The fine structure of the salivary glands of the desert locust Schistocerca gregaria Forskål

Summary This paper describes the structure of the salivary glands of Schistocerca gregaria as seen under the electron microscope and the light microscope. The salivary glands consist of a number of acini located on both sides of the pro-, meso-, and metathoracic segments of the locust. Each acinus is drained by a duct which unites with others from the same side to form a lateral collecting duct. The ducts from the two sides join in the head capsule and open into a salivary cup on the labium. Each acinus consists of parietal cells, zymogenic cells, duct cells, tracheoblasts, sheath cells and pigment cells. The parietal and zymogenic cells are the main sites for the production of the salivary gland secretions, which pass through microvilli from the zymogenic cells to the lumen of the ducts within the acinus. Outside the acinus each duct is composed of highly specialized cells with infolded basement membranes extending about a third of the way across the cell. The cytoplasm between the membranes contains elongated mitochondria and glycogen granules. The apical border of the cell is thrown into microvilli which are closely aggregated under the cuticle lining the duct. These cells have all the features of cells previously described in vertebrates and invertebrates which are known to absorb water and/or ions. Absorption of water from the gut could allow the excretion of hypertonic saliva by the locust.     

Ultrastructure of the excretory duct in the silk gland of the sugarcane borer Diatraea saccharalis (Lepidoptera: Pyralidae)

The excretory duct in the silk gland of the sugarcane borer Diatraea saccharalis consists of two morphologically distinct regions, recognized by scanning and transmission electron microscopy. The thin posterior region, adjacent to the glandular region, presents a regular surface. Secretory vesicles containing either electron-dense or fibrillar cuticular-like materials are observed in their apical cytoplasm; the same cuticular materials were detected as extracellular deposits among the microvilli. The short anterior region, near the common duct, exhibits surface protrusions; there are no secretory vesicles in their apical cytoplasm. These results show that only the duct cells at the posterior region are involved in the secretion of the cuticular intima elements. Desmosome-like structures were visualized linking together adjacent microvillar membranes only in the cells of anterior duct region, with unknown function. The transition between the duct and the glandular region is abrupt; the cells of the glandular and posterior duct regions present large amounts of microtubules. Nerve fibers can be observed between the duct cells in their two regions, suggesting that control of silk secretion may occur in the excretory duct via neurotransmitter liberation.     

Aquaporin-1在大鼠睾丸输出小管的免疫组织化学定位研究

目的研究正常大鼠睾丸输出小管上皮细胞上Aquaporin．1(AQP-1)的定位分布以期了解其在水重吸收上的作用机制。方法对正常wistar大鼠睾丸输出小管进行常规免疫组织化学方法染色观察。结果在睾丸输出小管非纤毛上皮细胞的刷状缘及基侧部AQP-1阳性表达强烈,核上区的胞内体的质膜上也有阳性表达;纤毛上皮细胞的纤毛亦呈阳性反应。结论Aquaporin-1可能与睾丸输出小管非纤毛上皮细胞水重吸收功能有密切关系。     

Studies on the silk glands of Calpodes ethlius stoll, (Lepidoptera,hesperiidae)

Each silk gland of Calpodes ethlius consists of five distinct regions: the duct, the green, anterior, middle and posterior regions. Although the gland increases approximately tenfold in length during the larval life, the number of cells remains constant with a concomitant increase in ploidy which is not constant either throughout larval life or in the different regions of the gland. Histochemistry on the glands of the mid-fifth instar larva shows that progressively more mucosubstances are deposited in the lumen, so that while in the distal regions there is only one weakly acidic deposit, this is increased to three more acidic bands in the proximal regions. These bands can be correlated with materials of different electron density. All five regions have characteristic secretory ultrastructure, with prominent secretory vesicles or granules and microvilli. However, the posterior and middle regions have electron-translucent vesicles and relatively short microvilli, while the other three regions have electron dense granules and a more complex, microvillate apical surface. This complexity is greatest in the duct which suggests that it may function in water reabsorption.     

Immunohistochemical demonstration of villin in the normal human pancreas and in chronic pancreatitis

Summary Human pancreatic tissue was investigated by immunohistochemistry using a polyclonal antibody against the actin binding protein villin, which participates in the formation of actin filament bundles in the microvilli. In cells of the different parts of the pancreatic duct system as well as in the acinar cells villin immunoreactivity was located mainly at the apical cell surface. This was confirmed by the ultrastructural demonstration of microvilli on the surface of duct and acinar cells, which exhibited the typical actin bundles. In chronic pancreatitis the staining for villin in duct-like structures of degenerative pancreatic tissue was irregular or even absent. This correlated with the electron microscopic observation of duct-like structures known as tubular complexes composed of cells devoid of microvilli at the apical cell surface. At the light microscopical level degenerative structures without lumen and of unknown origin showed a strong staining for villin at their basal cell surface.     

Immunohistochemical demonstration of villin in the normal human pancreas and in chronic pancreatitis

Human pancreatic tissue was investigated by immunohistochemistry using a polyclonal antibody against the actin binding protein villin, which participates in the formation of actin filament bundles in the microvilli. In cells of the different parts of the pancreatic duct system as well as in the acinar cells villin immunoreactivity was located mainly at the apical cell surface. This was confirmed by the ultrastructural demonstration of microvilli on the surface of duct and acinar cells, which exhibited the typical actin bundles. In chronic pancreatitis the staining for villin in duct-like structures of degenerative pancreatic tissue was irregular or even absent. This correlated with the electron microscopic observation of duct-like structures known as tubular complexes composed of cells devoid of microvilli at the apical cell surface. At the light microscopical level degenerative structures without lumen and of unknown origin showed a strong staining for villin at their basal cell surface.     

Fine structure of the salivary glands of Triatoma infestans (Hemiptera: Reduviidae)

The fine structure of the salivary glands of adult Triatoma infestans (Hemiptera: Reduviidae) bugs has been analyzed. Stereomicroscopy and scanning electron microscopy showed that each insect presents a pair of salivary glands, each pair containing three distinct units (main, supplementary, and accessory) with different sizes and colors. Transmission electron microscopy demonstrated that all gland units consist of a monolayer of epithelial cells surrounding a large central lumen. The gland units are enveloped by a thick basal lamina containing bundles of muscle cells. Microvilli are present at the apical plasma membrane domain of the gland cells, thus enlarging the available membrane area for saliva secretion towards the large gland lumen, although occasionally budding vesicles could be observed among the microvilli. Cytochemical analysis showed that the salivary gland cells of T. infestans present abundant endoplasmic reticulum profiles and several lipid droplets.     

Monoclonal antibodies as probes for plasma membrane domains in the exocrine pancreas

Monoclonal antibodies (mAb) were generated as probes for the plasma membrane domains of pancreatic acinar cells. Primary monolayer cultures of mouse pancreatic acinar cells, which have an expanded apical surface relative to normal pancreas, were used to immunize rats. With conventional immunization and fusion protocols, 3% of the hybridomas were positive against the acinar lumen by indirect immunofluorescence of mouse pancreas cryosections. Culturing of spleen cells from an immunized rat on the apical surface of acinar cell monolayer cultures before fusion with the myeloma (an in vitro boost) doubled the percentage of hybridomas producing apical membrane-specific mAb. Monoclonal antibodies were characterized by immunofluorescence, ultrastructural immunoperoxidase cytochemistry, immunoprecipitation, and immunoblotting. One antibody, acinar-1 (IgG2a), labeled the apical membranes of pancreatic acinar cells, hepatocytes, salivary and lacrimal gland acinar cells, and the brush border of small intestine enterocytes. This mAb precipitated and blotted a protein of 94 KD. Acinar-2 (IgM) also labeled pancreatic acinar cell apical membranes but did not label other tissues and did not precipitate or blot. Acinar-3 labeled pancreatic acinar cell lateral membranes. Duct-1 (IgM) labeled pancreatic duct apical membrane and ducts in liver and salivary glands but did not precipitate or blot. These domain-specific mAb demonstrate that common antigenic determinants occur in the apical surfaces of several exocrine epithelia and may be important in secretion.     

The ultrastructure and histochemistry of the spermathecae of Tubifex tubifex (Annelida: Oligochaeta)

The wall of the spermathecal ampulla in Tubifex tubifex consists of epithelial, muscular and peritoneal layers. The epithelial surface contains closely microvilli while lateral and basal plasma membranes are extensively convoluted. Epithelial cytoplasm exhibits a vertical zonation of subcellular components. The distal zone contains filiform secretory particles which are orientated perpendicular to the apical surface; extrusion occurs by their fusion with the plasma membrane between the bases of neighbouring microvilli. Mitochondiral and Golgi zones, the latter containing the nucleus, subtend the distal zone. The basal zone, composed of vertical compartments formed by the folded plasma membrane, is rich in α-glycogen rosettes. The distal epithelium and lumen material contain neutral mucopolysaccharides and carboxylated acid mucopolysaccharides in conjunction with neutral protein. The ultrastructure of the spermathecal duct wall is comparable with that of the ampulla but is characterized by extremely long microvilli and a prominent musculature.     

Surface defects in ventricular cells of brains of mouse embryos homozygous for the Loop-tail gene: scanning electron microscopic study.

Luminal surfaces in the mesencephalon and rhombencephalon in normal mouse embryos and those homozygous for Lopp-tail were studied by means of scanning electron microscopy. Ventricular cells in the ventrolateral regions of normal day-10 and -11 brains showed single apical cilia and microvilli, whereas those in ventromedial regions showed a dense network of microvilli and bulbous projections which tended to obscure the apical cilia and cellular outlines. Similar regional differences occurred in the Loop-tail brains, although there was a marked decrease in the number and density of microvilli and bulbous projections. At days 12-14 of gestation the latter brains also showed a flattening of cell surfaces, shallow depressions, and craterlike ruptures in the plasma membranes.     

黄胫小车蝗受精囊的亚显微结构

利用组织学方法,观察了黄胫小车蝗Oedaleus infernalis 受精囊的显微与亚显微结构。结果表明,黄胫小车蝗受精囊为单个,由高度卷曲的受精囊管和蚕豆状的端囊构成。受精囊壁主要由表皮层、上皮层、基膜和肌肉层构成;上皮层包含上皮细胞、导管细胞和腺细胞。上皮细胞在靠表皮层的边缘有大量的微绒毛,两相邻上皮细胞的细胞膜相互嵌入,并有细微的突起延伸在导管细胞及腺细胞之间,直到基膜,达基膜处的上皮细胞膜折叠,与腺细胞膜的折叠,一起形成迷宫样的指状突起,附着在基膜上。导管细胞有一个较大的核和分泌导管,连接于腺细胞的细胞腔和受精囊腔,将腺细胞中分泌物运输到受精囊腔中。腺细胞具有典型的分泌细胞特征： 含发达内质网、高尔基复合体及不同大小的囊泡。肌肉层位于受精囊最外层,附在基膜上。在受精囊不同部位的结构有差异。在交配前和交配后,受精囊腺细胞的亚显微结构也有差异。     

Ultrastructure of the Male Accessory Glands and Sperm Ducts of Cylindrotaenia hickmani(Cestoda,Cyclophyllidea)

Abstract The ultrastructure of unicellular accessory glands (= prostate glands) and external male ducts of the cestode Cylindrotaenia hickmaniare described. Accessory glands open into the lumen of the external common sperm duct (= external vas deferens). The gland cells contain abundant endoplasmic reticulum, Golgi bodies and secretory bodies, and have elongate necks that pierce the apical cytoplasm of the duct. Cell contact with the apical cytoplasm of the sperm duct is mediated by septate desmosomes. Accessory glands secrete spherical particles, with a diameter of approximately 70 nm, that adhere to spermatozoa. The roles of these accessory glands may relate to activity of the sperm or development of the female system after insemination. Paired sperm ducts arise from testes, and unite to form a common sperm duct. Each duct consists of a tubular anucleate cytoplasmic region which is supported by nucleated cytons that lie sunken in the parenchyma. The apical cytoplasm of the paired sperm ducts (= vasa efferentia) possesses apical microvilli and abundant mitochondria, but few other cytoplasmic features. The apical cytoplasm of the common sperm duct possesses sparse apical microvilli and numerous electronlucent vesicles. The male gonoducts form an elongate syncytium which is markedly polarized along the length of the ducts. The ducts also display apical–basal polarity in that sunken nucleated cytons support the apical cytoplasm which in turn has distinct basal and apical domains.     

Immunolocalization of AQP-5 in rat parotid and submandibular salivary glands after stimulation or inhibition of secretion in vivo

In vitro studies of cultured salivary gland cells and gland slices have indicated that there may be regulated translocation of aquaporin (AQP)-5 between the apical plasma membrane and intracellular compartments of the secretory cells. However, it remains unknown whether AQP-5 in salivary glands is subject to regulated trafficking in vivo. To examine this possibility, we have investigated the subcellular localization of AQP-5 in rat parotid and submandibular glands fixed in vivo under conditions of stimulated or inhibited salivary secretion. Immunofluorescence and immunoelectron microscopy was used to determine the subcellular distribution of AQP-5 in control conditions following the stimulation of secretion with pilocarpine (a muscarinic agonist) or epinephrine (an alpha-adrenoceptor agonist) or during inhibition of basal secretion with atropine (a muscarinic antagonist) or phentolamine (an alpha-adrenoceptor antagonist). Under control conditions, >90% of AQP-5 was associated with the apical plasma membrane of acinar and intercalated duct cells, with only rare gold particles associated with intracellular membrane domains. Pilocarpine treatment dramatically increased saliva production but had no discernible effect on AQP-5 distribution. However, the increased salivary secretion was associated with luminal dilation and the appearance of a markedly punctate AQP-5 labeling pattern due to clustering of AQP-5 at the microvilli (especially evident in the parotid gland) after 10 min of drug injection. No changes in the subcellular localization of AQP-5 were seen in response to epinephrine, atropine, or phentolamine treatment compared with control tissues. Thus AQP-5 is localized predominantly in the apical plasma membrane under control conditions, and neither the onset nor the cessation of secretion is associated in vivo with any significant short-term translocation of AQP-5 between intracellular structures and the apical plasma membrane.     

Ultrastructural and functional aspects of the spermatheca of the African Migratory Locust Locusta migratoria migratorioides (Reiche and Fairmaire) (Orthoptera: Acrididae)

The ultrastructure of the spermathecal epithelium of the African Migratory Locust Locusta migratoria migratorioides R. & F. (Orthoptera: Acrididae) was investigated with the aid of transmission and scanning electron microscopic methods. The unpaired spermatheca can be subdivided into a multiple coiled tube and a terminal bulb region with vestibule, small apical and extensive pre-apical diverticulum. The wall of the spermatheca consists of a chitin intima, a layer of epithelial cells with a distinct apical microvilli border and a layer of gland cells, whereby slender projections of the epithelial cells extend between the gland cells. Through extensive folding, the basal plasma membrane of the gland and epithelial cells form a huge labyrinth, which is bounded by a basal lamina. Extending into the above mentioned projections there are bundles of parallel-arrayed microtubules, which run perpendicular to the microvilli border of the epithelial cell. They end in the base region of the microvilli and in the basal labyrinth on hemidesmosomes and serve to provide a mechanically stressable anchorage for the epithelium. The gland cells show structures typical for the production of export proteins: ribosomes, rER, dictyosomes, as well as vesicles of different size and electron-density. Every gland cell contains an extracellular cavity, arising through invagination, which is coated with a microvilli border. Over an end-apparatus and a ductule joining onto it (also with chitin intima) the lumen of the extracellular cavity is connected with the spermathecal lumen. The release of secretions and other substances from the epithelium into the spermatheca lumen is as possible as the uptake of substances from the latter into the epithelium. Regional differences in the fine structure of the cuticular intima, epithelial and gland cells point to different functions of the epithelium in these regions.     

Fine structure of the larval midgut of the fly Rhynchosciara and its physiological implications

The midgut of Rhynchosciara americana larvae consists of a cylindrical ventriculus from which protrudes two gastric caeca formed by polyhedral cells with microvilli covering their apical faces. The basal plasma membrane of these cells is infolded and displays associated mitochondria which are, nevertheless, more conspicuous in the apical cytoplasm. The anterior ventricular cells possess elaborate mitochondria-associated basal plasma membrane infoldings extending almost to the tips of the cells, and small microvilli disposed in the cell apexes. Distal posterior ventricular cells with long apical microvilli are grouped into major epithelial foldings forming multicellular crypts. In these cells the majority of the mitochondria are dispersed in the apical cytoplasm, minor amounts being associated with moderately-developed basal plasma membrane infoldings. The proximal posterior ventriculus represents a transition region between the anterior ventriculus and the distal posterior ventriculus. The resemblance between the gastric caeca and distal posterior ventricular cells is stressed by the finding that their microvilli preparations display similar alkaline phosphatase-specific activities. The results lend support to the proposal, based mainly on previous data on enzyme excretion rates, that the endo-ectoperitrophic circulation of digestive enzymes is a consequence of fluid fluxes caused by the transport of water into the first two thirds of midgut lumen, and its transference back to the haemolymph in the gastric caeca and in the distal posterior ventriculus.     

Peculiar salivary glands in a silk‐producing mite Bakericheyla chanayi (Cheyletidae)

This is the first ultrastructural investigation of salivary glands in the family Cheyletidae. In both sexes of Bakericheyla chanayi, paired acinous salivary glands and tubular coxal glands were shown to be united into the common podocephalic system. The secretory portion of the salivary gland includes medial and lateral lobes composed of the five and two cells, respectively, with clearly distinct ultrastructure. The cytoplasm of the cells is occupied by the secretory granules containing fine fibrous material. The fine structure of both cell types suggest a proteinaceous nature of their secretions. A single central process extending from the apical face of each secretory cell passes through the common acinar cavity to enter the conducting duct. A pair of intercalary cells at the base of the conducting duct links it with the secretory portion of the gland. Extending towards the acinar cavity, protrusions of intercalary cells alternate the apical regions of the secretory cells and form with them highly‐specialized contacts characterized by the apical network of microtubules and microfilaments. Two possible ways of secretion are suggested: 1) exocytosis into the acinar cavity and 2) direct passage via the central processes. The detection of axon profiles in the gland body suggests a neural control for the glandular cell function. In tritonymphs, neither secretion nor large lateral lobe cells were observed up to the pharate stage when the lateral lobe undergoes rapid differentiation. The arrangement of the acinous gland is compared to that of other arthropods. Its composition appears to be close to the class three of insect glands. The involvement of the lateral lobe cells in silk production is discussed. J. Morphol. 276:772–786, 2015. © 2015 Wiley Periodicals, Inc.     

Carbonic anhydrase II associated with plasma membrane in a human pancreatic duct cell line (CAPAN-1).

The subcellular distribution of carbonic anhydrase II, either throughout the cytosol or in the cytoplasm close to the apical plasma membrane or vesicular compartments, suggests that this enzyme may have different roles in the regulation of pH in intra- or extracellular compartments. To throw more light on the role of pancreatic carbonic anhydrase II, we examined its expression and subcellular distribution in Capan-1 cells. Immunocytochemical analysis by light, confocal, and electron microscopy, as well as immunoblotting of cell homogenates or purified plasma membranes, was performed. A carbonic anhydrase II of 29 kD associated by weak bonds to the inner leaflet of apical plasma membranes of polarized cells was detected. This enzyme was co-localized with markers of Golgi compartments. Moreover, the defect of its targeting to apical plasma membranes in cells treated with brefeldin A was indicative of its transport by the Golgi apparatus. We show here that a carbonic anhydrase II is associated with the inner leaflet of apical plasma membranes and with the cytosolic side of the endomembranes of human cancerous pancreatic duct cells (Capan-1). These observations point to a role for this enzyme in the regulation of intra- and extracellular pH.     

Comparative ultrastructure of coxal glands in unfed larvae of Leptotrombidium orientale (Schluger, 1948) (Trombiculidae) and Hydryphantes ruber (de Geer, 1778) (Hydryphantidae)

Coxal glands of unfed larvae Leptotrombidium orientale (Schluger, 1948) (Trombiculidae), a terrestrial mite parasitizing vertebrates, and Hydryphantes ruber (de Geer, 1778) (Hydryphantidae), a water mite parasitizing insects were studied using transmission electron microscopy. In both species, the coxal glands are represented by a paired tubular organ extending on the sides of the brain from the mouthparts to the frontal midgut wall and are formed of the cells arranged around the central lumen. As in other Parasitengona, the coxal glands are devoid of a proximal sacculus. The excretory duct, joining with ducts of the prosomal salivary glands constitutes the common podocephalic duct, opening into the subcheliceral space. The coxal glands of L. orientale are composed of a distal tubule with a basal labyrinth, an intermediate segment without labyrinth, and a proximal tubule bearing tight microvilli on the apical cell surface and coiled around the intermediate segment. The coxal glands of H. ruber mainly consist of the uniformly organized proximal tubule with apical microvilli of the cells lacking the basal labyrinth. This tubule shows several loops running backward and forward in a vertical plane on the side of the brain. In contrast to L. orientale , larvae of H. ruber reveal a terminal cuticular sac/bladder for accumulation of secreted fluids. Organization of the coxal glands depends on the ecological conditions of mites. Larvae of terrestrial L. orientale possess distal tubule functioning in re‐absorption of ions and water. Conversely, water mite larvae H. ruber need to evacuate of the water excess, so the filtrating proximal tubule is prominent.     

Isolation and monolayer culture of guinea pig pancreatic duct epithelial cells

Summary Monolayers of cultured epithelial cells have been prepared from fragments of guinea pig pancreatic excretory ducts isolated by a simple procedure employing collagenase digestion and manual selection, through which virtually all of the ductal system can be recovered. The isolated fragments were cultured in enriched Waymouth's medium on extracellular matrices of various composition and thickness, including: thin (<5 μm) and thick (0.5 mm) layers of rat tail collagen; thin layers of human placental collagen; thin layers of Matrigel (a reconstituted basement membrane material); uncoated tissue culture plastic; and the cellulose ester membranes of Millipore Millicells. Cells spread rapidly from duct fragments cultured on uncoated plastic or on plastic coated with thin layers of rat tail collagen or human placental collagen and formed epithelial monolayers. However, these cells were squamous and lacked the abundant basolateral membrane amplification and apical microvilli characteristic of freshly isolated duct epithelial cells. Cells did not spread from duct fragments cultured on Matrigel. In contrast, when fragments of pancreatic ducts were explanted onto either a thick layer of rat tail collagen or onto Millicell membranes, cells readily spread and formed confluent monolayers of cuboidal epithelial cells characterized by abundant mitochondria, apical microvilli, and basolateral plasma membrane elaboration. These results demonstrate that different forms of extracellular matrix modulate the growth and differentiation of pancreatic duct epithelial cells, and that culture on a permeable substrate markedly enhances the maintenance of differentiated characteristics in this cell type. The monolayers formed on Millicell membranes should provide a useful model system for physiologic analysis of the regulation of electrolyte secretion by this epithelium. This research was supported by grants DK32994 and DK35912 from the National Institutes of Health, Bethesda, MD.     

Alkaline phosphatase activity of the IVth ventricular choroidal epithelium of rats during embryonic and neonatal development

The cytochemical localization of alkaline phosphatase (AlPase) activity in the developing IVth ventricular choroidal epithelium was investigated in embryonic and neonatal rats. During the initial development of the choroidal primodium the flattened and/or cuboidal epithelial cells of the ventricular roof were changed to columnar cells with well-developed microvilli and apical tight junctions. When compared to AlPase activity on the lateral plasma membranes of the surrounding ependymal cells, these columnar cells of the choroidal primodium revealed activity on the lateral and luminal plasma membranes, but no activity was found on the basal surface of these cells. On the other hand, the epithelial cells in the neonatal choroid plexus showed a continuous morphological alteration from columnar cells with short microvilli to mature cuboidal cells with numerous long microvilli. AlPase activity in immature columnar cells was observed on all plasma membranes, except for the apical junctional area of the lateral surface. With maturing of the choroidal epithelial cells, the activity appeared to be eliminated from the lateral and luminal plasma membranes of the cuboidal cells, and mature choroidal epithelial cells showed activity on the basal surface only. These findings suggest that AlPase may play an important role in the membrane activity of epithelial cells differentiating between the primitive epithelial cells of the ventricular roof and the mature choroidal epithelial cells.