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6. Growth and layer structure optimization of 2.26 µm (AlGaIn)(AsSb) diode lasers for room temperature operation

Author

Simanowski, S., Mermelstein, C., Walther, M., Herres, N., Kiefer, R., Rattunde, M., Schmitz, J., Wagner, J., Weimann, G., and Publica

Subjects
semiconducting quaternary alloy, quaternary alloy, laser diode, molecular beam epitaxy, antimonide, semiconducting III-V material, quaternäre Legierung, Molekularstrahlepitaxie, III-V Halbleiter
Abstract

The optimization of MBE growth conditions and layer structures for room temperature operation of 2.26 mu m AlGaAsSb/GalnAsSb laser structures is investigated. Index guided triple quantum well large optical cavity diode lasers with 64 mu m x 1000 mu m cavities and high reflection/antireflection coated facets reveal a cw output power of 350 mW at T = 280 K. An internal quantum efficiency eta(i) of 69 %, internal losses chi(i) of 7.7 cm(exp -1) and a threshold current density for infinite cavity length of 144 A/cm2 are obtained for this structure.

Published
2001

7. Room-temperature low-threshold low-loss continous-wave operation of 2.26 µm GaInAsSb/AlGaAsSb quantum-well laser diodes

Author

Mermelstein, C., Simanowski, S., Mayer, M., Kiefer, R., Schmitz, J., Walther, M., Wagner, J., and Publica

Subjects
GaSb, quantum efficiency, threshold current, loss coefficient, Laserspektrum, Verlustkoeffizient, cw-Betrieb, output power efficiency, GaInAsSb, Halbleiterlaserdiode, verbreiterte Wellenleiterstruktur, mid infrared, broadended waveguide, cw-operation, semiconductor laser diode, Quanteneffizienz, AlGaAsSb, mittleres Infrarot, quantum-well, Quantenfilm, Ausgangsleistungseffizienz, lasing spectra, Schwellstrom
Abstract

Strained single- and triple-quantum-well (SQW and TQW), large optical cavity GaInAsSb/ AlGaAsSb/GaSb laser diodes emitting at 2.26 mu m are investigated. Internal loss coefficients as low as 5 and 7.7 cm(exp -1) for the SQW and TQW, respectively, and relatively high internal quantum efficiencies of 65% (SQW) and 69% (TQW) were obtained. Extrapolated threshold current densities for infinite cavity lengths of 55 and 150 A/cm2 have been deduced for the SQW and TQW, respectively. These values scale very well with the number of QWs and are among the lowest reported for diode lasers in this wavelength range. A differential quantum efficiency as high as 50% and a total power efficiency of 23% were achieved at 280 K. The temperature dependence of the threshold current density revealed a high characteristic temperature of 110 K. Single-ended output powers of 240 mW in continuous-wave mode and exceeding 0.5 W in pulsed operation were obtained for a TQW laser with high-reflection/antireflection coated facets at 280 K, mounted substrate-side down.

Published
2000

8. Strain adjustment in (GaIn)(AsSb)/(AlGa)(AsSb) QWs for 2.3.-2.7. µm laser structures

Author

Simanowski, S., Herres, N., Mermelstein, C., Kiefer, R., Schmitz, J., Walther, M., Wagner, J., Weimann, G., and Publica

Subjects
GaSb, strain, AlGaAsSb, molecular beam epitaxy, pseudomorphe Verspannung, mittleres Infrarot, Halbleiterlaser, Molekularstrahlepitaxie, GaInAsSb, semiconductor laser, mid infrared
Abstract

The influence of strain in Ga(0.7)In(0.3)As(y)Sb(1-y) quantum wells (QWs) embedded in Al(0.24)Ga(0.76)As(y)Sb(1-Y) barriers on the photoluminescence (PL) emission wavelength and intensity has been investigated. The strain was adjusted by varying the As content in the QW and barrier layers. For As mole fractions in the (GaIn)(AsSb) QW layers between y = 0.25 and 0.05, the average strain perpendicular to the growth plane changes from (delta a/a) = 2.0 x 10(exp -3) to 10.4 x 10(exp -3) for lattice matched (AlGa)(AsSb) barriers. At room temperature, highest PL intensities are obtained for QW structures with a net compressive strain of (delta a/a) = 8.7 x 10(exp -3). In order to compensate the compressive strain in the QWs, strain-balanced laser core structures with barriers under tensile strain have been investigated. This was found to allow a reduction of the average strain in the laser core without shifting its emission wavelength. Ridge waveguide large optical cavity (LOC) laser diodes containing three compressively strained (Galn)(AsSb) QWs embedded between lattice matched (AlGa)(AsSb) barriers show room temperature cw laser emission at a wavelength of 2.26 mu m. For 64 mu m wide and 600 mu m long devices, a differential quantum efficiency of 43% and a threshold current density of 395 A/cm2 with a characteristic temperature of T(0) = 110 K are obtained.

Published
2000

9. Arsenic incorporation in molecular beam epitaxy (MBE) grown (AlGaIn)(AsSb) layers for 2.0-2.5 mu m laser structures on GaSb substrates

Author

Simanowski, S., Walther, M., Schmitz, J., Kiefer, R., Herres, N., Fuchs, F., Maier, M., Mermelstein, C., Wagner, J., Weimann, G., and Publica

Subjects
GaSb, AlGaAsSb, molecular beam epitaxy, Halbleiterlaser, mittleres Infrarot, Molekularstrahlepitaxie, GaInAsSb, semiconductor laser, mid infrared
Abstract

The incorporation of As and In during MBE growth in (AlGaIn)/(AsSb) layers used for the fabrication of diode lasers in the 2.0-2.5 mu m wavelength range has been investigated. The As content was found to depend linearly on the beam equivalent pressure for As mole fractions between y = 0.05 and y = 0.20. Broad area A1GaAsSb/GaInAsSb singlequantum well laser diodes with quasi-cw output at room temperature at an emission wavelength of 2.03 mu m and a threshold current density of 515 A/cm2 for 1370 mu m long and 70 mu m wide devices have been fabricated. In order to shift the emission wavelength of the laser structures to longer wavelengths, the growth of lattice matched AlGaAsSb/ GaInAsSb laser core structures with different In and As mole fractions in the quantum wells has been investigated.

Published
1999

13. Specific Preschool Executive Functions Predict Unique Aspects of Mathematics Development: A 3-Year Longitudinal Study.

Author

Simanowski S and Krajewski K

Subjects
Child, Child, Preschool, Factor Analysis, Statistical, Female, Humans, Longitudinal Studies, Male, Schools, Child Development physiology, Executive Function physiology, Inhibition, Psychological, Mathematical Concepts
Abstract

This study assessed the extent to which executive functions (EF), according to their factor structure in 5-year-olds (N = 244), influenced early quantity-number competencies, arithmetic fluency, and mathematics school achievement throughout first and second grades. A confirmatory factor analysis resulted in updating as a first, and inhibition and shifting as a combined second factor. In the structural equation model, updating significantly affected knowledge of the number word sequence, suggesting a facilitatory effect on basic encoding processes in numerical materials that can be learnt purely by rote. Shifting and inhibition significantly influenced quantity to number word linkages, indicating that these processes promote developing a profound understanding of numbers. These results show the supportive role of specific EF for specific aspects of a numerical foundation., (© 2017 The Authors. Child Development © 2017 Society for Research in Child Development, Inc.)

Published
2019
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14. The cell-cell junctions of mammalian testes: I. The adhering junctions of the seminiferous epithelium represent special differentiation structures.

Author

Domke LM, Rickelt S, Dörflinger Y, Kuhn C, Winter-Simanowski S, Zimbelmann R, Rosin-Arbesfeld R, Heid H, and Franke WW

Subjects
Adherens Junctions ultrastructure, Animals, Desmosomes metabolism, Fluorescent Antibody Technique, Glycoproteins metabolism, Male, Seminiferous Epithelium cytology, Seminiferous Epithelium ultrastructure, Adherens Junctions metabolism, Cell Differentiation, Seminiferous Epithelium metabolism, Testis metabolism
Abstract

The seminiferous tubules and the excurrent ducts of the mammalian testis are physiologically separated from the mesenchymal tissues and the blood and lymph system by a special structural barrier to paracellular translocations of molecules and particles: the "blood-testis barrier", formed by junctions connecting Sertoli cells with each other and with spermatogonial cells. In combined biochemical as well as light and electron microscopical studies we systematically determine the molecules located in the adhering junctions of adult mammalian (human, bovine, porcine, murine, i.e., rat and mouse) testis. We show that the seminiferous epithelium does not contain desmosomes, or "desmosome-like" junctions, nor any of the desmosome-specific marker molecules and that the adhering junctions of tubules and ductules are fundamentally different. While the ductules contain classical epithelial cell layers with E-cadherin-based adherens junctions (AJs) and typical desmosomes, the Sertoli cells of the tubules lack desmosomes and "desmosome-like" junctions but are connected by morphologically different forms of AJs. These junctions are based on N-cadherin anchored in cytoplasmic plaques, which in some subforms appear thick and dense but in other subforms contain only scarce and loosely arranged plaque structures formed by α- and β-catenin, proteins p120, p0071 and plakoglobin, together with a member of the striatin family and also, in rodents, the proteins ZO-1 and myozap. These N-cadherin-based AJs also include two novel types of junctions: the "areae adhaerentes", i.e., variously-sized, often very large cell-cell contacts and small sieve-plate-like AJs perforated by cytoplasm-to-cytoplasm channels of 5-7 nm internal diameter ("cribelliform junctions"). We emphasize the unique character of this epithelium that totally lacks major epithelial marker molecules and structures such as keratin filaments and desmosomal elements as well as EpCAM- and PERP-containing junctions. We also discuss the nature, development and possible functions of these junctions.

Published
2014
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15. Protein LUMA is a cytoplasmic plaque constituent of various epithelial adherens junctions and composite junctions of myocardial intercalated disks: a unifying finding for cell biology and cardiology.

Author

Franke WW, Dörflinger Y, Kuhn C, Zimbelmann R, Winter-Simanowski S, Frey N, and Heid H

Subjects
Adult, Aged, Amino Acid Sequence, Animals, Cattle, Cell Fractionation, Cells, Cultured, Epithelial Cells metabolism, Humans, Lumican, Male, Middle Aged, Molecular Sequence Data, Swine, Adherens Junctions metabolism, Chondroitin Sulfate Proteoglycans metabolism, Keratan Sulfate metabolism, Myocardium cytology, Myocardium metabolism
Abstract

In a series of recent reports, mutations in the gene encoding a protein called LUMA (or TMEM43), widely speculated to be a tetraspan transmembrane protein of the nuclear envelope, have been associated with a specific subtype of cardiomyopathy (arrhythmogenic cardiomyopathies) and cases of sudden death. However, using antibodies of high specificity in immunolocalization experiments, we have discovered that, in mammals, LUMA is a component of zonula adhaerens and punctum adhaerens plaques of diverse epithelia and epithelial cell cultures and is also located in (or in some species associated with) the plaques of composite junctions (CJs) in myocardiac intercalated disks (IDs). In CJs, LUMA often colocalizes with several other CJ marker proteins. In all these cells, LUMA has not been detected in the nuclear envelope. Surprisingly, under certain conditions, similar CJ localizations have also been seen with some antibodies commercially available for some time. The identification of LUMA as a plaque component of myocardiac CJs leads to reconsiderations of the molecular composition and architecture, the development, the functions, and the pathogenic states of CJs and IDs. These findings now also allow the general conclusion that LUMA has to be added to the list of mutations of cardiomyocyte junction proteins that may be involved in cardiomyopathies.

Published
2014
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16. Transmembrane protein PERP is a component of tessellate junctions and of other junctional and non-junctional plasma membrane regions in diverse epithelial and epithelium-derived cells.

Author

Franke WW, Heid H, Zimbelmann R, Kuhn C, Winter-Simanowski S, Dörflinger Y, Grund C, and Rickelt S

Subjects
3T3 Cells, Animals, Antibodies, Monoclonal immunology, Cattle, Cell Line, Tumor, Cell Membrane, Desmosomes metabolism, Epithelial Cells, Genes, Tumor Suppressor, HT29 Cells, Hep G2 Cells, Humans, MCF-7 Cells, Membrane Proteins analysis, Membrane Proteins immunology, Mice, Rats, Swine, Adherens Junctions metabolism, Epithelium metabolism, Membrane Proteins metabolism
Abstract

Protein PERP (p53 apoptosis effector related to PMP-22) is a small (21.4 kDa) transmembrane polypeptide with an amino acid sequence indicative of a tetraspanin character. It is enriched in the plasma membrane and apparently contributes to cell-cell contacts. Hitherto, it has been reported to be exclusively a component of desmosomes of some stratified epithelia. However, by using a series of newly generated mono- and polyclonal antibodies, we show that protein PERP is not only present in all kinds of stratified epithelia but also occurs in simple, columnar, complex and transitional epithelia, in various types of squamous metaplasia and epithelium-derived tumors, in diverse epithelium-derived cell cultures and in myocardial tissue. Immunofluorescence and immunoelectron microscopy allow us to localize PERP predominantly in small intradesmosomal locations and in variously sized, junction-like peri- and interdesmosomal regions ("tessellate junctions"), mostly in mosaic or amalgamated combinations with other molecules believed, to date, to be exclusive components of tight and adherens junctions. In the heart, PERP is a major component of the composite junctions of the intercalated disks connecting cardiomyocytes. Finally, protein PERP is a cobblestone-like general component of special plasma membrane regions such as the bile canaliculi of liver and subapical-to-lateral zones of diverse columnar epithelia and upper urothelial cell layers. We discuss possible organizational and architectonic functions of protein PERP and its potential value as an immunohistochemical diagnostic marker.

Published
2013
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17. The plaque protein myozap identified as a novel major component of adhering junctions in endothelia of the blood and the lymph vascular systems.

Author

Pieperhoff S, Rickelt S, Heid H, Claycomb WC, Zimbelmann R, Kuhn C, Winter-Simanowski S, Kuhn C, Frey N, and Franke WW

Subjects
Animals, Antibody Specificity immunology, Cattle, Cell Line, Electrophoresis, Polyacrylamide Gel, Endothelial Cells metabolism, Endothelium, Vascular ultrastructure, Fluorescent Antibody Technique, Humans, Immunoblotting, Immunoprecipitation, Mice, Myocardium cytology, Myocytes, Cardiac metabolism, Pulmonary Alveoli metabolism, Pulmonary Alveoli ultrastructure, Rats, Sus scrofa, Adherens Junctions metabolism, Endothelium, Vascular metabolism, Lymph metabolism, Lymphatic Vessels metabolism, Membrane Proteins blood, Membrane Proteins metabolism
Abstract

Recently the protein myozap, a 54-kD polypeptide which is not a member of any of the known cytoskeletal and junctional protein multigene families, has been identified as a constituent of the plaques of the composite junctions in the intercalated disks connecting the cardiomyocytes of mammalian hearts. Using a set of novel, highly sensitive and specific antibodies we now report that myozap is also a major constituent of the cytoplasmic plaques of the adherens junctions (AJs) connecting the endothelial cells of the mammalian blood and lymph vascular systems, including the desmoplakin-containing complexus adhaerentes of the virgultar cells of lymph node sinus. In light and electron microscopic immunolocalization experiments we show that myozap colocalizes with several proteins of desmosomal plaques as well as with AJ-specific transmembrane molecules, including VE-cadherin. In biochemical analyses, rigorous immunoprecipitation experiments have revealed N-cadherin, desmoplakin, desmoglein-2, plakophilin-2, plakoglobin and plectin as very stably bound complex partners. We conclude that myozap is a general component of cell-cell junctions not only in the myocardium but also in diverse endothelia of the blood and lymph vascular systems of adult mammals, suggesting that this protein not only serves a specific role in the heart but also a broader set of functions in the vessel systems. We also propose to use myozap as an endothelial cell type marker in diagnoses., (© 2011 The Authors Journal of Cellular and Molecular Medicine © 2011 Foundation for Cellular and Molecular Medicine/Blackwell Publishing Ltd.)

Published
2012
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18. The adhering junctions of valvular interstitial cells: molecular composition in fetal and adult hearts and the comings and goings of plakophilin-2 in situ, in cell culture and upon re-association with scaffolds.

Author

Barth M, Rickelt S, Noffz E, Winter-Simanowski S, Niemann H, Akhyari P, Lichtenberg A, and Franke WW

Subjects
Adult, Animals, Cell Culture Techniques, Electrophoresis, Gel, Two-Dimensional, Heart Valves cytology, Humans, Microscopy, Electron, Microscopy, Fluorescence, Swine, Adherens Junctions metabolism, Heart Valves metabolism, Plakophilins metabolism
Abstract

The interstitial cells of cardiac valves represent one of the most frequent cell types in the mammalian heart. In order to provide a cell and molecular biological basis for the growth of isolated valvular interstitial cells (VICs) in cell culture and for the use in re-implantation surgery we have examined VICs in situ and in culture, in fetal, postnatal and adult hearts, in re-associations with scaffolds of extracellular matrix (ECM) material and decellularized heart valves. In all four mammalian species examined (human, bovine, porcine and ovine), the typical mesenchymal-type cell-cell adherens junctions (AJs) connecting VICs appear as normal N-cadherin based puncta adhaerentia. Their molecular ensemble, however, changes under various growth conditions insofar as plakophilin-2 (Pkp2), known as a major cytoplasmic plaque component of epithelial desmosomes, is recruited to and integrated in the plaques of VIC-AJs as a major component under growth conditions characterized by enhanced proliferation, i.e., in fetal heart valves and in cell cultures. Upon re-seeding onto decellularized heart valves or in stages of growth in association with artificial scaffolds, Pkp2 is - for the most part - lost from the AJs. As Pkp2 has recently also been detected in AJs of cardiac myxomata and diverse other mesenchymal tumors, the demonstrated return to the normal Pkp2-negative state upon re-association with ECM scaffolds and decellularized heart valves may now provide a safe basis for the use of cultured VICs in valve replacement surgery. Even more surprising, this type of transient acquisition of Pkp2 has also been observed in distinct groups of endothelial cells of the endocardium, where it seems to correspond to the cell type ready for endothelial-mesenchymal transition (EMT).

Published
2012
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19. Protein myozap--a late addition to the molecular ensembles of various kinds of adherens junctions.

Author

Rickelt S, Kuhn C, Winter-Simanowski S, Zimbelmann R, Frey N, and Franke WW

Subjects
Animals, Cattle, Cell Adhesion physiology, Immunohistochemistry, Membrane Proteins chemistry, Mice, Microscopy, Fluorescence, Muscle Proteins chemistry, Phosphoproteins chemistry, Rats, Tight Junctions metabolism, Zonula Occludens-1 Protein, Adherens Junctions metabolism, Membrane Proteins metabolism, Muscle Proteins metabolism, Phosphoproteins metabolism
Abstract

The protein myozap, a polypeptide of 54 kDa, has recently been identified as a component of the cytoplasmic plaques of the composite junctions (areae compositae) in the myocardiac intercalated disks and of the adherens junctions (AJs) in vascular endothelia. Now we report that using very sensitive new antibodies and drastic localization methods, we have also identified this protein as a component of the AJ plaques in simple and complex epithelia, in the adluminal cell layer of the transitional epithelium of the urinary tract and in certain cell layers of diverse stratified epithelia, including gingiva, tongue, pharynx and esophagus, cervix, vagina and epidermis. Myozap has not been identified in desmosomal and tight junction plaques. We have also detected protein myozap in AJ structures of carcinomas. The discovery of a novel major protein in AJ plaques now calls for re-examinations of molecular interactions in AJ formation and maintenance and also offers a new marker for diagnostic immunocytochemistry. We also discuss the need for progressive unravelling, extractive treatments and buffer rinses of sections and cultured cells to reveal obscured or masked antigens, before definitive negative conclusions in immunohistochemistry can be made.

Published
2011
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20. Upregulation of plakophilin-2 and its acquisition to adherens junctions identifies a novel molecular ensemble of cell-cell-attachment characteristic for transformed mesenchymal cells.

Author

Rickelt S, Winter-Simanowski S, Noffz E, Kuhn C, and Franke WW

Subjects
Adherens Junctions chemistry, Animals, Cell Adhesion, Cells, Cultured, Humans, Mesenchymal Stem Cells chemistry, Mice, Plakophilins analysis, Plakophilins genetics, Up-Regulation, Adherens Junctions physiology, Cell Transformation, Neoplastic, Mesoderm pathology, Plakophilins physiology
Abstract

In contrast to the desmosome-containing epithelial and carcinoma cells, normal and malignantly transformed cells derived from mesenchymal tissues and tumors are connected only by adherens junctions (AJs) containing N-cadherins and/or cadherin-11, anchored in a cytoplasmic plaque assembled by alpha- and beta-catenin, plakoglobin, proteins p120 and p0071. Here, we report that the AJs of many malignantly transformed cell lines are characterized by the additional presence of plakophilin-2 (Pkp2), a protein hitherto known only as a major component of desmosomal plaques, i.e., AJs of epithelia and carcinomatous cells. This massive acquisition of Pkp2 and its integration into AJ plaques of a large number of transformed cell lines is demonstrated with biochemical and immunolocalization techniques. Upregulation of Pkp2 and its integration into AJs has also been noted in some soft tissue tumors insitu and some highly proliferative colonies of cultured mesenchymal stem cells. As Pkp2 has recently been identified as a functionally important major regulatory organizer in AJs and related junctions in epithelial cells and cardiomyocytes, we hypothesize that the integration of Pkp2 into AJs of "soft tissue tumor" cells also can serve functions in the upregulation of proliferation, the promotion of malignant growth in general as well as the close-packing of diverse kinds of cells and the metastatic behavior of such tumors. We propose to examine its presence in transformed mesenchymal cells and related tumors and to use it as an additional diagnostic criterion., ((c) 2009 UICC.)

Published
2009
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21. The area composita of adhering junctions connecting heart muscle cells of vertebrates - III: assembly and disintegration of intercalated disks in rat cardiomyocytes growing in culture.

Author

Franke WW, Schumacher H, Borrmann CM, Grund C, Winter-Simanowski S, Schlechter T, Pieperhoff S, and Hofmann I

Subjects
Adherens Junctions ultrastructure, Animals, Animals, Newborn, Antibody Specificity immunology, Cadherins ultrastructure, Cells, Cultured, Desmoglein 2 ultrastructure, Desmoplakins ultrastructure, Fluorescent Antibody Technique, Immunoblotting, Myocytes, Cardiac ultrastructure, Rats, Rats, Wistar, Adherens Junctions metabolism, Myocytes, Cardiac cytology, Myocytes, Cardiac metabolism, Vertebrates metabolism
Abstract

For cell and molecular biological studies of heart formation and function cell cultures of embryonal, neonatal or adult hearts of various vertebrates, notably rat and chicken, have been widely used. As the myocardium-specific cell-cell junctions, the intercalated disks (ID), have recently been found to be particularly sensitive to losses of - or mutations in - certain cytoskeletal proteins, resulting in cardiac damages, we have examined the ID organization in primary cultures of cardiomyocytes obtained from neonatal rats. Using immunofluorescence and immunoelectron microscopy, we have studied the major ID components for up to 2 weeks in culture, paying special attention to spontaneously beating, individual cardiomyocytes and myocardial cell colonies. While our results demonstrate the formation of some ID-like cardiomyocyte-connecting junction arrays, they also reveal a variety of structural disorders such as rather extended, junction-free ID regions, sac-like invaginations and endocytotic blebs as well as accumulations of intracytoplasmic structures suggestive of endocytosed forms of junction-derived vesicles or of junction fragments resembling fascia adhaerens elements. Moreover, we have noticed a novel type of small, obviously plaque-free cytoplasmic vesicles containing one or both of the desmosomal cadherins, desmocollin Dsc2 and desmoglein Dsg2. We conclude that cardiomyocyte cultures are useful model systems for studies of certain aspects of myocardiac differentiation and functions but, on the other hand, show progressive disintegration and deterioration. The potential value of molecular markers and reagents in studies of myocardial pathology as well as in the monitoring of myocardial differentiation of so-called stem cells is discussed.

Published
2007
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22. Cell type-specific desmosomal plaque proteins of the plakoglobin family: plakophilin 1 (band 6 protein).

Author

Heid HW, Schmidt A, Zimbelmann R, Schäfer S, Winter-Simanowski S, Stumpp S, Keith M, Figge U, Schnölzer M, and Franke WW

Subjects
Amino Acid Sequence, Animals, Antibodies, Monoclonal, Base Sequence, Blotting, Northern, Cattle, Cells, Cultured, Chickens, DNA, Complementary chemistry, Humans, Immunohistochemistry, Mice, Molecular Sequence Data, Plakophilins, Proteins chemistry, Rats, Sequence Homology, Amino Acid, Swine, Xenopus laevis, Desmosomes chemistry, Proteins analysis
Abstract

Desmosomes represent a special type of the plaque-bearing adhering junctions, characteristic of certain pathways of cell differentiation, which compositionally are not identical in the various kinds of desmosome-forming cells. While all desmosomes contain the cytoplasmic plaque proteins desmoplakin I and plakoglobin, they can vary in their specific complement of desmosomal cadherins and by the presence of additional plaque proteins. We have raised monoclonal antibodies recognizing one such 'accessory' plaque protein, the cytokeratin-binding, basic protein plakophilin 1, originally introduced as 'band 6 protein' or 'polypeptide D6', which is an abundant desmosomal component in certain epithelia. Using such antibodies, we have isolated cDNA clones encoding the bovine and the human protein and determined their complete amino acid sequences. The mRNAs, which on Northern blot tests appear as two bands corresponding to approximately 4 and 2.4 kb (bovine) or 5 and 2.6 kb (human), code for 727 amino acids (calculated mol. wt. 80,180; IEP 9.25) in bovine and 726 amino acids (mol. wt. 80,496; IEP 9.34) in human plakophilin. Sequence analyses have revealed the presence of 9.2 repeated units of the arm-motif sequence, confirming our previous conclusion that this protein is a member of a larger family of proteins including, inter alia, several membrane-associated plaque proteins such as vertebrate plakoglobin and beta-catenin as well as the product of the armadillo gene of Drosophila. The plakophilin antibodies and cDNA probes have also allowed us to examine its synthesis in various tissues and cell cultures. While we confirm the occurrence of the protein in cytoskeletal fractions from various stratified squamous, complex, glandular duct and bladder epithelia, where it can be localized to desmosomes, we have, surprisingly, also identified the protein, although at lower amounts, in cytoskeletal fractions from several cultured cell lines in which the protein has not been consistently localized to desmosomes by immunofluorescence microscopy. Examples include cultured cells derived from certain simple epithelia such as the kidney-derived line MDBK and cultured calf lens cells. We have also found that, in all plakophilin 1-positive cells examined, a pool of diffusible ('soluble') cytoplasmic plakophilin exists, including cell lines such as human mammary carcinoma MCF-7 cells in which this soluble plakophilin seems to be the only detectable form. In addition, we have identified some soluble proteins conspicuously cross-reacting with plakophilin 1. Possible functions of plakophilin and its potential value as a marker for specific states of cell differentiation are discussed, particularly with respect to tumor diagnosis.

Published
1994
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24. Cytokeratins and cytokeratin filaments in subpopulations of cultured human and rodent cells of nonepithelial origin: modes and patterns of formation.

Author

Knapp AC, Bosch FX, Hergt M, Kuhn C, Winter-Simanowski S, Schmid E, Regauer S, Bartek J, and Franke WW

Subjects
Animals, Antibodies, Monoclonal, Cell Line, Fibroblasts cytology, Humans, Immunohistochemistry, Keratins metabolism, Muscle, Smooth cytology, Neuroglia cytology, RNA, Messenger metabolism, Rats, Tumor Cells, Cultured, Fibroblasts metabolism, Gene Expression Regulation, Keratins genetics, Muscle, Smooth metabolism, Neuroglia metabolism
Abstract

Using immunofluorescence microscopy, we observed that in several established cell culture lines derived from different nonepithelial tissues and species, cells spontaneously emerge, usually at low frequencies, which contain cytoplasmic structures decorated by antibodies specific for cytokeratins 8 and 18. This phenomenon was further examined at both the protein (gel electrophoreses of cytoskeletal proteins, followed by immunoblotting) and the RNA (Northern blots, "nuclear run-on" analysis, in situ hybridization) level. Positive cell lines included simian virus (SV40)-transformed human fibroblasts (HF-SV80, WI-38 VA13), human astrocytic glioma cells (U333 CG/343MG), rat (RVF-SMC) and hamster (BHK-21/13) cells derived from vascular smooth muscle and murine sarcoma MS-180 cells. In two cell lines (HF-SV80 and BHK-21/13), the frequency of the cytokeratin-containing cells and of the cytokeratin fibril arrays per cell was drastically increased upon treatment with 5-azacytidine. The structural appearance of the cytokeratins was variable in the different cell lines but could also differ among cells of the same culture: While small granular or comma-shaped structures or bizarrely shaped filament arrays prevailed in WI-38, RVF and normally grown BHK-21 cells, most of the other lines revealed extended normal-looking, fibrillar arrays. In one line (MS-180), the appearance of cytokeratins was associated with a morphological change, as it was only found in a subpopulation of cells that had lost their typical elongated and spindle-shaped phenotype and assumed a rounded ("coccoid") shape. Our results show that the expression of the genes encoding cytokeratins 8 and 18 is not necessarily restricted to programs of epithelial differentiation and that factors stochastically effective appear in cultured cell lines that allow the synthesis of these cytoskeletal components. Mechanisms possibly involved in this spontaneous and selective advent of cytokeratins 8 and 18 and implications for tumor diagnosis are discussed.

Published
1989
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