ZFIN ID: ZDB-PUB-990507-14
Monitoring activity in neuronal populations with single-cell resolution in a behaving vertebrate
Fetcho, J.R., Cox, K.J., and O'Malley, D.M.
Date: 1998
Source: The Histochemical journal   30(3): 153-167 (Journal)
Registered Authors: Cox, Kingsley, Fetcho, Joseph R., O'Malley, Donald
Keywords: none
MeSH Terms:
  • Animals
  • Behavior, Animal/physiology*
  • Electric Stimulation
  • Escape Reaction/physiology
  • Fluorescent Dyes
  • Larva/physiology
  • Microscopy, Confocal/methods
  • Motor Neurons/physiology*
  • Organic Chemicals
  • Pons/cytology
  • Spinal Cord/cytology
  • Spinal Cord/physiology
  • Zebrafish/physiology*
PubMed: 10188924 Full text @ Histochem. J.
ABSTRACT
Vertebrate behaviours are produced by activity in populations of neurons, but the techniques typically used to study activity allow only one or very few nerve cells to be monitored at a time. This limitation has prompted the development of methods of imaging activity in the nervous system. The overall goal of these methods is to image neural activity non-invasively in populations of neurons, ideally with high spatial and temporal resolution. We have moved closer to this goal by using confocal calcium imaging to monitor neural activity in the transparent larvae of zebrafish. Neurons were labelled either by backfilling from injections of the calcium indicator (Calcium Green dextran) into muscle or spinal cord of larvae or by injections into blastomeres early in development. The labelled neurons were bright enough at resting calcium levels to allow the identification of individual neurons in the live, intact fish, based upon their dendritic and axonal morphology. The neurons from the live animal could also be reconstructed in three dimensions for morphometric study. Neurons increased their fluorescence during activity produced by direct electrical stimulation and during escape behaviours elicited by an abrupt touch to the head or tail of the fish. The rise in calcium associated with a single action potential could be detected as an increase in fluorescence of at least 7-10%, but neurons typically showed much larger increases during behaviour. Calcium signals in the dendrites, soma and nucleus could be resolved, especially when using the line-scanning mode, which provides 2-ms temporal resolution. The imaging was used to study activity in populations of motoneurons and hindbrain neurons during the escape behaviour fish use to avoid predators. We found a massive activation of the motoneuron pool and a differential activation of populations of hindbrain neurons during escapes. The latter finding confirms predictions that the activity pattern of hindbrain neurons may help to determine the directionality of the escape. This approach should prove useful for studying the activity of populations of neurons throughout the nervous system in both normal and mutant lines of fish.
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