Inactivity produces increases in neurotransmitter release and synapse size.

When hippocampal synapses in culture are pharmacologically silenced for several days, synaptic strength increases. The structural correlate of this change in strength is an increase in the size of the synapses, with all synaptic components--active zone, postsynaptic density, and bouton--becoming larger. Further, the number of docked vesicles and the total number of vesicles per synapse increases, although the number of docked vesicles per area of active zone is unchanged. In parallel with these anatomical changes, the physiologically measured size of the readily releasable pool (RRP) and the release probability are increased. Ultrastructural analysis of individual synapses in which the RRP was previously measured reveals that, within measurement error, the same number of vesicles are docked as are estimated to be in the RRP.

Morphological correlates of functionally defined synaptic vesicle populations.

By combining photoconversion of FM1-43-stained vesicles and electron microscopy of hippocampal synapses, we find evidence that the population of morphologically docked synaptic vesicles corresponds to the release-ready neurotransmitter quanta. Furthermore, those synaptic vesicles that are participating in cycles of exo- and endocytosis tend to be closer to the active zone than vesicles that are being held in reserve.

Quantitative fine-structural analysis of olfactory cortical synapses.

To determine the extent to which hippocampal synapses are typical of those found in other cortical regions, we have carried out a quantitative analysis of olfactory cortical excitatory synapses, reconstructed from serial electron micrograph sections of mouse brain, and have compared these new observations with previously obtained data from hippocampus. Both superficial and deep layer I olfactory cortical synapses were studied. Although individual synapses in each of the areas-CA1 hippocampus, olfactory cortical layer Ia, olfactory cortical area Ib-might plausibly have been found in any of the other areas, the average characteristics of the three synapse populations are distinct. Olfactory cortical synapses in both layers are, on average, about 2.5 times larger than their hippocampal counterparts. The layer Ia olfactory cortical synapses have fewer synaptic vesicles than do the layer Ib synapses, but the absolute number of vesicles docked to the active zone in the layer Ia olfactory cortical synapses is about equal to the docked vesicle number in the smaller hippocampal synapses. As would be predicted from studies on hippocampus that relate paired-pulse facilitation to the number of docked vesicles, the synapses in layer 1a exhibit facilitation, whereas the ones in layer 1b do not. Although hippocampal synapses provide as a good model system for central synapses in general, we conclude that significant differences in the average structure of synapses from one cortical region to another exist, and this means that generalizations based on a single synapse type must be made with caution.

Comparison of hippocampal dendritic spines in culture and in brain.

We have quantified hippocampal spine structure at the light and ultrastructural levels in cell cultures approximately 1- 3 weeks old and in the brains of rodents 5 and 21 d old. The number of spines bearing synapses increases with age in cultures and in brain, but the structures are similar in both. In culture, about half of the synapses are formed on spines and the remainder are formed on dendritic shafts. In the 5-d-old brain, about half of the synapses occur on dendritic shafts, by 3 weeks of age only approximately 20% of synapses are found on dendritic shafts, and in the adult shaft synapses are very rare.

An essential role for retinoid receptors RARbeta and RXRgamma in long-term potentiation and depression.

Hippocampal long-term potentiation (LTP) and long-term depression (LTD) are the most widely studied forms of synaptic plasticity thought to underlie spatial learning and memory. We report here that RARbeta deficiency in mice virtually eliminates hippocampal CA1 LTP and LTD. It also results in substantial performance deficits in spatial learning and memory tasks. Surprisingly, RXRgamma null mice exhibit a distinct phenotype in which LTD is lost whereas LTP is normal. Thus, while retinoid receptors contribute to both LTP and LTD, they do so in different ways. These findings not only genetically uncouple LTP and LTD but also reveal a novel and unexpected role for vitamin A in higher cognitive functions.

Quantitative ultrastructural analysis of hippocampal excitatory synapses.

From three-dimensional reconstructions of CA1 excitatory synapses in the rodent hippocampus and in culture, we have estimated statistical distributions of active zone and postsynaptic density (PSD) sizes (average area approximately 0.04 micron2), the number of active zones per bouton (usually one), the number of docked vesicles per active zone (approximately 10), and the total number of vesicles per bouton (approximately 200), and we have determined relationships between these quantities, all of which vary from synapse to synapse but are highly correlated. These measurements have been related to synaptic physiology. In particular, we propose that the distribution of active zone areas can account for the distribution of synaptic release probabilities and that each active zone constitutes a release site as identified in the standard quantal theory attributable to Katz (1969).

Immunocytochemical characterization of the synaptic innervation of a single spinal neuron, the electric catfish electromotoneuron.

The electric catfish, Malapterurus electricus, possesses electric organs that are innervated by a pair of identifiable electromotoneurons located within the cervical spinal cord. The pattern of synaptic innervation of the electromotoneurons can be revealed by an antibody against the synaptic vesicle protein SV2. Both somata and proximal dendrites are densely innervated. Several transmitters contribute to this innervation. Glutamate, the neurotransmitter of the dorsal root sensory fibers, reveals a weak punctuate immunoreactivity. The previously described electrical synapses of the electromotoneurons were visualized by an antibody against a gap-junctional protein. In contrast to the electromotoneurons of other electric fish, the electric catfish electromotoneurons possess many inhibitory synapses. With antibodies against glycine and against the glycine receptor, a dense immunoreactivity of the surface of the somata and proximal dendrites can be revealed. The glycine receptor-like immunoreactivity exhibits a patch-like distribution similar to that revealed by the anti-SV2 antibody. gamma-Aminobutyric acid (GABA)-immunopositive terminals contribute to the inhibitory electromotoneuron innervations to a lesser degree. The chemical characteristics of the electromotoneuron innervations of Malapterurus resemble those of other spinal motoneurons rather than spinal electromotoneurons of other electric fish. Thus our immunocytochemical study supports the view that the pattern of electromotoneuron innervations in Malapterurus reveals little specialization. The capacity for information processing required for the control of the electric organ discharge appears to be achieved by the increased integrational capacity of the newly evolved multiple dendrites and not by an additional parallel channel specific for the electromotor system.

Projection of brain stem neurons to the giant electromotoneurons in the cervical spinal cord of the electric catfish Malapterurus electricus.

Two giant electromotoneurons located within the cervical spinal cord form the centerpiece of the electromotor system in the electric catfish Malapterurus electricus. The cytoarchitectural organization suggests a high degree of input convergence onto the electromotoneurons. In order to obtain insights into the connectivities of the electromotor system, pre-neurons of the electromotoneurons within the brain stem and the spinal cord were labelled by application of FITC-dextran and horseradish peroxidase onto the surface of a single electromotoneuron. Our results show that the electromotoneurons receive their main inputs from the nucleus profundus mesencephali within the tegmentum and from large neurons of the medial reticular formation. Both nuclei possess an intimate connection to the optic tectum which mediates orientation responses. This pathway to the electromotoneurons could be instrumental in eliciting electric organ discharge during prey catching. The electric avoidance response in turn could be mediated by the Mauthner neurons which are also labelled. In addition to these neurons, cells of the nucleus fasciculi longitudinalis medialis, the descending octaval nucleus and the nucleus funicularis medialis were labelled. As compared to the corresponding neurons in ictalurid catfish, none of these neurons displays any alteration in its general morphology. It is concluded that the evolution of the electric organ from muscle tissue and the development of a central control system of the electromotor response in Malapterurus involved a minimum of alterations in central nervous system circuitry. In contrast to many other electric fishes the electromotor control is mainly accomplished at the level of the electromotoneurons.

Cytoplasmic segregation and cytoskeletal organization in the electric catfish giant electromotoneuron with special reference to the axon hillock region.

The cytoplasm of the highly polarized nerve cell is permanently segregated into domains with differing organellar composition. The mechanisms maintaining this segregation are largely unknown. In order to elucidate the potential role of cytoskeletal elements in this process we compared the cytoplasmic segregation within the giant electromotoneuron of the electric catfish (Malapterurus electricus) with the distribution of binding sites for antibodies against elements of the cytoskeleton. Most prominent cytoplasmic segregations include the formation of a subplasmalemmal cortical structure free of Nissl bodies and Golgi cisternae, the separation within the soma of domains containing rough endoplasmic reticulum and filament-rich domains, and the soma-axon transition. The cytoplasmic transition at the axon hillock forms a distinct borderline where Nissl bodies, Golgi cisternae and the bulk of lysosomes abruptly terminate and are excluded from the axoplasm. Synaptic vesicles and mitochondria are free to pass compartmental borders. Tropomyosin, spectrin, and alpha-actinin reveal a rather homogeneous immunofluorescence throughout the neuron. In contrast, neurofilament protein and tubulin display a distinctly increased immunofluorescence in the subplasmalemmal cortical layer, in dendrites as well as in the axon. The increase in immunofluorescence at the axon hillock exactly depicts the small transition zone from the somatic cytoplasm rich in Nissl bodies, Golgi cisternae and lysosomes to the differently structured axoplasm. The picture is similar for beta-tubulin, tyrosinylated and detyrosinylated alpha-tubulin. Detyrosinylated tubulin (glu-tubulin, which is contained in microtubules of increased stability) shows the most prominent enrichment in the axon. The distribution of myosin is comparable to that of neurofilament protein but there is less difference in immunofluorescence between the domains. Our results would be compatible with a role of microtubules together with (the closely associated) neurofilaments in the segregation of neuronal cytoplasmic domains. Active transport as well as stable binding to the somatic cytoskeleton might counteract a homogeneous cytoplasmic distribution of the various classes of organelles by diffusion.