Phase separation organizes the site of autophagosome formation

Many biomolecules undergo liquid–liquid phase separation to form liquid-like condensates that mediate diverse cellular functions 1 , 2 . Autophagy is able to degrade such condensates using autophagosomes—double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS...

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Vydáno v:Nature (London) Ročník 578; číslo 7794; s. 301 - 305
Hlavní autoři: Fujioka, Yuko, Alam, Jahangir Md, Noshiro, Daisuke, Mouri, Kazunari, Ando, Toshio, Okada, Yasushi, May, Alexander I., Knorr, Roland L., Suzuki, Kuninori, Ohsumi, Yoshinori, Noda, Nobuo N.
Médium: Journal Article
Jazyk:angličtina
Vydáno: London Nature Publishing Group UK 13.02.2020
Nature Publishing Group
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ISSN:0028-0836, 1476-4687, 1476-4687
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Abstract Many biomolecules undergo liquid–liquid phase separation to form liquid-like condensates that mediate diverse cellular functions 1 , 2 . Autophagy is able to degrade such condensates using autophagosomes—double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast 3 – 5 . Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein–protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS. The pre-autophagosomal structure in yeast is a liquid-like condensate of Atg proteins whose phase separation may have a critical, active role in autophagy.
AbstractList Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions1,2. Autophagy is able to degrade such condensates using autophagosomes-double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast3-5. Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atgl complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atgl-complex droplets can be tethered to membranes via specific protein-protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS.
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions.sup.1,2. Autophagy is able to degrade such condensates using autophagosomes--double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast.sup.3-5. Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein-protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS.
Many biomolecules undergo liquid–liquid phase separation to form liquid-like condensates that mediate diverse cellular functions 1 , 2 . Autophagy is able to degrade such condensates using autophagosomes—double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast 3 – 5 . Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein–protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS. The pre-autophagosomal structure in yeast is a liquid-like condensate of Atg proteins whose phase separation may have a critical, active role in autophagy.
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions.sup.1,2. Autophagy is able to degrade such condensates using autophagosomes--double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast.sup.3-5. Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein-protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS. The pre-autophagosomal structure in yeast is a liquid-like condensate of Atg proteins whose phase separation may have a critical, active role in autophagy.
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions . Autophagy is able to degrade such condensates using autophagosomes-double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast . Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein-protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS.
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions1,2. Autophagy is able to degrade such condensates using autophagosomes-double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast3-5. Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein-protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS.Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions1,2. Autophagy is able to degrade such condensates using autophagosomes-double-membrane structures that are synthesized de novo at the pre-autophagosomal structure (PAS) in yeast3-5. Whereas Atg proteins that associate with the PAS have been characterized, the physicochemical and functional properties of the PAS remain unclear owing to its small size and fragility. Here we show that the PAS is in fact a liquid-like condensate of Atg proteins. The autophagy-initiating Atg1 complex undergoes phase separation to form liquid droplets in vitro, and point mutations or phosphorylation that inhibit phase separation impair PAS formation in vivo. In vitro experiments show that Atg1-complex droplets can be tethered to membranes via specific protein-protein interactions, explaining the vacuolar membrane localization of the PAS in vivo. We propose that phase separation has a critical, active role in autophagy, whereby it organizes the autophagy machinery at the PAS.
Audience Academic
Author Mouri, Kazunari
Ohsumi, Yoshinori
Ando, Toshio
Fujioka, Yuko
Noshiro, Daisuke
May, Alexander I.
Okada, Yasushi
Alam, Jahangir Md
Knorr, Roland L.
Noda, Nobuo N.
Suzuki, Kuninori
Author_xml – sequence: 1
  givenname: Yuko
  surname: Fujioka
  fullname: Fujioka, Yuko
  organization: Institute of Microbial Chemistry (BIKAKEN)
– sequence: 2
  givenname: Jahangir Md
  surname: Alam
  fullname: Alam, Jahangir Md
  organization: Institute of Microbial Chemistry (BIKAKEN)
– sequence: 3
  givenname: Daisuke
  surname: Noshiro
  fullname: Noshiro, Daisuke
  organization: Institute of Microbial Chemistry (BIKAKEN), Nano Life Science Institute (WPI-NanoLSI), Kanazawa University
– sequence: 4
  givenname: Kazunari
  surname: Mouri
  fullname: Mouri, Kazunari
  organization: Center for Biosystems Dynamics Research (BDR), RIKEN
– sequence: 5
  givenname: Toshio
  surname: Ando
  fullname: Ando, Toshio
  organization: Nano Life Science Institute (WPI-NanoLSI), Kanazawa University
– sequence: 6
  givenname: Yasushi
  surname: Okada
  fullname: Okada, Yasushi
  organization: Center for Biosystems Dynamics Research (BDR), RIKEN, Department of Physics, Universal Biology Institute (UBI) and International Research Center for Neurointelligence (WPI-IRCN), The University of Tokyo
– sequence: 7
  givenname: Alexander I.
  surname: May
  fullname: May, Alexander I.
  organization: Cell Biology Center, Institute of Innovative Research, Tokyo Institute of Technology, Tokyo Tech World Research Hub Initiative (WRHI), Institute of Innovative Research, Tokyo Institute of Technology
– sequence: 8
  givenname: Roland L.
  surname: Knorr
  fullname: Knorr, Roland L.
  organization: Department of Theory and Bio-Systems, Max Planck Institute of Colloids and Interfaces, Graduate School and Faculty of Medicine, The University of Tokyo, Max Planck Institute of Molecular Plant Physiology
– sequence: 9
  givenname: Kuninori
  surname: Suzuki
  fullname: Suzuki, Kuninori
  organization: Life Science Data Research Center, Graduate School of Frontier Sciences, The University of Tokyo, Collaborative Research Institute for Innovative Microbiology, The University of Tokyo
– sequence: 10
  givenname: Yoshinori
  surname: Ohsumi
  fullname: Ohsumi, Yoshinori
  organization: Cell Biology Center, Institute of Innovative Research, Tokyo Institute of Technology
– sequence: 11
  givenname: Nobuo N.
  surname: Noda
  fullname: Noda, Nobuo N.
  email: nn@bikaken.or.jp
  organization: Institute of Microbial Chemistry (BIKAKEN)
BackLink https://www.ncbi.nlm.nih.gov/pubmed/32025038$$D View this record in MEDLINE/PubMed
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SSID ssj0005174
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Snippet Many biomolecules undergo liquid–liquid phase separation to form liquid-like condensates that mediate diverse cellular functions 1 , 2 . Autophagy is able to...
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions . Autophagy is able to degrade...
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions.sup.1,2. Autophagy is able to...
Many biomolecules undergo liquid-liquid phase separation to form liquid-like condensates that mediate diverse cellular functions1,2. Autophagy is able to...
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SubjectTerms 13/1
14/19
14/33
14/35
631/57/2267
631/80/39
631/80/458
82/83
Adaptor Proteins, Signal Transducing - chemistry
Adaptor Proteins, Signal Transducing - genetics
Adaptor Proteins, Signal Transducing - metabolism
Autophagosomes - chemistry
Autophagosomes - metabolism
Autophagy
Autophagy (Cytology)
Autophagy-Related Proteins - chemistry
Autophagy-Related Proteins - genetics
Autophagy-Related Proteins - metabolism
Biomolecules
Condensates
Droplets
Experiments
Fragility
Humanities and Social Sciences
Kinases
Liquid phases
Localization
Mechanistic Target of Rapamycin Complex 1 - chemistry
Mechanistic Target of Rapamycin Complex 1 - metabolism
Membrane structures
Membranes
Microscopy
multidisciplinary
Multiprotein Complexes - chemistry
Multiprotein Complexes - genetics
Multiprotein Complexes - metabolism
Mutation
Observations
Phagocytosis
Phagosomes
Phase separation
Phase transformations (Statistical physics)
Phosphorylation
Physiological aspects
Point Mutation
Protein Binding
Protein interaction
Protein Kinases - chemistry
Protein Kinases - genetics
Protein Kinases - metabolism
Proteins
Saccharomyces cerevisiae - chemistry
Saccharomyces cerevisiae - cytology
Saccharomyces cerevisiae - genetics
Saccharomyces cerevisiae - metabolism
Saccharomyces cerevisiae Proteins - chemistry
Saccharomyces cerevisiae Proteins - genetics
Saccharomyces cerevisiae Proteins - metabolism
Science
Science (multidisciplinary)
Vacuoles - metabolism
Yeast fungi
Title Phase separation organizes the site of autophagosome formation
URI https://link.springer.com/article/10.1038/s41586-020-1977-6
https://www.ncbi.nlm.nih.gov/pubmed/32025038
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