The ultrastructure of the subnucleus gelatinosus of the nucleus of the tractus solitarius in the cat

The dorsomedial region of the nucleus of the tractus solitarius termed the subnucleus gelatinosus (SNG) was studied at the light and electron microscopic level in the cat. In cresyl violet and luxol fast blue stained sections the SNG contained small neuronal somata that were scattered throughout a pale-staining neuropil containing few myelinated fibers. These neurons were difficult to impregnate with Golgi staining techniques, but in successful impregnations the somata were observed to be 10--19 micrometers in diameter and bore few sparsely branching primary dendrites. Spines were present on the dendrites of some neurons and were more numerous on distal portions of the dendritic tree. Ultrastructural examination of the SNG revealed that the neuronal complement consisted of round, oval, or spindle shaped neurons with little or no organized Nissl substance. Rare myelin-like ensheathments of neuronal perikarya were also observed. Bundles of fine unmyelinated axons that coursed mainly longitudinally were a prominent feature of the area. The most common type of axon terminal observed contained mainly round clear vesicles, approximately 31 nm in diameter, and made asymmetrical synaptic contact with a dendritic profile. Pleomorphic vesicle-containing terminals involved in symmetrical synaptic contact were also commonly seen. Axodendritic and axosomatic synapses were associated with terminals containing either round clear vesicles or pleomorphic vesicles. Less commonly, dendrodendritic and dendrosomatic synapses were seen, the presynaptic elements of which contained pleomorphic vesicles. Following removal of a nodose ganglion, degenerating terminals of vagal afferent fibers were observed throughout the neuropil. Such terminals contained round, clear vesicles with an occasional large, dense-cored vesicle, and made axodendritic and axosomatic synaptic contacts.     

Reorganization of corticorubral synapses following cross-innervation of flexor and extensor nerves of adult cat: a quantitative electron microscopic study

A quantitative electron microscopic study of corticorubral synapses was performed in the red nucleus (RN) of adult cats to determine the morphological correlates for the changes in time course of corticorubral excitatory post-synaptic potentials, which occur following cross-innervation of forelimb extensor and flexor nerves. Corticorubral synaptic endings were identified by anterograde degeneration after lesions of the ipsilateral sensorimotor cortex. Rubrospinal neurons innervating upper spinal segments were electrophysiologically identified and filled with horseradish peroxidase (HRP). These cells were mainly situated in the dorsomedial part of RN. Electron micrographs of the degenerating corticorubral synaptic endings were taken in the region surrounding HRP-filled neurons and the diameter of the dendrites contacted by such terminals was measured.In the cross-innervated animals many degenerating terminals were found to synapse on dendrites with large diameter and the somata of neurons in RN. This is in contrast to the previous observations in normal cats, in which very few corticorubral synapses were found to synapse on proximal dendrites and somata of RN neurons. The diameter of HRP-filled neurons in cats which were cross-innervated was slightly smaller than those observed in normal animals. These results indicate that new corticorubral synapses were formed on proximal dendrites and somata of RN neurons as a consequence of cross-innervation.     

Fine structure of rat locus coeruleus

Locus coeruleus of the rat was studied in material prepared by aldehyde-osmium fixation. Cell bodies of locus coeruleus neurons possess large nuclei with a prominent nucleolus, a homogeneous karyoplasm of moderate density, and occasional indentations of the nuclear membrane. The cytoplasm is rich in organelles, including an extensive network of endoplasmic reticulum which forms well organized Nissl bodies. The highly developed Golgi apparatus surrounds the nucleus and extends into large dendritic trunks. In coronal section, cell bodies appear elongated along an approximate dorso-ventral axis, and most dendrites as well as axons appear in cross-section. In parasagittal sections the cells are very elongate, with dendrites and axons in the neuropil mostly cut longitudinally. Thus, locus coeruleus neurons possess disc-shaped dendritic fields parallel to the anterior-posterior axis of the brainstem, with predominantly longitudinal axo-dendritic synaptic configurations. Presynaptic profiles in locus coeruleus neuropil were classified according to the characteristics of their vesicle populations and other features. The most frequently encountered synaptic ending was characterized by small, round, densely packed synaptic vesicles, and comprised approximately 41% of the total sample of 775 synapses. Another group having large, rounded synaptic vesicles, which could be traced in a number of instances to large myelinated axons, accounted for 20% of the sample. Synaptic endings having large, flattened vesicles were also numerous, comprising 23% of the total. Another category of presynaptic endings was identified as those possessing numerous, small, flattened vesicles and comprising about 11% of the sample. Presynaptic endings having many vesicles of mixed sizes accounted for 2% of the total, and another group of the same proportion having small, rounded synaptic vesicles but also an unusually large number of larger, dense-cored vesicles was also present. Two other categories of synaptic endings were encountered, each comprising less than 1% of the total. One of these was derived from small, unmyelinated axons and contained clusters of pleomorphic synaptic vesicles. The other consisted of dendro-dendritic synapses between locus coeruleus neurons and also displayed small clusters of pleomorphic synaptic vesicles near the zone of synaptic apposition. Quantitative analysis revealed that most afferents to the nucleus synapse onto dendrites ranging between 0.5 and 2.5 micrometers in diameter and onto spine-like appendages derived from somata and dendrites. There were no significant differences between different categories of afferent terminals and their spatial distribution onto various postsynaptic targets of locus coeruleus neurons.     

Axonal endings terminating on dendrites of identified large trigeminospinal projection neurons in rat trigeminal nucleus oralis

The retrograde horseradish peroxidase technique was used to: (1) identify and assess the overall morphology of large neurons in the ventrolateral portion (VL) of rat trigeminal nucleus oralis projecting to cervical, thoracic and lumbosacral levels of the spinal cord; and (2) characterize the synaptic endings terminating on their dendrites. The morphology of large VL neurons projecting to all spinal levels is similar. They have 25–50 μm pyramidal-shaped somata which emit 3–6 primary dendrites. These primary dendrites give rise to spherical to elliptical-shaped dendritic arbors measuring up to 700 μm in diameter. Labeled axons enter either a deep axon bundle or the medial portion of the spinal V tract. Dendrites of labeled neurons are contacted by axonal endings of 3 types. The most numerous endings are filled with clear, spherical synaptic vesicles and usually form a single asymmetrical contacts along the entire length of dendritic shafts. Synapsing less frequently on dendritic shafts are endings containing pleomorphic synaptic vesicles and forming single symmetrical synaptic contacts. The least frequently encountered synaptic terminal contains flattened synaptic vesicles and makes a single symmetrical synaptic contact with a dendritic shaft.     

Morphology and synaptic connections of myelinated primary axons in the ventrolateral region of rat trigeminal nucleus oralis

Neurons in the ventrolateral (VL) subdivision of rat trigeminal nucleus oralis (Vo) have most of their dendritic arbors confined within this region. This study examines the morphology and synaptic connections of a population of myelinated primary trigeminal axons that arborize within VL and are in a position to provide input directly to VL neurons. Primary axons were visualized for light and electron microscopic analysis by injecting 30% horseradish peroxidase (HRP) in 2% dimethylsulfoxide (DMSO) into the sensory root of the trigeminal nerve and allowing 24-36 hours for the anterograde transport of HRP into the terminal axonal arbors. This population is characterized by its cone-shaped terminal arbors, which generate many axonal endings (2-8 micron in diameter) along unmyelinated terminal strands. These arbors arise from collaterals emanating from thinly myelinated (2-5 micron in diameter) parent branches descending in the spinal V tract, which, on the basis of their size, are considered to be small myelinated (A sigma) primary trigeminal axons. HRP-labeled P endings belonging to this population of primary axons are scalloped, filled with spherical to ovoid (40-70 nm in diameter) synaptic vesicles, and lie centrally in glomeruli where they make asymmetrical axodendritic synapses on dendritic shafts and spine heads. It is at these synapses that this population of primary trigeminal axons is probably transferring its input directly to the dendritic arbors of VL neurons. The dendritic shafts and spine heads also receive symmetrical to intermediate axodendritic synapses from endings containing flattened (70 X 29 nm) synaptic vesicles. These terminals also establish axo-axonic synapses on the P ending. Other synaptic components found less often in the glomeruli include small terminals containing oval (14-23 nm) synaptic vesicles that establish symmetrical to intermediate synapses on the P ending, boutons containing pleomorphic (35-80 nm) synaptic vesicles that form symmetrical to intermediate synapses on the P ending as well as on dendritic shafts, and small peripheral endings containing round (20-40 nm) synaptic vesicles that establish asymmetrical synapses on dendritic shafts.     

A note on the synapses between vesicle containing profiles in the pontine nuclei of the cat

In the cat synapses between vesicle containing profiles were observed in ventral and dorsolateral pontine nuclei. The presynaptic elements consisted of two types of axon terminals: axon terminals characterized by a population of small (38-40 nm) round synaptic vesicles (SSV) and axon terminals containing pleomorphic synaptic vesicles (PSV). The postsynaptic pale elements (PP) had pleomorphic vesicles and some features attributed to dendrites. In the dorsolateral pontine nucleus most of PP profiles took part in serial synapses, usually as an intermediate component, they were rarely observed in triads. On the basis of their electron microscopical appearance and synaptic relations they might be considered to represent a dendritic part of putative interneurons.     

Synaptic organization of globular bushy cells in the ventral cochlear nucleus of the cat: a quantitative study.

The synaptic organization of globular bushy cells of the anteroventral cochlear nucleus was quantitatively analyzed in order to understand better their functional attributes. A method was devised to estimate the concentrations and relative proportions of synapses on the entire postsynaptic surface of Golgi-impregnated neurons, by sampling with limited series of sections for electron microscopy. This provided a characteristic synaptic profile which was homogeneous for the population measured. The total concentration of synaptic endings decreases with distance from the soma. The cochlear, presumably glutamatergic and excitatory, endings with large spherical vesicles (LS) account for most of this decrease. Of the noncochlear inputs, the putative glycinergic endings with flattened vesicles (FL) decrease slightly, and the presumed GABAergic terminals with pleomorphic vesicles (PL) maintain a relatively constant concentration, while endings with small spherical vesicles (SS) increase on the distal dendrites. LS endings have the largest proportion of synapses near the soma, while FL synapses maintain a constant proportion in all cell regions, and PL and SS proportions increase on higher-order dendrites. Excitatory and inhibitory synapses have significant inputs to the axon hillock and initial segment, as well as to the distal dendrites, where dual synapses may provide a way to sample the activity of surrounding neurons. These features must be considered in explanations of physiological properties, such as the synaptic security, level of spontaneous activity, and well-timed, rapid onset responses, as well as their potential for normalizing and synchronizing an important inhibitory pathway involved in binaural signal processing. Synaptic profile analysis should be useful for experimental studies and for developing realistic computational models.     

Monosynaptic cortical input and local axon collaterals of identified striatonigral neurons. A light and electron microscopic study using the golgi-peroxidase transport-degeneration procedure

Following the injection of horseradish peroxidase into the ipsilaeral substantia nigra, 36 retrogradely labelled neurons in the striatum were characterized (in three rats) by Golgi staining and gold toning: each neuron was of the medium-size, densely spinous type. Prior to the injection of horseradish peroxidase, two of the rats had had lesions placed in the ipsilateral motor cortex, the third rat had had a lesion placed in the ipsilateral frontal and prefrontal cortex. In the electron microscope, degenerating boutons of cortical neurons were found in asymmetrical synaptic contact with the spines of proximal and distal dendrites of all six of the identified striatonigral neurons that were studied. Some of the degenerating boutons were small (diameter 0.1–0.3 μ), while others were larger (1–2 μ). An individual dendrite of a striatonigral neuron was in synaptic contact with very few degenerating boutons Local axon collaterals im the striatum could be traced from two of the identified striatonigral neurons that received degenerating cortical boutons. These were studied in the electron microscope; their boutons formed symmetrical synapses with spines or dendritic shafts of other striatal neurons. The synaptic boutons contained large, clear, round and pleomorphic vesicles. The postsynaptic targets of these boutons morphologically resemble the dendrites of medium-size spiny neurons It is concluded that afferents from the cortex make monosynaptic contact with the dendritic spines of medium-size spiny striatonigral neurons and that such neurons have local axon collaterals in the striatum that form synapses with other spiny neurons.     

A light and electron microscope study of the basal optic system in the reptile Vipera aspis

The basal optic system of the reptile Vipera aspis was investigated under both light and electron microscopy. The basal optic root (BOR), mainly composed of large diameter myelinated fibers (congruent to 2 micrometers) terminates in he nucleus of the basal optic root (nBOR). The different histological techniques employed disclose a neuronal population distributed in the following three categories: 1) small neurons, of low proportion (21%), have cytological features which allow their classification as Golgi type II neurons, 2) medium-sized neurons (35%) and 3) large multipolar neurons (44%). Both of the latter types of neurons are contacted by optic terminals. Neuroglial elements, astrocytes, oligodendrocytes, and microgliacytes were observed either in an intermediate fascicular or perineuronal satellite position. The neuropil of nBOR is made up of both axonal and dendritic profiles. The dendrites which contain synaptic vesicles (DCSVs) are not numerous (15% of the total population of profiles containing synaptic vesicles, PCSVs) and have the peculiarity of participating in serial and triadic arrangements within glomerulus-like structures where they are postsynaptic to optic terminals. Six types of axon terminals have been identified. Those containing a more or less spheroidal synaptic vesicle population are subdivided in two classes: S 1, the optic terminals being the most numerous (48,5% of the total PCSVs) and S 2 (19% of the total PCSVs). On the basis of density of flattened synaptic vesicles, F type terminals are classified either as F 1 (9%) or F 2 (8%), the first being more densely packed with synaptic vesicles. A very low proportion of terminals (0,5%) comprises a mixed population of large granular vesicles (G) associated with rounded or ellipsoidal synaptic vesicles. Occasionally, gap junctions are observed between an axon terminal and a dendritic profile. The present results show a similarity of synaptic circuitry when compared to bird and mammal nBOR.     

Projections from auditory cortex to the cochlear nucleus in rats: Synapses on granule cell dendrites

Previous work has demonstrated that layer V pyramidal cells of primary auditory cortex project directly to the cochlear nucleus. The postsynaptic targets of these centrifugal projections, however, are not known. For the present study, biotinylated dextran amine, an anterograde tracer, was injected into the auditory cortex of rats, and labeled terminals were examined with light and electron microscopy. Labeled corticobulbar axons and terminals in the cochlear nucleus are found almost exclusively in the granule cell domain, and the terminals appear as boutons (1–2 μm in diameter) or as small mossy fiber endings (2–5 μm in diameter). These cortical endings contain round synaptic vesicles and form asymmetric synapses on hairy dendritic profiles, from which thin (0.1 μm in diameter), nonsynaptic “hairs” protrude deep into the labeled endings. These postsynaptic dendrites, which are typical of granule cells, surround and receive synapses from large, unlabeled mossy fiber endings containing round synaptic vesicles and are also postsynaptic to unlabeled axon terminals containing pleomorphic synaptic vesicles. No labeled fibers were observed synapsing on profiles that did not fit the characteristics of granule cell dendrites. We describe a circuit in the auditory system by which ascending information in the cochlear nucleus can be modified directly by descending cortical influences. © 1996 Wiley-Liss, Inc.     

The distribution of dorsal root axons in laminae I, II and III of the macaque spinal cord: a quantitative electron microscope study.

This study examines the projection of dorsal root fibers to the upper dorsal horn of the monkey lumbar spinal cord utilizing degeneration and autoradiographic methods. The animals survived dorsal rhizotomy for periods varying from 18 hours to 28 days. Electron microscopy reveals the earliest degeneration to be neurofilamentous alteration of large synaptic profiles in lamina III and the inner zone of the substantia gelatinosa (IIi). This degeneration begins 18 hours after rhizotomy, reaches a peak at three days postoperatively and disappears by the end of the first week. Degenerating myelinated axons in the spinal gray matter, dorsal column white matter and Lissauer's tract first appear three days postoperatively. The second tye of degeneration of synapses occurs in lamina I and outer gelatinosa (IIo) and consists of electron lucent alteration of moderate size synapses, especially those having large granular vesicles (LGVs) and some neurofilamentous and dense degeneration. This synaptic degeneration in lamina I begins two days following rhizotomy and reaches a peak between five to seven days, declines markedly by ten days and is absent at four weeks survival. The third type of degeneration occurs in the substantia gelatinosa (laminae IIo and IIi) initially as an enlargement of synaptic vesicles at two days and then progresses to large numbers of electron dense small synapses, the peak of degeneration occurring at seven days and persisting as long as four weeks postoperatively. Some of the dense synapses can be seen to arise from small, nonmyelinated axons. These axons are first seen to be degenerating in the gelatinosal and marginal layers at four days survival and the first definite degeneration of nonmyelinated axons in Lissauer's tract is at seven days postoperatively. It is concluded that the largest axons projecting to this region of the dorsal horn degenerate most rapidly and that these axons are distributed to laminae III and IIi. Axons of intermediate diameter degenerate next and are distributed principally to laminae I and IIo. Fine diameter axons, probably nonmyelinated, degenerate more slowly and terminate principally in the substantia gelatinosa (IIi and IIo). There is some overlap in these projection domains, in that the principal projection to lamina III extends into the lower part of the gelatinosa and the projection to the marginal layer overlaps the outer gelatinosa. The axon terminals in gelatinosa of C fibers are sometimes postsynaptic in axoaxonal synapses as are several of the axon terminals of larger A fibers in lamina III. Most of the synapses of primary afferent origin in lamina I are not involved in axoaxonal synapses. It is likely that the terminations of many primary afferent fibers in laminae II and III are subject to presynaptic inhibition and those in lamina I are not. Some of the primary afferents in all three laminae synapse upon presynaptic dendrites and thus may influence transmitter release from these profiles. The LGV profiles are distributed in a manner similar to the distribution of substance P and it is suggested that the degenerating LGV profiles may contain substance P. Most of the LGV profiles and many of the round vesicle profiles do not appear to be derived from dorsal root, but most of the central synaptic profiles are of primary afferent origin. In no case was there evidence that flat vesicle synapses were derived from primary afferents. Following dorsal root ganglia injections with H³ leucine, light microscopic autoradiography at short postoperative survival times demonstrated heavy grain distribution over marginal and gelatinosal layers with somewhat less numbers of grains over lamina III. There were also many grains over the dorsal column white matter and Lissauer's tract. Electron microscopic autoradiography revealed that the majority of labeled structures seen with fast axonal transport in the upper dorsal horn are not synapses but are myelinated and nonmyelinated axons. Labeled synapses were the same types as those undergoing degeneration following rhizotomy: round vesicle profiles, central synaptic profiles and LGV profiles. Each of the labeled types was distributed throughout the upper laminae, with the exception of LGV profiles which are uncommon in layers deep to the outer zone of the gelatinosa. It is concluded that fast axon transport autoradiography is not a selective label for synapses in the cord and light microscopic autoradiography does not provide direct estimates of synaptic densities in the dorsal horn.     

Dendroaxonic synapses in the substantia gelatinosa glomeruli of the spinal trigeminal nucleus of the cat

The glomeruli in the substantia gelatinosa layer of the spinal trigeminal nucleus of the cat contain three kinds of dendritic processes. One of these, the type 2 dendrite, contains large synaptic vesicles in its spine heads and in its shaft. The type 2 dendrite receives axodendritic synapses from primary trigeminal afferent (C) axons and an occasional axodendritic synapse from small axonal (P) endings with small synaptic vesicles. The type 2 dendrites in turn form dendroaxonic synapses on the C endings. The dendroaxonic synapse and the axodendritic synapse of the C ending typically occur in reciprocal pairs. The axodendritic synapse usually lies in the depths of scalloped depressions in the surface of the C ending while the dendroaxonic synapse is found on the rim of the depression. Type 1 spines, i.e., dendritic spines receiving axodendritic synapses from the primary ending and lacking synaptic vesicles, also receive dendrodendritic synapses from type 2 dendrites. The types 2 dendrite with its large, rounded synaptic vesicles is considered to be excitatory at its dendroaxonic and dendrodendritic synapses. The type 2 dendrites course from glomerulus to glomerulus receiving their excitatory input through the axodendritic synapses of C axons. A type 2 dendrite, in response to C axon excitation would activate type 1 spines directly through their dendrodendritic synapses (C→2→1) and indirectly by increasing transmitter release at the axodendritic synapses of the C axonal endings through their dendroaxonic synapses (2→C→1). The type 2 dendrites could serve two functions. First, they may prolong transmitter release from the axodendritic synapses of C axonal endings beyond the time of arrival of incoming action potentials because of the reciprocal pairing of dendroaxonic and axodendritic synapses (C?2). Second, they may extend the spatial range of the excitatory output of active primary afferent axons to type 1 spines of glomeruli whose primary afferent axons may be inactive (C→2→1).     

Observation of the ultrastructure and synaptic relationships of angiotensin II-like immunoreactive neurons in the rat area postrema

The ultrastructure and synaptic relationships of the angiotensin II-containing neurons in the area postrema of the rat were studied by immunocytochemistry using the avidin-biotin-complex-DAB method, and also using silver-gold intensification following the DAB reaction. At the light microscopic level, the angiotensin II-like immunoreactive neurons were observed within the area postrema, especially in the upper region. At the electron microscopic level, the angiotensin II-like immunoreactive cell bodies were observed as having a round, unindented nucleus. The nuclei of these neurons were not immunostained. The angiotensin II-like immunoreactive axon terminals often contained a few dense core vesicles in addition to many small clear synaptic vesicles. Numerous axon terminals were found to make synapses on immunonegative dendrites; they were also found to make synapses on angiotensin II-like immunoreactive dendrites. Many angiotensin II-like immunoreactive dendrites received synapses from immunonegative axon terminals. Although angiotensin II-like immunoreactive cell bodies were sometimes postsynaptic to immunoreactive axon terminals, they did not receive synapses from immunonegative axon terminals. These results provide solid morphological evidence of AP endogenous angiotensin II and confirm that in spite of circulating angiotensin II, the local neurons in the AP may also play an important role in angiotensin II-induced cardiovascular regulation.     

Synaptic plasticity in the medial superior olive of hearing, deaf, and cochlear-implanted cats

The medial superior olive (MSO) is a key auditory brainstem structure that receives binaural inputs and is implicated in processing interaural time disparities used for sound localization. The deaf white cat, a proven model of congenital deafness, was used to examine how deafness and cochlear implantation affected the synaptic organization at this binaural center in the ascending auditory pathway. The patterns of axosomatic and axodendritic organization were determined for principal neurons from the MSO of hearing, deaf, and deaf cats with cochlear implants. The nature of the synapses was evaluated through electron microscopy, ultrastructure analysis of the synaptic vesicles, and immunohistochemistry. The results show that the proportion of inhibitory axosomatic terminals was significantly smaller in deaf animals when compared with hearing animals. However, after a period of electrical stimulation via cochlear implants the proportion of inhibitory inputs resembled that of hearing animals. Additionally, the excitatory axodendritic boutons of hearing cats were found to be significantly larger than those of deaf cats. Boutons of stimulated cats were significantly larger than the boutons in deaf cats, although not as large as in the hearing cats, indicating a partial recovery of excitatory inputs to MSO dendrites after stimulation. These results exemplify dynamic plasticity in the auditory brainstem and reveal that electrical stimulation through cochlear implants has a restorative effect on synaptic organization in the MSO.     

Cell types and synaptic organization of the medullary electromotor nucleus in a constant frequency weakly electric fish,Sternarchus albifrons

The medullary electromotor nucleus (EMN) of Sternarchus albifrons was studied at the light and electron microscopic levels. The EMN consists of a dense meshwork of myelinated axons and glial elements with interposed large neurons; it is provided with an abundant supply of capillaries. Two types of essentially adendritic nerve cells were distinguished on the basis of size: giant neurons (approx. 70 μm in diameter) and large neurons (approx. 30 μm in diameter). Their population ratio is 1:4. Only giant cells are labelled following the injection of retrograde tracer into the spinal cord; they are therefore identified with the so-called “relay cells” of other gymnotids. Tracer experiments further suggest that the descending axons of these relay cells give off collateral branches throughout the elongated spinal electromotor nucleus. In contrast, the large cells remain unlabelled and therefore lack spinal projections; they most likely correspond to “pacemaker cells”. The perikaryal surface, including axon hillock and proximal part of initial segment of both types of EMN cells, is contacted by clusters of synaptic terminals and astrocytic processes. Two main varieties of synaptic terminals occur: (1) large endings and (2) ordinary end feet with standard size (S-type) and variable size (Sv-type) clear, spherical vesicles. The junction between large endings and EMN cells is characterized by the combination of gap junctions and surrounding intermediate junctions whose freeze-fracture characteristics were morphometrically analyzed. The large endings were formed by nodes of Ranvier as well as by fiber terminations, and synchronization within the EMN may be achieved by presynaptic fibers. Some of the contacts occur directly on the initial segment, which could allow activity to bypass the soma. It is concluded that the electromotor system of Sternarchus is comprised of a rapid conduction pathway where medullary pacemaker and relay cells as well as spinal electromotor neurons are coupled by synapses with gap junctions. In contrast to the spinal electromotor neurons, the medullary EMN cells receive synapses with morphological characteristics of chemical transmission, and the S-type and Sv-type terminals may possibly correspond to Gray's Type I and Type II synapses, respectively. These synapses may be involved in modulation of the electric organ discharge frequency.     

The synaptic organization of the motor nucleus of the trigeminal nerve in the opossum

The motor nucleus of the opossum trigeminal nerve consists of a main body and a small dorsomedial cell cluster. The cell bodies form a unimodal population with areas that range from 150–2700 μm². Golgi impregnations reveal that each neuron has three to six primary dendrites which radiate in all planes from the cell body. Within 300 μm from the soma, the primary dendrites divide into secondary branches and these, in turn, bifurcate into thinner distal dendrites. The overall diameter of the dendritic tree often extends as much as 1 mm, with a rare branch leaving the confines of the nucleus to enter the neighboring reticular formation. Somatic and dendritic spines are often present and are either sessile or complex appendage forms. The perikarya and initial dendritic trunks of trigeminal neurons are contacted by four types of presynaptic terminals which cover more than 40% of the membrane. Most endings are 1–3 μm long and contain either spherical (S) or pleomorphic (P) synaptic vesicles. Another, less common, type of bouton is marked by large dense-core (DC) vesicles. Approximately 8% of the terminals on trigeminal cell bodies are large (2–5 μm) with spherical synaptic vesicles and are always associated with a subsynaptic cistern (C-boutons). These terminals very often interdigitate with adjacent synaptic endings. S-, P-, and C-boutons synapse on the dendritic tree of trigeminal neurons in the following characteristic pattern: proximal dendrites (greater than 5 μm in diameter) are contacted by all three types of terminals; intermediate-sized dendrites (between 2.5 and 5.0 μm in diameter) are most often contacted by S-boutons although P-boutons are also present; and small, distal dendrites (less than 2.5 μm in diameter) are almost always contacted by S- boutons. Both S- and P-boutons contact spines. In order to determine the ultrastructural identity of some of the major afferent systems to the trigeminal motor nucleus, adult opossums were subjected to two different types of lesions. Three and 5 days subsequent to lesions which destroyed most of the trigeminal mesencephalic nucleus, degenerating terminals containing spherical vesicles were found. These endings were S-boutons on more distal parts of the dendritic tree while on the cell body and proximal dendrites they were C-boutons. Seven days after a mesencephalic lesion, expanded glial processes approximated the trigeminal cell membrane. Two days subsequent to lesions which transected commissural fibers from the contralateral trigeminal complex, degenerating S- and P-boutons were found in contact with intermediate and distal parts of the trigeminal dendritic tree.     

The fine structure of the rat subthalamic nucleus: an electron microscopic study

The normal ultrastructure of the rat subthalamic nucleus (STH) was studied. The STH consisted of tightly packed neurons distributed within a neuropil filled with large numbers of blood vessels and thinly myelinated fibers. The somata of STH neurons (diameters, D, between 10 and 25 micron) contained abundant organelles but had only a small amount of both smooth and rough endoplasmic reticulum. The nuclei had deeply invaginated nuclear envelopes and pale nucleoplasm with little heterochromatin. STH neurons often were tightly apposed without any intervening glial membranes. Similar appositions were also found between somata and dendrites, dendrites and dendrites, and dendrites and initial axon segments. Although puncta adhaerentia were often observed, no gap junctions were found on any of these membrane appositions. In the neuropil, the dendrites were mostly smooth and thin (D between 0.5 and 1 micron) with an occasional stubby spine or thin dendritic appendage. At least two types of axon terminals were identified. Type 1 terminals (D up to 1 micron) contained medium-sized round vesicles (D about 45 nm) and formed asymmetrical synapses. Type 2 terminals were often large (D up to 5 micron) and contained both round and slightly flattened vesicles (D up to 50 nm). The type 2 terminals frequently formed adherens junctions with their postsynaptic targets in addition to forming relatively symmetrical synaptic junctions. The remaining axon terminals included a small number of terminals with various morphological characteristics and possibly some tangentially sectioned type 1 and type 2 terminals. Therefore they have not been classified as individual types in this study. A quantitative analysis indicated that the type 1 terminals formed synapses mainly with thin dendrites whereas the type 2 terminals formed synapses mainly with somata and larger dendrites.     

Early postnatal development of entopeduncular neurons and their neostriatal connections

The early postnatal development of dendrites and axodendritic connectivity in the entopeduncular nucleus of kittens was studied by light and electron microscopy. We focused on the fine structure of neuropil and the organization of synaptic elements at several ages during the first weeks of life. We were able to define, in newborn to 1-week-old kittens, several of the distinct types of nerve endings seen previously by us in adult animals. They were found singly or in small clusters widely spaced along surfaces of dendrites and cell bodies. Most endings were small, contained 45 to 50-nm synaptic vesicles, and formed symmetrical synaptic junctions. Fewer large endings, filled with 30- to 35-nm vesicles, formed asymmetrical synapses. By the end of the second week, most dendrites and much of the cell body surfaces were ensheathed by these endings. Astroglial elements apposed nonsynaptic surfaces and enveloped arrays of axodendritic synapses. We used Fink and Heimer staining of degenerating axons to show that much of this early connectivity originated in the neostriatum. These morphologic studies support physiologic data that striopallidal pathways are functional at birth and suggest that many of the age-related changes in response parameters reflect a quantitative increase in axodendritic connectivity. To assess this notion, we initiated a computer-assisted study of Golgi-impregnated neurons and measured dendritic growth during this period. Preliminary data suggested dendritic fields are extensive in 3-day-old kittens (mean total dendritic length of 2800 μm) and individual dendrites radiate for long distances and branch sparsely (mean total branch length of 700 μm). By 18 days of age, these parameters had increased by about 40% to 4800 and 1200 μm, respectively.