DISSECTIFT
In vitro reconstitution and mechanistic dissection of Intraflagellar Transport in C.elegans sensory cilia
| Coordinatore | TECHNISCHE UNIVERSITAET MUENCHEN
Spiacenti, non ci sono informazioni su questo coordinatore. Contattare Fabio per maggiori infomrazioni, grazie. |
| Nazionalità Coordinatore | Germany [DE] |
| Totale costo | 1˙497˙740 € |
| EC contributo | 1˙497˙740 € |
| Programma | FP7-IDEAS-ERC
Specific programme: "Ideas" implementing the Seventh Framework Programme of the European Community for research, technological development and demonstration activities (2007 to 2013) |
| Code Call | ERC-2013-StG |
| Funding Scheme | ERC-SG |
| Anno di inizio | 2014 |
| Periodo (anno-mese-giorno) | 2014-03-01 - 2019-02-28 |
Partecipanti
| # | ||||
|---|---|---|---|---|
| 1 |
TECHNISCHE UNIVERSITAET MUENCHEN
Organization address
address: Arcisstrasse 21 contact info |
DE (MUENCHEN) | hostInstitution | 1˙497˙740.00 |
| 2 |
TECHNISCHE UNIVERSITAET MUENCHEN
Organization address
address: Arcisstrasse 21 contact info |
DE (MUENCHEN) | hostInstitution | 1˙497˙740.00 |
Mappa
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Obiettivo del progetto (Objective)
'Cilia are microtubule-based protrusions of the plasma membrane found on many eukaryotic cells, including most cell types of the human body. Whereas the functions of motile cilia were immediately obvious, the role of the immotile or so-called primary cilia remained largely unrecognized for many decades. Once referred to as aberrant solitary cilia with no obvious function, these ancient structures now hold the promise of revealing no less than the secrets of multicellularity and development. Even though the importance of primary cilia is now evident, molecular mechanisms underlying their assembly and function are far from being understood. The construction and maintenance of cilia relies on an ancient, universally conserved machinery termed IntraFlagellar Transport (IFT). IFT requires a multi-subunit, non-membranous protein complex assembled from more than 20 distinct subunits. At the heart of IFT are the microtubule-associated motors, -kinesin and dynein-, that continuously ferry cargo in a bi-directional fashion needed for ciliary assembly and function. To pave the way towards a molecular understanding of this fascinating organelle, we propose to employ a bottom-up approach in which we stepwise reconstitute the IFT complex from recombinantly expressed subunits of the so far best understood primary cilium from C.elegans. The structural integrity and stability of the IFT complex will be characterized using multifaceted approaches such as chemical crosslinking or thermophoresis. To mechanistically dissect the kinesin-dependent transport in vitro, we will make use of enzymatic bulk and single-molecule assays. Collectively, these results will provide a quantitative understanding of the assembly and kinesin-dependent motility of the IFT machinery. Given that cells mobilize ~600 components to build their cilia, this experimental platform will significantly streamline future efforts to identify novel cargoes and the effects of putative regulators of the IFT machinery.'