Periventricular-hypophysial dopaminergic neurons innervate the intermediate but not the neural lobe of the rat pituitary gland.

The purpose of the present study was to determine the relative distribution of axon terminals of A14 periventricular-hypophysial dopaminergic (PHDA) neurons in the neural and intermediate lobes of the rat pituitary gland. Discrete unilateral injections of the anterograde tracer Phaseolus vulgaris leucoagglutinin (PHA-L) into the periventricular nucleus resulted in labelling of extensively branched terminal axonal arbors in the intermediate lobe, but not the neural lobe of the pituitary gland. In contrast, unilateral injections of PHA-L into the paraventricular nucleus revealed thick, varicose terminal arborizations containing PHA-L in the neural lobe, but not the intermediate lobe. Terminal axonal branches and varicosities containing PHA-L immunoreactivity in the intermediate lobe were also immunoreactive for tyrosine hydroxylase. These results reveal that A14 PHDA neurons originating in the periventricular nucleus of the hypothalamus project axons to the intermediate lobe of the rat pituitary gland.

The spinotrigeminal pathway and its spatial relationship to the origin of trigeminospinal projections in the rat.

The anterograde transport of horseradish peroxidase and tritiated amino acids was used to examine the distribution and morphology of spinal afferent fibers terminating in the rat spinal trigeminal complex. The results confirm the existence of a direct, ipsilateral projection from the spinal cord which is distributed exclusively to the deepest layers of the medullary dorsal horn narrow regions subjacent to the spinal trigeminal tract in trigeminal nucleus interpolaris, trigeminal nucleus oralis and the trigeminal main sensory nucleus. Spinal inputs also terminated in the insular trigeminal-cuneatus lateralis nucleus which is a distinct component of the interstitial system of the spinal trigeminal tract. The spinal afferent fibers which terminated in the dorsolateral parts of the spinal trigeminal complex arose from the dorsal column funiculi, while those that terminated in ventral parts of the complex arose from both the dorsal column and lateral funiculi. The tritiated amino acid experiments indicate that at least part of the spinotrigeminal pathway originates from cells located in the cervical spinal dorsal horn. The present findings also document a complex spatial relationship between the spinotrigeminal and trigeminospinal pathways which includes an extensive overlap between spinotrigeminal fibers and spinal projecting neurons in each of the lateralmost regions of the complex. This spatial overlap supports the existence of anatomical substrates which may underlie functional reciprocal loops between the spinal trigeminal complex and cervical spinal cord. Since these regions are primarily concerned with the processing of sensory information from lateral and posterior parts of the face, it follows that the spinotrigeminal pathway may be primarily concerned with the integration of head and neck functions. In addition, the spatial convergence of spinal inputs and the distribution of other trigeminal efferent neurons suggests that part of the spinotrigeminal pathway may be involved in spino-trigemino-thalamic and spino-trigemino-cerebellar pathways in parallel with other spinobulbar pathways in the medulla.

A comparison of the distribution and morphology of thalamic, cerebellar and spinal projection neurons in rat trigeminal nucleus interpolaris.

The retrograde transport of horseradish peroxidase was used to examine and compare the distribution and morphology of thalamic, cerebellar and spinal projecting neurons in rat trigeminal nucleus interpolaris following large injections into their respective targets. The regional distribution of these three populations was evaluated in relation to the six cytoarchitecturally distinct regions which characterize the nucleus. Cerebellar projecting neurons were distributed throughout the rostrocaudal extent of trigeminal nucleus interpolaris, but were infrequently present in its dorsolateral region and in the rostral pole of the nucleus. Thalamic projecting neurons exhibited a distribution pattern that extensively overlapped with that of the trigeminocerebellar neurons: however, they were particularly concentrated in caudal, dorsomedial and rostral, ventrolateral regions of the nucleus. Trigeminospinal projecting neurons exhibited a more restricted distribution within ventral and lateral regions of trigeminal nucleus interpolaris. Although the three populations of projection neurons could not be distinguished solely on the basis of somatic size or shape, distinct regional variations in the distribution and somatodendritic and axonal morphology of these neurons indicated that they arise largely from independent cell populations. However, several regions were identified in which specific cell types were likely to contribute to axonal collaterilization among these pathways. In the ventrolateral magnocellular region of the nucleus, for example, more than half of the large multipolar-shaped neurons were retrogradely labeled after injections into each of the three target sites. The results of the present study indicate that the thalamic, cerebellar and spinal projections of trigeminal nucleus interpolaris arise from a morphologically heterogeneous group of neurons. In addition, regional variations in the distribution and morphology of these neurons provide evidence for the existence of functionally distinct regions that parallel the cytoarchitecturally defined regions of the nucleus. This study also provides indirect evidence for and against collateralization among these three projections within specific regions of the nucleus.

Fine structural characteristics and synaptic connections of trigeminocerebellar projection neurons in rat trigeminal nucleus oralis.

In order to classify the presynaptic terminals contacting trigeminocerebellar projection neurons (TCPNs) in rat trigeminal nucleus oralis (Vo), electron-microscopic examination of sequential thin sections made from TCPNs located in the border zone (BZ) of Vo, labeled by the retrograde transport of horseradish peroxidase, was undertaken. The use of BZ TCPNs, labeled in Golgi-like fashion so that many of their dendrites and axons were visible, allowed for the determination of the distribution of each bouton type along the soma and dendrites, as well as for the characterization of the morphology and synaptic relations of the labeled axon and its terminals. Three types of axon terminals contacting labeled BZ TCPNs have been recognized, depending upon whether they contain primarily spherical-shaped, agranular synaptic vesicles (S endings); predominantly flattened, agranular synaptic vesicles (F endings); or a population of pleomorphic-shaped, agranular synaptic vesicles (P endings). The S endings represent the majority of axon terminals contacting labeled BZ TCPNs and establish asymmetrical axosomatic and axodendritic synaptic contacts. Many S endings are situated in one of two types of synaptic glomeruli. One type of glomerulus has a large S ending at its core, whereas the other contains a small S ending. Large-S-ending glomeruli include only labeled distal dendrites of BZ TCPNs; small-S-ending glomeruli contain either a labeled soma, proximal dendrite, or distal dendritic shaft. The remaining S endings are extraglomerular, synapsing on distal dendrites. P endings are less frequently encountered and establish intermediate axosomatic and axodendritic synapses. These endings exhibit a generalized distribution along the entire somatodendritic tree. F endings make symmetrical axodendritic synapses with distal dendrites, are only found in glomeruli containing small S endings, and are the least frequently observed ending contacting labeled BZ TCPNs. The majority of axonal endings synapsing on labeled BZ TCPNs are located along distal dendrites, with only a relatively few synapsing terminals situated on proximal dendrites and somata. The axons of labeled BZ TCPNs arise from the cell body and generally give rise to a single short collateral near their points of origin. This collateral remains unbranched and generates several boutons within BZ, while the parent axon acquires a myelin sheath and, without branching further, travels dorsolaterally toward the inferior cerebellar peduncle. The collateral boutons resemble extraglomerular S endings. They contain agranular, spherical-shaped synaptic vesicles and make asymmetrical axodendritic synapses with small-diameter unlabeled dendritic shafts in the BZ neuropil.

The interstitial system of the spinal trigeminal tract in the rat: anatomical evidence for morphological and functional heterogeneity.

Utilizing cyto-, myelo-, and chemoarchitecture as well as connectional criteria, the present study reveals the interstitial system of the spinal trigeminal tract (InSy-SVT) in the rat to be composed of five morphologically and functionally distinct components that are distributed within spatially restricted regions of the lateral medulla. The first component is represented by scattered interstitial cells and neuropil, which extend laterally into SVT from the superficial laminae of the medullary dorsal horn (MDH). The second component, the dorsal paramarginal nucleus (PaMd), consists of a small group of marginal (lamina I)-like neurons and neuropil situated within the dorsolateral part of SVT at the rostral pole of MDH. The third component represents a trigeminal extension of the parvocellular reticular formation (V-Rpc) into the ventromedial aspect of SVT at levels extending from rostral MDH to the caudal part of trigeminal nucleus interpolaris (Vi). The fourth component, the paratrigeminal nucleus (PaV), consists of a large accumulation of neurons and neuropil situated within the dorsal part of SVT throughout the caudal half of Vi. The fifth component is the insular trigeminal-cuneatus lateralis nucleus (iV-Cul), which is a discontinuous collection of neurons and neuropil interspersed among fibers of SVT as well as wedged between it and the spinocerebellar tract. Thalamic projection neurons are located in PaMd and V-Rpc, whereas cerebellar projecting neurons are confined to iV-Cul.

A survey of the cytology and synaptic organization of the insular trigeminal-cuneatus lateralis nucleus in the rat, including an identification of spinal afferent inputs.

The cytology and synaptic organization of the insular trigeminal-cuneatus lateralis (iV-Cul) nucleus was examined in the rat. In addition, the ultrastructural morphology and synaptic connectivity of anterogradely labeled spinal afferent axons terminating in iV-Cul were examined following injection of horseradish peroxidase (HRP) into the cervical spinal cord. The uniformity of the ultrastructural features of iV-Cul neurons supports the presence of a homogeneous neuronal population. The most prominent feature of the iV-Cul neuropil is the presence of numerous interdigitating astrocytic processes, which extensively isolate neuronal somata and processes. iV-Cul contains a heterogeneous population of axonal endings that can be separated into three categories, depending upon whether they contain predominantly spherical-shaped agranular synaptic vesicles (R endings), predominantly pleomorphic-shaped agranular synaptic vesicles (P endings), or a heterogeneous population of dense-core vesicles (DC endings). The R endings represent the majority of axonal endings in iV-Cul and establish asymmetrical axodendritic and axospinous synaptic contacts, primarily along the distal portions of the dendritic tree. P endings establish symmetrical axosomatic, axodendritic, and axospinous synaptic contacts and exhibit a more generalized distribution along the somadendritic tree. DC terminals establish asymmetrical axodendritic synaptic contacts with distal dendritic processes and are the least frequently observed endings in the iV-Cul neuropil. Numerous synaptic glomeruli, exhibiting a single large central R bouton that establishes multiple axodendritic or axospinous synapses, characterize the iV-Cul neuropil. Axoaxonic synapses are conspicuously absent from the iV-Cul neuropil and glomeruli. The anterograde HRP labeling of spinal afferent axons that terminate in iV-Cul indicates that the terminals along these fibers are of the R type and that they are engaged predominantly in synaptic glomeruli. The results of this study indicate that the synaptic organization of iV-Cul is distinctly different from that of neighboring somatosensory nuclei, and supports the recent suggestion that this nucleus should be considered a separate precerebellar spinal relay nucleus in the lateral medulla.

An analysis of the cyto- and myeloarchitectonic organization of trigeminal nucleus interpolaris in the rat.

The cyto- and myeloarchitectonic organization of trigeminal nucleus interpolaris (Vi) was examined in the rat using correlated Nissl- and myelin-stained sections. The caudal boundary of Vi is marked by a spatial overlap with the rostral pole of the medullary dorsal horn (MDH), where there is a dorsal and medial displacement of the substantia gelatinosa (SG, lamina II) layer of MDH. This spatial displacement was further documented using cytochrome-oxidase-reacted sections through the periobex region (POR) of the medulla, where the relatively unstained SG contrasts sharply with the intensely stained Vi neuropil. The rostral boundary of Vi is characterized partly by a distinct overlap with the caudal pole of the dorsomedial region (DM) of trigeminal nucleus oralis (Vo), and partly by a more gradual transition with ventral and lateral regions of Vo. The presence of the distinct MDH-Vi overlap is discussed in terms of its impact on the widespread contention that Vi is involved in the processing of dental pain afferents in the POR. Six separate and distinct regions of rat Vi can be distinguished on the basis of differences in their overall cyto- and myeloarchitecture: (1) a ventrolateral parvocellular region (vlVipc), which occupies the ventrolateral caudal half of Vi; (2) a ventrolateral magnocellular region (vlVimc), which occupies a similar region in the rostral half of the nucleus; (3) a border region (brVi), interposed between the spinal trigeminal tract (SVT) and vlVipc and vlVimc; (4) a dorsolateral region (dlVi), which lies predominantly in the rostral two-thirds of Vi subjacent to the dorsal half of SVT; (5) a dorsal cap region (dcVi), occupying the dorsomedial aspect of the nucleus throughout its entire rostrocaudal extent; and (6) an intermediate region (irVi), which lies immediately ventral to dcVi within the concavity formed by the medial borders of vlVipc and vlVimc. It is proposed that these cyto- and myeloarchitecturally distinct regions of Vi may largely represent functionally distinct regions, based on reported differences in the organization of afferent and efferent projections within the nucleus.

Synaptic organization of primary axons in trigeminal nucleus oralis.

This report examines the morphology and synaptic connections of small-diameter primary trigeminal axons that terminate in the border zone (BZ) and ventrolateral (VL) subdivisions of rat trigeminal nucleus oralis (Vo). Primary axons were made visible for light and electron microscopic analysis by utilizing the method of anterograde transport of horseradish peroxidase. BZ receives the terminal arborizations of two different populations of small-diameter primary axons. One of these arises from unmyelinated parent fibers and terminates in the dorsal one-half of BZ, while the other has small myelinated parent branches that arborize throughout the subdivision. Terminating within VL are the arbors of a second population of small myelinated primary axons. The endings of all three populations of primary axons lie in synaptic glomeruli. Endings in both subdivisions derived from small myelinated parent fibers lie centrally in glomeruli. Those in VL form axodendritic synapses on numerous dendritic shafts and spines, while endings in BZ glomeruli make at least one axodendritic synapse on one or two dendritic shafts. Endings of unmyelinated primary axons in BZ lie at the periphery of glomeruli where each forms a single axodendritic synapse on a central dendrite. It is at these asymmetrical axodendritic synapses that these three populations of primary axons are thought to transfer their inputs directly to the dendritic arbors of second-order BZ and VL neurons. Common to all three glomeruli is one or more small axonal endings filled with flattened synaptic vesicles that establish axoaxonic synapses on the primary ending as well as axodendritic synapses on the dendritic element(s) receiving primary input. In view of their symmetrical to intermediate synaptic contacts, these endings are thought to belong to axons derived from at least one source that can inhibit or diminish the firing rate of second-order BZ and VL neurons in response to primary input.

Direct connections of primary trigeminal afferent axons with trigeminocerebellar projection neurons in the border zone of rat trigeminal nucleus oralis.

This study presents electron microscopical evidence for direct synaptic contact between primary trigeminal axonal (PR) endings and trigeminocerebellar projection neurons (TCPNs), in the border zone (BZ) of rat trigeminal nucleus oralis. The combined techniques of anterograde degeneration following trigeminal sensory root rhizotomy and retrograde transport of horseradish peroxidase subsequent to injections into the orofacial tactile portions of crura I and II of the cerebellar hemispheres were utilized. Degenerating PR endings lie centrally in glomeruli where they form axodendritic synapses on higher order dendrites of identified BZ TCPNs. It is at these synapses that the PR endings are probably transferring tactile input to BZ TCPNs for direct relay to the cerebellar cortex. Transmitter release at the axodendritic synapses may be modified within the glomeruli by axoaxonic synapses between terminals containing flattened synaptic vesicles and the PR ending.

Morphology and synaptic connections of unmyelinated primary axons in the border zone of rat trigeminal nucleus oralis.

This anterograde horseradish peroxidase study examines the morphology and synaptic connections of a population of primary axons which terminate in the dorsal one-half of the border zone (BZ) of rat trigeminal nucleus oralis. Unmyelinated parent fibers in the spinal V tract enter BZ directly and each terminate by continuing as a sparsely branched, long caudally directed strand containing several axonal endings. Primary endings lie in glomeruli where each forms an asymmetrical synapse on a central dendrite. Other glomerular components include two types of non-primary endings. One contains flattened synaptic vesicles, and forms a symmetrical synapse on either the primary ending or the central dendrite, while the other contains pleomorphic synaptic vesicles and establishes a symmetrical synapse on the central dendrite.

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.

Morphology and synaptic connections of small myelinated primary trigeminal axons arborizing among neurons in the border zone of rat trigeminal nucleus oralis.

The anterograde transport of horseradish peroxidase (HRP) was used to examine the morphology and synaptic connections of a morphologically distinct group of small-diameter primary trigeminal axons that arborize throughout the border zone (BZ) of rat trigeminal nucleus oralis. Thinly myelinated parent branches (0.75-1.5 micron in diameter) descending in the spinal V tract (SVT) were seen to issue medially directed collaterals that entered BZ, where they branched and eventually terminated by giving rise to thin terminal strands characterized by several relatively widely spaced axonal endings. Based on the size and morphology of the parent branches in SVT, in the root entry zone, and in the sensory root of the trigeminal nerve, these primary axonal (P) endings are considered to be derived from small-diameter myelinated primary trigeminal axons (SDMA). The P endings measured 1-2 micron in diameter and contained numerous agranular spherical (40-60 nm) synaptic vesicles. In the BZ neuropil, most P endings lay in glomeruli, where each formed at least one asymmetrical axodendritic synapse on a dendritic shaft. It is at these synapses that this group of primary axons is thought to transfer its input directly to the dendritic arbors of BZ neurons. A small (0.5-1.5 micron) axonal (F) ending filled with flattened synaptic vesicles (29 X 60 nm) was observed to form at least one symmetrical to intermediate axoaxonic synapse on the P ending, as well as at least one axodendritic synapse on the same dendritic shaft receiving the primary input. Some F endings only contacted dendritic shafts. In view of their symmetrical to intermediate synaptic contacts, F endings are thought to belong to axons derived from at least one source that can inhibit or diminish the firing rate of BZ neurons in response to SDMA input. This would be accomplished either postsynaptically through the axodendritic synapses on the dendritic shafts, and/or presynaptically through the axoaxonic synapses on the P endings.

Morphological features of identified trigeminocerebellar projection neurons in the border zone of rat trigeminal nucleus oralis.

The retrograde transport of horseradish peroxidase (HRP) was used to assess the overall morphology of neurons in the dorsal half of the border zone (BZ) of rat trigeminal nucleus oralis (Vo) that project to ipsilateral orofacial portions of four major tactile areas (crura I and II, the paramedian lobule, and the uvula) of the cerebellar cortex. We wished to answer two important questions: Does this group of cells consist of one or more morphologically distinct types, each projecting to different cerebellar tactile areas? Does the overall morphology or morphologies of these BZ neurons resemble one or more of the five types of identified trigeminocerebellar neurons in the dorsomedial (DM) subdivision of Vo, or do these trigeminocerebellar cells represent an additional morphologically distinct type or types restricted to BZ? The morphology of BZ neurons innervating the orofacial portions of all four cerebellar tactile areas was similar and did not resemble that of any of the five types of DM cells. They were characterized by a pyramidal- to fusiform-shaped cell body measuring 10-13 X 20-25 microns, which emitted three or four primary dendrites; one was directed dorsally, while the others took a more ventral trajectory. The primary dendrites generated a dendritic arbor arranged as a flattened disk oriented parallel to the spinal V tract. The dendritic field was largely restricted to BZ; it measured up to 150 microns in width, and spanned up to 450 microns dorsoventrally and rostrocaudally. An axon arose from the dorsal aspect of the cell body and gave rise to a single short collateral within 10 microns of its origin. This collateral remained unbranched and generated several boutons within BZ, while the parent axon, without branching further, traveled dorsolaterally toward the inferior cerebellar peduncle. Frequently, a second axon arose ventrally from the soma, and after a short unbranched course entered a deep axon bundle, where it assumed a descending trajectory. The intranuclear portion of this second axon was characterized by several boutons en passant.

The dorsomedial portion of trigeminal nucleus oralis (Vo) in the rat: cytology and projections to the cerebellum.

Electrophysiological studies have described four major tactile areas in the rat cerebellar cortex. These areas are in crus I, crus II, the paramedian lobule (PML), and the uvula, and a major portion of each is related to the ipsilateral orofacial region. This study demonstrates that neurons in trigeminal nucleus oralis (Vo) that project to the orofacial portions of these four major tactile areas are localized in the dorsomedial (DM) subdivision of the nucleus. The distribution, light-microscopic morphology, and relative densities of trigeminocerebellar neurons within DM, retrogradely labeled with horseradish peroxidase (HRP) following injections into each of the four major tactile areas, were analyzed and compared as well as correlated with the myelo- and cytoarchitecture of DM observed in Nissl sections, 1-micron sections, and Golgi material. On the basis of myelo- and cytoarchitectonic as well as trigeminocerebellar connectional criteria, three portions of DM were identified: caudal DM (CDM), middle DM (MDM), and rostral DM (RDM). The greatest portion of DM is made up of MDM (1.3 mm long), which can be further subdivided into dorsal (MDMd) and ventral (MDMv) zones. CDM forms the caudal 800 microns of DM, while RDM makes up the rostral 280 microns of the subdivision. Longitudinally running deep axon bundles permeate CDM, MDMv, and RDM, but are conspicuously absent from MDMd. The majority of neurons found throughout CDM, MDMv, and RDM have medium-sized (15- to 30-microns) somata and can be divided into two types on the basis of their somatodendritic morphology. CDM, MDMv, and RDM also contain a small neuronal cell type (5- to 15-microns cell body) that is encountered less frequently than either one of the two types of medium-sized cells. A fourth type of neuron with a large (25- to 50-microns) fusiform- to pyramidal-shaped cell body is the least frequently observed neuronal cell type and is located principally in CDM and MDMv. MDMd contains a fifth type of neuron characterized by a small (5- to 15-microns) oval soma. Data from the retrograde HRP experiments show that all five of these neuronal cell types in their respective portions of DM project to one or more of the orofacial portions of the four major tactile areas of the cerebellar cortex. Many medium-sized neurons of both types in CDM, MDMv, and RDM project to crus I, crus II, and/or PML.(ABSTRACT TRUNCATED AT 250 WORDS)

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 microns 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 microns 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 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.

The morphology of neurons in trigeminal nucleus oralis projecting to the medullary dorsal horn (trigeminal nucleus caudalis): a retrograde horseradish peroxidase and Golgi study.

This study demonstrates that trigeminal nucleus oralis, the most rostral subdivision of the spinal trigeminal nucleus, contains four morphologically distinct types of small neurons which project to the medullary dorsal horn (trigeminal nucleus caudalis) via descending intratrigeminal pathways. Using the retrograde transport of horseradish peroxidase following injections in the medullary dorsal horn, labeled small neurons with cell bodies ranging from 8-15 microns in diameter are found principally in the ventrolateral portion of the trigeminal nucleus oralis. Most neurons are labeled ipsilaterally throughout the entire rostrocaudal extent of the ventrolateral portion of the trigeminal nucleus oralis, but a few cells are also labeled contralaterally. From this aspect of the present study it can be concluded that a specific portion of the trigeminal nucleus oralis, i.e. the ventrolateral part, contains numerous small neurons which send descending projections to the medullary dorsal horn that could affect synaptic activity there. Utilizing both the methods of Golgi and retrograde horseradish peroxidase labeling four distinct types of small descending medullary dorsal horn projection neurons can be distinguished in the ventrolateral portion of the trigeminal nucleus oralis on the basis of their morphology and the distribution of their axons and dendrites. All four neuronal cell types are present throughout the entire rostrocaudal extent of the trigeminal nucleus oralis. Type I neurons are the most frequently labeled descending medullary dorsal horn projection neurons. They are concentrated in the medial 500-550 microns of the ventrolateral portion of the trigeminal nucleus oralis and display dendritic trees which occupy spherical domains approaching 300 microns in diameter. The unmyelinated axons of many of these cells arise either directly from the cell body or a primary dendrite and give rise to a single collateral within 50 microns of their site of origin. This collateral generates a fine axonal plexus within a portion of the dendritic arbor of the parent cell while the parent axon, without branching further, travels a short distance in the ventrolateral portion of the trigeminal nucleus oralis and enters a deep axon bundle. Type II neurons are the second most frequently labeled descending medullary dorsal horn projection neuron. They generate medial and lateral dendritic arbors which together span nearly the entire medial 500-550 microns of the ventrolateral portion of the trigeminal nucleus oralis. An unmyelinated axon emerges from the cell body and within 10-30 microns of its origin gives rise to two collaterals.(ABSTRACT TRUNCATED AT 400 WORDS)

Termination in trigeminal nucleus oralis of ascending intratrigeminal axons originating from neurons in the medullary dorsal horn: an HRP study in the rat employing light and electron microscopy.

The anterograde horseradish peroxidase (HRP) technique was used to identify ascending intratrigeminal axons originating from neurons in the medullary dorsal horn (MDH) which terminate in trigeminal nucleus oralis (Vo). HRP injections into the MDH labeled two populations of axons ascending ipsilaterally within the spinal trigeminal nucleus. The first population was composed of parent branches which each gave off a single branching collateral strand to Vo as they ascended. These collaterals were characterized by boutons filled with small, round synaptic vesicles and forming asymmetrical synaptic contacts with large diameter dendritic shafts. The second axonal population was made up of parent branches which terminated directly in Vo. Their short terminal strands were distinguished by axonal endings containing pleomorphic synaptic vesicles and forming symmetrical synaptic junctions with small diameter dendritic shafts and spines.

An intracellular HRP study of the rat globus pallidus. II. Fine structural characteristics and synaptic connections of medially located large GP neurons.

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.

A Golgi Type II neuron in trigeminal nucleus oralis: a Golgi study in the rat.

This Golgi study identifies a class of small neurons in trigeminal nucleus oralis (Vo) that satisfies all the morphological criteria for a Golgi Type II neuron. The cylindrical-shaped dendritic arbor extends up to 500 micron in the rostrocaudal axis and is confined to Vo. The unmyelinated axon generates a highly branched collateral axonal plexus within or near the dendritic tree and it does not project out of Vo. This Golgi Type II neuron is considered to be an inhibitory interneuron and probably participates in a variety of inhibitory phenomena known to occur in Vo.

An intracellular HRP study of the rat globus pallidus. I. Responses and light microscopic analysis.

A study of the intracellularly recorded responses of rat globus pallidus neurons to activation of striopallidal fibers was combined with light microscopic examination of the morphology of these same neurons using intracellular horseradish peroxidase. The response to stimulation of caudate-putamen is an inhibitory postsynaptic potential with observed latencies ranging from 5.1 to 9.8 msec. These values correspond to conduction velocities of 0.4 to 0.8 m/second for striopallidal fibers. Comparison with extracellular controls shows no excitatory component to the response. All recovered and analyzed neurons (n = 11) were of the large type of pallidal neuron known from Golgi studies but the addition that two subtypes could be recognized. Large neurons located medially in the nucleus had dendritic fields with large dorsoventral extent (ca. 1 mm) when compared to their mediolateral and rostrocaudal dimensions (ca. 0.4 mm) and these neurons emitted no axon collaterals. Large neurons located laterally in the nucleus had disklike dendritic fields with both dorsoventral and rostrocaudal dimensions being on the order of 1 mm but with a minor axis of approximately 100 micrometers. The axons of these neurons possessed collaterals. As a consequence of their disk-shaped dendritic field, neurons belonging to the laterally placed subgroup and occupying the narrow (ca. 100 micrometers thick) striopallidal border zone known to receive a distinct input from neostriatum have dendrites restricted to that zone.