Your search keyword '"Ilse Hurbain"' showing total 69 results

1. A role for Dynlt3 in melanosome movement, distribution, acidity and transfer

Author

Zackie Aktary, Alejandro Conde-Perez, Florian Rambow, Mathilde Di Marco, François Amblard, Ilse Hurbain, Graça Raposo, Cédric Delevoye, Sylvie Coscoy, and Lionel Larue

Subjects

Biology (General), QH301-705.5

Abstract

Aktary et al. identify novel roles for the dynein light chain Dynlt3 in melanosome transport, maturation, and transfer to keratinocytes. They also find that the Wnt/βcatenin signalling pathway controls Dynlt3 levels and thus also contributes to the regulation of melanocyte transport and skin pigmentation.

Published

2021

2. Coupling of melanocyte signaling and mechanics by caveolae is required for human skin pigmentation

Author

Lia Domingues, Ilse Hurbain, Floriane Gilles-Marsens, Julia Sirés-Campos, Nathalie André, Melissa Dewulf, Maryse Romao, Christine Viaris de Lesegno, Anne-Sophie Macé, Cédric Blouin, Christelle Guéré, Katell Vié, Graça Raposo, Christophe Lamaze, and Cédric Delevoye

Subjects

Science

Abstract

Caveolae are plasma membrane invaginations playing crucial functions, like signal transduction and mechanoprotection. Here, the authors show that caveolae contribute to skin pigmentation by integrating the biochemical and mechanical response of epidermal melanocytes to extracellular cues.

Published

2020

3. Human Cytomegalovirus Infection Changes the Pattern of Surface Markers of Small Extracellular Vesicles Isolated From First Trimester Placental Long-Term Histocultures

Author

Mathilde Bergamelli, Hélène Martin, Mélinda Bénard, Jérôme Ausseil, Jean-Michel Mansuy, Ilse Hurbain, Maïlys Mouysset, Marion Groussolles, Géraldine Cartron, Yann Tanguy le Gac, Nathalie Moinard, Elsa Suberbielle, Jacques Izopet, Charlotte Tscherning, Graça Raposo, Daniel Gonzalez-Dunia, Gisela D’Angelo, and Cécile E. Malnou

Subjects

early placenta, extracellular vesicles, congenital infection, human cytomegalovirus, placental histoculture, Biology (General), QH301-705.5

Abstract

Extracellular vesicles (EVs) have increasingly been recognized as key players in a wide variety of physiological and pathological contexts, including during pregnancy. Notably, EVs appear both as possible biomarkers and as mediators involved in the communication of the placenta with the maternal and fetal sides. A better understanding of the physiological and pathological roles of EVs strongly depends on the development of adequate and reliable study models, specifically at the beginning of pregnancy where many adverse pregnancy outcomes have their origin. In this study, we describe the isolation of small EVs from a histoculture model of first trimester placental explants in normal conditions as well as upon infection by human cytomegalovirus. Using bead-based multiplex cytometry and electron microscopy combined with biochemical approaches, we characterized these small EVs and defined their associated markers and ultrastructure. We observed that infection led to changes in the expression level of several surface markers, without affecting the secretion and integrity of small EVs. Our findings lay the foundation for studying the functional role of EVs during early pregnancy, along with the identification of new predictive biomarkers for the severity and outcome of this congenital infection, which are still sorely lacking.

Published

2021

4. Human Cytomegalovirus Modifies Placental Small Extracellular Vesicle Composition to Enhance Infection of Fetal Neural Cells In Vitro

Author

Mathilde Bergamelli, Hélène Martin, Yann Aubert, Jean-Michel Mansuy, Marlène Marcellin, Odile Burlet-Schiltz, Ilse Hurbain, Graça Raposo, Jacques Izopet, Thierry Fournier, Alexandra Benchoua, Mélinda Bénard, Marion Groussolles, Géraldine Cartron, Yann Tanguy Le Gac, Nathalie Moinard, Gisela D’Angelo, and Cécile E. Malnou

Subjects

hCMV, congenital infection, extracellular vesicles, placenta, cytotrophoblast, Microbiology, QR1-502

Abstract

Although placental small extracellular vesicles (sEVs) are extensively studied in the context of pregnancy, little is known about their role during viral congenital infection, especially at the beginning of pregnancy. In this study, we examined the consequences of human cytomegalovirus (hCMV) infection on sEVs production, composition, and function using an immortalized human cytotrophoblast cell line derived from first trimester placenta. By combining complementary approaches of biochemistry, electron microscopy, and quantitative proteomic analysis, we showed that hCMV infection increases the yield of sEVs produced by cytotrophoblasts and modifies their protein content towards a potential proviral phenotype. We further demonstrate that sEVs secreted by hCMV-infected cytotrophoblasts potentiate infection in naive recipient cells of fetal origin, including human neural stem cells. Importantly, these functional consequences are also observed with sEVs prepared from an ex vivo model of infected histocultures from early placenta. Based on these findings, we propose that placental sEVs could be important actors favoring viral dissemination to the fetal brain during hCMV congenital infection.

Published

2022

5. The post-abscission midbody is an intracellular signaling organelle that regulates cell proliferation

Author

Eric Peterman, Paulius Gibieža, Johnathon Schafer, Vytenis Arvydas Skeberdis, Algirdas Kaupinis, Mindaugas Valius, Xavier Heiligenstein, Ilse Hurbain, Graca Raposo, and Rytis Prekeris

Subjects

Science

Abstract

The midbody is a structure found between the two dividing daughter cells that recruits regulators during cell division, but its role after cell division is poorly understood. Here, the authors find that midbodies can be internalized and send out intracellular signals to stimulate cell proliferation.

Published

2019

6. Apolipoprotein E Regulates Amyloid Formation within Endosomes of Pigment Cells

Author

Guillaume van Niel, Ptissam Bergam, Aurelie Di Cicco, Ilse Hurbain, Alessandra Lo Cicero, Florent Dingli, Roberta Palmulli, Cecile Fort, Marie Claude Potier, Leon J. Schurgers, Damarys Loew, Daniel Levy, and Graça Raposo

Subjects

Biology (General), QH301-705.5

Abstract

Accumulation of toxic amyloid oligomers is a key feature in the pathogenesis of amyloid-related diseases. Formation of mature amyloid fibrils is one defense mechanism to neutralize toxic prefibrillar oligomers. This mechanism is notably influenced by apolipoprotein E variants. Cells that produce mature amyloid fibrils to serve physiological functions must exploit specific mechanisms to avoid potential accumulation of toxic species. Pigment cells have tuned their endosomes to maximize the formation of functional amyloid from the protein PMEL. Here, we show that ApoE is associated with intraluminal vesicles (ILV) within endosomes and remain associated with ILVs when they are secreted as exosomes. ApoE functions in the ESCRT-independent sorting mechanism of PMEL onto ILVs and regulates the endosomal formation of PMEL amyloid fibrils in vitro and in vivo. This process secures the physiological formation of amyloid fibrils by exploiting ILVs as amyloid nucleating platforms.

Published

2015

7. Primary ciliogenesis requires the distal appendage component Cep123

Author

James E. Sillibourne, Ilse Hurbain, Thierry Grand-Perret, Bruno Goud, Phong Tran, and Michel Bornens

Subjects

Centriolar satellites, Centrosome, Distal appendages, Primary cilium, Science, Biology (General), QH301-705.5

Abstract

Summary Primary cilium formation is initiated at the distal end of the mother centriole in a highly co-ordinated manner. This requires the capping of the distal end of the mother centriole with a ciliary vesicle and the anchoring of the basal body (mother centriole) to the cell cortex, both of which are mediated by the distal appendages. Here, we show that the distal appendage protein Cep123 (Cep89/CCDC123) is required for the assembly, but not the maintenance, of a primary cilium. In the absence of Cep123 ciliary vesicle formation fails, suggesting that it functions in the early stages of primary ciliogenesis. Consistent with such a role, Cep123 interacts with the centriolar satellite proteins PCM-1, Cep290 and OFD1, all of which play a role in primary ciliogenesis. These interactions are mediated by a domain in the C-terminus of Cep123 (400–783) that overlaps the distal appendage-targeting domain (500–600). Together, the data implicate Cep123 as a new player in the primary ciliogenesis pathway and expand upon the role of the distal appendages in this process.

Published

2013

8. Bloom's syndrome and PICH helicases cooperate with topoisomerase IIα in centromere disjunction before anaphase.

Author

Sébastien Rouzeau, Fabrice P Cordelières, Géraldine Buhagiar-Labarchède, Ilse Hurbain, Rosine Onclercq-Delic, Simon Gemble, Laura Magnaghi-Jaulin, Christian Jaulin, and Mounira Amor-Guéret

Subjects

Medicine, Science

Abstract

Centromeres are specialized chromosome domains that control chromosome segregation during mitosis, but little is known about the mechanisms underlying the maintenance of their integrity. Centromeric ultrafine anaphase bridges are physiological DNA structures thought to contain unresolved DNA catenations between the centromeres separating during anaphase. BLM and PICH helicases colocalize at these ultrafine anaphase bridges and promote their resolution. As PICH is detectable at centromeres from prometaphase onwards, we hypothesized that BLM might also be located at centromeres and that the two proteins might cooperate to resolve DNA catenations before the onset of anaphase. Using immunofluorescence analyses, we demonstrated the recruitment of BLM to centromeres from G2 phase to mitosis. With a combination of fluorescence in situ hybridization, electron microscopy, RNA interference, chromosome spreads and chromatin immunoprecipitation, we showed that both BLM-deficient and PICH-deficient prometaphase cells displayed changes in centromere structure. These cells also had a higher frequency of centromeric non disjunction in the absence of cohesin, suggesting the persistence of catenations. Both proteins were required for the correct recruitment to the centromere of active topoisomerase IIα, an enzyme specialized in the catenation/decatenation process. These observations reveal the existence of a functional relationship between BLM, PICH and topoisomerase IIα in the centromere decatenation process. They indicate that the higher frequency of centromeric ultrafine anaphase bridges in BLM-deficient cells and in cells treated with topoisomerase IIα inhibitors is probably due not only to unresolved physiological ultrafine anaphase bridges, but also to newly formed ultrafine anaphase bridges. We suggest that BLM and PICH cooperate in rendering centromeric catenates accessible to topoisomerase IIα, thereby facilitating correct centromere disjunction and preventing the formation of supernumerary centromeric ultrafine anaphase bridges.

Published

2012

9. A role for Dynlt3 in melanosome movement, distribution, acidity and transfer

Author

Alejandro Conde-Perez, Mathilde Di Marco, Sylvie Coscoy, Cédric Delevoye, Florian Rambow, Lionel Larue, Graça Raposo, Zackie Aktary, François Amblard, Ilse Hurbain, Signalisation, radiobiologie et cancer, Institut Curie [Paris]-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Paris-Saclay-Centre National de la Recherche Scientifique (CNRS), Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Laboratoire Physico-Chimie Curie [Institut Curie] (PCC), Institut Curie [Paris]-Institut de Chimie du CNRS (INC)-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Ulsan National Institute of Science and Technology (UNIST), and Gestionnaire, Hal Sorbonne Université

Subjects

Male, QH301-705.5, [SDV]Life Sciences [q-bio], Medicine (miscellaneous), Skin Pigmentation, Melanocyte, Article, General Biochemistry, Genetics and Molecular Biology, Mice, 03 medical and health sciences, 0302 clinical medicine, DYNLT3, Cytoplasmic dynein complex, medicine, Animals, Biology (General), 030304 developmental biology, Melanosome, Organelles, 0303 health sciences, Melanosomes, Chemistry, Dynein, Wnt signaling pathway, Dyneins, Hedgehog signaling pathway, Cell biology, Mice, Inbred C57BL, Skin diseases, [SDV] Life Sciences [q-bio], medicine.anatomical_structure, Melanosome transport, Melanocytes, General Agricultural and Biological Sciences, 030217 neurology & neurosurgery, Biogenesis

Abstract

Skin pigmentation is dependent on cellular processes including melanosome biogenesis, transport, maturation and transfer to keratinocytes. However, how the cells finely control these processes in space and time to ensure proper pigmentation remains unclear. Here, we show that a component of the cytoplasmic dynein complex, Dynlt3, is required for efficient melanosome transport, acidity and transfer. In Mus musculus melanocytes with decreased levels of Dynlt3, pigmented melanosomes undergo a more directional motion, leading to their peripheral location in the cell. Stage IV melanosomes are more acidic, but still heavily pigmented, resulting in a less efficient melanosome transfer. Finally, the level of Dynlt3 is dependent on β-catenin activity, revealing a function of the Wnt/β-catenin signalling pathway during melanocyte and skin pigmentation, by coupling the transport, positioning and acidity of melanosomes required for their transfer., Aktary et al. identify novel roles for the dynein light chain Dynlt3 in melanosome transport, maturation, and transfer to keratinocytes. They also find that the Wnt/βcatenin signalling pathway controls Dynlt3 levels and thus also contributes to the regulation of melanocyte transport and skin pigmentation.

Published

2021

10. Microvilli-derived Extracellular Vesicles Govern Morphogenesis in Drosophila wing epithelium

Author

Graça Raposo, Laurent Ruel, Gisela D’Angelo, Anne-Sophie Macé, Renata Basto, Maryse Romao, Lucie Sengmanivong, Ilse Hurbain, Pascal P. Thérond, Centre de recherche de l'Institut Curie [Paris], Institut Curie [Paris], Structure and Membrane Compartments [Paris], Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), BioImaging Cell and Tissue Core Facility (PICT-IBiSA), Institut de signalisation, biologie du développement et cancer (ISBDC), Centre National de la Recherche Scientifique (CNRS)-Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Université Côte d'Azur (UCA), Institut de Biologie Valrose (IBV), Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Côte d'Azur (UCA)-Centre National de la Recherche Scientifique (CNRS), Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-Université Côte d'Azur (UCA), Compartimentation et dynamique cellulaires (CDC), Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Université Pierre et Marie Curie - Paris 6 (UPMC), COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Université Côte d'Azur (UCA), COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Côte d'Azur (UCA)-Centre National de la Recherche Scientifique (CNRS), COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015 - 2019) (COMUE UCA)-Centre National de la Recherche Scientifique (CNRS)-Université Côte d'Azur (UCA), and Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut Curie [Paris]-Centre National de la Recherche Scientifique (CNRS)

Subjects

0303 health sciences, animal structures, Chemistry, [SDV]Life Sciences [q-bio], Morphogenesis, Extracellular vesicle, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, Epithelium, Cell biology, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, embryonic structures, medicine, Secretion, Cytoskeleton, Hedgehog, 030217 neurology & neurosurgery, Biogenesis, 030304 developmental biology, Morphogen

Abstract

The regulation and coordination of developmental processes involves the secretion of morphogens and membrane carriers, including extracellular vesicles, which facilitate their transport over long distance. The long-range activity of the Hedgehog morphogen is conveyed by extracellular vesicles. However, the site and the molecular basis of their biogenesis remains unknown. By combining fluorescence and electron microscopy combined with genetics and cell biology approaches, we investigated the origin and the cellular mechanisms underlying extracellular vesicle biogenesis, and their contribution to Drosophila wing disc development, exploiting Hedgehog as a long-range morphogen. We show that microvilli of Drosophila wing disc epithelium are the site of generation of small extracellular vesicles that transport Hedgehog across the tissue. This process requires the Prominin-like protein, whose activity, together with interacting cytoskeleton components and lipids, is critical for maintaining microvilli integrity and function in secretion. Our results provide the first evidence that microvilli-derived extracellular vesicles contribute to Hedgehog long-range signaling activity highlighting their physiological significance in tissue development in vivo.

Published

2021

11. PI4P and BLOC-1 remodel endosomal membranes into tubules

Author

Daniel Lévy, Feng-Ching Tsai, Daniel Hamaoui, Sílvia Vale-Costa, Maria João Amorim, Aurélie Di Cicco, Yueyao Zhu, Anne-Sophie Macé, Tal Keren-Kaplan, Mathilde Dimarco, Cédric Delevoye, Patricia Bassereau, Ilse Hurbain, Juan S. Bonifacino, Michael S. Marks, Agathe Subtil, Riddhi Atul Jani, Graça Raposo, Laboratoire Physico-Chimie Curie [Institut Curie] (PCC), Institut Curie [Paris]-Institut de Chimie du CNRS (INC)-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Biologie cellulaire de l'Infection microbienne - Cellular Biology of Microbial Infection, Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS)-Université Paris Cité (UPCité), and Veritati - Repositório Institucional da Universidade Católica Portuguesa

Subjects

Endosome, Physiology, Membrane lipids, Phospholipid, Biophysics, Endosomes, [SDV.BC.BC]Life Sciences [q-bio]/Cellular Biology/Subcellular Processes [q-bio.SC], [SDV.BC]Life Sciences [q-bio]/Cellular Biology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Phosphatidylinositol Phosphates, Organelle, 030304 developmental biology, Organelles, 0303 health sciences, Chemistry, Intracellular parasite, Cell Membrane, Intracellular Signaling Peptides and Proteins, Intracellular Membranes, Cell Biology, Cell biology, [SDV.BBM.BP]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Biophysics, Protein Transport, Membrane, Lysosomes, [PHYS.COND.CM-SCM]Physics [physics]/Condensed Matter [cond-mat]/Soft Condensed Matter [cond-mat.soft], 030217 neurology & neurosurgery, Biogenesis, Intracellular, Membrane and lipid biology

Abstract

International audience; The endosomal sorting complexes required for transport (ESCRT) system is an ancient and ubiquitous membrane scission machinery that catalyzes the budding and scission of membranes. ESCRT-mediated scission events, exemplified by those involved in the budding of HIV-1, are usually directed away from the cytosol (“reverse topology”), but they can also be directed toward the cytosol (“normal topology”). The ESCRT-III subunits CHMP1B and IST1 can coat and constrict positively curved membrane tubes, suggesting that these subunits could catalyze normal topology membrane severing. CHMP1B and IST1 bind and recruit the microtubule-severing AAA + ATPase spastin, a close relative of VPS4, suggesting that spastin could have a VPS4-like role in normal-topology membrane scission. Here, we reconstituted the process in vitro using membrane nanotubes pulled from giant unilamellar vesicles using an optical trap in order to determine whether CHMP1B and IST1 are capable of membrane severing on their own or in concert with VPS4 or spastin. CHMP1B and IST1 copolymerize on membrane nanotubes, forming stable scaffolds that constrict the tubes, but do not, on their own, lead to scission. However, CHMP1B–IST1 scaffolded tubes were severed when an additional extensional force was applied, consistent with a friction-driven scission mechanism. We found that spastin colocalized with CHMP1B-enriched sites but did not disassemble the CHMP1B–IST1 coat from the membrane. VPS4 resolubilized CHMP1B and IST1 without leading to scission. These observations show that the CHMP1B–IST1 ESCRT-III combination is capable of severing membranes by a friction-driven mechanism that is independent of VPS4 and spastin.

Published

2021

12. Human Cytomegalovirus modifies placental small extracellular vesicle secretion and composition towards a proviral phenotype to enhance infection of fetal recipient cells

Author

Géraldine Cartron, Thierry Fournier, Melinda Benard, Graça Raposo, Jacques Izopet, Nathalie Moinard, Marion Groussolles, Hélène Martin, Jean-Michel Mansuy, Alexandra Benchoua, Y. Aubert, Y. Tanguy le Gac, Gisela D’Angelo, Cécile E. Malnou, Ilse Hurbain, M. Marcellin, Mathilde Bergamelli, and O. Burlet-Schiltz

Subjects

Human cytomegalovirus, Fetus, Cytotrophoblast, viruses, virus diseases, Context (language use), Extracellular vesicle, Biology, medicine.disease, Virology, medicine.anatomical_structure, Cell culture, Placenta, medicine, Cytotrophoblasts

Abstract

Although placental small extracellular vesicles (sEVs) are extensively studied in the context of pregnancy, little is known about their role during human cytomegalovirus (hCMV) congenital infection, especially at the beginning of pregnancy. In this study, we examined the consequences of hCMV infection on sEVs production, composition and function using an immortalized human cytotrophoblast cell line derived from first trimester placenta. By combining complementary approaches of biochemistry, electron microscopy and quantitative proteomic analysis, we showed that hCMV infection increases the yield of sEVs produced by cytotrophoblasts and modifies their protein content towards a proviral phenotype. We further demonstrate that sEVs secreted by hCMV-infected cytotrophoblasts potentiate infection in naive recipient cells of fetal origin, including human neural stem cells. Importantly, these functional consequences are also observed with sEVs prepared from either anex vivomodel of infected histocultures from early placenta or from the amniotic fluid of patients naturally infected by hCMV at the beginning of pregnancy. Based on these findings, we propose that placental sEVs could be key actors favoring viral dissemination to the fetal brain during hCMV congenital infection.Significance StatementHuman cytomegalovirus (hCMV) infection is a major issue during pregnancy, affecting 1% of births in western countries. Despite extensive research, the pathophysiology of this congenital infection remains unclear. Recently, increasing evidence point to the key role of placental small extracellular vesicles (sEVs) in materno-fetal communication during pregnancy. Here, we examined the impact of hCMV infection on the protein composition and function of placental sEVs. We observe that hCMV infection leads to major changes in placental sEV protein content. Functional studies show the ability of sEVs produced by placental infected cells to facilitate further infection of naive recipient fetal cells, notably human neural stem cells. Our study demonstrates that placental sEVs are key players of hCMV pathophysiology during congenital infection.

Published

2021

13. Catabolism of lysosome-related organelles in color-changing spiders supports intracellular turnover of pigments

Author

Cédric Delevoye, Graça Raposo, Andrea Somogyi, Xavier Heiligenstein, Kadda Medjoubi, Jérôme Casas, Arnaud Lanoue, Ilse Hurbain, Sylvain Trépout, Florent Figon, Institut de recherche sur la biologie de l'insecte UMR7261 (IRBI), Université de Tours (UT)-Centre National de la Recherche Scientifique (CNRS), Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), CryoCapCell, Institut Curie [Paris], Biomolécules et biotechnologies végétales (BBV EA 2106), Université de Tours (UT), Synchrotron SOLEIL (SSOLEIL), Centre National de la Recherche Scientifique (CNRS), Université de Tours-Centre National de la Recherche Scientifique (CNRS), and Université de Tours

Subjects

food.ingredient, [SDV]Life Sciences [q-bio], Color, Context (language use), [SDV.BC.BC]Life Sciences [q-bio]/Cellular Biology/Subcellular Processes [q-bio.SC], Endosomes, 03 medical and health sciences, 0302 clinical medicine, food, Organelle, Crab spiders, Animals, Ommochrome, 030304 developmental biology, Melanosome, Skin, Organelles, 0303 health sciences, Multidisciplinary, Melanosomes, Catabolism, Chemistry, Spiders, Pigments, Biological, Biological Sciences, Cell biology, Pigment granule, Ultrastructure, sense organs, Lysosomes, 030217 neurology & neurosurgery

Abstract

International audience; Pigment organelles of vertebrates belong to the lysosome-related organelle (LRO) family, of which melanin-producing melanosomes are the prototypes. While their anabolism has been extensively unraveled through the study of melanosomes in skin melanocytes, their catabolism remains poorly known. Here, we tap into the unique ability of crab spiders to reversibly change body coloration to examine the catabolism of their pigment organelles. By combining ultrastructural and metal analyses on high-pressure frozen integuments, we first assess whether pigment organelles of crab spiders belong to the LRO family and second, how their catabolism is intracellularly processed. Using scanning transmission electron microscopy, electron tomography, and nanoscale Synchrotron-based scanning X-ray fluorescence, we show that pigment organelles possess ultrastructural and chemical hallmarks of LROs, including intraluminal vesicles and metal deposits, similar to melanosomes. Monitoring ultrastructural changes during bleaching suggests that the catabolism of pigment organelles involves the degradation and removal of their intraluminal content, possibly through lysosomal mechanisms. In contrast to skin melanosomes, anabolism and catabolism of pigments proceed within the same cell without requiring either cell death or secretion/phagocytosis. Our work hence provides support for the hypothesis that the endolysosomal system is fully functionalized for within-cell turnover of pigments, leading to functional maintenance under adverse conditions and phenotypic plasticity. First formulated for eye melanosomes in the context of human vision, the hypothesis of intracellular turnover of pigments gets unprecedented strong support from pigment organelles of spiders.

Published

2021

14. Catabolism of lysosome-related organelles in color-changing spiders supports intracellular turnover of pigments

Author

Andrea Somogyi, Kadda Medjoubi, Graça Raposo, Jérôme Casas, Xavier Heiligenstein, Sylvain Trépout, Cédric Delevoye, Florent Figon, and Ilse Hurbain

Subjects

food.ingredient, food, Catabolism, Chemistry, Vesicle, Organelle, Ultrastructure, Crab spiders, Context (language use), sense organs, Intracellular, Cell biology, Melanosome

Abstract

Pigment organelles of vertebrates belong to the lysosome-related organelle (LRO) family, of which melanin-producing melanosomes are the prototypes. While their anabolism has been extensively unraveled through the study of melanosomes in skin melanocytes, their catabolism remains poorly known. Here, we tap into the unique ability of crab spiders to reversibly change body coloration to examine the catabolism of their pigment organelles. By combining ultrastructural and metal analyses on high-pressure frozen integuments, we first assess whether pigment organelles of crab spiders belong to the LRO family and, second, how their catabolism is intracellularly processed. Using scanning-transmission electron microscopy, electron tomography and nanoscale Synchrotron-based scanning X-ray fluorescence, we show that pigment organelles possess ultrastructural and chemical hallmarks of LROs, including intraluminal vesicles and metal deposits, similar to melanosomes. Monitoring ultrastructural changes during bleaching suggests that the catabolism of pigment organelles involves the degradation and removal of their intraluminal content, possibly through lysosomal mechanisms. In contrast to skin melanosomes, anabolism and catabolism of pigments proceed within the same cell without requiring either cell death or secretion/phagocytosis. Our work hence provides support for the hypothesis that the endolysosomal system is fully functionalized for within-cell turnover of pigments, leading to functional maintenance under adverse conditions and phenotypic plasticity. First formulated for eye melanosomes in the context of human vision, the hypothesis of intracellular turnover of pigments gets unprecedented strong support from pigment organelles of spiders.

Published

2021

15. Dynlt3, a novel fundamental regulator of melanosome movement, distribution, maturation and transfer

Author

Graça Raposo, Mathilde Di Marco, François Amblard, Zackie Aktary, Alejandro Conde-Perez, Ilse Hurbain, Cédric Delevoye, Lionel Larue, Sylvie Coscoy, and Florian Rambow

Subjects

medicine.anatomical_structure, Chemistry, Melanosome transport, DYNLT3, Cytoplasmic dynein complex, Wnt signaling pathway, medicine, Melanocyte, Hedgehog signaling pathway, Biogenesis, Cell biology, Melanosome

Abstract

Skin pigmentation is dependent on cellular processes including melanosome biogenesis, transport, maturation and transfer to keratinocytes. However, how the cells finely control these processes in space and time to ensure proper pigmentation remains unclear. Here, we show that a component of the cytoplasmic dynein complex, Dynlt3, is required for efficient melanosome transport, maturation and transfer. In melanocytes with decreased levels of Dynlt3, pigmented melanosomes undergo a more directional (convective) motion leading to their peripheral location in the cell, and are not fully matured. Stage IV melanosomes are more acidic, but still heavily pigmented, resulting in a less efficient melanosome transfer. Finally, the level of Dynlt3 is dependent on β-catenin activity, revealing a novel function of the Wnt/β-catenin signalling pathway during melanocyte and skin pigmentation, by coupling the transport, position and maturation of melanosomes required for their transfer.

Published

2021

16. Human cytomegalovirus infection changes the pattern of surface markers of small extracellular vesicles isolated from first trimester placental histocultures

Author

Maïlys Mouysset, Jérôme Ausseil, Yann Tanguy le Gac, Jean-Michel Mansuy, Elsa Suberbielle, Jacques Izopet, Géraldine Cartron, Marion Groussolles, Graça Raposo, Hélène Martin, Daniel Gonzalez-Dunia, Cécile E. Malnou, Melinda Benard, Charlotte Tscherning, Nathalie Moinard, Mathilde Bergamelli, Ilse Hurbain, and Gisela D’Angelo

Subjects

Human cytomegalovirus, 0303 health sciences, Pregnancy, 030219 obstetrics & reproductive medicine, business.industry, viruses, virus diseases, respiratory system, medicine.disease, Extracellular vesicles, 3. Good health, 03 medical and health sciences, First trimester, 0302 clinical medicine, Immunology, medicine, Multiplex, Secretion, business, Pathological, Cytometry, 030304 developmental biology

Abstract

Currently, research on the use of non-invasive biomarkers as diagnosis and prognosis tools during pathological pregnancies is in full development. Among these, placenta-derived small extracellular vesicles (sEVs) are considered as serious candidates, since their composition is modified during many pregnancy pathologies. Moreover, sEVs are found in maternal serum and can thus be easily purified from a simple blood sample. In this study, we describe the isolation of sEVs from a histoculture model of first trimester placental explants. Using bead-based multiplex cytometry and electron microscopy combined with biochemical approaches, we characterized these sEVs and defined their associated markers and ultrastructure. We next examined the consequences of infection by human cytomegalovirus on sEVs secretion and characteristics. We observed that infection led to increased levels of expression of several surface markers, without any impact on the secretion and integrity of sEVs. Our findings open the prospect for the identification of new predictive biomarkers for the severity and outcome of this congenital infection early during pregnancy, which are still sorely lacking.

Published

2020

17. Coupling of melanocyte signaling and mechanics by caveolae is required for human skin pigmentation

Author

Anne-Sophie Macé, Katell Vié, Cédric M. Blouin, Christelle Guéré, Lia Domingues, Graça Raposo, Julia Sirés-Campos, Christophe Lamaze, Floriane Gilles-Marsens, Melissa Dewulf, Ilse Hurbain, Maryse Romao, Christine Viaris de Lesegno, Cédric Delevoye, Nathalie André, Structure and Membrane Compartments [Paris], Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), BioImaging Cell and Tissue Core Facility (PICT-IBiSA), Institut Curie [Paris], Génétique et Neurobiologie de C. Elegans [Lyon], Institut NeuroMyoGène (INMG), Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM), Laboratoire Clarins [Pontoise], Chimie biologique des membranes et ciblage thérapeutique (CBMCT - UMR 3666 / U1143), Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Institut National de la Santé et de la Recherche Médicale (INSERM)-Institut de Chimie du CNRS (INC), We acknowledge the Nikon Imaging Center at the Institut Curie/Centre National de la Recherche Scientifique and the PICT-IBiSA, a member of the France-BioImaging national research infrastructure (ANR-10-INBS-04). This work has received support under the program 'Investissement d’Avenir' launched by the French Government and implemented by the Agence Nationale de la Recherche (ANR) with the references ANR-10-LBX-0038 and ANR-10-IDEX-0001-02 PSL, Fondation pour la Recherche Médicale (Equipe FRM DEQ20140329491 Team label to G.R.), Agence Nationale de la Recherche ('MOTICAV' ANR-17-CE13-0020-01 to C.L., and 'MYOACTIONS' ANR-17-CE11-0029-03 to C.D.), Fondation ARC pour la Recherche sur le Cancer (PJA20161204965 to C.D., and Programme Labellisé PGA1-RF20170205456 to C.L.). This work received support from the grants ANR-11-LABX-0038, ANR-10-IDEX-0001-02 (Labex CelTisPhyBio to L.D.), Groupe Clarins, Institut Curie, CNRS and INSERM., ANR-10-INBS-0004,France-BioImaging,Développment d'une infrastructure française distribuée coordonnée(2010), ANR-10-IDEX-0001,PSL,Paris Sciences et Lettres(2010), ANR-17-CE13-0020,MOTICAV,Cavéoles et Tension Membranaire dans la Migration Cellulaire(2017), ANR-17-CE11-0029,MyoActions,Rôle des partenaires pour définir la fonction cellulaire de la myosine VI(2017), Bodescot, Myriam, Développment d'une infrastructure française distribuée coordonnée - - France-BioImaging2010 - ANR-10-INBS-0004 - INBS - VALID, Initiative d'excellence - Paris Sciences et Lettres - - PSL2010 - ANR-10-IDEX-0001 - IDEX - VALID, Cavéoles et Tension Membranaire dans la Migration Cellulaire - - MOTICAV2017 - ANR-17-CE13-0020 - AAPG2017 - VALID, Rôle des partenaires pour définir la fonction cellulaire de la myosine VI - - MyoActions2017 - ANR-17-CE11-0029 - AAPG2017 - VALID, Université de Lyon-Université de Lyon-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS), and Institut Curie [Paris]-Institut National de la Santé et de la Recherche Médicale (INSERM)-Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)

Subjects

0301 basic medicine, Keratinocytes, Cell signaling, Ultraviolet Rays, Science, Caveolin 1, General Physics and Astronomy, Human skin, Skin Pigmentation, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, Cell Communication, Melanocyte, Caveolae, General Biochemistry, Genetics and Molecular Biology, Article, Melanin, 03 medical and health sciences, 0302 clinical medicine, Downregulation and upregulation, Microscopy, Electron, Transmission, medicine, Humans, lcsh:Science, [SDV.BC] Life Sciences [q-bio]/Cellular Biology, Tissue homeostasis, Cells, Cultured, Skin, Multidisciplinary, Epidermis (botany), integumentary system, Chemistry, General Chemistry, Coculture Techniques, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Epidermal Cells, Microscopy, Fluorescence, 030220 oncology & carcinogenesis, Cell polarity, Melanocytes, lcsh:Q, sense organs, Epidermis, Cell signalling, HeLa Cells, Signal Transduction

Abstract

Tissue homeostasis requires regulation of cell–cell communication, which relies on signaling molecules and cell contacts. In skin epidermis, keratinocytes secrete factors transduced by melanocytes into signaling cues promoting their pigmentation and dendrite outgrowth, while melanocytes transfer melanin pigments to keratinocytes to convey skin photoprotection. How epidermal cells integrate these functions remains poorly characterized. Here, we show that caveolae are asymmetrically distributed in melanocytes and particularly abundant at the melanocyte–keratinocyte interface in epidermis. Caveolae in melanocytes are modulated by ultraviolet radiations and keratinocytes-released factors, like miRNAs. Preventing caveolae formation in melanocytes increases melanin pigment synthesis through upregulation of cAMP signaling and decreases cell protrusions, cell–cell contacts, pigment transfer and epidermis pigmentation. Altogether, we identify that caveolae serve as molecular hubs that couple signaling outputs from keratinocytes to mechanical plasticity of pigment cells. The coordination of intercellular communication and contacts by caveolae is thus crucial to skin pigmentation and tissue homeostasis., Caveolae are plasma membrane invaginations playing crucial functions, like signal transduction and mechanoprotection. Here, the authors show that caveolae contribute to skin pigmentation by integrating the biochemical and mechanical response of epidermal melanocytes to extracellular cues.

Published

2020

18. Microvilli-derived extracellular vesicles carry Hedgehog morphogenic signals for Drosophila wing imaginal disc development

Author

Ilse Hurbain, Anne-Sophie Macé, Maryse Romao, Elodie Prince, Lucie Sengmanivong, Laurent Ruel, Renata Basto, Pascal P. Thérond, Graça Raposo, Gisela D’Angelo, Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Structure and Membrane Compartments [Paris], Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Institut de Biologie Valrose (IBV), Université Nice Sophia Antipolis (... - 2019) (UNS), COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Côte d'Azur (UCA)-Centre National de la Recherche Scientifique (CNRS), Institut de signalisation, biologie du développement et cancer (ISBDC), Centre National de la Recherche Scientifique (CNRS)-Université Nice Sophia Antipolis (... - 2019) (UNS), and COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-COMUE Université Côte d'Azur (2015-2019) (COMUE UCA)-Université Côte d'Azur (UCA)

Subjects

0303 health sciences, Microvilli, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, General Biochemistry, Genetics and Molecular Biology, Extracellular Vesicles, 03 medical and health sciences, Drosophila melanogaster, 0302 clinical medicine, Imaginal Discs, [SDV.BC.IC]Life Sciences [q-bio]/Cellular Biology/Cell Behavior [q-bio.CB], Morphogenesis, Animals, Drosophila Proteins, Wings, Animal, Drosophila, Hedgehog Proteins, AC133 Antigen, General Agricultural and Biological Sciences, [SDV.BDD]Life Sciences [q-bio]/Development Biology, ComputingMilieux_MISCELLANEOUS, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Morphogens are secreted molecules that regulate and coordinate major developmental processes, such as cell differentiation and tissue morphogenesis. Depending on the mechanisms of secretion and the nature of their carriers, morphogens act at short and long range. We investigated the paradigmatic long-range activity of Hedgehog (Hh), a well-known morphogen, and its contribution to the growth and patterning of the Drosophila wing imaginal disc. Extracellular vesicles (EVs) contribute to Hh long-range activity; however, the nature, the site, and the mechanisms underlying the biogenesis of these vesicular carriers remain unknown. Here, through the analysis of mutants and a series of Drosophila RNAi-depleted wing imaginal discs using fluorescence and live-imaging electron microscopy, including tomography and 3D reconstruction, we demonstrate that microvilli of the wing imaginal disc epithelium are the site of generation of small EVs that transport Hh across the tissue. Further, we show that the Prominin-like (PromL) protein is critical for microvilli integrity. Together with actin cytoskeleton and membrane phospholipids, PromL maintains microvilli architecture that is essential to promote its secretory function. Importantly, the distribution of Hh to microvilli and its release via these EVs contribute to the proper morphogenesis of the wing imaginal disc. Our results demonstrate that microvilli-derived EVs are carriers for Hh long-range signaling in vivo. By establishing that members of the Prominin protein family are key determinants of microvilli formation and integrity, our findings support the view that microvilli-derived EVs conveying Hh may provide a means for exchanging signaling cues of high significance in tissue development and cancer.

Published

2022

19. Replacement and desmoplastic histopathological growth patterns: A pilot study of prediction of outcome in patients with uveal melanoma liver metastases

Author

Sofie Daelemans, Sophie Gardrat, Sergio Roman-Roman, Claire Lugassy, Nathalie Cassoux, Gaëlle Pierron, Rémi Dendale, Raymond L. Barnhill, Sophie Piperno-Neumann, André Nicolas, Graça Raposa, Peter A. van Dam, Laurence Desjardins, Peter B. Vermeulen, Ilse Hurbain, Vincent Servois, and Pascale Mariani

Subjects

0301 basic medicine, medicine.medical_specialty, Monosomy, business.industry, Melanoma, medicine.medical_treatment, Enucleation, Hazard ratio, medicine.disease, Gastroenterology, Pathology and Forensic Medicine, Metastasis, Radiation therapy, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, 030220 oncology & carcinogenesis, Internal medicine, medicine, Stage (cooking), Breast carcinoma, business

Abstract

Up to 50% of uveal melanomas (UM) metastasise to the liver within 10 years of diagnosis, and these almost always prove rapidly fatal. As histopathological growth patterns (HGPs) of liver metastases of the replacement and desmoplastic type, particularly from colon and breast carcinoma, may import valuable biological and prognostic information, we have studied HGP in a series of 41 UM liver metastases originating from 41 patients from the period 2006-2017. Twenty patients underwent enucleation while 21 had radiation therapy. Analysis of UM by array comparative genomic hybridisation revealed: 25 (64%) patients with high risk (monosomy3/8q gain); 13 (33%) intermediate risk (M3/8normal or disomy3/8q gain); and 1 low risk (disomy3/8normal). The principal HGP was replacement in 30 (73%) cases and desmoplastic in 11 (27%) cases. Cases with replacement demonstrated striking vascular co-option/angiotropism. With the development of liver metastasis, only the replacement pattern, largest primary tumour diameter, and R2 (incomplete resection) status predicted diminished overall survival (OS; p < 0.041, p < 0.017, p < 0.047, respectively). On multivariate analysis, only HGP (hazard ratio; HR = 6.51, p = 0.008) and resection status remained significant. The genomic high-risk variable had no prognostic value at this stage of liver metastasis. Chi-square test showed no association of HGP with monosomy 3 or 8q gain. Eighteen of 41 (44%) patients are alive with disease and 23 (56%) patients died with follow-up ranging from 12 to 318 months (mean: 70 months, median: 47 months). In conclusion, we report for the first time the frequency of the replacement and desmoplastic HGPs in liver UM metastases resected from living patients, and their potential important prognostic value for UM patients, as in other solid cancers. These results may potentially be utilised to develop radiological correlates and therapeutic targets for following and treating patients with UM metastases.

Published

2018

20. Melanosome Distribution in Keratinocytes in Different Skin Types: Melanosome Clusters Are Not Degradative Organelles

Author

Graça Raposo, Maryse Romao, Céline Marchal, Françoise Bernerd, Ilse Hurbain, Peggy Sextius, Christine Duval, and Emilie Bourreau

Subjects

Adult, Keratinocytes, 0301 basic medicine, Skin Pigmentation, Human skin, Dermatology, Biology, Biochemistry, law.invention, 03 medical and health sciences, law, Organelle, medicine, Humans, Molecular Biology, Cellular compartment, Melanosome, Organelles, Melanosomes, integumentary system, Endoplasmic reticulum, Autophagosomes, Cell Biology, Immunogold labelling, Cell biology, Microscopy, Electron, 030104 developmental biology, medicine.anatomical_structure, Female, Epidermis, Electron microscope

Abstract

The melanosome pattern was characterized systematically in keratinocytes in situ in highly, moderately, and lightly pigmented human skin, classified according to the individual typological angle, a colorimetric measure of skin color phenotype. Electron microscopy of skin samples showed qualitatively and quantitatively that in highly pigmented skin, although melanosomes are mostly isolated and distributed throughout the entire epidermis, clusters are also observed in the basal layer. In moderately and lightly pigmented skin, melanosomes are concentrated in the first layer of the epidermis, isolated-but for most of them, grouped as clusters of melanocores delimited by a single membrane. Electron tomography resolving intracellular three-dimensional organization of organelles showed that clustered melanocores depict contacts with other cellular compartments, such as endoplasmic reticulum and mitochondria. Additionally, immunogold labelling showed that clusters of melanocores do not correspond to autophagosomes or melanophagosomes but that they present, similarly to melanosomes in melanocytes, features of nonacidic, nondegradative organelles. Overall, these observations suggest that melanocore clusters do not correspond to autophagic organelles but represent reservoirs or protective structures for melanosome integrity and function. These results open avenues for understanding the basis of skin pigmentation in different skin color phenotypes.

Published

2018

21. Caveolae coupling of melanocytes signaling and mechanics is required for human skin pigmentation

Author

Floriane Gilles-Marsens, Cédric M. Blouin, Katell Vié, Graça Raposo, Christine Viaris de Lesegno, Christophe Lamaze, Cédric Delevoye, Ilse Hurbain, Lia Domingues, Maryse Romao, Christelle Guéré, Melissa Dewulf, and Nathalie André

Subjects

0303 health sciences, Cell signaling, Epidermis (botany), integumentary system, Chemistry, Cell, Human skin, Cell biology, Melanin, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, Caveolae, medicine, sense organs, 030217 neurology & neurosurgery, Tissue homeostasis, Intracellular, 030304 developmental biology

Abstract

SummaryTissue homeostasis requires regulation of cell-cell communication, which relies on signaling molecules and cell contacts. In skin epidermis, keratinocytes secrete specific factors transduced by melanocytes into signaling cues to promote their pigmentation and dendrite outgrowth, while melanocytes transfer melanin pigments to keratinocytes to convey skin photoprotection. How epidermal cells integrate these functions remains poorly characterized. Here, we found that caveolae polarize in melanocytes and are particularly abundant at melanocyte-keratinocyte interface. Caveolae in melanocytes are sensitive to ultra-violet radiations and miRNAs released by keratinocytes. Preventing caveolae formation in melanocytes results in increased production of intracellular cAMP and melanin pigments, but decreases cell protrusions, cell-cell contacts, pigment transfer and epidermis pigmentation. Altogether, our data establish that, in melanocytes, caveolae serve as key molecular hubs that couple signaling outputs from keratinocytes to mechanical plasticity. This process is crucial to maintain cell-cell contacts and intercellular communication, skin pigmentation and tissue homeostasis.

Published

2019

22. Correction: The PIKfyve complex regulates the early melanosome homeostasis required for physiological amyloid formation (doi:10.1242/jcs.229500)

Author

Guillaume van Niel, Miriam H. Meisler, Graça Raposo, Xavier Heiligenstein, Christin Bissig, Ragna Sannerud, Emily Kaufman, Guy M. Lenk, Ilse Hurbain, Pauline Croisé, Wim Annaert, and Lois S. Weisman

Subjects

0303 health sciences, Amyloid, Cell, Cell Biology, Biology, Cell biology, Blot, 03 medical and health sciences, PIKFYVE, 0302 clinical medicine, Image presentation, medicine.anatomical_structure, medicine, 030217 neurology & neurosurgery, Homeostasis, 030304 developmental biology, Melanosome, Research Article

Abstract

The metabolism of PI(3,5)P2 is regulated by the PIKfyve, VAC14 and FIG4 complex, mutations in which are associated with hypopigmentation in mice. These pigmentation defects indicate a key, but as yet unexplored, physiological relevance of this complex in the biogenesis of melanosomes. Here, we show that PIKfyve activity regulates formation of amyloid matrix composed of PMEL protein within the early endosomes in melanocytes, called stage I melanosomes. PIKfyve activity controls the membrane remodeling of stage I melanosomes, which regulates PMEL abundance, sorting and processing. PIKfyve activity also affects stage I melanosome kiss-and-run interactions with lysosomes, which are required for PMEL amyloidogenesis and the establishment of melanosome identity. Mechanistically, PIKfyve activity promotes both the formation of membrane tubules from stage I melanosomes and their release by modulating endosomal actin branching. Taken together, our data indicate that PIKfyve activity is a key regulator of the melanosomal import–export machinery that fine tunes the formation of functional amyloid fibrils in melanosomes and the maintenance of melanosome identity. This article has an associated First Person interview with the first author of the paper.

Published

2019

23. The PIKfyve complex regulates the early melanosome homeostasis required for physiological amyloid formation

Author

Guy M. Lenk, Graça Raposo, Lois S. Weisman, Miriam H. Meisler, Wim Annaert, Ilse Hurbain, Emily Kaufman, Ragna Sannerud, Xavier Heiligenstein, Christin Bissig, Guillaume van Niel, Pauline Croisé, Départment of Biochemistry, Université de Genève (UNIGE), Équipe 'Rythme, vie et mort de la rétine', Institut des Neurosciences Cellulaires et Intégratives (INCI), Université de Strasbourg (UNISTRA)-Centre National de la Recherche Scientifique (CNRS)-Université de Strasbourg (UNISTRA)-Centre National de la Recherche Scientifique (CNRS), Compartimentation et dynamique cellulaires (CDC), Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Université Pierre et Marie Curie - Paris 6 (UPMC), Biology of Myelin Unit, San Raffaele Scientific Institute, Laboratory of Membrane Trafficking and VIB11, Center for Human Genetics, Catholic University of Leuven - Katholieke Universiteit Leuven (KU Leuven), Department of Human Genetics, University of Michigan [Ann Arbor], University of Michigan System-University of Michigan System, Life Science Institute, Institut Curie-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), and Centre National de la Recherche Scientifique (CNRS)-Institut Curie-Université Pierre et Marie Curie - Paris 6 (UPMC)

Subjects

BLOC-1, SORTING SIGNAL, [SDV]Life Sciences [q-bio], PROTEIN, Retinal Pigment Epithelium, [SDV.BC.BC]Life Sciences [q-bio]/Cellular Biology/Subcellular Processes [q-bio.SC], Phosphoinositide, PHOSPHATIDYLINOSITOL 3,5-BISPHOSPHATE, ACTIN DYNAMICS, Mice, Phosphatidylinositol 3-Kinases, PI(3,5)P-2, PIKFYVE, 0302 clinical medicine, Homeostasis, LYSOSOMES, Cells, Cultured, Mice, Knockout, 0303 health sciences, Melanosomes, Intracellular Signaling Peptides and Proteins, FIG4, ENDOSOMES, Lysosome, Cell biology, PMEL, Protein Transport, medicine.anatomical_structure, Melanocytes, Phosphoinositide Phosphatases, Life Sciences & Biomedicine, gp100 Melanoma Antigen, Melanosome, Amyloid, Endosome, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, Biology, 03 medical and health sciences, medicine, Animals, Actin, 030304 developmental biology, Science & Technology, Flavoproteins, PI(3,5)P2, Membrane Proteins, Correction, Cell Biology, PIKfyve, TRANSPORT, VAC14, Lysosomes, 030217 neurology & neurosurgery, Biogenesis

Abstract

The metabolism of PI(3,5)P2 is regulated by the PIKfyve, VAC14 and FIG4 complex, mutations in which are associated with hypopigmentation in mice. These pigmentation defects indicate a key, but as yet unexplored, physiological relevance of this complex in the biogenesis of melanosomes. Here, we show that PIKfyve activity regulates formation of amyloid matrix composed of PMEL protein within the early endosomes in melanocytes, called stage I melanosomes. PIKfyve activity controls the membrane remodeling of stage I melanosomes, which regulates PMEL abundance, sorting and processing. PIKfyve activity also affects stage I melanosome kiss-and-run interactions with lysosomes, which are required for PMEL amyloidogenesis and the establishment of melanosome identity. Mechanistically, PIKfyve activity promotes both the formation of membrane tubules from stage I melanosomes and their release by modulating endosomal actin branching. Taken together, our data indicate that PIKfyve activity is a key regulator of the melanosomal import-export machinery that fine tunes the formation of functional amyloid fibrils in melanosomes and the maintenance of melanosome identity.This article has an associated First Person interview with the first author of the paper. ispartof: JOURNAL OF CELL SCIENCE vol:132 issue:5 ispartof: location:England status: published

Published

2019

24. The post-abscission midbody is an intracellular signaling organelle that regulates cell proliferation

Author

Graça Raposo, Mindaugas Valius, Algirdas Kaupinis, Paulius Gibieža, Ilse Hurbain, Xavier Heiligenstein, Rytis Prekeris, Eric Peterman, Vytenis Arvydas Skeberdis, and Johnathon Schafer

Subjects

0301 basic medicine, Integrins, Cell division, Science, education, Mitosis, General Physics and Astronomy, Cell Communication, Phosphatidylserines, 02 engineering and technology, Article, General Biochemistry, Genetics and Molecular Biology, Cell growth, 03 medical and health sciences, Cell Line, Tumor, Integrin complex, Organelle, Humans, lcsh:Science, Cell Proliferation, Organelles, Multidisciplinary, Chemistry, Cell Membrane, General Chemistry, 021001 nanoscience & nanotechnology, Cell biology, ErbB Receptors, Midbody, 030104 developmental biology, Cytoplasm, Multiprotein Complexes, lcsh:Q, Signal transduction, 0210 nano-technology, Cell Division, Intracellular, HeLa Cells, Signal Transduction

Abstract

Once thought to be a remnant of cell division, the midbody (MB) has recently been shown to have roles beyond its primary function of orchestrating abscission. Despite the emerging roles of post-abscission MBs, how MBs accumulate in the cytoplasm and signal to regulate cellular functions remains unknown. Here, we show that extracellular post-abscission MBs can be internalized by interphase cells, where they reside in the cytoplasm as a membrane-bound signaling structure that we have named the MBsome. We demonstrate that MBsomes stimulate cell proliferation and that MBsome formation is a phagocytosis-like process that depends on a phosphatidylserine/integrin complex, driven by actin-rich membrane protrusions. Finally, we show that MBsomes rely on dynamic actin coats to slow lysosomal degradation and propagate their signaling function. In summary, MBsomes may sometimes serve as intracellular organelles that signal via integrin and EGFR-dependent pathways to promote cell proliferation and anchorage-independent growth and survival., The midbody is a structure found between the two dividing daughter cells that recruits regulators during cell division, but its role after cell division is poorly understood. Here, the authors find that midbodies can be internalized and send out intracellular signals to stimulate cell proliferation.

Published

2019

25. BLOC-1 and BLOC-3 regulate VAMP7 cycling to and from melanosomes via distinct tubular transport carriers

Author

Geoffrey G. Hesketh, David J. Owen, Dorothy C. Bennett, J. Paul Luzio, Michael S. Marks, Graça Raposo, Elena V. Sviderskaya, Cédric Delevoye, Megan K. Dennis, Amanda Acosta-Ruiz, Philip S. Goff, Ilse Hurbain, Thierry Galli, Maryse Romao, Dennis, Megan K [0000-0002-8986-5021], Acosta-Ruiz, Amanda [0000-0002-7591-4128], Hurbain, Ilse [0000-0002-0097-7773], Hesketh, Geoffrey G [0000-0002-5570-7615], Goff, Philip S [0000-0003-4371-5527], Sviderskaya, Elena V [0000-0002-4177-8236], Bennett, Dorothy C [0000-0002-3639-7527], Luzio, J Paul [0000-0003-3912-9760], Galli, Thierry [0000-0001-8514-7455], Marks, Michael S [0000-0001-7435-7262], and Apollo - University of Cambridge Repository

Subjects

0301 basic medicine, Scaffold protein, Endosome, Recombinant Fusion Proteins, Green Fluorescent Proteins, Nerve Tissue Proteins, Biology, Endocytosis, Article, Mitochondrial Proteins, R-SNARE Proteins, 03 medical and health sciences, Lectins, Animals, Humans, Endomembrane system, Transport Vesicles, Research Articles, Melanosome, Melanosomes, Membrane Glycoproteins, Pigmentation, Qa-SNARE Proteins, Cell Membrane, Intracellular Signaling Peptides and Proteins, Cell Biology, Membrane transport, eye diseases, Transport protein, Cell biology, Mice, Inbred C57BL, Protein Transport, 030104 developmental biology, rab GTP-Binding Proteins, Melanocytes, Rab, Carrier Proteins, Oxidoreductases

Abstract

Dennis et al. analyze cycling of the v-SNARE VAMP7 during melanosome biogenesis in melanocytes. VAMP7 is targeted to and retrieved from maturing melanosomes in separate tubular carriers whose formation requires distinct BLOCs, each defective in variants of Hermansky–Pudlak syndrome., Endomembrane organelle maturation requires cargo delivery via fusion with membrane transport intermediates and recycling of fusion factors to their sites of origin. Melanosomes and other lysosome-related organelles obtain cargoes from early endosomes, but the fusion machinery involved and its recycling pathway are unknown. Here, we show that the v-SNARE VAMP7 mediates fusion of melanosomes with tubular transport carriers that also carry the cargo protein TYRP1 and that require BLOC-1 for their formation. Using live-cell imaging, we identify a pathway for VAMP7 recycling from melanosomes that employs distinct tubular carriers. The recycling carriers also harbor the VAMP7-binding scaffold protein VARP and the tissue-restricted Rab GTPase RAB38. Recycling carrier formation is dependent on the RAB38 exchange factor BLOC-3. Our data suggest that VAMP7 mediates fusion of BLOC-1–dependent transport carriers with melanosomes, illuminate SNARE recycling from melanosomes as a critical BLOC-3–dependent step, and likely explain the distinct hypopigmentation phenotypes associated with BLOC-1 and BLOC-3 deficiency in Hermansky–Pudlak syndrome variants.

Published

2016

26. Myosin VI and branched actin filaments mediate membrane constriction and fission of melanosomal tubule carriers

Author

Florent Figon, Michael S. Marks, Megan K. Dennis, Graça Raposo, Cédric Delevoye, Léa Ripoll, Karl J. Petersen, Lia Domingues, Xavier Heiligenstein, Ilse Hurbain, Anne Houdusse, Structure and Membrane Compartments [Paris], Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Children’s Hospital of Philadelphia (CHOP ), Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Compartimentation et dynamique cellulaires (CDC), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut Curie [Paris]-Centre National de la Recherche Scientifique (CNRS), Institut de recherche sur la biologie de l'insecte UMR7261 (IRBI), Université de Tours-Centre National de la Recherche Scientifique (CNRS), Centre National de la Recherche Scientifique (CNRS)-Institut Curie-Université Pierre et Marie Curie - Paris 6 (UPMC), and Institut Curie-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS)

Subjects

0301 basic medicine, Cell Cycle Proteins, [SDV.BC.BC]Life Sciences [q-bio]/Cellular Biology/Subcellular Processes [q-bio.SC], macromolecular substances, Biology, Microfilament, Microtubules, Article, Cell Line, 03 medical and health sciences, Membrane fission, Transcription Factor TFIIIA, Myosin, Molecular motor, Humans, Cytoskeleton, Actin, Research Articles, ComputingMilieux_MISCELLANEOUS, Actin nucleation, Melanosomes, Myosin Heavy Chains, [SDV.BBM.BS]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Structural Biology [q-bio.BM], Membrane Transport Proteins, Cell Biology, Actin Cytoskeleton, 030104 developmental biology, Tubule, Biophysics

Abstract

Pinching the neck of a budding tubule or vesicle requires mechanical forces. Ripoll et al. show that myosin VI, together with branched actin filaments, constricts the membrane of tubular carriers released from melanosomes, which allows for the export of components from melanosomes and promotes melanosome homeostasis, maturation, and transfer to keratinocytes., Vesicular and tubular transport intermediates regulate organellar cargo dynamics. Transport carrier release involves local and profound membrane remodeling before fission. Pinching the neck of a budding tubule or vesicle requires mechanical forces, likely exerted by the action of molecular motors on the cytoskeleton. Here, we show that myosin VI, together with branched actin filaments, constricts the membrane of tubular carriers that are then released from melanosomes, the pigment containing lysosome-related organelles of melanocytes. By combining superresolution fluorescence microscopy, correlative light and electron microscopy, and biochemical analyses, we find that myosin VI motor activity mediates severing by constricting the neck of the tubule at specific melanosomal subdomains. Pinching of the tubules involves the cooperation of the myosin adaptor optineurin and the activity of actin nucleation machineries, including the WASH and Arp2/3 complexes. The fission and release of these tubules allows for the export of components from melanosomes, such as the SNARE VAMP7, and promotes melanosome maturation and transfer to keratinocytes. Our data reveal a new myosin VI– and actin-dependent membrane fission mechanism required for organelle function.

Published

2018

27. Quantifying exosome secretion from single cells reveals a modulatory role for GPCR signaling

Author

Juan J. Garcia-Vallejo, D. Michiel Pegtel, Connie R. Jimenez, Martine J. Smit, Anoek Zomer, Frederik J. Verweij, Marc G. Coppolino, Graça Raposo, S. Rubina Baglio, Hans Janssen, Jaco C. Knol, Jacques Neefjes, Sander R. Piersma, Jacco van Rheenen, Maarten P. Bebelman, Matthijs Verhage, Guillaume van Niel, Jaap M. Middeldorp, Richard de Goeij-de Haas, Ruud F. Toonen, Ilse Hurbain, van Niel, Guillaume, VU University Medical Center [Amsterdam], Biologie Cellulaire et Cancer, Institut Curie [Paris]-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), BioImaging Cell and Tissue Core Facility (PICT-IBiSA), Institut Curie [Paris], Netherlands Cancer Institute (NKI), Antoni van Leeuwenhoek Hospital, Leiden University Medical Center (LUMC), Hubrecht Institute [Utrecht, Netherlands], University Medical Center [Utrecht]-Royal Netherlands Academy of Arts and Sciences (KNAW), University Medical Center [Utrecht], University of Guelph, Vrije Universiteit Amsterdam [Amsterdam] (VU), Functional Genomics, Amsterdam Neuroscience - Cellular & Molecular Mechanisms, Medicinal chemistry, AIMMS, Pathology, CCA - Imaging and biomarkers, Medical oncology laboratory, AGEM - Re-generation and cancer of the digestive system, Molecular cell biology and Immunology, Human genetics, Vrije universiteit = Free university of Amsterdam [Amsterdam] (VU), and VU University Amsterdam

Subjects

0301 basic medicine, Endosome, [SDV]Life Sciences [q-bio], [SDV.BC]Life Sciences [q-bio]/Cellular Biology, macromolecular substances, Biology, [SDV.BC.IC] Life Sciences [q-bio]/Cellular Biology/Cell Behavior [q-bio.CB], Exosome, Exocytosis, Article, 03 medical and health sciences, Tetraspanin, Single-cell analysis, [SDV.BC.IC]Life Sciences [q-bio]/Cellular Biology/Cell Behavior [q-bio.CB], Journal Article, Secretion, [SDV.BC] Life Sciences [q-bio]/Cellular Biology, Research Articles, Cell Biology, Microvesicles, Cell biology, [SDV] Life Sciences [q-bio], 030104 developmental biology, Signal transduction

Abstract

All mammalian cells release small endosome-derived exosomes that function in intercellular communication, but the secretion process is poorly understood. Verweij et al. developed a live-imaging approach and demonstrate that external cues can trigger exosome release from a subpopulation of multivesicular bodies by phosphorylating the target membrane SNARE SNAP23 at serine residue 110., Exosomes are small endosome-derived extracellular vesicles implicated in cell–cell communication and are secreted by living cells when multivesicular bodies (MVBs) fuse with the plasma membrane (PM). Current techniques to study exosome physiology are based on isolation procedures after secretion, precluding direct and dynamic insight into the mechanics of exosome biogenesis and the regulation of their release. In this study, we propose real-time visualization of MVB–PM fusion to overcome these limitations. We designed tetraspanin-based pH-sensitive optical reporters that detect MVB–PM fusion using live total internal reflection fluorescence and dynamic correlative light–electron microscopy. Quantitative analysis demonstrates that MVB–PM fusion frequency is reduced by depleting the target membrane SNAREs SNAP23 and syntaxin-4 but also can be induced in single cells by stimulation of the histamine H1 receptor (H1HR). Interestingly, activation of H1R1 in HeLa cells increases Ser110 phosphorylation of SNAP23, promoting MVB–PM fusion and the release of CD63-enriched exosomes. Using this single-cell resolution approach, we highlight the modulatory dynamics of MVB exocytosis that will help to increase our understanding of exosome physiology and identify druggable targets in exosome-associated pathologies.

Published

2018

28. Phenotypic characterisation ofRAB6Aknockout mouse embryonic fibroblasts

Author

Graça Raposo, Daniela Garcia-Castillo, Sabine Bardin, Stéphanie Miserey-Lenkei, Bruno Goud, and Ilse Hurbain

Subjects

Endosome, Endoplasmic reticulum, Cell Biology, General Medicine, Biology, Golgi apparatus, Null allele, Molecular biology, Cell biology, symbols.namesake, RAB6A, Myosin, symbols, Secretion, Rab

Abstract

Background Information Rab6 is one of the most conserved Rab GTPaes throughout evolution and the most abundant Rab protein associated with the Golgi complex. The two ubiquitous Rab isoforms, Rab6A and Rab6A′, that are generated by alternative splicing of the RAB6A gene, regulate several transport steps at the Golgi level, including retrograde transport between endosomes and Golgi, anterograde transport between Golgi and the plasma membrane, and intra-Golgi and Golgi to endoplasmic reticulum transport. Results We have generated mice with a conditional null allele of RAB6A. Mice homozygous for the RAB6A null allele died at an early stage of embryonic development. Mouse embryonic fibroblasts (MEFs) were isolated from RAB6AloxP/loxPRosa26-CreERT2 and incubated with 4-hydroxy tamoxifen, resulting in the efficient depletion of Rab6A and Rab6A′. We show that Rab6 depletion affects cell growth, alters Golgi morphology and decreases the Golgi-associated levels of some known Rab6 effectors such as Bicaudal-D and myosin II. We also show that Rab6 depletion protects MEFs against ricin toxin and delays VSV-G secretion. Conclusions Our study shows that RAB6 is an essential gene required for normal embryonic development. We confirm in MEF cells most of the functions previously attributed to the two ubiquitous Rab6 isoforms.

Published

2015

29. Analyzing Lysosome-Related Organelles by Electron Microscopy

Author

Ilse, Hurbain, Maryse, Romao, Ptissam, Bergam, Xavier, Heiligenstein, and Graça, Raposo

Subjects

Organelles, Microscopy, Electron, Transmission, Animals, Humans, Lysosomes

Abstract

Intracellular organelles have a particular morphological signature that can only be appreciated by ultrastructural analysis at the electron microscopy level. Optical imaging and associated methodologies allow to explore organelle localization and their dynamics at the cellular level. Deciphering the biogenesis and functions of lysosomes and lysosome-related organelles (LROs) and their dysfunctions requires their visualization and detailed characterization at high resolution by electron microscopy. Here, we provide detailed protocols for studying LROs by transmission electron microscopy. While conventional electron microscopy and its recent improvements is the method of choice to investigate organelle morphology, immunoelectron microscopy allows to localize organelle components and description of their molecular make up qualitatively and quantitatively.

Published

2017

30. Analyzing Lysosome-Related Organelles by Electron Microscopy

Author

Graça Raposo, Ilse Hurbain, Ptissam Bergam, Maryse Romao, and Xavier Heiligenstein

Subjects

0301 basic medicine, Chemistry, Immunoelectron microscopy, law.invention, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Freeze substitution, law, Transmission electron microscopy, Organelle, Ultrastructure, Biophysics, Electron microscope, 030217 neurology & neurosurgery, Organelle localization, Biogenesis

Abstract

Intracellular organelles have a particular morphological signature that can only be appreciated by ultrastructural analysis at the electron microscopy level. Optical imaging and associated methodologies allow to explore organelle localization and their dynamics at the cellular level. Deciphering the biogenesis and functions of lysosomes and lysosome-related organelles (LROs) and their dysfunctions requires their visualization and detailed characterization at high resolution by electron microscopy. Here, we provide detailed protocols for studying LROs by transmission electron microscopy. While conventional electron microscopy and its recent improvements is the method of choice to investigate organelle morphology, immunoelectron microscopy allows to localize organelle components and description of their molecular make up qualitatively and quantitatively.

Published

2017

31. The CryoCapsule: Simplifying Correlative Light to Electron Microscopy

Author

Ilse Hurbain, Claude Antony, Perrine Paul-Gilloteaux, Graça Raposo, Gilles Régnier, Sabine Bardin, Xavier Heiligenstein, Cédric Delevoye, Lucie Sengmanivong, Jean Salamero, and Jérôme Heiligenstein

Subjects

Correlative, Fluorescence-lifetime imaging microscopy, Cell Biology, Biology, Biochemistry, Fluorescence, law.invention, Cell biology, Biological specimen, Freeze substitution, Structural Biology, law, Microscopy, Organelle, Genetics, Electron microscope, Molecular Biology

Abstract

Correlating complementary multiple scale images of the same object is a straightforward means to decipher biological processes. Light microscopy and electron microscopy are the most commonly used imaging techniques, yet despite their complementarity, the experimental procedures available to correlate them are technically complex. We designed and manufactured a new device adapted to many biological specimens, the CryoCapsule, that simplifies the multiple sample preparation steps, which at present separate live cell fluorescence imaging from contextual high-resolution electron microscopy, thus opening new strategies for full correlative light to electron microscopy. We tested the biological application of this highly optimized tool on three different specimens: the in vitro Xenopus laevis mitotic spindle, melanoma cells over-expressing YFP-langerin sequestered in organized membranous subcellular organelles and a pigmented melanocytic cell in which the endosomal system was labeled with internalized fluorescent transferrin.

Published

2014

32. Primary ciliogenesis requires the distal appendage component Cep123

Author

Phong T. Tran, James E. Sillibourne, Michel Bornens, Ilse Hurbain, Thierry Grand-Perret, and Bruno Goud

Subjects

Appendage, Centrosome, Primary cilium, QH301-705.5, Science, Cilium, Anatomy, Biology, General Biochemistry, Genetics and Molecular Biology, Cell biology, Ciliogenesis, Distal appendages, Cell cortex, Centriolar satellites, Basal body, Centriolar satellite, Biology (General), General Agricultural and Biological Sciences, Process (anatomy), Research Article

Abstract

Summary Primary cilium formation is initiated at the distal end of the mother centriole in a highly co-ordinated manner. This requires the capping of the distal end of the mother centriole with a ciliary vesicle and the anchoring of the basal body (mother centriole) to the cell cortex, both of which are mediated by the distal appendages. Here, we show that the distal appendage protein Cep123 (Cep89/CCDC123) is required for the assembly, but not the maintenance, of a primary cilium. In the absence of Cep123 ciliary vesicle formation fails, suggesting that it functions in the early stages of primary ciliogenesis. Consistent with such a role, Cep123 interacts with the centriolar satellite proteins PCM-1, Cep290 and OFD1, all of which play a role in primary ciliogenesis. These interactions are mediated by a domain in the C-terminus of Cep123 (400–783) that overlaps the distal appendage-targeting domain (500–600). Together, the data implicate Cep123 as a new player in the primary ciliogenesis pathway and expand upon the role of the distal appendages in this process.

Published

2013

33. Assessing the localization of centrosomal proteins by PALM/STORM nanoscopy

Author

Michel Bornens, Phong T. Tran, Maxime Dahan, Ignacio Izeddin, Antoine Triller, Christian G. Specht, Xavier Darzacq, Ilse Hurbain, and James E. Sillibourne

Subjects

Centrosome, Molecular composition, Centriole, Molecular Sequence Data, Cell Biology, Anatomy, Biology, Optical reconstruction, Cell biology, Cytoskeletal Proteins, Microscopy, Fluorescence, Structural Biology, Microscopy, CEP164, Microtubule Proteins, Humans, Nanotechnology, Photoactivated localization microscopy, Amino Acid Sequence, Nanoscopic scale, Centrioles

Abstract

The structure of the centrosome was resolved by EM many years ago to reveal a pair of centrioles embedded in a dense network of proteins. More recently, the molecular composition of the centrosome was catalogued by mass spectroscopy and many novel components were identified. Determining precisely where a novel component localizes to within the centrosome remains a challenge, and until now it has required the use of immuno-EM. This technique is both time-consuming and unreliable, as it often fails due to problems with antigen accessibility. We have investigated the use of two nanoscopic techniques, photoactivated localization microscopy (PALM) and stochastic optical reconstruction microscopy (STORM), as alternative techniques for localizing centrosomal proteins. The localization of a known centrosomal component, the distal appendage protein Cep164 was investigated by direct STORM (dSTORM) and resolved with a high spatial resolution. We further validated the use of nanoscopic PALM imaging by showing that the previously uncharacterized centrosomal protein CCDC123 (Cep123) localizes to the distal appendages, forming ring-like structures with a diameter of 500 nm. Our results demonstrate that both PALM and STORM imaging have great potential as alternatives to immuno-EM. © 2011 Wiley Periodicals, Inc.

Published

2011

34. Sas-4 proteins are required during basal body duplication inParamecium

Author

Graça Raposo, Delphine Gogendeau, Renata Basto, Jean Cohen, Ilse Hurbain, Centre de recherche de l'Institut Curie [Paris], Institut Curie [Paris], and Curie Institute

Subjects

Paramecium, Centriole, Recombinant Fusion Proteins, [SDV]Life Sciences [q-bio], sports, Protozoan Proteins, 03 medical and health sciences, Procentriole, 0302 clinical medicine, Tubulin, Microtubule, Gene duplication, Animals, Humans, Basal body, Cilia, Gene Silencing, Molecular Biology, Cytoskeleton, Centrioles, 030304 developmental biology, Genetics, 0303 health sciences, biology, Cilium, Articles, Cell Biology, biology.organism_classification, Cell biology, sports.league, Paramecium tetraurelia, 030217 neurology & neurosurgery

Abstract

This study investigated the role of Sas-4 in basal body duplication in Paramecium and found that Sas-4 proteins are required to assemble and stabilize the germinative disk and cartwheel, which suggests that Sas-4 plays an essential role in basal body duplication., Centrioles and basal bodies are structurally related organelles composed of nine microtubule (MT) triplets. Studies performed in Caenorhabditis elegans embryos have shown that centriole duplication takes place in sequential way, in which different proteins are recruited in a specific order to assemble a procentriole. ZYG-1 initiates centriole duplication by triggering the recruitment of a complex of SAS-5 and SAS-6, which then recruits the final player, SAS-4, to allow the incorporation of MT singlets. It is thought that a similar mechanism (that also involves additional proteins) is present in other animal cells, but it remains to be investigated whether the same players and their ascribed functions are conserved during basal body duplication in cells that exclusively contain basal bodies. To investigate this question, we have used the multiciliated protist Paramecium tetraurelia. Here we show that in the absence of PtSas4, two types of defects in basal body duplication can be identified. In the majority of cases, the germinative disk and cartwheel, the first structures assembled during duplication, are not detected. In addition, if daughter basal bodies were formed, they invariably had defects in MT recruitment. Our results suggest that PtSas4 has a broader function than its animal orthologues.

Published

2011

35. Correction: Quantifying exosome secretion from single cells reveals a modulatory role for GPCR signaling

Author

Martine J. Smit, Hans Janssen, Connie R. Jimenez, Frederik J. Verweij, Matthijs Verhage, Guillaume van Niel, S. Rubina Baglio, Jacques Neefjes, Jaap M. Middeldorp, Graça Raposo, Richard de Goeij-de Haas, Juan J. Garcia-Vallejo, D. Michiel Pegtel, Maarten P. Bebelman, Anoek Zomer, Jaco C. Knol, Ilse Hurbain, Sander R. Piersma, Ruud F. Toonen, Jacco van Rheenen, Marc G. Coppolino, Medicinal chemistry, Molecular and Cellular Neurobiology, Functional Genomics, Amsterdam Neuroscience - Cellular & Molecular Mechanisms, and AIMMS

Subjects

0301 basic medicine, Tetraspanins, Computational biology, Cell Communication, Biology, Exosome, Membrane Fusion, Exocytosis, GPCR Signaling, Potassium Chloride, Receptors, G-Protein-Coupled, 03 medical and health sciences, Human Umbilical Vein Endothelial Cells, Humans, Secretion, Qc-SNARE Proteins, Receptors, Histamine H1, Phosphorylation, G protein-coupled receptor, 030102 biochemistry & molecular biology, Qa-SNARE Proteins, Cell Membrane, Multivesicular Bodies, Correction, Cell Biology, Qb-SNARE Proteins, HCT116 Cells, Microvesicles, Graph (abstract data type), Single-Cell Analysis, HeLa Cells, Histamine

Abstract

Exosomes are small endosome-derived extracellular vesicles implicated in cell-cell communication and are secreted by living cells when multivesicular bodies (MVBs) fuse with the plasma membrane (PM). Current techniques to study exosome physiology are based on isolation procedures after secretion, precluding direct and dynamic insight into the mechanics of exosome biogenesis and the regulation of their release. In this study, we propose real-time visualization of MVB-PM fusion to overcome these limitations. We designed tetraspanin-based pH-sensitive optical reporters that detect MVB-PM fusion using live total internal reflection fluorescence and dynamic correlative light-electron microscopy. Quantitative analysis demonstrates that MVB-PM fusion frequency is reduced by depleting the target membrane SNAREs SNAP23 and syntaxin-4 but also can be induced in single cells by stimulation of the histamine H1 receptor (H1HR). Interestingly, activation of H1R1 in HeLa cells increases Ser110 phosphorylation of SNAP23, promoting MVB-PM fusion and the release of CD63-enriched exosomes. Using this single-cell resolution approach, we highlight the modulatory dynamics of MVB exocytosis that will help to increase our understanding of exosome physiology and identify druggable targets in exosome-associated pathologies.

Published

2018

36. AP-1 and KIF13A coordinate endosomal sorting and positioning during melanosome biogenesis

Author

Stéphanie Uzan-Gafsou, Willie J. C. Geerts, Arie J. Verkleij, Danièle Tenza, Cédric Delevoye, Michael S. Marks, Ilse Hurbain, Graça Raposo, Jean Salamero, Hiroshi Ohno, and Jean-Baptiste Sibarita

Subjects

0303 health sciences, biology, Endosome, 030302 biochemistry & molecular biology, Cell Biology, medicine.disease_cause, Clathrin, 3. Good health, Cell biology, 03 medical and health sciences, Live cell imaging, Protein targeting, Organelle, biology.protein, medicine, Kinesin, Biogenesis, 030304 developmental biology, Melanosome

Abstract

Specialized cell types exploit endosomal trafficking to deliver protein cargoes to cell type–specific lysosome-related organelles (LROs), but how endosomes are specified for this function is not known. In this study, we show that the clathrin adaptor AP-1 and the kinesin motor KIF13A together create peripheral recycling endosomal subdomains in melanocytes required for cargo delivery to maturing melanosomes. In cells depleted of AP-1 or KIF13A, a subpopulation of recycling endosomes redistributes to pericentriolar clusters, resulting in sequestration of melanosomal enzymes like Tyrp1 in vacuolar endosomes and consequent inhibition of melanin synthesis and melanosome maturation. Immunocytochemistry, live cell imaging, and electron tomography reveal AP-1– and KIF13A-dependent dynamic close appositions and continuities between peripheral endosomal tubules and melanosomes. Our results reveal that LRO protein sorting is coupled to cell type–specific positioning of endosomes that facilitate endosome–LRO contacts and are required for organelle maturation.

Published

2009

37. Electron tomography of early melanosomes: Implications for melanogenesis and the generation of fibrillar amyloid sheets

Author

Arie J. Verkleij, Michael S. Marks, Sergio Marco, Graça Raposo, Thomas Boudier, Willie J. C. Geerts, and Ilse Hurbain

Subjects

Amyloid, Cytochalasin D, Endosome, Endosomes, macromolecular substances, Biology, Fibril, Protein Structure, Secondary, Mice, Myosin Type I, Cell Line, Tumor, Freezing, Pressure, Animals, Humans, Integral membrane protein, Melanosome, Melanins, Melanosomes, Membrane Glycoproteins, Multidisciplinary, Vesicle, Cryoelectron Microscopy, Biological Sciences, Cell biology, Freeze substitution, Ultrastructure, Melanocytes, gp100 Melanoma Antigen

Abstract

Melanosomes are lysosome-related organelles (LROs) in which melanins are synthesized and stored. Early stage melanosomes are characterized morphologically by intralumenal fibrils upon which melanins are deposited in later stages. The integral membrane protein Pmel17 is a component of the fibrils, can nucleate fibril formation in the absence of other pigment cell-specific proteins, and forms amyloid-like fibrils in vitro. Before fibril formation Pmel17 traffics through multivesicular endosomal compartments, but how these compartments participate in downstream events leading to fibril formation is not fully known. By using high-pressure freezing of MNT-1 melanoma cells and freeze substitution to optimize ultrastructural preservation followed by double tilt 3D electron tomography, we show that the amyloid-like fibrils begin to form in multivesicular compartments, where they radiate from the luminal side of intralumenal membrane vesicles. The fibrils in fully formed stage II premelanosomes organize into sheet-like arrays and exclude the remaining intralumenal vesicles, which are smaller and often in continuity with the limiting membrane. These observations indicate that premelanosome fibrils form in association with intralumenal endosomal membranes. We suggest that similar processes regulate amyloid formation in pathological models.

Published

2008

38. Meningeal Melanocytes in the Mouse: Distribution and Dependence on Mitf

Author

Diahann A. M. Atacho, Eiríkur Steingrímsson, Stefán A. H. Gudjohnsen, Pétur Henry Petersen, Ilse Hurbain, Graça Raposo, Franck Gesbert, and Lionel Larue

Subjects

Pathology, medicine.medical_specialty, Mouse, Neuroscience (miscellaneous), Melanocyte, lcsh:RC321-571, lcsh:QM1-695, Cellular and Molecular Neuroscience, Meninges, medicine, meningeal melanoma, Distribution (pharmacology), lcsh:Neurosciences. Biological psychiatry. Neuropsychiatry, Original Research, Melanosome, MITF, integumentary system, business.industry, Neural crest, lcsh:Human anatomy, Microphthalmia-associated transcription factor, Meningeal Melanoma, Cell biology, medicine.anatomical_structure, Melanocytes, sense organs, Anatomy, business, Mouse Meninges, Neuroscience

Abstract

Summary: Melanocytes are pigment producing cells derived from the neural crest. They are primarily found in the skin and hair follicles, but can also be found in other tissues including the eye, ear and heart. Here, we describe the distribution of pigmented cells in C57BL/6J mouse meninges, the membranes that envelope the brain. These cells contain melanosomes of all four stages of development and they depend on Microphthalmia associated transcription factor (MITF), the master regulator of melanocyte development, suggesting that they are bona-fide melanocytes. The location of these pigmented cells is consistent with the location of meningeal melanomas in humans and animal models. Significance: Here, we document and define pigmented cells in the meninges of the mouse brain and confirm that they are melanocytes. This is important for understanding the role of this cell type and for understanding primary meningeal melanoma, a rare disease that likely arises from normal meningeal melanocytes.

Published

2015

39. Annual Meeting of the German Society for Cell Biology (29.3.-1.4. 2006)

Author

Eva-Maria S. Grimm-Günter, Sonia Ramos, Graça Raposo, Ilse Hurbain, Céline Revenu, Neil Smyth, Francisco Rivero, and Sylvie Robine

Subjects

Gene isoform, Histology, Brush border, Cell Biology, General Medicine, Biology, Apical membrane, Small intestine, Pathology and Forensic Medicine, Cell biology, medicine.anatomical_structure, Biochemistry, Intestinal mucosa, Knockout mouse, biology.protein, medicine, Villin, Actin

Abstract

Plastin (or fi mbrin) is an actin-bundling protein consisting of two actin-binding domains in tandem preceded by two calcium-binding EF-hands. In mammals three different isoforms are expressed in a cell-type specifi c manner. Iplastin is specifi cally expressed in the small intestine, colon and kidney, where it localizes in microvilli, specialized surface structures with highly ordered microfi lament bundles. We have generated knockout mice lacking I-plastin. I-plastin defi cient mice showed no overt phenotype at the whole animal level: growth rate, reproductive rate and litter size were normal. Antibodies specifi c for T- and L-plastin were used to demonstrate that lacking of I-plastin is not compensated by another plastin isoform. Transmission electron microscopy studies revealed morphological differences between wildtype and I-plastin defi cient mice in the microvilli. Brush border preparations of knockout mice are sensitive and seem to degrade easily. In immunofl uorescence studies of intestinal mucosa cryosections decreased actin staining of the apical membrane was observed. Another abundant actin cross-linker of the brush border, villin, was found to be absent from the apical membrane. I-plastin seems to be an important regulator of the morphological structure and stability of microvilli.

Published

2006

40. A Lumenal Domain-Dependent Pathway for Sorting to Intralumenal Vesicles of Multivesicular Endosomes Involved in Organelle Morphogenesis

Author

Michael S. Marks, Ilse Hurbain, Danielle Tenza, Graça Raposo, Steven T. Truschel, Penelope C. Thomas, Alexander C. Theos, Joanne F. Berson, and Dawn C. Harper

Subjects

Endosome, Vesicle, Viral budding, macromolecular substances, Cell Biology, Biology, General Biochemistry, Genetics and Molecular Biology, Cell biology, Transport protein, ESCRT complex, Cytoplasm, Organelle, Molecular Biology, Biogenesis, Developmental Biology

Abstract

Cargo partitioning into intralumenal vesicles (ILVs) of multivesicular endosomes underlies such cellular processes as receptor downregulation, viral budding, and biogenesis of lysosome-related organelles such as melanosomes. We show that the melanosomal protein Pmel17 is sorted into ILVs by a mechanism that is dependent upon lumenal determinants and conserved in nonpigment cells. Pmel17 targeting to ILVs does not require its native cytoplasmic domain or cytoplasmic residues targeted by ubiquitylation and, unlike sorting of ubiquitylated cargo, is insensitive to functional inhibition of Hrs and ESCRT complexes. Chimeric protein and deletion analyses indicate that two N-terminal lumenal subdomains are necessary and sufficient for ILV targeting. Pmel17 fibril formation, which occurs during melanosome maturation in melanocytes, requires a third lumenal subdomain and proteolytic processing that itself requires ILV localization. These results establish an Hrs- and perhaps ESCRT-independent pathway of ILV sorting by lumenal determinants and a requirement for ILV sorting in fibril formation.

Published

2006

41. Galectin-3 immunodetection in follicular thyroid neoplasms: a prospective study on fine-needle aspiration samples

Author

Ilse Hurbain, C. Prengel, J.F. Collet, Anne Fajac, F. Scetbon, O. Utzmann, and Jean-François Bernaudin

Subjects

Cancer Research, Pathology, medicine.medical_specialty, Galectin 3, Biopsy, Fine-Needle, thyroid, Cell Line, Tumor, Positive predicative value, Cytology, galectin-3, Adenocarcinoma, Follicular, Biopsy, Biomarkers, Tumor, medicine, Humans, fine-needle aspiration, Prospective Studies, Thyroid Neoplasms, Prospective cohort study, Molecular Diagnostics, Thyroid cancer, medicine.diagnostic_test, follicular neoplasms, business.industry, Thyroid, medicine.disease, Immunohistochemistry, Fine-needle aspiration, medicine.anatomical_structure, Oncology, cytology, Adenocarcinoma, business

Abstract

Fine-needle aspiration cytology, which is well established to be accurate for the diagnosis of thyroid cancer, may be inconclusive for the follicular thyroid neoplasms. As galectin-3 was suggested to be a marker of malignant thyrocytes, we investigated whether this protein might be helpful in the diagnosis of aspirates classified as undeterminate by cytology. After establishing an easy processing of aspirates for galectin-3 immunodetection, a series of aspirates categorised as benign (n=63), malignant (n=17) or undeterminate (n=34) was prospectively analysed for galectin-3. Only the patients with malignant or undeterminate lesions underwent surgery. Most lesions (86%) diagnosed as malignant by cytology or after surgery were positive for galectin-3. The majority of lesions (94%) classified as benign by cytology or after surgery was negative for galectin-3. The positive and negative predictive values were 83 and 95%, respectively. When focusing on the undeterminate lesions, the sensitivity and specificity were 75 and 90%, respectively, while the positive and negative predictive values were 82 and 87%, respectively. The specificity and the positive predictive value were higher (100%) when considering the percentage of stained cells. Altogether these results show that galectin-3 constitutes a useful marker in the diagnosis of thyroid lesions classified as undeterminate by conventional cytology.

Published

2005

42. Chloride Transport in Nasal Ciliated Cells of Cystic Fibrosis Heterozygotes

Author

Jean Louis Bresson, Rémi Marianovski, Emanuelle Girodon, Isabelle Sermet-Gaudelus, Anne Fajac, Thao Nguyen-Khoa, Ilse Hurbain, Aleksander Edelman, Michèle Dechaux, Gérard Lenoir, and Benoit Vallée

Subjects

Male, Pulmonary and Respiratory Medicine, Heterozygote, medicine.medical_specialty, Pancreatic disease, Cystic Fibrosis, Cystic Fibrosis Transmembrane Conductance Regulator, Critical Care and Intensive Care Medicine, medicine.disease_cause, Cystic fibrosis, Membrane Potentials, Loss of heterozygosity, Chlorides, Internal medicine, Intensive care, medicine, Humans, Mutation, biology, business.industry, Respiratory disease, Heterozygote advantage, respiratory system, medicine.disease, Introns, Cystic fibrosis transmembrane conductance regulator, Nasal Mucosa, Endocrinology, biology.protein, Female, business

Abstract

Studying subjects heterozygous for mutations of the cystic fibrosis (CF) gene may help clarify the impact on disease onset of CF transmembrane conductance regulator protein (CFTR-)-dependent chloride secretion. CFTR-mediated chloride transport was evaluated in 52 heterozygous subjects, 32 healthy control subjects, and 77 patients with CF with class I or II mutations. We measured the change in nasal potential difference in response to chloride-free isoproterenol solution for each subject and used a video-imaging fluorescent dye assay to assess the percentage of nasal ciliated cells with cAMP-dependent anion conductance. Our findings did not confirm the standard assumption that heterozygosity implies 50% of normal CFTR function. Half the heterozygous subjects had CFTR-mediated chloride transport levels below 50% of the normal range, and one-third had levels similar to those of the patients with CF. This reduced CFTR function was not associated with an elevated prevalence of CF-like symptoms in heterozygous subjects but was highly related to respiratory status in the patients with CF. These data suggest that CFTR-dependent chloride conductance does not directly modulate disease severity but may be part of a more global defect in patients with CF involving other CFTR functions or currently unknown modulatory factors.

Published

2005

43. Molecular and functional MDR1-Pgp and MRPs expression in human glioblastoma multiforme cell lines

Author

Jean-Louis Laplanche, Xavier Declèves, Jean-François Bernaudin, Marcienne Tardy, Jacqueline Lehmann-Che, Jean-Michel Scherrmann, Ilse Hurbain, Claire Mercier, and Anne Fajac

Subjects

Cancer Research, Pathology, medicine.medical_specialty, biology, Multidrug resistance-associated protein 2, medicine.disease, Molecular biology, Cell membrane, medicine.anatomical_structure, Oncology, Cell culture, Glioma, Gene expression, biology.protein, medicine, Intracellular, Etoposide, P-glycoprotein, medicine.drug

Abstract

The aim of our study was to investigate the functional expression of P-glycoprotein (Pgp) and multidrug resistance-associated proteins (MRPs) in 2 distinct glioma cells (GL15 and 8MG) from patients with glioblastoma multiforme. MDR1 gene and Pgp expression was not detected in either cell line by RT-PCR and Western blotting, respectively. In contrast, MRP1 was detected at both mRNA and protein level in both cell lines, with a higher expression in the 8MG cells that occur predominantly at the cell membrane. Three other MRPs (MRP3, MRP4 and MRP5) were detected by RT-PCR in both cell lines, whereas MRP2 was not expressed. In addition, MRP3 protein was also detected by immunocytochemistry in both GL15 and 8MG cell lines. Indomethacin and probenecid, 2 modulators of MRPs activity, increased the accumulation of vincristine and etoposide, 2 substrates of MRPs, by both cell lines. These modulators also decreased the efflux of vincristine from both cell lines with a more pronounced effect in 8MG cells. In conclusion, our results show functional expression of MRPs leading to a decrease in the intracellular vincristine and etoposide concentrations in human glioblastoma cell lines. Furthermore, our results that exhibit protein expression of MRP1 and MRP3 and gene expression of MRP4 and MRP5 in these 2 glioblastoma cell lines suggest new mechanisms that could lead to a MDR phenotype of tumour cells in patients with glioblastoma multiforme.

Published

2002

44. Apolipoprotein E Regulates Amyloid Formation within Endosomes of Pigment Cells

Author

Alessandra Lo Cicero, Guillaume van Niel, Florent Dingli, Ilse Hurbain, Marie-Claude Potier, Graça Raposo, Aurélie Di Cicco, Ptissam Bergam, Leon J. Schurgers, Damarys Loew, Cecile Fort, Daniel Lévy, Roberta Palmulli, Compartimentation et dynamique cellulaires (CDC), Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Université Pierre et Marie Curie - Paris 6 (UPMC), BioImaging Cell and Tissue Core Facility (PICT-IBiSA), Institut Curie [Paris], Research University Chimie Paristech (PSL), Physico-Chimie-Curie (PCC), Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut de Chimie du CNRS (INC), Laboratoire de Spectrométrie de Masse Protéomique, Institut du Cerveau et de la Moëlle Epinière = Brain and Spine Institute (ICM), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-CHU Pitié-Salpêtrière [AP-HP], Sorbonne Université (SU)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Sorbonne Université (SU)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP), Cardiovascular Research Institute Maastricht (CARIM), Maastricht University [Maastricht], HAL UPMC, Gestionnaire, Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut Curie [Paris]-Centre National de la Recherche Scientifique (CNRS), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut Curie [Paris]-Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut National de la Santé et de la Recherche Médicale (INSERM)-CHU Pitié-Salpêtrière [AP-HP], Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Sorbonne Université (SU)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Sorbonne Université (SU)-Centre National de la Recherche Scientifique (CNRS), Biochemie, RS: CARIM - R1 - Thrombosis and haemostasis, van Niel G., Bergam P., Di Cicco A., Hurbain I., Lo Cicero A., Dingli F., Palmulli R., Fort C., Potier M.C., Schurgers L.J., Loew D., Levy D., and Raposo G.

Subjects

Apolipoprotein E, Amyloid, Endosome, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, Endosomes, Biology, Exosomes, General Biochemistry, Genetics and Molecular Biology, Mice, Apolipoproteins E, mental disorders, Animals, Humans, amyloid-related diseases, lcsh:QH301-705.5, [SDV.BC] Life Sciences [q-bio]/Cellular Biology, Melanosome, Mice, Knockout, Melanosomes, Endosomal Sorting Complexes Required for Transport, Vesicle, Microvesicles, PMEL, Cell biology, Mice, Inbred C57BL, lcsh:Biology (General), Biochemistry, Gene Expression Regulation, Melanocytes, Signal transduction, HeLa Cells, Signal Transduction

Abstract

International audience; Accumulation of toxic amyloid oligomers is a key feature in the pathogenesis of amyloid-related diseases. Formation of mature amyloid fibrils is one defense mechanism to neutralize toxic prefibrillar oligomers. This mechanism is notably influenced by apolipoprotein E variants. Cells that produce mature amyloid fibrils to serve physiological functions must exploit specific mechanisms to avoid potential accumulation of toxic species. Pigment cells have tuned their endosomes to maximize the formation of functional amyloid from the protein PMEL. Here, we show that ApoE is associated with intraluminal vesicles (ILV) within endosomes and remain associated with ILVs when they are secreted as exosomes. ApoE functions in the ESCRT-independent sorting mechanism of PMEL onto ILVs and regulates the endosomal formation of PMEL amyloid fibrils in vitro and in vivo. This process secures the physiological formation of amyloid fibrils by exploiting ILVs as amyloid nucleating platforms.

Published

2014

45. Phenotypic characterisation of RAB6A knockout mouse embryonic fibroblasts

Author

Sabine, Bardin, Stéphanie, Miserey-Lenkei, Ilse, Hurbain, Daniela, Garcia-Castillo, Graça, Raposo, and Bruno, Goud

Subjects

Mice, Knockout, Cell Membrane, Embryonic Development, Gene Expression Regulation, Developmental, Golgi Apparatus, Ricin, Fibroblasts, Endoplasmic Reticulum, Alternative Splicing, Mice, Tamoxifen, rab GTP-Binding Proteins, Animals, Humans

Abstract

Rab6 is one of the most conserved Rab GTPaes throughout evolution and the most abundant Rab protein associated with the Golgi complex. The two ubiquitous Rab isoforms, Rab6A and Rab6A', that are generated by alternative splicing of the RAB6A gene, regulate several transport steps at the Golgi level, including retrograde transport between endosomes and Golgi, anterograde transport between Golgi and the plasma membrane, and intra-Golgi and Golgi to endoplasmic reticulum transport.We have generated mice with a conditional null allele of RAB6A. Mice homozygous for the RAB6A null allele died at an early stage of embryonic development. Mouse embryonic fibroblasts (MEFs) were isolated from RAB6A(loxP/loxP) Rosa26-CreERT2 and incubated with 4-hydroxy tamoxifen, resulting in the efficient depletion of Rab6A and Rab6A'. We show that Rab6 depletion affects cell growth, alters Golgi morphology and decreases the Golgi-associated levels of some known Rab6 effectors such as Bicaudal-D and myosin II. We also show that Rab6 depletion protects MEFs against ricin toxin and delays VSV-G secretion.Our study shows that RAB6 is an essential gene required for normal embryonic development. We confirm in MEF cells most of the functions previously attributed to the two ubiquitous Rab6 isoforms.

Published

2014

46. Step by step manipulation of the CryoCapsule with HPM high pressure freezers

Author

Xavier, Heiligenstein, Ilse, Hurbain, Cédric, Delevoye, Jean, Salamero, Claude, Antony, and Graca, Raposo

Subjects

Cryopreservation, Luminescent Proteins, Mannose-Binding Lectins, Bacterial Proteins, Microscopy, Electron, Transmission, Microscopy, Fluorescence, Antigens, CD, Cell Line, Tumor, Recombinant Fusion Proteins, Pressure, Humans, Lectins, C-Type

Abstract

The CryoCapsule is a tool dedicated to correlative light to electron microscopy experiments. Focused on simplifying the specimen manipulation throughout the entire workflow from live-cell imaging to freeze substitution following cryofixation by high pressure freezing, we introduce here a step by step procedure to use the CryoCapsule either with the high pressure freezing machines: HPM010 or the HPM100.

Published

2014

47. Step by Step Manipulation of the CryoCapsule with HPM High Pressure Freezers

Author

Claude Antony, Graça Raposo, Ilse Hurbain, Cédric Delevoye, Jean Salamero, and Xavier Heiligenstein

Subjects

Freeze substitution, Live cell imaging, law, High pressure, Biophysics, High pressure freezing, Electron microscope, Biology, Cryopreservation, Cryofixation, law.invention, Luminescent Proteins

Abstract

The CryoCapsule is a tool dedicated to correlative light to electron microscopy experiments. Focused on simplifying the specimen manipulation throughout the entire workflow from live-cell imaging to freeze substitution following cryofixation by high pressure freezing, we introduce here a step by step procedure to use the CryoCapsule either with the high pressure freezing machines: HPM010 or the HPM100.

Published

2014

48. The capsids of HIV-1 and HIV-2 determine immune detection of the viral cDNA by the innate sensor cGAS in dendritic cells

Author

Matteo Gentili, Christine Lacabaratz, Ilse Hurbain, Xavier Lahaye, Ahmed El Marjou, Cécile Conrad, Jean-Daniel Lelièvre, Takeshi Satoh, Nicolas Manel, Silvia Cerboni, Immunité et cancer (U932), Université Paris Descartes - Paris 5 (UPD5)-Institut Curie [Paris]-Institut National de la Santé et de la Recherche Médicale (INSERM), Compartimentation et dynamique cellulaires (CDC), Université Pierre et Marie Curie - Paris 6 (UPMC)-Institut Curie [Paris]-Centre National de la Recherche Scientifique (CNRS), Institut Mondor de Recherche Biomédicale (IMRB), Institut National de la Santé et de la Recherche Médicale (INSERM)-IFR10-Université Paris-Est Créteil Val-de-Marne - Paris 12 (UPEC UP12), Immunologie Clinique, Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Hôpital Henri Mondor-Hôpital Albert Chenevier, This work was supported by Institut Curie, Institut National de la Santé et de la Recherche Médicale (INSERM), ATIP-Avenir program, Agence Nationale de Recherche sur le SIDA (ANRS), Ville de Paris Emergence program, European FP7 Marie Curie Actions, European Research Council, LABEX VRI and LABEX DCBIOL., Centre National de la Recherche Scientifique (CNRS)-Institut Curie [Paris]-Université Pierre et Marie Curie - Paris 6 (UPMC), Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Paris-Est Créteil Val-de-Marne - Paris 12 (UPEC UP12)-IFR10, Immunité et cancer ( U932 ), Université Paris Descartes - Paris 5 ( UPD5 ) -Institut Curie-Institut National de la Santé et de la Recherche Médicale ( INSERM ), Compartimentation et dynamique cellulaires ( CDC ), Centre National de la Recherche Scientifique ( CNRS ) -INSTITUT CURIE-Université Pierre et Marie Curie - Paris 6 ( UPMC ), Institut Mondor de Recherche Biomédicale ( IMRB ), Université Paris-Est Créteil Val-de-Marne - Paris 12 ( UPEC UP12 ) -Institut National de la Santé et de la Recherche Médicale ( INSERM ) -IFR10, Assistance publique - Hôpitaux de Paris (AP-HP)-Hôpital Henri Mondor-Hôpital Albert Chenevier, and Guellaen, Georges

Subjects

MESH : DNA, Complementary, viruses, HIV Infections, MESH : Models, Biological, Genome, MESH: HIV-1, chemistry.chemical_compound, 0302 clinical medicine, MESH: HIV-2, Immunology and Allergy, MESH: Nucleotidyltransferases, MESH: Capsid, MESH : DNA, Viral, Cells, Cultured, MESH : Nucleotidyltransferases, 0303 health sciences, MESH: Dendritic Cells, virus diseases, MESH: HIV Infections, MESH : Immunity, Innate, Nucleotidyltransferases, 3. Good health, Infectious Diseases, Capsid, 030220 oncology & carcinogenesis, MESH: Immunity, Innate, MESH : Capsid, MESH : HIV-2, MESH : HIV-1, MESH: Cells, Cultured, DNA, Complementary, CypA, Immunology, innate antiviral immunity, chemical and pharmacologic phenomena, Biology, Models, Biological, Virus, 03 medical and health sciences, Immune system, Immunity, Complementary DNA, MESH : Cells, Cultured, [SDV.BBM] Life Sciences [q-bio]/Biochemistry, Molecular Biology, MESH : HIV Infections, Humans, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, [ SDV.BBM ] Life Sciences [q-bio]/Biochemistry, Molecular Biology, 030304 developmental biology, Innate immune system, MESH: Humans, HIV-1 capsid, MESH : Humans, MESH: Models, Biological, Dendritic Cells, MESH: DNA, Complementary, biochemical phenomena, metabolism, and nutrition, Virology, Immunity, Innate, MESH: DNA, Viral, Prospects & Overviews, chemistry, MESH : Dendritic Cells, DNA, Viral, HIV-2, HIV-1, cytosolic DNA sensor, DNA, cGAS

Abstract

International audience; HIV-2 is less pathogenic for humans than HIV-1 and might provide partial cross-protection from HIV-1-induced pathology. Although both viruses replicate in the T cells of infected patients, only HIV-2 replicates efficiently in dendritic cells (DCs) and activates innate immune pathways. How HIV is sensed in DC is unknown. Capsid-mutated HIV-2 revealed that sensing by the host requires viral cDNA synthesis, but not nuclear entry or genome integration. The HIV-1 capsid prevented viral cDNA sensing up to integration, allowing the virus to escape innate recognition. In contrast, DCs sensed capsid-mutated HIV-1 and enhanced stimulation of T cells in the absence of productive infection. Finally, we found that DC sensing of HIV-1 and HIV-2 required the DNA sensor cGAS. Thus, the HIV capsid is a determinant of innate sensing of the viral cDNA by cGAS in dendritic cells. This pathway might potentially be harnessed to develop effective vaccines against HIV-1.

Published

2013

49. Different Pattern of MRP Localization in Ciliated and Basal Cells from Human Bronchial Epithelium

Author

Jean-François Bernaudin, Ilse Hurbain, Nicole Daty, Jeanne-Marie Bréchot, and Anne Fajac

Subjects

Male, 0301 basic medicine, Cell type, Histology, Transcription, Genetic, medicine.drug_class, Bronchi, Biology, Monoclonal antibody, Polymerase Chain Reaction, Epithelium, 03 medical and health sciences, stomatognathic system, medicine, Humans, Cilia, Messenger RNA, 030102 biochemistry & molecular biology, Transporter, Immunohistochemistry, Drug Resistance, Multiple, Transmembrane protein, Cell biology, 030104 developmental biology, Cancer cell, Keratins, ATP-Binding Cassette Transporters, Female, Multidrug Resistance-Associated Proteins, Anatomy, Immunostaining

Abstract

The MRP (multidrug resistance-associated protein) transmembrane transporter, which actively transports a wide variety of lipophilic substrates out of cancer cells, has been suggested to play a major role in cell detoxification via efflux of glutathione conjugates. Because bronchial epithelial cells are constantly exposed to environmental pollutants, MRP might be a particularly important defense mechanism against xenobiotics. This study was therefore designed to investigate MRP localization by immunohistochemistry in bronchial epithelial cells collected by scraping from surgical specimens. In parallel, MRP mRNA was detected by reverse transcriptase chain reaction (rt-PCR) in bronchial cell lysates. However, the pattern of protein expression differed markedly according to cell type. In ciliated epithelial cells, immunostaining was restricted to the basolateral surface, without any labeling at the apical surface, which is at variance with the localization of CFTR and MDR1 proteins, other members of the same family of transporters. In basal cells, MRP was present over the entire circumference of the plasma membrane. Basal cells were identified by their morphology and specifically after incubation with an anticytokeratin 17 monoclonal antibody. In conclusion, the different patterns of localization suggest specific roles for MRP in basal and ciliated cells.

Published

1998

50. BACE2 processes PMEL to form the melanosome amyloid matrix in pigment cells

Author

Michael S. Marks, Guillaume van Niel, Ilse Hurbain, Bart De Strooper, Leila Rochin, Cecile Fort, Graça Raposo, Brenda Watt, Pascal Leblanc, Lutgarde Serneels, Institut NeuroMyoGène (INMG), Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Centre National de la Recherche Scientifique (CNRS)-Institut National de la Santé et de la Recherche Médicale (INSERM), Center for Human Genetics, University of Leuven School of Medicine, SCHOOL of MEDICINE [Louvain], and Université Catholique de Louvain = Catholic University of Louvain (UCL)-Université Catholique de Louvain = Catholic University of Louvain (UCL)

Subjects

[SDV.BIO]Life Sciences [q-bio]/Biotechnology, [SDV.NEU.NB]Life Sciences [q-bio]/Neurons and Cognition [q-bio.NC]/Neurobiology, Skin Pigmentation, [SDV.BC.BC]Life Sciences [q-bio]/Cellular Biology/Subcellular Processes [q-bio.SC], Mice, 0302 clinical medicine, [SDV.MHEP.MI]Life Sciences [q-bio]/Human health and pathology/Infectious diseases, [SDV.BC.IC]Life Sciences [q-bio]/Cellular Biology/Cell Behavior [q-bio.CB], Amyloid precursor protein, Aspartic Acid Endopeptidases, RNA, Small Interfering, Pigment Epithelium of Eye, ComputingMilieux_MISCELLANEOUS, Mice, Knockout, 0303 health sciences, Multidisciplinary, Melanosomes, medicine.diagnostic_test, Biological Sciences, PMEL, Cell biology, medicine.anatomical_structure, Biochemistry, [SDV.MP.VIR]Life Sciences [q-bio]/Microbiology and Parasitology/Virology, Melanocytes, gp100 Melanoma Antigen, Proteases, Amyloid, Proteolysis, Biology, Melanocyte, Cell Line, 03 medical and health sciences, [SDV.BBM.GTP]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Genomics [q-bio.GN], mental disorders, medicine, Animals, Humans, RNA, Messenger, [SDV.BBM.BC]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Biochemistry [q-bio.BM], 030304 developmental biology, Melanosome, Melanins, [SDV.BBM.BM]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Molecular biology, Mice, Inbred C57BL, [SDV.GEN.GA]Life Sciences [q-bio]/Genetics/Animal genetics, [SDV.GEN.GH]Life Sciences [q-bio]/Genetics/Human genetics, biology.protein, Amyloid Precursor Protein Secretases, Amyloid precursor protein secretase, Protein Processing, Post-Translational, 030217 neurology & neurosurgery, HeLa Cells

Abstract

Amyloids are often associated with pathologic processes such as in Alzheimer’s disease (AD), but can also underlie physiological processes such as pigmentation. Formation of pathological and functional amyloidogenic substrates can require precursor processing by proteases, as exemplified by the generation of Aβ peptide from amyloid precursor protein (APP) by beta-site APP cleaving enzyme (BACE)1 and γ-secretase. Proteolytic processing of the pigment cell-specific Melanocyte Protein (PMEL) is also required to form functional amyloid fibrils during melanogenesis, but the enzymes involved are incompletely characterized. Here we show that the BACE1 homologue BACE2 processes PMEL to generate functional amyloids. BACE2 is highly expressed in pigment cells and Bace2 −/− but not Bace1 −/− mice display coat color defects, implying a specific role for BACE2 during melanogenesis. By using biochemical and morphological analyses, combined with RNA silencing, pharmacologic inhibition, and BACE2 overexpression in a human melanocytic cell line, we show that BACE2 cleaves the integral membrane form of PMEL within the juxtamembrane domain, releasing the PMEL luminal domain into endosomal precursors for the formation of amyloid fibrils and downstream melanosome morphogenesis. These studies identify an amyloidogenic substrate of BACE2, reveal an important physiological role for BACE2 in pigmentation, and highlight analogies in the generation of PMEL-derived functional amyloids and APP-derived pathological amyloids.

Published

2013