Screening Method Using Selected Reaction Monitoring for Targeted Proteomics Studies of Nasal Lavage Fluid.

Mörtstedt, Harriet; Kåredal, Monica; Jönsson, Bo A; Lindh, Christian

Screening Method Using Selected Reaction Monitoring for Targeted Proteomics Studies of Nasal Lavage Fluid.

Mark

Mörtstedt, Harriet ^LU ; Kåredal, Monica ^LU

; Jönsson, Bo A ^LU and Lindh, Christian ^LU

(2012) In Journal of Proteome Research

Abstract: Proteomic-based studies of nasal lavage fluid (NLF) may identify molecular pathways associated with disease pathology and new biomarker candidates of upper airway diseases. However, most studies have used rather tedious untargeted MS techniques. Selected reaction monitoring (SRM) is a sensitive and specific technique that can be used with high throughput. In this study, we developed a semiquantitative SRM-based method targeting 244 NLF proteins. The protein set was identified through a literature study in combination with untargeted LC-MS/MS analyses of trypsin-digested NLF samples. The SRM assays were designed using MS/MS data either downloaded from a proteomic data repository or experimentally obtained. Each protein is represented by one... (More); Proteomic-based studies of nasal lavage fluid (NLF) may identify molecular pathways associated with disease pathology and new biomarker candidates of upper airway diseases. However, most studies have used rather tedious untargeted MS techniques. Selected reaction monitoring (SRM) is a sensitive and specific technique that can be used with high throughput. In this study, we developed a semiquantitative SRM-based method targeting 244 NLF proteins. The protein set was identified through a literature study in combination with untargeted LC-MS/MS analyses of trypsin-digested NLF samples. The SRM assays were designed using MS/MS data either downloaded from a proteomic data repository or experimentally obtained. Each protein is represented by one to five peptides, resulting in 708 SRM assays. Three to four transitions per assay were used to ensure analyte specificity. The majority (69%) of the assays showed good within-day precision (coefficient of variation ≤20%). The accuracy of the method was evaluated by analyzing four samples prepared with varying amounts of four proteins. Peptide and protein ratios were in good agreement with expected ratios. In conclusion, a high throughput screening method for relative quantification of 244 NLF proteins was developed. The method should be of general use in any proteomic study of the upper airways. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/3347589

author

Mörtstedt, Harriet ^LU ; Kåredal, Monica ^LU

; Jönsson, Bo A ^LU and Lindh, Christian ^LU

organization

Division of Occupational and Environmental Medicine, Lund University

publishing date

2012-12-14

type

Contribution to journal

publication status

published

subject

Environmental Health and Occupational Health

in

Journal of Proteome Research

publisher

The American Chemical Society (ACS)

external identifiers

wos:000313156300044
pmid:23214469
scopus:84874053586
pmid:23214469

ISSN

1535-3893

DOI

10.1021/pr300802g

language

English

LU publication?

yes

id

4583f6a3-7cb0-44b3-b432-cb529b18e9d8 (old id 3347589)

alternative location

http://www.ncbi.nlm.nih.gov/pubmed/23214469?dopt=Abstract

date added to LUP

2016-04-04 08:53:58

date last changed

2022-03-23 03:09:10

@article{4583f6a3-7cb0-44b3-b432-cb529b18e9d8,
  abstract     = {{Proteomic-based studies of nasal lavage fluid (NLF) may identify molecular pathways associated with disease pathology and new biomarker candidates of upper airway diseases. However, most studies have used rather tedious untargeted MS techniques. Selected reaction monitoring (SRM) is a sensitive and specific technique that can be used with high throughput. In this study, we developed a semiquantitative SRM-based method targeting 244 NLF proteins. The protein set was identified through a literature study in combination with untargeted LC-MS/MS analyses of trypsin-digested NLF samples. The SRM assays were designed using MS/MS data either downloaded from a proteomic data repository or experimentally obtained. Each protein is represented by one to five peptides, resulting in 708 SRM assays. Three to four transitions per assay were used to ensure analyte specificity. The majority (69%) of the assays showed good within-day precision (coefficient of variation ≤20%). The accuracy of the method was evaluated by analyzing four samples prepared with varying amounts of four proteins. Peptide and protein ratios were in good agreement with expected ratios. In conclusion, a high throughput screening method for relative quantification of 244 NLF proteins was developed. The method should be of general use in any proteomic study of the upper airways.}},
  author       = {{Mörtstedt, Harriet and Kåredal, Monica and Jönsson, Bo A and Lindh, Christian}},
  issn         = {{1535-3893}},
  language     = {{eng}},
  month        = {{12}},
  publisher    = {{The American Chemical Society (ACS)}},
  series       = {{Journal of Proteome Research}},
  title        = {{Screening Method Using Selected Reaction Monitoring for Targeted Proteomics Studies of Nasal Lavage Fluid.}},
  url          = {{http://dx.doi.org/10.1021/pr300802g}},
  doi          = {{10.1021/pr300802g}},
  year         = {{2012}},
}

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Screening Method Using Selected Reaction Monitoring for Targeted Proteomics Studies of Nasal Lavage Fluid.