Miro proteins coordinate microtubule‐ and actin‐dependent mitochondrial transport and distribution

López‐Doménech, Guillermo; Covill‐Cooke, Christian; Ivankovic, Davor; Halff, Els F.; Sheehan, David F.; Norkett, Rosalind; Birsa, Nicol; Kittler, Josef T.

doi:10.15252/embj.201696380

Cited by 251 publications

(367 citation statements)

References 55 publications

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“…Miro has been extensively documented to be critical for mitochondrial distribution through bidirectional microtubule-dependent trafficking in a wide variety of species and cell types [31,[41][42][43][44]. Miro has been extensively documented to be critical for mitochondrial distribution through bidirectional microtubule-dependent trafficking in a wide variety of species and cell types [31,[41][42][43][44].…”

Section: Resultsmentioning

confidence: 99%

“…To quantify whether Miro is also required to establish peroxisomal distribution, a Sholl-based quantification method was applied [30,31]. Organelle distribution was then measured by concentric circles being drawn from the centre of the cell at 1-lm intervals and the inter-circle organelle marker signal being quantified, and plotted with distance ( Fig EV3A) [31]. Organelle distribution was then measured by concentric circles being drawn from the centre of the cell at 1-lm intervals and the inter-circle organelle marker signal being quantified, and plotted with distance ( Fig EV3A) [31].…”

Section: Resultsmentioning

confidence: 99%

“…The mitochondrial Rho-GTPases, Miro1 and Miro2, are outer mitochondrial membrane (OMM) proteins critical for mitochondrial trafficking [27][28][29][30][31]. Taking advantage of Miro knockout mouse embryonic fibroblasts (MEFs), we find that in contrast to previous reports, and its role at mitochondria, Miro is not required to establish steady-state peroxisomal distribution through long-range microtubule-dependent trafficking [26,31,34]. Here, we confirm that Miro1 and Miro2 are not strictly localised to mitochondria but are also localised Neuroscience, Physiology and Pharmacology Department, University College London, London, UK *Corresponding author.…”

Section: Introductionmentioning

confidence: 99%

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Peroxisomal fission is modulated by the mitochondrial Rho‐GTPases, Miro1 and Miro2

et al. 2020

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Peroxisomes are essential for a number of cellular functions, including reactive oxygen species metabolism, fatty acid b-oxidation and lipid synthesis. To ensure optimal functionality, peroxisomal size, shape and number must be dynamically maintained; however, many aspects of how this is regulated remain poorly characterised. Here, we show that the localisation of Miro1 and Miro2-outer mitochondrial membrane proteins essential for mitochondrial trafficking-to peroxisomes is not required for basal peroxisomal distribution and long-range trafficking, but rather for the maintenance of peroxisomal size and morphology through peroxisomal fission. Mechanistically, this is achieved by Miro negatively regulating Drp1-dependent fission, a function that is shared with the mitochondria. We further find that the peroxisomal localisation of Miro is regulated by its first GTPase domain and is mediated by an interaction through its transmembrane domain with the peroxisomal-membrane protein chaperone, Pex19. Our work highlights a shared regulatory role of Miro in maintaining the morphology of both peroxisomes and mitochondria, supporting a crosstalk between peroxisomal and mitochondrial biology.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Peroxisomal fission is modulated by the mitochondrial Rho‐GTPases, Miro1 and Miro2

et al. 2020

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“…Since its initial discovery, Myo19 has been implicated in a range of functions, including targeting mitochondria to stress induced filopodia [38,39] and coordinating mitochondrial inheritance upon cytokinesis [40]. Most recently, Myo19 localization to mitochondria was shown to be dependent on Miro proteins, suggesting that Miro may regulate both actin and microtubule based mitochondrial motility [41]. In addition to Myo19, there is evidence that other myosin motors facilitate mitochondria dynamics.…”

Section: Actin Dynamics In Mitochondrial Motility and Remodelingmentioning

confidence: 99%

Mitochondrial-cytoskeletal interactions: dynamic associations that facilitate network function and remodeling

Moore

Holzbaur

2018

Current Opinion in Physiology

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Mitochondria are dynamic organelles that can form complex networks in the cell. These networks can be rapidly remodeled in response to environmental changes or to support cellular needs. Mitochondrial dynamics are dependent on interactions with the cellular cytoskeleton – both microtubules and actin filaments. Mitochondrial-cytoskeletal interactions have a well-established role in mitochondrial motility. Recent progress indicates that these interactions also regulate the balance of mitochondrial fission/fusion, as well as mitochondria turnover and mitochondrial inheritance during cell division. We review these advances, and how this work has deepened our understanding of mitochondrial dynamics in the cell.

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“…Instead, Covill-Cooke and colleagues observed a decrease in peroxisome oscillatory movement. This type of short-range motility accounts for 85–95% of peroxisome movements in the cell, and although poorly characterized, might rely on diffusive behaviour and interactions with the actin cytoskeleton [27,28]. Although conflicting with the expression and silencing results, it is possible that in the absence of Miro1, other motor complexes enable fast and directed motility of peroxisomes, but also that Miro1 plays additional roles in peroxisome motility.…”

Section: Miro1 and Peroxisome Motilitymentioning

confidence: 99%

Miro1 – the missing link to peroxisome motility

Castro

Schrader

2018

Communicative & Integrative Biology

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Peroxisomes are ubiquitous, highly dynamic, multifunctional compartments in eukaryotic cells, which perform key roles in cellular lipid metabolism and redox balance. Like other membrane-bound organelles, peroxisomes must move in the cellular landscape to perform localized functions, interact with other organelles and to properly distribute during cell division. However, our current knowledge of peroxisome motility in mammalian cells is still very limited. Recently, three independent studies have identified Miro1 as a regulator of peroxisome motility in mammalian cells. In these studies, the authors show that Miro1 is targeted to peroxisomes in several cell lines, in a process that relies on its interaction with the peroxisomal chaperone Pex19. Interestingly, however, different conclusions are drawn about which Miro1 isoforms are targeted to peroxisomes, how it interacts with Pex19 and most importantly, the type of motility Miro1 is regulating.

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Miro proteins coordinate microtubule‐ and actin‐dependent mitochondrial transport and distribution

Cited by 251 publications

References 55 publications

Peroxisomal fission is modulated by the mitochondrial Rho‐GTPases, Miro1 and Miro2

Peroxisomal fission is modulated by the mitochondrial Rho‐GTPases, Miro1 and Miro2

Mitochondrial-cytoskeletal interactions: dynamic associations that facilitate network function and remodeling

Miro1 – the missing link to peroxisome motility

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