Ultrastructural studies of retinal, visual cortical (area 17), and parabigeminal terminals within the superior colliculus of Galago crassicaudatus.

The morphology and synaptic relationships of anterogradely labeled retinal, visual cortical (area 17), and parabigeminal terminals have been analyzed within the superficial gray (stratum griseum superficiale) of Galago crassicaudatus. Our data regarding the retinocollicular projection reveal two populations of terminals based upon size. The population of smaller terminals are found in clusters, while the larger occur in isolation. Both populations of retinocollicular terminals form synapses primarily with dendritic spines, but synapses upon pale vesicle filled (PVF) profiles and dendritic shafts also occur. Corticotectal terminals contain round vesicles and make asymmetrical synapses, primarily onto dendritic spines; few form synapses with PVF profiles. Our findings suggest the possibility that there are two populations of corticotectal terminals based upon differences in size and morphology. Parabigeminotectal profiles contain densely packed round vesicles and make asymmetrical synapses. These terminals, which are exclusively cholinergic in Galago, are presynaptic to dendrites of various sizes. Convergence of retinal and cortical terminals has been observed. This convergence occurs on distinctly separate regions of the postsynaptic membrane. In contrast, convergence of retinal and parabigeminal terminals occurs on the same region of the postsynaptic cell(s).     

Ultrastuctural studies of the primate lateral geniculate nucleus: Morphology and spatial relationships of axon terminals arising from the retina,visual cortex (area 17), superior colliculus,parabigminal nucleus,and pretectum of Galago crassicaudatus

The electron microscopic autoradiographic tracing method has been used to examine the morphology and postsynaptic relationships of five projections (retina, cortical area 17, superior colliculus (tectal), parabigeminal nucleus, and pretectum) to the dorsal lateral geniculate nucleus of the greater bush baby galago crassicaudatus. Retinal terminals have been examined in the contralaterally innervated layer of each of the three matched pairs [parvi-(X-cell), magno- (Y--cell), and koniocellular (small, W-cell)] of geniculate layers. These terminals are large and contain pale mitochondria and round vesicles (RLPs). RLPs are presynaptic to juxtasomatic regions of parvi-and magnocellular neurons. In contrast, RLPs innervate more distal regions of konicellular neurons. Labeled cortical, tectal, and parabigeminal terminals are relatively small and contain round vesicles na dark mitochondria. Cortical terminals in each of the three representative layers are presynaptic to small diameter dendrites. No convergence of cortical and retinal terminals has been seen in any layer. Labeled tectal and parabigminal terminals are found primarily in the koniocellular layers, but the latter are also seen in all other layers. Tectal and parabigeminal terminals have been observed converging with retinal terminals on dendrites of some koniocellular neurons. Labeled pretectogeniculate terminals contain densely packed pleomorphic vesicles, dark mitochondria, and a dark cytoplasmic matric. These terminals, which are present in each of the representative layers, are presynaptic to conventional dendrites and profiles containing loosely despersed pleomorphic vesicles and a pale cytoplasmic matrix. © 1994 Wiley-Liss, Inc.     

The pregeniculate nucleus of the monkey (Macaca multatta). II. A study at the electron microscopic level

An electron microscope study of the ultrastructure of the pregeniculate nucleus of the monkey (Macaca mulatta) shows it to contain three neuronal types and four varieties of presynaptic terminals. Type I neurons are found only in the inner lamina, have small rounded profiles with few axosomatic synapses; the cytoplasm is poor in organelles and the nucleus is deeplly infolded. Type II neurons were observed infrequently and only in the outer lamina; they have large oblong profiles, exhibiting many axosomatic contacts, and containing abundant cytoplasm rich in organelles, particularly arrays of granular and agranular endoplasmic reticulum. Type III neurons were the most frequently seen and are found in both laminae; their profiles are elliptical and exhibit only a few axosomatic synapses. The cytoplasm surrounding the infolded nucleus is moderately rich in organelles with agranular endoplasmic reticulum predominating. These three neuronal types were found to correlate well with types of neurons found in material stained with cresylecht violet or impregnated by the Golgi method. Four presynaptic terminal types were discerned: a small cup-shaped profile containing spheroid vesicles and found predominantly in the outer lamina, a larger elliptical profile containing flattened spheroid vesicles, a large ramifying profile also containing round vesicles and largely restricted to the inner lamina, and a rounded profile containing larger flattened vesicles. Three days after eye enucleation, darkened degenerating profiles containing vesicles and forming asymmetric synapses were observed in the inner lamina, while the third terminal type described above could no longer be seen. The first three types are usually associated with asymmetric synaptic densities, whereas in the case of the last type, the postsynaptic synapse is symmetrical. The profile of this last terminal type was also sometimes observed to be both postsynaptic as well as presynaptic to other profiles; however, it was never observed to contain ribosomes. Such a pre- and postsynaptic terminal always forms part of the in series or triadic configuration of terminals occasionally observed in the pregeniculate nucleus.U     

Postembedding immunocytochemistry demonstrates directly that both retinal and cortical terminals in the cat superior colliculus are glutamate immunoreactive

Although the excitatory neurotransmitter glutamate is known to be present in the cat superior colliculus (SC), the types of synapses that contain glutamate have not been examined. We, therefore, studied the ultrastructure of synaptic profiles labeled by a glutamate antibody by using electron microscopic postembedding immunocytochemistry. In addition, unilateral aspiration lesions of areas 17–18 were made at 5–28 days before death in order to determine whether degenerating terminals from visual cortex were glutamate immunoreactive (Glu-ir). Three types of axon terminal were glu-ir: 1) those containing large, round synaptic vesicles and pale mitochondria, characteristic of retinal terminals (RT profiles); 2) those containing small, round synaptic vesicles and dark mitochondria (RSD profiles); and 3) those containing large, round synaptic vesicles and dark mitochondria (RLD profiles). Measures of mean gold particle density revealed that RT, RSD, and RLD profiles had similar average grain densities (11.3–12.7 particles/unit area). Other labeled profile types included cell bodies, large-calibre dendrites, and myelinated axons. Axon terminals containing flattened synaptic vesicles and vesicle-containing presynaptic dendrites, both of which contain γ-aminobutyric acid (GABA), had many fewer gold particles (3.6 and 4.8 mean particles/unit area, respectively). Following unilateral removal of visual cortex, normal RSD terminals were observed infrequently in the SC ipsilateral to the lesion. Synaptic terminals in the initial stages of degeneration were heavily labeled by the glutamate antibody, as were axon terminals and myelinated axons undergoing hypertrophied or neurofilamentous degeneration. These results show that both major sensory afferents to the superficial layers of cat SC contain glutamate—RT terminals from the retina and RSD terminals from visual cortex. The origin of RLD terminals is unknown. © 1996 Wiley-Liss, Inc.     

Observations on the synaptology of intracellularly injected spinothalamic tract neurons in the cat

Single spinothalamic tract cells in the deep lumbar group have been injected with horseradish peroxidase and their dendritic trees examined on the electron microscope. Large dendrites are surrounded by rosettes of from 5 to 12 synaptic terminals. Most terminals contain round vesicles but some terminals contain flattened clear vesicles and others contain membranous tubes or cisterns. Large (mean diameter 100 nm) round, dense-core vesicles are found in both terminals containing clear round vesicles and terminals containing flattened vesicles. As yet none of those terminals on STT cell dendrites have been found participating in axo-axonic synapses, suggesting that presynaptic inhibition or facilitation plays no role in modulating the responses of these cells to presynaptic activity.     

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.     

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.     

Fine structure of the lateral mammillary projection to the dorsal tegmental nucleus of Gudden in the rat.

The synaptic organization of projections from the lateral mammillary neurons within the dorsal tegmental nucleus of Gudden is studied in the rat with the aid of anterograde transport of horseradish peroxidase conjugated with wheat germ agglutinin (WGA-HRP) and visualized with tetramethylbenzidine. The dorsal tegmental nucleus consists of the pars ventralis (TDV) and the pars dorsalis (TDD). The normal neuropil of the dorsal tegmental nucleus contains three classes of axodendritic terminals, that is, terminals containing round, flat, and pleomorphic vesicles. They make up 44%, 5%, and 51%, respectively, of all axodendritic terminals in the TDV, and 62%, 1%, and 37% in the TDD. Injection of WGA-HRP into the lateral mammillary nucleus permits ultrastructural recognition of many anterograde labeled terminals within both the TDV and TDD. In the TDV, 81% of the labeled terminals contain round synaptic vesicles and make asymmetric synaptic contacts. A few of the labeled terminals contain pleomorphic vesicles and make symmetric synaptic contacts. More than 50% of the labeled terminals contact intermediate dendrites (1-2 microns diameter). In the TDD, almost all labeled terminals are small, contain round vesicles, and make asymmetric synaptic contacts. These terminals mainly contact intermediate as well as distal (less than 1 micron diameter) dendrites. There are only a few labeled terminals with pleomorphic vesicles and no terminals with flat vesicles. The termination pattern of the lateral mammillary neurons in the TDV is similar to that in the TDD. Anterograde labeled axon terminals often contact retrograde labeled dendrites in the TDV. No reciprocal connections are present in the TDD. These results suggest that the TDV and the TDD receive mainly excitatory and a few inhibitory inputs from the lateral mammillary nucleus. The TDV neurons also have direct reciprocal connections with the lateral mammillary neurons.     

Ultrastructure of the mammillotegmental projections to the ventral tegmental nucleus of Gudden in the rat.

This study examines the termination pattern of axons from the medial mammillary nucleus within the ventral tegmental nucleus of Gudden (TV) in rats by using anterograde transport of horseradish peroxidase conjugated with wheat germ agglutinin (WGA-HRP) and visualized with tetramethylbenzidine. The neuropil of TV contains three classes of axodendritic terminals, that is, terminals containing round, flat, and pleomorphic synaptic vesicles. These types make up 55.6%, 26.1%, and 18.3%, respectively, of all normal axodendritic terminals. Injection of WGA-HRP into the medial mammillary nucleus permits ultrastructural recognition of anterogradely labeled terminals within the TV. More than 80% of the labeled terminals contain round synaptic vesicles and form asymmetric synaptic contacts, whereas about 16% contain flat synaptic vesicles with symmetric synaptic contacts. There are a few labeled terminals with pleomorphic vesicles and only a few axosomatic terminals. Almost all labeled terminals are small, having diameters of less than 1.5 microns. Compared with the distributions of normal and labeled terminals with round vesicles, there is an increase of the percentage of labeled terminals with round vesicles on the intermediate dendrites (1-2 microns diameter) and a decrease on the distal dendrites (less than 1 micron diameter). Anterogradely labeled axon terminals often contact retrogradely labeled dendrites. These results suggest that the medial mammillary neurons send mainly excitatory as well as a few inhibitory inputs to the dendrites of TV and have direct reciprocal contacts with the TV neurons.     

Ultrastructure of synapses from the A-laminae of the lateral geniculate nucleus in layer IV of the cat striate cortex

The morphology of synapses in layer IV of the cat striate cortex was studied by electron microscope (EM) autoradiography of serial sections following injection of tritiated amino acids into the lateral geniculate nucleus. Of the terminals in the neuropil, 22% had 2 or more silver grains in 10 successive sections and were labeled at 8-80 times the background level. These terminals were considered to be specifically labeled and to be derived from the lateral geniculate. Two forms of geniculate synapse were observed. One had medium-size, round vesicles and a modest postsynaptic asymmetry (RA); the other had smaller, pleomorphic vesicles and hardly any postsynaptic opacity; that is, it appeared symmetrical (PS). The geniculate RA terminals were presynaptic to dendritic spines, fine processes, and cell bodies; the geniculate PS terminals were presynaptic to dendrites and cell bodies but not to spines. The possible sources of geniculate PS terminals are discussed.     

Electron microscopic analysis of the mesencephalic ventromedial tegmentum in the cat

We have studied the normal ultrastructure of the ventral mesencephalic tegmentum (VMT) in the cat, particularly the morphology and distribution of presynaptic terminals and the types of synaptic junctions. The following subnuclei of the region were examined: n. linearis rostralis (LR), n. paranigralis (PN), and n. interfascicularis (IF). The qualitative and quantitative data revealed significant ultrastructural differences between these subnuclei. Each subnucleus had a characteristic dendritic structure. In LR the dendrites were nonspinous and cylindrical and had presynaptic terminals randomly distributed over their surface. In PN we observed varicose dendrites with spines; the presynaptic terminals formed clusters on the narrow segments of the dendrites and around the spines. Dendrodendritic synapses were also observed in this nucleus. In IF, there was an internal division regarding dendritic structure: in the rostral part of the nucleus there were cylindrical dendrites while in the caudal part irregularly shaped dendrites bearing long spines were found. In IF and LR some of the cylindrical dendrites were seen to be in direct contact with the basal lamina of blood vessels. Four types of presynaptic terminals were distinguished by the morphology of their vesicles, and the proportion of each type in the total terminal population was determined. On this basis the compositions of the presynaptic terminal population in the three subnuclei were found to be very similar. Most terminals contained clear, round vesicles (62.6%), or both clear and dense-cored vesicles (35.1%). Few terminals were seen with dense-cored vesicles only (1.4%) or with pleomorphic vesicles (0.9%). The majority of synapses in the VMT were found to have symmetrical densities. LR had twice as many asymmetrical synapses as the other two subnuclei. Eighty percent of the terminals formed synapses with dendrites, although axosomatic and axoaxonic synapses were also seen. The density of the terminals was significantly different for each subnucleus: 191/1,000 micrometers 2 in IF, 120/1,000 micrometers 2 in PN, and 81/1,000 micrometers 2 in LR. These data indicate that while the subnuclei of the VMT receive morphologically similar afferents, each has a unique way of processing the information provided by them, through a different internal circuitry.     

Distribution of glycine-immunoreactive profiles in the monkey spinal cord: A light microscopic and ultrastructural study

The present study analyzed the relationships of glycine (GLY)-immunoreactive (-IR) and unlabeled profiles in the primate spinal cord. Light microscopic analysis demonstrated GLY-IR profiles in laminae III-VII, with fewer labeled profiles in laminae I, II, VIII, IX and X. The dorsal part of the lateral funiculus and the dorsal funiculus contained few labeled axons, in contrast to all other areas of white matter, which were heavily labeled. At the electron microscopic level, GLY-IR terminals in monkeys contained mainly round, with occasional pleomorphic, clear vesicles; however, F-type GLY-IR terminals synapsing on motoneurons contained pleomorphic vesicles. This seems to be an important species difference because vesicles in GLY-IR terminals in rat and cat are predominantly oval or elliptical. GLY-IR terminals synapsed on unlabeled as well as GLY-IR cell bodies and dendrites. This is morphological evidence that GLY may be both an inhibitor (GLY-IR terminals synapse on and presumably inhibit non-GLY cell bodies and dendrites) and a disinhibitor (GLY-IR terminals synapse on and presumably inhibit other GLY elements) of spinal activity. Also noteworthy was the conspicuous absence of axoaxonic interactions involving GLY-IR terminals. A related finding was that GLY profiles were always postsynaptic, never presynaptic, to glomerular primary afferent terminals. The functional implications would seem to be that primary afferent input can activate the spinal GLY system but that there is little GLY presynaptic control of afferent input in monkeys. This is in contrast to rats and cats, in which axoaxonic interactions involving GLY-IR terminals have been observed and where it is common to find GLY-IR terminals presynaptic to glomerular primary afferent terminals. © 1996 Wiley-Liss, Inc.     

Parvalbumin immunoreactivity in the thalamus of guinea pig: Light and electron microscopic correlation with gamma-aminobutyric acid immunoreactivity

The relationship of the calcium binding protein parvalbumin (PV) with gamma-aminobutyric acidergic (GABAergic) neurons differs within different thalamic nuclei and animal species. In this study, the distribution of PV and GABA throughout the thalamus of the guinea pig was investigated at the light microscopic level by using immunoperoxidase methods. Intense PV labelling was found in all the GABAergic neurons of the reticular nucleus and in scattered GABAergic neurons in the anteroventral nucleus, whereas GABAergic interneurons in the ventrobasal and lateral geniculate nuclei were not PV labelled. At the electron microscopic level, preembedding immunuperoxidase for PV was combined with postembedding immunogold for GABA. In the ventrobasal nucleus, four types of profiles were recognized: 1) terminals with flattened vesicles and forming symmetric synapses, which were labelled with both PV and GABA and could therefore be identified as afferents from the reticular nucleus; 2) boutons morphologically similar to presynaptic dendrites of interneurons, labelled only with GABA; 3) large terminals with round vesicles and asymmetric synapses, labelled only with PV, which contacted GABAergic presynaptic dendrites in glomerular arrangements and resembled ascending excitatory afferents; and 4) terminals unlabelled by either antiserum. In the ventrobasal nucleus of the guinea pig a double immunocytochemical labelling permits therefore the differentiation of two populations of GABAergic vesicle-containing profiles, i. e., the terminals originating from reticular nucleus (that are double labelled) and the presynaptic dendrites originating from interneurons (that are GABA-labelled only). The possibility to differentiate GABAergic inputs from the reticular nucleus and from interneurons can shed light to the functional interpretation of synaptic circuits in thalamic sensory nuclei. © 1994 Wiley-Liss, Inc.     

Relative distribution of synapses in the pulvinar nucleus of the cat: implications regarding the "driver/modulator" theory of thalamic function

To provide a quantitative comparison of the synaptic organization of "first-order" and "higher-order" thalamic nuclei, we followed bias-corrected sampling methods identical to a previous study of the cat dorsal lateral geniculate nucleus (dLGN; Van Horn et al. [2000] J. Comp. Neurol. 416:509-520) to examine the distribution of terminal types within the cat pulvinar nucleus. We observed the following distribution of synaptic contacts: large terminals that contain loosely packed round vesicles (RL profiles), 3.5%; presynaptic profiles that contain densely packed pleomorphic vesicles (F1 profiles), 7.3%; profiles that could be both presynaptic and postsynaptic that contain loosely packed pleomorphic vesicles (F2 profiles), 5.0%; and small terminals that contain densely packed round vesicles (RS profiles), 84.2%. Postembedding immunocytochemistry for gamma-aminobutyric acid (GABA) was used to distinguish the postsynaptic targets as thalamocortical cells or interneurons. The distribution of synaptic contacts on thalamocortical cells was as follows: RL profiles, 2.1%; F1 profiles, 6.9%; F2 profiles, 5.4%; and RS profiles, 85.6%. The distribution of synaptic contacts on interneurons was as follows: RL profiles, 11.8%; F1 profiles, 9.7%; F2 profiles, 2.8%; and RS profiles, 75.6%. These distributions are similar to that found within the dLGN in that the RS inputs (the presumed "modulators") far outnumber the RL inputs (the presumed "drivers"). However, in comparison to the dLGN, the pulvinar nucleus receives significantly fewer numbers of RL, F1, and F2 contacts and significantly higher numbers of RS contacts. Thus, the RS/RL synapse ratio in the pulvinar nucleus is 24:1, in contrast to the 5:1 RS/RL synapse ratio in the dLGN (Van Horn et al., 2000). In first-order nuclei, the lower RS/RL synapse ratio may result in the transfer of visual information that is largely unmodified. In contrast, in higher-order nuclei, the higher RS/RL synapse ratio may allow for a finer modulation of driving inputs.     

Synaptic patterns of the superficial layers of the superior colliculus of the rat

An electron microscopic study has been undertaken of the upper layers of the superior colliculus, into which run fibers from the retina and visual cortex. Study of the normal synaptic patterns shows large numbers of serial synapses, particularly near the surface of the colliculus. The presynaptic components usually contain round vesicles and the intermediate profiles always contain flattened vesicles. The latter may be dendrites, dendrite-like or dilatations of such profiles. Degeneration studies indicate that optic terminals are especially dense near the surface and that they are often the presynaptic terminal of a serial synapse. Very few optic terminals occur in the stratum opticum. Cortical afferents from the visual area mostly end deep in the stratum griseum superficiale, and in superficial stratum opticum, usually on small clear profiles. Studies of the progress of degeneration indicate that optic terminals first show a predominantly neurofilamentous and associated glycogen reaction, and later a predominantly electron dense reaction. Cortical terminals show an initial dense reaction, with occasional neurofilamentous endings. These time course fit well with light microscope data from Nauta and Glees stained material. The synaptic patterns described here closely resemble patterns described in retina and dorsal lateral geniculate body. How these reflect functional similarities has yet to be resolved.     

Projections of physiologically characterized spherical bushy cell axons from the cochlear nucleus of the cat: Evidence for delay lines to the medial superior olive

The dorsal octavolateralis nucleus of lampreys is a primary nucleus for electroreceptive stimuli in the medulla. In Lampetra japonica, the rostral and caudal thirds of this nucleus are exclusively occupied by giant terminals, which become evident when the primary fibers of an electrosensory nerve (recurrent branch of the anterior lateral line nerve) are labeled with horseradish peroxidase. We studied the ultrastructure of these terminals. They contain neurofilaments, mitochondria, microtubules, and tubular membranous structures. Many synapses, all of the chemical type, are located around the neck region of the terminal swellings. Many vesicular structures, which are clear, round, and uniform in size, and most of which are probably synaptic vesicles, are densely clustered in a single large mass in the neck region of the terminals. Some of the tubular structures may serve as a membrane reservoir for the large number of synaptic vesicles required in the giant terminals. © 1993 Wiley-Liss, Inc.     

The fine structures of the suprachiasmatic nucleus of the golden hamster

The fine structure of the suprachiasmatic nucleus of the golden hamster was studied with special reference to the synaptic endings. The somata of SCN neurons contained well developed cytoplasmic organelles including the Golgi complex, mitochondria and polysomes. The nuclei had deeply invaginated nuclear membrane. Some neurons were characterized by the presence of a large number of granulated vesicles and an abundance of cytoplasmic organelles. Several kinds of synapses and gap junctions were also observed. Axo-somatic synapses were identified and could be differentiated based upon possessing two types of presynaptic elements. The first contained clear round synaptic vesicles (40-60 nm in diameter), the second contained clear round vesicles (40-60 nm in diameter) and dense cored vesicles (70-120 nm in diameter). Asymmetrical synaptic membrane thickening were observed on both the pre- and postsynaptic sides of most of the axosomatic synapses. Axo-dendritic synapses could also be divided into two sub-types according to their membrane specializations. In Type 1, the axon terminals contained both clear round vesicles and dense cored vesicles and formed asymmetrical synapses. Terminals in the second group (type 2) were characterized by symmetrical synapses that contained clear, round vesicles as well as dense cored vesicles. The type 1 terminals were evenly distributed throughout the SCN, but the type 2 terminals were encountered more frequently in the ventral SCN. These observations indicate that the ventral and dorsal components of the SCN may possess different functional roles.     

Spatial relationships between the terminations of somatic sensory motor pathways in the rostral brainstem of cats and monkeys. II. Cerebellar projections compared with those of the ascending somatic sensory pathways in lateral diencephalon

In order to classify the presynaptic elements contacting the principle class of globus pallidus neurons, electron microscopic examination of serial sections made from a medially located large globus pallidus neuron, labeled with intracellular horseradish peroxidase, was undertaken. In addition, the use of labeled and light microscopically reconstructed material allowed us to quantitatively determine the distribution of each bouton type along the soma and dendrites. Six types of presynaptic terminals contacting the labeled cell have been recognized. Type 1 endings, the most numerous (84%), make symmetrical contacts on all portions of the cell, except spines, contain large pleomorphic, and a few large dense-core vesicles. Type 2 endings are filled with small spherical-to-ellipsoidal synaptic vesicles. They make asymmetrical contacts only with higher-order dendrites and account for 12% of synaptic contacts onto the labeled neuron. Type 3 endings are large, contain sparsely distributed large pleomorphic vesicles, and make two symmetrical synapses per bouton, one onto a spine head and the other onto the underlying dendritic shaft. They are infrequent (0.2%), being found only in association with dendritic spines. Type 4 endings contain large pleomorphic synaptic vesicles and no dense-core vesicles. They make symmetrical contacts with the short primary dendrites. Type 5 endings contain a mixture of small clear pleomorphic vesicles and numerous large dense-core vesicles. They contact only the cell body and the short primary dendrites, making up 20% of somatic synaptic contacts but less than 1% of contacts onto dendrites. Type 6 boutons contain oval and flattened synaptic vesicles and establish symmetrical contacts with higher-order dendritic branches and the cell body.     

Organization of cholinergic synapses in the cat's dorsal lateral geniculate and perigeniculate nuclei

In the preceding article, we showed that cholinergic fibers originating from the brainstem reticular formation provide a dense innervation of the lateral geniculate nucleus. In this report we describe the ultrastructure of these fibers and their relations with other elements in the neuropil of the lateral geniculate nucleus. Cholinergic fibers were labeled with an antibody to choline acetyltransferase (ChAT), the synthesizing enzyme for acetylcholine (ACh). In the A-laminae of the lateral geniculate nucleus, ChAT + profiles are small and contain tightly packed, mostly round vesicles. Some end in encapsulated synaptic zones where they form asymmetrical synaptic contacts with processes of both projection cells and interneurons. Others form synapses upon the shafts of dendrites. Of the four classical types of vesicle-containing profiles identified by Guillery (Z. Zellforsch. Mikrosk. 96:1-38, '69; Vision Res. [Suppl.] 3:211-227, '71), ChAT + profiles most closely resemble RSD profiles (Round vesicles, Small profile, Dark mitochondria). However, as a population, ChAT + profiles can be distinguished from the unlabeled population of RSD profiles because they are larger in size, contain more mitochondria, and make synapses with smaller postsynaptic membrane specializations. Each of these differences is statistically significant and together they indicate that ChAT + profiles are a distinct morphological type of synaptic profile. ChAT + profiles in the perigeniculate nucleus resemble those found in the lateral geniculate nucleus; they also make synapses with obvious postsynaptic thickenings.     

Synaptic interrelationships between the optic tectum and the ipsilateral nucleus isthmi in Rana pipiens

The nucleus isthmi is reciprocally connected to the ipsilateral optic tectum. Ablation of the nucleus isthmi compromises visually guided behavior that is mediated by the tectum. In this paper, horseradish peroxidase (HRP) histochemistry and electron microscopy were used to explore the synaptic interrelationships between the optic tectum and the ipsilateral nucleus isthmi. After localized injections of HRP into the optic tectum, there are retrogradely labeled isthmotectal neurons and orthogradely labeled fibers and terminals in the ipsilateral nucleus isthmi. These terminals contain round. Clear vesicles of medium diameter (40–52 nm). These terminals make synaptic contact with dendrites of nucleus isthmi cells. Almost half of these postsynaptic dendrites are retrogradely labeled, indicating that there are monosynaptic tectoisthmotectal connections. Localized HRP injection into the nucleus isthmi labels terminals primarily in tectal layers B, E, F, and 8. The terminals contain medium-sized clear vesicles and they form synaptic contacts with tectal dendrites. There are no instances of labeled isthmotectal terminals contacting labeled dendrites. Retrogradely labeled tectoisthmal neurons are contacted by unlabeled terminals containing medium-sized and small clear vesicles. Fifty-four percent of the labeled fibers connecting the nucleus isthmi and ipsilateral tectum are myelinated fibers (average diameter approximately 0.6 μm). The remainder are unmyelinated fibers (average diameter approximately 0.4 μm). © 1994 Wiley-Liss, Inc.