Your search keyword '"Eugenio F. Fornasiero"' showing total 54 results

1. Protocol for differential multi-omic analyses of distinct cell types in the mouse cerebral cortex

Author

Durga Praveen Meka, Melanie Richter, Tabitha Rücker, Hannah Voss, Anne Rissiek, Christoph Krisp, Nisha Hemandhar Kumar, Birgit Schwanke, Eugenio F. Fornasiero, Hartmut Schlüter, and Froylan Calderon de Anda

Subjects

Bioinformatics, Genomics, RNA-seq, Neuroscience, Proteomics, Science (General), Q1-390

Abstract

Summary: Here, we present a protocol for differential multi-omic analyses of distinct cell types in the developing mouse cerebral cortex. We describe steps for in utero electroporation, subsequent flow-cytometry-based isolation of developing mouse cortical cells, bulk RNA sequencing or quantitative liquid chromatography-tandem mass spectrometry, and bioinformatic analyses. This protocol can be applied to compare the proteomes and transcriptomes of developing mouse cortical cell populations after various manipulations (e.g., epigenetic).For complete details on the use and execution of this protocol, please refer to Meka et al. (2022).1 : Publisher’s note: Undertaking any experimental protocol requires adherence to local institutional guidelines for laboratory safety and ethics.

Published

2024

2. Age-dependent structural reorganization of utricular ribbon synapses

Author

Susann Michanski, Timo Henneck, Mohona Mukhopadhyay, Anna M. Steyer, Paola Agüi Gonzalez, Katharina Grewe, Peter Ilgen, Mehmet Gültas, Eugenio F. Fornasiero, Stefan Jakobs, Wiebke Möbius, Christian Vogl, Tina Pangršič, Silvio O. Rizzoli, and Carolin Wichmann

Subjects

aging, ribbon synapse, synaptogenesis, utricle, vestibular hair cells, Biology (General), QH301-705.5

Abstract

In mammals, spatial orientation is synaptically-encoded by sensory hair cells of the vestibular labyrinth. Vestibular hair cells (VHCs) harbor synaptic ribbons at their presynaptic active zones (AZs), which play a critical role in molecular scaffolding and facilitate synaptic release and vesicular replenishment. With advancing age, the prevalence of vestibular deficits increases; yet, the underlying mechanisms are not well understood and the possible accompanying morphological changes in the VHC synapses have not yet been systematically examined. We investigated the effects of maturation and aging on the ultrastructure of the ribbon-type AZs in murine utricles using various electron microscopic techniques and combined them with confocal and super-resolution light microscopy as well as metabolic imaging up to 1 year of age. In older animals, we detected predominantly in type I VHCs the formation of floating ribbon clusters, mostly consisting of newly synthesized ribbon material. Our findings suggest that VHC ribbon-type AZs undergo dramatic structural alterations upon aging.

Published

2023

3. NanoSIMS observations of mouse retinal cells reveal strict metabolic controls on nitrogen turnover

Author

Elisa A. Bonnin, Eugenio F. Fornasiero, Felix Lange, Christoph W. Turck, and Silvio O. Rizzoli

Subjects

Secondary ion mass spectrometry, Imaging, Metabolic labelling, Protein turnover, Retina, Cytology, QH573-671

Abstract

Abstract Background Most of the cells of the mammalian retina are terminally differentiated, and do not regenerate once fully developed. This implies that these cells have strict controls over their metabolic processes, including protein turnover. We report the use of metabolic labelling procedures and secondary ion mass spectrometry imaging to examine nitrogen turnover in retinal cells, with a focus on the outer nuclear layer, inner nuclear layer, and outer plexiform layer. Results We find that turnover can be observed in all cells imaged using NanoSIMS. However, the rate of turnover is not constant, but varies between different cellular types and cell regions. In the inner and outer nuclear layers, turnover rate is higher in the cytosol than in the nucleus of each cell. Turnover rates are also higher in the outer plexiform layer. An examination of retinal cells from mice that were isotopically labeled very early in embryonic development shows that proteins produced during this period can be found in all cells and cell regions up to 2 months after birth, even in regions of high turnover. Conclusions Our results indicate that turnover in retinal cells is a highly regulated process, with strict metabolic controls. We also observe that turnover is several-fold higher in the synaptic layer than in cell layers. Nevertheless, embryonic proteins can still be found in this layer 2 months after birth, suggesting that stable structures persist within the synapses, which remain to be determined.

Published

2021

4. A nanobody-based fluorescent reporter reveals human α-synuclein in the cell cytosol

Author

Christoph Gerdes, Natalia Waal, Thomas Offner, Eugenio F. Fornasiero, Nora Wender, Hannes Verbarg, Ivan Manzini, Claudia Trenkwalder, Brit Mollenhauer, Timo Strohäker, Markus Zweckstetter, Stefan Becker, Silvio O. Rizzoli, Fitnat Buket Basmanav, and Felipe Opazo

Subjects

Science

Abstract

α-Syn in CSF is a biomarker of neurodegenerative diseases; however, the detection of clinically relevant species is difficult. Here, the authors create a nanobody biosensor that reveals the presence of α-Syn in cells, which allow the detection of transmittable forms of α-Syn present in human CSF.

Published

2020

5. Pathological changes are associated with shifts in the employment of synonymous codons at the transcriptome level

Author

Eugenio F. Fornasiero and Silvio O. Rizzoli

Subjects

Codon usage, mRNA abundance, Molecular diagnostics, Pathology meta-analysis, Biotechnology, TP248.13-248.65, Genetics, QH426-470

Abstract

Abstract Background The usage of different synonymous codons reflects the genome organization and has been connected to parameters such as mRNA abundance and protein folding. It is also been established that mutations targeting specific synonymous codons can trigger disease. Results We performed a systematic meta-analysis of transcriptome results from 75 datasets representing 40 pathologies. We found that a subset of codons was preferentially employed in abundant transcripts, while other codons were preferentially found in low-abundance transcripts. By comparing control and pathological transcriptomes, we observed a shift in the employment of synonymous codons for every analyzed disease. For example, cancerous tissue employed preferentially A- or U-ending codons, shifting from G- or C-ending codons, which were preferred by control tissues. This analysis was able to discriminate patients and controls with high specificity and sensitivity. Conclusions Here we show that the employment of specific synonymous codons, quantified at the whole transcriptome level, changes profoundly in many diseases. We propose that the changes in codon employment offer a novel perspective for disease studies, and could be used to design new diagnostic tools.

Published

2019

6. Precisely measured protein lifetimes in the mouse brain reveal differences across tissues and subcellular fractions

Author

Eugenio F. Fornasiero, Sunit Mandad, Hanna Wildhagen, Mihai Alevra, Burkhard Rammner, Sarva Keihani, Felipe Opazo, Inga Urban, Till Ischebeck, M. Sadman Sakib, Maryam K. Fard, Koray Kirli, Tonatiuh Pena Centeno, Ramon O. Vidal, Raza-Ur Rahman, Eva Benito, André Fischer, Sven Dennerlein, Peter Rehling, Ivo Feussner, Stefan Bonn, Mikael Simons, Henning Urlaub, and Silvio O. Rizzoli

Subjects

Science

Abstract

Measuring precise protein turnover rates in animals is technically challenging at the proteomic level. Here, Fornasiero and colleagues use isotopic labeling with mass spectrometry and mathematical modeling to accurately determine protein lifetimes in the mouse brain

Published

2018

7. Influence of Subcellular Localization and Functional State on Protein Turnover

Author

Roya Yousefi, Kristina Jevdokimenko, Verena Kluever, David Pacheu-Grau, and Eugenio F. Fornasiero

Subjects

protein stability, optical analysis of protein turnover, SNAP-tag, pulse-chase, Rab5a, Cytology, QH573-671

Abstract

Protein homeostasis is an equilibrium of paramount importance that maintains cellular performance by preserving an efficient proteome. This equilibrium avoids the accumulation of potentially toxic proteins, which could lead to cellular stress and death. While the regulators of proteostasis are the machineries controlling protein production, folding and degradation, several other factors can influence this process. Here, we have considered two factors influencing protein turnover: the subcellular localization of a protein and its functional state. For this purpose, we used an imaging approach based on the pulse-labeling of 17 representative SNAP-tag constructs for measuring protein lifetimes. With this approach, we obtained precise measurements of protein turnover rates in several subcellular compartments. We also tested a selection of mutants modulating the function of three extensively studied proteins, the Ca2+ sensor calmodulin, the small GTPase Rab5a and the brain creatine kinase (CKB). Finally, we followed up on the increased lifetime observed for the constitutively active Rab5a (Q79L), and we found that its stabilization correlates with enlarged endosomes and increased interaction with membranes. Overall, our data reveal that both changes in protein localization and functional state are key modulators of protein turnover, and protein lifetime fluctuations can be considered to infer changes in cellular behavior.

Published

2021

8. Brain Long Noncoding RNAs: Multitask Regulators of Neuronal Differentiation and Function

Author

Sarva Keihani, Verena Kluever, and Eugenio F. Fornasiero

Subjects

long noncoding RNAs, neurons, neuronal development, neuronal differentiation, neurogenesis, synaptic activity, Organic chemistry, QD241-441

Abstract

The extraordinary cellular diversity and the complex connections established within different cells types render the nervous system of vertebrates one of the most sophisticated tissues found in living organisms. Such complexity is ensured by numerous regulatory mechanisms that provide tight spatiotemporal control, robustness and reliability. While the unusual abundance of long noncoding RNAs (lncRNAs) in nervous tissues was traditionally puzzling, it is becoming clear that these molecules have genuine regulatory functions in the brain and they are essential for neuronal physiology. The canonical view of RNA as predominantly a ‘coding molecule’ has been largely surpassed, together with the conception that lncRNAs only represent ‘waste material’ produced by cells as a side effect of pervasive transcription. Here we review a growing body of evidence showing that lncRNAs play key roles in several regulatory mechanisms of neurons and other brain cells. In particular, neuronal lncRNAs are crucial for orchestrating neurogenesis, for tuning neuronal differentiation and for the exact calibration of neuronal excitability. Moreover, their diversity and the association to neurodegenerative diseases render them particularly interesting as putative biomarkers for brain disease. Overall, we foresee that in the future a more systematic scrutiny of lncRNA functions will be instrumental for an exhaustive understanding of neuronal pathophysiology.

Published

2021

9. Determining and interpreting protein lifetimes in mammalian tissues

Author

Jeffrey Savas and Eugenio F. Fornasiero

Subjects

Molecular Biology, Biochemistry

Abstract

The orchestration of protein production and degradation, and the regulation of protein lifetimes, play a central role in the majority of biological processes. Recent advances in proteomics have enabled the estimation of protein half-lives for thousands of proteins in vivo. What is the utility of these measurements, and how can they be leveraged to interpret the proteome changes occurring during development, aging, and disease? This opinion article summarizes leading technical approaches and highlights their strengths and weaknesses. We also disambiguate frequently used terminology, illustrate recent mechanistic insights, and provide guidance for interpreting and validating protein turnover measurements. Overall, protein lifetimes, coupled to estimates of protein levels, are essential for obtaining a deep understanding of mammalian biology and the basic processes defining life itself.

Published

2023

10. Spatial proteomics in neurons at single-protein resolution

Author

Eduard M. Unterauer, Sayedali Shetab Boushehri, Kristina Jevdokimenko, Luciano A. Masullo, Mahipal Ganji, Shama Sograte-Idrissi, Rafal Kowalewski, Sebastian Strauss, Susanne C.M. Reinhardt, Ana Perovic, Carsten Marr, Felipe Opazo, Eugenio F. Fornasiero, and Ralf Jungmann

Abstract

SUMMARYTo fully understand biological processes and functions, it is necessary to reveal the molecular heterogeneity of cells and even subcellular assemblies by gaining access to the location and interaction of all biomolecules. The study of protein arrangements has seen significant advancements through super-resolution microscopy, but such methods are still far from reaching the multiplexing capacity of spatial proteomics. Here, we introduce Secondary label-based Unlimited Multiplexed DNA-PAINT (SUM-PAINT), a high-throughput imaging method capable of achieving virtually unlimited multiplexing at better than 15 nm spatial resolution. Using SUM-PAINT, we generated the most extensive multiprotein dataset to date at single-protein spatial resolution, comprising up to 30 distinct protein targets in parallel and adapted omics-inspired analysis workflows to explore these feature-rich datasets. Remarkably, by examining the multiplexed protein content of almost 900 individual synapses at single-protein resolution, we revealed the complexity of synaptic heterogeneity, ultimately leading to the discovery of a new synapse type. This work provides not only a feature-rich resource for researchers, but also an integrated data acquisition and analysis workflow for comprehensive spatial proteomics at single-protein resolution, paving the way for ‘Localizomics’.

Published

2023

11. Generalizing the definition of protein turnover to out‐of‐equilibrium conditions

Author

Eugenio F. Fornasiero

Subjects

General Biochemistry, Genetics and Molecular Biology

Published

2023

12. A versatile synaptotagmin-1 nanobody provides perturbation-free live synaptic imaging and low linkage-error in super-resolution microscopy

Author

Karine Queiroz Zetune Villa Real, Nikolaos Mougios, Ronja Rehm, Shama Sograte-Idrissi, László Albert, Amir Mohammad Rahimi, Manuel Maidorn, Jannik Hentze, Markel Martínez-Carranza, Hassan Hosseini, Kim-Ann Saal, Nazar Oleksiievets, Matthias Prigge, Roman Tsukanov, Pål Stenmark, Eugenio F. Fornasiero, and Felipe Opazo

Abstract

Imaging of living synapses has relied for over two decades on the overexpression of synaptic proteins fused to fluorescent reporters. This strategy changes the stoichiometry of synaptic components and ultimately affects synapse physiology. To overcome these limitations, here we introduce a nanobody that binds the calcium sensor synaptotagmin-1 (NbSyt1). This nanobody functions in living neurons as an intrabody (iNbSyt1) and is minimally invasive, leaving synaptic transmission almost unaffected, as demonstrated by the crystal structure of the NbSyt1 bound to synaptotagmin-1 and by our physiological data. Its single-domain nature enables the generation of protein-based fluorescent reporters, as we showcase here by measuring spatially-localized presynaptic Ca2+with an NbSyt1-jGCaMP8 chimera. Moreover, its small size makes the NbSyt1 ideal for various super-resolution imaging methods. Overall, NbSyt1 is a versatile binder that will enable imaging in cellular and molecular neuroscience at a higher precision than possible in the past, over multiple spatiotemporal scales.

Published

2023

13. The PPAR-γ Agonist Pioglitazone Modulates Proliferation and Migration in HUVEC, HAOSMC and Human Arteriovenous Fistula-Derived Cells

Author

Carmen Ciavarella, Ilenia Motta, Francesco Vasuri, Teresa Palumbo, Anthony Paul Lisi, Alice Costa, Annalisa Astolfi, Sabrina Valente, Piera Versura, Eugenio F. Fornasiero, Raffaella Mauro, Mauro Gargiulo, Gianandrea Pasquinelli, Ciavarella, Carmen, Motta, Ilenia, Vasuri, Francesco, Palumbo, Teresa, Lisi, Anthony Paul, Costa, Alice, Astolfi, Annalisa, Valente, Sabrina, Versura, Piera, Fornasiero, Eugenio F., Mauro, Raffaella, Gargiulo, Mauro, and Pasquinelli, Gianandrea

Subjects

PPAR-γ, arteriovenous fistula (AVF), proliferation, Organic Chemistry, General Medicine, migration, Catalysis, Computer Science Applications, Inorganic Chemistry, primary arteriovenous fistula cell model (AVFCs), HAOSMC, HUVEC, pioglitazone, intimal hyperplasia (IH), Physical and Theoretical Chemistry, Molecular Biology, Spectroscopy

Abstract

The failure of arteriovenous fistulas (AVFs) following intimal hyperplasia (IH) increases morbidity and mortality rates in patients undergoing hemodialysis for chronic kidney disease. The peroxisome-proliferator associated receptor (PPAR-γ) may be a therapeutic target in IH regulation. In the present study, we investigated PPAR-γ expression and tested the effect of pioglitazone, a PPAR-γ agonist, in different cell types involved in IH. As cell models, we used Human Endothelial Umbilical Vein Cells (HUVEC), Human Aortic Smooth Muscle Cells (HAOSMC), and AVF cells (AVFCs) isolated from (i) normal veins collected at the first AVF establishment (T0), and (ii) failed AVF with IH (T1). PPAR-γ was downregulated in AVF T1 tissues and cells, in comparison to T0 group. HUVEC, HAOSMC, and AVFC (T0 and T1) proliferation and migration were analyzed after pioglitazone administration, alone or in combination with the PPAR-γ inhibitor, GW9662. Pioglitazone negatively regulated HUVEC and HAOSMC proliferation and migration. The effect was antagonized by GW9662. These data were confirmed in AVFCs T1, where pioglitazone induced PPAR-γ expression and downregulated the invasive genes SLUG, MMP-9, and VIMENTIN. In summary, PPAR-γ modulation may represent a promising strategy to reduce the AVF failure risk by modulating cell proliferation and migration.

Published

2023

14. Age-dependent structural reorganization of utricular ribbon synapses

Author

Susann Michanski, Timo Henneck, Mohona Mukhopadhyay, Anna M. Steyer, Paola Agüi Gonzalez, Katharina Grewe, Peter Ilgen, Mehmet Gültas, Eugenio F. Fornasiero, Stefan Jakobs, Wiebke Möbius, Christian Vogl, Tina Pangršič, Silvio O. Rizzoli, and Carolin Wichmann

Abstract

In mammals, spatial orientation is synaptically-encoded by sensory hair cells of the vestibular labyrinth. Vestibular hair cells (VHCs) harbor synaptic ribbons at their presynaptic active zones (AZs), which play a critical role in molecular scaffolding and facilitate synaptic release and vesicular replenishment. With advancing age, the prevalence of vestibular deficits increases; yet, a direct link to the functional decline of VHC ribbon synapses remains to be demonstrated. To address this issue, we investigated the effects of aging on the ultrastructure of the ribbon-type AZs in murine utricles using various electron microscopic techniques and combined them with confocal and super-resolution light microscopy as well as metabolic imaging up to one year of age. In older animals, we detected predominantly in type I VHCs the formation of floating ribbon clusters. Our findings suggest that VHC ribbon-type AZs undergo dramatic structural alterations upon aging.

Published

2022

15. IGF-1 receptor regulates upward firing rate homeostasis via the mitochondrial calcium uniporter

Author

Maxim Katsenelson, Ilana Shapira, Eman Abbas, Kristina Jevdokimenko, Boaz Styr, Antonella Ruggiero, Saba Aïd, Eugenio F. Fornasiero, Martin Holzenberger, Silvio O. Rizzoli, and Inna Slutsky

Subjects

Mice, Neuronal Plasticity, Multidisciplinary, Animals, Homeostasis, Reproducibility of Results, Calcium, Calcium Channels, Gene Deletion, Receptor, IGF Type 1

Abstract

Regulation of firing rate homeostasis constitutes a fundamental property of central neural circuits. While intracellular Ca 2+ has long been hypothesized to be a feedback control signal, the molecular machinery enabling a network-wide homeostatic response remains largely unknown. We show that deletion of insulin-like growth factor-1 receptor (IGF-1R) limits firing rate homeostasis in response to inactivity, without altering the distribution of baseline firing rates. The deficient firing rate homeostatic response was due to disruption of both postsynaptic and intrinsic plasticity. At the cellular level, we detected a fraction of IGF-1Rs in mitochondria, colocalized with the mitochondrial calcium uniporter complex (MCUc). IGF-1R deletion suppressed transcription of the MCUc members and burst-evoked mitochondrial Ca 2+ (mitoCa 2+ ) by weakening mitochondria-to-cytosol Ca 2+ coupling. Overexpression of either mitochondria-targeted IGF-1R or MCUc in IGF-1R–deficient neurons was sufficient to rescue the deficits in burst-to-mitoCa 2+ coupling and firing rate homeostasis. Our findings indicate that mitochondrial IGF-1R is a key regulator of the integrated homeostatic response by tuning the reliability of burst transfer by MCUc. Based on these results, we propose that MCUc acts as a homeostatic Ca 2+ sensor. Faulty activation of MCUc may drive dysregulation of firing rate homeostasis in aging and in brain disorders associated with aberrant IGF-1R/MCUc signaling.

Published

2022

16. Protein lifetimes in aged brains reveal a proteostatic adaptation linking physiological aging to neurodegeneration

Author

Verena Kluever, Belisa Russo, Sunit Mandad, Nisha Hemandhar Kumar, Mihai Alevra, Alessandro Ori, Silvio O. Rizzoli, Henning Urlaub, Anja Schneider, and Eugenio F. Fornasiero

Subjects

Proteomics, Aging, Mice, Multidisciplinary, metabolism [Brain], Proteolysis, Brain, Animals, Neurodegenerative Diseases, ddc:500, metabolism [Aging], metabolism [Neurodegenerative Diseases], etiology [Neurodegenerative Diseases]

Abstract

Aging is a prominent risk factor for neurodegenerative disorders (NDDs); however, the molecular mechanisms rendering the aged brain particularly susceptible to neurodegeneration remain unclear. Here, we aim to determine the link between physiological aging and NDDs by exploring protein turnover using metabolic labeling and quantitative pulse-SILAC proteomics. By comparing protein lifetimes between physiologically aged and young adult mice, we found that in aged brains protein lifetimes are increased by ~20% and that aging affects distinct pathways linked to NDDs. Specifically, a set of neuroprotective proteins are longer-lived in aged brains, while some mitochondrial proteins linked to neurodegeneration are shorter-lived. Strikingly, we observed a previously unknown alteration in proteostasis that correlates to parsimonious turnover of proteins with high biosynthetic costs, revealing an overall metabolic adaptation that preludes neurodegeneration. Our findings suggest that future therapeutic paradigms, aimed at addressing these metabolic adaptations, might be able to delay NDD onset.

Published

2022

17. Toward a hypothesis‐free understanding of how phosphorylation dynamically impacts protein turnover

Author

Wenxue Li, Barbora Salovska, Eugenio F. Fornasiero, and Yansheng Liu

Subjects

Molecular Biology, Biochemistry

Abstract

The turnover measurement of proteins and proteoforms has been largely facilitated by workflows coupling metabolic labeling with mass spectrometry (MS), including dynamic stable isotope labeling by amino acids in cell culture (dynamic SILAC) or pulsed SILAC (pSILAC). Very recent studies including ours have integrated themeasurement of post-translational modifications (PTMs) at the proteome level (i.e., phosphoproteomics) with pSILAC experiments in steady state systems, exploring the link between PTMs and turnover at the proteome-scale. An open question in the field is how to exactly interpret these complex datasets in a biological perspective. Here, we present a novel pSILAC phosphoproteomic dataset which was obtained during a dynamic process of cell starvation using data-independent acquisition MS (DIA-MS). To provide an unbiased "hypothesis-free" analysis framework, we developed a strategy to interrogate how phosphorylation dynamically impacts protein turnover across the time series data. With this strategy, we discovered a complex relationship between phosphorylation and protein turnover that was previously underexplored. Our results further revealed a link between phosphorylation stoichiometry with the turnover of phosphorylated peptidoforms. Moreover, our results suggested that phosphoproteomic turnover diversity cannot directly explain the abundance regulation of phosphorylation during cell starvation, underscoring the importance of future studies addressing PTM site-resolved protein turnover.

Published

2022

18. Respective, Time‐dependent Phosphorylation Modules Shaping Phosphoproteome Abundance and Turnover

Author

Qian Ba, Archer Hamidzadeh, Eugenio F. Fornasiero, Wenxue Li, Anatoly Kiyatkin, Barbora Salovska, and Yansheng Liu

Subjects

0303 health sciences, 03 medical and health sciences, 0302 clinical medicine, Chemistry, Abundance (ecology), Genetics, Phosphorylation, Molecular Biology, Biochemistry, 030217 neurology & neurosurgery, 030304 developmental biology, Biotechnology, Cell biology

Published

2021

19. Influence of Subcellular Localization and Functional State on Protein Turnover

Author

Kristina Jevdokimenko, Eugenio F. Fornasiero, Verena Kluever, Roya Yousefi, and David Pacheu-Grau

Subjects

Calmodulin, QH301-705.5, Recombinant Fusion Proteins, Rab5a, Article, pulse-chase, 03 medical and health sciences, 0302 clinical medicine, Protein biosynthesis, Humans, Biology (General), 030304 developmental biology, 0303 health sciences, SNAP-tag, biology, Chemistry, Cell Membrane, Protein turnover, optical analysis of protein turnover, Proteins, Reproducibility of Results, General Medicine, Subcellular localization, Protein subcellular localization prediction, Cell biology, Protein Transport, Proteostasis, protein stability, Proteome, biology.protein, Mutant Proteins, 030217 neurology & neurosurgery, HeLa Cells, Protein Binding, Subcellular Fractions

Abstract

Protein homeostasis is an equilibrium of paramount importance that maintains cellular performance by preserving an efficient proteome. This equilibrium avoids the accumulation of potentially toxic proteins, which could lead to cellular stress and death. While the regulators of proteostasis are the machineries controlling protein production, folding and degradation, several other factors can influence this process. Here, we have considered two factors influencing protein turnover: the subcellular localization of a protein and its functional state. For this purpose, we used an imaging approach based on the pulse-labeling of 17 representative SNAP-tag constructs for measuring protein lifetimes. With this approach, we obtained precise measurements of protein turnover rates in several subcellular compartments. We also tested a selection of mutants modulating the function of three extensively studied proteins, the Ca2+ sensor calmodulin, the small GTPase Rab5a and the brain creatine kinase (CKB). Finally, we followed up on the increased lifetime observed for the constitutively active Rab5a (Q79L), and we found that its stabilization correlates with enlarged endosomes and increased interaction with membranes. Overall, our data reveal that both changes in protein localization and functional state are key modulators of protein turnover, and protein lifetime fluctuations can be considered to infer changes in cellular behavior.

Published

2021

20. In Vivo Protein Lifetime Measurements Across Multiple Organs in the Zebrafish

Author

Sunit, Mandad, Gudrun, Kracht, and Eugenio F, Fornasiero

Subjects

Male, Proteomics, Proteome, Isotope Labeling, Lysine, Animals, Female, Amino Acids, Zebrafish Proteins, Zebrafish, Half-Life

Abstract

Protein production and degradation are tightly regulated to prevent cellular structures from accumulating damage and to allow their correct functioning. A key aspect of this regulation is the protein half-life, corresponding to the time in which half of a specific protein population is exchanged with respect to its initial state. Proteome-wide techniques to investigate protein half-lives in vivo are emerging. Recently, we have established and thoroughly tested a metabolic labeling approach using

Published

2021

21. Monitoring mitochondrial translation in living cells

Author

Julio Montoya, Eugenio F. Fornasiero, David Pacheu-Grau, Peter Rehling, Stefan Jakobs, Silvio O. Rizzoli, Roya Yousefi, and Lukas Cyganek

Subjects

Mitochondrial DNA, Mitochondrial translation, Cellular differentiation, translation, Context (language use), Methods & Resources, Mitochondrion, Biology, Biochemistry, Genome, Oxidative Phosphorylation, Mitochondrial Proteins, 03 medical and health sciences, 0302 clinical medicine, synapse, Report, Genetics, Humans, Molecular Biology, 030304 developmental biology, 0303 health sciences, Organelle Biogenesis, Translation (biology), Protein Biosynthesis & Quality Control, Mitochondria, Cell biology, hippocampal neuron, Mitochondrial biogenesis, Protein Biosynthesis, gene expression, 030217 neurology & neurosurgery, Reports

Abstract

Mitochondria possess a small genome that codes for core subunits of the oxidative phosphorylation system and whose expression is essential for energy production. Information on the regulation and spatial organization of mitochondrial gene expression in the cellular context has been difficult to obtain. Here we devise an imaging approach to analyze mitochondrial translation within the context of single cells, by following the incorporation of clickable non‐canonical amino acids. We apply this method to multiple cell types, including specialized cells such as cardiomyocytes and neurons, and monitor with spatial resolution mitochondrial translation in axons and dendrites. We also show that translation imaging allows to monitor mitochondrial protein expression in patient fibroblasts. Approaching mitochondrial translation with click chemistry opens new avenues to understand how mitochondrial biogenesis is integrated into the cellular context and can be used to assess mitochondrial gene expression in mitochondrial diseases., This study monitors mitochondrial protein synthesis with spatial resolution in single cells of multiple cell types.

Published

2021

22. Centrosome-dependent microtubule modifications set the conditions for axon formation

Author

Durga Praveen Meka, Oliver Kobler, Shuai Hong, Carina Meta Friedrich, Souhaila Wuesthoff, Melad Henis, Birgit Schwanke, Christoph Krisp, Nessa Schmuelling, René Rueter, Tabitha Ruecker, Ewelina Betleja, Tao Cheng, Moe R. Mahjoub, Peter Soba, Hartmut Schlüter, Eugenio F. Fornasiero, and Froylan Calderon de Anda

Subjects

Centrosome, Neurons, Actin Cytoskeleton, nervous system, microtubules, Cell biology, acetylated microtubules, neuronal polarity, axon formation, centrosome, Cep120, Microtubule-Associated Proteins, Microtubules, General Biochemistry, Genetics and Molecular Biology, Axons

Abstract

Microtubule (MT) modifications are critical during axon development, with stable MTs populating the axon. How these modifications are spatially coordinated is unclear. Here, via high-resolution microscopy, we show that early developing neurons have fewer somatic acetylated MTs restricted near the centrosome. At later stages, however, acetylated MTs spread out in soma and concentrate in growing axon. Live imaging in early plated neurons of the MT plus-end protein, EB3, show increased displacement and growth rate near the MTOC, suggesting local differences that might support axon selection. Moreover, F-actin disruption in early developing neurons, which show fewer somatic acetylated MTs, does not induce multiple axons, unlike later stages. Overexpression of centrosomal protein 120 (Cep120), which promotes MT acetylation/stabilization, induces multiple axons, while its knockdown downregulates proteins modulating MT dynamics and stability, hampering axon formation. Collectively, we show how centrosome-dependent MT modifications contribute to axon formation.

Published

2021

23. Protein Phosphorylation in Depolarized Synaptosomes: Dissecting Primary Effects of Calcium from Synaptic Vesicle Cycling

Author

Ivan Silbern, Henning Urlaub, Reinhard Jahn, Kuan-Ting Pan, Stefan Bonn, Maksims Fiosins, Silvio O. Rizzoli, and Eugenio F. Fornasiero

Subjects

Botulinum Toxins, CK1, casein kinase 1, SNAP-25, synaptosomal-associated protein, 25kDa, Syntaxin 1, synaptobrevin, CLK, SRPK1 and Clk/Sty protein kinase, Biochemistry, CREB1, CAMP-responsive element binding protein 1, PAK, p21-activated kinase, Analytical Chemistry, SV, synaptic vesicle, AAV, adeno-associated virus, Receptor, Cannabinoid, CB1, TEAB, triethylammonium bicarbonate buffer, Clostridium botulinum, Syntaxin, metabolism [Calcium], metabolism [Syntaxin 1], NMDAR, N-methyl-d-aspartate receptor, metabolism [Phosphoproteins], Neurons, 0303 health sciences, AGC, automatic gain control, 030302 biochemistry & molecular biology, pharmacology [Neurotoxins], STE, “sterile” serine/threonine protein kinases, Endocytosis, Cell biology, DAPK, death-associated protein kinase, metabolism [Neurons], SNARE, RT, room temperature, GRK, G-protein-coupled receptor kinase, GluDH, glutamate dehydrogenase, Synaptic vesicle, Exocytosis, 03 medical and health sciences, PKC, protein kinase C, Humans, Rats, Wistar, Molecular Biology, metabolism [Synaptic Vesicles], metabolism [Glutamic Acid], CAA, chloroacetamide, cytology [Hippocampus], CaMKII, calcium-calmodulin kinase 2, MAPK, mitogen-activated protein kinase, HeLa Cells, ITR, inverted terminal repeat (sequence), Proteome, SNARE, N-ethylmaleimide-sensitive factor-attachment protein receptors, BoNT, botulinum neurotoxin, Hippocampus, R-SNARE Proteins, synapse, botulinum neurotoxins, Protein phosphorylation, POI, protein of interest, Phosphorylation, bRP, basic reversed-phase chromatography, CDK, cyclin-dependent kinase, FA, formic acid, TFE, trifluoroethanol, Voltage-dependent calcium channel, Chemistry, Depolarization, PP1, protein phosphatase 1, metabolism [Receptor, Cannabinoid, CB1], AMPAR, α-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptor, Synaptic Vesicles, exocytosis, syntaxin, TCEP, tris(2-carboxyethyl)phosphine, Neurotoxins, PNGase F, peptide-N(4)-(N-acetyl-beta-glucosaminyl)asparagine amidase, Glutamic Acid, AMPA receptor, Neurotransmission, phosphomimetic studies, pharmacology [Botulinum Toxins], GSK3, glycogen synthase kinase 3, Animals, AGC, protein kinase A, G, C kinase group, ddc:610, metabolism [Synaptosomes], 030304 developmental biology, GO, gene ontology, metabolism [R-SNARE Proteins], Research, cannabinoid receptor, ACN, acetonitrile, Phosphoproteins, CK2, casein kinase 2, RAS, rat sarcoma gene, Calcium, AP, action potential, CMGC, CDK, MAP, GSK, CDKL kinase group, GABA, γ-aminobutyric acid, Synaptosomes

Abstract

Synaptic transmission is mediated by the regulated exocytosis of synaptic vesicles. When the presynaptic membrane is depolarized by an incoming action potential, voltage-gated calcium channels open, resulting in the influx of calcium ions that triggers the fusion of synaptic vesicles (SVs) with the plasma membrane. SVs are recycled by endocytosis. Phosphorylation of synaptic proteins plays a major role in these processes, and several studies have shown that the synaptic phosphoproteome changes rapidly in response to depolarization. However, it is unclear which of these changes are directly linked to SV cycling and which might regulate other presynaptic functions that are also controlled by calcium-dependent kinases and phosphatases. To address this question, we analyzed changes in the phosphoproteome using rat synaptosomes in which exocytosis was blocked with botulinum neurotoxins (BoNTs) while depolarization-induced calcium influx remained unchanged. BoNT-treatment significantly alters the response of the synaptic phoshoproteome to depolarization and results in reduced phosphorylation levels when compared with stimulation of synaptosomes by depolarization with KCl alone. We dissect the primary Ca2+-dependent phosphorylation from SV-cycling-dependent phosphorylation and confirm an effect of such SV-cycling-dependent phosphorylation events on syntaxin-1a-T21/T23, synaptobrevin-S75, and cannabinoid receptor-1-S314/T322 on exo- and endocytosis in cultured hippocampal neurons., Graphical Abstract, Highlights • KCl-depolarization induces phosphoproteome changes in isolated nerve terminals (synaptosomes). • Botulinum neurotoxin affects protein phosphorylation in depolarized synaptosomes. • BoNT treatment reveals phosphorylation sites that depend on SV-cycling activity. • SV-cycling-dependent sites on Vamp2, Stx1a, and Cnr1 affect exo- and endocytosis., In Brief Analysis of protein phosphorylation in isolated nerve terminals (synaptosomes) treated with C. botulinum neurotoxins (BoNT) to inhibit synaptic vesicle (SV) cycling reveals phosphorylation events that are primarily dependent on depolarization-induced Ca2+ influx and those that also require active SV-cycling machinery. In particular, SV-cycling-dependent phosphorylation sites on synaptobrevin (Vamp2), syntaxin-1 (Stx1a), and cannabinoid receptor-1 (Cnr1) are capable of changing the rate of exo- and endocytosis in cultured hippocampal neurons.

Published

2021

24. In Vivo Protein Lifetime Measurements Across Multiple Organs in the Zebrafish

Author

Sunit Mandad, Eugenio F. Fornasiero, and Gudrun Kracht

Subjects

chemistry.chemical_classification, 0303 health sciences, education.field_of_study, biology, Protein mass spectrometry, Population, Protein turnover, Computational biology, biology.organism_classification, Amino acid, 03 medical and health sciences, 0302 clinical medicine, chemistry, Stable isotope labeling by amino acids in cell culture, Proteome, Protein biosynthesis, education, Zebrafish, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Protein production and degradation are tightly regulated to prevent cellular structures from accumulating damage and to allow their correct functioning. A key aspect of this regulation is the protein half-life, corresponding to the time in which half of a specific protein population is exchanged with respect to its initial state. Proteome-wide techniques to investigate protein half-lives in vivo are emerging. Recently, we have established and thoroughly tested a metabolic labeling approach using 13C lysine (Lys(6)) for measuring protein lifetimes in mice. The approach is based on the fact that different proteins will incorporate a metabolic label at a rate that is dependent on their half-life. Using amino acid pool modeling and mass spectrometry, it is possible to measure the fraction of newly synthesized proteins and determine protein half-lives. In this chapter, we show how to extend this approach to zebrafish (Danio rerio), using a commercially available fish diet based on the stable isotope labeling by amino acids in cell culture (SILAC) technology. We describe the methods for labeling animals and subsequently use mass spectrometry to determine the lifetimes of a large number of proteins. In the mass spectrometry workflow proposed here, we have implemented the BoxCar data acquisition approach for increasing sample coverage and optimize machine use. To establish the proteome library used in the BoxCar approach, we recommend performing an in-solution digestion followed by peptide fractionation through basic reversed-phase chromatography. Overall, this chapter extends the use of current proteome technologies for the quantification of protein turnover to zebrafish and similar organisms and permits the study of germline changes following specific manipulations.

Published

2021

25. Centrosome-dependent microtubule organization sets the conditions for axon formation

Author

T. Ruecker, Oliver Kobler, R. Rueter, Christoph Krisp, N. Schmuelling, Eugenio F. Fornasiero, Hartmut Schlüter, F. Calderon de Anda, Birgit Schwanke, S. Wuesthoff, and Durga Praveen Meka

Subjects

0303 health sciences, Somatic cell, Microtubule organizing center, Biology, Cell biology, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, nervous system, Microtubule, Acetylation, Centrosome, medicine, Soma, Axon, Cytoskeleton, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Microtubule remodeling is critical during axon development when the more stable microtubules populate the axon. It is not completely understood, however, how this local cytoskeleton remodeling is coordinated. The centrosome, the main microtubule-organizing center (MTOC), has been suggested to be crucial for axon specification 1–5. Conversely, it was proposed that axon elongation is independent of centrosomal functions 6. Here we report that microtubule dynamics in early neurons follow a radial organization which establishes the conditions for the axon formation. Using high-resolution microscopy of early developing neurons, we demonstrate that few somatic acetylated microtubules are restricted near the centrosome. At later stages, however, acetylated microtubules spread out in the soma and concentrate in the growing axon. Furthermore, live-imaging of the microtubule plus-end binding protein EB3 in early differentiating neurons shows that growing microtubules have increased length and growth speed near the MTOC, suggesting local differences that might favor axon selection. Importantly, due to the lack of somatic stable/acetylated microtubules in early developing neurons, disruption of the F-actin cytoskeleton does not induce multiple axons, as it does at later stages of differentiation. Finally, we demonstrate that overexpression of the centrosomal protein 120 (Cep120), known for promoting microtubule acetylation and stabilization, induces multiple axons, while its downregulation decreases the content of proteins regulating microtubule dynamics and stability, hence hampering axon formation. Collectively, our data show that early centrosome-dependent microtubule organization contributes to axon formation.

Published

2020

26. Local translation in synaptic mitochondria influences synaptic transmission

Author

Eugenio F. Fornasiero, Peter Rehling, Roya Yousefi, David Pacheu Grau, Stefan Jakobs, Silvio O. Rizzoli, and Lukas Cyganek

Subjects

Mitochondrial DNA, Cell type, Mitochondrial translation, Context (language use), Translation (biology), Mitochondrion, Neurotransmission, Biology, Genome, Cell biology

Abstract

Mitochondria possess a small genome that codes for core subunits of the oxidative phosphorylation system, and whose expression is essential for energy production. Information on the regulation and spatial organization of mitochondrial gene expression in the cellular context has been difficult to obtain. Here we addressed this by devising an imaging approach to analyze mitochondrial translation, by following the incorporation of clickable non-canonical amino acids. We applied this method to multiple cell types, including hippocampal neurons, where we found ample evidence for mitochondrial translation in both dendrites and axons. Translation levels were surprisingly heterogeneous, were typically stronger in axons, and were independent of their distance from the cell soma, where mitochondria presumably descent from. Presynaptic mitochondrial translation correlated with local synaptic activity, and blocking mitochondria translation reduced synaptic function. Overall, these findings demonstrate that mitochondrial gene expression in neurons is intimately linked to neuronal function.

Published

2020

27. A Reliable Approach for Revealing Molecular Targets in Secondary Ion Mass Spectrometry

Author

Fengxia Li, Eugenio F. Fornasiero, Tal M. Dankovich, Verena Kluever, and Silvio O. Rizzoli

Subjects

Organelles, Organic Chemistry, Spectrometry, Mass, Secondary Ion, General Medicine, nanoSIMS, mass spectrometry imaging, immunogold labeling, protein turnover, Catalysis, Computer Science Applications, Inorganic Chemistry, Microscopy, Electron, Microscopy, Fluorescence, Gold, Physical and Theoretical Chemistry, Molecular Biology, Spectroscopy

Abstract

Nano secondary ion mass spectrometry (nanoSIMS) imaging is a rapidly growing field in biological sciences, which enables investigators to describe the chemical composition of cells and tissues with high resolution. One of the major challenges of nanoSIMS is to identify specific molecules or organelles, as these are not immediately recognizable in nanoSIMS and need to be revealed by SIMS-compatible probes. Few laboratories have generated such probes, and none are commercially available. To address this, we performed a systematic study of probes initially developed for electron microscopy. Relying on nanoscale SIMS, we found that antibodies coupled to 6 nm gold particles are surprisingly efficient in terms of labeling specificity while offering a reliable detection threshold. These tools enabled accurate visualization and sample analysis and were easily employed in correlating SIMS with other imaging approaches, such as fluorescence microscopy. We conclude that antibodies conjugated to moderately sized gold particles are promising tools for SIMS imaging.

Published

2022

28. Synapsin I deletion reduces neuronal damage and ameliorates clinical progression of experimental autoimmune encephalomyelitis

Author

Luca Muzio, Roberto Furlan, Annamaria Finardi, Eugenio F. Fornasiero, Elena Monzani, Flavia Valtorta, Andrea Bergamaschi, Serena Bellani, Latefa Yekhlef, Riccardo Fesce, Fabrizia C. Guarnieri, Gianvito Martino, Davide Pozzi, Stefano Taverna, Michela Matteoli, Guarnieri, Fabrizia C., Bellani, Serena, Yekhlef, Latefa, Bergamaschi, Andrea, Finardi, Annamaria, Fesce, Riccardo, Pozzi, Davide, Monzani, Elena, Fornasiero, Eugenio F., Matteoli, Michela, Martino, Gianvito, Furlan, Roberto, Taverna, Stefano, Muzio, Luca, and Valtorta, Flavia

Subjects

0301 basic medicine, Synapsin I, Encephalomyelitis, Autoimmune, Experimental, MAP Kinase Signaling System, Immunology, Biology, Hippocampus, Synaptic vesicle, Endocrine and Autonomic System, Multiple sclerosis, Synapse, Mice, 03 medical and health sciences, Behavioral Neuroscience, 0302 clinical medicine, medicine, Animals, Multiple sclerosi, Phosphorylation, Cognitive decline, Cytokine, Inflammation, Mice, Knockout, Neurons, Endocrine and Autonomic Systems, Experimental autoimmune encephalomyelitis, Brain, Synapsin, Neuron, Synapsins, medicine.disease, Mice, Inbred C57BL, Disease Models, Animal, Neuroprotective Agents, 030104 developmental biology, medicine.anatomical_structure, Synapses, Disease Progression, Cytokines, Synaptic Vesicles, Neuroscience, 030217 neurology & neurosurgery

Abstract

The classical view of multiple sclerosis (MS) pathogenesis states that inflammation-mediated demyelination is responsible for neuronal damage and loss. However, recent findings show that impairment of neuronal functions and demyelination can be independent events, suggesting the coexistence of other pathogenic mechanisms. Due to the inflammatory milieu, subtle alterations in synaptic function occur, which are probably at the basis of the early cognitive decline that often precedes the neurodegenerative phases in MS patients. In particular, it has been reported that inflammation enhances excitatory synaptic transmission while it decreases GABAergic transmission in vitro and ex vivo. This evidence points to the idea that an excitation/inhibition imbalance occurs in the inflamed MS brain, even though the exact molecular mechanisms leading to this synaptic dysfunction are as yet not completely clear. Along this line, we observed that acute treatment of primary hippocampal neurons in culture with pro-inflammatory cytokines leads to an increased phosphorylation of synapsin I (SynI) by ERK1/2 kinase and to an increase in the frequency of spontaneous synaptic vesicle release events, which is prevented by SynI deletion. In vivo, the ablation of SynI expression is protective in terms of disease progression and neuronal damage in the experimental autoimmune encephalomyelitis mouse model of MS. Our results point to a possible key role in MS pathogenesis of the neuronal protein SynI, a regulator of excitation/inhibition balance in neuronal networks.

Published

2018

29. Principles of brain aging: Status and challenges of modeling human molecular changes in mice

Author

Eugenio F. Fornasiero and Verena Kluever

Subjects

Aging, Future studies, Context (language use), Biology, Biochemistry, Mice, 03 medical and health sciences, Life Expectancy, 0302 clinical medicine, medicine, Animals, Humans, Dementia, Cognitive Dysfunction, Cognitive decline, Molecular Biology, Brain aging, 030304 developmental biology, 0303 health sciences, Neurodegeneration, Brain, medicine.disease, Molecular analysis, Disease Models, Animal, Neurology, Life expectancy, Neuroscience, 030217 neurology & neurosurgery, Biotechnology

Abstract

Due to the extension of human life expectancy, the prevalence of cognitive impairment is rising in the older portion of society. Developing new strategies to delay or attenuate cognitive decline is vital. For this purpose, it is imperative to understand the cellular and molecular events at the basis of brain aging. While several organs are directly accessible to molecular analysis through biopsies, the brain constitutes a notable exception. Most of the molecular studies are performed on postmortem tissues, where cell death and tissue damage have already occurred. Hence, the study of the molecular aspects of cognitive decline largely relies on animal models and in particular on small mammals such as mice. What have we learned from these models? Do these animals recapitulate the changes observed in humans? What should we expect from future mouse studies? In this review we answer these questions by summarizing the state of the research that has addressed cognitive decline in mice from several perspectives, including genetic manipulation and omics strategies. We conclude that, while extremely valuable, mouse models have limitations that can be addressed by the optimal design of future studies and by ensuring that results are cross-validated in the human context.

Published

2021

30. A comparative analysis of the mobility of 45 proteins in the synaptic bouton

Author

Burkhard Rammner, Silvio O. Rizzoli, Eugenio F. Fornasiero, Jan-Eike Ußling, Thomas Schikorski, Sarah Köster, Sofiia Reshetniak, Eleonora Perego, and Sven Truckenbrodt

Subjects

Resource, Models, Neurological, Nerve Tissue Proteins, Neurotransmission, Biology, Synaptic vesicle, Hippocampus, Synaptic Transmission, General Biochemistry, Genetics and Molecular Biology, Exocytosis, Synapse, 03 medical and health sciences, 0302 clinical medicine, synapse, Animals, Cytoskeleton, Molecular Biology, vesicle, 030304 developmental biology, Neurons, 0303 health sciences, General Immunology and Microbiology, General Neuroscience, Vesicle, diffusion, Fluorescence recovery after photobleaching, Rats, Protein Transport, Membrane protein, Biophysics, Synaptic Vesicles, movement, 030217 neurology & neurosurgery, protein mobility, Neuroscience

Abstract

Many proteins involved in synaptic transmission are well known, and their features, as their abundance or spatial distribution, have been analyzed in systematic studies. This has not been the case, however, for their mobility. To solve this, we analyzed the motion of 45 GFP‐tagged synaptic proteins expressed in cultured hippocampal neurons, using fluorescence recovery after photobleaching, particle tracking, and modeling. We compared synaptic vesicle proteins, endo‐ and exocytosis cofactors, cytoskeleton components, and trafficking proteins. We found that movement was influenced by the protein association with synaptic vesicles, especially for membrane proteins. Surprisingly, protein mobility also correlated significantly with parameters as the protein lifetimes, or the nucleotide composition of their mRNAs. We then analyzed protein movement thoroughly, taking into account the spatial characteristics of the system. This resulted in a first visualization of overall protein motion in the synapse, which should enable future modeling studies of synaptic physiology., Live imaging reveals global protein dynamics in the synaptic bouton, providing a first visualization of overall protein motion in the synapse and showing connections between protein characteristics and mobility in vivo.

Published

2020

31. A mass spectrometry workflow for measuring protein turnover rates in vivo

Author

Mihai Alevra, Sunit Mandad, Henning Urlaub, Eugenio F. Fornasiero, Till Ischebeck, and Silvio O. Rizzoli

Subjects

Male, Proteomics, Proteome, Computer science, Computational biology, Mass spectrometry, General Biochemistry, Genetics and Molecular Biology, Mass Spectrometry, Workflow, 03 medical and health sciences, Mice, 0302 clinical medicine, Time frame, In vivo, Animals, Amino Acids, 030304 developmental biology, 0303 health sciences, Protein turnover, Proteins, Reproducibility of Results, Mice, Inbred C57BL, Metabolic labeling, Isotope Labeling, Protein Biosynthesis, Proteolysis, Stable Isotope Labeling, 030217 neurology & neurosurgery

Abstract

Proteins are continually produced and degraded, to avoid the accumulation of old or damaged molecules and to maintain the efficiency of physiological processes. Despite its importance, protein turnover has been difficult to measure in vivo. Previous approaches to evaluating turnover in vivo have required custom labeling approaches, involved complex mass spectrometry (MS) analyses, or used comparative strategies that do not allow direct quantitative measurements. Here, we describe a robust protocol for quantitative proteome turnover analysis in mice that is based on a commercially available diet for stable isotope labeling of amino acids in mammals (SILAM). We start by discussing fundamental concepts of protein turnover, including different methodological approaches. We then cover in detail the practical aspects of metabolic labeling and explain both the experimental and computational steps that must be taken to obtain accurate in vivo results. Finally, we present a simple experimental workflow that enables measurement of precise turnover rates in a time frame of ~4-5 weeks, including the labeling time. We also provide all the scripts needed for the interpretation of the MS results and for comparing turnover across different conditions. Overall, the workflow presented here comprises several improvements in the determination of protein lifetimes with respect to other available methods, including a minimally invasive labeling strategy and a robust interpretation of MS results, thus enhancing reproducibility across laboratories.

Published

2019

32. Global and Site-Specific Effect of Phosphorylation on Protein Turnover

Author

George Rosenberger, Barbora Salovska, Yansheng Liu, Chongde Wu, Qian Ba, Erli Gao, Dayun Lu, Torsten Mueller, Hu Zhou, Pingfu Hou, Eugenio F. Fornasiero, Yi Di, and Wenxue Li

Subjects

Proteomics, Cell signaling, Proteome, Biology, Article, Mass Spectrometry, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, 0302 clinical medicine, Glutamates, Cell Line, Tumor, Humans, Data-independent acquisition, Amino Acid Sequence, Phosphorylation, Molecular Biology, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, Kinase, Cell Cycle, Protein turnover, Phosphoproteomics, Cell Biology, Phosphoproteins, Cyclin-Dependent Kinases, Cell biology, Amino acid, chemistry, Isotope Labeling, Proteolysis, RNA Splicing Factors, Peptides, 030217 neurology & neurosurgery, Peroxiredoxin VI, Signal Transduction, Developmental Biology

Abstract

To date, the effects of specific modification types and sites on protein lifetime have not been systematically illustrated. Here, we describe a proteomic method, DeltaSILAC, to quantitatively assess the impact of site-specific phosphorylation on the turnover of thousands of proteins in live cells. Based on the accurate and reproducible mass spectrometry-based method, a pulse labeling approach using stable isotope-labeled amino acids in cells (pSILAC), phosphoproteomics, and a unique peptide-level matching strategy, our DeltaSILAC profiling revealed a global, unexpected delaying effect of many phosphosites on protein turnover. We further found that phosphorylated sites accelerating protein turnover are functionally selected for cell fitness, enriched in Cyclin-dependent kinase substrates, and evolutionarily conserved, whereas the glutamic acids surrounding phosphosites significantly delay protein turnover. Our method represents a generalizable approach and provides a rich resource for prioritizing the effects of phosphorylation sites on protein lifetime in the context of cell signaling and disease biology.

Published

2021

33. The long noncoding RNA neuroLNC regulates presynaptic activity by interacting with the neurodegeneration-associated protein TDP-43

Author

Verena Kluever, Stefan Bonn, Vikas Bansal, Henning Urlaub, J. D. Wren, Silvio O. Rizzoli, E. Fritsch, Eugenio F. Fornasiero, Annette Gärtner, L. Caldi Gomes, Sunit Mandad, Raza-Ur Rahman, Sarva Keihani, and S. Kügler

Subjects

Hippocampus, Interactome, chemistry.chemical_compound, Mice, 0302 clinical medicine, Cell Movement, Neurotransmitter, Research Articles, Neurons, Neurotransmitter Agents, 0303 health sciences, Multidisciplinary, Neurodegeneration, SciAdv r-articles, metabolism [Neurotransmitter Agents], Long non-coding RNA, Chromatin, Cell biology, DNA-Binding Proteins, genetics [Neurogenesis], metabolism [Neurons], RNA, Long Noncoding, Synaptic Vesicles, RNA extraction, ddc:500, metabolism [DNA-Binding Proteins], Research Article, Neurogenesis, Neurophysiology, genetics [DNA-Binding Proteins], Mice, Transgenic, Transfection, Synaptic vesicle, metabolism [RNA, Messenger], protein TDP-43, RNA neuroLNC, 03 medical and health sciences, Developmental Neuroscience, mental disorders, medicine, Animals, Humans, RNA, Messenger, Rats, Wistar, metabolism [Synaptic Vesicles], 030304 developmental biology, genetics [Cell Movement], nutritional and metabolic diseases, RNA, medicine.disease, nervous system diseases, Rats, HEK293 Cells, chemistry, cytology [Hippocampus], metabolism [RNA, Long Noncoding], 030217 neurology & neurosurgery

Abstract

NeuroLNC, a previously unknown long ncRNA, regulates neuronal activity by interacting with the neurodegeneration protein TDP-43., The cellular and the molecular mechanisms by which long noncoding RNAs (lncRNAs) may regulate presynaptic function and neuronal activity are largely unexplored. Here, we established an integrated screening strategy to discover lncRNAs implicated in neurotransmitter and synaptic vesicle release. With this approach, we identified neuroLNC, a neuron-specific nuclear lncRNA conserved from rodents to humans. NeuroLNC is tuned by synaptic activity and influences several other essential aspects of neuronal development including calcium influx, neuritogenesis, and neuronal migration in vivo. We defined the molecular interactors of neuroLNC in detail using chromatin isolation by RNA purification, RNA interactome analysis, and protein mass spectrometry. We found that the effects of neuroLNC on synaptic vesicle release require interaction with the RNA-binding protein TDP-43 (TAR DNA binding protein-43) and the selective stabilization of mRNAs encoding for presynaptic proteins. These results provide the first proof of an lncRNA that orchestrates neuronal excitability by influencing presynaptic function.

Published

2019

34. The codon sequences predict protein lifetimes and other parameters of the protein life cycle in the mouse brain

Author

Tonatiuh Pena Centeno, Koray Kirli, Sunit Mandad, Inga Urban, Hanna Wildhagen, Ramon O. Vidal, Eva Benito, Burkhard Rammner, Eugenio F. Fornasiero, Andre Fischer, Peter Rehling, Ivo Feussner, Sven Dennerlein, Roya Yousefi, Till Ischebeck, Stefan Bonn, Sarva Keihani, Raza-Ur Rahman, Felipe Opazo, Henning Urlaub, and Silvio O. Rizzoli

Subjects

0301 basic medicine, mouse brain, protein life cycle, lcsh:Medicine, Nerve Tissue Proteins, Biology, Proteomics, metabolism [RNA, Messenger], Article, Mice, genetics [RNA, Messenger], 03 medical and health sciences, 0302 clinical medicine, In vivo, Animals, Nucleotide, Amino Acid Sequence, RNA, Messenger, Amino Acids, lcsh:Science, Codon, genetics [Nerve Tissue Proteins], genetics [Amino Acids], chemistry.chemical_classification, Base Composition, Messenger RNA, Multidisciplinary, Base Sequence, Nucleotides, lcsh:R, genetics [Codon], Brain, Translation (biology), In vitro, Amino acid, Cell biology, genetics [Nucleotides], 030104 developmental biology, chemistry, metabolism [Brain], Proteome, Proteostasis, lcsh:Q, genetics [Base Composition], chemistry [Nerve Tissue Proteins], ddc:600, 030217 neurology & neurosurgery

Abstract

The homeostasis of the proteome depends on the tight regulation of the mRNA and protein abundances, of the translation rates, and of the protein lifetimes. Results from several studies on prokaryotes or eukaryotic cell cultures have suggested that protein homeostasis is connected to, and perhaps regulated by, the protein and the codon sequences. However, this has been little investigated for mammals in vivo. Moreover, the link between the coding sequences and one critical parameter, the protein lifetime, has remained largely unexplored, both in vivo and in vitro. We tested this in the mouse brain, and found that the percentages of amino acids and codons in the sequences could predict all of the homeostasis parameters with a precision approaching experimental measurements. A key predictive element was the wobble nucleotide. G-/C-ending codons correlated with higher protein lifetimes, protein abundances, mRNA abundances and translation rates than A-/U-ending codons. Modifying the proportions of G-/C-ending codons could tune these parameters in cell cultures, in a proof-of-principle experiment. We suggest that the coding sequences are strongly linked to protein homeostasis in vivo, albeit it still remains to be determined whether this relation is causal in nature.

Published

2018

35. Newly produced synaptic vesicle proteins are preferentially used in synaptic transmission

Author

Sven Truckenbrodt, Sebastian Jähne, Hanna Wildhagen, Angela Vogts, Annette Denker, Eugenio F. Fornasiero, Abhiyan Viplav, and Silvio O. Rizzoli

Subjects

0301 basic medicine, Neurotransmitter transporter, Synaptosomal-Associated Protein 25, Vesicle-Associated Membrane Protein 2, Vesicular Inhibitory Amino Acid Transport Proteins, Biology, Neurotransmission, Synaptic vesicle, Hippocampus, Synaptic Transmission, General Biochemistry, Genetics and Molecular Biology, Synaptotagmin 1, Article, Exocytosis, Mass Spectrometry, synaptic vesicle, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, organelle aging, Animals, Neurotransmitter, Molecular Biology, Cells, Cultured, vesicle pools, Neurons, General Immunology and Microbiology, VAMP2, General Neuroscience, Vesicle, turnover, Articles, Fusion protein, Cell biology, Rats, 030104 developmental biology, chemistry, Protein Biosynthesis, Synaptotagmin I, Synaptic Vesicles, 030217 neurology & neurosurgery, protein aging, Neuroscience

Abstract

Aged proteins can become hazardous to cellular function, by accumulating molecular damage. This implies that cells should preferentially rely on newly produced ones. We tested this hypothesis in cultured hippocampal neurons, focusing on synaptic transmission. We found that newly synthesized vesicle proteins were incorporated in the actively recycling pool of vesicles responsible for all neurotransmitter release during physiological activity. We observed this for the calcium sensor Synaptotagmin 1, for the neurotransmitter transporter VGAT, and for the fusion protein VAMP2 (Synaptobrevin 2). Metabolic labeling of proteins and visualization by secondary ion mass spectrometry enabled us to query the entire protein makeup of the actively recycling vesicles, which we found to be younger than that of non‐recycling vesicles. The young vesicle proteins remained in use for up to ~ 24 h, during which they participated in recycling a few hundred times. They were afterward reluctant to release and were degraded after an additional ~ 24–48 h. We suggest that the recycling pool of synaptic vesicles relies on newly synthesized proteins, while the inactive reserve pool contains older proteins.

Published

2018

36. Super-resolution imaging for cell biologists

Author

Felipe Opazo and Eugenio F. Fornasiero

Subjects

Microscopy, Computer science, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, STED microscopy, Multiple target, Data science, Superresolution, General Biochemistry, Genetics and Molecular Biology, Characterization (materials science)

Abstract

The recent 2014 Nobel Prize in chemistry honored an era of discoveries and technical advancements in the field of super-resolution microscopy. However, the applications of diffraction-unlimited imaging in biology have a long road ahead and persistently engage scientists with new challenges. Some of the bottlenecks that restrain the dissemination of super-resolution techniques are tangible, and include the limited performance of affinity probes and the yet not capillary diffusion of imaging setups. Likewise, super-resolution microscopy has introduced new paradigms in the design of projects that require imaging with nanometer-resolution and in the interpretation of biological images. Besides structural or morphological characterization, super-resolution imaging is quickly expanding towards interaction mapping, multiple target detection and live imaging. Here we review the recent progress of biologists employing super-resolution imaging, some pitfalls, implications and new trends, with the purpose of animating the field and spurring future developments.

Published

2015

37. BCAS1 expression defines a population of early myelinating oligodendrocytes in multiple sclerosis lesions

Author

Sebastian Schmitt, Mikael Simons, Christina Sergiou, Laura Starost, Marc Ehrlich, Eugenio F. Fornasiero, Henning Urlaub, Ludovico Cantuti-Castelvetri, Leda Dimou, Paula Sánchez, Christine Stadelmann, Verena Schultz, Sarah Jäkel, Sunit Mandad, Wolfgang Brück, Maryam K. Fard, Claudia Wrzos, Tanja Kuhlmann, and Franziska van der Meer

Subjects

0301 basic medicine, Multiple Sclerosis, metabolism [Myelin Sheath], Central nervous system, Population, Biology, Article, metabolism [Oligodendroglia], White matter, Mice, 03 medical and health sciences, medicine, Animals, Humans, Remyelination, Progenitor cell, education, Myelin Sheath, education.field_of_study, Multiple sclerosis, Bcas1 protein, mouse, pathology [Multiple Sclerosis], General Medicine, Human brain, medicine.disease, Oligodendrocyte, Neoplasm Proteins, Oligodendroglia, metabolism [Multiple Sclerosis], 030104 developmental biology, medicine.anatomical_structure, BCAS1 protein, human, metabolism [Neoplasm Proteins], ddc:500, Neuroscience, Demyelinating Diseases

Abstract

Investigations into brain function and disease depend on the precise classification of neural cell types. Cells of the oligodendrocyte lineage differ greatly in their morphology, but accurate identification has thus far only been possible for oligodendrocyte progenitor cells and mature oligodendrocytes in humans. We find that breast carcinoma amplified sequence 1 (BCAS1) expression identifies an oligodendroglial subpopulation in the mouse and human brain. These cells are newly formed, myelinating oligodendrocytes that segregate from oligodendrocyte progenitor cells and mature oligodendrocytes and mark regions of active myelin formation in development and in the adult. We find that BCAS1(+) oligodendrocytes are restricted to the fetal and early postnatal human white matter but remain in the cortical gray matter until old age. BCAS1(+) oligodendrocytes are reformed after experimental demyelination and found in a proportion of chronic white matter lesions of patients with multiple sclerosis (MS) even in a subset of patients with advanced disease. Our work identifies a means to map ongoing myelin formation in health and disease and presents a potential cellular target for remyelination therapies in MS.

Published

2017

38. Ageing synaptic vesicles are inactivated by contamination with SNAP25

Author

Angela Vogts, Annette Denker, Sven Truckenbrodt, Eugenio F. Fornasiero, Sebastian Jaehne, Silvio O. Rizzoli, Abhiyan Viplav, and Hanna Wildhagen

Subjects

0303 health sciences, Neurite, Vesicle, SNAP25, Hippocampal formation, Biology, Synaptic vesicle, Cell biology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, chemistry, Chaperone (protein), Organelle, biology.protein, Neurotransmitter, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Old organelles can become a hazard to cellular function, by accumulating molecular damage. Mechanisms that identify aged organelles, and prevent them from participating in cellular reactions, are therefore necessary. We describe here one such mechanism for the synaptic vesicle recycling pathway. Using cultured hippocampal neurons, we found that newly synthesized vesicle proteins were incorporated in the active (recycling) pool, and were preferentially employed in neurotransmitter release. They remained in use for up to ~24 hours, during which they recycled up to a few hundred times. We could only detect one change in the molecular composition of the vesicles, an apparent accumulation of SNAP25 in the aged synaptic vesicles. Overexpression of SNAP25, both in wild-type form or in vesicle-bound form, inhibited exocytosis and promoted the co-localization of the vesicle molecules with a recycling endosome marker. This is in line with the hypothesis that the SNAP25 contamination causes the inactivation of the aged vesicles. The SNAP25 overexpression effect could be alleviated by co-expressing the vesicle-associated molecule CSPa, which has been previously shown to be involved in chaperoning SNAP25 in the vesicle priming process. Overall, these results suggest that newly synthesized vesicle molecules are preferred in vesicle recycling, probably through a mechanism that renders their priming more efficient than that of aged vesicles.

Published

2017

39. Synapsins Contribute to the Dynamic Spatial Organization of Synaptic Vesicles in an Activity-Dependent Manner

Author

Riccardo Fesce, Eugenio F. Fornasiero, Fabrizia C. Guarnieri, Flavia Valtorta, Andrea Raimondi, Marta Orlando, Fabio Benfenati, Fornasiero, Ef, Raimondi, A, Guarnieri, F, Orlando, M, Fesce, R, Benfenati, F, and Valtorta, Flavia

Subjects

Male, Primary Cell Culture, Neurotransmission, Biology, Synaptic Transmission, Synaptic vesicle, Exocytosis, neural development, Rats, Sprague-Dawley, Mice, chemistry.chemical_compound, synaptic vesicles, Animals, Humans, Premovement neuronal activity, synapsins, Neurotransmitter, Mice, Knockout, neurobiology, General Neuroscience, Articles, Synapsin, Actin cytoskeleton, Rats, Cell biology, Mice, Inbred C57BL, HEK293 Cells, Synaptic fatigue, nervous system, chemistry, Female, Neuroscience

Abstract

"\"The precise subcellular organization of synaptic vesicles (SVs) at presynaptic sites allows for rapid and spatially restricted exocytotic release of neurotransmitter. The synapsins (Syns) are a family of presynaptic proteins that control the availability of SVs for exocytosis by reversibly tethering them to each other and to the actin cytoskeleton in a phosphorylation-dependent manner. Syn ablation leads to reduction in the density of SV proteins in nerve terminals and increased synaptic fatigue under high frequency stimulation, accompanied by the development of an epileptic phenotype. We analyzed cultured neurons from wild type and Syn I,II,III \\\/- triple knocked-out (TKO) mice and found that vesicular components were severely dispersed in the absence of Syns. Vesicle dispersion did not affect the readily releasable pool of SVs, whereas the total number of SVs was considerably reduced in TKO mice. Interestingly, the higher mobility observed in TKO apparently involved exocytosis competent SVs as well; it was not affected by stimulation but was reverted by chronic neuronal activity blockade. In summary, our data show that while a Syn-dependent mechanism reduces the mobility of a subpopulation of SVs, by reversibly tethering them to the synaptic region, an additional Syn-independent mechanism, whose molecular substrate remains to be clarified, targets SVs to synaptic boutons at rest, and might be outpaced by activity. Altogether these findings indicate that Syns are essential to maintain the dynamic structural organization of synapses and the size of the reserve pool of SVs during intense SV recycling.\""

Published

2012

40. The synapsins: Multitask modulators of neuronal development

Author

Eugenio F. Fornasiero, Davide Pozzi, Fabio Benfenati, Flavia Valtorta, Valtorta, Flavia, D., Pozzi, F., Benfenati, and E. F., Fornasiero

Subjects

Neurite, Neurogenesis, Cellular differentiation, Synaptogenesis, Nerve Tissue Proteins, Biology, Synapse, Neurites, Asymmetric cell division, Animals, Humans, Phosphorylation, Growth cone, Neurons, Chromosome Pairing, Synapsins, SYNAPTIC VESICLES, Cell Biology, Synapsin, nerve terminal, protein phosphorylation, Cell biology, nervous system, Developmental Biology

Abstract

Neurons are examples of specialized cells that evolved the extraordinary ability to transmit electrochemical information in complex networks of interconnected cells. During their development, neurons undergo precisely regulated processes that define their lineage, positioning, morphogenesis and pattern of activity. The events leading to the establishment of functional neuronal networks follow a number of key steps, including asymmetric cell division from neuronal precursors, migration, establishment of polarity, neurite outgrowth and synaptogenesis. Synapsins are a family of abundant neuronal phosphoproteins that have been extensively studied for their role in the regulation of neurotransmission in presynaptic terminals. Beside their implication in the homeostasis of adult cells, synapsins influence the development of young neurons, interacting with cytoskeletal and vesicular components and regulating their dynamics. Although the exact molecular mechanisms determining synapsin function in neuronal development are still largely unknown, in this review we summarize the most important literature on the subject, providing a conceptual framework for the progress of present and future research.

Published

2011

41. Cadherins as regulators of neuronal polarity

Author

Eugenio F. Fornasiero, Carlos G. Dotti, and Annette Gärtner

Subjects

neuronal polarity, Brain development, Polarity (physics), Neurogenesis, Reviews, Biology, migration, Synapse, Cellular and Molecular Neuroscience, Mice, Cell Movement, medicine, Cell Adhesion, Animals, Humans, Axon, Neurulation, N-cadherin, Cadherin, Cell Polarity, Cell Biology, Cadherins, Axons, Cell biology, Rats, medicine.anatomical_structure, Adhesion, Neuronal polarity, Signal Transduction

Abstract

A compelling amount of data is accumulating about the polyphonic role of neuronal cadherins during brain development throughout all developmental stages, starting from the involvement of cadherins in the organization of neurulation up to synapse development and plasticity. Recent work has confirmed that specifically N-cadherins play an important role in asymmetrical cellular processes in developing neurons that are at the basis of polarity. In this review we will summarize recent data, which demonstrate how N-cadherin orchestrates distinct processes of polarity establishment in neurons.

Published

2014

42. Distinct temporal hierarchies in membrane and cytoskeleton dynamics precede the morphological polarization of developing neurons

Author

Eugenio F. Fornasiero, Carlos G. Dotti, Flavia Valtorta, Annette Gärtner, A., Gärtner, E. F., Fornasiero, Valtorta, Flavia, and C. G., Dotti

Subjects

Neurite, Neurogenesis, Hippocampal formation, Biology, Hippocampus, Time-Lapse Imaging, Mice, Organ Culture Techniques, Bipolar neuron, Pregnancy, medicine, Animals, Axon, Cytoskeleton, Mitosis, development, Cells, Cultured, Neurons, Cell Membrane, Cell Polarity, cytoskeleton, Rats, Inbred Strains, Cell Biology, neuron, Actins, Cell biology, Rats, Protein Transport, medicine.anatomical_structure, nervous system, Female, Neuron, Unipolar neuron

Abstract

Final morphological polarization of neurons, with the development of a distinct axon and of several dendrites, is preceded by phases of non-polarized architecture. The earliest of these phases is that of the round neuron arising from the last mitosis. A second non polarized stage corresponds to the bipolar neuron, with two morphologically identical neurites. Both phases have their distinctive relevance in the establishment of neuronal polarity. During the round cell stage a decision is made as to where from the cell periphery a first neurite will form, thus creating the first sign of asymmetry. At the bipolar stage a decision is made as to which of the two neurites becomes the axon in neurons polarizing in vitro and the leading edge in neurons in situ. In this study we analysed cytoskeletal and membrane dynamics in cells at these two "pre-polarity" stages. By mean of time lapse imaging in dissociated hippocampal neurons and ex vivo cortical slices we show that both stages are characterized by polarized intracellular arrangements, however with distinct temporal hierarchies: polarized actin dynamics marks the site of first polarization in round cells, whereas polarized membrane dynamics precedes asymmetric growth in the bipolar stage. ispartof: Journal of Cell Science vol:127 issue:20 pages:4409-19 ispartof: location:England status: published

Published

2014

43. Super-Resolution Microscopy Techniques in the Neurosciences

Author

Eugenio F. Fornasiero

Published

2014

44. Cellular and Molecular Applications of Super-resolution Microscopy

Author

Eugenio F. Fornasiero and Felipe Opazo

Subjects

Antibody mimetic, 0303 health sciences, Super-resolution microscopy, Aptamer, Resolution (electron density), STED microscopy, Nanotechnology, Biology, 03 medical and health sciences, 0302 clinical medicine, Live cell imaging, Microscopy, Biological imaging, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

In the last two decades, a number of continuously improving imaging techniques have allowed us to overcome the light diffraction barrier and to obtain nanometer-scale resolution in biological imaging. Together with the development of novel imaging modalities, new probes are being implemented in sample preparation, including new classes of dyes, photoswitchable fluorescent proteins, and smaller probes such as aptamers, nanobodies, and antibody mimetic technology. How is biology coping with these technical revolutions? In this chapter, we describe some super-resolution imaging techniques of particular relevance for biological research, including sample preparation, live imaging, multicolor labeling, and three-dimensional reconstruction. Finally, with the purpose of inspiring a more pervasive use of super-resolution imaging, we review some practical applications of nanometer-scale microscopy, covering a wide array of biological topics such as organization of cell contacts, recycling of synaptic vesicles, sporulation of bacteria, and organization of nucleic acids and membranes.

Published

2014

45. List of Contributors

Author

Daniel Axelrod, Melanie Bokstad, Martin J. Booth, Julian Borejdo, Alessandra Cambi, Julien Colombelli, Ali Ertürk, Eugenio F. Fornasiero, Sung-Sik Han, Samie R. Jaffrey, Min-Kyo Jung, Sandra de Keijzer, Jun-Sung Kim, Lynlee L. Lin, Er Liu, Corinne Lorenzo, Ohad Medalia, Marjolein B.M. Meddens, John P. Nolan, Felipe Opazo, Chan-Gi Pack, Brian R. Patton, Daniel A. Peterson, Jeremy Pike, Tarl W. Prow, Joshua Z. Rappoport, E. Hesper Rego, Yasushi Sako, Lin Shao, Alex Small, Mi-Roung Song, Shane Stahlheber, Rita L. Strack, Jennifer A. Thorley, and Miko Yamada

Published

2014

46. N-cadherin: A new player in neuronal polarity

Author

Carlos G. Dotti, Eugenio F. Fornasiero, and Annette Gärtner

Subjects

Neurite, Centrosome, Cadherin, education, Cell Biology, Biology, Neuronal polarity, Molecular Biology, Developmental Biology, Cell biology

Published

2012

47. N-cadherin specifies first asymmetry in developing neurons

Author

Annette, Gärtner, Eugenio F, Fornasiero, Sebastian, Munck, Krist'l, Vennekens, Eve, Seuntjens, Wieland B, Huttner, Flavia, Valtorta, and Carlos G, Dotti

Subjects

Centrosome, Neurons, Cell Polarity, Golgi Apparatus, Nerve Tissue Proteins, macromolecular substances, Cadherins, Article, Rats, nervous system, Neurites, Animals, Phosphatidylinositol 3-Kinase, Cell Division, Cytoskeleton

Abstract

The precise polarization and orientation of developing neurons is essential for the correct wiring of the brain. In pyramidal excitatory neurons, polarization begins with the sprouting of opposite neurites, which later define directed migration and axo-dendritic domains. We here show that endogenous N-cadherin concentrates at one pole of the newborn neuron, from where the first neurite subsequently emerges. Ectopic N-cadherin is sufficient to favour the place of appearance of the first neurite. The Golgi and centrosome move towards this newly formed morphological pole in a second step, which is regulated by PI3K and the actin/microtubule cytoskeleton. Moreover, loss of function experiments in vivo showed that developing neurons with a non-functional N-cadherin misorient their cell axis. These results show that polarization of N-cadherin in the immediate post-mitotic stage is an early and crucial mechanism in neuronal polarity.

Published

2011

48. Effects of phosphorylation and neuronal activity on the control of synapse formation by synapsin I

Author

Francesca Botti, Fabio Benfenati, Flavia Valtorta, Dario Bonanomi, Maila Giannandrea, Mario Amendola, Luigi Naldini, Laura E. Perlini, Eugenio F. Fornasiero, Perlini, Le, Botti, F, Fornasiero, Ef, Giannandrea, M, Bonanomi, D, Amendola, M, Naldini, Luigi, Benfenati, F, Valtorta, Flavia, Approches génétiques intégrées et nouvelles thérapies pour les maladies rares (INTEGRARE), and Université d'Évry-Val-d'Essonne (UEVE)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Université Paris-Saclay-Généthon

Subjects

Synapsin I, [SDV.BIO]Life Sciences [q-bio]/Biotechnology, Synaptogenesis, [SDV.BC]Life Sciences [q-bio]/Cellular Biology, Biology, Neurotransmission, Bioinformatics, Synaptic vesicle, environment and public health, Synapse, Rats, Sprague-Dawley, Animals, Humans, Phosphorylation, Protein kinase A, Cells, Cultured, Neurons, [SDV.MHEP.HEM]Life Sciences [q-bio]/Human health and pathology/Hematology, Cell Biology, Synapsin, Synapsins, Cell biology, Rats, nervous system, Synapses

Abstract

International audience; Synapsins are synaptic vesicle (SV)-associated proteins that regulate synaptic transmission and neuronal differentiation. At early stages, Syn I and II phosphorylation at Ser9 by cAMP-dependent protein kinase (PKA) and Ca2+/calmodulin-dependent protein kinase I/IV modulates axon elongation and SV-precursor dynamics. We evaluated the requirement of Syn I for synapse formation by siRNA-mediated knockdown as well as by overexpression of either its wild-type (WT) form or its phosphorylation mutants. Syn1 knockdown at 14 days in vitro caused a decrease in the number of synapses, accompanied by a reduction of SV recycling. Although overexpression of WT Syn I was ineffective, overexpression of its phosphorylation mutants resulted in a complex temporal regulation of synapse density. At early stages of synaptogenesis, phosphomimetic Syn I S9E significantly increased the number of synapses. Conversely, dephosphomimetic Syn I S9A decreased synapse number at more advanced stages. Overexpression of either WT Syn I or its phosphomimetic S9E mutant rescued the decrease in synapse number caused by chronic treatment with tetrodotoxin at early stages, suggesting that Syn I participates in an alternative PKA-dependent mechanism that can compensate for the impairment of the activity-dependent synaptogenic pathway. Altogether these results indicate that Syn I is an important regulator of synapse formation, which adjusts synapse number in response to extracellular signals.

Published

2011

49. QuickPALM: 3D real-time photoactivation nanoscopy image processing in ImageJ

Author

Mickaël Lelek, Musa M. Mhlanga, Ricardo Henriques, Flavia Valtorta, Christophe Zimmer, Eugenio F. Fornasiero, Universidade de Lisboa (ULISBOA), Imagerie et Modélisation, Institut Pasteur [Paris]-Centre National de la Recherche Scientifique (CNRS), Imagerie et Modélisation - Imaging and Modeling, Istituto Italiano di Tecnologia (IIT), Universita Vita Salute San Raffaele = Vita-Salute San Raffaele University [Milan, Italie] (UniSR), Council for Scientific and Industrial Research [Pretoria] (CSIR), We thank J. Enninga for assistance with experiments, and T. Duong and R. Fesce for helpful insight in the preparation of the manuscript., R., Henrique, M., Lelek, E., Fornasiero, Valtorta, Flavia, C., Zimmer, M., Mhlanga, Universidade de Lisboa = University of Lisbon (ULISBOA), and Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS)

Subjects

Single molecule localization, Diffraction, Microscope, Materials science, MESH: Microscopy, Image processing, 02 engineering and technology, MESH: Imaging, Three-Dimensional, Microtubules, Biochemistry, law.invention, Mice, 03 medical and health sciences, MESH: Software, Imaging, Three-Dimensional, Optics, law, Microscopy, Image Processing, Computer-Assisted, Animals, MESH: Animals, IMAGE ANALYSIS, Molecular Biology, MESH: Mice, 030304 developmental biology, 0303 health sciences, Total internal reflection fluorescence microscope, business.industry, MESH: Microtubules, Resolution (electron density), MICROSCOPY, Cell Biology, 021001 nanoscience & nanotechnology, MESH: Image Processing, Computer-Assisted, Wavelength, RESOLUTION, Biophysics, [SDV.SPEE]Life Sciences [q-bio]/Santé publique et épidémiologie, 0210 nano-technology, business, Software, Biotechnology

Abstract

To the Editor: Although conventional microscopes have a reso-lution limited by diffraction to about half the wavelength of light, several recent advances have led to microscopy methods that achieve roughly tenfold improvements in resolution. Among them, photoactivated light microscopy (PALM) and stochastic optical resolution microscopy (STORM) have become particularly popular, as they only require relatively simple and affordable modifications to a standard total internal reflection fluorescence (TIRF) microscope and have been extended to three-dimensional (3D) super-resolution and multicolor imaging.

Published

2010

50. The role of synapsins in neuronal development

Author

Eugenio F. Fornasiero, Dario Bonanomi, Fabio Benfenati, Flavia Valtorta, E., Fornasiero, D., Bonanomi, F., Benfenati, and Valtorta, Flavia

Subjects

Gene isoform, Neurite, Neurogenesis, Growth Cones, Neurotransmission, Biology, Synaptic vesicle, Synaptic Transmission, Cellular and Molecular Neuroscience, Animals, Humans, Protein Isoforms, Phosphorylation, Cytoskeleton, Growth cone, Molecular Biology, Pharmacology, Neurons, membrane trafficking, Cell Biology, Synapsin, Actin cytoskeleton, Synapsins, nerve terminal, Cell biology, nervous system, neurotransmitter release, Synapses, Molecular Medicine

Abstract

The synapsins, the first identified synaptic vesicle-specific proteins, are phosphorylated on multiple sites by a number of protein kinases and are involved in neurite outgrowth and synapse formation as well as in synaptic transmission. In mammals, the synapsin family consists of at least 10 isoforms encoded by three distinct genes and composed by a mosaic of conserved and variable domains. The synapsins are highly conserved evolutionarily and orthologues have been found in invertebrates and lower vertebrates. Within nerve terminals, synapsins are implicated in multiple interactions with presynaptic proteins and the actin cytoskeleton. Via these interactions, synapsins control several mechanisms important for neuronal homeostasis. In this review, we describe the main functional features of the synapsins, in relation to the complex role played by these phosphoproteins in neuronal development.

Published

2010