Your search keyword '"Tooth Germ metabolism"' showing total 63 results

1. Liver-type of tissue non-specific alkaline phosphatase is induced during mouse bone and tooth cell differentiation.

Author

Baba TT, Terashima T, and Oida S

Subjects

Alkaline Phosphatase genetics, Animals, Bone Morphogenetic Protein 2 metabolism, Bone and Bones pathology, Cell Line, Female, Gene Expression, Mice, Myoblasts, Organ Culture Techniques, Osteoblasts pathology, RNA, Messenger metabolism, Tooth Germ pathology, Alkaline Phosphatase metabolism, Bone and Bones metabolism, Cell Differentiation, Liver metabolism, Tooth Germ metabolism

Abstract

Background and Objective: Tissue non-specific alkaline phosphatase (TNSALP) contains two types-bone- and liver-type-which are produced from the same gene due to differences in splicing. These two differ in their promoter, but the amino acid sequences of the mature proteins are identical. In this study, we examined the relationship between the two types of TNSALP expression and osteoblast differentiation., Design: Gene expression of the two types of TNSALP was observed by reverse transcription-polymerase chain reaction. MC3T3-NM4 was sub-cloned from an established mouse osteoblastic cell line in which osteoblast characters do not appear without dexamethasone. The C2C12 mouse myoblastic cell line, which can be induced to osteoblasts with bone morphogenic protein 2, and organ-cultured tooth germs were also used in this work., Results: The gene expression of liver-type TNSALP was observed in only MC3T3-NM4 activated by dexamethasone. For C2C12, the gene expression of bone-type TNSALP was observed even in non-induced conditions where myotubes were formed, whereas the liver-type TNSALP mRNA was only expressed when C2C12 differentiated into osteoblasts by bone morphogenic protein 2. Furthermore, in the organ-cultured tooth germs, the liver-type TNSALP mRNA was expressed according to differentiation of tooth germs., Conclusion: These results suggest that the liver-type TNSALP mRNA is induced according to differentiation of bone and tooth., (Copyright © 2018 Elsevier Ltd. All rights reserved.)

Published

2019

2. Expression of planar cell polarity genes during mouse tooth development.

Author

Obara N, Suzuki Y, Irie K, and Shibata S

Subjects

Animals, Cadherins, Dishevelled Proteins, Frizzled Receptors, Gene Expression Regulation, Developmental, In Situ Hybridization, Mice, Nerve Tissue Proteins, Receptors, G-Protein-Coupled, Signal Transduction, Tooth Germ metabolism, Carrier Proteins genetics, Cell Polarity genetics, Membrane Proteins genetics, Odontoblasts metabolism, Odontogenesis genetics

Abstract

Objective: Planar cell polarity (PCP) refers to the cell polarity across the tissue plane and controls various cell behaviors and structures. Although the expression of several PCP signaling components has been detected in tooth germs, knowledge of the gene expression patterns of these PCP components during tooth development remains incomplete. The aim of this study is to characterize the temporal and spatial changes in PCP gene expression during tooth development., Design: Expression of Celsr1 and 2, Fzd3 and 6, Vangl1 and 2, and Dvl1-3 genes was analyzed in mouse molar germs from the bud to the bell stage using in situ hybridization., Results: At the bud stage, all target genes were expressed in all areas of the tooth bud. In the enamel organ at the cap stage, expression of Fzd3 was suppressed in the enamel knot, whereas Fzd6 was strongly expressed there. Expression of Vangl2 was strongly expressed in the inner dental epithelium from the cap stage onwards. In the inner dental epithelium, strong expression of Fzd3, Dvl2 and Vangl2 was noted at the early bell stage, and of Celsr1, Fzd3, Fzd6, Vangl2 and Dvl2 at the bell stage. Furthermore, differentiated odontoblasts strongly expressed Celsr1, Vangl2, and Dvl2., Conclusion: The gene expression patterns delineated in this study improve our understanding of the role(s) of PCP components during tooth development., (Copyright © 2017 Elsevier Ltd. All rights reserved.)

Published

2017

3. Different expression patterns of Lin28 and Lin28b in mouse molar development.

Author

Dong N, Liu Y, Zhang T, Zhao L, Tian J, and Ruan J

Subjects

Animals, Blotting, Western, Cell Differentiation, Immunoenzyme Techniques, Mice, Tooth Germ cytology, DNA-Binding Proteins metabolism, Molar embryology, Odontogenesis physiology, RNA-Binding Proteins metabolism, Tooth Germ metabolism

Abstract

Objective: The RNA-binding proteins Lin28 and Lin28b are expressed in many developing tissues and are involved in the biosynthesis of the microRNA let-7 family and embryogenesis processes. However, their roles in mammalian tooth development remain ill-defined., Design: The spatiotemporal expressions of Lin28 and Lin28b during mouse molar odontogenesis from day E11.5 to P21 were examined through immunohistochemistry and western blot analysis., Results: Both Lin28 and Lin28b were initially expressed in dental epithelium, but the expression patterns varied thereafter. Lin28 was expressed in tooth germ from early embryonic stages and was consistently expressed in the ameloblasts and odontoblasts throughout all stages of tooth development. However, positive staining of Lin28b gradually faded out with tooth germ development, before finally disappearing in tooth organ cells after birth., Conclusions: These results indicate that Lin28 was spatiotemporally expressed in tooth germ throughout tooth development progression and may play an active role in ameloblast and odontoblast differentiation, as well as matrix secretion and the mineralization of enamel and dentin. Its paralogue Lin28b may have a distinct function in tooth germ formation., (Copyright © 2017 Elsevier Ltd. All rights reserved.)

Published

2017

4. F-spondin negatively regulates dental follicle differentiation through the inhibition of TGF-β activity.

Author

Orimoto A, Kurokawa M, Handa K, Ishikawa M, Nishida E, Aino M, Mitani A, Ogawa M, Tsuji T, and Saito M

Subjects

Adenoviridae genetics, Animals, Animals, Genetically Modified, Cell Adhesion Molecules genetics, Cell Adhesion Molecules metabolism, Cell Differentiation physiology, Cell Line, Collagen Type I genetics, Collagen Type I metabolism, Core Binding Factor Alpha 1 Subunit genetics, Core Binding Factor Alpha 1 Subunit metabolism, Dental Sac cytology, Dental Sac metabolism, Extracellular Matrix Proteins genetics, Gene Expression drug effects, Gene Knockdown Techniques, In Situ Hybridization, Mesenchymal Stem Cells cytology, Mice, Inbred C57BL, Periodontal Ligament cytology, Periodontal Ligament drug effects, Periodontal Ligament growth & development, Periodontal Ligament metabolism, Recombinant Proteins, Tooth Germ cytology, Tooth Germ drug effects, Tooth Germ metabolism, Tooth Root growth & development, Tooth Root metabolism, Transforming Growth Factor beta metabolism, Cell Differentiation drug effects, Dental Sac drug effects, Extracellular Matrix Proteins metabolism, Transforming Growth Factor beta pharmacology

Abstract

Objective: F-spondin is an extracellular matrix (ECM) protein that belongs to the thrombospondin type I repeat superfamily and is a negative regulator of bone mass. We have previously shown that f-spondin is specifically expressed in the dental follicle (DF), which gives rise to the periodontal ligament (PDL) during the tooth root formation stage. To investigate the molecular mechanism of PDL formation, we investigated the function of f-spondin in DF differentiation., Design: The expression patterning of f-spondin in the developing tooth germ was compared with that of periodontal ligament-related genes, including runx2, type I collagen and periostin, by in situ hybridization analysis. To investigate the function of f-spondin during periodontal ligament formation, an f-spondin adenovirus was infected into the bell stage of the developing tooth germ, and the effect on dental differentiation was analyzed., Results: F-spondin was specifically expressed in the DF of the developing tooth germ; by contrast, type I collagen, runx2 and periostin were expressed in the DF and in the alveolar bone. F-spondin-overexpresssing tooth germ exhibited a reduction in gene expression of periostin and type I collagen in the DF. By contrast, the knockdown of f-spondin in primary DF cells increased the expression of these genes. Treatment with recombinant f-spondin protein functionally inhibited periostin expression induced by transforming growth factor-β (TGF-β)., Conclusion: Our data indicated that f-spondin inhibits the differentiation of DF cells into periodontal ligament cells by inhibiting TGF-β. These data suggested that f-spondin negatively regulates PDL differentiation which may play an important role in the immature phenotype of DF., (Copyright © 2017 Elsevier Ltd. All rights reserved.)

Published

2017

5. Altered distribution of Ghrelin protein in mice molar development.

Author

Liu B, Han X, Feng W, Cui J, Hasegawa T, Amizuka N, Xu X, and Li M

Subjects

Ameloblasts cytology, Ameloblasts metabolism, Animals, Apoptosis drug effects, Cell Differentiation drug effects, Cell Proliferation drug effects, Dental Enamel cytology, Dental Enamel embryology, Dental Enamel metabolism, Enamel Organ embryology, Enamel Organ growth & development, Enamel Organ metabolism, Epithelium embryology, Epithelium metabolism, Female, Immunohistochemistry, Mice, Mice, Inbred ICR, Molar cytology, Molar drug effects, Molar growth & development, Odontoblasts cytology, Odontoblasts metabolism, Odontogenesis drug effects, Odontogenesis physiology, Pregnancy, Tooth Germ embryology, Tooth Germ growth & development, Tooth Germ metabolism, Tooth Root embryology, Tooth Root growth & development, Tooth Root metabolism, Ghrelin biosynthesis, Ghrelin metabolism, Molar metabolism

Abstract

Objective: Ghrelin, an appetite-stimulating hormone, plays diverse regulatory functions in cell growth, proliferation, differentiation and apoptosis during mammalian development. There is limited information currently available regarding Ghrelin expression during mammalian tooth development, thus we aimed to establish the spatiotemporal expression of Ghrelin during murine molar odontogenesis., Design: Immunohistochemistry was performed to detect the expression pattern of Ghrelin in mandible molar from E15.5 to PN7 during murine tooth development., Results: The results showed that Ghrelin initially expressed in the inner enamel epithelium and the adjacent mesenchymal cells below, further with persistent expression in the ameloblasts and odontoblasts throughout the following developmental stages. In addition, Ghrelin was also present in Hertwig's epithelial root sheath at the beginning of tooth root formation., Conclusions: These results suggest that Ghrelin was present in tooth organs throughout the stages of tooth development, especially in ameloblasts and odontoblasts with little spatiotemporal expression differences. However, the potential regulatory roles of this hormone in tooth development still need to be validated by functional studies., (Copyright © 2016 Elsevier Ltd. All rights reserved.)

Published

2016

6. Analysis of expression patterns of IGF-1, caspase-3 and HSP-70 in developing human tooth germs.

Author

Kero D, Kalibovic Govorko D, Medvedec Mikic I, Vukojevic K, Cigic L, and Saraga-Babic M

Subjects

Cell Differentiation, Cuspid cytology, Cuspid embryology, Cuspid metabolism, Dental Enamel metabolism, Dental Papilla cytology, Dental Papilla embryology, Dental Papilla growth & development, Dental Papilla metabolism, Enamel Organ cytology, Enamel Organ embryology, Enamel Organ metabolism, Fetus, Humans, Immunohistochemistry, Incisor embryology, Incisor metabolism, Odontogenesis, Tooth Germ cytology, Tooth Germ embryology, Caspase 3 biosynthesis, HSP70 Heat-Shock Proteins biosynthesis, Insulin-Like Growth Factor I biosynthesis, Tooth Germ metabolism

Abstract

Aims: To analyze expression patterns of IGF-1, caspase-3 and HSP-70 in human incisor and canine tooth germs during the late bud, cap and bell stages of odontogenesis., Materials and Methods: Head areas or parts of jaw containing teeth from 10 human fetuses aged between 9th and 20th developmental weeks were immunohistochemically analyzed using IGF-1, active caspase-3 and HSP-70 markers. Semi-quantitative analysis of each marker's expression pattern was also performed., Results: During the analyzed period, IGF-1 and HSP-70 were mostly expressed in enamel organ. As development progressed, expression of IGF-1 and HSP-70 became more confined to differentiating tissues in the future cusp tip area, as well as in highly proliferating cervical loops. Few apoptotic bodies highly positive to active caspase-3 were observed in enamel organ and dental papilla from the cap stage onward. However, both enamel epithelia moderately expressed active caspase-3 throughout the investigated period., Conclusions: Expression patterns of IGF-1, active caspase-3 and HSP-70 imply importance of these factors for early human tooth development. IGF-1 and HSP-70 have versatile functions in control of proliferation, differentiation and anti-apoptotic protection of epithelial parts of human enamel organ. Active caspase-3 is partially involved in formation and apoptotic removal of primary enamel knot, although present findings might reflect its ability to perform other non-death functions such as differentiation of hard dental tissues secreting cells and guidance of ingrowth of proliferating cervical loops., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

7. Immunohistochemical expression of CD56 in dog (Canis familiaris) odontogenesis.

Author

Nel S, van Heerden M, and van Heerden W

Subjects

Ameloblastoma metabolism, Ameloblastoma veterinary, Animals, Cell Differentiation physiology, Dental Papilla cytology, Dental Papilla metabolism, Enamel Organ cytology, Enamel Organ metabolism, Epithelial Cells cytology, Epithelial Cells metabolism, Female, Immunohistochemistry veterinary, Tooth Germ cytology, Tooth Germ metabolism, Vagus Nerve cytology, Vagus Nerve metabolism, CD56 Antigen biosynthesis, Dogs growth & development, Dogs metabolism, Odontogenesis physiology

Abstract

Aim: To investigate the expression of CD56 in dog odontogenesis in order to elucidate the expression found in ameloblastomas., Materials and Methods: Immunohistochemical analysis of CD56 expression of developing dog teeth in the bud, cap and bell stages including the remnants of the dental lamina., Results: Weak CD56 expression was observed in the dental epithelium during the bud stage with intense staining of certain peripheral epithelial cells. Positive staining of epithelial cells was also observed in the cap stage with intense staining of the inner enamel epithelium at this stage. During the bell stage the staining was concentrated on the cervical loop areas. The dental papilla revealed positive staining throughout the cap and bell stages while the dental follicle stained intensely positive throughout all the phases examined. The dental lamina and Serres rests also stained positive for CD56., Conclusions: The expression of CD56 in dog odontogenic tissue varies according to the stage of tooth development. There is a positive correlation between the positive staining observed in ameloblastomas and their odontogenic cells of origin., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

8. Expression of Ki-67, Oct-4, γ-tubulin and α-tubulin in human tooth development.

Author

Kero D, Novakovic J, Vukojevic K, Petricevic J, Kalibovic Govorko D, Biocina-Lukenda D, and Saraga-Babic M

Subjects

Ameloblasts metabolism, Cell Differentiation, Cell Proliferation, Dental Enamel metabolism, Fluorescent Antibody Technique, Humans, Immunoenzyme Techniques, Tooth Germ metabolism, Ki-67 Antigen metabolism, Octamer Transcription Factor-3 metabolism, Odontogenesis physiology, Tooth embryology, Tooth metabolism, Tubulin metabolism

Abstract

Aims: To analyze factors controlling cell proliferation and differentiation, and appearance of primary cilia during the cap and bell stages of incisor or/and canine human enamel organs., Materials and Methods: Qualitative and quantitative analysis of proliferating Ki-67 positive cells and expression of γ-tubulin, α-tubulin and Oct-4 was immunohistochemically analyzed in the cap an bell stages of 10 developing human incisor and canine germs, 8-21 weeks old., Results: During the analyzed period, ratio of Ki-67 positive cells changed in outer enamel epithelium from 48.86% to 24.52%, in inner enamel epithelium increased from 56.11% to 60.06% and then dropped to 44.24%. While in dental papilla proliferation first increased from 46.26% to 55.45%, and then dropped to 22.08%, a constant decrease of proliferation characterized enamel reticulum (from 46.26% to 15.49%). Strong cytoplasmic Oct-4 expression characterized epithelial parts of enamel organ, particularly the differentiating ameloblasts. During further development, Oct-4 expression shifted to both nuclear and cytoplasmic expression in mesenchymal tooth components. Primary cilia characterized most of the cells in developing enamel organ. While non-ciliated (proliferating) cells mainly contained two centrioles (γ-tubulin), the primary cilia (α-tubulin) were arising from basal bodies (γ-tubulin) of non-proliferating cells., Conclusions: We suggest that increase in cell proliferation enables growth of enamel organ, while its selective decrease leads to disintegration of some tooth parts. Drop of proliferation coincided with initiation of ameloblast and odontoblast differentiation. Additionally, cell differentiation was accompanied by increased expression of Oct-4 and probably by signalling via primary cilia, both regulating processes of cell proliferation and differentiation., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2014

9. Regulation of CCN2 gene expression and possible roles in developing tooth germs.

Author

Kanyama M, Shimo T, Sugito H, Nagayama M, Kuboki T, Pacifici M, and Koyama E

Subjects

Analysis of Variance, Animals, CCN Intercellular Signaling Proteins metabolism, Cell Culture Techniques, Enzyme-Linked Immunosorbent Assay, In Situ Hybridization, Mesenchymal Stem Cells, Mice, Odontogenesis physiology, Tooth Germ metabolism, Bone Morphogenetic Proteins metabolism, CCN Intercellular Signaling Proteins genetics, Fibroblast Growth Factors metabolism, Gene Expression Regulation, Developmental physiology, Odontogenesis genetics, Tooth Germ embryology

Abstract

CCN proteins are extracellular and cell-associated molecules involved in several developmental processes, but their expression patterns and regulation in tooth development remain unclear. Here we first determined the expression patterns of CCN genes in mouse tooth germs. We found that at early stages CCN2 was detected in dental lamina, dental mesenchyme, and primary enamel knot, while other CCN family members were expressed broadly. By the bell stage, all members were expressed in differentiating odontoblasts and ameloblasts, but CCN1 and CCN2 transcripts were conspicuous in differentiating osteoblasts in dental follicle. Next, we asked what signalling molecules regulate CCN2 expression and what roles CCN2 may have. We found that upon surgical removal of dental epithelium CCN2 was not longer expressed in dental mesenchyme in cultured bud stage germs. Implantation of beads pre-coated with BMPs and FGFs onto E12-13 mandibular explants induced CCN2 expression in dental mesenchyme. There was a dose-dependent effect of BMP-4 on CCN2 induction; a concentration of 100 ng/μl was able to induce strong CCN2 expression while a minimum concentration of 25 ng/μl was needed to elicit appreciable expression. Importantly, Noggin treatment inhibited endogenous and BMP-induced CCN2 expression, verifying that CCN2 expression in developing tooth germs requires BMP signalling. Lastly, we found that rCCN2 stimulated proliferation in dental mesenchyme in a dose-dependent manner. Together, the data indicate that expression of CCN genes is spatio-temporally regulated in developing tooth germs. CCN2 expression appears to depend on epithelial and mesenchymal-derived signalling factors, and CCN2 can elicit strong proliferation in dental mesenchyme., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published

2013

10. Expression, localisation and synthesis of versican by the enamel organ of developing mouse molar tooth germ: an in vivo and in vitro study.

Author

Jiang BZ, Yokohama-Tamaki T, Wang ZL, Obara N, and Shibata S

Subjects

Animals, Chondroitin Sulfates analysis, Chromatography, Gel, Dental Papilla embryology, Dental Sac embryology, Enamel Organ metabolism, Epithelium embryology, Gestational Age, Immunohistochemistry, In Situ Hybridization, Keratin-14 analysis, Mesoderm embryology, Mice, Mice, Inbred ICR, Molar embryology, Organ Culture Techniques, Proteoglycans analysis, Radiopharmaceuticals, Reverse Transcriptase Polymerase Chain Reaction, Sulfur Radioisotopes, Tooth Germ metabolism, Versicans biosynthesis, Vimentin analysis, Enamel Organ embryology, Tooth Germ embryology, Versicans analysis

Abstract

Objective: Versican is a large, aggregating chondroitin sulphate proteoglycan. In dental tissue, versican expression occurs primarily in mesenchymal tissue but rarely in epithelial tissue. We investigated the expression, localisation and synthesis of versican in the enamel organ of the developing tooth germ., Design: To elucidate versican localisation in vivo, in situ hybridisation and immunohistochemistry were conducted in foetal ICR mice at E11.5-E18.5. Epithelium and mesenchyme from the lower first molars at E16.0 were enzymatically separated and versican mRNA expression was investigated by semi-quantitative RT-PCR. Organ culture of the separated samples combined with metabolic labelling with [(35)S], followed by gel filtration, was performed to analyse secreted proteoglycans., Results: Versican mRNA was first expressed in the thickened dental epithelium at E12.0 and continued to be expressed in the enamel organ until the bell stage. Versican immunostaining was detected in the stellate reticulum areas from the bud stage to the apposition stage. The enamel organ at E16.0 expressed versican mRNA at a level comparable to that in dental mesenchyme. Furthermore, when compared to dental mesenchyme, about 1/2-3/4 of the [(35)S]-labelled versican-like large proteoglycan was synthesised and released into tissue explants by the enamel organ., Conclusions: The dental epithelium of developing tooth germ is able to synthesise significant amounts of versican., (Copyright © 2010 Elsevier Ltd. All rights reserved.)

Published

2010

11. Development of deciduous and permanent dentitions in the upper jaw of the house shrew (Suncus murinus).

Author

Yamanaka A, Yasui K, Sonomura T, Iwai H, and Uemura M

Subjects

Animals, Dentition, Permanent, Hedgehog Proteins metabolism, Imaging, Three-Dimensional, In Situ Hybridization, Shrews metabolism, Tooth Germ metabolism, Tooth, Deciduous, Maxilla embryology, Odontogenesis physiology, Shrews embryology, Tooth Germ embryology

Abstract

The diphyodont tooth replacement in mammals is characterized by a single replacement of a deciduous dentition by a permanent dentition. Despite its significance in mammalian biology and paleontology, little is known about the developmental mechanisms regulating the diphyodont replacement. Because the mouse never replaces its teeth, this study used the house shrew, Suncus murinus, as a model to investigate the control of the diphyodont replacement of a deciduous dentition by successions and additions of permanent teeth. Using morphological and gene expression analyses of serial sections, we have demonstrated the development of the upper dentition of the house shrew. In this species, the deciduous tooth germs are formed but soon become vestigial, whereas the successional and accessional (molar) germs are subsequently formed and developed. There are distinct Shh expression domains in the deciduous, successional, and accessional tooth germs, and those of the latter two germs are identified from the appearance of their primary enamel knots. The developmental sequence of tooth germs in the house shrew indicates that two adjacent primary enamel knots of the successional and accessional germs do not develop simultaneously, but with a constant time lag. We suggest that this mode of tooth succession and accession can be explained by a sequential inhibitory cascade model in which the timing of initiation and the spacing of tooth development are determined by the inhibition from the primary enamel knots of developmentally preceding adjacent tooth germs.

Published

2010

12. Expression of Wnt5a in tooth germs and the related signal transduction analysis.

Author

Peng L, Dong G, Xu P, Ren LB, Wang CL, Aragon M, Zhou XD, and Ye L

Subjects

Adenoviridae, Analysis of Variance, Blotting, Western, Cadaver, Fetus embryology, Humans, Immunohistochemistry, In Situ Hybridization, Odontogenesis, Reverse Transcriptase Polymerase Chain Reaction, Tooth Germ embryology, Transcription Factors metabolism, Wnt-5a Protein, Proto-Oncogene Proteins metabolism, Signal Transduction physiology, Tooth Germ metabolism, Wnt Proteins metabolism

Abstract

Objective: Wnt5a is generally considered a non-canonical Wnt family member and plays an important role in the development of several tissues through regulation of cell fate, proliferation, migration, polarity and death. This study investigates its expression mode in human tooth development and the involved cell signal transduction pathways, as they remain unclear., Design: The expression of Wnt5a was analyzed by immunohistochemistry method. Recombinant adenovirus encoding full-length Wnt5a cDNA was constructed to investigate four cell signal pathways and nine dentinogenesis nuclear transcription factors in response to Wnt5a in human dental papilla cells (HDPCs)., Results: Immunostaining revealed that Wnt5a was expressed in enamel epithelium cells from the bud stage, and in odontoblast layers and dental papilla tissues from early bell stage of human tooth development onward. Western blot analysis indicated that p42/44 MAPK, p38 MAPK, JNK and AKT signal pathways could be phosphorylated by WNT5A. RT-PCR analysis showed that Wnt5a increased the expression of DLX1, DLX2, LEF1, MSX2, PAX9 and RUNX2 mRNA, but decreased BARX1 and PITX2 mRNA., Conclusions: It was concluded that WNT5A is expressed in human tooth development, and that p42/44 MAPK, p38 MAPK, JNK and AKT signal pathways and DLX1, DLX2, LEF1, MSX2, PAX9, RUNX2 could be activated by Wnt5a., (Crown Copyright 2009. Published by Elsevier Ltd. All rights reserved.)

Published

2010

13. ClC-5 regulates dentin development through TGF-beta1 pathway.

Author

Duan X, Mao Y, Yang T, Wen X, Wang H, Hou J, Xue Y, and Zhang R

Subjects

Animals, Animals, Newborn, Cells, Cultured, Chloride Channels deficiency, Dentin pathology, Extracellular Matrix Proteins biosynthesis, Gene Expression, Mice, Mice, Knockout, Odontoblasts metabolism, Phosphoproteins biosynthesis, RNA Interference, Sialoglycoproteins biosynthesis, Up-Regulation, Chloride Channels metabolism, Dentin growth & development, Dentin metabolism, Tooth Germ metabolism, Transforming Growth Factor beta1 metabolism

Abstract

ClC-5 is one of the voltage-dependent chloride channel (ClC) family members. Mutations involving CLCN5 cause an X-linked nephropathy associated with Dent's disease. Some Clcn5 gene knockout (ClC-5 KO) mice have abnormal growth of the teeth; however, the expression and function of ClC-5 during tooth development is still unknown. Herein we report abnormal dentin structure, decreased DSPP and increased TGF-beta1 protein level in ClC-5 KO teeth. In odontoblast-like MDPC-23 cells, the mRNA levels of Tgfb1, Dspp and Dmp-1 were upregulated with Clcn5 RNAi after 48h treatment; whilst there was no change in those of TGF-beta receptor Tgfbr1 and Tgfbr2. We suggest that the dentin changes in ClC-5 KO mice might be a result of increasing TGF-beta1, and the interplay between ClC-5 and TGF-beta1 needs further identified.

Published

2009

14. ClC chloride channels in tooth germ and odontoblast-like MDPC-23 cells.

Author

Hou J, Situ Z, and Duan X

Subjects

Animals, Animals, Newborn, Cell Cycle genetics, Cell Line, Cell Proliferation drug effects, Chloride Channels antagonists & inhibitors, Chloride Channels genetics, Flow Cytometry, Gene Expression drug effects, Gene Expression Regulation, Mice, Propanols administration & dosage, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction, Tooth Germ drug effects, Cell Cycle drug effects, Chloride Channels metabolism, Odontoblasts metabolism, Tooth Germ metabolism

Abstract

Objective: To detect expression of ClC chloride channel mRNA in tooth germ and odontoblasts, and explore the affect of chloride channel function on cell proliferation and cell cycle., Design: We extracted total RNA of tooth germ from newborn C57BL mice and mouse odontoblast-like cells (MDPC-23), then detected mRNA expression of chloride channel genes Clcn1-7 with RT-PCR. We used chloride channel blocker 5-nitro-2-(3- phenylpropylamino)benzoic acid (NPPB) to interfere with chloride channel function of MDPC-23 cells. Cell proliferation rate and cell cycle were detected with MTT assay and flow cytometry, respectively. Student's t-test was used to determine statistical significance between control and treatment groups., Results: The mRNA of Clcn1-7 chloride channel genes was expressed in tooth germ of newborn mice. Clcn3, Clcn5 and Clcn7 mRNAs were expressed in MDPC-23 cells. NPPB slowed down the proliferation rate of MDPC-23 cells from day 2 to day 4 (P<0.01), and also changed the proportion of cell cycle phase. Comparing to the control, the proportion of G2/M phase cells reduced from 3.93+/-2.62% to 0.54+/-0.25% (P<0.05). The ratio of G1/G2 increased from 1.86+/-0.01 to 1.95+/-0.02 (P<0.05)., Conclusions: There is abundant chloride channel gene expression in tooth germ. Some of these chloride channels may regulate tooth development through effects on cell proliferation and cell cycle signal pathway.

Published

2008

15. MicroRNA expression profiling of the developing murine molar tooth germ and the developing murine submandibular salivary gland.

Author

Jevnaker AM and Osmundsen H

Subjects

Animals, Animals, Newborn, Cell Proliferation, Dental Enamel Proteins metabolism, Female, Gene Expression Profiling methods, Mice, MicroRNAs genetics, Molar metabolism, Morphogenesis physiology, Pregnancy, Reverse Transcriptase Polymerase Chain Reaction methods, MicroRNAs metabolism, Molar embryology, Submandibular Gland metabolism, Tooth Germ metabolism

Abstract

Using microarrays, miRNA expression profiles have been established at selected times during development (E15.5, P0 and P5) of the murine first molar mandibular tooth germ and the right submandibular salivary gland (E15.5, P0, P5 and P25). Microarray data was validated using real-time PCR, also facilitating RT-PCR profiling of nine selected miRNAs. In general, good agreement between microarray data and real-time PCR data was found. Further, miRNA expression profiles of foetal and adult liver were also investigated, and found to agree with published data. In tooth germ and salivary gland up to 88 different miRNAs were detected. In all tissues examined miRNA expression was highly dynamic; miRNA profiles changing extensively with time of development. Additionally, the expression of some miRNAs was tissue-specific. Bioinformatic analysis of clusters of miRNAs was attempted using the miRGate software, the results suggesting miRNAs to be involved in the regulation of essential developmental processes, e.g., epithelical cell proliferation, mesodermal cell fate determination and salivary gland morphogenesis.

Published

2008

16. Relationship of vitamin D with calbindin D9k and D28k expression in ameloblasts.

Author

Onishi T, Shintani S, Wakisaka S, and Ooshima T

Subjects

Animals, Calbindins, Immunohistochemistry, Mice, RNA, Messenger metabolism, Rats, Rats, Sprague-Dawley, Receptors, Calcitriol metabolism, S100 Calcium Binding Protein G genetics, Ameloblasts metabolism, S100 Calcium Binding Protein G metabolism, Tooth Germ metabolism, Vitamin D Deficiency metabolism

Abstract

Objective: Calbindin D9k (CB9k) and D28k (CB28k) are intracellular soluble calcium-binding proteins, whose expressions are considered to be regulated by vitamin D. However, the amount of CB28k expression in the kidneys of vitamin D receptor-null mice was reported to be similar to that in wild type mice, suggesting no dependence on vitamin D for its expression in kidneys. In the present study, we evaluated the effects of vitamin D on the expressions of CB9k and CB28k during amelogenesis., Design: Rats fed a vitamin D-deficient diet (VD(-) rats) or a standard diet (VD(+) rats) were subjected to immunohistochemical assays using anti-CB9k and anti-CB28k anti-serum. Further, after culturing in medium containing 1,25(OH)(2)D(3) at various doses, quantitative RT-PCR analyses of CB9k and CB28k mRNA were performed using tooth germs from the lower first molars of ICR mice., Results: CB9k-immunoreactivity was detected faintly during the secretory stage of ameloblasts in the incisors of VD(+) rats, with increased staining observed during the maturation stage, whereas no such immunoreactivity was detected in those of VD(-) rats. In contrast, the distribution of CB28k in the teeth of VD(-) rats was nearly identical to that in teeth of VD(+) rats, with immunoreactivity detected in both secretory and maturation ameloblasts. Further, quantitative RT-PCR analyses revealed that the amount of CB9k mRNA was increased in a dose-dependent manner, whereas that of CB28k mRNA was not changed., Conclusions: Vitamin D has no effect on the expression of CB28k, whereas it has a significant effect on that of CB9k in ameloblasts.

Published

2008

17. Dentinal defects in Hyp mice not caused by hypophosphatemia alone.

Author

Ogawa T, Onishi T, Hayashibara T, Sakashita S, Okawa R, and Ooshima T

Subjects

Animals, Dentin abnormalities, Dentin metabolism, Disease Models, Animal, Gene Expression, Gene Expression Regulation, Developmental, Hypophosphatemia, Familial metabolism, Mice, Mice, Inbred C57BL, Mice, Mutant Strains, Phosphates blood, Reverse Transcriptase Polymerase Chain Reaction, Tooth Germ metabolism, Dentin pathology, Hypophosphatemia, Familial pathology, Odontoblasts metabolism, Osteocalcin genetics, RNA, Messenger analysis

Abstract

The Hyp mouse is a murine homolog of human X-linked hypophosphatemic rickets and displays hypo-mineralization in bone and dentin due to a defect of the phosphate-regulating gene with homology to endopeptidase on the X chromosome (Phex) gene. It has long been considered that the bone and dentin defects in Hyp mice are caused by hypophosphatemia alone, however, several recent studies have indicated the possibility that intrinsic defects are present in Hyp mice osteoblasts. Further, we previously found a hyper-expression of osteocalcin (OC) mRNA in Hyp mouse odontoblasts and suggested the possibility of the presence of intrinsic defects. In the present study, we evaluated morphological features and OC mRNA expression levels in tooth germs of Nor mice with a normal phex gene and a low concentration of serum phosphate, and compared them to those in Hyp and wild-type mice. Nor mice exhibited low serum phosphate levels, however, did not show the characteristic features of dentin defects seen in Hyp mice, such as widened predentin and hyper-expression of OC mRNA. These results suggest that the hypo-mineralization of dentin in Hyp mice is not dependent on serum phosphate level, but rather is affected by intrinsic defects in odontoblasts.

Published

2006

18. Histological description of tooth formation in adult Eretmodus cf. cyanostictus (Teleostei, Cichlidae).

Author

Vandervennet E and Huysseune A

Subjects

Animals, Calcification, Physiologic physiology, Dental Enamel anatomy & histology, Dental Enamel metabolism, Dentin metabolism, Enamel Organ anatomy & histology, Iron metabolism, Morphogenesis physiology, Odontometry methods, Tooth Calcification physiology, Tooth Germ anatomy & histology, Tooth Germ metabolism, Cichlids, Tooth Germ growth & development

Abstract

The Eretmodini, a tribe of closely related cichlids (Teleostei, Cichlidae) originating from Lake Tanganyika, possess oral tooth shapes ranging from conical (in Tanganicodus) over cylindrical (in Spathodus) to spatulate (in Eretmodus). Prior to a study aiming to understand how these distinctly different tooth shapes can be acquired in such closely related taxa, a detailed histological study was required of tooth formation in a representative of the eretmodines. Here, we present a histological description of replacement tooth development in Eretmodus cf. cyanostictus. Using light-microscopic observations on semithin as well as on ground sections, microradiographs and stereo-microscopic observations of both alizarine red S stained and unstained jaws we can conclude that tooth formation in adult E. cf. cyanostictus roughly corresponds with what is known for teleost tooth development in general. Remarkable features include the localization and shape of the epithelial downgrowth, the transient presence of a layer intermediate between inner dental epithelium (IDE) and outer dental epithelium (ODE), the asymmetric shape of the enamel organ, the fact that the pulp cavity recedes in front of the forming enameloid during enameloid formation, and finally, the pattern of matrix mineralisation and maturation, and the presence of pigment in the enameloid. The observation that the enamel organ in adult E. cf. cyanostictus develops asymmetrically is significant for understanding tooth shape variation in the Eretmodini.

Published

2005

19. Tissue distribution and nucleotide sequence of bovine mRNA for salivary proline-rich protein P-B.

Author

Isemura S, Watanabe S, Fujiwara S, and Sanada K

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cattle, DNA, Complementary genetics, Gene Expression, Humans, Molecular Sequence Data, Peptides genetics, Polymerase Chain Reaction methods, Proline-Rich Protein Domains, RNA, Messenger genetics, Tissue Distribution, Tooth Germ metabolism, Peptides metabolism, Saliva metabolism

Abstract

The tissue distribution of P-B was investigated to obtain information on the physiological significance of this proline-rich protein. To design primers and probes for a tissue distribution analysis, a polymerase chain reaction (PCR)-based cloning of bovine P-B cDNA was performed using tooth germ and the nucleotide sequence was determined. The cloned bovine P-B cDNA was composed of 356 bp and included the region corresponding to the mature P-B protein and part of the 3' non-coding sequence. This part of the sequence is identical to the corresponding region of human P-B cDNA from the submaxillary gland. DNA corresponding to the P-B mRNA was amplified by PCR using cDNAs from various bovine tissues including tooth germ, submaxillary gland, parotid gland, lachrymal gland, heart, liver, stomach, pancreas, spleen, kidney, adrenal, and ovary. A quantitative analysis indicated the heart, submaxillary gland, tooth germ and kidney to be major sites of P-B expression. The ubiquitous distribution of P-B mRNA among bovine tissues together with findings of the presence of genes hybridizable with a DNA probe for P-B among species such as human, bovine, rat, mouse, and yeast as reported previously suggested a fundamental physiological role for this protein.

Published

2004

20. Expression of aquaporin isoforms during human and mouse tooth development.

Author

Felszeghy S, Módis L, Németh P, Nagy G, Zelles T, Agre P, Laurikkala J, Fejerskov O, Thesleff I, and Nielsen S

Subjects

Animals, Humans, Immunohistochemistry, Mice, Mouth Mucosa metabolism, Tooth metabolism, Tooth Germ growth & development, Tooth Germ metabolism, Aquaporins metabolism, Tooth growth & development

Abstract

Previously, we described the development of hyaluronan (HA) deposition in human tooth germ tissues that are consistent with water transport in different stages of tooth development. The aquaporins (AQP) constitute a family of membrane water channels that are expressed in many organs. However, there are no data available about the expression pattern of aquaporin water channels in dental structures. In the present study we have characterised the expression of six different aquaporin isoforms (AQP1-5, AQP-9) in developing human and mouse tooth germs by immunohistochemistry using isoform specific antibodies. In the "bell stage" AQP1 was expressed in endothelial cells of small vessels whereas no other structures of the tooth primordial were labeled. AQP2, AQP3 and AQP9 immunoreactivity was not observed in tooth germs, whereas strong AQP4 and AQP5 expression was observed in dental lamina, inner enamel epithelium, stratum intermedium, stellate reticulum and the outer enamel epithelium. Oral epithelium also exhibited AQP4 and AQP5 immunolabeling. During development of the matrices of the dental hard tissues AQP4 and AQP5 immunostaining was observed in the odontoblasts and their processes, as well as in the secretory ameloblast and their apical processes. Immunolabeling controls were negative. In conclusion, AQP4 and AQP5 are expressed in tooth germ tissues in early development in cells that previously have been shown to express HA and/or CD44, indicating that AQP water channels may play a role for ECM hydration during tooth development.

Published

2004

21. Expression of neural cell-adhesion molecule mRNA during mouse molar tooth development.

Author

Obara N, Suzuki Y, Nagai Y, Nishiyama H, Mizoguchi I, and Takeda M

Subjects

Animals, Dental Papilla embryology, Dental Papilla metabolism, Enamel Organ embryology, Enamel Organ metabolism, Fluorescent Antibody Technique, Indirect, In Situ Hybridization, Mesoderm metabolism, Mice, Mice, Inbred Strains, Molar metabolism, Neural Cell Adhesion Molecules genetics, Tooth Germ embryology, Tooth Germ metabolism, Gene Expression Regulation, Developmental, Molar embryology, Neural Cell Adhesion Molecules metabolism, Odontogenesis genetics, RNA, Messenger metabolism

Abstract

This study employed in situ hybridisation using a probe recognising all isoforms of the molecule. Expression of the molecule in tooth germs started at embryonic day 13, when they were at the bud stage. Both inner cells of the epithelial bud and peripheral cells of the dental mesenchyme were positive. At the cap stage, positive cells were found in the inner part of the enamel organ but only in a limited area near the outer enamel epithelium. In the mesenchyme at the cap stage, expression was weak in the dental papilla and strong in the follicle. From the bell stage onward, epithelial cells in the enamel organ were negative except for the cells of the stratum intermedium, which were transiently positive at early and late bell stages. In the dental papilla, expression had mostly ceased during and after the bell stage, although transient expression was found in cuspal areas at the early bell stage. The dental follicle strongly expressed neural cell-adhesion molecule (NCAM) to the end of the experimental period, at post-natal day 4. In contrast to the first molar at its earliest stage of appearance, in which both the thickened epithelium and surrounding mesenchyme were negative for the expression of the molecule, the second molar appeared as a combination of extending epithelial thickenings and mesenchymal cells strongly positive for its expression. This study newly identifies the dental papilla and the stratum intermedium as NCAM-expressing sites.

Published

2002

22. The spatial and temporal expression of calretinin in developing rat molars (Rattus norvegicus).

Author

Mistry D, Altini M, Coleman HG, Ali H, and Maiorano E

Subjects

Age Factors, Ameloblasts metabolism, Animals, Calbindin 2, Embryonic and Fetal Development, Epithelium metabolism, Female, Gene Expression, Immunohistochemistry, Male, Molar metabolism, Odontogenesis physiology, Rabbits, Rats, Rats, Sprague-Dawley, Molar embryology, S100 Calcium Binding Protein G biosynthesis, Tooth Germ metabolism

Abstract

Calretinin is a 29-kDa calcium-binding protein abundantly expressed in central and peripheral neural tissues. The aim here was to determine its expression during various stages of odontogenesis. Five categories of embryonic (E) and postnatal (P) rats at various ages (E17, E18, E20, P0, and P7), both male and female, were used to represent the various stages of molar tooth development. The heads of the experimental animals were harvested at the appropriate time and each was cut mid-sagittally and coronally to locate the tooth germs. Selected sections were stained immunohistochemically with polyclonal rabbit anticalretinin at a concentration of 1:25 after microwave irradiation. The results showed that calretinin is distributed widely in epithelium-derived tissues during odontogenesis in rat molar tooth germs. It was expressed focally in the dental lamina, outer enamel epithelium, stellate reticulum and stratum intermedium at different stages. In contrast, it was expressed diffusely and intensely in the inner enamel epithelium and presecretory ameloblasts, although it was discontinuous over the cusp tips. In the secretory ameloblasts, the staining was less intense, being restricted to the cytoplasm, including Tomes' processes. This distribution suggests that calretinin may play a part in enamel formation.

Published

2001

23. The distribution pattern of the hyaluronan receptor CD44 during human tooth development.

Author

Felszeghy S, Módis L, Tammi M, and Tammi R

Subjects

Age Factors, Ameloblasts chemistry, Ameloblasts metabolism, Antibodies, Monoclonal, Embryonic and Fetal Development, Humans, Hyaluronan Receptors biosynthesis, Immunohistochemistry, Infant, Infant, Newborn, Odontoblasts chemistry, Odontoblasts metabolism, Tooth Germ metabolism, Hyaluronan Receptors analysis, Tooth Germ chemistry

Abstract

The aim was to investigate the expression pattern of the major cell-surface hyaluronan receptor CD44, as there are no existing data on its presence or absence in human dental structures at different developmental stages. Immunohistochemical localization of CD44 was studied using a monoclonal antibody, H3, that specifically recognizes an epitope in the common backbone of all CD44 isoforms. The dental lamina displayed a strong CD44 signal; the external enamel epithelium was negative. In the coronal region of the tooth germ the presecretory ameloblasts showed an intense reaction whereas the less differentiated inner enamel epithelial cells showed no signal at the cervical loop where they meet the external enamel epithelium. In the stellate reticulum a moderate reaction was detected. The secretory ameloblasts and the stratum intermedium showed a strong cell-surface CD44 signal. A strong signal was also observed on the odontoblasts and their processes. In the pulp, close to the odontoblastic layer, weak labelling was seen in the walls of capillary vessels. The distribution of CD44 in the human tooth germ corresponds to that of hyaluronan in most locations, suggesting that during tooth development this transmembrane protein plays an important part in hyaluronan-mediated events.

Published

2001

24. Characterization of dental follicle cells in developing mouse molar.

Author

Hou LT, Liu CM, Chen YJ, Wong MY, Chen KC, Chen J, and Thomas HF

Subjects

Alkaline Phosphatase analysis, Alkaline Phosphatase drug effects, Alkaline Phosphatase genetics, Animals, Animals, Newborn, Calcitriol pharmacology, Calcium Channel Agonists pharmacology, Cell Lineage, Cells, Cultured, Collagen analysis, Collagen genetics, Dental Sac metabolism, Epithelial Cells cytology, Epithelial Cells metabolism, Fibronectins analysis, Fibronectins genetics, Gene Expression Regulation, Immunohistochemistry, Integrin-Binding Sialoprotein, Keratins analysis, Keratins genetics, Mice, Mice, Inbred Strains, Molar, Osteopontin, Phenotype, Phosphoproteins analysis, Phosphoproteins genetics, Pilot Projects, Sialoglycoproteins analysis, Sialoglycoproteins genetics, Tooth Germ cytology, Tooth Germ metabolism, Tooth Root cytology, Tooth Root metabolism, Dental Sac cytology

Abstract

Dental follicle has been implicated as the origin of alveolar bone, cementum and periodontal ligament, but there is no direct evidence of their cellular lineage. The present pilot study was designed to characterize the phenotype of cultured cells obtained from the dental follicle of neonatal mouse molars. Developing mandibular molars from 6-day-old CD-1 mice were subjected to 1% trypsin in Hank's balanced salt solution. After trypsinization, the dental follicle was enucleated from the tooth germ and separated from the associated epithelial root sheath. Pure dental follicle tissue was cultured in alpha-minimal essential medium containing 10% fetal bovine serum and antibiotics. The nature of the cultured follicle cells was determined in situ by immunocytochemical staining for type I and III collagen, fibronectin, and alkaline phosphatase expression. Earlier phenotypic markers for mineralization such as bone sialoprotein and osteopontin were also examined by in situ hybridization of matched molar tissues. The extracellular matrix proteins (such as type I collagen and fibronectin) were moderately expressed cytochemically. However, type III collagen was strongly stained. Gene expression of bone sialoprotein and osteopontin was detected in sections of mouse molars of similar age. The ALPase activity showed moderate to strong intensity in these primary cultured cells and responded to 1,25(OH)2 vitamin D3 treatment. Cytokeratin stains were not noted in these cells. In conclusion, the 6-day-old dental follicle cells exhibit partial characteristics of a mineralized tissue-forming phenotype even though the expression of osteopontin, type I collagen and fibronectin was low at this stage.

Published

1999

25. Effects of inositol hexasulphate, a casein kinase inhibitor, on dentine phosphorylated proteins in organ culture of mouse tooth germs.

Author

Torres-Quintana MA, Lécolle S, and Goldberg M

Subjects

Analysis of Variance, Animals, Autoradiography, Casein Kinase II, Casein Kinases, Dentin chemistry, Dose-Response Relationship, Drug, Mice, Microscopy, Electron, Odontoblasts chemistry, Odontoblasts cytology, Odontoblasts drug effects, Organ Culture Techniques, Phosphorylation drug effects, Phytic Acid toxicity, Protein Kinase Inhibitors, Protein Processing, Post-Translational drug effects, Protein Serine-Threonine Kinases antagonists & inhibitors, Tooth Germ metabolism, Dentinogenesis drug effects, Phosphoproteins biosynthesis, Phytic Acid pharmacology, Tooth Germ drug effects

Abstract

To study the effects of impaired protein phosphorylation on dentine formation and mineralization, inositol hexasulphate, an intracellular type I and type II casein kinase inhibitor, was used in an in vitro organotypic culture system. Mandibular first molar tooth germs were dissected from 18-day-old mouse embryos and cultured for 11 days with and without inositol hexasulphate at different concentrations. At 0.04-0.08 mM inhibitor, cellular alterations were not detected. Dentine displayed the characteristic purple-blue colour when Stains all, a specific stain for extracellular phosphoproteins, was used. At 0.1 mM, dentine failed to stain and mineralization did not occur, as seen from the von Kossa method. The presence of numerous lysosome-like vesicles inside cells indicated that the experiment was at the limits of cytotoxicity; higher concentrations induced severe cellular alterations. Therefore, quantitative radioautography was carried out on germs treated or not with the inhibitor at 0.1 mM. [33P]-phosphate incorporation showed that grain density in inhibited germs compared with that in control germs was about double in odontoblasts and half in the predentine/dentine compartment. In the presence of inositol hexasulphate the incorporation of [3H]serine into odontoblast cell bodies was unchanged between 2 and 24 h while in predentine/dentine, grain density was higher between 1 and 4 h, and reduced at 24 h. Both with [33P]phosphate and [3H]serine, labelling was seen throughout the porous dentine formed in vitro and not as a band located at the predentine/dentine junction, as is the case in vivo. With [3H]proline, in the presence of the inhibitor, a small reduction of grain density occurred in cell bodies, no significant difference was seen between 1 and 4 h in predentine/dentine, and more silver grains were present after 24 h both in cells and in the matrix. The radioautographic data support the view that the inhibitor interacts mostly with post-transductional phosphorylation and does not alter significantly other cell synthetic pathways and functions. Finally, the experiments presented here confirm that phophorylated proteins have a key role in dentine mineralization.

Published

1998

26. Spatiotemporal expression of the homeobox gene S8 during mouse tooth development.

Author

Karg H, Burger EH, Lyaruu DM, Bronckers AL, and Wöltgens JH

Subjects

Animals, Dental Pulp embryology, Dental Pulp metabolism, Dental Sac embryology, Dental Sac metabolism, Ectoderm metabolism, Epithelium embryology, Epithelium metabolism, Face embryology, Homeodomain Proteins genetics, In Situ Hybridization, Incisor embryology, Incisor metabolism, Jaw embryology, Mesoderm metabolism, Mice, Molar embryology, Molar metabolism, Neural Crest metabolism, Odontoblasts metabolism, Organ Culture Techniques, Osteogenesis genetics, RNA, Messenger analysis, RNA, Messenger genetics, Skull embryology, Skull metabolism, Tooth Germ metabolism, Transcription Factors genetics, Gene Expression Regulation, Developmental, Genes, Homeobox genetics, Odontogenesis genetics

Abstract

The murine S8 gene encodes a nuclear homeodomain containing transcription factor that is expressed at sites of epithelial-mesenchymal interactions, including those in cranofacial tissues. The spatiotemporal expression of S8 mRNA was examined in tooth primordia by in situ hybridization. S8 transcripts were found in all stages of tooth development in 13- to 16.5-day-old mouse embryos (E13-E16.5), covering the early bud stage up to the late bell stage. S8 mRNA was found exclusively in the ectomesenchyme and its derivatives that originate from the neural crest: future pulp cells, odontoblast precursors and dental follicle cells. Expression was highest at the late cap and early bud stages and declined at the mid-bell stage, in both first molar and incisor primordia. In E13 jaw explants grown in organ culture for 48 h, S8 mRNA was still present in first and second molar primordia after culture. At E15.5, S8 mRNA was also transiently present in the surrounding osteogenic tissue. It is concluded that the distribution pattern of S8 mRNA during tooth development indicates a role for the gene in defining the identity of dental papilla and follicle cells. It is speculated that the time-restricted expression of S8 in tooth primordia involves establishing the definitive form of the tooth organ.

Published

1997

27. An amelogenin gene defect associated with human X-linked amelogenesis imperfecta.

Author

Collier PM, Sauk JJ, Rosenbloom SJ, Yuan ZA, and Gibson CW

Subjects

Adenine, Ameloblasts metabolism, Amelogenin, Base Sequence, Cytosine, Dental Enamel abnormalities, Dental Enamel metabolism, Exons genetics, Female, Humans, Male, Pedigree, Point Mutation genetics, Proline genetics, Threonine genetics, Amelogenesis Imperfecta genetics, Dental Enamel Proteins genetics, Genetic Linkage genetics, Tooth Germ metabolism, X Chromosome genetics

Abstract

Dental enamel is a product of ameloblast cells, which secrete a mineralizing organic matrix, composed primarily of amelogenin proteins. The amelogenins are thought to be crucial for development of normal, highly mineralized enamel. The X-chromosomal amelogenin gene is a candidate gene for those cases of amelogenesis imperfecta, resulting in defective enamel, in which inheritance is X-linked. In this report, a kindred is described that has a C to A mutation resulting in a pro to thr change in exon 6 of the X-chromosomal amelogenin gene in three affected individuals, a change not found in unaffected members of the kindred. The proline that is changed by the mutation is conserved in amelogenin genes from all species examined to date.

Published

1997

28. Expression of cytokeratin 14 in ameloblast-lineage cells of the developing tooth of rat, both in vivo and in vitro.

Author

Tabata MJ, Matsumura T, Liu JG, Wakisaka S, and Kurisu K

Subjects

Amelogenin, Animals, Animals, Newborn, Biomarkers analysis, Cell Division, Cell Lineage, Cells, Cultured, Dental Enamel metabolism, Dental Enamel Proteins analysis, Dental Enamel Proteins genetics, Epithelium metabolism, Fluorescein-5-isothiocyanate, Fluorescent Antibody Technique, Direct, Fluorescent Dyes, Gene Expression Regulation, Developmental, Hepatocyte Growth Factor analysis, Hepatocyte Growth Factor genetics, In Vitro Techniques, Keratins analysis, Proto-Oncogene Proteins analysis, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins c-met, Rats, Rats, Sprague-Dawley, Receptor Protein-Tyrosine Kinases analysis, Receptor Protein-Tyrosine Kinases genetics, Time Factors, Ameloblasts metabolism, Keratins genetics, Tooth Germ metabolism

Abstract

In the search for a cell marker useful for studying tooth development, immunohistochemical studies using antibodies against cytokeratin 14 (K14), c-Met/hepatocyte growth factor receptor and amelogenin were carried out in the developing tooth of the newborn rat and in primary cultured cells of the ameloblast lineage, including inner enamel epithelium cells, preameloblasts and ameloblasts, prepared from the mandibular incisors of postnatal 7-day-old rats. The appearance of K14 was cell- and differentiation-stage specific, i.e. there was a weak expression signal within inner enamel epithelial cells that were in the proliferating stage, and there were strong signals within preameloblasts and ameloblasts that were in the post-proliferating and amelogenesis stages, respectively. In the culture system, c-Met appeared in all cells, whereas K14 and amelogenin appeared mainly in clustered cells that were considered to be in the post-proliferating stage. K14 was detected earlier than amelogenin, and it was also confirmed by immunofluorostaining that c-Met, K14 and amelogenin were coexpressed in ameloblasts. These findings indicate that K14 is a good new marker for ameloblast-lineage cells during rat tooth development both in vivo and in vitro.

Published

1996

29. Determination of enamel protein synthesized by recombined mouse molar tooth germs in organ culture.

Author

Baba T, Terashima T, Oida S, and Sasaki S

Subjects

Ameloblasts, Amelogenin, Animals, Cell Differentiation, Dental Enamel Proteins analysis, Enzyme-Linked Immunosorbent Assay, Epithelium physiology, Mesoderm physiology, Mice, Odontogenesis, Organ Culture Techniques, Tooth Germ embryology, Dental Enamel Proteins biosynthesis, Tooth Germ cytology, Tooth Germ metabolism

Abstract

Epithelial-mesenchymal interaction is a prerequisite for tooth morphogenesis. To study this interaction, inner enamel epithelium and dental papilla mesenchyme of molar tooth germs from a 16.5-day mouse embryo were dissociated enzymatically and cultured alone or after recombination. Characteristic matrix protein synthesized and secreted by recombined tooth germ was determined quantitatively by enzyme-linked immunosorbent assay. The protein was detected in the culture of recombined tooth germ but not of dissociated enamel epithelium alone. The amount of enamel protein increased until 8 days in culture. Morphological differentiation of the recombined epithelial rudiment into ameloblasts and enamel protein production were confirmed.

Published

1996

30. Spatial distribution of enamel proteins and fibronectin at early stages of rat incisor tooth formation.

Author

Sawada T and Nanci A

Subjects

Ameloblasts cytology, Ameloblasts metabolism, Amelogenesis, Animals, Basement Membrane cytology, Basement Membrane metabolism, Cell Differentiation, Cell Membrane metabolism, Cell Membrane ultrastructure, Collagen metabolism, Dental Pulp cytology, Dental Pulp metabolism, Dentin cytology, Dentin metabolism, Epithelial Cells, Epithelium metabolism, Extracellular Matrix metabolism, Extracellular Matrix ultrastructure, Immunohistochemistry, Incisor, Male, Mesoderm cytology, Mesoderm metabolism, Odontoblasts cytology, Odontoblasts metabolism, Rats, Rats, Wistar, Tooth Germ cytology, Dental Enamel Proteins metabolism, Fibronectins metabolism, Odontogenesis, Tooth Germ metabolism

Abstract

Enamel proteins are secreted very early during amelogenesis, that is prior to mantle dentine formation, raising the possibility that they may participate in epithelial-mesenchymal interactions taking place during tooth development. These first enamel proteins associate with elements of the basement membrane interposed between the differentiating ameloblasts and odontoblasts. Fibronectin, a component of the basement membrane, is redistributed and accumulates along the apical portion of odontoblasts during their terminal differentiation. In order to determine whether any correlation exists between the redistribution of fibronectin and the secretion of the first enamel proteins, the spatial distribution of these two extracellular matrix proteins was examined during the presecretory stage of amelogenesis. Male Wistar rats were perfused with a formaldehyde-based fixative, and undemineralized and EDTA demineralized incisors were dehydrated in methanol and embedded in Lowicryl K4M resin. Ultrathin tissue sections were then processed for post-embedding, colloidal-gold immunocytochemistry with antibodies to enamel proteins, fibronectin or type III collagen. In the region of ameloblasts facing pulp, labelling for fibronectin was weak and mostly associated with the lamina fibroreticularis of the basement membrane separating differentiating ameloblasts and odontoblasts. As the mantle predentine formed the immunoreaction for fibronectin increased, particularly in the region of the basement membrane. Enamel proteins were also immunodetected in association with the lamina fibroreticularis and gradually accumulated as patches within mantle dentine and at its interface with ameloblasts. Von Korff collagen bundles, present between odontoblasts and in dentine, were immunolabelled for fibronectin and for type III collagen. Patches of granular material, immunoreactive for fibronectin and/or enamel proteins, were found along the odontoblastic processes and cell bodies. Although no evidence was obtained indicating a precise colocalization of fibronectin and enamel proteins, the results confirm that these two proteins can be found within similar extracellular compartments during mantle predentine-dentine formation. These data suggest that enamel proteins, by themselves or synergistically with other proteins, may play a part in the differentiation and/or formative events taking place at the ameloblast-odontoblast interface during the early stages of tooth development.

Published

1995

31. Spatial and temporal distribution of sonic hedgehog mRNA in the embryonic mouse mandible by reverse transcription/polymerase chain reaction and in situ hybridization analysis.

Author

Kronmiller JE, Nguyen T, Berndt W, and Wickson A

Subjects

Actins genetics, Actins metabolism, Animals, Blotting, Northern, Dental Sac embryology, Dental Sac metabolism, Epithelium embryology, Epithelium metabolism, Gestational Age, Incisor, Mandible metabolism, Mice, Molar, Odontogenesis genetics, Tooth Germ embryology, Tooth Germ metabolism, Gene Expression Regulation, Developmental, In Situ Hybridization, Mandible embryology, Polymerase Chain Reaction, Proteins genetics, RNA, Messenger genetics, Transcription, Genetic

Abstract

Hedgehog genes have recently been implicated in the control of pattern formation in many developing organ system. Vertebrate homologues of the Drosophila hedgehog have been identified in mouse and rate embryos. The temporal regulation of sonic hedgehog (mouse homologue) has previously been studied by Northern analysis of whole embryos with varying results. Sonic hedgehog transcript expression in the mouse mandibular process was now characterized using polymerase chain reaction (PCR) an in situ hybridization techniques. PCR analysis revealed transcripts at gestational days 10 and 11, before the formation of the dental lamina, but not at days 12-14, after tooth buds have formed. Transcripts were localized to, primarily, the epithelium in the presumptive incisor region of the mandibular midline at gestational day 10. No mRNA was detected by in situ hybridization techniques in the presumptive molar regions of odontogenic epithelium. Sonic hedgehog expression may be involved in the regulation of pattern formation through establishment of an incisor-molar axis of polarity.

Published

1995

32. Bone morphogenetic protein-2 and -4 expression during murine orofacial development.

Author

Bennett JH, Hunt P, and Thorogood P

Subjects

Animals, Bone Morphogenetic Proteins, Cell Differentiation, Dental Papilla embryology, Dental Papilla metabolism, Dental Sac embryology, Dental Sac metabolism, Epithelium embryology, Epithelium metabolism, Gestational Age, Mandible embryology, Mandible metabolism, Mesoderm metabolism, Mice, Mice, Inbred CBA, Mouth Floor embryology, Mouth Floor metabolism, Mouth Mucosa embryology, Mouth Mucosa metabolism, Palate embryology, Palate metabolism, RNA, Messenger genetics, Signal Transduction genetics, Tongue embryology, Tongue metabolism, Tooth Germ embryology, Tooth Germ metabolism, Face embryology, Gene Expression Regulation, Developmental, Growth Substances genetics, Mouth embryology, Proteins genetics

Abstract

In the developing orofacial region, epithelial-mesenchymal interactions induce a differentiation cascade leading to bone and cartilage formation. Although the nature of this interaction is unknown, bone morphogenetic proteins (BMP)-2 and -4 have been suggested as putative signalling molecules. Using 35S-labelled cDNA probes, the expression patterns of BMP-2 and -4 mRNA were examined in murine perioral tissues preceding, during and following the time of the epithelial-mesenchymal interaction leading to mandibular formation. At embryonic age (e) 9.5 days, a restricted pattern of BMP-4 mRNA was expressed in the epithelium of the developing facial processes. This decreased rapidly, with little or no signal on E10.5 or E11.5. By E13.5, BMP-4 signal was restricted to the dental lamina, follicle and papilla. BMP-2 expression was not prominent in the developing face until E13.5. At this stage, signal was widespread throughout mesenchyme of neural-crest, but not somatic origin. Different domains of expression were present in the developing epithelium: for example, there was strong signal in the floor of the mouth and the ventral tongue, in contrast to that of the dorsum of the tongue and primary palate, which were negative. These results support the role of BMP-2 and -4 as regulators of orofacial development and demonstrates different fields of BMP-2 expression in developing oral mucosal epithelium.

Published

1995

33. Effects of the intermediate retinoid metabolite retinal on the pattern of the dental lamina in vitro.

Author

Kronmiller JE, Beeman CS, Kwiecien K, and Rollins T

Subjects

Animals, Chromatography, High Pressure Liquid, Epithelium chemistry, Epithelium drug effects, Epithelium embryology, Mandible chemistry, Mandible embryology, Mandible metabolism, Mesoderm chemistry, Mesoderm drug effects, Mesoderm ultrastructure, Mice, Mitotic Index, Organ Culture Techniques, Retinaldehyde analysis, Retinaldehyde metabolism, Retinoids analysis, Retinoids metabolism, Tooth Germ chemistry, Tooth Germ embryology, Tooth Germ metabolism, Tooth, Supernumerary chemically induced, Tooth, Supernumerary embryology, Odontogenesis drug effects, Retinaldehyde pharmacology, Tooth Germ drug effects

Abstract

Retinoids have important roles in pattern formation during embryonic development and might act as endogenous morphogens. They are necessary for normal odontogenesis and excess retinol alters the pattern of odontogenesis producing supernumerary buds of the dental lamina in the diastema region of the mouse mandible. Because the metabolism of retinoids in the developing mandible is unknown, the effects of retinal (an intermediate metabolite in the local conversion of retinol to retinoic acid) on the patterning of odontogenesis were examined. Retinal produces supernumerary buds and enhanced epithelial proliferation in day-9 mandibles in vitro. The endogenous levels of retinal in the mandible at the time of initiation of odontogenesis were also measured by high-performance liquid chromatography. Retinal was detected only at day 10 and not at later stages of development. Local metabolism of this intermediate retinoid may be a rate-determining step in the production of active retinoid metabolites that may control the pattern of the dentition, which is established at the time of the appearance of the dental lamina at embryonic day 12.

Published

1994

34. Expression of c-erbB-2 proto-oncogene-encoded protein (p185erbB-2) in functional rat ameloblasts.

Author

Casasco A, Casasco M, Corbett IP, and Calligaro A

Subjects

Animals, Dental Enamel embryology, Dental Enamel metabolism, Enamel Organ metabolism, Gene Expression, Membrane Glycoproteins genetics, Membrane Glycoproteins metabolism, Mitosis genetics, Odontogenesis genetics, Protein-Tyrosine Kinases genetics, Protein-Tyrosine Kinases metabolism, Rats, Rats, Wistar, Receptor, ErbB-2 metabolism, Ameloblasts metabolism, Receptor, ErbB-2 genetics, Tooth Germ metabolism

Abstract

The c-erbB-2 proto-oncogene encodes a transmembrane glycoprotein with tyrosine kinase activity, p185erbB-2, that has been previously localized in some developing and mature epithelia. The possible occurrence of p185 in the inner enamel epithelium of rat tooth germ was here investigated immunocytochemically. Postmitotic functional ameloblasts displayed intense p185-immunoreactivity, thus suggesting that c-erbB-2 proto-oncogene is active during odontogenesis. The expression of this gene in differentiated and functional cells of the enamel organ suggests that its role is not restricted to mitotic events but may also be important in signalling pathways related to other cell activities.

Published

1994

35. Cholesterol in the distal portions of differentiating and fully differentiated rat odontoblasts observed by freeze-fracture.

Author

Franklin DL, Arana-Chavez VE, and Katchburian E

Subjects

Animals, Biomarkers, Cell Differentiation, Cell Membrane metabolism, Cell Membrane ultrastructure, Filipin, Freeze Fracturing, Membrane Fluidity, Molar, Odontoblasts cytology, Rats, Rats, Sprague-Dawley, Replica Techniques, Tooth Germ cytology, Tooth Germ metabolism, Tooth Germ ultrastructure, Vacuoles metabolism, Vacuoles ultrastructure, Cholesterol metabolism, Odontoblasts metabolism, Odontoblasts ultrastructure

Abstract

Freeze-fracture replicas of rat molar tooth germs in conjunction with the 3-beta-hydroxysterol marker filipin were used to study the distribution of cholesterol in the distal portions of odontoblast plasma membrane. Filipin-sterol deformations (interactions) appeared as clusters interspersed with deformation-free regions on the distal plasma membrane of early differentiating odontoblasts. In fully differentiated odontoblasts, the whole distal membrane, including the process, was occupied by packed deformations with no free regions. It seems that early developing odontoblasts are poorer in cholesterol than the fully differentiated cells. As the content and/or distribution of 3-beta-hydroxysterols (cholesterol) is known to influence membrane fluidity, the low cholesterol content of early differentiating odontoblasts might be related to the fluidity required for the budding off of matrix vesicles.

Published

1994

36. Dynamic variations in the expression of type I collagen and its molecular chaperone Hsp47 in cells of the mouse dental follicle during tooth eruption.

Author

Shroff B, Pileggi R, Norris K, Orbegoso R, Wilson T, and Sauk JJ

Subjects

Animals, Culture Techniques, Cytoplasm metabolism, Cytoplasm ultrastructure, Dental Cementum metabolism, Dental Cementum physiology, Dental Cementum ultrastructure, Dental Sac physiology, Dental Sac ultrastructure, Extracellular Matrix metabolism, Extracellular Matrix physiology, Extracellular Matrix ultrastructure, Fibroblasts metabolism, Fibroblasts physiology, Fibroblasts ultrastructure, Fluorescent Antibody Technique, Gene Expression Regulation, HSP47 Heat-Shock Proteins, Mice, Molar, Odontogenesis genetics, Tooth Germ metabolism, Tooth Germ physiology, Tooth Germ ultrastructure, Collagen genetics, Dental Sac metabolism, Heat-Shock Proteins genetics, Tooth Eruption genetics

Abstract

Tooth eruption is a precisely timed and sequenced event that brings the tooth from within bone into a functional position in the mouth. Every part of the developing tooth has been theoretically implicated as a primary factor in this process, but it now appears that eruption is multifactorial, with the dental follicle and type I collagen playing an important part. Immunological probes were used here to investigate in vivo and in vitro the temporal and spatial expression of type I collagen and its molecular chaperone Hsp47 in the dental follicle during eruption. Mandibles were dissected from 2-, 5-, 9- and 11-day-old neonatal mice and fixed in 95% ethanol overnight. Sections of 7 microns were obtained and reacted with antibodies directed against type I collagen. Dental follicles were isolated from 2-, 5-, 9- and 11-day-old neonates and cells were grown in culture for 8 days. Slides were then reacted with antibodies directed against type I collagen and Hsp47. The production of type I collagen and Hsp47 in the follicle varied with the stage of dental development and eruption. There was a progressive decrease of type I collagen in the coronal part of the follicle, leading to an arrest of its production in these areas. These findings support the notion that cells of the coronal portion of the dental follicle stop producing type I collagen as a prerequisite to the initiation of tooth eruption and that this phenotype persists in vitro.

Published

1994

37. In vivo and in vitro study of the effects of chlorpromazine on tooth mineralization in rats and mice.

Author

Togari A, Kondo M, Arai M, and Matsumoto S

Subjects

Alkaline Phosphatase metabolism, Animals, Calcium blood, Calmodulin antagonists & inhibitors, Calmodulin physiology, Dentin enzymology, Dentin metabolism, Dose-Response Relationship, Drug, Female, Male, Mice, Mice, Inbred Strains, Phosphates blood, Rats, Rats, Wistar, Tooth Germ enzymology, Tooth Germ metabolism, Chlorpromazine toxicity, Dentin drug effects, Tooth Calcification drug effects, Tooth Germ drug effects

Abstract

The effects of chlorpromazine (CPZ) on tooth mineralization were examined using incisor dentine in adult rats and cultured tooth germs of mandibular first molars dissected from mouse embryos. CPZ (10, 50 and 250 mg/kg, s.c.) substantially inhibited dentine mineralization as evaluated by contact microradiographs. Plasma calcium and phosphorus concentrations were not decreased by CPZ (10 and 50 mg/kg). Physicochemical effects were not involved in the action of CPZ on the mineralization. In vitro experiments showed that CPZ (1 and 10 microM) inhibited mineralization and alkaline phosphatase (ALP) activity in the tooth germs. As CPZ has the properties of a calmodulin antagonist, the calmodulin antagonists W-7 and W-5 were also examined. Both inhibited mineralization and ALP activity in tooth germs; W-5 had less effect than W-7. These in vivo and in vitro findings suggest that CPZ inhibited cell-mediated mineralization in dentine without affecting the calcium-regulating system and physicochemical mineral deposition. In addition, calmodulin could be involved in cell-mediated mineralization.

Published

1993

38. The correlation of temporal regulation of glycosaminoglycan synthesis with morphogenetic events in mouse tooth development.

Author

Galbraith DB, Cutler LS, and Kollar EJ

Subjects

Animals, Cell Differentiation, Chondroitin Sulfates metabolism, Heparitin Sulfate metabolism, Mice, Morphogenesis, Time Factors, Glycosaminoglycans biosynthesis, Odontogenesis, Tooth Germ embryology, Tooth Germ metabolism

Abstract

The purpose of this study was to investigate the pattern of sulphated glycosaminoglycan synthesis during morphogenesis and cytodifferentiation in mouse tooth rudiments and to compare the results with those obtained in another study for salivary gland, a branched organ. Sulphated glycosaminoglycan was labelled by incubating molar rudiments from day 15 of gestation to day 1 post partum in medium containing [35S]-sodium sulphate. The rudiments were washed, homogenized and digested in pronase and then were sequentially digested by chondroitinase ABC and chemically degraded by nitrous acid oxidation. The fractions from each of these procedures were analysed by chromatography on Sephadex G-50 columns. The analysis revealed that, during morphogenesis, levels of chondroitin sulphate increased to a peak of 91% at day 18 and levels of heparan sulphate diminished to 8% during this period. As cytodifferentiation occurred, the level of chondroitin sulphate dropped to 64% and that of heparan sulphate increased to 35%. These results are similar to those reported for rat submaxillary gland, a branching organ. It appears that this pattern of sulphated glycosaminoglycan synthesis is not a unique feature of branching morphogenesis but may be one which marks the transition between morphogenesis and cytodifferentiation in non-branching rudiments as well.

Published

1992

39. Immunofluorescent lectin binding patterns and glycoprotein co-localization in the developing murine molar tooth.

Author

Jowett AK, Kimber SJ, and Ferguson MW

Subjects

Acetylgalactosamine metabolism, Acetylglucosamine metabolism, Ameloblasts metabolism, Animals, Basement Membrane metabolism, Cell Adhesion Molecules, Neuronal metabolism, Cell Division, Dental Enamel cytology, Dental Enamel metabolism, Epithelium metabolism, Extracellular Matrix Proteins metabolism, Fluorescent Antibody Technique, Glucose metabolism, Laminin metabolism, Mannose metabolism, Mesoderm metabolism, Mice, Odontoblasts metabolism, Protein Binding, Tenascin, Tooth Germ cytology, Extracellular Matrix metabolism, Glycoproteins metabolism, Lectins metabolism, Odontogenesis physiology, Tooth Germ metabolism

Abstract

Fluorescein-conjugated lectins were used in conjunction with antibodies to laminin, tenascin and amelogenin to investigate saccharide expression in the developing tooth germ. At the bud stage, peanut agglutinin (PNA) binding demonstrated residues that may be D-galactose-(beta 1----3)DGalNAc, and this staining occurred after the expression of tenascin. Only the cap-stage enamel organ suprabasal cells and the enamel knot stained intensely with Ulex europeus agglutinin-I, but not Lotus tetragonolobus agglutinin, implying the transient presence of blood group H type I oligosaccharides. At the late stages of amelogenesis, enamel synthesis is preceded by en bloc loss of inner enamel basement membrane components. Before this, Bandeiraea (Griffonia) simplicifolia--I (BSL-I) staining was lost from postmitotic ameloblasts, suggesting that a glycosylated species is initially removed. Additionally, PNA was co-localized with amelogenin protein, suggesting that it may express beta-D-galactosyl sequences. These results indicate that the glycosylation patterns of matrix components during odontogenesis may be important as they vary in a manner similar to that of the well-known glycoproteins.

Published

1992

40. An autoradiographic study of calcium movement in the enamel organ of rat molar tooth germs.

Author

Hanawa M, Takano Y, and Wakita M

Subjects

Ameloblasts metabolism, Animals, Autoradiography, Calcium Radioisotopes, Cell Nucleus metabolism, Connective Tissue metabolism, Cytoplasm metabolism, Dental Enamel metabolism, Dental Enamel ultrastructure, Enamel Organ ultrastructure, Freezing, Histological Techniques, Molar, Rats, Rats, Inbred Strains, Time Factors, Tooth Germ ultrastructure, Calcium pharmacokinetics, Enamel Organ metabolism, Tooth Germ metabolism

Abstract

The distribution and movement of calcium through the enamel organ and into the forming enamel was studied in 6-day-old rats, intravenously injected with 45Ca. To prevent dislocation of radiocalcium in the specimens, the tooth germs were rapidly frozen/freeze-substituted and processed for 45Ca autoradiography under dry conditions. At 30 s after the 45Ca injection, there was a decrease in labelling intensity progressing from the overlying connective tissue to the enamel organ and, in the secretory ameloblasts, from the proximal to distal cytoplasm. The most intense labelling was in the enamel matrix, where it was restricted to the superficial layer extending approx. 15 microns below the surface. At later times the density of silver grains over the connective tissue decreased considerably, whereas secretory ameloblasts showed an increasing intensity in the distal portions. Enamel had the heaviest labelling: the width of the labelled enamel increased gradually to only 40 microns from the surface 60 min after the injection. The use of wet emulsion over similarly prepared sections caused a severe dislocation of radiocalcium in the specimens. These findings confirm the rapid penetration of systemically administered calcium to newly formed enamel, probably due to isotopic exchange. A relatively slow diffusion through the enamel organ and into the surface layer of enamel suggests that net transport of calcium through the enamel organ is transcellular.

Published

1990

41. A histological and biochemical study of the effect of vitamin C-deficiency on induction of amelogenesis in hamster molars in vitro.

Author

Bronckers AL

Subjects

Animals, Ascorbic Acid Deficiency pathology, Calcium metabolism, Cricetinae, Mesocricetus, Microbial Collagenase pharmacology, Molar, Organ Culture Techniques, Phosphates metabolism, Proline metabolism, Tooth Germ drug effects, Tooth Germ metabolism, Tooth Germ pathology, Amelogenesis, Ascorbic Acid Deficiency metabolism

Abstract

Second maxillary molars of hamsters were cultured in the presence or absence of 250 micrograms/ml vitamin C for periods up to 12 days. At various days, cultured explants were studied with histological and biochemical methods to investigate effects of vitamin C-deficiency on matrix production and mineralization in vitro. As biochemical parameters for protein synthesis and mineralization, uptake and incorporation of [3H]-proline, 45Ca and 32PO4 were used. To discriminate between synthesis of collagenous and non-collagenous proteins digestion of the [3H]-proline-labelled material by purified collagenase and its degree of hydroxylation were measured. Histologically, in control explants cultured with vitamin C, normal dentinogenesis, amelogenesis and mineralization in vitro were observed. In the vitamin C-deficient explants, odontoblasts produced an abnormal predentine matrix and de-differentiated. Eventually, this matrix mineralized aspecifically. In the presence of this abnormal matrix, ameloblasts failed to differentiate, which suggests that a cell-matrix type of interaction is involved in the differentiation of the pre-ameloblasts. Biochemically, in the vitamin C-deficient explants protein synthesis and collagen synthesis were reduced by about the same extent; the in-vitro produced collagens appeared under-hydroxylated and could, in degraded form, easily be extracted in formic acid. An increase of [3H]-proline solubility in formic acid in the control explants, however, paralleled enamel matrix production and was attributed to the solubilization of proline-rich enamel matrix proteins. The production of acid insoluble phosphate was not affected by vitamin C-deficiency. The uptakes of 45Ca and 32PO4 were retarded and the molar Ca:PO4 uptake ratio was lower, reflecting the histologically observed aspecific mineralization.

Published

1983

42. In-vitro study of cadmium-109 uptake by rat molar enamel during the secretory stage of formation.

Author

Bawden JW and Deaton TG

Subjects

Animals, Autoradiography, Dental Enamel metabolism, In Vitro Techniques, Radioisotopes metabolism, Rats, Amelogenesis, Cadmium metabolism, Enamel Organ metabolism, Tooth Germ metabolism

Published

1980

43. Purine salvage in vitro by mouse tooth germs exposed to mycophenolic acid.

Author

Dye FJ

Subjects

Animals, Guanine metabolism, Mice, Mice, Inbred C57BL, Molar, Odontogenesis drug effects, Organ Culture Techniques, Tooth Germ drug effects, Guanine Nucleotides biosynthesis, Mycophenolic Acid pharmacology, Tooth Germ metabolism

Published

1980

44. Effect of different combinations of calcium, magnesium and phosphate on the inorganic composition of rat molars in vitro.

Author

Ameloot PC, Coomans D, Smeyers-Verbeke J, and Boute P

Subjects

Animals, Calcium metabolism, Magnesium metabolism, Molar, Organ Culture Techniques, Organ Size drug effects, Phosphates metabolism, Rats, Regression Analysis, Tooth Germ metabolism, Calcium pharmacology, Magnesium pharmacology, Phosphates pharmacology, Tooth Germ drug effects

Abstract

Second upper molars from 3-day-old rats were cultured by the Trowell method for 14 days. One of each pair of molars was kept as an uncultured control; the other was cultured. Explants were exposed to eight different combinations of Ca, Mg and P additions to BGJb medium. This resulted in eight groups of explants (control, Ca, Mg, P, CaMg, CaP, PMg and CaMgP) and their eight uncultured contralateral groups. The additions were calculated to double the original measured media concentration. Cultured and uncultured germs were analysed for dry weight (D), ash weight (A), Ca, Mg and P content. The organic fraction (D-A) was calculated. The analysis of covariance by means of multiple regression revealed that Ca-addition to the culture medium stimulated D, A, Ca and P in the explants; P-addition was stimulatory for D, A, D-A and P whereas Mg addition was inhibitory for A, D-A and Ca. A positive interaction for all the tooth-germ variables was demonstrated after CaMg addition; an antagonistic effect was found for the tooth-germ variables D, A, Ca and P after CaP addition. The value of the tooth-germ variables at the time of explantation (covariate) had no significant effect on the value for the variables of the explants (except on their P content). The highest absolute values for all the variables were obtained after CaMg and CaMgP additions. Furthermore, taking into consideration morphological results, the addition of CaMgP can be recommended as medium supplement in the organ culture of rat tooth germs.

Published

1987

45. Light-microscopic studies on spatial and temporal binding of the lectins concanavalin A, wheat-germ agglutinin and peanut agglutinin in early rat odontogenesis.

Author

Blottner D and Lindner E

Subjects

Animals, Arachis, Carbohydrate Metabolism, Concanavalin A metabolism, Microscopy, Peanut Agglutinin, Plant Lectins, Rats, Rats, Inbred Strains, Wheat Germ Agglutinins metabolism, Extracellular Matrix metabolism, Lectins metabolism, Odontogenesis, Tooth Germ metabolism

Abstract

The spatial distribution and temporal expression of alpha-D-mannosyl(glucosyl)-, N-acetyl-D-glucosaminyl- and beta-D-galactosyl residues as detected by peroxidase-conjugated lectins correlated with early odontogenic events in six principal developmental stages (fetal days 13.5, 14, 15, 17, 18.5 and 19.5). The odontogenic epithelium of 13.5- and 14-day-old fetuses was characterized by strong concanavalin A (Con A) binding and between days 17 and 19.5, the stellate reticulum displayed strong peanut agglutinin (PNA) binding. Between 15 and 19.5, differentiation of dental ectomesenchyme was characterized by a rhythmic expression of terminal galactosyl residues shown by PNA-binding. At the developing dental basement membrane, there were various carbohydrate-specific regions. At days 13.5 and 14, the odontogenic basement membrane was specific for N-acetyl-D-glucosamines detected by wheat-germ agglutinin (WGA). The results suggest that the carbohydrates present at the inner dental basement membrane at days 17 to 19.5 may be involved in cell-matrix interactions during cytodifferentiation.

Published

1987

46. Electron microscopy of horseradish peroxidase uptake by papillary cells of the mouse incisor enamel organ.

Author

Skobe Z and Garant PR

Subjects

Ameloblasts metabolism, Animals, Biphenyl Compounds, Diamines, Formaldehyde, Incisor, Injections, Intravenous, Mice, Microscopy, Electron, Osmium, Peroxidases metabolism, Tooth Germ metabolism

Published

1974

47. Effect of developmental stage of explants on further in-vitro development of hamster molars.

Author

Bronckers AL, Bervoets TJ, and Wöltgens JH

Subjects

Alkaline Phosphatase metabolism, Animals, Calcium metabolism, Cricetinae, Culture Techniques, Dental Enamel growth & development, Dentin growth & development, Mesocricetus, Molar growth & development, Odontogenesis, Tooth Germ metabolism, Tooth Germ growth & development

Abstract

With morphometrical and biochemical methods the in-vitro development of 1-4-day-old 2nd maxillary molars was studied up to 10 days and compared with previously reported in-vivo development. Incorporation of [3H]-thymidine and increase in dry weight were used as biochemical parameters for cell proliferation and growth respectively specific alkaline phosphatase activity and uptake of 45Ca as the measure for mineralization. In explants of 2-4-day-old hamsters, formation of dentine and enamel matrix was consistent: both mineralized. These explants attained stages beyond enamel matrix formation, possibly the transitional stages of amelogenesis. The amounts of matrices produced appeared to be related to the final size the explants attained. Best in-vitro development histologically was in explants of 2 and 3-day-olds. Thus in-vitro development was qualitatively similar to in vivo.

Published

1983

48. Effect of alkaline-phosphatase inhibition by 1-p-bromotetramisole on the formation of trichloroacetic acid-[32P]-insoluble phosphate from inorganic [32P]-phosphate and [32P]-pyrophosphate in non-mineralizing and mineralizing hamster molar tooth-germs in vitro.

Author

Lyaruu DM, Wöltgens JH, and Bervoets TJ

Subjects

Animals, Cricetinae, Diphosphates metabolism, Mesocricetus, Molar, Phosphorus Radioisotopes, Tetramisole pharmacology, Time Factors, Tooth Calcification, Tooth Germ enzymology, Trichloroacetic Acid, Alkaline Phosphatase antagonists & inhibitors, Phosphates metabolism, Tetramisole analogs & derivatives, Tooth Germ metabolism

Abstract

In culture, 1-p-bromotetramisole (pBTM), a specific inhibitor of alkaline phosphatase, significantly inhibited the formation of trichloroacetic acid (TCA)-insoluble [32P]-phosphate from inorganic [32P]-phosphate in the proliferating non-mineralizing second (M2) maxillary molar germs but had no effect in the actively mineralizing first (M1) germs. Addition of 10(-5) M inorganic pyrophosphate in the culture medium with a [32P]-phosphate label increased the inhibition of the formation of TCA-insoluble [32P]-phosphate in the M2. pBTM almost completely inhibited the formation of TCA-insoluble [32P]-phosphate from inorganic [32P]-pyrophosphate in the non-mineralizing M2. In the actively mineralizing M1, the compound significantly inhibited but did not abolish the formation of TCA-insoluble phosphate. These results confirm earlier biochemical findings that alkaline phosphatase possesses a pyrophosphatase activity probably related to the turnover of phosphorylated macromolecules necessary for cell differentiation and proliferation.

Published

1987

49. An in-vitro study of enamel protein degradation in developing bovine enamel.

Author

Menanteau J, Mitre D, and Raher S

Subjects

Amelogenin, Animals, Cattle, Chemical Fractionation methods, Chromatography, High Pressure Liquid, Fetus, Dental Enamel Proteins metabolism, Tooth Germ metabolism

Abstract

An immature enamel fraction, as far as possible without cells, was prepared from fetal bovine molars, using aqueous-density fractionation. Portions were incubated at 37 degrees C with or without protease inhibitors. Amelogenins and enamelins were then examined for their molecular weight using HPLC-gel permeation. Degradation of amelogenins occurred rapidly and appeared to be related to proteolytic activity, probably localized extra-cellularly. Enamelins remained almost stable over the time intervals used.

Published

1986

50. The effects of ATP depletion and ionophore A23187 on calcium transport in the secretory rat enamel organ.

Author

Vicars TM, Stanfield CN, Crenshaw MA, and Bawden JW

Subjects

Animals, Biological Transport drug effects, Culture Techniques, Dental Enamel growth & development, Dental Enamel metabolism, Rats, Rats, Inbred Strains, Adenosine Triphosphate metabolism, Calcimycin pharmacology, Calcium metabolism, Enamel Organ metabolism, Tooth Germ metabolism

Abstract

An in-vitro system was used to study the effects of ATP depletion in the cells of the enamel organ and the use of the calcium ionophore A23187 on the mineralization of rat molar secretory stage enamel and 45Ca-movement through the enamel organ. Mineralization of the explants and 45Ca-uptake by the enamel were both enhanced by ATP depletion. No changes in these parameters were observed when the ionophore was added to the medium. The mechanism that limits the rate of calcium transport through the enamel organ during the secretory phase of enamel development is thus ATP-dependent. The result is consistent with the Takano-Crenshaw hypothesis for transcellular calcium transport. Use of the calcium ionophore A23187 failed to define further the nature of the calcium transport mechanism.

Published

1983