Development and differentiation of the eye in Platynereis dumerilii (Annelida,Polychaeta)

The nereid polychaete, Platynereis dumerilii, possess two pairs of post-trochophoral eyes with one vitreous body each. The development of these eyes has first been observed in 2-day-old larvae. Whether the eye anlagen arise from stem cells or from undifferentiated ectodermal tissue was not determined. At first, the anlagen of the anterior and the posterior eyes adjoin each other. They separate in late 3-day-old larvae. The first separated eye complexes consist each of two supporting and two sensory cells. The supporting cells synthesize two different kinds of granules, the pigment granules of the pigment cup and the prospective tubules of the vitreous body. These tubules accumulate in the distal process of the supporting cell. The vitreous body is formed by compartments of the supporting cells filled with the osmiophilic vitreous body tubules. The short, bulbar photosensory processes bear microvilli that emerge into the ocular cavity. At the apex of each sensory cell process, a single cilium (or occasionally two) arises. The sensory cells contain a different kind of pigment granule within their necks at the level of the pigment cup. The rate of eye development and differentiation varies. New supporting cells are added to the rim of the eye cup. They contribute to the periphery of the vitreous body like onion skins, and sensory cells move between supporting cells. The older the individual compartments of the vitreous body are, the more densely packed is their content of vitreous body tubules. Elongation of the sensory and supporting cell processes of the older cells increases the volume of the eye. The eyespots of the trochophore are briefly described as of the two-celled rhabdomeric type with a single basal body with ciliary rootlet.     

Ultrastructure of the eye of the amber snail Succinea putris (L.) (Gastropoda, Stylommatophora)]

The structure and some aspects of the development of the eye of Succinea putris were studied with the aid of the electron microscope. The eye is of the closed vesicle type and is composed of retina, cornea, vitreous body, lens and optic nerve. Three different types of cell are to be found in the retina: (1) the small elongated pigment cell with an avoid nucleus, many pigment granulae and short microvilli at the apical end of the cell; (2) the sensory cell type I with a large irregular nucleus, long microvilli, which extend to under the surface of the lens, a large number of light-cored vesicles, 700 A in diameter and the axon; (3) the elongated slender sensory cell type II with many dense cored vesicles, several pigment granulae in the distal region of the cell and short irregular microvilli at the apical end of the cell. This type is few in number. Two results of the study of the embryonic eye are described: the cornea cells differ from those in the adult eye in the nucleus-cytoplasm relation and the optic nerve is smaller than in the adult eye.     

Adrenomedullin in the eye

Adrenomedullin (AM) is a multifunctional regulatory peptide that is produced and secreted by various types of cells. We showed the presence of high concentrations of adrenomedullin-immunoreactivity in the vitreous fluid, and the levels were elevated in patients with proliferative vitreoretinopathy. Furthermore, adrenomedullin mRNA expression levels were elevated in the tissues of intraocular tumors and orbital tumors. Adrenomedullin is produced and secreted by cultured human retinal pigment epithelial (RPE) cells. Inflammatory cytokines and hypoxia are strong stimulators for the adrenomedullin expression in retinal pigment epithelial cells. Adrenomedullin stimulated the proliferation of retinal pigment epithelial cells both under normoxia and hypoxia. Dexamethasone (DEX) increased the adrenomedullin expression in two cultured cell lines of human retinal pigment epithelial cells; ARPE-19 cells and D407 cells, while it had no noticeable effects on the cytokine-induced adrenomedullin expression. These findings suggest that adrenomedullin is involved in the pathophysiology of inflammatory and neoplastic eye diseases as an autocrine or paracrine growth stimulator. The findings on glucocorticoid-induced AM expression raise the possibility that it may be related to the pathogenesis of some eye diseases, such as central serous chorioretinopathy and multifocal posterior pigment epitheliopathy, which are frequently seen in patients treated with high doses of glucocorticoids.     

Down-regulation of pigment epithelium-derived factor in uveitic lesion associates with focal vascular endothelial growth factor expression and breakdown of the blood-retinal barrier

Spontaneous equine recurrent uveitis (ERU) is an incurable autoimmune disease affecting the eye. Identifying biological markers or pathways associated with this disease may allow the understanding of its pathogenesis at a molecular level. The vitreous is the body fluid closest to the disease-affected tissue and possibly also an effector of pathological processes relevant for ERU. Surgical removal of vitreous leads to cessation of relapses in spontaneous uveitis of both man and horse, therefore vitreous composites are likely to contribute to disease progression. Uveitic vitreous is likely to contain potential biomarkers in relatively undiluted quantities. With the goal to identify these markers, we systematically compared vitreous from healthy and disease-affected eyes by proteomic profiling. Nine differentially expressed proteins were identified, that are functionally related to immune response, inflammation, and maintenance of the blood-retinal barrier. One of these, pigment epithelium-derived factor, a protein involved in maintaining a proper blood-retina barrier as well as protecting from neoangiogenesis was additionally found to be down-regulated within uveitic retinal lesions whereas, conversely, vascular endothelial growth factor was found to be up-regulated at these sites. Together, these changes point to as of yet undiscovered biological pathways involved in the pathogenesis of this autoimmune disease.     

Mutations in KCNJ13 cause autosomal-dominant snowflake vitreoretinal degeneration

Snowflake vitreoretinal degeneration (SVD, MIM 193230) is a developmental and progressive hereditary eye disorder that affects multiple tissues within the eye. Diagnostic features of SVD include fibrillar degeneration of the vitreous humor, early-onset cataract, minute crystalline deposits in the neurosensory retina, and retinal detachment. A genome-wide scan previously localized the genetic locus for SVD to a 20 Mb region flanked by D2S2158 and D2S2202. This region contains 59 genes, of which 20 were sequenced, disclosing a heterozygous mutation (484C > T, R162W) in KCNJ13, member 13 of subfamily J of the potassium inwardly rectifying channel family in all affected individuals. The mutation in KCNJ13, the gene encoding Kir7.1, was not present in unaffected family members and 210 control individuals. Kir7.1 localized to human retina and retinal pigment epithelium and was especially prevalent in the internal limiting membrane adjacent to the vitreous body. Molecular modeling of this mutation predicted disruption of the structure of the potassium channel in the closed state located immediately adjacent to the cell-membrane inner boundary. Functionally, unlike wild-type Kir7.1 whose overexpression in CHO-K1 cells line produces highly selective potassium current, overexpression of R162W mutant Kir7.1 produces a nonselective cation current that depolarizes transfected cells and increases their fragility. These results indicate that the KCNJ13 R162W mutation can cause SVD and further show that vitreoretinal degeneration can arise through mutations in genes whose products are not structural components of the vitreous.     

Vitreous body collagen. Evidence for a dual origin from the neural retina and hyalocytes

Two different cells types have been shown to synthesize embryonic chick vitreous collagen (vitrosin) at different stages of development. Identification of vitrosin was established by labeling the embryos in ovo [3H]proline at stages 23 and 28 and separating the extracted vitreous collagen alpha-chains by carboxymethylcellulose chromatography. The labeled collagen consisted predominately of alpha 1 chains, indicating a molecule in the form of a trimer of identical chains designated (alpha 1)3. The molecular weight of the labeled chains measured approximately 95,000 daltons by molecular sieve chromatography, and contained 41% of their imino acid as 4- hydroxyproline. To establish which eye tissues synthesize vitrosine, the collagens produced in organ culture by the isolated neural retina, lens and vitreous body from stages 26-27, 29-30, and 40 were examined. At the two earlier stages, only the neural retina synthesized large quantities of (alpha 1)3 collagen whereas the lens and the cells within the vitreous body itself synthesized relatively small amounts of collagen characterized by an alpha 1:alpha 2 ratio of about 2:1. At stage 40, however, the cells of the vitreous body itself synthesized the greatest quantities of collagen, which now was predominantly an (alpha 1)3 type molecule. Stage 40 neural retina and lens synthesized lesser amounts of collagen with an alpha 1:alpha 2 ratio of 2 to 3:1. Chick vitrosin thus appears to be synthesized by the neural retina in early embryonic stages, whereas the major contribution derives from cells within the vitreous body in later development.     

Vitreous-induced cytoskeletal rearrangements via the Rac1 GTPase-dependent signaling pathway in human retinal pigment epithelial cells

Proliferative vitreoretinopathy (PVR) is mainly caused by retinal pigment epithelial (RPE) cell migration, invasion, proliferation and transformation into fibroblast-like cells that produce the extracellular matrix (ECM). The vitreous humor is known to play an important role in PVR. An epithelial-to-mesenchymal transdifferentiation (EMT) of human RPE cells induced by 25% vitreous treatment has been linked to stimulation of the mesenchymal phenotype, migration and invasion. Here, we characterized the effects of the vitreous on the cell morphology and cytoskeleton in human RPE cells. The signaling pathway that mediates these effects was investigated. Serum-starved RPE cells were incubated with 25% vitreous, and the morphological changes were examined by phase-contrast microscopy. Filamentous actin (F-actin) was examined by immunofluorescence and confocal microscopy. Protein phosphorylation of AKT, ERK1/2, Smad2/3, LIM kinase (LIMK) 1 and cofilin was analyzed by Western blot analysis. Vitreous treatment induced cytoskeletal rearrangements, activated Rac1 and enhanced the phosphorylation of AKT, ERK1/2 and Smad2/3. When the cells were treated with a Rac activation-specific inhibitor, the cytoskeletal rearrangements were prevented, and the phosphorylation of Smad2/3 was blocked. Vitreous treatment also enhanced the phosphorylation of LIMK1 and cofilin and the Rac inhibitor blocked this effect. We propose that vitreous-transformed human RPE cells undergo cytoskeletal rearrangements via Rac1 GTPase-dependent pathways that modulate LIMK1 and cofilin activity. The TGFβ-like activity of the vitreous may participate in this effect. Actin polymerization causes the cytoskeletal rearrangements that lead to the plasticity of vitreous-transformed RPE cells in PVR.     

Structure of the visual system of the two-spotted spider-mite, Tetranychus urticae

The pair of eyes on each side of Tetranychus urticae consists of fifteen retinular cells, six pigment cells, six corneal cells, and one vitreous cell. Five rhabdomeres lie beneath the anterior lens, twelve beneath the posterior lens. The pigment and corneal cells appear to determine the positions at which rhabdomeres occur. The volumes of all rhabdomeres have been measured. A pair of fibrous masses are associated with tendons at the dorsal apodemes; the nerves of these ‘apodemal organs’ join the optic nerves en route to the brain. There are a pair of optic neuropiles, each surmounted by a large secretory cell.     

Ultrastructure of the vitreous body of the rabbit

Examination in the scanning and the transmission electron microscope showed three morphologically and structurally different types of cells in the vitreous body of the healthy rabbit eye: 1. cells with numerous cytoplasm processes, whose high metabolic activity is represented by the presence of a large number of organelles and which are capable of synthesizing fibrillar material; 2. elongate cells with a flattened nucleus, with long, narrow cytoplasm processes arising from both their poles and with only a few organelles in their cytoplasm; 3. large spherical cells with structureless contents, whose nucleus and few organelles are situated below the cell membrane. The organized component of the intercellular matter of the rabbit vitreous body is composed of collagen fibrils with a very variable diameter (24-180 nm), The collagen fibrils form the basis of the three-dimensional skeleton of the intercellular matter of the vitreous body.     

Über den Bau und die Hell-Dunkel-Adaptation der Augen des Polychäten Platynereis dumerilii

Summary The eye of Platynereis dumerilii consists of three components: a short optic nerve, a cup-shaped retina, and a vitreous body within the cup. The opening of the retinal cup is called pupil. The retina is composed of supporting cells and visual cells. The supporting cells are stuffed with dark blue violet pigment granules. The visual cells have orange pigment granules which are only found in the narrow middle piece of the cells. The supporting cell pigment may be lacking in abnormally pigmented eyes. The jellylike matter of the vitreous body apparently is produced by the supporting cells. It is of high protein contents and does not seem to be derived from the cuticle which consists of polysaccharides.The ultrastructure of the photoreceptor region shows club-shaped processes of visual cells. Each club is of low electron density and contains elongate membranous structures. It is surrounded by many microvilli. The clubs correspond to the rods in light microscopy.The eye of Platynereis dumerilii adapts to changes in light intensity by movements of the retina and the rods. The cup-shaped retina spreads towards its pupillar opening thus adapting the pupil area to light intensity. The length of the rods in darkfixed immature specimens is about 20, in light-fixed ones about 7 . In mature specimens (Heteronereis) the length is 46 or 19 respectively.During metamorphosis the eyes enlarge to about three times their original volume. This enlargement is due to an increase in volume of the retina and the vitreous body, not to cell divisions.

---

---

Durchgeführt mit Unterstützung durch ein Stipendium aus Mitteln der Fritz-Thyssen-Stiftung, ferner mit Hilfe der Deutschen Forschungsgemeinschaft.

---

Die Anregung zu dieser Arbeit und das Platynereis-Zuchtmaterial verdanke ich Herrn Prof. Dr. C. Hauenschild. Für Hilfe bei der Herstellung des Bildmaterials danke ich Frl. U. Poltz (Freiburg).     

Phosphorylation of small molecular weight polypeptides in the iris-ciliary complex, aqueous humor and vitreous humor

The polypeptides of vitreous humor, aqueous humor and iris-ciliary complex cells of eyes were phosphorylated with [gamma-32P]ATP without exogenous protein kinase. Phosphorylated polypeptides were analyzed by sodium dodecyl sulfate gel electrophoresis and autoradiography. The phosphorylated polypeptides of rabbit vitreous humor showed many high molecular weight prominent bands, but no detectable phosphoproteins were found in the 12 kDa or lower range. Bovine vitreous humor has predominantly acidic polypeptides and some of them are below 20 kDa. Rabbit and bovine iris-ciliary complex and rabbit aqueous humor showed a prominent common 4 kDa phosphopolypeptide which could also be synthesized by cloned populations of cells from the bovine iris and the rabbit iris-ciliary body. It is possible that the 4 kDa phosphopolypeptide of the aqueous humor is synthesized by the iris-ciliary complex cells.     

Method of determining the colloidal status of the vitreous body

A new method for the quantitative estimation of the vitreous body colloidal state has been suggested. For realization of the method a fragment of the vitreous body and an equal volume of water are dried out, and the drying time is registered. The higher is the ratio between the drying time of the vitreous body fragment and water, the higher is the density of the vitreous body gel. The drying out of the vitreous body fragment and water on the analytical balance cups permits the registration of the drying out process in the time course. Thus some additional parameters are obtained that characterize the object studied more completely. The method can be used in experimental and clinical investigations of the vitreous body and other biological liquids.     

The eyes of a “nobody”,Anoplodactylus petiolatus (Pantopoda; Anoplodactylidae)

The fine structure of the four ocelli ofAnoplodactylus petiolatus was examined using serial longitudinal and transversal sections of the eye hill. Each pigment cup ocellus is composed of a (planconvex) cuticular lens, lens forming hypodermal cells, inverse retinula cells with latticed rhabdom and surrounding tapetum and pigment layers. Within the retinula cells a distal “vitreous” zone, a nucleus zone and a proximal rhabdomeric zone can be distinguished. Retinula cell axons originate proximally. The tapetum cells contain several layers of reflecting crystals. Distally, they have a common microvillous region. The intraretinal “vitreous” zone contains glycogen-like particles in the centre and rough ER in the periphery. Contrary to other Pantopoda vitreous cells, a praeretinal membrane and a vertical lens groove have not been observed inAnoplodactylus. While the presence of four (median) ocelli appears to be a primitive characteristic, the inverse orientation of the retinula cells in combination with a tapetum lucidum represents a highly derived characteristic among arthropod median eyes.     

Development of pigment in the echiuran worm Bonellia viridis

An account is given of the development of green pigment in the early larval stages of the echiuran worm, Bonellia viridis . The green pigment first appears in scattered epidermal cells of the gastrula, before the development of the trochal rings. It is contained in spherical vacuoles (0.5-1.0 μm in diameter). As the gastrula develops into the trochophore there is an increase in total pigment content, as well as an increase in number of pigment cells and size of pigment vacuoles. The increase in pigment cell number in the trochophore results from the proliferation of the pigment cells of the gastrula. The pigment content increases rapidly before the trochophores hatch but shows little relative increase after hatching whilst the trochophores remain undifferentiated. We suggest that the pigment may have a protective role in the free-living trochophore for camouflage or chemical defence. In trochophores that undergo male differentiation the pigmentation is lost. Since the males do not lead a free-living existence but live as commensals inside the uterus of the female camouflage or chemical defence would be unnecessary. In trochophores undergoing female differentiation there is an increase in pigment content of the preoral lobe which develops into the proboscis. Following the enlargement of the coelom, clusters of coelomic cells accumulate green pigment whilst still in the coelom and then migrate to the integument of the body wall.     

Synthesis and migration of 3H-fucose-labeled glycoproteins in the retinal pigment epithelium of albino rats, as visualized by radioautography

3H-fucose was injected into the vitreous body of the eye(s) of 250-gm rats, which were then killed by means of an intracardiac perfusion with glutaraldehyde after intervals of 10 min, 1 and 4 hr, and 1 and 7 days. The eyes were removed and further fixed, and pieces of retina were processed for light and electron microscope radioautography. Light microscope radioautography showed that the pigment epithelial cells actively incorporated 3H-fucose label. The intensity of reaction peaked at 4 hr after injection of the label and then slowly declined. Quantitative electron microscope radioautography revealed that, at 10 min after 3H-fucose injection, over 70% of the label was localized to the Golgi apparatus, indicating that fucose residues are added to newly synthesized glycoproteins principally at this site. With time the proportion of label associated with the Golgi apparatus decreased, but that assigned to the infolded basal plasma membrane, the apical microvilli, and various apical lysosomes increased. These results indicate that in retinal pigment epithelial cells newly synthesized glycoproteins continuously migrate from the Golgi apparatus to lysosomes and to various regions of the plasma membrane. In this case, the membrane glycoproteins may play specific roles in receptor functions of the basal plasma membrane or phagocytic activities at the apical surface. Very little label migrated to Bruch's membrane, indicating either a very slow turnover or a paucity of fucose-containing glycoproteins at this site.     

The fine structure of the pigment body complex in the intrapigmented aesthetes of Callochiton achatinus (Mollusca: Polyplacophora)

The detailed ultrastructure of the pigment body complex located on the dorsal surface of each intrapigmented megalaesthete in the valves of Callochiton achatinus (Brown, 1827) is described. The pigment body complex comprises a single, large rhabdomer, surrounded by a number of pigment cells, linked to an adjacent myeloid body which characteristically consists of an area of extensive, complex, lamellate whorls consisting of myelin. The rhabdomer probably has no specific visual function. However, the simultaneous contraction of the myeloid body and the increased pigmentation of the cells surrounding the rhabdomer after long-term exposure to light suggests that the myeloid body is involved in a mechanism controlling pigment movement which would modify the amount of light penetrating the rhabdomer.     

豹纹鳃棘鲈体色变异的色素细胞差异分析

为了揭示豹纹鳃棘鲈(Plectropomus leopardus)体色变异机制,研究选取了不同体色个体的样本,利用石蜡切片、冰冻切片及体视显微镜观察等方法揭示不同皮肤部位色素细胞的类型、分布和数量的差异,并对应激和非应激状态下色素细胞的变化进行了研究。结果显示,黑色素细胞在背部和尾部分布比较密集,在腹部较为稀疏,黑色个体的黑色素细胞数量较红色个体多;在应激状态下个体能迅速发生体色变化,主要由于色素细胞快速扩张和收缩导致。研究为进一步揭示豹纹鳃棘鲈体色变异的分子机制和优良品种选育奠定了基础。     

Interneurones of the central complex in the bee brain (Apis mellifera,L.)

The response characteristics of 46 interneurones of the central complex in the bee brain to visual, various antennal and mechanical stimuli were studied. Different types of neurones can be distinguished anatomically. Intrinsic cells arborize only in the central complex. Segmental neurones innervate a segment of the protocerebral bridge and the central body and project to the lateral accessory lobes. Fan-shaped neurones have arborizations throughout the whole upper or lower division of the central body.Intrinsic neurones of the protocerebral bridge process visual information, the other cells display different and often multimodal response characteristics, which cannot be correlated with the neuroanatomical groups. Seventeen per cent of the cells did not respond at all to the stimuli presented. The role of the central complex in the processing of sensory information is discussed and compared with the mushroom bodies and the diffuse protocerebral lobes.     

Neuronal types in the striatum of man

Summary Nerve cells of the human striatum were investigated with the use of a newly developed technique that reveals the pattern of pigmentation of individual nerve cells by means of transparent Golgi impregnations of their cell bodies and processes. Five types of neurons are distinguished:Type I is a medium-sized spine-laden neuron with an axon giving off a great number of collateral branches. The vast majority of the cells in the striatum belong to this type. Numerous intensely stained lipofuscin granules are contained in one pole of the cell body and may also extend into adjacent portions of a dendrite.Type II is a medium-sized to large neuron with long intertwining dendrites decorated with spines of uncommon shape. A distinguishing feature of this cell type is the presence of somal spines. This cell type is devoid of pigment or contains only a few tiny lipofuscin granules.Type III is a large multipolar neuron. The cell body generates a few rather extended dendrites that are very sparsely spined. The finely granulated pigment is evenly dispersed within a large portion of the cytoplasm.Type IV is a large aspiny neuron with rounded cell body and richly branching tortuous dendrites. The axon branches frequently in the vicinity of the parent soma. Large pigment granules are concentrated within a circumscribed part of the cell body close to the cell membrane.Type V is a small to medium-sized aspiny neuron. The dendrites break up into a swirling mass of thin branches. More than one axon may be given off from the soma. The axons branch close to the soma into terminal twigs. Cells of this type contain numerous large and well-stained lipofuscin granules.Each of the cell types has a characteristic pattern of pigmentation. The different varieties of nerve cells in the striatum can therefore be distinguished not only in Golgi impregnations but also in pigment-Nissl preparations.     

Evidence of lipofuscin and melanin in the brown body of the earthworm Eisenia fetida andrei

By means of histochemical and electron-microscopic techniques, two pigments were identified in the brown body of the earthworm Eisenia fetida andrei. Lipofuscin, often called the aging pigment, was the more abundant pigment and the first to be synthesized. Melanin was also found but was only present in the mature brown body. A computer-assisted image analysis was used to quantify the relative abundance of the two pigments at different stages of the formation of the brown body. A previous study showing phenoloxidase activity in the coelomocytes and the present demonstration of the ability of these cells to produce reactive oxygen systems when agglutinated can be correlated with the simultaneous presence of the two pigments in the brown body. The physiological significance of pigment synthesis by brown bodies is discussed with respect to the immune response in earthworms.