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Literature DB >> 18522437

Quantitative analysis of isotope distributions in proteomic mass spectrometry using least-squares Fourier transform convolution.

Edit Sperling¹, Anne E Bunner, Michael T Sykes, James R Williamson.

Abstract

Quantitative proteomic mass spectrometry involves comparison of the amplitudes of peaks resulting from different isotope labeling patterns, including fractional atomic labeling and fractional residue labeling. We have developed a general and flexible analytical treatment of the complex isotope distributions that arise in these experiments, using Fourier transform convolution to calculate labeled isotope distributions and least-squares for quantitative comparison with experimental peaks. The degree of fractional atomic and fractional residue labeling can be determined from experimental peaks at the same time as the integrated intensity of all of the isotopomers in the isotope distribution. The approach is illustrated using data with fractional (15)N-labeling and fractional (13)C-isoleucine labeling. The least-squares Fourier transform convolution approach can be applied to many types of quantitative proteomic data, including data from stable isotope labeling by amino acids in cell culture and pulse labeling experiments.

Entities: Chemical

Mesh：

Substances：

Year: 2008 PMID： 18522437 PMCID： PMC2502059 DOI： 10.1021/ac800080v

Source DB: PubMed Journal: Anal Chem ISSN： 0003-2700 Impact factor: 6.986

29 in total

1. Automatic analysis of hydrogen/deuterium exchange mass spectra of peptides and proteins using calculations of isotopic distributions.

Authors: M Palmblad; J Buijs; P Håkansson
Journal: J Am Soc Mass Spectrom Date: 2001-11 Impact factor: 3.109

2. Accurate quantitation of protein expression and site-specific phosphorylation.

Authors: Y Oda; K Huang; F R Cross; D Cowburn; B T Chait
Journal: Proc Natl Acad Sci U S A Date: 1999-06-08 Impact factor: 11.205

3. Proteome dynamics in complex organisms: using stable isotopes to monitor individual protein turnover rates.

Authors: Mary K Doherty; Colin Whitehead; Heather McCormack; Simon J Gaskell; Robert J Beynon
Journal: Proteomics Date: 2005-02 Impact factor: 3.984

4. Measurement of protein turnover rates by heavy water labeling of nonessential amino acids.

Authors: Robert Busch; Yoo-Kyeong Kim; Richard A Neese; Valerie Schade-Serin; Michelle Collins; Mohamad Awada; James L Gardner; Carine Beysen; Michael E Marino; Lisa M Misell; Marc K Hellerstein
Journal: Biochim Biophys Acta Date: 2006-01-24

Review 5. Avian proteomics: advances, challenges and new technologies.

Authors: M K Doherty; L McLean; R J Beynon
Journal: Cytogenet Genome Res Date: 2007 Impact factor: 1.636

6. Automated extraction of backbone deuteration levels from amide H/2H mass spectrometry experiments.

Authors: Matthew Hotchko; Ganesh S Anand; Elizabeth A Komives; Lynn F Ten Eyck
Journal: Protein Sci Date: 2006-03 Impact factor: 6.725

7. Global internal standard technology for comparative proteomics.

Authors: Asish Chakraborty; Fred E Regnier
Journal: J Chromatogr A Date: 2002-03-08 Impact factor: 4.759

8. Dissection of proteolytic 18O labeling: endoprotease-catalyzed 16O-to-18O exchange of truncated peptide substrates.

Authors: Xudong Yao; Carlos Afonso; Catherine Fenselau
Journal: J Proteome Res Date: 2003 Mar-Apr Impact factor: 4.466

9. Absolute multiplexed quantitative analysis of protein expression during muscle development using QconCAT.

Authors: Jenny Rivers; Deborah M Simpson; Duncan H L Robertson; Simon J Gaskell; Robert J Beynon
Journal: Mol Cell Proteomics Date: 2007-05-17 Impact factor: 5.911

10. The Deuterator: software for the determination of backbone amide deuterium levels from H/D exchange MS data.

Authors: B D Pascal; M J Chalmers; S A Busby; C C Mader; M R Southern; N F Tsinoremas; P R Griffin
Journal: BMC Bioinformatics Date: 2007-05-16 Impact factor: 3.169

32 in total

1. Protein turnover quantification in a multilabeling approach: from data calculation to evaluation.

Authors: Christian Trötschel; Stefan P Albaum; Daniel Wolff; Simon Schröder; Alexander Goesmann; Tim W Nattkemper; Ansgar Poetsch
Journal: Mol Cell Proteomics Date: 2012-04-06 Impact factor: 5.911

2. Kinetic cooperativity in Escherichia coli 30S ribosomal subunit reconstitution reveals additional complexity in the assembly landscape.

Authors: Anne E Bunner; Andrea H Beck; James R Williamson
Journal: Proc Natl Acad Sci U S A Date: 2010-03-05 Impact factor: 11.205

3. Subcomplexes of ancestral respiratory complex I subunits rapidly turn over in vivo as productive assembly intermediates in Arabidopsis.

Authors: Lei Li; Clark J Nelson; Chris Carrie; Ryan M R Gawryluk; Cory Solheim; Michael W Gray; James Whelan; A Harvey Millar
Journal: J Biol Chem Date: 2012-12-27 Impact factor: 5.157

Quantitative analysis of isotope distributions in proteomic mass spectrometry using least-squares Fourier transform convolution.

1. Automatic analysis of hydrogen/deuterium exchange mass spectra of peptides and proteins using calculations of isotopic distributions.

2. Accurate quantitation of protein expression and site-specific phosphorylation.

3. Proteome dynamics in complex organisms: using stable isotopes to monitor individual protein turnover rates.

4. Measurement of protein turnover rates by heavy water labeling of nonessential amino acids.

Review 5. Avian proteomics: advances, challenges and new technologies.

6. Automated extraction of backbone deuteration levels from amide H/2H mass spectrometry experiments.

7. Global internal standard technology for comparative proteomics.

8. Dissection of proteolytic 18O labeling: endoprotease-catalyzed 16O-to-18O exchange of truncated peptide substrates.

9. Absolute multiplexed quantitative analysis of protein expression during muscle development using QconCAT.

10. The Deuterator: software for the determination of backbone amide deuterium levels from H/D exchange MS data.

1. Protein turnover quantification in a multilabeling approach: from data calculation to evaluation.

2. Kinetic cooperativity in Escherichia coli 30S ribosomal subunit reconstitution reveals additional complexity in the assembly landscape.

3. Subcomplexes of ancestral respiratory complex I subunits rapidly turn over in vivo as productive assembly intermediates in Arabidopsis.

4. Systematic chromosomal deletion of bacterial ribosomal protein genes.

5. Measuring the dynamics of E. coli ribosome biogenesis using pulse-labeling and quantitative mass spectrometry.

6. Characterization of the ribosome biogenesis landscape in E. coli using quantitative mass spectrometry.

7. Reduction of translating ribosomes enables Escherichia coli to maintain elongation rates during slow growth.

8. A dominant negative mutant of the E. coli RNA helicase DbpA blocks assembly of the 50S ribosomal subunit.

9. Hydra: software for tailored processing of H/D exchange data from MS or tandem MS analyses.

10. Envelope: interactive software for modeling and fitting complex isotope distributions.