Fine structure of the photosensitive iris of the toad, Bufo marinus

The iris of the toad Bufo marinus is directly photosensitive and will constrict in response to light striking only the iris. This is true even when the iris is isolated from the rest of the eye, and therefore from reflex neuronal influences initiated in the retina. This autonomous response is probably mediated by the sphincter pupillae muscle, since no specialized photoreceptors are present in the iris, nor does the sphincter exhibit any specializations likely to subserve a purely photoreceptive function. The photosensitive sphincter appears typical of smooth muscle and, like mammalian sphincters, possesses many intercellular junctions. The iris possesses a well-developed neuronal plexus with fibers projecting into the sphincter muscle layer. Nerve terminals contain small, agranular (30-70nm) and large, dense-cored (80-120nm) vesicles. No consistent postsynaptic specializations are seen on any cells of the iris, including the cells of the sphincter muscle. The anterior pigment epithelial cells of the iris appear specialized and resemble the myoepithelial dilator muscle described by Kelly and Arnold ('72) for the iris of rats.     

A quantitative model of myosin phosphorylation and the photomechanical response of the isolated sphincter pupillae of the frog iris.

The time courses of isometrically recorded photomechanical responses of isolated sphincter pupillae of Rana pipiens can be accurately predicted by a set of differential equations derived from phosphorylation theory of smooth muscle contraction. We compared actual light-stimulated contractions with calculated ones over a wide range of stimulus intensities (56-fold) and durations (0.4-4.0 s). The hypothetical Ca++-calmodulin-myosin light chain kinase cascade acts as a "valve" to control the flow of ATP through a phosphorylation-dephosphorylation cycle. When the rate of flow of ATP through the phosphorylation-dephosphorylation cycle is increased, the percentage of phosphorylated myosin increases. The time courses of the concentrations of phosphorylated myosin during different responses are seen to be functions of the time courses of the opening and closing of the coupling cascade "valve." The calculations predict experimentally measurable intermediate variables, which can aid the investigation of the application of quantitative phosphorylation theory to amphibian sphincter pupillae and to smooth muscle in general.     

Projection of statocyst sensory neurons associated with crescent hairs in the crayfish Procambarus clarkii Girard

Summary Both smooth muscle and striated muscle are present in the iris of the chick embryo. The two types of musculature form mixed clusters which include undifferentiated cells and many nerve fibres, but they are structurally quite distinct and have different origins. The smooth musculature originates around the 10th day from a laminar invagination (iridial lamella) of the posterior epithelium, and is therefore an ectodermal derivative. The striated musculature appears slightly later than the smooth musculature and originates from undifferentiated cells which are regarded as mesenchymal. After the 15th day in ovo the smooth musculature stops growing; its cells become confined to an area very near the pupillary margin and many develop pigment granules in the sarcoplasm. Many smooth muscle cells seem to undergo regressive changes; however, cells with the typical appearance of visceral muscle cells are still present in the iris of 3-month-old chickens. High density of innervation and vasculari/ation, wide range of striated muscle fibre diameters, presence of lipid vacuoles and of large clusters of mitochondria in the striated fibres, occurrence of peripheral couplings of the sarcoplasmic reticulum, and presence of numerous fibroblast processes in the interstices between fibres, characterize the sphincter pupillae of the mature iris.This work was supported by grants from the Medical Research Council and the Central Research Fund of the University of London     

Freeze-fracture studies of nexuses between smooth muscle cells. Close relationship to sarcoplasmic reticulum

The freeze-fracture appearance of the nexus was compared in the smooth muscle of guinea pig sphincter pupillac, portal vein, pulmonary artery, taenia coli, uretzr, and vas diferens, mouse vas deferens, chicken gizzard and anterior mesenteric artery, and toad stomach. Nexuses are particularly numerous in the guinea pig sphincter pupillae; they are usually oval and their average area is 0.15 mum2, although some as large as 0.6 mum2 were seen. Small aggregations of particles were observed which would not be recognizable as nexuses in thin section. What constitutes the minimum size of a nexus is discussed. It is estimated that the number of nexuses per cell in this preparation is of the order of tens rather than hundreds. All nexuses examined had 6-9-nm particles in the PF face, with corresponding 3-4-nm pits on the EF face forming a polygonal tending towards a hexagonal lattice. The nexuses are arranged in rows parallel to the main axis of the cell, usually alternating with longitudinal rows of plasmalemmal vesicles. Many nexuses in the guinea pig sphincter pupillae, chicken gizzard, and toad stomach show a close relationship with sarcoplasmic reticulum. The possibility that this may have some role in current flow across this specialized junction is discussed.     

Morphology of the canine pyloric sphincter in relation to function

The ultrastructure and immunocytochemistry of the canine distal pyloric muscle loop, the pyloric sphincter, were studied. Cells in this muscle were connected by gap junctions, fewer than in the antrum or corpus. The sphincter had a dense innervation and a sparse population of interstitial cells of Cajal. Most such cells were of the circular muscle type but a few were of the type in the myenteric plexus. Nerves were sometimes associated with interstitial cell profiles, but most nerves were neither close to nor associated with interstitial cells nor close to smooth muscle cells. Nerve profiles were characterized by an unusually high proportion of varicosities with a majority or a high proportion of large granular vesicles. Many of these were shown to contain material immunoreactive for vasoactive intestinal polypeptide (VIP) and some had substance P (SP) immunoreactive material. All were presumed to be peptidergic. VIP was present in a higher concentration in this muscle than in adjacent antral or duodenal circular muscle. Interstitial cells of Cajal made gap junctions to smooth muscle and to one another and might provide myogenic pacemaking activity for this muscle, but there was no evidence of a close or special relationship between nerves with VIP or SP and these cells. The absence of close relationships between nerves and either interstitial cells or smooth muscle cells leaves unanswered questions about the structural basis for previous observations of discrete excitatory responses or pyloric sphincter to single stimuli or nerves up to one per second. In conclusion, the structural observations suggest that this muscle has special neural and myogenic control systems and that interstitial cells may function to control myogenic activity of this muscle but not to mediate neural signals.     

Distribution of opioidergic,sympathetic and neuropeptide Y-positive nerves in the sphincter of Oddi and biliary tree of the monkey,Macaca fascicularis

Summary The opioidergic, sympathetic and neuropeptide Y-positive innervation of the sphincter of Oddi (common bile duct sphincter and pancreatic duct sphincter), as well as other segments of the extrahepatic biliary tree was studied in the monkey by use of immunohistochemistry. Methionine-enkephalin-positive nerves were seen to innervate the smooth muscle of all portions of the sphincter of Oddi and also local ganglion cells. No methionine-enkephalin-positive nerves could be detected in the common bile duct, pancreatic duct or gallbladder. Tyrosine hydroxylase-positive nerves occurred between smooth muscle bundles and also ran to local ganglion cells as well as along the common bile duct. Neuropeptide Y-positive nerves were observed within smooth muscle of the sphincter of Oddi (all portions), common bile duct, pancreatic duct and gallbladder. No evidence of any differential innervation of the pancreatic duct and common bile duct sphincters could be detected with these markers.     

Substance P-immunoreactive nerve fibres in the anterior segment of the rabbit eye

Summary Substance P-immunoreactive nerve terminals were found in several locations in the anterior segment of the rabbit eye. In the iris they occurred in the sphincter muscle and were randomly distributed in the iris stroma with some fibres running close to the dilator muscle. In the ciliary body these immunoreactive elements were few and occurred within bundles of nerve fibres, while in the ciliary processes they were more numerous with a predominantly subepithelial location. Blood vessels in the anterior uvea were often surrounded by substance P-immunoreactive fibres. No substance P-fibres were found in the cornea, while the sclera contained very few such elements.Using conventional in vitro techniques it was found that the sphincter pupillae muscle of the iris responded to electrical stimulation with a contraction that was resistant to cholinergic and adrenergic blockade, but was inhibited by the neuronal blocker tetrodotoxin. This indicates the existence of a non-cholinergic, non-adrenergic neuronal mediator of the contractile response. Exogenously applied substance P produced a long-lasting contraction of the spincter muscle, an observation compatible with the view that substance P is the noncholinergic, non-adrenergic neurotransmitter involved.     

Electron microscopic observations on the innervation of the sphincter of oddi in the dog

The ultrastructure and acetylcholinesterase activity of the intrinsic innervation of the sphincter of Oddi of eight adult dogs was studied by electron microscopy. A rich distribution of unmyelinated axons embedded individually or as groups within Schwann cell cytoplasm ("innervation fasciculee"), is to be observed. A few myelinated fibres were also observed. Many of the axons are acetylcholinesterase-positive. Three main types of nerve terminals are distinguished according to their vesicle populations. Individual nerve cells or small groups of nerve cells were scattered between the smooth muscle bundles and in the lamina glandularis mucosae. The cytoplasm of some neurons contains many electron dense spherical bodies resembling "myeloid bodies", and many lysosomes. Nerve terminals synapse onto both neuronal perikarya and their dendrites. Within the nerve fascicles, close appositions between the terminals occur frequently probably representing the most peripheral inter-neuronal integrative link in the neural regulation of the function of the sphincter of Oddi. -- The gap between nerve terminals and smooth muscle cells usually measures several thousands of A. Closer appositions are seldom seen, and no synaptic complexes can be observed.     

A new concept of the anatomy of the anal sphincter mechanism and the physiology of defecation. The involuntary action of the external anal sphincter: histologic study.

The histologic changes in the external anal sphincter after internal anal sphincter excision were studied in 20 dogs. An external sphincter biopsy was taken before internal sphincterectomy and 2 weeks and monthly thereafter for 10 months. The excised material was studied microscopically after being stained with hematoxylin and eosin, Verhoeff-van Gieson and succinic dehydrogenase. 70% of external sphincter specimens before internal sphincter excision showed smooth muscle fibers scattered between the striated fibers. These smooth fibers could be responsible for the resting tone of the external sphincter. After internal sphincter excision, characteristic histologic changes could be identified in the external sphincter. From the 2nd week to the 5th month after excision, the external sphincter showed degenerative and hypertrophic changes. From the 6th to the 10th month, there were regeneration of the striated muscle fibers and increase in the number of smooth fibers so that by the 10th month a 'compound' muscle of striated and smooth fibers was identified. Two theories were put forward to explain the smooth fiber preponderance in the external sphincter after internal sphincter excision: mutant and replacement theories. The increased nonstriated element in the external sphincter seems to be a structural-functional adaptation so that the external sphincter takes on the involuntary function of the excised muscle.     

Quantitative Beziehungen zwischen Lichtreiz und Kontraktion des Musculus sphincter pupillae vom Scheibenzüngler (Discoglossus pictus)

Summary The Musculus sphincter pupillae of the toad Discoglossus pictus contracts when exposed to light, even if the iris with the muscle is cut out of the eye. Normally the size of the pupil is controlled by this photosensitivity and in addition by a nervous control mechanism. —Experiments are discribed in which the M. sphincter pupillae of the isolated iris was stimulated by various light programs. The contractile force was measured isometrically with a compensation system. It is shown that the response of the sphincter-muscle to changing light stimuli depends on the mean light intensity; i.e. the sphincter-muscle is an adapting system. The amplitude and phaseshift of the reactions to sinusoidal light stimuli were measured. When stimulus and response are both considered as functions of time, the transformation of stimulus in response by the muscle is linear, provided that the frequency of the sinusoidal light is high and its intensity and modulation degree are low. From this result the hypothesis is derived, that the transformation of stimulus into response is linear only when the level of adaptation does not change during contraction. From the response to sinusoidal light program it was possible to predict the reaction to square wave light programs. The time-course of the reaction to step up light stimuli are similar to the time-course of receptor potentials of phasic-tonic sense cells, showing a maximum, a minimum and a plateau. Within certain limits the amplitude of the reaction depends linearly on the tension of the muscle. Since in isometric experiments the reaction consists of an increase of muscle tension, the muscle becomes more sensitive during reaction and the contractile force increases for a long time, even when light intensity is held constant.     

The sphincter of the efferent filament artery in teleost gills: I. Structure and parasympathetic innervation

Previous studies have shown the existence of a sphincter in the efferent filament artery of the teleost gill and its constrictory response to acetylcholine (ACH) and vagal stimulation. This study deals with the muscular organization of this sphincter and the distribution of its innervation as elucidated by degeneration methods and cytochemistry. The sphincter innervation is supplied by the protrematic vagus nerves. Nerve endings filled with cholinergic-type vesicles are located in close association with the adventitial smooth muscle cells and display a strong acetylcholinesterase (ACHE) activity. Section of the protrematic vagus nerve induces a nearly complete degeneration of the sphincter innervation. ACHE-positive nerve cell bodies are present both in the sphincter area and in the protrematic vagus nerve. These results suggest that innervation of the sphincter in the efferent filament artery is cholinergic through the activity of postganglionic axons of the parasympathetic system.     

Direct Action of Light in Naturally Pigmented Muscle Fibers : I. Action spectrum for contraction in eel iris sphincter

Contraction due to light in excised eel irises appears to follow a simple first order law. The action spectrum for contraction has a maximum which agrees with the eel rhodopsin absorption maximum. Inasmuch as rhodopsin is the rod pigment-opsin complex and the iris sphincter pupillae evolves from the pigment epithelium of the retina in the region of the iris, the muscle pigment might be the same as the visual pigment. In the human eye the contraction of the iris sphincter is activated only by light incident on the retina and the pupil diameter varies inversely with the square root of the light intensity. The inverse first power relation observed in the present experiments suggests a more primitive origin for the light reaction in eel irises. Relaxation is a much slower process and can be approximated as the sum of two first order processes.     

Untersuchungen über Feinstruktur und Innervation der inneren Augenmuskulatur des Huhnes

Zusammenfassung Die innere Augenmuskulatur des Huhnes besteht ausschließlich aus sehr kurzen, dünnen quergestreiften Muskelfasern, die einfach innerviert sind. Die Fasern des M.ciliaris sind 280–1700 m lang. Die Irismuskelfasern sind stark verzweigt und zu einem dreidimensionalen Netz zusammengefügt. Die Verbindung der einzelnen Fasern erfolgt entweder durch Zwischensehnen, die aus ungewöhnlich dicken (3000–4000 Å) kollagenen Fibrillen und einer elektronendichten, amorph erscheinenden Zwischensubstanz bestehen, oder nur durch basalmembranartiges Material, das Cholinesteraseaktivität zeigt.Der überwiegende Teil des dreidimensionalen Faserwerks der Irismuskulatur folgt einer circulären Grundanordnung (M. sphincter pupillae), nur ein kleiner Teil der Fasern zeigt eine radiäre Vorzugsrichtung (M. dilatator pupillae).Das Sarkoplasma der inneren Augenmuskulatur enthält sehr viele Mitochondrien (bis zu 12% des Gesamtquerschnittes), zumeist auch zahlreiche Triglyceridtröpfchen und Glykogen-Granula. Im reich entwickelten sarkoplasmatischen Retikulum ist eine große Zahl von Triaden erkennbar, die bei den Mm. ciliaris und sphincter pupillae meist regelmäßig nahe der A-I-Grenze im A-Band-Bereich liegen, beim M. dilatator pupillae meist unregelmäßig über das ganze A-Band verstreut sind.Das Querstreifungsmuster läßt deutlich ein M-Band, schwer nur eine Pseudo-H-Zone erkennen. Der Z-Streifen ist mit 1200–1600 Å auffallend breit und zeigt einen unregelmäßigen Verlauf. Die Sarkomere einer Faser können verschiedene Größen zeigen, die beiden I-Band-Hälften ein und desselben Sarkomers verschieden breit sein.Die periphere motorische Nervenbahn besteht aus 2 Neuronen. Das im Ganglion ciliare beginnende periphere Neuron besitzt eine Markscheide und endet an motorischen Endplatten der inneren Augenmuskelfasern. Einem Neuron können etwa 4 Muskelfasern zugeordnet werden. Die motorischen Endplatten sind groß; die Relative Innervationsgröße m² synaptischer Fläche/1,000.000 m³ Muskelfaservolumen) zeigt den ganz außergewöhnlichen Wert von 10.000. Die synaptische Membran ist faltenfrei, das terminale Axoplasma enthält neben zahlreichen normalen synaptischen Bläschen eine Anzahl größerer Vesikel mit dunklem Kern.Acetylcholin führt zu einer Kontraktur des M. sphincter pupillae. Adrenalin zeigt keine Pupillenveränderung. Bei Reizung des postganglionären Nerven erhält man maximale tetanische Kontraktion bei einer Reizfrequenz von 200 Hz (SV).

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Summary The inner eye muscles of the chicken consist exclusively of very thin striated muscle fibers which are singly innervated. The fibers of the ciliary muscle are 280–1700 m long. The muscle fibers of the iris are richly ramified and build up a three-dimensional network.The connection of the single fibers is effectuated either by short tendons, consisting of unusually thick (3000–4000 Å) collagenous fibrils and an intermediate substance of electrondense and amorphous appearance, or by a basal membrane-like material, showing CHE-activity.The predominant part of the three-dimensional network of iris muscle fibers are circularly arranged (sphincter pupillae muscle), only a small part (dilatator pupillae muscle) shows radial arrangement.The sarcoplasm of the inner eye muscles contains numerous mitochondria (up to 12% of the whole cross-section-area), usually also, a lot of triglycerid-droplets and glycogen granules. The sarcoplasmatic reticulum is richly developed. A great number of triads can be seen; in the ciliary and sphincter pupillae muscles they lie regularly near the A-I border within the area of A, in the dilatator pupillae muscle they usually are scattered irregularly over the whole A-band.The striated pattern shows a marked M-line, whereas the pseudo-H-zone is scarcely distinguishable. The Z-line is remarkably broad (1200–1600 Å) and shows an irregular course. The sarcomeres of a fiber may be of varying size; the two I-band halves of one single sarcomere may vary in width.The peripheral motor pathway consists of two neurons. The peripheral neuron beginning in the ciliary ganglion, possesses a myelin sheath and ends at motor endplates of the inner eye muscle fibers. Approximately four muscle fibers can be related to one neuron. The motor endplates are large; the relative size of innervation (m² synaptic area/1,000.000 m³ muscle fiber volume) has the extraordinary value of 10.000. The synaptic membranes have no folds, the terminal axoplasma, besides numerous normal synaptic vesicles, contains a number of larger vesicles with dark cores. Acetylcholine induces a contracture of sphincter pupillae muscle. Adrenaline shows no influence upon the width of the pupil. Maximal tetanic contraction is brought about by stimulation of the postganglionic nerve at the frequency of 200 Hz.

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Herrn Prof. Dr. K. Goerttler mit den besten Wünschen zum 70. Geburtstag zugeeignet.     

神经激肽B及其生殖内分泌作用

神经激肽B(neurokinkin B,NKB)是速激肽家族的一员,主要通过其受体NK3R发挥作用。NKB及NK3R在神经系统分布广泛。NKB具有使空腔脏器平滑肌收缩、松弛血管、降低平均动脉压、减慢心率、兴奋离体大鼠脊髓神经元及收缩瞳孔括约肌缩小瞳孔等生物学作用。近年来NKB在生殖内分泌中的调控作用越来越受到关注,关于其调节下丘脑-垂体-性腺轴(HPGA)的作用的研究也越来越深入。本文综述了NKB及其受体的分布范围、生理功能、NKB在生殖内分泌调控过程中的作用,其具体的作用机制还有待于进一步研究。     

Substance P in the control of extrahepatic biliary motility in the cat

The effects of regional intra-arterial injections of substance P (SP) or efferent electrical stimulation of the vagal nerves on feline extrahepatic biliary motility were studied in anesthetized cats using a constant perfusion model. Each of these procedures elicited contractile motor responses of the gallbladder and the sphincter of Oddi. Since SP is present in feline vagal axons, these findings may indicate a role of SP in the vagal motor control of biliary motility. Immunocytochemically neurons with SP-like immunoreactivity were found in the smooth muscle layers of the biliary tree as well as adjacent to acetylcholinesterase-positive ganglion cells indicating either direct activation of smooth muscle cells and/or indirect activation via cholinergic neurons. Depending on the type of stimulation different SP mechanisms were demonstrated; exogenous SP induced contraction of both the sphincter and the gallbladder which were probably direct (resistant to atropine but sensitive to a SP analogue), while vagal stimulation elicited contraction of both regions via a mechanism sensitive to atropine and to a SP analogue.     

Immunocytochemical study on the triple origin of the sphincter iris in the chick embryo

The ontogenic development of the sphincter iris has been studied by immunocytochemistry and standard staining on chick embryos from stage 25 HH to the time of hatching. We have used the monoclonal antibody 13F4, a highly specific marker of muscular cells. We have observed three different regions in the iris. In the pupillary region, immunoreactive cells are in continuous contact with the inner epithelium of the pupillary margin. In the intermediate region, the outer epithelium forms buds of pigmented cells that emigrate toward the stroma. In this epithelium cells that are totally or partially unpigmented exist, and they are 13F4 positive. In the sphincter we have observed 13F4 positive cells with melanin granules. In the ciliary region, the immunoreactivity appears in dispersed mesenchymal cells. The present findings are consistent with a triple origin of the sphincter iris in the chick embryo. This muscle is derived from the inner epithelium of the pupillary margin, the intermediate region of the outer epithelium, and from the mesenchymal cells. The cells of the inner epithelium of the pupillary margin are differentiated into smooth muscle cells, and the remaining cells form striated muscle cells. Received: 17 March 1999 / Accepted: 17 May 1999     

Development of a three-dimensional physiological model of the internal anal sphincter bioengineered in vitro from isolated smooth muscle cells

Fecal incontinence affects people of all ages and social backgrounds and can have devastating psychological and economic consequences. This disorder is largely attributed to decreased mechanical efficiency of the internal anal sphincter (IAS), yet little is known about the pathophysiological mechanisms responsible for the malfunction of sphincteric smooth muscle at the cellular level. The object of this study was to develop a three-dimensional (3-D) physiological model of the IAS bioengineered in vitro from isolated smooth muscle cells. Smooth muscle cells isolated from the IAS of rabbits were seeded in culture on top of a loose fibrin gel, where they migrated and self-assembled in circumferential alignment. As the cells proliferated, the fibrin gel contracted around a 5-mm-diameter SYLGARD mold, resulting in a 3-D cylindrical ring of sphincteric tissue. We found that 1) the bioengineered IAS rings generated a spontaneous basal tone, 2) stimulation with 8-bromo-cAMP (8-Br-cAMP) caused a sustained decrease in the basal tone (relaxation) that was calcium-independent, 3) upon stimulation with ACh, bioengineered IAS rings showed a calcium- and concentration-dependent peak contraction at 30 s that was sustained for 4 min, 4) addition of 8-Br-cAMP induced rapid relaxation of ACh-induced contraction and force generation of IAS rings, and 5) bioengineered sphincter rings show striking functional differences when compared with bioengineered rings made from isolated colonic smooth muscle cells. This is the first report of a 3-D in vitro model of a gastrointestinal smooth muscle IAS. Bioengineered IAS rings demonstrate physiological functionality and may be used in the elucidation of the mechanisms causing sphincter malfunction.     

An ultrastructural study of the melanophages in the cerebrospinal fluid of the tadpoles of Xenopus

Melanin deposits in the brain ventricles of Xenopus tadpoles were studied with light and electron microscopy (TEM and SEM). They appeared to be aggregations of melanophages which accumulated free pigment granules excreted by ependymal cells into the cerebrospinal fluid. Whereas the meningeal melanophores contained oval melanosomes of various sizes, the melanosomes in the scavenger cells were all spherical, large (0.6–1.1 μm) and fairly uniform in size. Moreover, they were arranged in spherical groups which were never seen in the cytoplasm of the melanophores. The melanosomes within the cells were identical to the free melanosomes found in the cerebrospinal fluid and those which occurred within the ependymal cells in the young larva, suggesting a common origin from the egg cytoplasm. The number of the melanosomes in the melanophages increased with age. Fine cytoplasmic projections were involved in catching and engulfing the melanosomes. Some other features of the cytoplasm, e.g., large deposits of cell detritus, also indicated that the cells were macrophages. In the later stages, (48, 49) no projections were observed, but the cells were totally filled with melanosomes.     

Differential expression of caveolin-3 in mouse smooth muscle cells in vivo

Expression of caveolin-1 and -3 in mouse smooth muscle cells in vivo was examined by immunohistochemistry. Caveolin-1 was detected in almost all smooth muscles examined, except for the pupillary dilator muscle, whereas caveolin-3 was present only in smooth muscles of some specific tissues. In the eye, the pupillary sphincter muscle was intensely positive for caveolin-3, whereas the ciliary muscle and pupillary dilator muscle were negative. In the gastrointestinal tract, caveolin-3 was detected in the inner circular layer, but not in the outer longitudinal layer. Vascular smooth muscle cells of the resistance-sized artery in the uterus and corpus cavernosum were intensely positive for caveolin-3, whereas those of the aorta were only weakly positive and those of the vena cava were negative. Caveolin-3 was also detected in smooth muscle cells of the urinary bladder, ureter, prostatic vas deferens, and seminal vesicle. The different levels of caveolin-3 expression among various smooth muscle tissues were confirmed by Western blot analysis. Even within the same muscle, the relative expression levels of caveolin-1 and -3 were variable among neighboring cells, suggesting distinct fine regulation of expression of these two caveolins. Moreover, even in the same cell, caveolin-1 and -3 showed different distributions. These results indicate that the two caveolins form distinct caveolae in smooth muscles, and that caveolin-1 and -3 serve different functions. Their differential expression may therefore be related to the functional diversity of smooth muscles. This work was supported by Grants-in-Aid for Scientific Research from the Ministry of Education, Science, Sports, and Culture of the Japanese Government.