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Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer

Maintenance of cellular size is a fundamental systems level process that requires balancing of cell growth with proliferation. This is achieved via the cell division cycle, which is driven by the sequential accumulation and destruction of cyclins. The regulatory network around these cyclins, particu...

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Autores principales: Spiesser, Thomas W., Kühn, Clemens, Krantz, Marcus, Klipp, Edda
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4429581/
https://www.ncbi.nlm.nih.gov/pubmed/25910075
http://dx.doi.org/10.1371/journal.pcbi.1004223
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author Spiesser, Thomas W.
Kühn, Clemens
Krantz, Marcus
Klipp, Edda
author_facet Spiesser, Thomas W.
Kühn, Clemens
Krantz, Marcus
Klipp, Edda
author_sort Spiesser, Thomas W.
collection PubMed
description Maintenance of cellular size is a fundamental systems level process that requires balancing of cell growth with proliferation. This is achieved via the cell division cycle, which is driven by the sequential accumulation and destruction of cyclins. The regulatory network around these cyclins, particularly in G(1), has been interpreted as a size control network in budding yeast, and cell size as being decisive for the START transition. However, it is not clear why disruptions in the G(1) network may lead to altered size rather than loss of size control, or why the S-G(2)-M duration also depends on nutrients. With a mathematical population model comprised of individually growing cells, we show that cyclin translation would suffice to explain the observed growth rate dependence of cell volume at START. Moreover, we assess the impact of the observed bud-localisation of the G(2) cyclin CLB2 mRNA, and find that localised cyclin translation could provide an efficient mechanism for measuring the biosynthetic capacity in specific compartments: The mother in G(1), and the growing bud in G(2). Hence, iteration of the same principle can ensure that the mother cell is strong enough to grow a bud, and that the bud is strong enough for independent life. Cell sizes emerge in the model, which predicts that a single CDK-cyclin pair per growth phase suffices for size control in budding yeast, despite the necessity of the cell cycle network around the cyclins to integrate other cues. Size control seems to be exerted twice, where the G(2)/M control affects bud size through bud-localized translation of CLB2 mRNA, explaining the dependence of the S-G(2)-M duration on nutrients. Taken together, our findings suggest that cell size is an emergent rather than a regulatory property of the network linking growth and proliferation.
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spelling pubmed-44295812015-05-27 Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer Spiesser, Thomas W. Kühn, Clemens Krantz, Marcus Klipp, Edda PLoS Comput Biol Research Article Maintenance of cellular size is a fundamental systems level process that requires balancing of cell growth with proliferation. This is achieved via the cell division cycle, which is driven by the sequential accumulation and destruction of cyclins. The regulatory network around these cyclins, particularly in G(1), has been interpreted as a size control network in budding yeast, and cell size as being decisive for the START transition. However, it is not clear why disruptions in the G(1) network may lead to altered size rather than loss of size control, or why the S-G(2)-M duration also depends on nutrients. With a mathematical population model comprised of individually growing cells, we show that cyclin translation would suffice to explain the observed growth rate dependence of cell volume at START. Moreover, we assess the impact of the observed bud-localisation of the G(2) cyclin CLB2 mRNA, and find that localised cyclin translation could provide an efficient mechanism for measuring the biosynthetic capacity in specific compartments: The mother in G(1), and the growing bud in G(2). Hence, iteration of the same principle can ensure that the mother cell is strong enough to grow a bud, and that the bud is strong enough for independent life. Cell sizes emerge in the model, which predicts that a single CDK-cyclin pair per growth phase suffices for size control in budding yeast, despite the necessity of the cell cycle network around the cyclins to integrate other cues. Size control seems to be exerted twice, where the G(2)/M control affects bud size through bud-localized translation of CLB2 mRNA, explaining the dependence of the S-G(2)-M duration on nutrients. Taken together, our findings suggest that cell size is an emergent rather than a regulatory property of the network linking growth and proliferation. Public Library of Science 2015-04-24 /pmc/articles/PMC4429581/ /pubmed/25910075 http://dx.doi.org/10.1371/journal.pcbi.1004223 Text en © 2015 Spiesser et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Spiesser, Thomas W.
Kühn, Clemens
Krantz, Marcus
Klipp, Edda
Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer
title Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer
title_full Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer
title_fullStr Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer
title_full_unstemmed Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer
title_short Bud-Localization of CLB2 mRNA Can Constitute a Growth Rate Dependent Daughter Sizer
title_sort bud-localization of clb2 mrna can constitute a growth rate dependent daughter sizer
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4429581/
https://www.ncbi.nlm.nih.gov/pubmed/25910075
http://dx.doi.org/10.1371/journal.pcbi.1004223
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