Unravelling mitochondrial dynamics and turnover in the synapse

Detalhes bibliográficos
Autor(a) principal: Cardanho-Ramos, Carlos
Data de Publicação: 2024
Idioma: eng
Título da fonte: Repositórios Científicos de Acesso Aberto de Portugal (RCAAP)
Texto Completo: http://hdl.handle.net/10400.5/98699
Resumo: Neurons rely on mitochondria for ATP production and Ca2+ homeostasis, particularly at the synapse. As subcompartmentalized cells, they have different pools of mitochondria in each compartment. Achieving a non-uniform distribution requires mitochondria not only to be transported, but also to be retained in regions with high energy demands and high levels of Ca2+ . One of the goals of this thesis was to understand what makes mitochondria travel back and forward in a neuron and which mechanisms were activated to retain this organelle at the synapse. To address this, mouse primary neuron cultures, with fluorescent labelled mitochondria, were used to study the impact of the actomyosin cytoskeleton in mitochondrial transport and anchoring at the synapse. Taking advantage of a proteomic screen comparing synaptic with non-synaptic mitochondria, we selected two candidate proteins related with organelle movement: cell division control protein 42 (cdc-42), involved in actin polymerization; and myosin-VI, capable of anchoring mitochondria to actin cables. In the course of this project, a paper was published addressing all our questions, forcing us to focus on a different topic. In the other project of this thesis, we focused on understanding how mitochondria replicate in neurons. It is assumed that mitochondria are generated in the cell body and travel to the synapse to exert their functions. However, considering the rate of mitochondrial transport in neurons, the time it would take for a single mitochondrion to travel from the cell body to the synapse exceeds the half-life of most mitochondrial proteins. Our goal was to understand whether mitochondrial replication occurred in the periphery of neurons and which mechanisms were involved. We developed a technique to assess mitochondrial replication in mouse primary neuron cultures using 5-bromo-2′- deoxyuridine (BrdU)- and 5-ethynyl-2´-deoxyuridine (EdU)-labelling, two thymidine analogues that are incorporated into mtDNA upon replication. Most BrdU/EdU staining was observed in the cell body, but staining was also present to a lower extent in the periphery. Using microfluidic devices, where axons can be isolated from the cell body, we were able to add EdU only to the axonal side, without interfering with the cell body. In these conditions, EdU staining was only present in axons, confirming that mitochondrial replication in neurons can occur away from the cell body. We hypothesized that mRNA and local translation must be at place in the periphery of neurons in order to provide all the necessary machinery for mitochondria to replicate. To test this, we assessed mitochondrial replication upon inhibition of both nuclear-encoded and mitochondrial-encoded protein translation. Mitochondrial replication in neurons decreased when nuclear-encoded protein translation was inhibited. However, no differences were observed upon inhibition of mitochondrial-encoded protein translation. Taking advantage of the proteomic screen comparing synaptic with non-synaptic mitochondria, two candidate proteins related with protein translation were found upregulated in the synaptic fraction – eukaryotic elongation factor 1 alpha 1 (eEF1a1), involved in nuclear-encoded protein translation; and mitochondrial translation elongation factor Tu (TUFM), involved in mitochondrial-encoded protein translation. We performed loss and gain of function assays with our candidate proteins and assessed their impact on mitochondrial replication. When eEF1A1 was downregulated, we observed a decrease in mitochondrial replication in the periphery of neurons. This effect was rescued by reintroducing eEF1A1. Regarding TUFM, no differences were observed. Our results confirm that mitochondrial replication can occur in the periphery of neurons, and that this process requires nuclear-encoded protein translation, mediated by eEF1A1. Understanding how mitochondrial replication occurs in neurons, particularly at the level of the synapse, provides novel lines of research to tackle the pathophysiological mechanisms underlying neurodegenerative diseases.
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spelling Unravelling mitochondrial dynamics and turnover in the synapsebiogénese mitocondrialneuróniofator de elongação da traduçãoeEF1A1síntese proteicamitochondrial biogenesisneurontranslation elongation factorprotein synthesis.Domínio/Área Científica::Ciências Médicas::Medicina BásicaNeurons rely on mitochondria for ATP production and Ca2+ homeostasis, particularly at the synapse. As subcompartmentalized cells, they have different pools of mitochondria in each compartment. Achieving a non-uniform distribution requires mitochondria not only to be transported, but also to be retained in regions with high energy demands and high levels of Ca2+ . One of the goals of this thesis was to understand what makes mitochondria travel back and forward in a neuron and which mechanisms were activated to retain this organelle at the synapse. To address this, mouse primary neuron cultures, with fluorescent labelled mitochondria, were used to study the impact of the actomyosin cytoskeleton in mitochondrial transport and anchoring at the synapse. Taking advantage of a proteomic screen comparing synaptic with non-synaptic mitochondria, we selected two candidate proteins related with organelle movement: cell division control protein 42 (cdc-42), involved in actin polymerization; and myosin-VI, capable of anchoring mitochondria to actin cables. In the course of this project, a paper was published addressing all our questions, forcing us to focus on a different topic. In the other project of this thesis, we focused on understanding how mitochondria replicate in neurons. It is assumed that mitochondria are generated in the cell body and travel to the synapse to exert their functions. However, considering the rate of mitochondrial transport in neurons, the time it would take for a single mitochondrion to travel from the cell body to the synapse exceeds the half-life of most mitochondrial proteins. Our goal was to understand whether mitochondrial replication occurred in the periphery of neurons and which mechanisms were involved. We developed a technique to assess mitochondrial replication in mouse primary neuron cultures using 5-bromo-2′- deoxyuridine (BrdU)- and 5-ethynyl-2´-deoxyuridine (EdU)-labelling, two thymidine analogues that are incorporated into mtDNA upon replication. Most BrdU/EdU staining was observed in the cell body, but staining was also present to a lower extent in the periphery. Using microfluidic devices, where axons can be isolated from the cell body, we were able to add EdU only to the axonal side, without interfering with the cell body. In these conditions, EdU staining was only present in axons, confirming that mitochondrial replication in neurons can occur away from the cell body. We hypothesized that mRNA and local translation must be at place in the periphery of neurons in order to provide all the necessary machinery for mitochondria to replicate. To test this, we assessed mitochondrial replication upon inhibition of both nuclear-encoded and mitochondrial-encoded protein translation. Mitochondrial replication in neurons decreased when nuclear-encoded protein translation was inhibited. However, no differences were observed upon inhibition of mitochondrial-encoded protein translation. Taking advantage of the proteomic screen comparing synaptic with non-synaptic mitochondria, two candidate proteins related with protein translation were found upregulated in the synaptic fraction – eukaryotic elongation factor 1 alpha 1 (eEF1a1), involved in nuclear-encoded protein translation; and mitochondrial translation elongation factor Tu (TUFM), involved in mitochondrial-encoded protein translation. We performed loss and gain of function assays with our candidate proteins and assessed their impact on mitochondrial replication. When eEF1A1 was downregulated, we observed a decrease in mitochondrial replication in the periphery of neurons. This effect was rescued by reintroducing eEF1A1. Regarding TUFM, no differences were observed. Our results confirm that mitochondrial replication can occur in the periphery of neurons, and that this process requires nuclear-encoded protein translation, mediated by eEF1A1. Understanding how mitochondrial replication occurs in neurons, particularly at the level of the synapse, provides novel lines of research to tackle the pathophysiological mechanisms underlying neurodegenerative diseases.Epifânio, Vanessa Alexandra dos Santos MoraisRepositório da Universidade de LisboaCardanho-Ramos, Carlos2025-02-24T18:38:44Z2024-042024-012024-04-01T00:00:00Zdoctoral thesisinfo:eu-repo/semantics/publishedVersionapplication/pdfhttp://hdl.handle.net/10400.5/98699TID:101603886enginfo:eu-repo/semantics/openAccessreponame:Repositórios Científicos de Acesso Aberto de Portugal (RCAAP)instname:FCCN, serviços digitais da FCT – Fundação para a Ciência e a Tecnologiainstacron:RCAAP2025-03-17T16:34:42Zoai:repositorio.ulisboa.pt:10400.5/98699Portal AgregadorONGhttps://www.rcaap.pt/oai/openaireinfo@rcaap.ptopendoar:https://opendoar.ac.uk/repository/71602025-05-29T04:20:36.841634Repositórios Científicos de Acesso Aberto de Portugal (RCAAP) - FCCN, serviços digitais da FCT – Fundação para a Ciência e a Tecnologiafalse
dc.title.none.fl_str_mv Unravelling mitochondrial dynamics and turnover in the synapse
title Unravelling mitochondrial dynamics and turnover in the synapse
spellingShingle Unravelling mitochondrial dynamics and turnover in the synapse
Cardanho-Ramos, Carlos
biogénese mitocondrial
neurónio
fator de elongação da tradução
eEF1A1
síntese proteica
mitochondrial biogenesis
neuron
translation elongation factor
protein synthesis.
Domínio/Área Científica::Ciências Médicas::Medicina Básica
title_short Unravelling mitochondrial dynamics and turnover in the synapse
title_full Unravelling mitochondrial dynamics and turnover in the synapse
title_fullStr Unravelling mitochondrial dynamics and turnover in the synapse
title_full_unstemmed Unravelling mitochondrial dynamics and turnover in the synapse
title_sort Unravelling mitochondrial dynamics and turnover in the synapse
author Cardanho-Ramos, Carlos
author_facet Cardanho-Ramos, Carlos
author_role author
dc.contributor.none.fl_str_mv Epifânio, Vanessa Alexandra dos Santos Morais
Repositório da Universidade de Lisboa
dc.contributor.author.fl_str_mv Cardanho-Ramos, Carlos
dc.subject.por.fl_str_mv biogénese mitocondrial
neurónio
fator de elongação da tradução
eEF1A1
síntese proteica
mitochondrial biogenesis
neuron
translation elongation factor
protein synthesis.
Domínio/Área Científica::Ciências Médicas::Medicina Básica
topic biogénese mitocondrial
neurónio
fator de elongação da tradução
eEF1A1
síntese proteica
mitochondrial biogenesis
neuron
translation elongation factor
protein synthesis.
Domínio/Área Científica::Ciências Médicas::Medicina Básica
description Neurons rely on mitochondria for ATP production and Ca2+ homeostasis, particularly at the synapse. As subcompartmentalized cells, they have different pools of mitochondria in each compartment. Achieving a non-uniform distribution requires mitochondria not only to be transported, but also to be retained in regions with high energy demands and high levels of Ca2+ . One of the goals of this thesis was to understand what makes mitochondria travel back and forward in a neuron and which mechanisms were activated to retain this organelle at the synapse. To address this, mouse primary neuron cultures, with fluorescent labelled mitochondria, were used to study the impact of the actomyosin cytoskeleton in mitochondrial transport and anchoring at the synapse. Taking advantage of a proteomic screen comparing synaptic with non-synaptic mitochondria, we selected two candidate proteins related with organelle movement: cell division control protein 42 (cdc-42), involved in actin polymerization; and myosin-VI, capable of anchoring mitochondria to actin cables. In the course of this project, a paper was published addressing all our questions, forcing us to focus on a different topic. In the other project of this thesis, we focused on understanding how mitochondria replicate in neurons. It is assumed that mitochondria are generated in the cell body and travel to the synapse to exert their functions. However, considering the rate of mitochondrial transport in neurons, the time it would take for a single mitochondrion to travel from the cell body to the synapse exceeds the half-life of most mitochondrial proteins. Our goal was to understand whether mitochondrial replication occurred in the periphery of neurons and which mechanisms were involved. We developed a technique to assess mitochondrial replication in mouse primary neuron cultures using 5-bromo-2′- deoxyuridine (BrdU)- and 5-ethynyl-2´-deoxyuridine (EdU)-labelling, two thymidine analogues that are incorporated into mtDNA upon replication. Most BrdU/EdU staining was observed in the cell body, but staining was also present to a lower extent in the periphery. Using microfluidic devices, where axons can be isolated from the cell body, we were able to add EdU only to the axonal side, without interfering with the cell body. In these conditions, EdU staining was only present in axons, confirming that mitochondrial replication in neurons can occur away from the cell body. We hypothesized that mRNA and local translation must be at place in the periphery of neurons in order to provide all the necessary machinery for mitochondria to replicate. To test this, we assessed mitochondrial replication upon inhibition of both nuclear-encoded and mitochondrial-encoded protein translation. Mitochondrial replication in neurons decreased when nuclear-encoded protein translation was inhibited. However, no differences were observed upon inhibition of mitochondrial-encoded protein translation. Taking advantage of the proteomic screen comparing synaptic with non-synaptic mitochondria, two candidate proteins related with protein translation were found upregulated in the synaptic fraction – eukaryotic elongation factor 1 alpha 1 (eEF1a1), involved in nuclear-encoded protein translation; and mitochondrial translation elongation factor Tu (TUFM), involved in mitochondrial-encoded protein translation. We performed loss and gain of function assays with our candidate proteins and assessed their impact on mitochondrial replication. When eEF1A1 was downregulated, we observed a decrease in mitochondrial replication in the periphery of neurons. This effect was rescued by reintroducing eEF1A1. Regarding TUFM, no differences were observed. Our results confirm that mitochondrial replication can occur in the periphery of neurons, and that this process requires nuclear-encoded protein translation, mediated by eEF1A1. Understanding how mitochondrial replication occurs in neurons, particularly at the level of the synapse, provides novel lines of research to tackle the pathophysiological mechanisms underlying neurodegenerative diseases.
publishDate 2024
dc.date.none.fl_str_mv 2024-04
2024-01
2024-04-01T00:00:00Z
2025-02-24T18:38:44Z
dc.type.driver.fl_str_mv doctoral thesis
dc.type.status.fl_str_mv info:eu-repo/semantics/publishedVersion
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dc.identifier.uri.fl_str_mv http://hdl.handle.net/10400.5/98699
TID:101603886
url http://hdl.handle.net/10400.5/98699
identifier_str_mv TID:101603886
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