Imaging brain circuits in health and disease

Roscoff (Brittany), France, June 30-July 4, 2010

 

Deadline for application: March 15, 2010

 

Chairperson: Arthur Konnerth

Institute of Neurosciences, TUM,
Biedersteiner Str. 29, 80802 München, Allemagne
Téléphone : + 49 89 4140-3350 – Télécopie : + 49 89 4140-3352
Mèl : arthur.konnerth@lrz.tum.de

 

Vice-Chairperson: Daniel Choquet

CNRS UMR 5091 - Université Bordeaux 2, Physiologie Cellulaire de la Synapse,
rue Camille Saint-Saëns, 33077 Bordeaux, France
Phone: 33 (0) 5 57 57 40 90 – Fax: 33 (0) 5 57 57 40 82
Mèl : dchoquet@u-bordeaux2.fr

 

Imaging the brain at the cellular level provides essential information about its anatomy, function and pathology. Ever since the groundbreaking work of Golgi and Ramón y Cajal more than a century ago, many approaches have been developed to label and visualize nerve cells. Using specific labeling molecules in brain tissue, images can be obtained by using illumination, magnetization, radiation, or other physical processes. Changes in intracellular calcium ion concentrations [Ca²⁺]_i, for example, have been extensively studied in brain tissue over the past two decades. Ca²⁺ is an intracellular messenger involved in many cellular functions such as contraction, secretion, excitability and neuronal plasticity. Because calcium fluxes are tightly linked to neuronal electrical activity, recordings of intracellular free calcium dynamics are used to monitor indirectly the electrical activity of individual neurons.

The development of calcium indicators for fluorometric microscopy has opened up a wide field of research in calcium signaling. Originally, Roger Tsien and his colleagues developed small synthetic molecules, like fura-2 and fluo-3, which were rapidly adopted by many laboratories world-wide and still intensively used. The introduction of fluorescent proteins, like GFP, allowed tagging specific cell types or subcellular compartments. Recently, genetically engineered fluorescent proteins have been combined with calcium-sensitive proteins in order to measure calcium directly in defined subsets of cells. An advantage of genetically-encoded calcium indicators compared to synthetic dyes is the possibility of performing long-term calcium imaging in vivo, not only at the cellular level but also in specific subcellular compartments. Some genetically-encoded calcium indicators contain a single fluorescent protein while others have been engineered based on changes in fluorescence resonance energy transfer (FRET) efficiency between two different mutants of GFP, a technique that had previously been widely applied to image protein-protein interactions.

The goal of the conference “Imaging brain circuits in health and disease” is to show how these new advances have allowed neurobiologists to investigate the brain circuits at the level of single neurons, synapses and small brain ensembles such as cortical columns, in the living brain of healthy and diseased animals. The conference is structured in several topics:

• Probes and approaches for in vivo imaging
• Analysis of synaptic function at the nano-scale
• Probes to manipulate neural activity
• Super-resolution
• Functional analysis of brain circuits in vitro
• Functional analysis of brain circuits in vivo
• Connectome analysis
• Functional analyses in behaving animals
• Imaging brain disease

 

Invited speakers

(provisional titles)

 

BRECHT Michael (Berlin, Germany)
Mapping a small mammalian brain

CHARPAK Serge (Paris, France)
Two-photon imaging of neuronal activity and blood flow

CHOQUET Daniel (Bordeaux, France)
Glutamate receptor trafficking

COSSART Rosa (Marseille, France)
Imaging of network activity

DEISSEROTH Karl (Stanford, USA)
Optical control of neuronal activity

DENK Winfried (Heidelberg, Germany)
Imaging the brain with photons and electrons

DIEUDONNÉ Stéphane (Paris, France)
High-speed two photon imaging

DI GREGORIO David (Paris, France)
Subcellular optical detection of membrane voltage

FELLER Marla (Berkeley, USA)
Retinal waves

FITZPATRICK David (Durham, USA)
Functional organization of neural circuits in primary visual cortex

HÄUSSER Michael (London, UK)
Cerebellar circuit function in vivo

HELMCHEN Fritjof (Zürich, Switzerland)
New imaging approaches to record neuronal activity in vivo

HÜBENER Mark (München, Allemagne)
Brain circuit plasticity

KANO Masanobu (Tokyo, Japon)
Cerebellar synapse elimination

KONNERTH Arthur (München, Germany)
Optical monitoring of dendritic activity in vivo

LARKUM Matthew (Bern, Switzerland)
Imaging dendritic spike activity in vivo

LICHTMAN Jeff (Boston, USA)
Connectome analysis

LIVET Jean (Paris, France)
Brainbow mice: a tool for circuit analysis

LLANO Isabel (Paris, France)
Cerebellar calcium signalling

MARTY Alain (Paris, France)
Dynamics of the cerebellar inhibitory circuitry

MIESENBOCK Gero (Oxford, UK)
Lighting up the brain

MIYAWAKI Atsushi (Riken, Japan)
Development of fluorescent indicators

MULLE Christophe (Bordeaux, France)
Kainate receptors and synaptic transmission

MURPHY Tim (Vancouver, Canada)
Imaging mouse models of stroke

NÄGERL Valentin (Bordeaux, France)
Live-cell imaging at nanoscopic resolution by STED microscopy

OHEIM Martin (Paris, France)
Single molecule imaging

ROCHEFORT Nathalie (München, Germany)
Two-photon imaging of the mouse visual cortex in vivo

SAKMANN Bert (München, Germany)
Neurophysiology of decision making in the rodent brain

SCHNITZER Mark (Stanford, USA)
Microendoscopy in behaving animals

SILVER Angus (London, UK)
Synaptic mechanisms and signal processing

TANK David (Princeton, USA)
Imaging in behaving animals

TRAUNER Dirk (München, Germany)
Optical control of neuronal activity: functional reengineering of ion channels

TRILLER Antoine (Paris, France)
GABA receptor trafficking

 

Deadline for application: March 15, 2010

 

Registration fee (including board and lodging)

320 € for PhD students
500 € for other participants

 

Application for registration

The total number of participants is limited to about 115 and all participants are expected to attend for the whole duration of the conference. Selection is made on the basis of the affinity of potential participants with the topics of the conference. Scientists and PhD Students interested in the meeting should send:

• their curriculum vitae
• the list of their main publications for the 3 last years
• the abstract of their presentation

 

to the Chairperson of the conference before the deadline. After it, the chairman will select the participants. Except in some particular cases approved by the Chairperson, it is recommended that all selected participants present their work during the conference, either in poster form or by a brief in- session talk. The organizers choose the form in which the presentations are made. No payment will be sent with application. Information on how and when to pay will be mailed in due time to those selected.