Maturation of tight junctions in guinea-pig cecal epithelium

Summary By means of the freeze-fracture technique and in tracer studies it is demonstrated that the structure of tight junctions and the permeability to lanthanum of the guinea-pig cecal epithelium change during maturation of cells. Height and strand number of tight junctions in the apical-basal direction increase as crypt cells migrate to the surface of the epithelium. Likewise, the interlacing of continuous strands was greater in surface than in crypt junctions. The numerous free-ends, isolated individual freestrands and maculae occludentes found in crypt cells were absent in surface epithelial cells. Goblet cells, located at the bottom of crypts, displayed tight junctions similar in characteristics to those of cells located in the middle region of crypts. Cells at the surface and in middle regions of crypts possess tight junctions impermeable to lanthanum, whereas junctions between cells located at the bottom of crypts often were permeable to the tracer, indicating that permeability decreases as the epithelial cells mature. Genesis and maturation mechanisms related to structural configuration of tight junctions are discussed.     

A novel perspective: the occluding zonule encircles the apex of the Sertoli cell as observed in birds

The modulation of Sertoli cell junctions was studied in the non-seasonal rooster (Gallus domesticus) and in the seasonally breeding mallard duck (Anas platyrynchos anatidae) using thin sectioning, a junction permeability tracer, and freeze-fracture replication. During the active spermatogenic phase, the junctions of the duck appeared similar to those of the rooster, thereby establishing the duck as an avian model of seasonal modulation of Sertoli cell junctions. As with mammalian seasonal breeders, during the active phase, occluding, gap, and adhering junctions formed a junctional complex all along the long axis of the Sertoli cell. Unlike in mammals, however, no 7-nm filaments were associated with the occluding junctions. An occluding zonule encircled the Sertoli cell apico-lateral membrane domain situated above the young germ cells, and constituted a barrier to the entry of lanthanum in the basal third of the seminiferous epithelium. Toward the basal side, forming focal junctions were located on the lateral Sertoli cell membrane domain facing the young germ cells. Toward the apical side, dismantling focal junctions were located on the apical Sertoli cell membrane domain facing the older germ cells. During the duck's testicular regression, 7-nm filaments were associated with an occluding junction. In freeze-fracture replicas, each junction was formed by a continuous junctional strand that encircled the apex of the cell. The strands composed a delicate narrow meshwork: an occluding zonule. The blood-testis barrier was localized near the apex of the epithelium. The seasonal reduction in the number of the strands and the changes in their orientation did not coincide with a change in the permeability of the occluding zonule to lanthanum. In addition, the cyclic disappearance of junction-associated filaments was not correlated with a change in the permeability of the junctions but with a change in the affinity of junctional particles for one or the other fracture face. It is proposed that the Sertoli cell plasma membrane domains situated apical and basal with respect to the occluding zonule be considered apical and lateral, respectively. The remaining domain facing the basement membrane would therefore be called basal. In the duck, the occluding zonule is not seasonally shifted from the base to the apex of the Sertoli cell. Instead, it remains stationed above the younger germ cells throughout the year.(ABSTRACT TRUNCATED AT 400 WORDS)     

Diffusion barriers in the vaginal epithelium during the estrous cycle in guinea pigs

Summary In the present study the permeability barriers of the multilayered vaginal epithelium were examined using tracer perfusion techniques, freeze-fracture and thin sectioning. During diestrus and proestrus the upper layers of mucified epithelial cells exhibit tight-junctional belts, which restrict tracer molecules such as lanthanum and horseradish peroxidase. When the highly mucified cells begin to degenerate toward the end of proestrus the underlying epithelium is already keratinized as typical for estrus. The keratinized epithelial cells have a tight-junctional network that joins the basal plasma membranes with the apical membranes of subjacent cells and blocks paracellular diffusion of the tracer molecules. During conversion of the cornified epithelium to a mucified epithelium in metestrus the intercellular space of the epithelium is stained by tracer molecules even though tight-junctional belts can be observed.These results indicate that during cyclic changes of the vaginal epithelium tight junctions can, in general, be considered for the restriction of paracellular diffusion. In metestrus, however, junctions become functionally leaky although they remain morphologically intact.Intercellular lipids, which are normally common in cornified epithelia, are extremely rare and cannot constitute an effective barrier to diffusion in the vagina of the guinea pig. The significance of a strategy that bases the regulation of the permeability on tight junctions rather than on intercellular lipids is discussed.     

The uterovaginal sperm host glands of the quail (Coturnix coturnix japonica)

Summary Ultrastructural and ultrahistochemical studies were performed on the uterovaginal sperm host glands of the quail (Coturnix coturnix japonica). The proximal parts of the glandular necks are lined by a pseudostratified epithelium, consisting of high columnar ciliated cells and small, irregular shaped, basal cells.The true glandular epithelium is composed only of columnar cells with microvilli on their luminal end. A characteristic luminal feature is a large lipid droplet in the perinuclear region. In the subplasmalemmal region numerous tubular profiles are seen which could represent a cellular resorption system.To evaluate the absorptive capacity of the Uterovaginal sperm host glands, tracer studies with HRP, ferritin, lanthanum and ruthenium red were undertaken. Since between 5 min and 3 h after injection no absorption could be found with the techniques mentioned, it is suggested that phagocytosis of spermatozoa by the glandular epithelium is not likely to occur.     

The cell junctions of the notochord of Xenopus laevis tadpoles

The cell junctions of the notochord of Xenopus laevis tadpoles were examined with the electron microscope using thin sections, lanthanum tracer experiments, and freeze-fracture replicas. Both the peripheral and vacuolated cells of the notochord are connected by numerous spot desmosomes characterized by an intercellular desmogloea and intermediate filaments on the cytoplasmic sides. The peripheral cells also display numerous hemidesmosomes facing the underlying basal lamina. Staining with rhodamine-phalloidin for F-actin yielded negative results and suggested that adhaerens-type junctions are absent. Tracer experiments with lanthanum and freeze-fracture replicas clearly revealed the presence of gap junctions between both cell types but no indications of tight junctions were found and no intercellular barrier existed for tracer infiltration of the notochord.     

A freeze-fracture and lanthanum tracer study of the complex junction between Sertoli cells of the canine testis

What appear to be true septate junctions by all techniques currently available for the cytological identification of intercellular junctions are part of a complex junction that interconnects the Sertoli cells of the canine testis. In the seminiferous epithelium, septate junctions are located basal to belts of tight junctions. In thin sections, septate junctions appear as double, parallel, transverse connections or septa spanning an approximately 90-A intercellular space between adjacent Sertoli cells. In en face sections of lanthanum-aldehyde-perfused specimens, the septa themselves exclude lanthanum and appear as electron-lucent lines arranged in a series of double, parallel rows on a background of electron-dense lanthanum. In freeze-fracture replicas this vertebrate septate junction appears as double, parallel rows of individual or fused particles which conform to the distribution of the intercellular septa. Septate junctions can be clearly distinguished from tight junctions as tight junctions prevent the movement of lanthanum tracer toward the lumen, appear as single rows of individual or fused particles in interlacing patterns within freeze-fracture replicas, and are seen as areas of close membrane apposition in thin sections. Both the septate junction and the tight junction are associated with specializations of the Sertoli cell cytoplasm. This is the first demonstration in a vertebrate tissue of a true septate junction.     

PERMEABILITY OF SERTOLI CELL TIGHT JUNCTIONS TO LANTHANUM AFTER LIGATION OF DUCTUS DEFERENS AND DUCTULI EFFERENTES

The permeability of Sertoli cell tight junctions to lanthanum administered during fixation has been compared in rats after ligation of the ductus deferens and after ligation of the ductuli efferentes. In both control and vasoligated testes, lanthanum penetrated only short distances into the Sertoli cell tight junctions before stopping abruptly. The tight junction, consisting of numerous pentalaminar fusions of contiguous Sertoli cell membranes, prevented diffusion of lanthanum into the adluminal compartment of the seminiferous epithelium. In rats with ligated ductuli efferentes, lanthanum completely permeated many Sertoli cell tight junctions and occupied intercellular spaces of the adluminal compartment. In spite of their newly acquired permeability to lanthanum, tight junctions retained characteristic ultrastructural features, including numerous membrane fusions. When lanthanum-filled tight junctions were sectioned en face, membrane fusions appeared as pale lines in lakes of electron-opaque tracer. These linearly extensive fasciae occludentes occasionally ended blindly, suggesting that lanthanum may have traversed the junction by diffusing around such incomplete barriers. The increased permeability of Sertoli cell tight junctions after efferent ductule ligation, which caused rapid testicular weight gain followed by atrophy, indicates that tight junctions are sensitive to enforced retention of testicular secretions inside the seminiferous tubules. The apparent normalcy of Sertoli cell tight junctions after vasoligation, which had no effect on testis weight, supports the view that blockage of testicular secretions distal to the epididymis is relatively innocuous.     

The terminal bar in the larval midgut epithelium ofAeshna cyanea

Summary Thin section and freeze-fracture electron microscopy revealed that the terminal bars of the larval midgut epithelium ofAeshna cyanea consisted of extended smooth septate junctions (SSJ), multiple adhesive junctions and rare gap junctions. Freeze-fractures of native tissue suggested that the septal building units were anchored only in the external membrane leaflet by partially integrated proteins while the interseptal pegs were anchored partly in both leaflets by completely integrated proteins and partly by presumed peripheral proteins.Reversible depletion of the physiological Ca⁺⁺ concentration had no apparent structural effect on the SSJ of the terminal bars, but led to a reversible formation of junctional septa between the foot processes concomitant with a rearrangement of IMPs in the basolateral plasma membranes. The basolateral SSJ assembly and disassembly induced by reversible Ca⁺⁺ deprivation was interpreted as exaggerated response of an intrinsic capability normally related to the apical growth of regenerative cells and to the extrusion of degenerating cells. Lanthanum tracer ingested with hyperosmotic drinking solution was always found excluded from the basolateral intercellular spaces underneath the terminal bar, but there was a dual effect on the SSJ structure. Part of the junctions remained structurally intact, part was dissociated in the apical portion and invaded by tracer.Abbreviations EF exoplasmic fracture face - EGTA ethylenglycol-bis(2-aminoethylether)-N,N-tetraacetic acid - IMP intramembrane particle - PAS periodic acid Schiff reagent - PF protoplasmic fracture face - PSJ pleated septate junction - SDS sodium dodecyl sulphate - SSJ smooth septate junction Dedicated to Prof. Dr. E.Scholtyseck in honour of his 65th birthday.     

ASSEMBLY OF GAP JUNCTIONS DURING AMPHIBIAN NEURULATION

Sequential thin-section, tracer (K-pyroantimonate, lanthanum, ruthenium red, and horseradish peroxidase), and freeze-fracture studies were conducted on embryos and larvae of Rana pipiens to determine the steps involved in gap junction assembly during neurulation. The zonulae occludentes, which join contiguous neuroepithelial cells, fragment into solitary domains as the neural groove deepens. These plaque-like contacts also become permeable to a variety of tracers at this juncture. Where the ridges of these domains intersect, numerous 85-Å participles apparently pile up against tight junctional remnants, creating arrays recognizable as gap junctions. With neural fold closure, the remaining tight junctional elements disappear and are replaced by macular gap junctions. Well below the junctional complex, gap junctions form independent of any visible, preexisting structure. Small, variegated clusters, containing 4–30 particles located in flat, particle-free regions, characterize this area. The number of particles within these arrays increases and they subsequently blend together into a polygonally packed aggregate resembling a gap junction. The assembly process in both apical and basal regions conforms with the concept of translational movement of particles within a fluid plasma membrane.     

A permeability barrier in the testis of an insect Triatoma: A freeze-fracture and lanthanum tracer study

In vertebrates, the testicular permeability barrier has been the subject of numerous studies. Some recent observations also indicate the existence of such a barrier in some invertebrates, e.g. insects and worms. With the aim of determining whether the morphological features of the blood-testis barrier generally found in vertebrates can be extended to other animals, we studied the testis of the insect Triatoma infestans using electron-dense tracers and freeze-fracture techniques. This organ is divided into cysts timed in synchroneous maturation. The intercellular tracer (lanthanum hydroxide) freely penetrates the basal areas of the seminiferous epithelium surrounding spermatogonia and spermatocytes devoid of synaptonemal complexes (pre-leptotene and leptone). Zygotene spermatocytes indicate the establishment of the barrier. Freeze-fracture techniques exhibit the morphological correlate of the barrier consisting of 9-10 nm particle rows on the P faces of the Sertoli cell membranes. These rows are relatively loose showing an undulating disposition and correspond to the septate junctions found in thin sections. The percolation of intercellular tracers demonstrates that septate junctions between the basal membraneous areas of Sertoli cells possess the barrier properties.     

Polarity reversal of inside-out thyroid follicles cultured within collagen gel: structure of the junctions assessed by freeze-fracture and lanthanum permeability

The organization of tight junctional complexes (TJs) was studied in cultured porcine thyroid cells during the inversion of polarity induced by collagen-embedding of inside-out follicles, using freeze-fracture replicas and lanthanum penetration. During the early steps of polarity reversal, freeze-fractures showed that TJs generally persisted. They increased in width and progressively branched out into the basolateral surfaces, towards the basal pole. Later, the number of TJ strands decreased and gap junctions inserted within TJ networks were found between cells in reversed follicles, in the same manner as in typically polarized follicles, embedded in collagen or in suspension. The de novo formation of TJ complexes was rarely found in the reversing structures. Despite the heterogeneity of TJs assessed by freeze-fracture, impermeability to lanthanum tracer was noted in inside-out structures. During the reversal process, some TJs remained unstained, whereas others displayed permeability to lanthanum. This heterogeneity might be due to the "opening" of a small number of junctions (perhaps only one by aggregate). When the process was achieved after 48 hr in collagen, the tightness of the junctions was complete, confirmed by the absence of lanthanum in luminal cavities of newly formed follicles.     

Permeability of the Body Wall of Romanomermis culicivorax to Lanthanum

Ultrastructural study of the body wall of preparasitic, parasitic, and postparasitic stages of Romanomermis culicivorax showed that the cuticle of all three stages was permeable to lanthanum. The cuticle of the parasitic stage was the thinnest and showed the greatest permeability. Lanthanum accumulated on the apical surfaces of the hypodermal cells but was not found intracellularly. The negative staining characteristics of lanthanum enhanced the detection of numerous smooth septate junctions in the hypodermis of the parasitic stage.     

Freeze-fracture study of the epidermal cells of a teleost with particular reference to intercellular junctions and permeability to tracer

The plasmatic membranes, the intercellular junctions and the intercellular spaces of the epidermis of the fish Pimelodus maculatus were studied by freeze-fracture and by lanthanum methods. The observations has confirmed the presence of desmosomes. Gap junctions were not found and the tight junctions can be seen very rarely, arranged to form small discrete maculae. The finger-print pattern due to the microridges of the apical plasma membrane of the superficial cells was studied by direct replicas. The tracer penetrates all the intercellular epidermal spaces but failed to penetrate the dermis, suggesting the presence of a barrier at the dermo-epidermal level.     

Uptake of Peroxidase and Lanthanum by the Teleost Choroid Plexuses

The absorbing capability of the choroidal epithelium in the third and the fourth ventricles of the teleost Leuciscus rutilus was studied by using the electron dense tracers lanthanum and peroxidase. The tracers were either injected into the third ventricle or applied onto the leptomeninx. Peroxidase was rapidly absorbed by coated vesicles after being injected into the ventricle. This reaction product was retained in multivesicular bodies which remained localized at the apical pole of the cell. However, when peroxidase was applied onto the leptomeninx only a limited uptake was observed. Lanthanum was not absorbed by the epithelial cells. The zonulae occludentes between two adjacent cells prevented the tracers from reaching the ventricular or vascular sides. Thus, the epithelium of the saccus dorsalis and the plexus choroideus posterior act as a barrier prohibiting the transport of these tracers from the blood to the cerebrospinal fluid or also in the reverse direction.     

Mitochondria-rich cells and carbonic anhydrase content of toad skin epithelium

Summary The density and carbonic anhydrase (CA) content of the mitochondria-rich cells (MRCs) in the skin epithelium of the toad, Bufo viridis, were studied under conditions of acclimation to various chlorinities. Long-term (days to weeks) acclimation to chloride-free solutions induced a great increase in the MRC density and the area occupied by the apical portion of these cells on the surface of the epithelium. The CA content of the epithelium, and individual MR cells, showed a 5- to 10-fold reduction after acclimation to solutions containing high chloride levels. The MRC density and their relative apical surface area correlated with the chloride permeability of the skin in acclimated (long-term) toads. It is concluded that the MRCs are the principal site of chloride permeability across the amphibian skin, and they respond in an adaptive manner to long-term changes in environmental chloride levels.This study was partially supported by the J. and A. Taub Fund for Biological Research at The Technion, and by the basic research fund of the Israel Academy of Sciences     

The fine structure of the nephronic tubule of the mudskipper Periophthalmus koelreuteri (Pallas)

Ultrastructural examination of the head kidney of Periophthalmus koelreuteri (Pallas) (Teleostei, Gobiidae) revealed that the nephronic tubule cells are bound by tight junctions and desmosomes with little intercellular space. The first proximal segment (PI) consists of low columnar cells with well developed brush borders, indented nuclei, and numerous apical endocytic vesicles and lysosomes. A second cell type possessing clusters of apical cilia and lacking brush border and lysosomes is occasionally found between PI cells. The second proximal segment (PII) is formed of high columnar cells with brush border, regular spherical nuclei and numerous mitochondria located between well developed infoldings of the basal membrane. Single ciliary structures protrude into the lumen from PI and PII cells. The distal segment is lined by low columnar epithelium with few microvilli, regular spherical nuclei, numerous scattered mitochondria, and microbodies. The collecting tubule cells are cuboidal with few euchromatic nuclei, some mitochondria, and secondary lysosomes.     

The structure and function of the smooth septate junction in a transporting epithelium: The malpighian tubules of the new zealand glow-worm Arachnocampa luminosa

Junctional complexes between the epithelial cells in the four distinct regions of the glow-worm Malpighian tubule were investigated by electron microscopy using thin sectioning, freeze-fracturing, osmotic disruption and tracer techniques. The lateral plasma membranes of all four cell types are joined by smooth septate junctions but the extent of the complex across the cell depth varies in the four different regions. The width of the septa, the interseptal spacing and the separation between the outer leaflets of the adjacent plasma membranes are different for each cell type. Gap junctions were identified only in the junctional complex between Type IV cells and were intercalated amongst large lateral sinuses. In oblique sections of lanthanum infiltrated tissue, the electron-lucent septa at the basal side of the junction are outlined by the tracer as it penetrates. In the Junctional complexes of all four regions the septa appear as short, distinct, linear bars. In tangential sections of gap junctions between Type IV cells, the junctions appear as a hexagonal array of intermembrane particles with a centre to centre spacing of 18 nm. Horseradish peroxidase did not penetrate the junctional complexes very far but readily passed through the basal lamina into the spaces between extracellular invaginations of the basement membrane of the cells. Junctional complexes in all four areas of the tubule have similar freeze-fracture faces. In freeze-fracture replicas of fixed tissue continuous ridges of fused particles are seen on the P face and complementary furrows are found on the E face. Junctional response to osmotically adjusted Ringer solutions was similar in all four cell types. Distortion or ‘blistering’ of the intercellular space between the septa of the junction occurred when the tissue was bathed in or injected with a hypertonic Ringer solution. The structure of these junctions, visualized by the different techniques, and the role of the septate junction in a transporting epithelium, are discussed.     

Fine structural analysis of membrane changes during reaggregation culture of chick optic tectum

Thin section and freeze-fracture electron microscopy have been used to characterize the changes in membrane morphology of reaggregating cultures of chick optic tectum. The cells are rounded and freely dispersed at 0 hr after dissociation. Between 2 and 6 hr the cells become closely apposed on all sides by other cells and form small aggregates. At this time punta adhaerentia junctions and focal densities are seen along the membranes of neighboring cells. Between 1 and 5 days in vitro (DIV) neurites containing growth cone regions are present. At 5 DIV the first synaptic contacts are observed. Between 7 and 14 DIV, the number of synaptic contacts increase and fewer growth cone regions are observed. As early as 7 DIV profiles are observed which strongly resemble both astrocytic and oligodendroglial cell somata and processes. Freeze-fracture analysis of aggregates at 0–4 hr reveals a sparse particle distribution on the P and E faces of apposed cells. By 1 DIV small clusters of loosely packed, large sized particles are seen on the P face of apposed cell membranes which may represent junctional contacts. Apparent coated vesicle fusion sites are common on the P face at 1–2 DIV. By 7 DIV, E face particle arrays are seen on cell bodies and neurites which correspond to specializations characteristic of excitatory synaptic junctions. By 8–10 DIV particle arrays are seen on the P face of post-synaptic membrane which may represent inhibitory synaptic contacts. Other types of particle specializations seen in freeze-fracture replicas include: specializations characteristic of gap junctions between cells and orthogonal assemblies of particles thought to be characteristic of astrocytes.     

Changes in the lanthanum distribution following decapitation of the sporophytes of an aquatic fern,Marsilea drummondii A. Br.

Summary The active terminal bud and the quiescent lateral buds and corresponding nodes inserted at different levels on the main rhizome ofMarsilea drummondii were examined with the EM afterin vivo feeding with lanthanum nitrate. These tracer experiments demonstrate that all the buds are fed by their phloem cells. In the lateral bud axis the labelling of the sieve elements apoplast indicates that a solute transfer took place in the node between xylem and phloem via xylem transfer cells. La³⁺ deposits are completely absent from the apical dome of inhibited buds indicating that the walls of the quiescent meristematic cells are not permeated by the tracer. The removal of the terminal bud has two effects. It rapidly (in 2 hours) allows the lanthanum to penetrate the lateral bud tip walls at a stage when no fine structural changes are discernable and to bind to the outer surface of the plasmalemma as it does in the active terminal bud. This study including inhibited buds and buds released from apical dominance support the view that changes in the state of the cell surface (cell wall and plasma membrane) may be a prerequisite for the resumption growth activity.This study was supported in part by a grant from the Centre National de la Recherche Scientifique to L.Sossountzov (AI 031275).     

Rhombic particle arrays in gill epithelium of a mollusc, Aplysia californica.

Gill epithelia from adult and juvenile Aplysia were examined by conventional thin section and freeze-fracture methods. Freeze-fracture replicas of adult gill epithelium revealed septate and gap junctions, which served as membrane markers for the epithelial cells. In these same cell membranes, non-junctional rhombic arrays of intramembranous particles were observed on prominent ridges on the membrane P fracture face of some epithelial cells. In thin sections of adult epithelium, nerve terminals were observed abutting the lateral plasma membranes near the basal lamina of some epithelial cells. Correlative areas of plasma membrane in freeze-fracture replicas showed a close association between rhombic particle arrays and abutting nerve terminals. In thin sections of juvenile Aplysia, nerve terminals abutting the epithelial cells were not recognizable, and rhombic arrays were not observed in freeze-fracture replicas. This suggested that a developmental association existed between the appearance of rhombic arrays in adult epithelia and their innervation. It is not known with certainty if, in invertebrates, rhombic arrays are an essential structural entity of all innervated cell membranes; however, in the cells thus far studied, there appears to be an associative condition. In the case of the gill epithelium of Aplysia, rhombic arrays are located in the same vicinity as the abutting nerve terminals. Similar arrays of intramembranous particles have been observed in myoneural postjunctional complexes of other invertebrates and have been interpreted to be the morphological expression of neurotransmitter receptors. An analogous explanation is put forth, namely that rhombic arrays may represent the structural correlates of neurotransmitter receptors and/or ionic channels in innervated membranes of invertebrates.