AI Article Synopsis

  • Researchers used a dual fluorescence resonance energy transfer (FRET) imaging platform to study how glutamate release rates affect enzyme activation in hippocampal neurons.
  • At a 5 Hz glutamate uncaging frequency, calcineurin was activated without notable spine changes, while CaMKIIα remained inactive.
  • When the frequency increased to 20 Hz, both enzymes were activated, but their responses were distinct; CaMKIIα acted as a decoder for input frequency and number, while calcineurin primarily counted inputs without strong frequency sensitivity.

Article Abstract

How information encoded in glutamate release rates at individual synapses is converted into biochemical activation patterns of postsynaptic enzymes remains unexplored. To address this, we developed a dual fluorescence resonance energy transfer (FRET) imaging platform and recorded CaMKIIα and calcineurin activities in hippocampal neurons while varying glutamate uncaging frequencies. With little spine morphological change, 5 Hz spine glutamate uncaging strongly stimulated calcineurin, but not CaMKIIα. In contrast, 20 Hz spine glutamate uncaging, which induced spine growth, activated both CaMKIIα and calcineurin with distinct spatiotemporal kinetics. Higher temporal resolution recording in the soma revealed that CaMKIIα activity summed supralinearly and sensed both higher frequency and input number, thus acting as an input frequency/number decoder. In contrast, calcineurin activity summated sublinearly with increasing input number and showed little frequency dependence, thus functioning as an input number counter. These results provide evidence that CaMKIIα and calcineurin are fine-tuned to unique bandwidths and compute input variables in an asymmetric manner.

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Source
http://dx.doi.org/10.1016/j.celrep.2013.03.033DOI Listing

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