Structure-function analysis on the level of individual synapses

Excitatory synapses in the mammalian brain are made on small protrusions of the postsynaptic cell called dendritic spines. Dendritic spines are highly variable in their morphology and in their microanatomy (e.g. presence of subsynaptic organelles). It is unclear whether and how variability in spine morphological and anatomical properties translates into differences in synaptic function. Using two photon imaging, we analyzed how spine properties can affect synaptic signals and the potential for synaptic plasticity at single identified spine synapses. We show that synaptic signals can be tightly regulated on the level of individual synapses and that differences in spine morphology and microanatomy regulate synaptic function. We also provide evidence for the existence of functionally distinct populations of synapses in regard to their potential for synaptic plasticity. The present thesis is subdivided into three main sections. The first section is dedicated to the analysis of the function of specialized subsynaptic organelles in regulating synaptic plasticity. In the second section we studied the impact of spine morphology on synaptic signals and in the third section we examined whether critical proteins can be tagged to individual synapses in response to plasticity inducing stimuli. In pyramidal cells, only a subset of dendritic spines contains endoplasmic reticulum (ER). Spine ER often forms a ‘spine apparatus’, a specialized organelle with unknown function. It is unclear whether these specialized subsynaptic structures can affect the function of the synapse on the spine head. The possible involvement of spine ER in shaping spine calcium transients, a key trigger for synaptic plasticity, raises the possibility that spine ER could modulate the potential of a given synapse to undergo activity dependent modifications. Using a genetic approach to label the ER in living neurons, we find that the ER preferentially localizes to spines containing strong synapses. We demonstrate that spine ER represents a specialized calcium signaling machinery required for the induction of metabotropic glutamate receptor dependent long term depression at individual synapses. We demonstrate that different subsets of synapses exist in regard to their potential to undergo specific forms of plasticity. Spine ER represents the anatomical correlate for a mechanism by which strong synapses can be retuned in an activity dependent manner. Dendritic spines are separated from their parent dendrite by a thin spine neck. The spine neck slows down diffusion of molecules from the spine head to the parent dendrite, allowing spine-specific action of second messengers and activated enzymes. The resistance of the spine neck is crucial in determining whether spines can also be considered electrical compartments. Only a high enough spine neck resistance leads to electrical compartmentalization and activation of voltage gated channels in the spine in response to synaptic stimulation. We show that spine neck resistance can change in an activity dependent manner. Using single spine calcium imaging as a reporter of NMDA receptor activation and spine head depolarization, we show that spines can indeed act as electrical compartments. Using pharmacological experiments and modeling, we demonstrate that different voltage dependent channels cooperatively participate in shaping spine head depolarization and spine calcium transients. We also show that in vivo the spine neck resistance is higher compared to the situation in acutely sliced brain tissue, demonstrating that in the living animal a higher fraction of spines can be considered electrical compartments compared to the in vitro situation. We provide strong evidence that the spine neck can profoundly affect synaptic calcium signals. Biochemical and electrical compartmentalization is dynamically regulated in an activity dependent way. Spine calcium signals can activate key signaling cascades responsible for the induction of synaptic plasticity. Long term potentiation (LTP) has been shown to require the activity of CaMKII, a serine/ threonine kinase. A chemical protocol leading to LTP has been shown to induce translocation of CaMKII to dendritic spines. It is however unclear whether this molecule acts at single synapses or whether it can spread and modulate neighboring synapses in response to more physiological protocols. Using a new optical approach to induce LTP at single visualized synapses, we show that LTP induction is accompanied by a long-lasting increase of CaMKII at the stimulated synapse. This increase was specific to the stimulated spine and did not spread to neighboring spines. We provide evidence that CaMKII acts locally, on the micrometer scale, to regulate plasticity. We show that the concentration of proteins involved in regulating synaptic plasticity can be tightly regulated at the level of single synapses

Polycomb group genes are required for neural stem cell survival in postembryonic neurogenesis of Drosophila

Genes of the Polycomb group (PcG) are part of a cellular memory system that maintains appropriate inactive states of Hox gene expression in Drosophila. Here, we investigate the role of PcG genes in postembryonic development of the Drosophila CNS. We use mosaic-based MARCM techniques to analyze the role of these genes in the persistent larval neuroblasts and progeny of the central brain and thoracic ganglia. We find that proliferation in postembryonic neuroblast clones is dramatically reduced in the absence of Polycomb, Sex combs extra, Sex combs on midleg, Enhancer of zeste or Suppressor of zeste 12. The proliferation defects in these PcG mutants are due to the loss of neuroblasts by apoptosis in the mutant clones. Mutation of PcG genes in postembryonic lineages results in the ectopic expression of posterior Hox genes, and experimentally induced misexpression of posterior Hox genes, which in the wild type causes neuroblast death, mimics the PcG loss-of-function phenotype. Significantly, full restoration of wild-type-like properties in the PcG mutant lineages is achieved by blocking apoptosis in the neuroblast clones. These findings indicate that loss of PcG genes leads to aberrant derepression of posterior Hox gene expression in postembryonic neuroblasts, which causes neuroblast death and termination of proliferation in the mutant clones. Our findings demonstrate that PcG genes are essential for normal neuroblast survival in the postembryonic CNS of Drosophila. Moreover, together with data on mammalian PcG genes, they imply that repression of aberrant reactivation of Hox genes may be a general and evolutionarily conserved role for PcG genes in CNS development

NMDA receptor-dependent GABAB receptor internalization via CaMKII phosphorylation of serine 867 in GABAB1

GABAB receptors are the G-protein–coupled receptors for GABA, the main inhibitory neurotransmitter in the brain. GABAB receptors are abundant on dendritic spines, where they dampen postsynaptic excitability and inhibit Ca2+ influx through NMDA receptors when activated by spillover of GABA from neighboring GABAergic terminals. Here, we show that an excitatory signaling cascade enables spines to counteract this GABAB-mediated inhibition. We found that NMDA application to cultured hippocampal neurons promotes dynamin-dependent endocytosis of GABAB receptors. NMDA-dependent internalization of GABAB receptors requires activation of Ca2+/Calmodulin-dependent protein kinase II (CaMKII), which associates with GABAB receptors in vivo and phosphorylates serine 867 (S867) in the intracellular C terminus of the GABAB1 subunit. Blockade of either CaMKII or phosphorylation of S867 renders GABAB receptors refractory to NMDA-mediated internalization. Time-lapse two-photon imaging of organotypic hippocampal slices reveals that activation of NMDA receptors removes GABAB receptors within minutes from the surface of dendritic spines and shafts. NMDA-dependent S867 phosphorylation and internalization is predominantly detectable with the GABAB1b subunit isoform, which is the isoform that clusters with inhibitory effector K+ channels in the spines. Consistent with this, NMDA receptor activation in neurons impairs the ability of GABAB receptors to activate K+ channels. Thus, our data support that NMDA receptor activity endocytoses postsynaptic GABAB receptors through CaMKII-mediated phosphorylation of S867. This provides a means to spare NMDA receptors at individual glutamatergic synapses from reciprocal inhibition through GABAB receptors