Quantitative Analysis of the Human Spindle Phosphoproteome at Distinct Mitotic Stages

During mitosis, phosphorylation of spindle associated proteins is a key regulatory mechanism for spindle formation, mitotic progression, and cytokinesis. In the recent past, mass spectrometry has been applied successfully to identify spindle proteomes and phosphoproteomes, but did not address their...

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Published inJournal of proteome research Vol. 8; no. 10; pp. 4553 - 4563
Main Authors Malik, Rainer, Lenobel, René, Santamaria, Anna, Ries, Albert, Nigg, Erich A, Körner, Roman
Format Journal Article
LanguageEnglish
Published United States American Chemical Society 01.10.2009
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Abstract During mitosis, phosphorylation of spindle associated proteins is a key regulatory mechanism for spindle formation, mitotic progression, and cytokinesis. In the recent past, mass spectrometry has been applied successfully to identify spindle proteomes and phosphoproteomes, but did not address their dynamics. Here, we present a quantitative comparison of spindle phosphoproteomes prepared from different mitotic stages. In total, we report the identification and SILAC based relative quantitation of 1940 unique phosphorylation sites and find that late mitosis (anaphase, telophase) is correlated with a drastic alteration in protein phosphorylation. Further statistical cluster analyses demonstrate a strong dependency of phosphorylation dynamics on kinase consensus patterns, thus, linking subgroups of identified phosphorylation sites to known key mitotic kinases. Surprisingly, we observed that during late mitosis strong dephosphorylation occurred on a significantly larger fraction of phospho-threonine than phospho-serine residues, suggesting a substrate preference of phosphatases for phospho-threonine at this stage. Taken together, our results constitute a large quantitative data resource of phosphorylation abundances at distinct mitotic stages and they provide insight into the systems properties of phosphorylation dynamics during mitosis.
AbstractList During mitosis, phosphorylation of spindle associated proteins is a key regulatory mechanism for spindle formation, mitotic progression, and cytokinesis. In the recent past, mass spectrometry has been applied successfully to identify spindle proteomes and phosphoproteomes, but did not address their dynamics. Here, we present a quantitative comparison of spindle phosphoproteomes prepared from different mitotic stages. In total, we report the identification and SILAC based relative quantitation of 1940 unique phosphorylation sites and find that late mitosis (anaphase, telophase) is correlated with a drastic alteration in protein phosphorylation. Further statistical cluster analyses demonstrate a strong dependency of phosphorylation dynamics on kinase consensus patterns, thus, linking subgroups of identified phosphorylation sites to known key mitotic kinases. Surprisingly, we observed that during late mitosis strong dephosphorylation occurred on a significantly larger fraction of phospho-threonine than phospho-serine residues, suggesting a substrate preference of phosphatases for phospho-threonine at this stage. Taken together, our results constitute a large quantitative data resource of phosphorylation abundances at distinct mitotic stages and they provide insight into the systems properties of phosphorylation dynamics during mitosis.
Author Lenobel, René
Ries, Albert
Malik, Rainer
Santamaria, Anna
Körner, Roman
Nigg, Erich A
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Snippet During mitosis, phosphorylation of spindle associated proteins is a key regulatory mechanism for spindle formation, mitotic progression, and cytokinesis. In...
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pubmed
acs
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StartPage 4553
SubjectTerms Cluster Analysis
Consensus Sequence
Culture Media
HeLa Cells
Humans
Mitosis - physiology
Phosphoproteins - analysis
Phosphorylation
Phosphoserine
Phosphothreonine
Phosphotransferases
Proteome - analysis
Reproducibility of Results
Spindle Apparatus - metabolism
Time Factors
Title Quantitative Analysis of the Human Spindle Phosphoproteome at Distinct Mitotic Stages
URI http://dx.doi.org/10.1021/pr9003773
https://www.ncbi.nlm.nih.gov/pubmed/19691289
https://search.proquest.com/docview/734071277
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