Reconstitution of a microtubule plus-end tracking system in vitro

The microtubule cytoskeleton is essential to cell morphogenesis. Growing microtubule plus ends have emerged as dynamic regulatory sites in which specialized proteins, called plus-end-binding proteins (+TIPs), bind and regulate the proper functioning of microtubules. However, the molecular mechanism...

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Published inNature Vol. 450; no. 7172; pp. 1100 - 1105
Main Authors Bieling, Peter, Brunner, Damian, Munteanu, E. Laura, Surrey, Thomas, Sandblad, Linda, Dogterom, Marileen, Schek, Henry, Laan, Liedewij
Format Journal Article
LanguageEnglish
Published London Nature Publishing 13.12.2007
Nature Publishing Group
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Abstract The microtubule cytoskeleton is essential to cell morphogenesis. Growing microtubule plus ends have emerged as dynamic regulatory sites in which specialized proteins, called plus-end-binding proteins (+TIPs), bind and regulate the proper functioning of microtubules. However, the molecular mechanism of plus-end association by +TIPs and their ability to track the growing end are not well understood. Here we report the in vitro reconstitution of a minimal plus-end tracking system consisting of the three fission yeast proteins Mal3, Tip1 and the kinesin Tea2. Using time-lapse total internal reflection fluorescence microscopy, we show that the EB1 homologue Mal3 has an enhanced affinity for growing microtubule end structures as opposed to the microtubule lattice. This allows it to track growing microtubule ends autonomously by an end recognition mechanism. In addition, Mal3 acts as a factor that mediates loading of the processive motor Tea2 and its cargo, the Clip170 homologue Tip1, onto the microtubule lattice. The interaction of all three proteins is required for the selective tracking of growing microtubule plus ends by both Tea2 and Tip1. Our results dissect the collective interactions of the constituents of this plus-end tracking system and show how these interactions lead to the emergence of its dynamic behaviour. We expect that such in vitro reconstitutions will also be essential for the mechanistic dissection of other plus-end tracking systems.
AbstractList The microtubule cytoskeleton is essential to cell morphogenesis. Growing microtubule plus ends have emerged as dynamic regulatory sites in which specialized proteins, called plus-end-binding proteins (+TIPs), bind and regulate the proper functioning of microtubules. However, the molecular mechanism of plus-end association by +TIPs and their ability to track the growing end are not well understood. Here we report the in vitro reconstitution of a minimal plus-end tracking system consisting of the three fission yeast proteins Mal3, Tip1 and the kinesin Tea2. Using time-lapse total internal reflection fluorescence microscopy, we show that the EB1 homologue Mal3 has an enhanced affinity for growing microtubule end structures as opposed to the microtubule lattice. This allows it to track growing microtubule ends autonomously by an end recognition mechanism. In addition, Mal3 acts as a factor that mediates loading of the processive motor Tea2 and its cargo, the Clip170 homologue Tip1, onto the microtubule lattice. The interaction of all three proteins is required for the selective tracking of growing microtubule plus ends by both Tea2 and Tip1. Our results dissect the collective interactions of the constituents of this plus-end tracking system and show how these interactions lead to the emergence of its dynamic behaviour. We expect that such in vitro reconstitutions will also be essential for the mechanistic dissection of other plus-end tracking systems.
The microtubule cytoskeleton is essential to cell morphogenesis. Growing microtubule plus ends have emerged as dynamic regulatory sites in which specialized proteins, called plus-end-binding proteins (+TIPs), bind and regulate the proper functioning of microtubules. However, the molecular mechanism of plus-end association by +TIPs and their ability to track the growing end are not well understood. Here we report the in vitro reconstitution of a minimal plus-end tracking system consisting of the three fission yeast proteins Mal3, Tip1 and the kinesin Tea2. Using time-lapse total internal reflection fluorescence microscopy, we show that the EB1 homologue Mal3 has an enhanced affinity for growing microtubule end structures as opposed to the microtubule lattice. This allows it to track growing microtubule ends autonomously by an end recognition mechanism. In addition, Mal3 acts as a factor that mediates loading of the processive motor Tea2 and its cargo, the Clip170 homologue Tip1, onto the microtubule lattice. The interaction of all three proteins is required for the selective tracking of growing microtubule plus ends by both Tea2 and Tip1. Our results dissect the collective interactions of the constituents of this plus-end tracking system and show how these interactions lead to the emergence of its dynamic behaviour. We expect that such in vitro reconstitutions will also be essential for the mechanistic dissection of other plus-end tracking systems. [PUBLICATION ABSTRACT]
Audience Academic
Author Surrey, Thomas
Laan, Liedewij
Bieling, Peter
Schek, Henry
Dogterom, Marileen
Brunner, Damian
Sandblad, Linda
Munteanu, E. Laura
Author_xml – givenname: Peter
  surname: Bieling
  fullname: Bieling, Peter
  organization: European Molecular Biology Laboratory, Cell Biology and Biophysics Unit
– givenname: Damian
  surname: Brunner
  fullname: Brunner, Damian
  organization: European Molecular Biology Laboratory, Cell Biology and Biophysics Unit
– givenname: E. Laura
  surname: Munteanu
  fullname: Munteanu, E. Laura
  organization: FOM Institute for Atomic and Molecular Physics (AMOLF)
– givenname: Thomas
  surname: Surrey
  fullname: Surrey, Thomas
  organization: European Molecular Biology Laboratory, Cell Biology and Biophysics Unit
– givenname: Linda
  surname: Sandblad
  fullname: Sandblad, Linda
  organization: European Molecular Biology Laboratory, Cell Biology and Biophysics Unit
– givenname: Marileen
  surname: Dogterom
  fullname: Dogterom, Marileen
  organization: FOM Institute for Atomic and Molecular Physics (AMOLF)
– givenname: Henry
  surname: Schek
  fullname: Schek, Henry
  organization: European Molecular Biology Laboratory, Cell Biology and Biophysics Unit
– givenname: Liedewij
  surname: Laan
  fullname: Laan, Liedewij
  organization: FOM Institute for Atomic and Molecular Physics (AMOLF)
BackLink http://pascal-francis.inist.fr/vibad/index.php?action=getRecordDetail&idt=19893827$$DView record in Pascal Francis
https://www.ncbi.nlm.nih.gov/pubmed/18059460$$D View this record in MEDLINE/PubMed
https://urn.kb.se/resolve?urn=urn:nbn:se:umu:diva-59010$$DView record from Swedish Publication Index
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Keywords Ascomycota
Fungi
Schizosaccharomyces pombe
Cytoskeleton
Molecular interaction
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Reconstitution
Microtubule
In vitro
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D Brunner (BFnature06386_CR16) 2000; 102
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H Browning (BFnature06386_CR25) 2005; 280
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H Browning (BFnature06386_CR18) 2000; 151
ES Folker (BFnature06386_CR29) 2005; 16
D Axelrod (BFnature06386_CR21) 2001; 2
Y Mimori-Kiyosue (BFnature06386_CR7) 2000; 148
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Snippet The microtubule cytoskeleton is essential to cell morphogenesis. Growing microtubule plus ends have emerged as dynamic regulatory sites in which specialized...
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SubjectTerms Biological and medical sciences
Cell structures and functions
Cell-Free System
Cellular biology
Cytoskeleton, cytoplasm. Intracellular movements
Fluorescence
Fluorescence microscopy
Fundamental and applied biological sciences. Psychology
Heat-Shock Proteins - metabolism
Intermediate Filament Proteins - metabolism
Microscopy
Microscopy, Fluorescence
Microtubule-Associated Proteins - metabolism
Microtubules - chemistry
Microtubules - metabolism
Molecular and cellular biology
Molecular biology
Proteins
Schizosaccharomyces - chemistry
Schizosaccharomyces - cytology
Schizosaccharomyces pombe
Schizosaccharomyces pombe Proteins - metabolism
Yeast
Yeasts
Title Reconstitution of a microtubule plus-end tracking system in vitro
URI http://dx.doi.org/10.1038/nature06386
https://www.ncbi.nlm.nih.gov/pubmed/18059460
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https://search.proquest.com/docview/743410133
https://urn.kb.se/resolve?urn=urn:nbn:se:umu:diva-59010
Volume 450
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