Characterization of Merkel cells and mechanosensory axons of the rat by styryl pyridinium dyes

Summary The epidermal Merkel cells and their sensory innervation serve tactile sensation in vertebrates. In this study the fluorescent cationic mitochondrial dye, 4-(4-diethylaminostyryl)-N-methylpyridinium iodide (4-Di-2-ASP), which has recently been used as a vital stain for motor and autonomic nerve terminals, was tested for its ability to stain Merkel cells and sensory fibers in the snout of the rat. Brightly-fluorescent structures resembling Merkel cells as well as nerve fibers and their terminations were evident in whole mounts of the vibrissal follicle. Unilateral denervation of the vibrissal follicles soon after birth resulted in a staining pattern remarkably similar to that obtained after labelling of the Merkel cells selectively with the fluorescent marker quinacrine, but all fiber staining was abolished. Likewise, in the separated epidermis of other skin regions, including the hairy and glabrous skin of the nose, the staining pattern revealed by 4-Di-2-ASP was indistinguishable from that obtained by quinacrine fluorescence. These results indicate that certain styryl pyridinium dyes may be used as vital stains for epidermal Merkel cells as well as cutaneous mechanosensory axons.     

Serotonin-containing Cells in the Nervous System and Other Tissues During Ontogeny of a Lancelet,Branchiostoma floridae

Abstract Serotonin-containing cells are described by immunohistochemistry throughout lancelet ontogeny. Such cells are first detected in the 2-day larva: these are (1) enterochromaffin cells in the inner epithelium of the gut and (2) anterior serotonergic neurons at the rostral end of the nerve cord. In the 6-day larva, relatively low levels of serotonin appear in ventro-lateral perikarya and cell processes of intraspinal serotonergic neurons scattered along the nerve cord. In the 18-day (early metamorphic) larva, antero-lateral serotonergic neurons are detected near the rostral end of the nerve cord as two small, bilateral clusters of perikarya with axons that descend the nerve cord; at later developmental stages, these axons extend almost to the posterior end of the body. In the 21-day (mid-metamorphic) larva, serotonin can no longer be detected in the anterior serotonergic neurons, but serotonin-containing cells are found subjacent to the inner epithelium of the digestive caecum and in the peribranchial epithelium covering the primary gill bars. In the discussion, we suggest that the anterior serotonergic neurons may play a role in larval photoreception and that the antero-lateral serotonergic neurons may be homologous to vertebrate hindbrain neurons with axons descending the spinal cord to modulate undulation (if this homology is valid, the anterior limit of the lancelet hindbrain would be roughly 100 μm behind the rostral tip of the nerve cord).     

Somatostatinergic nerves in the cervical spinal cord of the monkey

Somatostatinergic nerves in the spinal cord of the monkey were investigated utilizing immunohistochemistry with various antibodies against synthetic somatostatin. In contrast to earlier investigations, it is shown that somatostatinergic nerve endings occur in most of the areas of the grey matter of the spinal cord. The somatostatinergic axons are, however, characteristically distributed in three main regions: (1) Densely-packed endings are seen in lamina II of the substantia gelatinosa, forming a crescent-shaped pattern in the columna dorsalis. Somatostatin immunoreactivity is also seen in lamina I and in the Lissauer tract. (2) A fine network of fibers is observed around the central canal; the endings are concentrated on special cell bodies. Some single perikarya are also stained in this region. (3) A loose network of single fibers is found ending on perikarya of the columna lateralis or ventralis. The perikarya of the nerve axons, with the exception of those terminating in the columna dorsalis, have as yet not been identified. In order to better understand the somatostatinergic system of the spinal cord, these newly-detected somatostatinergic nerves must be studied and their exact pathways analyzed.     

Fine structure of probable mechano- and chemoreceptors in the caudal epidermis of the lugworm Arenicola marina (Annelida,Polychaeta)

Summary The caudal part of the lugworm Arenicola marina shows numerous epidermal papillae formed by a thick glandular epidermis in which ciliated sensory buds have been found. These buds comprise supporting cells and two types of receptors, R1 and R2, which are primary sensory cells whose axons are connected to the basiepidermal nerve plexus. The receptors possess several typical cilia projecting into the surrounding seawater, stout intracuticular microvilli filled with filaments, and they contain dense vesicles. The R1 cells, more numerous, show features of chemosensory cells. The rarer R2 cells have large striated rootlets surrounded by a dense sheath of fibrillar material and are probably mechanoreceptors. The physiological functions of these receptors are discussed.     

Embryos and Larvae of a Lancelet,Branchiostoma floridae,from Hatching through Metamorphosis: Growth in the Laboratory and External Morphology

Florida lancelets were raised in laboratory cultures from the egg to the juvenile stage. At frequent intervals during development, elongation of the embryonic and larval body was measured at room temperature (22.5°C) and at the approximate temperature of the natural environment (30°C). Development was slower at the lower temperature, with metamorphosis commencing during the fifth week as compared to the third week at the higher temperature. Scanning electron microscopy (SEM) was used to describe a frequently sampled series of hatched embryos, pre-metamorphic larvae, metamorphic larvae, and juveniles. The advent (and sometimes subsequent disappearance) of the following structures was determined from the SEM data: general epidermal ciliation, peroral pit, mouth, primary gill slits, ciliary tuft, external opening of the club-shaped gland, sense cells, anus, metapleural folds, and preoral cirri. Our SEM did not substantiate the claims of van Wijhe for a transitory larval mouth near the anteriovental end of the larvae. The general epidermal cilation, which is uniformly distributed in the embryos, becomes somewhat reduced in the pre-metamorphic larvae and then disappears almost entirely during metamorphosis. The epidermis includes two distinct sense cell types (I and II) and possibly a third type (the ventral pit cells, to which an adhesive role has alternatively been attributed). The anus first opens on the right-hand side and only later migrates across the mid-ventral line to assume a position on the left-hand side of the larva; this is contrary to the established view that the anus of the larval lancelets opens on the left-hand side and remains there.     

Plasma membrane glycoproteins during anuran amphibian epidermal development

Summary A cytochemical and biochemical study of galactose (Gal) and N-acetyl-glucosamine (GlcNAc) containing glycoproteins of the anuran amphibian epidermis during development has been carried out. In premetamorphic tadpoles, theGriffonia simplicifolia II lectin (GS II, specific for N-acetyl glucosamine) bound to a glycoprotein of 49 kDa in the plasma membrane of all the epidermal strata showing a basal-to-apical binding gradient. During metamorphic climax GS II labeling was progressively polarized to the outermost plasma membrane. In epidermis from juveniles and adults the staining was observed mainly in a 52 kDa band.Griffonia simplicifolia I lectin (GS I, specific for galactose) also bound to a glycoprotein of about 49 kDa in tadpoles and 52 kDa in frogs. Furthermore, a GS I labeling in bands of about 110–150 kDa appears during metamorphosis. After this process, a definitive pattern of lectin staining and K⁺-stimulated, ouabain-sensitive p-nitrophenyl phosphatase activity is established.     

Development of the caudal neurosecretory system of the chum salmon,Oncorhynchus keta,as revealed by immunohistochemistry for urotensins I and II

In order to make an immunohistochemical analysis of the development of the caudal neurosecretory system of the chum salmon, Oncorhynchus keta, we employed the peroxidase-anti-peroxidase technique using antisera specific for urotensins (U) I and II on artificially reared embryos, larvae, and juveniles of this species. Immunoreactivities for UI and UII were first demonstrated in the embryo immediately before hatching, showing labeled perikarya and fibers in the most caudal region of the spinal cord where the presumptive caudal neurosecretory system is located. However, distinct differentiation of the histological neurohemal organ had not yet begun in the embryo. Immunoreactive perikarya and fibers gradually increased in number, and an elaborate urophysis comparable to that of adults was demonstrated in the larvae about 5 months after hatching. At this stage, weak immunoreactivity against UI was detected in the neurohypophysis.     

Nerve growth factor regulates central terminals of primary sensory neurons

Transection of peripheral sensory axons results in transganglionic degenerative atrophy of central terminals of the affected primary sensory neurons. Nerve growth factor applied at the central stump of the transected nerve prevents or delays transganglionic degenerative atrophy. It is concluded that, under normal conditions, nerve growth factor taken up by receptors at peripheral sensory nerve endings and transported retrogradely to perikarya in dorsal root ganglia, regulates synthesis of neuroproteins destined for maintenance of central terminals of these neurons. Accordingly, transganglionic degenerative atrophy is the consequence of failure of nerve growth factor to reach perikarya of primary sensory neurons.     

Nervous system of ascidian larvae: Caudal primary sensory neurons

Summary In larvae of Diplosoma macdonaldi one sensory nerve extends along the dorsal midline of the tail and another extends along the ventral midline. Each nerve is composed of 50–70 naked axons lying in a groove in the base of the epidermis, and each projects to the visceral ganglion. The cell bodies of the caudal sensory neurons occur in pairs within the epidermis, and are situated along the courses of the nerves. A single cilium arises from an invagination in the soma of each neuron, passes through the inner cuticular layer of the tunic and enters a tail fin formed by the outer cuticular layer. We propose that these cells are mechanoreceptors. The caudal sensory system is similar in representative species of ten families of ascidians.Abbreviations a axial complex of the tail - ac accessory centriole - ax axon - bb basal body - bl basal lamina - c cilium - cep common epidermal cells - cs ciliary sheath - dcv dense-cored vesicles - dsn dorsal sensory nerve - ec ependymal cells - ep epidermis - gj gap junction - h hemocoel - hc hemocoelic chamber - icl inner cuticular layer of the tunic - m caudal muscle - nc dorsal nerve cord - ncl neurocoel - no notochord - ocl outer cuticular layer of the tunic - sc sensory cell - sn sensory nerve - sv sensory vesicle - vg visceral ganglion - vsn ventral sensory nerve     

Further Ultrastructural Studies on the Encapsulated Larva of Kronborgia isopodicola (Platyhelminthes,Fecampiidae), with Particular Reference to Nuclei

During development of the encapsulated Kronborgia isopodicola larva, nuclei of the body tissues and differentiating eyes undergo a continuous condensation, the progression of which is described. The brain is composed of a central neuropil and an outer layer of nerve cell perikarya. Neurosecretory cells are located at the sides of the brain. Some neurosecretory cell extensions are interposed between the cerebral neuropil and nerve cell perikarya; others overlie the photoreceptor cell processes of the eyes. The advanced encapsulated larva possesses a frontal complex, consisting of modified epidermis, secretory cells, gland ducts and nerve cell processes. The advanced larva is transparent and diminished in size, advantages possibly due in part to the extraordinary process of comprehensive nuclear condensation during ontogeny. The larva has a uniform epidermal ciliation and, while sharing certain features with trochophore larvae, is not of the trochophore type.     

Alterations in the morphology of ganglion cell dendrites in the adult rat retina after optic nerve transection and grafting of peripheral nerve segments

Summary Transected ganglion cell axons from the adult retina are capable of reinnervating their central targets by growing into transplanted peripheral nerve (PN) segments. Injury of the optic nerve causes various metabolic and morphological changes in the retinal ganglion cell (RGC) perikarya and in the dendrites. The present work examined the dendritic trees of those ganglion cells surviving axotomy and of those whose severed axons re-elongated in PN grafts to reach either the superior colliculus (SC), transplanted SC, or transplanted autologous thigh muscle. The elaboration of the dendritic trees was visualized by means of the strongly fluorescent carbocyanine dye DiI, which is taken up by axons and transported to the cell bodies and from there to the dendritic branches. Alternatively, retinofugal axons regrowing through PN grafts were anterogradely filled from the eye cup with rhodamine B-isothiocyanate. The transection of the optic nerve resulted in characteristic changes in the ganglion cell dendrites, particularly in the degeneration of most of the terminal and preterminal dendritic branches. This occurred within the first 1 to 2 weeks following axotomy. The different types of ganglion cells appear to vary in their sensitivity to axotomy, as reflected by a rapid degeneration of certain cell dendrites after severance of the optic nerve. The most vulnerable cells were those with small perikarya and small dendritic fields (type II), whereas larger cells with larger dendritic fields (type I and III) were slower to respond and less dramatically affected. Regrowth of the lesioned axons in peripheral nerve grafts and reconnection of the retina with various tissues did not result in a significant immediate recovery of ganglion cell dendrites, although it did prevent some axotomized cells from further progression toward posttraumatic cell death.     

Acetylcholinesterase-containing nerve cells and their distribution in the pineal organ of the goldfish,Carassius auratus

Summary Histochemically, an intense acetylcholinesterase (AChE) reaction has been observed in the perikarya of the nerve cells and in the neuropil formations of the pineal organ in the goldfish, Carassius auratus. A group of AChE-rich nerve cells has also been observed between the caudal end of the pineal stalk and the habenular ganglion. No component of the complex revealed butyrylcholinesterase (BuChE) activity.Two different types of nerve cells were recognized on the basis of their size, AChE activity and distribution. Type I cells are characterized by large perikarya possessing a moderate AChE activity and by the presence of an extensive AChE-rich neuropil formation in their vicinity; they are restricted to the rostro-lateral regions of the pineal vesicle. Type II cells are situated in the medio-rostral area of the pineal vesicle and along the entire length of the stalk, and are smaller than Type I cells; they show an intense AChE activity in their perikarya.The neuropil formations in the medio-rostral area of the pineal vesicle are almost as large as those in the vicinity of the Type I cells; they exhibit a strong AChE activity. In the rostral half of the vesicle several sensory cells are associated with each nerve cell, while in the caudal portion only a few cells are apposed to each nerve cell. Thus, the ratio of the number of sensory cells to that of AChE-containing nerve cells in the anterior half of the pineal vesicle is high when compared with the remaining area. In the anterior half of the vesicle the outer segments of the sensory cells are more distinct and their inner segments possess a higher AChE activity than those in the posterior region and the stalk. A gradation in the degree of development of neuropil formations along the pineal axis is remarkable; their size and AChE activity gradually diminish in a caudal direction. In view of the structural specialization of the rostral region of the pineal organ, it has been argued that its terminal portion is more photosensitive.This work was supported by a fellowship from the Alexander von Humboldt Foundation, Federal Republic of Germany.     

Nervous network in larvae of the ascidian Ciona intestinalis

 With the use of the monoclonal antibody UA301, which specifically recognizes the nervous system in ascidian larvae, the neuronal connections of the peripheral and central nervous systems in the ascidian Ciona intestinalis were observed. Three types of peripheral nervous system neurons were found: two located in the larval trunk and the other in the larval tail. These neurons were epidermal and their axons extended to the central nervous system and connected with the visceral ganglion directly or indirectly. The most rostral system (rostral trunk epidermal neurons, RTEN) was distributed bilateral-symmetrically. In addition, presumptive papillar neurons in palps were found which might be related to the RTEN. Another neuron group (apical trunk epidermal neurons, ATEN) was located in the apical part of the trunk. The caudal peripheral nervous system (caudal epidermal neurons, CEN) was located at the dorsal and ventral midline of the caudal epidermis. In the larval central nervous system, two major axon bundles were observed: one was of a photoreceptor complex and the other was connected with RTEN. These axon bundles joined in the posterior sensory vesicle, ran posteriorly through the visceral ganglion and branched into two caudal nerves which ran along the lateral walls of the caudal nerve tube. In addition, some immunopositive cells existed in the most proximal part of the caudal nerve tube and may be motoneurons. Received: 8 September 1997 / Accepted: 14 December 1997     

Immunohistochemical localization of gastrin-cholecystokinin-like material in the central nervous system of the migratory locust

Brain, corpora cardiaca (CC)-corpora allata (CA) complex, suboesophageal ganglion, thoracic and abdominal ganglia of adults, larvae and embryos of Locusta migratoria have been immunohistochemically screened for gastrin cholecystokinin (CCK-8(s]-like material. In adult, numerous immunoreactive neurons and nerve fibres are located, with a marked symmetry, in various parts of the brain and throughout the ventral nerve cord. In the median part of the brain, cell bodies belonging neither to cellular type A1 nor A2 (following Victoria blue-paraldehyde fuchsin staining) are immunopositive; their processes terminate in the upper protocerebral neuropile. In lateral parts of the brain, external cell bodies send axons into CC and some up to CA, other internal have processes which terminate in the neuropile of the brain. Two of these latter cells react also with methionine-enkephalin antiserum. In the ventral nerve cord, in addition to numerous perikarya, immunoreactive arborizations terminate in the neuropile or in close association with the sheath, at the dorsal part of all ganglia. This CCK-8(s) distribution pattern is observed only at the two last larval instars, but is precociously detected in the abdominal nerve cord of embryos, one day before hatching.     

Scanning electron microscope observations on the muscle innervation of Oikopleura dioica fol (appendicularia,tunicata) with notes on the arrangement of connective tissue fibres

Critical point dried and fractured appendicularia of the species Oikopleura dioica have been examined in the scanning electron microscope. The dorsal nerve cord with ganglion cells and peripheral nerve fibres could easily be observed. Thick peripheral nerve fibres leave the nerve cord as bilateral pairs at constant intervals along the tail. Most of these fibres branch from the naked nerve cord, but some evidently originate in ganglion perikarya bulging out from the nerve cord itself. These paired peripheral nerves always have elaborate end-arborizations on the medial surface of the lateral muscle cells. They are accordingly interpreted as motor axons. Some thinner peripheral nerve fibres originate at irregular intervals from both the nerve cord and the ganglion cells. Due to the numerous extracellular fibrils that connect the bilateral layers of the epidermal fins and the muscle cells to each other, these thin nerve fibres can seldom be traced to their termination. A few ones can, however, be traced ventrally between the notochord and the muscle cells and seem to end in singular bulb-like expansions. Clusters of synaptic vesicles are present in transmission electron micrographs of such nerves, and they are accordingly believed to carry efferent impulses. The extracellular fibrils are arranged in a highly ordered pattern with thick bundles crossing the gap between the structures to be interconnected and with numerous radiating insertions on the surface of the tissues.     

Loss of sensory elements in the apical sensory organ during metamorphosis in the nudibranch Phestilla sibogae

Larvae of the nudibranch Phestilla sibogae are induced to metamorphose by a water-borne chemical cue released by the adult nudibranch's prey, the coral Porites compressa. In competent larvae, the apical sensory organ (ASO) includes five serotonergic parampullary neurons; five ampullary neurons, the ampullae of which are filled with sensory cilia; and a basal neuropil. After sensing the coral cue, the ASO undergoes radical morphological changes: a deterioration of sensory elements in the ASO and serotonergic axons originating from them to innervate the velum. Three hours after metamorphic induction, the velar lobes are lost, the serotonergic axons begin to break apart, the five parampullary neurons begin to degenerate, and the five ampullary neurons retract away from the epidermal surface. The extent of deterioration evident by this time suggests that the parampullary and ampullary components of the ASO are no longer functional. By 10 h after metamorphic induction, labeling of the ciliary bundles in the ampullary neurons has disappeared, and it is likely that these cells have degenerated. The results presented here provide evidence that the sensory neurons of the ASO and probably the entire organ are solely larval structures that do not persist into the adult sensory-nervous system in P. sibogae.     

Characterization of metamorphic changes in anuran larval epidermis using lectins as probes

The skin of an adult frog of Xenopus laevis was characterized by the reactivity of 20 lectins. The lectins were classified into six groups in their binding to the epidermal cells: Lycopersicon esculentum lectin (LEL)-type which was positive for all epidermal cells; Pisum sativum agglutinin (PSA)-type for stratum germinativum; succinylated wheat germ agglutinin (sWGA)-type for strata spinosum, granulosum and corneum; Dolichos biflorus agglutinin (DBA)-type for strata germinativum and spinosum; peanut agglutinin (PNA)-type for stratum spinosum; and Ulex europaeus agglutinin (UEA-I)-type for strata granulosum and corneum. PSA and sWGA were utilized as markers of mitotically active germinative cells and the differentiated cells of the epidermis, respectively, to describe the metamorphic conversion of larval epidermal cells to adult type. PSA stained all epidermal cells of tadpoles before metamorphic climax. At the end of metamorphosis, PSA-positive cells were restricted to cells in the basal layer of body epidermis while all the tail epidermis remained PSA-positive. The other cell marker, sWGA, only stained apical cells in tadpole epidermis. During the metamorphic climax, sWGA-positive cells appeared in the cells beneath the stratum corneum of the body region, but not in the tail region. The present study demonstrates that PSA and sWGA are useful to investigate metamorphic changes in tadpole epidermal cells.     

Immunohistochemical localization of gastrin-cholecystokinin-like material in the central nervous system of the migratory locust

Summary Brain, corpora cardiaca (CC)-corpora allata (CA) complex, suboesophageal ganglion, thoracic and abdominal ganglia of adults, larvae and embryos of Locusta migratoria have been immunohistochemically screened for gastrin cholecystokinin (CCK-8(s))-like material. In adult, numerous immunoreactive neurons and nerve fibres are located, with a marked symmetry, in various parts of the brain and throughout the ventral nerve cord. In the median part of the brain, cell bodies belonging neither to cellular type A1 nor A2 (following Victoria blue-paraldehyde fuchsin staining) are immunopositive; their processes terminate in the upper protocerebral neuropile. In lateral parts of the brain, external cell bodies send axons into CC and some up to CA, other internal have processes which terminate in the neuropile of the brain. Two of these latter cells react also with methionine-enkephalin antiserum. In the ventral nerve cord, in addition to numerous perikarya, immunore-active arborizations terminate in the neuropile or in close association with the sheath, at the dorsal part of all ganglia.This CCK-8(s) distribution pattern is observed only at the two last larval instars, but is precociously detected in the abdominal nerve cord of embryos, one day before hatching.     

Development of Some Elements of the Peripheral Nervous System of the Locust Locusta migratoria during Larval Ontogenesis

Using supravital Methylene blue staining, development of elements of the peripheral nervous system was traced in the 1st–5th instar larvae of the locust Locusta migratoria L. Data were obtained on sensory cells of the I and II types in larvae of different instars, as well as on character of their changes in the course of larval development of the insect. The studied elements of the peripheral nervous system have been shown to be essentially transformed in the course of larval ontogenesis. The data are presented about the sensory cells of the proximal parts of the nerve trunks; they indicate that in the course of larvae development the cell number in these trunks near the ganglia of the nerve chain decreases, which might be due to their partial degeneration. With growth of muscle, changes in their sensory innervation take place. Subepithelial nerve plexus in larvae is largely represented in areas with hard and soft cuticles.     

Expression of arginine vasotocin receptors in the developing zebrafish CNS

Vasotocin/vasopressin is a neuropeptide that regulates social and reproductive behaviors in a variety of animals including fish. Arginine vasotocin (AVT) is expressed by cells in the ventral hypothalamic and preoptic areas in the diencephalon during embryogenesis in zebrafish suggesting that vasotocin might mediate other functions within the CNS prior to the development of social and reproductive behaviors. In order to examine potential early roles for vasotocin we cloned two zebrafish vasotocin receptors homologous to AVPR_1a. The receptors are expressed primarily in the CNS in similar but generally non-overlapping patterns. Both receptors are expressed in the forebrain, midbrain and hindbrain by larval stage. Of note, AVTR_1a-expressing neurons in the hindbrain appear to be contacted by the axons of preoptic neurons in the forebrain that include avt+ neurons and sensory axons in the lateral longitudinal fasciculus (LLF). Furthermore, AVTR_1a-expressing hindbrain neurons extend axons into the medial longitudinal fasciculus (MLF) that contains axons of many neurons thought to be involved in locomotor responses to sensory stimulation. One hypothesis consistent with this anatomy is that AVT signaling mediates or gates sensory input to motor circuits in the hindbrain and spinal cord.