Comparison of slow and fast neocortical neuron migration using a new in vitro model

Mutations, toxic insults and radiation exposure are known to slow or arrest the migration of cortical neurons, in most cases by unknown mechanisms. The movement of migrating neurons is saltatory, reflecting the intermittent movement of the nucleus (nucleokinesis) within the confines of the plasma me...

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Published inBMC neuroscience Vol. 9; no. 1; p. 50
Main Authors Nichols, Anna J, Carney, Laurel H, Olson, Eric C
Format Journal Article
LanguageEnglish
Published England BioMed Central Ltd 05.06.2008
BioMed Central
BMC
Subjects
Animals
Cell Adhesion - drug effects
Cell Adhesion - physiology
Cell culture
Cell Culture Techniques
Cell Movement - physiology
Cells, Cultured
Cytoskeleton
Dextran Sulfate - pharmacology
Immunohistochemistry
Kinetics
Methodology
Methods
Mice
Neocortex - cytology
Neuroglia - physiology
Neurons
Neurons - cytology
Neurons - physiology
Physiological aspects
Properties
United States
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Summary:Mutations, toxic insults and radiation exposure are known to slow or arrest the migration of cortical neurons, in most cases by unknown mechanisms. The movement of migrating neurons is saltatory, reflecting the intermittent movement of the nucleus (nucleokinesis) within the confines of the plasma membrane. Each nucleokinetic movement is analogous to a step. Thus, average migration speed could be reduced by lowering step frequency and/or step distance. To assess the kinetic features of cortical neuron migration we developed a cell culture system that supports fiber-guided migration. In this system, the majority of fiber-apposed cells were neurons, expressed age-appropriate cortical-layer specific markers and migrated during a 30 min imaging period. Comparison of the slowest and fastest quartiles of cells revealed a 5-fold difference in average speed. The major determinant of average speed in slower cells (6-26 microm/hr) was step frequency, while step distance was the critical determinant of average speed in faster cells (>26 microm/hr). Surprisingly, step distance was largely determined by the average duration of the step, rather than the speed of nucleokinesis during the step, which differed by only 1.3-fold between the slowest and fastest quartiles. Saltatory event frequency and duration, not nucleokinetic speed, are the major determinants of average migration speed in healthy neurons. Alteration of either saltatory event frequency or duration should be considered along with nucleokinetic abnormalities as possible contributors to pathological conditions.
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ISSN:1471-2202
1471-2202
DOI:10.1186/1471-2202-9-50