Calculation of partial isotope incorporation into peptides measured by mass spectrometry

Calculation of partial isotope incorporation into peptides measured by mass spectrometry

<p>Abstract</p> <p>Background</p> <p>Stable isotope probing (SIP) technique was developed to link function, structure and activity of microbial cultures metabolizing carbon and nitrogen containing substrates to synthesize their biomass. Currently, available methods are...

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Main Authors: Harms Hauke, Seifert Jana, Richnow Hans-Hermann, Vogt Carsten, Jehmlich Nico, Fetzer Ingo, von Bergen Martin, Schmidt Frank
Format: Article
Language:English
Published: BMC 2010-06-01
Series:BMC Research Notes
Online Access:http://www.biomedcentral.com/1756-0500/3/178
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spelling doaj-50cb0bac1ebb4f9fbfa941e22c9ea1b72020-11-25T02:54:18ZengBMCBMC Research Notes1756-05002010-06-013117810.1186/1756-0500-3-178Calculation of partial isotope incorporation into peptides measured by mass spectrometryHarms HaukeSeifert JanaRichnow Hans-HermannVogt CarstenJehmlich NicoFetzer Ingovon Bergen MartinSchmidt Frank<p>Abstract</p> <p>Background</p> <p>Stable isotope probing (SIP) technique was developed to link function, structure and activity of microbial cultures metabolizing carbon and nitrogen containing substrates to synthesize their biomass. Currently, available methods are restricted solely to the estimation of fully saturated heavy stable isotope incorporation and convenient methods with sufficient accuracy are still missing. However in order to track carbon fluxes in microbial communities new methods are required that allow the calculation of partial incorporation into biomolecules.</p> <p>Results</p> <p>In this study, we use the characteristics of the so-called 'half decimal place rule' (HDPR) in order to accurately calculate the partial<sup>13</sup>C incorporation in peptides from enzymatic digested proteins. Due to the clade-crossing universality of proteins within bacteria, any available high-resolution mass spectrometry generated dataset consisting of tryptically-digested peptides can be used as reference.</p> <p>We used a freely available peptide mass dataset from <it>Mycobacterium tuberculosis </it>consisting of 315,579 entries. From this the error of estimated versus known heavy stable isotope incorporation from an increasing number of randomly drawn peptide sub-samples (100 times each; no repetition) was calculated. To acquire an estimated incorporation error of less than 5 atom %, about 100 peptide masses were needed. Finally, for testing the general applicability of our method, peptide masses of tryptically digested proteins from <it>Pseudomonas putida </it>ML2 grown on labeled substrate of various known concentrations were used and<sup>13</sup>C isotopic incorporation was successfully predicted. An easy-to-use script <abbrgrp><abbr bid="B1">1</abbr></abbrgrp> was further developed to guide users through the calculation procedure for their own data series.</p> <p>Conclusion</p> <p>Our method is valuable for estimating<sup>13</sup>C incorporation into peptides/proteins accurately and with high sensitivity. Generally, our method holds promise for wider applications in qualitative and especially quantitative proteomics.</p> http://www.biomedcentral.com/1756-0500/3/178
collection DOAJ
language English
format Article
sources DOAJ
author Harms Hauke
Seifert Jana
Richnow Hans-Hermann
Vogt Carsten
Jehmlich Nico
Fetzer Ingo
von Bergen Martin
Schmidt Frank
spellingShingle Harms Hauke
Seifert Jana
Richnow Hans-Hermann
Vogt Carsten
Jehmlich Nico
Fetzer Ingo
von Bergen Martin
Schmidt Frank
Calculation of partial isotope incorporation into peptides measured by mass spectrometry
BMC Research Notes
author_facet Harms Hauke
Seifert Jana
Richnow Hans-Hermann
Vogt Carsten
Jehmlich Nico
Fetzer Ingo
von Bergen Martin
Schmidt Frank
author_sort Harms Hauke
title Calculation of partial isotope incorporation into peptides measured by mass spectrometry
title_short Calculation of partial isotope incorporation into peptides measured by mass spectrometry
title_full Calculation of partial isotope incorporation into peptides measured by mass spectrometry
title_fullStr Calculation of partial isotope incorporation into peptides measured by mass spectrometry
title_full_unstemmed Calculation of partial isotope incorporation into peptides measured by mass spectrometry
title_sort calculation of partial isotope incorporation into peptides measured by mass spectrometry
publisher BMC
series BMC Research Notes
issn 1756-0500
publishDate 2010-06-01
description <p>Abstract</p> <p>Background</p> <p>Stable isotope probing (SIP) technique was developed to link function, structure and activity of microbial cultures metabolizing carbon and nitrogen containing substrates to synthesize their biomass. Currently, available methods are restricted solely to the estimation of fully saturated heavy stable isotope incorporation and convenient methods with sufficient accuracy are still missing. However in order to track carbon fluxes in microbial communities new methods are required that allow the calculation of partial incorporation into biomolecules.</p> <p>Results</p> <p>In this study, we use the characteristics of the so-called 'half decimal place rule' (HDPR) in order to accurately calculate the partial<sup>13</sup>C incorporation in peptides from enzymatic digested proteins. Due to the clade-crossing universality of proteins within bacteria, any available high-resolution mass spectrometry generated dataset consisting of tryptically-digested peptides can be used as reference.</p> <p>We used a freely available peptide mass dataset from <it>Mycobacterium tuberculosis </it>consisting of 315,579 entries. From this the error of estimated versus known heavy stable isotope incorporation from an increasing number of randomly drawn peptide sub-samples (100 times each; no repetition) was calculated. To acquire an estimated incorporation error of less than 5 atom %, about 100 peptide masses were needed. Finally, for testing the general applicability of our method, peptide masses of tryptically digested proteins from <it>Pseudomonas putida </it>ML2 grown on labeled substrate of various known concentrations were used and<sup>13</sup>C isotopic incorporation was successfully predicted. An easy-to-use script <abbrgrp><abbr bid="B1">1</abbr></abbrgrp> was further developed to guide users through the calculation procedure for their own data series.</p> <p>Conclusion</p> <p>Our method is valuable for estimating<sup>13</sup>C incorporation into peptides/proteins accurately and with high sensitivity. Generally, our method holds promise for wider applications in qualitative and especially quantitative proteomics.</p>
url http://www.biomedcentral.com/1756-0500/3/178
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