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Survival lessons from stress assemblies

by Angelica Aguilera-Gomez

Institution: University Utrecht
Year: 2017
Posted: 02/01/2018
Record ID: 2154752
Full text PDF: http://dspace.library.uu.nl/handle/1874/348386;URN:NBN:NL:UI:10-1874-348386;urn:isbn:978-94-028-0572-7


Abstract

During the last decade, a novel concept of cellular architecture and organization has re-emerged with the recognition of high-order compartmentalization via non membrane-bound macromolecular structures. These membrane-less structures are in most of the cases the result of several stress conditions. The aim of this thesis is to depict the mechanisms behind the formation of Sec bodies and Stress granules in Drosophila S2 cells upon amino-acid starvation. These stress assemblies are formed as a result of the stalled of protein transport and protein translation respectively. First we investigate the behavior of ERES components upon amino-acid starvation. This nutrient stress leads to the stalling of protein secretion, which results in the formation of a novel membrane-less stress assembly that we have named the Sec body. This assembly is mainly composed of COPII proteins as well as the large scaffold protein Sec16. We demonstrate that Sec bodies are reversible, pro-survival structures with liquid droplets properties. Sec bodies act as reservoir for ERES components for the duration that this nutrient stress is taking place. Therefore, upon the relief of the stress the secretory pathway is rapidly reconstituted and functional. Post-translational modifications Mono and Poly-ADP-ribosylation have been proposed to be involved in the formation of aggregates and RNA granules. For this purpose, we designed and build specific fluorescent probes that allow us to follow these post-translational modifications in vivo. We discover that mono-ADP-ribosylation by the mono-ADP-ribose dPARP16 plays a crucial role in Sec body formation, as it modifies the Sec body component Sec16 on a very specific sequence in its Cterminus. In summary, we demonstrate that dPARP16 catalytic activity on Sec16 is a necessary and sufficient step to induce Sec body assembly and cell survival. Furthermore, we propose that Sec16 is a key factor for the stress response to amino acid starvation. Further we investigate the post-translation mechanism behind the formation of stress granules upon amino-acid starvation. We report that mono-ADP-ribosylation by dPARP16 is necessary but not sufficient for their formation. Our experimental data points also towards a role for Poly-ADP-ribosylation. In this regard, we show that the nuclear resident, poly-ADP-ribose dPARP1 plays a crucial role. Interestingly, in order to induce stress granule formation dPARP1 has to localize at the cytoplasm. Critically, dPARP1 localization out of the nucleus depends on dPARP16, possibly through the mono-ADP-ribosylation of the nuclear exporter Karyopherin beta 3. These findings provide a link between the stress responses exerted at the secretory pathway, nuclear export and the translation turnover upon nutrient stress. And as last we approach the role of Sec16 in the formation of the stress granules upon amino-acid starvation. We have identified that Sec16 plays a crucial role in stress granule formation upon this nutrient stress. Using mass spectrometry and a plasma membrane anchor-awayAdvisors/Committee Members: van Oudenaarden, Alexander, Rabouille, C.

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