4.7 Article

Divergent Synaptic Scaling of Miniature EPSCs following Activity Blockade in Dissociated Neuronal Cultures

期刊

JOURNAL OF NEUROSCIENCE
卷 40, 期 21, 页码 4090-4102

出版社

SOC NEUROSCIENCE
DOI: 10.1523/JNEUROSCI.1393-19.2020

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资金

  1. National Institute of Neurological Disorders and Stroke (NINDS) [P01 NS057228]
  2. NINDS [R01NS065992]
  3. Canadian Institutes of Health Research
  4. Natural Sciences and Engineering Research Council of Canada
  5. National Science Foundation [GRFP 09-603]
  6. Heart and Stroke Foundation, Canada

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Neurons can respond to decreased network activity with a homeostatic increase in the amplitudes of miniature EPSCs (mEPSCs). The prevailing view is that mEPSC amplitudes are uniformly multiplied by a single factor, termed synaptic scaling. Deviations from purely multiplicative scaling have been attributed to biological differences, or to a distortion imposed by a detection threshold limit. Here, we demonstrate in neurons dissociated from cortices of male and female mice that the shift in mEPSC amplitudes observed in the experimental data cannot be reproduced by simulation of uniform multiplicative scaling, with or without the distortion caused by applying a detection threshold. Furthermore, we demonstrate explicitly that the scaling factor is not uniform but is close to 1 for small mEPSCs, and increases with increasing mEPSC amplitude across a substantial portion of the data. This pattern was also observed for previously published data from dissociated mouse hippocampal neurons and dissociated rat cortical neurons. The finding of divergent scaling shifts the current view of homeostatic plasticity as a process that alters all synapses on a neuron equally to one that must accommodate the differential effect observed for small versus large mEPSCs. Divergent scaling still accomplishes the essential homeostatic task of modifying synaptic strengths in the opposite direction of the activity change, but the consequences are greatest for those synapses which individually are more likely to bring a neuron to threshold.

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