Synthesis and secretion of the enamel matrix precursor by the kitten secretory ameloblast

Secretory ameloblasts in kitten molar tooth germs were examined with an electron microscope to analyze the synthesis and secretion processes of the enamel matrix precursor. The contents of the secretion granule were identified as fine granular material, which observed in both the rough endoplasmic reticulum and the Golgi cisterns, accumulated in the dilated margins of the innermost Golgi cistern and formed condensing vacuoles. The same kind of condensing vacuoles was also produced from the GERL cisterns. During the secretion granule maturation processes in the Golgi region, the contents accumulated densely and the granules grew smaller. In addition, granule-limiting membranes acquired fine, bristle coats. The mature secretion granules then migrated, along microtubules, into the surfaces of the Tomes processes and finally released their contents by a process of exocytosis at the type 1 face which faces the enamel growth region.     

Cell-matrix adhesion: the Wech connection

Integrins link the extracellular matrix to the cytoskeleton via a complex of proteins: the integrin-cytoskeleton link. A recent study in Drosophila has uncovered a new component of the link, Wech, and shown that it is essential for integrin-mediated adhesion.     

The secretory ameloblast of the mini-pig foetus

Electron microscopic investigations of secretory ameloblasts from deciduous tooth germs of mini-pig foetuses and investigations of the ability of various fixatives to preserve these cells in tooth germs immersion-fixed in toto 5 min, 10 min, 15 min, 20 min and 40 min after death of the mother gave the following results:

Calmodulin blocker inhibits Ca++-ATPase activity in secretory ameloblast of rat incisor

Summary The effects of the calmodulin blocker, trifluoperazine (TEP), on membrane-bound Ca⁺⁺ -ATPase, Na⁺ -K⁺ -ATPase (EC 3.6.1.3.) and the ultrastructure of the enamel organ were investigated in the lower incisors of normal and TFP-injected rats. The rats, of about 100 g body weight, were given either 0.2 ml physiological saline or 100 g TFP dissolved in 0.2 ml physiological saline through a jugular vein and fixed by transcardiac perfusion with a formaldehyde-glutaraldehyde mixture at 1 and 2 h after TFP administration. Non-decalcified sections of the enamel organ less than 50 m in thickness, prepared from dissected lower incisors, were processed for the ultracytochemical demonstration of Ca⁺⁺-ATPase and Na⁺-K⁺ -ATPase by the one-step lead method at alkaline pH. In control saline-injected animals the most intense enzymatic reaction of Ca⁺⁺-ATPase was demonstrated along the plasma membranes of the entire cell surfaces of secretory ameloblasts. Moderate enzymatic reaction was also observed in the plasma membranes of the cells of stratum intermedium and papillary layer. Reaction precipitates of Na⁺-K⁺-ATPase activity were localized clearly along the plasma membranes of only the cells of stratum intermedium and papillary layer. The most drastic effect of TFP was a marked disappearance of enzymatic reaction of Ca⁺⁺-ATPase from the plasma membranes of secretory ameloblasts, except for a weak persistent reaction in the basolateral cell surfaces of the infranuclear region facing the stratum intermedium. The cells of stratum intermedium and papillary layer, however, continued to react for Ca⁺⁺-ATPase even after TFP treatment. Similarly, Na⁺-K⁺-ATPase activity in these cells was not inhibited by TFP administration. Ultrastructural examination of secretory ameloblasts revealed that administration of TFP caused no considerable cytological changes and did not act as a cytotoxic agent. These results suggest that secretory ameloblasts may have an active Ca⁺⁺ transport system, which is modulated by an endogenous calmodulin.     

Cytodifferentiation and degeneration of odontoclasts in physiologic root resorption of kitten deciduous teeth

To investigate the cytodifferentiation and degeneration of odontoclasts in physiologic root resorption, we studied deciduous incisors undergoing resorption in 6-month-old kittens by electron microscopy of ultrathin sections. The endogenous peroxidase activity within the cells was also examined by incubating the tissue slices in diaminobenzidine-H2O2 medium. The resorbing tissues, consisting of multinucleated giant cells, macrophages, granular leukocytes, fibroblasts and many blood vessels, were observed at the resorbing surface of the root dentine. Macrophages and granular leukocytes exhibited endogenous peroxidase activity, but mononuclear and multinucleated preodontoclasts and multinucleated odontoclasts did not. These preodontoclasts contained abundant mitochondria, a moderate amount of rough endoplasmic reticulum, stacks of Golgi membranes, lysosomes and numerous polyribosomes scattered throughout the cytoplasm. Many cellular processes extended from their cell surfaces by which the preodontoclasts appeared to fuse to one another during their multinucleation. Concomitant with the multinucleation process, the preodontoclasts developed numerous pale vacuoles throughout the cytoplasm. These vacuoles seemed to arise from some smooth endoplasmic reticula, perhaps representing Golgi-endoplasmic reticulum-lysosome, and the Golgi saccules. However, the preodontoclasts did not yet form a ruffled border and clear zones. When these preodontoclasts came into direct contact with resorbing dentine surfaces, they began to form the clear zones against dentine surfaces. Characteristically, numerous pale vacuoles were accumulated in the cytoplasm adjacent to the clear zone, then they penetrated into the cytoplasm of the clear zone, and with this, ruffles of the plasma membranes appeared. Through a further movement of more pale vacuoles towards the ruffled plasma membranes, the odontoclasts developed typical ruffled borders against the resorbing dentine surfaces. At this differential phase, little pale vacuoles appeared in the Golgi area, but the cisterns of the Golgi apparatus themselves reached their greatest extent during cellular differentiation. Fully differentiated odontoclasts frequently extended long broad cellular processes into the dentinal tubules exposed to the resorption lacunae. Although some odontoclastic processes penetrating the dentinal tubules contained vacuoles and lysosomal structures, most processes lacked any cytoplasmic organelles, and their cytoplasm resembled that of the clear zone. But these processes never exhibited ruffled-border-like structures.(ABSTRACT TRUNCATED AT 400 WORDS)     

The interrelation between the number of deciduous teeth and the morphological maturity of a child

The process of the first dentition is part of a very short period during human development characterised by an extraordinary intensity of growth processes. The main purpose of the present study is to provide information on the relationship between three criteria of biological maturity of children: body height, body weight and the number of milk teeth. The present study is based on a cross-sectional material collected in 30 nurseries in ?ód? (Poland). The analysis was carried out on 1901 children (981 boys and 920 girls) aged from 2 to 36 months. All coefficients of Pearson correlation and partial correlations between the analysed variables are statistically significant at the 0.01 level. The highest value of coefficient correlation was noticed for the relation between dental and chronological age, as well as between dental and morphological age based on body height (about 0.90 and 0.85, respectively). Through an analysis of regression (backward) equations for predicting the number of teeth from chronological age, body weight and body height were calculated. These mathematical equations were confirmed in practice in about 80% of the children. Coefficients of determinations between the analysed variables are high for boys and girls (about 72% and 74%, respectively). This observations demonstrate conclusively that there exists a highly significant relation between deciduous tooth age and morphological age.     

The role of mitochondria in direct cell-to-cell connection dependent rescue of postischemic cardiomyoblasts

In this in vitro study we induced ischemic injury on H9c2 rat cardiomyoblasts using the oxygen-glucose deprivation model (OGD). We monitored if the addition of healthy or mitochondria-depleted cells can save OGD treated cells from post-ischemic injury. We were able to significantly improve the surviving cell number of oxidatively damaged H9c2 cells by the addition of healthy cells to the culture. On the contrary, cells with disturbed mitochondria did not increase the number of surviving cells. High-resolution confocal time-lapse imaging also proved that mitochondria are drifting from cell-to-cell through tunneling membrane bridges, however, they do not get into the cytoplasm of the other cell. We conclude that addition of healthy cells to severly injured post-ischemic cardiomyoblasts can rescue them from death during the first 24h after reoxigenation. Grafted cells must maintain their mitochondria in an actively respiring state, and although cell contact is required for the mechanism, neither cell fusion nor organelle transfer occurs. This novel mechanism opens a new possiblity for cell-based cardiac repair in ischemic heart disease.     

Fine structure of the secretory and non-secretory ameloblasts in the frog. II. Fine structure of the non-secretory ameloblast.

The non-secretory ameloblasts present at the enamel-free surfaces of maxillary teeth in the frog Rana pipiens were examined by electron microscopy at different stages of tooth development. Their main fine structural features seem to reflect a transport function. During early tooth development, the non-secretory ameloblasts adjacent to odontoblasts and predentin exhibit extensive lateral surface specializations and numerous cytoplasmic vesicles. During late tooth development, the non-secretory ameloblasts adjacent to mineralizing dentin show numerous cellular junctions, well-developed intercellular channels with numerous interdigitating processes and labyrinthine configurations at their distal surfaces. An intact basal lamina is present between the non-secretory ameloblasts and the dentin surface until the dentin becomes fully mineralized. At this stage the adjacent cells no longer exhibit surface specializations. It is suggested that the non-secretory ameloblasts may participate in the mineralization of adjacent dentin at the enamel-free surfaces. This surface dentin becomes fully mineralized at a later stage of development than the underlying dentin.     

Spatial organization and interrelation of structural elements of the 1st layer of the neocortex

Investigating topography and structure of elements in the layer I of the fields 4, 3, 1 of the human neocortex (4 cases) and M1, Ep zones in the cat neocortex (5 cases) by means of modified methods of Golgi, Peters and Kluver-Barerr, it became possible to work out an original classification of astrocytes and to reveal the neurono-glio-vascular complexes consisting of the neuronal base and two glial-vascular links. Three main varieties of protoplasmic astrocytes are determined: short-rayed with a long dendrite-like process, short-rayed cap-like and long-rayed with a double bush of branchings. In the latter forms axon-like processes are revealed, some of them make complex basket-like branchings and each of them surrounds a group of neuronal bodies, predominantly the pyramidal ones in the layer III. Distribution of the marginal glia and the three mentioned varieties of astrocytes is subjected to a single plan. The raws of gliocytes along the horizontal and vertical lines are connected with each other and with the neuronal elements. Peculiar receptive apparatuses performing interrelation are ball-like formations revealed on the apical dendrites of the pyramidal neurons. The information that gets into them is processed automatically. Problems concerning the importance of the ball-like formations in integration of the layer I is discussed, and the role of the glial cells with axon-like processes in the active transport of various substances and in regulating metabolism of the pyramidal cells of the layer III is also dealt with.     

Ameloblastic secretion and calcification of the enamel layer in shark teeth

Tooth primordia at early stages of mineralization in the sharks Negaprion brevirostris and Triaenodon obesus were examined electron microscopically for evidence of ameloblastic secretion and its relation to calcification of the enamel (enameloid) layer. Ameloblasts are polarized with most of the mitochondria and all of the Golgi dictyosomes localized in the infranuclear end of the cell toward the squamous outer cells of the enamel organ. Endoplasmic reticular membranes and ribosomes are also abundant in this region. Ameloblastic vesicles bud from the Golgi membranes and evidently move through perinuclear and supranuclear zones to accumulate at the apical end of the cell. The vesicles secrete their contents through the apical cell membrane in merocrine fashion and appear to contribute precursor material both for the basal lamina and the enameline matrix. The enamel layer consists of four zones: a juxta-laminar zone containing newly polymerized mineralizing fibrils (tubules); a pre-enamel zone of assembly of matrix constituents; palisadal zones of mineralizing fibrils (tubules); and interpalisadal zones containing granular amorphous matrix, fine unit fibrils, and giant cross-banded fibers with a periodicity of 17.9 nm. It seems probable that amorphous, non-mineralizing fibrillar and mineralizing fibrillar constituents of the matrix are all products of ameloblastic secretion. Odontoblastic processes are tightly embedded in the matrix of the palisadal zones and do not appear to be secretory at the stages investigated. The shark tooth enamel layer is considered homologous with that of other vertebrates with respect to origin of its mineralizing fibrils from the innerental epithelium. The term enameloid is appropriate to connote the histological distinction that the enamel layer contains odontoblastic processes but should not signify that shark tooth enamel is a modified type of dentine. How amelogenins and/or enamelins secreted by amelo- blasts in the shark and other vertebrates are related to nucleation and growth of enamel crystallites is still not known.     

On the pattern of ameloblast migration

Abstract The kinetics of ameloblast cells in continuously growing guinea pig molars were studied using autoradiography. The results showed that there was no direct relationship between ameloblast migration rate and ameloblast production rate, which indicated that ameloblasts actively migrated coronally. It was found that ameloblast migration rate was maximal at the root apex, and then reduced to a minimum value as the ameloblasts left their proliferative compartment and migrated coronally. A multiple regression model was found to be the most suitable one to represent the ameloblast migration pattern.     

On the pattern of ameloblast migration

The kinetics of ameloblast cells in continuously growing guinea pig molars were studied using autoradiography. The results showed that there was no direct relationship between ameloblast migration rate and ameloblast production rate, which indicated that ameloblasts actively migrated coronally. It was found that ameloblast migration rate was maximal at the root apex, and then reduced to a minimum value as the ameloblasts left their proliferative compartment and migrated coronally. A multiple regression model was found to be the most suitable one to represent the ameloblast migration pattern.     

Influence of nitric oxide on the secretory function of the bovine corpus luteum: dependence on cell composition and cell-to-cell communication

The objective of the present study was to investigate the role of cell-to-cell contact in the influence of nitric oxide (NO) on the secretory function of the bovine corpus luteum (CL). In Experiment 1, separate small luteal cells (SLC) or large (LLC) luteal cells were perfused with 100 micro M spermineNONOate, a NO donor, or with 100 micro M Nomega-nitro-L-arginine methyl ester (L-NAME), a NO synthase (NOS) inhibitor; in Experiment 2, a mixture of LLC and SLC and endothelial cells was cultured and incubated with spermineNONOate or L-NAME; in Experiment 3, spermineNONOate was perfused into the CL (100 mg/4 hr) by a microdialysis system in vivo. Perfusion of isolated SLC and LLC with the NO donor or NOS inhibitor (Experiment 1) did not affect (P > 0.05) secretion of progesterone (P(4)) or oxytocin (OT). L-NAME perfusion increased (P < 0.05) leukotriene C(4) (LTC(4)) secretion by both SLC and LLC cells. Treatment of mixtures of luteal cells with an NO donor (Experiment 2) significantly decreased (P < 0.001) secretion of P(4) and OT and increased (P < 0.001) production of prostaglandin F(2alpha) (PGF(2alpha)) and LTC(4). L-NAME stimulated (P < 0.001) P(4) secretion, but did not influence (P > 0.05) OT, PGF(2alpha) or LTC(4) production. Intraluteal administration (Experiment 3) of spermineNONOate increased (P < 0.001) LTC(4) and PGF(2alpha), decreased OT, but did not change P(4) levels in perfusate samples. These data indicate that cell-to-cell contact and cell composition play important roles in the response of bovine CL to treatment with NO donors or NOS inhibitors, and that paracrine mechanisms are required for the full secretory response of the CL in NO action. Endothelial cells appear to be required for the full secretory response of the CL to NO.     

Finite Element Modeling Predictions of Region-specific Cell-matrix Mechanics in the Meniscus

The knee meniscus exhibits significant spatial variations in biochemical composition and cell morphology that reflect distinct phenotypes of cells located in the radial inner and outer regions. Associated with these cell phenotypes is a spatially heterogeneous microstructure and mechanical environment with the innermost regions experiencing higher fluid pressures and lower tensile strains than the outer regions. It is presently unknown, however, how meniscus tissue mechanics correlate with the local micromechanical environment of cells. In this study, theoretical models were developed to study mechanics of inner and outer meniscus cells with varying geometries. The results for an applied biaxial strain predict significant regional differences in the cellular mechanical environment with evidence of tensile strains along the collagen fiber direction of ~0.07 for the rounded inner cells, as compared to levels of 0.02–0.04 for the elongated outer meniscus cells. The results demonstrate an important mechanical role of extracellular matrix anisotropy and cell morphology in regulating the region-specific micromechanics of meniscus cells, that may further play a role in modulating cellular responses to mechanical stimuli.     

Effects of short-term and prolonged flickering on the system of cytochromeoxidase modules of the kitten primary visual cortex IV layer

CO "spots" in layer IV of primary visual cortex were investigated in 33, 49 and 93-days kittens that were subjected to flickering light stimulation. Kittens from first group were stimulated since eye opening (long-term stimulation), other kittens--since postnatal day 26, 42 or 85 until euthanasia (short-term stimulation). Both types of stimulation did not disturb CO "spots" spatial organization but obviously increased a contrast of splenial CO "spots". Lateral "spots" contrast increasing took place after long-term stimulation until the 93rd postnatal day or after short stimulation since 26th to 33rd postnatal day. Flickering light stimulation seems to lead to structural and metabolic alterations in primary visual cortex. These alterations are processed in different way in regions of area 17 that is responsible for central and peripheral vision, respectively. It seems to reflect, firstly, primary activation of Y processing stream and, secondly, the strengthening of contralateral input to area 17.     

Histochemical and electron probe analysis of secretory ameloblasts of developing rat molar teeth

Calcium was not found in secretory ameloblasts and stratum intermedium cells when treated with OsO4-pyroantimonate or when surfaces prepared by fracturing fresh, rapidly frozen, developing molar tooth germs were subject to electron probe X-ray analysis. Pyroantimonate reaction product, considered to be calcium, was found in mitochondria of enamel organ cells which were first placed in a bath containing calcium and potassium. The plasma membrane was disrupted in cells ehich showed mitochondrial localization of reaction product. The results provide no data which indicates that enamel organ cells have a direct, active role in the movement of calcium into the enamel. Rather, it is suggested that the secretory enamel organ might serve as a selective barrier in regulating the initial mineralization of enamel.     

成釉质细胞分化机制的研究进展

牙齿的发育是由牙上皮和神经脊来源的间充质之间的连续的相互诱导产生的.上皮和间充质之间连续的相互诱导,使得上皮细胞分化为具有分泌牙釉质功能的成釉质细胞,而间充质细胞分化为具有分泌牙本质功能的成牙本质细胞.成釉质细胞的正常分化对于形成正常的牙釉质是至关重要的,本文主要对细胞信号分子、细胞黏附分子、釉质特异性基因和转录因子等在成釉质细胞分化过程中的作用做一概述.