - Balkan, Wayne

AU - Hare, Joshua M.

AU - Kass, David A.

AU - Van Eyk, Jennifer E.

PY - 2015/10/23

Y1 - 2015/10/23

N2 - Rationale: S-nitrosylation (SNO), an oxidative post-translational modification of cysteine residues, responds to changes in the cardiac redox-environment. Classic biotin-switch assay and its derivatives are the most common methods used for detecting SNO. In this approach, the labile SNO group is selectively replaced with a single stable tag. To date, a variety of thiol-reactive tags have been introduced. However, these methods have not produced a consistent data set, which suggests an incomplete capture by a single tag and potentially the presence of different cysteine subpopulations. Objective: To investigate potential labeling bias in the existing methods with a single tag to detect SNO, explore if there are distinct cysteine subpopulations, and then, develop a strategy to maximize the coverage of SNO proteome. Methods and Results: We obtained SNO-modified cysteine data sets for wild-type and S-nitrosoglutathione reductase knockout mouse hearts (S-nitrosoglutathione reductase is a negative regulator of S-nitrosoglutathione production) and nitric oxide-induced human embryonic kidney cell using 2 labeling reagents: the cysteine-reactive pyridyldithiol and iodoacetyl based tandem mass tags. Comparison revealed that <30% of the SNO-modified residues were detected by both tags, whereas the remaining SNO sites were only labeled by 1 reagent. Characterization of the 2 distinct subpopulations of SNO residues indicated that pyridyldithiol reagent preferentially labels cysteine residues that are more basic and hydrophobic. On the basis of this observation, we proposed a parallel dual-labeling strategy followed by an optimized proteomics workflow. This enabled the profiling of 493 SNO sites in S-nitrosoglutathione reductase knockout hearts. Conclusions: Using a protocol comprising 2 tags for dual-labeling maximizes overall detection of SNO by reducing the previously unrecognized labeling bias derived from different cysteine subpopulations.

AB - Rationale: S-nitrosylation (SNO), an oxidative post-translational modification of cysteine residues, responds to changes in the cardiac redox-environment. Classic biotin-switch assay and its derivatives are the most common methods used for detecting SNO. In this approach, the labile SNO group is selectively replaced with a single stable tag. To date, a variety of thiol-reactive tags have been introduced. However, these methods have not produced a consistent data set, which suggests an incomplete capture by a single tag and potentially the presence of different cysteine subpopulations. Objective: To investigate potential labeling bias in the existing methods with a single tag to detect SNO, explore if there are distinct cysteine subpopulations, and then, develop a strategy to maximize the coverage of SNO proteome. Methods and Results: We obtained SNO-modified cysteine data sets for wild-type and S-nitrosoglutathione reductase knockout mouse hearts (S-nitrosoglutathione reductase is a negative regulator of S-nitrosoglutathione production) and nitric oxide-induced human embryonic kidney cell using 2 labeling reagents: the cysteine-reactive pyridyldithiol and iodoacetyl based tandem mass tags. Comparison revealed that <30% of the SNO-modified residues were detected by both tags, whereas the remaining SNO sites were only labeled by 1 reagent. Characterization of the 2 distinct subpopulations of SNO residues indicated that pyridyldithiol reagent preferentially labels cysteine residues that are more basic and hydrophobic. On the basis of this observation, we proposed a parallel dual-labeling strategy followed by an optimized proteomics workflow. This enabled the profiling of 493 SNO sites in S-nitrosoglutathione reductase knockout hearts. Conclusions: Using a protocol comprising 2 tags for dual-labeling maximizes overall detection of SNO by reducing the previously unrecognized labeling bias derived from different cysteine subpopulations.

KW - S-nitrosothiols

KW - nitric oxide

KW - oxidation-reduction

KW - proteomics

UR - http://www.scopus.com/inward/record.url?scp=84945464603&partnerID=8YFLogxK

UR - http://www.scopus.com/inward/citedby.url?scp=84945464603&partnerID=8YFLogxK

U2 - 10.1161/CIRCRESAHA.115.307336

DO - 10.1161/CIRCRESAHA.115.307336

M3 - Article

C2 - 26338901

AN - SCOPUS:84945464603

SN - 0009-7330

VL - 117

SP - 846

EP - 857

JO - Circulation research

JF - Circulation research

IS - 10

ER -

Dual Labeling Biotin Switch Assay to Reduce Bias Derived from Different Cysteine Subpopulations: A Method to Maximize S-Nitrosylation Detection

Abstract

Keywords

ASJC Scopus subject areas

Access to Document

Other files and links

Fingerprint

Cite this