Your search keyword '"Gratzl, M"' showing total 114 results

1. Stimulation-dependent uptake of an extracellular marker to subcellular fractions of isolated neurohypophysial tissue

Author

Gratzl, M., Russell, J. T., and Thorn, N. A.

Published

1983

2. 'A nose in the gut': Olfactory receptors in the human gastrointestinal tract

Author

Braun, T, Voland, P, Kunz, L, Prinz, C, Gratzl, M, Braun, T, Voland, P, Kunz, L, Prinz, C, and Gratzl, M

Published

2009

3. 'Die Nase im Darm': olfaktorische Rezeptoren im menschlichen Magen-Darm-Trakt

Author

Braun, T, Voland, P, Kunz, L, Prinz, C, Gratzl, M, Braun, T, Voland, P, Kunz, L, Prinz, C, and Gratzl, M

Published

2009

4. Mechanismen der Endo- und Exozytose in Enterochromaffin-like (ECL) Zellen des Rattenmagens

Author

Prinz, Chr. (apl. Prof. Dr.), Gratzl, M. (Univ.-Prof. Dr., Ludwig-Maximilians-Universität München), Fend, F. (Univ.-Prof. Dr.), Zanner, Robert, Prinz, Chr. (apl. Prof. Dr.), Gratzl, M. (Univ.-Prof. Dr., Ludwig-Maximilians-Universität München), Fend, F. (Univ.-Prof. Dr.), and Zanner, Robert

Abstract

Enterochromaffin-like (ECL) Zellen sind neuroendokrine Zellen der Magenschleimhaut, die eine wichtige Rolle bei der peripheren Regulation der Magensäureproduktion spielen. Nach Stimulation mit Gastrin kommt es zur calciumabhängigen Freisetzung von Histamin, das in Parietalzellen die Synthese und Sekretion von Magensäure auslöst. In vorliegender Arbeit wurden Bedeutung und Entstehung des Calciumsignals für die gastrininduzierte Histaminsekretion sowie Expression der Endozytoseproteine Amphiphysin und Dynamin untersucht. Für die Erhöhung von [Ca2+]i war die Aktivierung von InsP3-Rezeptoren, nicht jedoch die Entleerung intrazellulärer Calciumspeicher nötig. Der für die Exozytose notwendige Calciumeinstrom konnte durch Nimodipin gehemmt werden, was eine Beteilung spannungsgesteuerter L-Typ Calciumkanäle nahe legt. Alle Dynamin- und Amphiphysin-Isoformen konnten auf mRNA- und Proteinebene nachgewiesen werden. Eine neue Splice-Variante von Amphiphysin-2 wurde ebenfalls entdeckt., Enterochromaffin-like (ECL) cells are neuroendocrine cells of the gastric mucosa that are important for the peripheral regulation of gastric acid secretion. Following stimulation with gastrin, histamine is released from ECL cells in a calcium-dependent manner, inducing synthesis and secretion of gastric acid in parietal cells. In this thesis, importance and generation of the calcium signal necessary for gastrin-induced histamine secretion were investigated, as well as the expression of the endocytic proteins amphiphysin and dynamin. Activation of InsP3 receports but not calcium release from intracellular stores was nessecary for the increase in [Ca2+]i. Calcium influx could be inhibited by nimodipine, indicating involvement of voltage-activated L-type calcium channels. All known dynamin and amphiphysin isoforms could be detected on mRNA and protein levels. Furthermore, a novel splice form of amphiphysin-2 was found to be expressed in ECL cells.

Published

2005

5. GABAerges System in Leydigzellen und die Stimulation der Zellproliferation durch GABA

Author

Mayerhofer, A. (Univ.-Prof. Dr.), Ring, J. (Univ.-Prof. Dr. Dr.), Gratzl, M. (Univ.-Prof. Dr. , Ludwig-Maximilians-Universität München), Geigerseder, Christof, Mayerhofer, A. (Univ.-Prof. Dr.), Ring, J. (Univ.-Prof. Dr. Dr.), Gratzl, M. (Univ.-Prof. Dr. , Ludwig-Maximilians-Universität München), and Geigerseder, Christof

Abstract

Im Rahmen dieser Arbeit wurde das den Neurotransmitter GABA synthetisierende Enzym GAD, der vesikuläre GABA-Transporter VGAT und GABA-Rezeptoren im Hoden von Nagern und Menschen nachgewiesen. Sowohl die Quelle von GABA, als auch GABA-Rezeptoren wurden in endokrinen Zellen des Hodens, den Testosteron bildenden Leydigzellen, lokalisiert. Weiterhin zeigten zellbiologische Untersuchungen, dass die etablierte Leydigzelllinie TM3 enzymatisch aktives GAD besitzt und auf GABAerge Stimulation mit einem Anstieg ihrer Zellproliferation reagiert. Die pharmakologische Charakterisierung der Proliferationswirkung ergab eine Übertragung durch GABA-A-Rezeptoren. Außerdem wurden die Gene c-fos und hsf-1 durch einen cDNA-Array als Bestandteile des Signaltransduktionswegs der GABA-A-Rezeptor vermittelten Wirkung nachgewiesen. Leydigzellen verfügen demnach über ein GABAerges System, wobei GABA auto- bzw. parakrin durch GABA-A-Rezeptoren die Proliferation von Leydigzellen reguliert., In context of this work the GABA synthesizing enzyme GAD, the vesicular GABA transporter VGAT and GABA receptors were identified in rodent and human testis. GABAergic sources, as well as GABA receptors were localized in testosteron producing Leydig cells in the endocrine compartment of the testis. Furthermore cell biological studies showed that the established Leydig cell line TM3 exhibits enzymatically active GAD and that GABAergic stimulation of TM3 cells leads to increased cell proliferation. Pharmacological characterization of this proliferative action of GABA revealed an GABA-A receptor mediated mechanism. Moreover the genes c-fos and hsf-1 were identified by c-DNA-array experiments to be components of the GABA-A receptor mediated signal transduction cascade. In conclusion Leydig cells posses a GABAergic system, whereby GABA regulates Leydig cell proliferation via GABA-A receptors in an auto- or paracrine manner.

Published

2005

6. GABAerges System in Leydigzellen und die Stimulation der Zellproliferation durch GABA

Author

Ring, J. (Univ.-Prof. Dr. Dr.);Mayerhofer, A. (Univ.-Prof. Dr.), Ring, J. (Univ.-Prof. Dr. Dr.);Gratzl, M. (Univ.-Prof. Dr. , Ludwig-Maximilians-Universität München), Geigerseder, Christof, Ring, J. (Univ.-Prof. Dr. Dr.);Mayerhofer, A. (Univ.-Prof. Dr.), Ring, J. (Univ.-Prof. Dr. Dr.);Gratzl, M. (Univ.-Prof. Dr. , Ludwig-Maximilians-Universität München), and Geigerseder, Christof

Abstract

Im Rahmen dieser Arbeit wurde das den Neurotransmitter GABA synthetisierende Enzym GAD, der vesikuläre GABA-Transporter VGAT und GABA-Rezeptoren im Hoden von Nagern und Menschen nachgewiesen. Sowohl die Quelle von GABA, als auch GABA-Rezeptoren wurden in endokrinen Zellen des Hodens, den Testosteron bildenden Leydigzellen, lokalisiert. Weiterhin zeigten zellbiologische Untersuchungen, dass die etablierte Leydigzelllinie TM3 enzymatisch aktives GAD besitzt und auf GABAerge Stimulation mit einem Anstieg ihrer Zellproliferation reagiert. Die pharmakologische Charakterisierung der Proliferationswirkung ergab eine Übertragung durch GABA-A-Rezeptoren. Außerdem wurden die Gene c-fos und hsf-1 durch einen cDNA-Array als Bestandteile des Signaltransduktionswegs der GABA-A-Rezeptor vermittelten Wirkung nachgewiesen. Leydigzellen verfügen demnach über ein GABAerges System, wobei GABA auto- bzw. parakrin durch GABA-A-Rezeptoren die Proliferation von Leydigzellen reguliert., In context of this work the GABA synthesizing enzyme GAD, the vesicular GABA transporter VGAT and GABA receptors were identified in rodent and human testis. GABAergic sources, as well as GABA receptors were localized in testosteron producing Leydig cells in the endocrine compartment of the testis. Furthermore cell biological studies showed that the established Leydig cell line TM3 exhibits enzymatically active GAD and that GABAergic stimulation of TM3 cells leads to increased cell proliferation. Pharmacological characterization of this proliferative action of GABA revealed an GABA-A receptor mediated mechanism. Moreover the genes c-fos and hsf-1 were identified by c-DNA-array experiments to be components of the GABA-A receptor mediated signal transduction cascade. In conclusion Leydig cells posses a GABAergic system, whereby GABA regulates Leydig cell proliferation via GABA-A receptors in an auto- or paracrine manner.

Published

2005

7. Einfluß der synaptischen Vesikelproteine Synaptophysin und Synaptobrevin auf Wachstum und Differenzierung der hippocampalen Zellkultur

Author

Grosse, G., Gratzl, M., Schulze, W., Gorsleben, Martin, Grosse, G., Gratzl, M., Schulze, W., and Gorsleben, Martin

Abstract

Ziel der vorliegenden Arbeit war es, die Rolle der synaptischen Vesikelproteine Synaptophysin und Synaptobrevin bei Wachstum und Differenzierung der primär dissoziierten hippocampalen Zellkultur 17 Tage alter Mäuseembryonen zu untersuchen. Besonderes Interesse galt dabei dem Fortsatzwachstum und der Synaptogenese. Durch Beobachtung von Zellmorphologie und Zellwachstum wurde gezeigt, daß die Ausbildung charakteristischer Zelltypen ein intrinsischer Prozeß der hippocampalen Neurone ist. Die Synaptogenese wurde durch die Darstellung der entwicklungsabhängigen Verteilung der synaptischen Vesikelproteine Synaptophysin und Synaptobrevin mittels Immunfluoreszenzmarkierung dokumentiert. Durch elektronenmikroskopische Aufnahmen wurde die Differenzierung subzellulärer Strukturen der hippocampalen Zellkultur charakterisiert und die Verteilung von Synaptophysin und Synaptobrevin entwicklungsabhängig dargestellt. Synaptophysin fand sich nicht nur in axonalen Präsynapsen, sondern auch in Dendriten. Synaptobrevin war im Gegensatz zu Synaptophysin nicht in allen synaptischen Vesikeln der Axonterminalen darstellbar. Um die Wirkungen von Synaptophysin und Synaptobrevin auf hippocampale Neurone in der Kultur genauer zu untersuchen, standen zwei Versuchsmodelle zur Verfügung: 1. die Synaptophysin-defiziente Maus und 2. das clostridiale Neurotoxin Tetanustoxin (TeNT), das Synaptobrevin spezifisch spaltet. Anhand der Depletion von Synaptophysin wurde untersucht, ob in vitro das Fehlen des Proteins Konsequenzen in Bezug auf Synapsenbildung und morphologisches Erscheinungsbild der Neurone hat. Es konnten lichtmikroskopisch und auch im elektronenmikroskopischen Bild keine Unterschiede zu Kontrollkulturen festgestellt werden. Durch morphometrische Messungen zeigte sich, daß in der Kultur der Synaptophysin-depletierten Maus nach 2 DIV mit hoher Signifikanz die Dendriten länger als in Kontrollkulturen waren. Dies spricht für regulatorische Funktionen des Proteins bei Exo- und Endozytosevorgäng, Goal of this work was to investigate the role of the synaptic vesicle proteins synaptophysin and synaptobrevin during development and differentiation of mouse fetal hippocampal neurons in primary culture. The outgrowth of dendritic and axonal fibers and the mechanisms of synaptogenesis were of special interest. Observation of morphology and development showed that generation of characteristic cell types is an intrinsic process of hippocampal neurons. Differentiation of cellular and subcellular structures in hippocampal cell culture, characteristics of synaptogenesis and the stage-dependent distribution of synaptophysin and synaptobrevin were demonstrated by immunofluorescence and electron microscopy. Synaptophysin was localized in presynaptic axon terminals but also in dendrites. In contrast with synaptophysin immunoreaction for synaptobrevin could not be found in all synaptic vesicles of the presynaptic axon terminal. To investigate the influence of synaptophysin and synaptobrevin on hippocampal neurons in culture two experimental models were used, first a synaptophysin-knock-out-mouse and second the clostridial neurotoxin tetanustoxin (TeNT) which selectively cleaves synaptobrevin. With the depletion of synaptophysin we investigated if there are consequences in development of synapses and morphological features of the neurons in vitro. In both, light and electron microscopy, there was no difference to control cultures. In morphometric measurements there was a significant difference in the lenght of developing dendrites after 2 DIV with longer dendrites in the synaptophysin-knock-out-mouse. Therefore synaptophysin may have a regulatory function for exo-/ endocytosis during dendritic growth. Specific inactivation of synaptobrevin by tetanustoxin had no consequences in morphological features, synaptogenesis and growing of the hippoacampal neurons in vitro. Morphometric measurements showed no significant differences between TeNT and control. Therefore we conclude that

Published

1999

8. Der Einfluß von Botulinumneurotoxin A auf Wachstum und Differenzierung primär dissoziierter hippocampaler Zellkulturen

Author

Grosse, G., Bergmann, M., Gratzl, M., Fetter, Ingmar, Grosse, G., Bergmann, M., Gratzl, M., and Fetter, Ingmar

Abstract

Obwohl die Struktur und das Ausmaß dendritischer Verzweigungen eine wichtige Rolle bei der Informationsübertragung neuronaler Zellen spielen, ist bislang wenig über die Bausteine und Molekularmechanismen des Dendritenwachstums bekannt. Unter der Verwendung primär dissoziierter hippocampaler Zellkulturen embryonaler Mäuse untersuchte ich frühe Stadien des Zellfortsatzwachstums. Dabei konnte ich SNAP-25 (synaptosomal associated protein of 25 kDA), ein Schlüsselprotein der regulierten Exozytose, nicht nur in Axonen und terminalen Axonendigungen, sondern auch anhand von Doppelimmunmarkierungen mit den dendritischen Markern Transferrin-Rezeptor und MAP-2 in Dendriten lokalisieren. Die spezifische Inaktivierung von SNAP-25 durch Botulinumneurotoxin A (BoNT/A) führte zur Hemmung des Axonwachstums und des Vesikelrecyclings in terminalen Axonendigungen. Darüberhinaus wurde auch das Wachstum dendritischer Fortsätze von Körner- und Pyramidenzellen durch BoNT/A signifikant gehemmt. Daraus läßt sich schließen, daß SNAP-25, im Gegensatz zu Synaptobrevin, an konstitutiven Prozessen in den Axonen und Dendriten hippocampaler Neurone beteiligt ist., Structure and dimension of the dendritic arbor are important determinants of information processing by the nerve cell, but mechanisms and molecules involved in dendritic growth are essentially unknown. I investigated early mechanisms of dendritic growth using mouse fetal hippocampal neurons in primary culture, which form processes during the first week in vitro. I detected a key component of regulated exocytosis, SNAP-25 (synaptosomal associated protein of 25 kDa)., in axons and axonal terminals as well as in dendrites identified by the occurrence of the dendritic markers transferrin receptor and MAP2. Selective inactivation of SNAP-25 by botulinum neurotoxin A (BoNTA) resulted in inhibition of axonal growth and of vesicle recycling in axonal terminals. In addition, dendritic growth of hippocampal pyramidal and granule neurons was significantly inhibited by BoNTA. These observations indicate that SNAP-25, but not synaptobrevin, is involved in constitutive axonal growth and dendrite formation by hippocampal neurons.

Published

1999

9. Synaptosome-Associated Protein of 25 Kilodaltons in Oocytes and Steroid-Producing Cells of Rat and Human Ovary: Molecular Analysis and Regulation by Gonadotropins1

Author

Grosse, J., primary, Bulling, A., additional, Brucker, C., additional, Berg, U., additional, Amsterdam, A., additional, Mayerhofer, A., additional, and Gratzl, M., additional

Published

2000

10. Different histamine pools in rat gastric enterochromaffin-like cells

Author

Prinz, C., primary, Zanner, R., additional, Galler, A., additional, Classen, M., additional, Höhne-Zell, B., additional, and Gratzl, M., additional

Published

1998

11. Chromogranin A in neurons of the rat cerebellum and spinal cord: quantification and sites of expression.

Author

Lahr, G, primary, Mayerhofer, A, additional, Bergmann, M, additional, Takiyyuddin, M A, additional, and Gratzl, M, additional

Published

1992

12. Amylase release from streptolysin O-permeabilized pancreatic acinar cells. Effects of Ca2+, guanosine 5′-[γ-thio]triphosphate, cyclic AMP, tetanus toxin and botulinum A toxin

Author

Stecher, B, primary, Ahnert-Hilger, G, additional, Weller, U, additional, Kemmer, T P, additional, and Gratzl, M, additional

Published

1992

13. Cellular distribution and amount of chromogranin A in bovine endocrine pancreas.

Author

Ehrhart, M, Jörns, A, Grube, D, and Gratzl, M

Abstract

We determined the cellular distribution and the amount of chromogranin A in endocrine cells of bovine pancreas using a polyclonal antibody against bovine adrenomedullary chromogranin A. The relative amounts of chromogranin A in the different cells of the endocrine pancreas were determined by computer-assisted analyses of the optical densities of the immunoreactivities in the stained sections. More than 80% of the immunoreactive chromogranin A was located in the pancreatic B-cells. In immunoblots of acid tissue extracts, only one chromogranin A band (MW 74 KD) was observed. Quantification of the immunoblots revealed that 3 micrograms of chromogranin A and 918 micrograms of insulin were present per gram pancreas (wet weight), equivalent to a molar ratio of 460 mumol chromogranin A per mol insulin.

Published

1988

14. Expression of the neural cell adhesion molecule NCAM in endocrine cells.

Author

Langley, O K, Aletsee-Ufrecht, M C, Grant, N J, and Gratzl, M

Abstract

We examined the expression of the neural cell adhesion molecule NCAM in a number of endocrine tissues of adult rat and in an endocrine tumor cell line. NCAM was found by immunoelectron microscopy to be present on the surface of all endocrine cells in the three lobes of the hypophysis, although staining was relatively less intense in the intermediate lobe, and in pancreatic islets. Pituicytes, hypophyseal glial cells, were also labeled for NCAM. A rat insulinoma cell line (RIN A2) also expressed NCAM as judged by immunocytochemistry. Analysis of NCAM antigenic determinants (Mr 180, 140, and 120 KD) revealed large variations in the relative proportions of NCAM polypeptides present in the different tissues. Although all tissues and cell lines expressed NCAM-140, NCAM-180 was not detected in the adenohypophysis, pancreas, or adrenal medulla, and NCAM-120 was found in none of the endocrine tissues or cell lines except at low levels in the neurohypophysis. The tumor cell line expressed significant levels of NCAM-180, which was most abundant in the neurohypophysis. These results show that NCAM expression appears to be a general property of endocrine cells, although the antigenic composition differs markedly from that in brain tissue. These data are discussed with regard to the embryological origins of the different endocrine tissues, and possible functional implications are suggested.

Published

1989

15. Chromogranin A in the pancreatic islet: cellular and subcellular distribution.

Author

Ehrhart, M, Grube, D, Bader, M F, Aunis, D, and Gratzl, M

Abstract

Chromogranin A (CGA) is the major soluble protein within secretory vesicles of chromaffin cells. A polyclonal antiserum was raised against bovine CGA and characterized in two-dimensional immunoblots. Cellular and subcellular distribution of CGA in bovine pancreatic islet was investigated by immunocytochemistry. At the light microscopic level, CGA-like immunoreactivity was found in the same cells that react with antibodies against insulin, glucagon, and somatostatin. A minority of cells containing pancreatic polypeptide also showed faint immunostaining. At the ultrastructural level (protein A-gold technique), CGA-like immunoreactivity was confined exclusively to the secretory vesicles. Whereas the hormones were localized mainly in the central part of the secretory vesicles, CGA was present predominantly in the periphery. These findings indicate that a CGA-like protein is a regular constituent of the matrix of secretory vesicles in pancreatic endocrine cells.

Published

1986

16. Characterization of hormone and protein release from alpha-toxin-permeabilized chromaffin cells in primary culture.

Author

Bader, M F, Thiersé, D, Aunis, D, Ahnert-Hilger, G, and Gratzl, M

Abstract

Addition of Staphylococcus aureus alpha-toxin to adult bovine chromaffin cells maintained in primary culture causes permeabilization of cell membrane as shown by the release of intracellular 86Rb+. The alpha-toxin does not provoke a spontaneous release of either catecholamines or chromogranin A, a protein marker of the secretory granule, showing the integrity of the secretory vesicle membrane. However the addition of micromolar free Ca2+ concentration induced the co-release of noradrenaline and chromogranin A. In alpha-toxin-treated cells, the released chromogranin A could not be sedimented and lactate dehydrogenase was still associated within cells, which provides direct evidence that secretory product is liberated by exocytosis. By contrast, permeabilization of cells with digitonin caused a Ca2+-dependent but also a Ca2+-independent release of secretory product, a dramatic loss of lactate dehydrogenase, as well as release of secretory product in a sedimentable form. Ca2+-dependent exocytosis from alpha-toxin-permeabilized cells required Mg2+-ATP and did not occur in the presence of other nucleotides. Thus alpha-toxin is a convenient tool to permeabilize chromaffin cells, and has the advantage of keeping intracellular structures, specifically the exocytotic machinery, intact.

Published

1986

17. Ca2+‐induced fusion of golgi‐derived secretory vesicles isolated from rat liver

Author

Gratzl, M. and Dahl, G.

Published

1976

18. Optimal Parameters of Silver Metal Based Air-Gap Cyanide Sensors

Author

Gratzl, M., Fligier, J., and Pungor, E.

Abstract

Analytical characteristics of air-gap cyanide sensor incorporating metallic silver as indicator electrode have been investigated as function of chemical composition, pH, buffer capacity, concentration and volume of the absorbent electrolyte film covering the indicator electrode. Simple silver nitrate electrolyte provides results equivalent to those obtained with a dicyanoargentate(l) electrolyte, but its preparation is easier. The pH of absorbing solution should be kept at pKHCN=9.3. Convenient buffer capacity can be assured by a medium concentrated (10-1M) appropriate buffer system (e.g. borax-borate). Optimal electrolyte concentration is about 10"* mol/l, while the volume of electrolyte must be of several microlitres for assuring good reproducibility. For interpretation of the results an equation correlating equilibrium activity of the acidified sample solution with that of the absorbing film has been determined, and the relationship between the e.m.f. and the pH of the film has been derived. Thus, the entire 4-phase system (sample solution, air-gap, absorbing film, potentiometric sensor) can be described as a closed equilibrium system.

Published

1986

19. Endocrine cells share expression of N-CAM with neurones

Author

Langley, O.K., Aletsee, M.C., and Gratzl, M.

Abstract

The expression of the neural cell adhesion molecule, N-CAM, was examined in the anterior lobe of rat hypophysis by immunocytochemistry at light and electron microscope levels. In addition, N-CAM antigenic determinants present in adrenal medulla, anterior hypophysis and PC12 cells were compared by immunoblotting with those found in cerebellum. All secretory cells in the anterior hypophysis were found to be N-CAM positive on their surfaces, but not all of the three polypeptide determinants typical of cerebellum were present in the endocrine tissues or cell line tested. In addition, a new N-CAM determinant of 49 kDa not present in cerebellum was found in adrenal medulla and hypophysis, although it was absent from PC12 cells. The possible implications of these data are discussed.

Published

1987

20. The light chain but not the heavy chain of botulinum A toxin inhibits exocytosis from permeabilized adrenal chromaffin cells

Author

Stecher, B., Weller, U., Habermann, E., Gratzl, M., and Ahnert-Hilger, G.

Abstract

The heavy and light chains of botulinum A toxin were separated by anion exchange chromatography. Their intracellular actions were studied using bovine adrenal chromaffin cells permeabilized with streptolysin O. Purified light chain inhibited the Ca 2+-stimulated [ 3H]noradrenaline release with a half-maximal effect at about 1.8 nM. The inhibition was incomplete. Heavy chain up to 28 nM was neither effective by itself nor did it enhance the inhibitory effect of light chain. It is concluded that the light chain of botulinum A toxin contains the functional domain responsible for the inhibition of exocytosis.

Published

1989

21. Ca 2+-induced fusion of golgi-derived secretory vesicles isolated from rat liver

Author

Gratzl, M. and Dahl, G.

Published

1976

22. Reductive chain separation of botulinum A toxin — a prerequisite to its inhibitory action on exocytosis in chromaffin cells

Author

Stecher, B., Gratzl, M., and Ahnert-Hilger, G.

Abstract

Cleavage of the disulfide bond linking the heavy and the light chains of tetanus toxin is necessary for its inhibitory action on exocytotic release of catecholamines from permeabilized chromaffin cells [(1989) FEBS Lett. 242, 245–248; (1989) J. Neurochem., in press]. The related botulinum A toxin also consists of a heavy and a light chain linked by a disulfide bond. The actions of both neurotoxins on exocytosis were presently compared using streptolysin O-permeabilized bovine adrenal chromaffin cells. Botulinum A toxin inhibited Ca2+-stimulated catecholamine release from these cells. Addition of dithiothreitol lowered the effective doses to values below 5 nM. Under the same conditions, the effective doses of tetanus toxin were decreased by a factor of five. This indicates that the interchain SS bond of botulinum A toxin must also be split before the neurotoxin can exert its effect on exocytosis.

Published

1989

23. Na+/Ca2+ exchange in coated microvesicles

Author

Saermark, T and Gratzl, M

Abstract

Coated microvesicles isolated from bovine neurohypophyses could be loaded with Ca2+ in two different ways, either by incubation in the presence of ATP or by imposition of an outwardly directed Na+ gradient. Na+, but not K+, was able to release Ca2+ accumulated by the coated microvesicles. These results suggest the existence of an ATP-dependent Ca2+-transport system as well as of a Na+/Ca2+ carrier in the membrane of coated microvesicles similar to that present in the membranes of secretory vesicles from the neurohypophysis. A kinetic analysis of transport indicates that the apparent Km for free Ca2+ of the ATP-dependent uptake was 0.8 microM. The average Vmax. was 2 nmol of Ca2+/5 min per mg of protein. The total capacity of microvesicles for Ca2+ uptake was 3.7 nmol/mg of protein. Both nifedipine (10 microM) and NH4Cl (50 mM) inhibited Ca2+ uptake. The ATPase activity in purified coated-microvesicles fractions from brain and neurohypophysis was characterized. Micromolar concentrations of Ca2+ in the presence of millimolar concentrations of Mg2+ did not change enzyme activity. Ionophores increasing the proton permeability across membranes activated the ATPase activity in preparations of coated microvesicles from brain as well as from the neurohypophysis. Thus the enzyme exhibits properties of a proton-transporting ATPase. This enzyme seems to be linked to the ion accumulation by coated microvesicles, although the precise coupling of the proton transport to Ca2+ and Na+ fluxes remains to be determined.

Published

1986

24. Minimal requirements for exocytosis. A study using PC 12 cells permeabilized with staphylococcal alpha-toxin.

Author

Ahnert-Hilger, G, Bhakdi, S, and Gratzl, M

Abstract

The membrane-permeabilizing effects of streptolysin O, staphylococcal alpha-toxin, and digitonin on cultured rat pheochromocytoma cells were studied. All three agents perturbed the plasma membrane, causing release of intracellular 86Rb+ and uptake of trypan blue. In addition, streptolysin O and digitonin also damaged the membranes of secretory vesicles, including a parallel release of dopamine. In contrast, the effects of alpha-toxin appeared to be strictly confined to the plasma membrane, and no dopamine release was observed with this agent. The exocytotic machinery, however, remained intact and could be triggered by subsequent introduction of micromolar concentrations of Ca2+ into the medium. Dopamine release was entirely Ca2+ specific and occurred independent of the presence or absence of other cations or anions including K+ glutamate, K+ acetate, or Na+ chloride. Ca2+-induced exocytosis did not require the presence of Mg2+-ATP in the medium. The process was insensitive to pH alterations in the range pH 6.6-7.2, and appeared optimal at an osmolarity of 300 mosm/kg. Toxin permeabilization seems to be an excellent method for studying the minimal requirements for exocytosis.

Published

1985

25. Characterization of the inositol 1,4,5-trisphosphate-induced calcium release from permeabilized endocrine cells and its inhibition by decavanadate and p-hydroxymercuribenzoate

Author

Föhr, K J, Scott, J, Ahnert-Hilger, G, and Gratzl, M

Abstract

The inositol 1,4,5-trisphosphate (IP3)-sensitive Ca2+ compartment of endocrine cells was studied with alpha-toxin- and digitonin-permeabilized rat insulinoma (RINA2) and rat pheochromocytoma (PC12) cells. The Ca2+ uptake was ATP-dependent, and submicromolar concentrations of IP3 specifically released the stored Ca2+. Half-maximal Ca2+ release was observed with 0.25-0.5 mumol of IP3/l, and the amount of Ca2+ released due to IP3 could be enhanced by additional loading of the Ca2+ compartment. Consecutive additions of the same concentration of IP3 for 1-2 h always released the same amount of Ca2+ without desensitization, providing an ideal basis to further characterize the IP3-induced Ca2+ release. Here we describe for the first time a reversible inhibitory effect of decavanadate on the IP3-induced Ca2+ release. Among the vanadium species tested (decavanadate, oligovanadate and monovanadate), only decavanadate was inhibitory, with a half-maximal effect at 5 mumol/l in both cell types. The effect of decavanadate could be overcome by increasing the amount of sequestered Ca2+ or added IP3. Decavanadate did not affect the ATP-driven Ca2+ uptake but oligovanadate was inhibitory on Ca2+ uptake. p-Hydroxymercuribenzoate (pHMB) at concentrations between 10 and 30 mumol/l also inhibited the Ca2+ release due to IP3. Thiol compounds such as dithiothreitol (DTT; 1 mmol/l) added before pHMB removed all its inhibitory effect on the IP3-induced Ca2+ release, whereas the inhibition caused by decavanadate was unaffected by DTT. Thus, the decavanadate-dependent inhibition functions by a distinctly different mechanism than pHMB and could serve as a specific tool to analyse various aspects of the IP3-induced Ca2+ release within endocrine cells.

Published

1989

26. Quantification of p38/synaptophysin in highly purified adrenal medullary chromaffin vesicles

Author

Schilling, K., primary and Gratzl, M., additional

Published

1988

27. Aliphatic polyesters II. The degradation of poly (DL-lactide), poly (ε-caprolactone), and their copolymers in vivo

Author

PITT, G, primary, GRATZL, M, additional, KIMMEL, G, additional, SURLES, J, additional, and SOHINDLER, A, additional

Published

1981

28. Mechanisms of endocytosis and exocytosis in rat gastric enterochromaffin-like (ECL) cells

Author

Zanner, Robert, Prinz, Chr. (apl. Prof. Dr.), Fend, F. (Univ.-Prof. Dr.), and Gratzl, M. (Univ.-Prof. Dr., Ludwig-Maximilians-Universität München)

Subjects

endocrine system, Medizin, ddc:610, Enterochromaffin-like, ECL, Amphiphysin, Dynamin, Calcium, Endozytose, Exozytose, IP3, Histamin, Magensäuresekretion, enterochromaffin-like, amphiphysin, dynamin, calcium, endocytosis, exocytosis, histamine, gastric acid secretion

Abstract

Enterochromaffin-like (ECL) Zellen sind neuroendokrine Zellen der Magenschleimhaut, die eine wichtige Rolle bei der peripheren Regulation der Magensäureproduktion spielen. Nach Stimulation mit Gastrin kommt es zur calciumabhängigen Freisetzung von Histamin, das in Parietalzellen die Synthese und Sekretion von Magensäure auslöst. In vorliegender Arbeit wurden Bedeutung und Entstehung des Calciumsignals für die gastrininduzierte Histaminsekretion sowie Expression der Endozytoseproteine Amphiphysin und Dynamin untersucht. Für die Erhöhung von [Ca2+]i war die Aktivierung von InsP3-Rezeptoren, nicht jedoch die Entleerung intrazellulärer Calciumspeicher nötig. Der für die Exozytose notwendige Calciumeinstrom konnte durch Nimodipin gehemmt werden, was eine Beteilung spannungsgesteuerter L-Typ Calciumkanäle nahe legt. Alle Dynamin- und Amphiphysin-Isoformen konnten auf mRNA- und Proteinebene nachgewiesen werden. Eine neue Splice-Variante von Amphiphysin-2 wurde ebenfalls entdeckt. Enterochromaffin-like (ECL) cells are neuroendocrine cells of the gastric mucosa that are important for the peripheral regulation of gastric acid secretion. Following stimulation with gastrin, histamine is released from ECL cells in a calcium-dependent manner, inducing synthesis and secretion of gastric acid in parietal cells. In this thesis, importance and generation of the calcium signal necessary for gastrin-induced histamine secretion were investigated, as well as the expression of the endocytic proteins amphiphysin and dynamin. Activation of InsP3 receports but not calcium release from intracellular stores was nessecary for the increase in [Ca2+]i. Calcium influx could be inhibited by nimodipine, indicating involvement of voltage-activated L-type calcium channels. All known dynamin and amphiphysin isoforms could be detected on mRNA and protein levels. Furthermore, a novel splice form of amphiphysin-2 was found to be expressed in ECL cells.

Published

2005

29. GABAergic system in Leydig cells and stimulation of cell proliferation by GABA

Author

Geigerseder, Christof, Ring, J. (Univ.-Prof. Dr. Dr.), Mayerhofer, A. (Univ.-Prof. Dr.), and Gratzl, M. (Univ.-Prof. Dr. , Ludwig-Maximilians-Universität München)

Subjects

endocrine system, nervous system, Medizin, ddc:610, infertility, GABA, neurotransmitter, GAD, VGAT, testis, Leydig cell, Leydig, GABA receptors, testosterone, Infertilität, Neurotransmitter, Hoden, Leydigzellen, GABA-Rezeptoren, Testosteron

Abstract

Im Rahmen dieser Arbeit wurde das den Neurotransmitter GABA synthetisierende Enzym GAD, der vesikuläre GABA-Transporter VGAT und GABA-Rezeptoren im Hoden von Nagern und Menschen nachgewiesen. Sowohl die Quelle von GABA, als auch GABA-Rezeptoren wurden in endokrinen Zellen des Hodens, den Testosteron bildenden Leydigzellen, lokalisiert. Weiterhin zeigten zellbiologische Untersuchungen, dass die etablierte Leydigzelllinie TM3 enzymatisch aktives GAD besitzt und auf GABAerge Stimulation mit einem Anstieg ihrer Zellproliferation reagiert. Die pharmakologische Charakterisierung der Proliferationswirkung ergab eine Übertragung durch GABA-A-Rezeptoren. Außerdem wurden die Gene c-fos und hsf-1 durch einen cDNA-Array als Bestandteile des Signaltransduktionswegs der GABA-A-Rezeptor vermittelten Wirkung nachgewiesen. Leydigzellen verfügen demnach über ein GABAerges System, wobei GABA auto- bzw. parakrin durch GABA-A-Rezeptoren die Proliferation von Leydigzellen reguliert. In context of this work the GABA synthesizing enzyme GAD, the vesicular GABA transporter VGAT and GABA receptors were identified in rodent and human testis. GABAergic sources, as well as GABA receptors were localized in testosteron producing Leydig cells in the endocrine compartment of the testis. Furthermore cell biological studies showed that the established Leydig cell line TM3 exhibits enzymatically active GAD and that GABAergic stimulation of TM3 cells leads to increased cell proliferation. Pharmacological characterization of this proliferative action of GABA revealed an GABA-A receptor mediated mechanism. Moreover the genes c-fos and hsf-1 were identified by c-DNA-array experiments to be components of the GABA-A receptor mediated signal transduction cascade. In conclusion Leydig cells posses a GABAergic system, whereby GABA regulates Leydig cell proliferation via GABA-A receptors in an auto- or paracrine manner.

Published

2005

30. Einfluß der synaptischen Vesikelproteine Synaptophysin und Synaptobrevin auf Wachstum und Differenzierung der hippocampalen Zellkultur

Author

Gorsleben, Martin, Grosse, G., Gratzl, M., and Schulze, W.

Subjects

WW 2480, tetanustoxin, synaptophysin, 610 Medizin, synaptobrevin, ddc:610, 33 Medizin, hippocampale Zellkultur, hippocampal cell culture

Abstract

Ziel der vorliegenden Arbeit war es, die Rolle der synaptischen Vesikelproteine Synaptophysin und Synaptobrevin bei Wachstum und Differenzierung der primär dissoziierten hippocampalen Zellkultur 17 Tage alter Mäuseembryonen zu untersuchen. Besonderes Interesse galt dabei dem Fortsatzwachstum und der Synaptogenese. Durch Beobachtung von Zellmorphologie und Zellwachstum wurde gezeigt, daß die Ausbildung charakteristischer Zelltypen ein intrinsischer Prozeß der hippocampalen Neurone ist. Die Synaptogenese wurde durch die Darstellung der entwicklungsabhängigen Verteilung der synaptischen Vesikelproteine Synaptophysin und Synaptobrevin mittels Immunfluoreszenzmarkierung dokumentiert. Durch elektronenmikroskopische Aufnahmen wurde die Differenzierung subzellulärer Strukturen der hippocampalen Zellkultur charakterisiert und die Verteilung von Synaptophysin und Synaptobrevin entwicklungsabhängig dargestellt. Synaptophysin fand sich nicht nur in axonalen Präsynapsen, sondern auch in Dendriten. Synaptobrevin war im Gegensatz zu Synaptophysin nicht in allen synaptischen Vesikeln der Axonterminalen darstellbar. Um die Wirkungen von Synaptophysin und Synaptobrevin auf hippocampale Neurone in der Kultur genauer zu untersuchen, standen zwei Versuchsmodelle zur Verfügung: 1. die Synaptophysin-defiziente Maus und 2. das clostridiale Neurotoxin Tetanustoxin (TeNT), das Synaptobrevin spezifisch spaltet. Anhand der Depletion von Synaptophysin wurde untersucht, ob in vitro das Fehlen des Proteins Konsequenzen in Bezug auf Synapsenbildung und morphologisches Erscheinungsbild der Neurone hat. Es konnten lichtmikroskopisch und auch im elektronenmikroskopischen Bild keine Unterschiede zu Kontrollkulturen festgestellt werden. Durch morphometrische Messungen zeigte sich, daß in der Kultur der Synaptophysin-depletierten Maus nach 2 DIV mit hoher Signifikanz die Dendriten länger als in Kontrollkulturen waren. Dies spricht für regulatorische Funktionen des Proteins bei Exo- und Endozytosevorgängen während des dendritischen Wachstums. Nach Zugabe von Tetanustoxin zur pränatalen Zellkultur konnte gezeigt werden, daß die Inaktivierung von Synaptobrevin durch TeNT in vitro keine Konsequenzen in Bezug auf das morphologische Erscheinungsbild der Neurone, die Synapsenbildung und das Wachstumsverhalten hat. Mit morphometrischen Messungen konnten für TeTx-behandelte Neurone keine hochsignifikanten Unterschiede zu Kontrollkulturen festgestellt werden. Synaptobrevin scheint also sowohl beim Axon- als auch beim Dendritenwachstum keine essentielle Rolle zu spielen., Goal of this work was to investigate the role of the synaptic vesicle proteins synaptophysin and synaptobrevin during development and differentiation of mouse fetal hippocampal neurons in primary culture. The outgrowth of dendritic and axonal fibers and the mechanisms of synaptogenesis were of special interest. Observation of morphology and development showed that generation of characteristic cell types is an intrinsic process of hippocampal neurons. Differentiation of cellular and subcellular structures in hippocampal cell culture, characteristics of synaptogenesis and the stage-dependent distribution of synaptophysin and synaptobrevin were demonstrated by immunofluorescence and electron microscopy. Synaptophysin was localized in presynaptic axon terminals but also in dendrites. In contrast with synaptophysin immunoreaction for synaptobrevin could not be found in all synaptic vesicles of the presynaptic axon terminal. To investigate the influence of synaptophysin and synaptobrevin on hippocampal neurons in culture two experimental models were used, first a synaptophysin-knock-out-mouse and second the clostridial neurotoxin tetanustoxin (TeNT) which selectively cleaves synaptobrevin. With the depletion of synaptophysin we investigated if there are consequences in development of synapses and morphological features of the neurons in vitro. In both, light and electron microscopy, there was no difference to control cultures. In morphometric measurements there was a significant difference in the lenght of developing dendrites after 2 DIV with longer dendrites in the synaptophysin-knock-out-mouse. Therefore synaptophysin may have a regulatory function for exo-/ endocytosis during dendritic growth. Specific inactivation of synaptobrevin by tetanustoxin had no consequences in morphological features, synaptogenesis and growing of the hippoacampal neurons in vitro. Morphometric measurements showed no significant differences between TeNT and control. Therefore we conclude that synaptobrevin has no essential function during axon growth or dendrite elongation.

Published

1999

31. Functional Imaging of Chemically Active Surfaces with Optical Reporter Microbeads.

Author

Ahuja P, Nair S, Narayan S, and Gratzl M

Subjects

Color, Diffusion, Equipment Design, Hydrogen-Ion Concentration, Membranes, Artificial, Microspheres, Porosity, Surface Properties, Agar chemistry, Hydrogel, Polyethylene Glycol Dimethacrylate chemistry, Microscopy instrumentation

Abstract

We have developed a novel approach to allow for continuous imaging of concentration fields that evolve at surfaces due to release, uptake, and mass transport of molecules, without significant interference of the concentration fields by the chemical imaging itself. The technique utilizes optical "reporter" microbeads immobilized in a thin layer of transparent and inert hydrogel on top of the surface. The hydrogel has minimal density and therefore diffusion in and across it is like in water. Imaging the immobilized microbeads over time provides quantitative concentration measurements at each location where an optical reporter resides. Using image analysis in post-processing these spatially discrete measurements can be transformed into contiguous maps of the dynamic concentration field across the entire surface. If the microbeads are small enough relative to the dimensions of the region of interest and sparsely applied then chemical imaging will not noticeably affect the evolution of concentration fields. In this work colorimetric optode microbeads a few micrometers in diameter were used to image surface concentration distributions on the millimeter scale.

Published

2015

32. Computational modeling and analysis of iron release from macrophages.

Author

Potdar AA, Sarkar J, Das NK, Ghosh P, Gratzl M, Fox PL, and Saidel GM

Subjects

Computational Biology, Humans, Intracellular Space metabolism, Macrophages cytology, Computer Simulation, Homeostasis physiology, Iron metabolism, Macrophages metabolism, Models, Biological

Abstract

A major process of iron homeostasis in whole-body iron metabolism is the release of iron from the macrophages of the reticuloendothelial system. Macrophages recognize and phagocytose senescent or damaged erythrocytes. Then, they process the heme iron, which is returned to the circulation for reutilization by red blood cell precursors during erythropoiesis. The amount of iron released, compared to the amount shunted for storage as ferritin, is greater during iron deficiency. A currently accepted model of iron release assumes a passive-gradient with free diffusion of intracellular labile iron (Fe2+) through ferroportin (FPN), the transporter on the plasma membrane. Outside the cell, a multi-copper ferroxidase, ceruloplasmin (Cp), oxidizes ferrous to ferric ion. Apo-transferrin (Tf), the primary carrier of soluble iron in the plasma, binds ferric ion to form mono-ferric and di-ferric transferrin. According to the passive-gradient model, the removal of ferrous ion from the site of release sustains the gradient that maintains the iron release. Subcellular localization of FPN, however, indicates that the role of FPN may be more complex. By experiments and mathematical modeling, we have investigated the detailed mechanism of iron release from macrophages focusing on the roles of the Cp, FPN and apo-Tf. The passive-gradient model is quantitatively analyzed using a mathematical model for the first time. A comparison of experimental data with model simulations shows that the passive-gradient model cannot explain macrophage iron release. However, a facilitated-transport model associated with FPN can explain the iron release mechanism. According to the facilitated-transport model, intracellular FPN carries labile iron to the macrophage membrane. Extracellular Cp accelerates the oxidation of ferrous ion bound to FPN. Apo-Tf in the extracellular environment binds to the oxidized ferrous ion, completing the release process. Facilitated-transport model can correctly predict cellular iron efflux and is essential for physiologically relevant whole-body model of iron metabolism.

Published

2014

33. Differential linear scan voltammetry: analytical performance in comparison with pulsed voltammetry techniques.

Author

Sheth DB and Gratzl M

Subjects

Carbon, Carbon Fiber, Electrochemical Techniques instrumentation, Equipment Design, Gold, Microelectrodes, Sensitivity and Specificity, Electrochemical Techniques methods, Oxygen analysis

Abstract

We report here on differential linear scan voltammetry, DLSV, that combines the working principles of linear scan voltammetry, LSV, and the numerous existing pulsed voltammetry techniques. DLSV preserves the information from continuous interrogation in voltage and high accuracy that LSV provides about electrochemical processes, and the much better sensitivity of differential pulsed techniques. DLSV also minimizes the background current compared to both LSV and pulsed voltammetry. An early version of DLSV, derivative stationary electrode polarography, DSEP, had been proposed in the 1960s but soon abandoned in favor of the emerging differential pulsed techniques. Relative to DSEP, DLSV takes advantage of the flexibility of discrete smoothing differentiation that was not available to early investigators. Also, DSEP had been explored in pure solutions and with reversible electrochemical reactions. DLSV is tested in this work in more challenging experimental contexts: the measurement of oxygen with a carbon fiber microelectrode in buffer, and with a gold microdisc electrode exposed to a live biological preparation. This work compares the analytical performance of DLSV and square wave voltammetry, the most popular pulsed voltammetry technique.

Published

2013

34. Temporal ratiometry to assess dynamic concentration distributions of fluorescent molecules in single live cells during continuous diffusional dosing.

Author

Oruganti P and Gratzl M

Subjects

Animals, Cell Line, Cell Line, Tumor, Diffusion, Humans, Image Processing, Computer-Assisted, Kidney cytology, Rats, Cytoplasm metabolism, Epithelial Cells cytology, Isoquinolines analysis, Microscopy, Fluorescence methods, Myocytes, Smooth Muscle cytology

Abstract

The introduction of specific molecules into live cells is a widely used approach to probe cellular mechanisms. Recently, we have reported on the sustained dosing of molecules into single cells via a microscopic diffusion port. Here we describe temporal ratiometry, a method to reconstruct intracellular concentration distribution of the delivered molecules as it varies in time during dosing. To characterize this method, we analyzed fluorescence intensity maps obtained during delivery of Lucifer Yellow CH, LY, a polar fluorophore into A7r5 vascular smooth muscle cells, normal rat kidney epithelial cells (NRKE), and MCF-7 human breast cancer cells. Temporal ratiometry indicates a linear increase in concentration of LY in these cells with a nearly uniform distribution during 20 min of delivery. The method cancels the effects of varying cell height and variable accessible volume on the measured intensities at different locations within the cell. Temporal ratiometry will be useful to estimate dynamic changes in intracellular concentration distributions and thus, facilitate the understanding of transport, binding, sequestration, and efflux of molecules introduced into cells.

Published

2009

35. Successful antiangiogenic combination therapy for pseudomyxoma peritonei with bevacizumab and capecitabine.

Author

Sun WL, Hutarew G, Gradl J, Gratzl M, Denz H, and Fiegl M

Subjects

Adenoma, Villous complications, Adenoma, Villous drug therapy, Adenoma, Villous metabolism, Adenoma, Villous surgery, Angiogenesis Inhibitors administration & dosage, Antibodies, Monoclonal administration & dosage, Antibodies, Monoclonal, Humanized, Antineoplastic Combined Chemotherapy Protocols administration & dosage, Antineoplastic Combined Chemotherapy Protocols adverse effects, Appendiceal Neoplasms surgery, Bevacizumab, Capecitabine, Combined Modality Therapy, Deoxycytidine administration & dosage, Deoxycytidine analogs & derivatives, Disease Progression, Fluorouracil administration & dosage, Fluorouracil adverse effects, Fluorouracil analogs & derivatives, Hernia, Inguinal complications, Hernia, Inguinal surgery, Humans, Ileocecal Valve surgery, Leucovorin administration & dosage, Leucovorin adverse effects, Male, Middle Aged, Organoplatinum Compounds administration & dosage, Organoplatinum Compounds adverse effects, Peritoneal Neoplasms blood supply, Peritoneal Neoplasms drug therapy, Peritoneal Neoplasms etiology, Peritoneal Neoplasms metabolism, Peritoneal Neoplasms surgery, Pseudomyxoma Peritonei etiology, Pseudomyxoma Peritonei surgery, Treatment Outcome, Adenoma, Villous secondary, Angiogenesis Inhibitors therapeutic use, Antineoplastic Combined Chemotherapy Protocols therapeutic use, Appendiceal Neoplasms complications, Peritoneal Neoplasms secondary, Pseudomyxoma Peritonei drug therapy

Abstract

Effective systemic therapy for advanced pseudomyxoma peritonei (PMP) is the focus of investigation. We describe a case of PMP arising from an adenoma of the appendix in a 58-year-old man. First, the patient underwent explorative laparotomy with ileocoecal resection, but without possibility of major tumor debulking due to adhesive gross tumor masses. Subsequently, six cycles of Folfox IV chemotherapy were administered, without response, but with severe side effects. Upon progressive disease, a combination of bevacizumab and capecitabine led to a long term stabilization of disease and obvious improvement of performance status. Our case suggests that modulation of tumor microenvironment and angiogenesis by bevacizumab, potentially augmented by moochemotherapy, may be beneficial in borderline tumors such as PMP.

Published

2009

36. Determination of critical micelle concentration with the rotating sample system.

Author

Kao LT, Shetty GN, and Gratzl M

Subjects

Electrochemistry methods, Octoxynol, Rotation, Micelles, Rheology methods, Surface-Active Agents chemistry

Abstract

A novel experimental approach using the rotating sample system (RSS) is proposed here for the determination of the critical micelle concentration (CMC) of surfactants. The RSS has been conceived in our laboratory as a convection platform for physicochemical studies and analyses in microliter-sized sample drops. The scheme allows for vigorous rotation of the drop despite its small size through efficient air-liquid mechanical coupling. Thus, changes in surface properties of aqueous samples result in corresponding modulation of the hydrodynamic performance of the RSS, which can be utilized to investigate interfacial phenomena. In this work, we demonstrate that the RSS can be used to study the effects of surfactants on the surface and in the bulk of very small samples with hydrodynamic electrochemistry. Potassium ferrocyanide is employed here with cyclic voltammetry to probe the air-water interface of solutions containing Triton X-100. The CMC of this surfactant determined using this approach is 140 ppm, which agrees well with reported values obtained with conventional methods in much larger samples. The results also demonstrate that besides the CMC, variations in bulk rheological properties can also be investigated in very small specimens using the RSS with a simple method.

Published

2008

37. Controlled diffusion for laboratory solution preparation.

Author

Yoshida M, Tohda K, and Gratzl M

Subjects

Calibration, Diffusion, Solutions analysis, Solutions chemistry

Abstract

We report here on a method for preparation of precise laboratory solutions using controlled diffusion for dosing. The desired chemical is delivered into the target solution from a stock solution through a mass-transport-limiting delivery port that blocks convection but allows reproducible diffusive transport. Solution making with this approach involves a single step irrespective of how low the desired concentration is. Diffusional delivery of chemicals involves no appreciable movement of water and, thus, no addition of volume. The approach is therefore particularly suitable for standard addition. Precise solutions of usual laboratory volumes can be made within a short time period with proper design of the delivery port or ports. Comparison with the performance of conventional methods of routine solution preparation shows that better precision can be achieved with less labor using this approach.

Published

2008

38. Enterochromaffin cells of the human gut: sensors for spices and odorants.

Author

Braun T, Voland P, Kunz L, Prinz C, and Gratzl M

Subjects

Aniline Compounds, Calcium metabolism, Cells, Cultured, Fluorescent Dyes, Gastrointestinal Motility physiology, Gastrointestinal Tract cytology, Gene Expression Regulation physiology, Humans, Receptors, Odorant genetics, Serotonin metabolism, Xanthenes, Enterochromaffin Cells physiology, Gastrointestinal Tract physiology, Odorants, Receptors, Odorant metabolism, Spices

Abstract

Background & Aims: Release of serotonin from mucosal enterochromaffin cells triggered by luminal substances is the key event in the regulation of gut motility and secretion. We were interested to know whether nasal olfactory receptors are also expressed in the human gut mucosa by enterochromaffin cells and whether their ligands and odorants present in spices, fragrances, detergents, and cosmetics cause serotonin release., Methods: Receptor expression was studied by the reverse-transcription polymerase chain reaction method in human mucosal enterochromaffin cells isolated by laser microdissection and in a cell line derived from human enterochromaffin cells. Activation of the cells by odorants was investigated by digital fluorescence imaging using the fluorescent Ca(2+) indicator Fluo-4. Serotonin release was measured in culture supernatants by a serotonin enzyme immunoassay and amperometry using carbon fiber microelectrodes placed on single cells., Results: We found expression of 4 olfactory receptors in microdissected human mucosal enterochromaffin cells and in a cell line derived from human enterochromaffin cells. Ca(2+) imaging studies revealed that odorant ligands of the identified olfactory receptors cause Ca(2+) influx, elevation of intracellular free Ca(2+) levels, and, consequently, serotonin release., Conclusions: Our results show that odorants present in the luminal environment of the gut may stimulate serotonin release via olfactory receptors present in human enterochromaffin cells. Serotonin controls both gut motility and secretion and is implicated in pathologic conditions such as vomiting, diarrhea, and irritable bowel syndrome. Thus, olfactory receptors are potential novel targets for the treatment of gastrointestinal diseases and motility disorders.

Published

2007

39. Micro-miniature autonomous optical sensor array for monitoring ions and metabolites 2: color responses to pH, K+ and glucose.

Author

Tohda K and Gratzl M

Subjects

Cellulose chemistry, Cellulose metabolism, Glucose Oxidase chemistry, Hydrogen-Ion Concentration, Ions chemistry, Optics and Photonics, Sensitivity and Specificity, Biosensing Techniques methods, Cellulose analogs & derivatives, Glucose chemistry, Potassium chemistry

Abstract

In Part 1 of this series (Anal. Sci., 2006, 22, 383), design, fabrication, and optical data acquisition of an array of tiny color changing capsules embedded in a cellulose acetate bar, called the "sliver sensor", have been described. Capsule colors are read by a CCD camera and translated into blue, red and green Kubelka-Munk variables for quantitative analysis. The respective concentrations are determined using prior calibration. The approach may be adapted to different non-biological analytical problems, as well as in vitro and in vivo applications. To demonstrate this adaptability to potential in vivo use as an example, sensitivity for each target ion was tuned to cover the respective interstitial levels by varying the relative amount of ionophore used in the corresponding microscopic beads. After optimizing the ratio of glucose oxidase (GOX)-containing beads relative to the coupled pH sensing beads and their composition, reversible color response to glucose was obtained in the entire clinically relevant glucose concentration range (10 to 600 mg/dL, 0.55 to 33 mM). Decoupling of pH and glucose sensing from possible variations in interstitial sodium level and buffer capacity is currently being optimized for future in vivo use. In vitro and non-biological applications are also being explored.

Published

2006

40. Micro-miniature autonomous optical sensor array for monitoring ions and metabolites 1: design, fabrication, and data analysis.

Author

Tohda K and Gratzl M

Subjects

Biosensing Techniques instrumentation, Borates chemistry, Cellulose analogs & derivatives, Cellulose chemistry, Crown Ethers chemistry, Decanoic Acids chemistry, Glucose chemistry, Glucose Oxidase chemistry, Hydrogen-Ion Concentration, Ionophores chemistry, Microarray Analysis instrumentation, Polyvinyl Chloride chemistry, Potassium analysis, Silver chemistry, Biosensing Techniques methods, Blood Glucose analysis, Electrolytes analysis, Microarray Analysis methods

Abstract

A micro-miniature array of sensing capsules for optical monitoring of pH, potassium and glucose is described. Optode technology translates the respective ionic levels into variable colors of ionophore/dye/polymeric liquid micro-beads stuffed into individual capsules. Glucose is monitored indirectly, by coupling through glucose oxidase (GOX) immobilized in cellulose acetate phthalate (CAP) based microscopic beads that are stuffed into another microcapsule together with pH sensitive optical microscopic beads. The electrolyte and glucose sensing capsules are embedded in a transparent cellulose acetate bar 300-500 microm wide and 2-2.5 mm long called the sliver sensor that includes also a white capsule made of micro-beads without dye for optical reference. By adding further capsules custom combinations of analytes can be monitored in biomedical and non-biological contexts. In this work, as an example, design, fabrication and testing of a sliver sensor that could be developed for in vivo use are described.

Published

2006

41. Hydrodynamic electrochemistry in 20 microL drops in the rotating sample system.

Author

Shetty GN, Syed N, Tohda K, and Gratzl M

Subjects

Electrochemistry, Microfluidic Analytical Techniques methods, Rotation, Trace Elements blood, Lead analysis, Microfluidic Analytical Techniques instrumentation, Water chemistry

Abstract

The Rotating Sample System (RSS) has been conceived in the authors' laboratory as a convection platform for microliter-sized solution volumes. Convection is achieved by rotating a small drop of sample on a stationary substrate by humidified gas jets directed tangentially at the drop base with the working electrode and a liquid junction embedded in it. Simplicity and portability of the device, and substrates complete with microfabricated electrode and junction made potentially disposable, are further competitive advantages with respect to competing, conventional analytical systems. In this work the RSS' performance with variation of system parameters such as the position and size of gas jets used for sample rotation, and position of the working electrode in the substrate are studied. Trace levels of Pb could be detected with this system and is reported here.

Published

2005

42. An Intrinsic gamma-aminobutyric acid (GABA)ergic system in the adrenal cortex: findings from human and rat adrenal glands and the NCI-H295R cell line.

Author

Metzeler K, Agoston A, and Gratzl M

Subjects

Adrenal Cortex chemistry, Alternative Splicing, Animals, Baclofen pharmacology, Calcium Channels, T-Type physiology, Carrier Proteins analysis, Carrier Proteins genetics, Carrier Proteins metabolism, Cell Line, Electric Conductivity, GABA Agonists pharmacology, GABA Plasma Membrane Transport Proteins, Gene Expression, Glutamate Decarboxylase analysis, Glutamate Decarboxylase genetics, Glutamate Decarboxylase metabolism, Glutamic Acid metabolism, Humans, Immunohistochemistry, Isoenzymes analysis, Isoenzymes genetics, Isoenzymes metabolism, Membrane Proteins analysis, Membrane Proteins genetics, Membrane Proteins metabolism, Patch-Clamp Techniques, Rats, Receptors, GABA-B analysis, Receptors, GABA-B genetics, Receptors, GABA-B physiology, Reverse Transcriptase Polymerase Chain Reaction, gamma-Aminobutyric Acid physiology, Adrenal Cortex metabolism, Membrane Transport Proteins, Organic Anion Transporters, gamma-Aminobutyric Acid biosynthesis

Abstract

gamma-Aminobutyric acid (GABA), a major neurotransmitter in the central nervous system, also acts as a paracrine or autocrine signaling molecule in endocrine tissues such as the pancreatic islets, adenohypophysis, and testis. In the present study, we describe local GABA production and functional GABA(B) receptors in the adrenal cortex, possibly forming an auto- or paracrine GABAergic system. Using immunohistochemistry and RT-PCR, we localized the GABA-synthesizing enzyme glutamate decarboxylase 67 and the vesicular GABA transporter in steroid-producing cells of the human and rat adrenal cortex. Immunocytochemistry, Western blots, and RT-PCR experiments demonstrated the presence of glutamate decarboxylase 67 in the human adrenocortical cell line NCI-H295R. Measurements of glutamate decarboxylase activity confirmed that, in these cells and in rat adrenals, glutamate is decarboxylated to form GABA. In addition, we found expression of the GABA(B(1a)), GABA(B(1e)), and GABA(B(2)) subunits of the heterodimeric GABA(B) receptor in NCI-H295R cells as shown by RT-PCR. GABA(B(1a)) and its truncated splice variant GABA(B(1e)) were also found in human and rat adrenal glands. Immunostaining for the GABA(B(2)) subunit revealed its presence in the human and rat adrenal cortex and in NCI-H295R cells. The GABA(B) receptors we identified were functional because the GABA(B) agonist baclofen inhibited T-type Ca(2+) currents in whole-cell patch clamp experiments on NCI-H295R cells. This effect was blocked by pertussis toxin. Furthermore, the alpha(2)-, alpha(3)-, beta(2)-, beta(3)- gamma(2)-, and epsilon-subunits of the GABA(A) receptor were detected in this cell line by RT-PCR. Hence, we conclude that GABA is synthesized and stored by steroid-producing cells of the adrenal cortex and may influence these cells in a paracrine or autocrine manner.

Published

2004

43. Expression of the endocytic proteins dynamin and amphiphysin in rat gastric enterochromaffin-like cells.

Author

Zanner R, Gratzl M, and Prinz C

Subjects

Animals, Cell Membrane metabolism, Cell Separation, Cells, Cultured, Cytoplasm metabolism, Dynamin I genetics, Dynamin I metabolism, Dynamin II genetics, Dynamin II metabolism, Dynamin III genetics, Dynamin III metabolism, Dynamins genetics, Enterochromaffin-like Cells ultrastructure, Nerve Tissue Proteins genetics, Protein Binding, Protein Isoforms genetics, Protein Isoforms metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Rats, Dynamins metabolism, Enterochromaffin-like Cells metabolism, Gene Expression Profiling, Nerve Tissue Proteins metabolism

Abstract

Dynamin and amphiphysin play crucial roles in a variety of endocytic processes. Previous investigations of expression and functions of these proteins were performed mostly on neurons. The aim of this study was to investigate the presence and interaction of dyn and amph in gastric enterochromaffin-like cells. These endocrine cells of the gastric mucosa play a pivotal role in the regulation of acid secretion. Exocytosis of histamine-containing secretory vesicles has been described in detail. However, the mechanisms of endocytosis are unknown in this neuroendocrine cell type. Using RT-PCR and western blotting, we detected dynamin-1, -2 and -3 in highly enriched isolated enterochromaffin-like cells. Dynamin-1 and -2 were expressed at similar high levels, whereas dynamin-3 was of low abundance. Immunofluorescence microscopy located dynamin-1 and -2 to the cytoplasm and cell surface, whereas dynamin-3 was distributed differently in the perinuclear area. The presence of amphiphysin-1 and -2 RNAs was revealed by RT-PCR and a new splice variant of amphiphysin-2 was detected. Amphiphysin-1 and -2 were also detected in enterochromaffin-like cells by immunohistochemistry in the same locations as dynamin-1 and -2. Amphiphysin-1 and dynamin-1 co-immunoprecipitated with amphiphysin-2. In addition, dynamin-1 and amphiphysin-2 partially colocalized at the plasma membrane. Our results confirm the interaction of dynamin and amphiphysin and imply a role in endocytosis in enterochromaffin-like cells. To our knowledge, this is the first demonstration of the co-expression of all three dynamin isoforms in a non-tumor cell.

Published

2004

44. Molecular and physiological evidence for functional gamma-aminobutyric acid (GABA)-C receptors in growth hormone-secreting cells.

Author

Gamel-Didelon K, Kunz L, Fohr KJ, Gratzl M, and Mayerhofer A

Subjects

Animals, Base Sequence, Calcium metabolism, Cell Line, DNA Primers, Immunohistochemistry, Patch-Clamp Techniques, Pituitary Gland cytology, Rats, Rats, Sprague-Dawley, Receptors, GABA metabolism, Growth Hormone metabolism, Pituitary Gland metabolism, Receptors, GABA physiology

Abstract

The neurotransmitter gamma-aminobutyric acid (GABA), released by hypothalamic neurons as well as by growth hormone- (GH) and adrenocorticotropin-producing cells, is a regulator of pituitary endocrine functions. Different classes of GABA receptors may be involved. In this study, we report that GH cells, isolated by laser microdissection from rat pituitary slices, possess the GABA-C receptor subunit rho2. We also demonstrate that in the GH adenoma cell line, GH3, GABA-C receptor subunits are not only expressed but also form functional channels. GABA-induced Cl- currents were recorded using the whole cell patch clamp technique; these currents were insensitive to bicuculline (a GABA-A antagonist) but could be induced by the GABA-C agonist cis-4-aminocrotonic acid. In contrast to typical GABA-C mediated currents in neurons, they quickly desensitized. Ca2+i recordings were also performed on GH3 cells. The application of either GABA or cis-4-aminocrotonic acid led to Ca2+ transients of similar amplitude, indicating that the activation of GABA-C receptors in GH3 cells may cause membrane depolarization, opening of voltage-gated Ca2+ channels, and a subsequent Ca2+ influx. Our results point at a role for GABA in pituitary GH cells and disclose an additional pathway to the one known via GABA-B receptors.

Published

2003

45. Expression of histidine decarboxylase and synthesis of histamine by human small cell lung carcinoma.

Author

Graff L, Frungieri M, Zanner R, Pohlinger A, Prinz C, and Gratzl M

Subjects

Adult, Aged, Aged, 80 and over, Carcinoma, Small Cell metabolism, Dose-Response Relationship, Drug, Female, Histidine pharmacology, Humans, Immunoblotting, Immunohistochemistry, Lung Neoplasms metabolism, Male, Middle Aged, Time Factors, Tumor Cells, Cultured drug effects, Tumor Cells, Cultured metabolism, Carcinoma, Small Cell pathology, Histamine biosynthesis, Histidine Decarboxylase biosynthesis, Lung Neoplasms pathology

Abstract

We recently found that human small cell lung carcinomas (SCLCs) express, in addition to other neuroendocrine markers, vesicular monoamine transporters. Our present results indicate that SCLCs are histaminergic. We detected the biosynthetic enzyme histidine decarboxylase by immunohistochemistry in paraffin sections of 12 biopsies of SCLC tumors. This finding was supported by immunoblotting and reverse transcription-polymerase chain reaction experiments using established SCLC cell lines, frozen and paraffin-embedded SCLC tumors. Moreover, we found histamine to be synthesized, stored, and released by cultured SCLC cells. Our novel observations may be useful for developing new diagnostic tools for this frequent and highly malignant tumor.

Published

2002

46. Intracellular signal transduction during gastrin-induced histamine secretion in rat gastric ECL cells.

Author

Zanner R, Hapfelmeier G, Gratzl M, and Prinz C

Subjects

Animals, Calcium metabolism, Calcium Channel Blockers pharmacology, Calcium Channels metabolism, Cell Membrane metabolism, Cells, Cultured, Female, Fluorescent Dyes, Fura-2, Histamine Release drug effects, Inositol 1,4,5-Trisphosphate physiology, Inositol 1,4,5-Trisphosphate Receptors, Rats, Rats, Sprague-Dawley, Receptors, Cytoplasmic and Nuclear metabolism, Stomach cytology, Enterochromaffin Cells physiology, Gastrins pharmacology, Histamine Release physiology, Intracellular Membranes physiology, Signal Transduction physiology, Stomach physiology

Abstract

Activation of G(q) protein-coupled receptors usually causes a biphasic increase in intracellular calcium concentration ([Ca(2+)](i)) that is crucial for secretion in nonexcitable cells. In gastric enterochromaffin-like (ECL) cells, stimulation with gastrin leads to a prompt biphasic calcium response followed by histamine secretion. This study investigates the underlying signaling events in this neuroendocrine cell type. In ECL cells, RT-PCR suggested the presence of inositol 1,4,5-trisphosphate receptor (IP(3)R) subtypes 1-3. The IP(3)R antagonist 2-aminoethoxydiphenyl borate abolished both gastrin-induced elevation of [Ca(2+)](i) and histamine release. Thapsigargin increased [Ca(2+)](i), however, without inducing histamine secretion. In thapsigargin-pretreated cells, gastrin increased [Ca(2+)](i) through calcium influx across the plasma membrane. Both nimodipine and SKF-96365 inhibited gastrin-induced histamine release. The protein kinase C (PKC) activator phorbol 12-myristate 13-acetate induced histamine secretion, an effect that was prevented by nimodipine. In summary, gastrin-stimulated histamine release depends on IP(3)R activation and plasmalemmal calcium entry. Gastrin-induced calcium influx was mediated by dihydropyridine-sensitive calcium channels that appear to be L-type channels activated through a pathway involving activation of PKC.

Published

2002

47. Expression of vesicular monoamine transporters, synaptosomal-associated protein 25 and syntaxin1: a signature of human small cell lung carcinoma.

Author

Graff L, Castrop F, Bauer M, Höfler H, and Gratzl M

Subjects

Adenocarcinoma genetics, Adenocarcinoma metabolism, Antigens, Surface genetics, Biomarkers, Tumor genetics, Blotting, Northern, Carcinoma, Small Cell genetics, Humans, Immunohistochemistry, Lung Neoplasms genetics, Membrane Glycoproteins genetics, Nerve Tissue Proteins genetics, RNA, Messenger biosynthesis, RNA, Messenger genetics, Reverse Transcriptase Polymerase Chain Reaction, Synaptosomal-Associated Protein 25, Syntaxin 1, Tumor Cells, Cultured, Vesicular Biogenic Amine Transport Proteins, Vesicular Monoamine Transport Proteins, Antigens, Surface biosynthesis, Biomarkers, Tumor biosynthesis, Carcinoma, Small Cell metabolism, Lung Neoplasms metabolism, Membrane Glycoproteins biosynthesis, Membrane Proteins, Membrane Transport Proteins, Nerve Tissue Proteins biosynthesis, Neuropeptides

Abstract

Vesicular monoamine transporters (VMATs) are a prerequisite for the uptake of biogenic amines into intracellular storage organelles, whereas soluble N-ethylmaleimide-sensitive factor attachment protein receptors (SNAREs; such as SNAP-25 and syntaxin1) are essential for exocytosis of biogenic amines by neurons and endocrine cells. In this study, we examined whether these proteins exist in high-grade malignant small cell lung carcinomas (SCLCs), large cell carcinomas, adenocarcinomas, and squamous cell carcinomas of the lung. We analyzed two established human SCLC cell lines, one adenocarcinoma cell line, paraffin-embedded tumors (SCLC, n = 25; large cell carcinoma, n = 10; adenocarcinoma, n = 10; squamous cell carcinoma, n = 10), and snap-frozen SCLC samples (n = 2). Using immunocytochemistry, Western blotting, Northern blotting, RT-PCR, and sequencing, we identified VMAT1, VMAT2, SNAP-25, and syntaxin1 in cultured SCLC cells. Immunohistochemistry carried out on paraffin sections revealed that all SCLC tumors express VMAT1, VMAT2, SNAP-25, and syntaxin1. The presence of SNAP-25 and syntaxin1 in SCLC was confirmed by RT-PCR performed with material extracted from paraffin sections. Western blot analysis and RT-PCR carried out with snap-frozen SCLC tumors revealed the presence of SNAREs and VMATs. Immunohistochemistry showed that non-SCLC tumors were negative for SNAREs and VMATs, with the exception of immunostaining for SNAP-25 and syntaxin1 in 3 of 10 adenocarcinomas. Our findings indicate that SCLC cells are endowed with transporters necessary for intracellular storage of biogenic amines and with proteins required for exocytosis of secretory products. These proteins may be used as markers of differentiation of human lung tumors. Moreover, the presence of VMATs provides the basis for a diagnostic application of biogenic amine-derived tracers in positron emission tomography of SCLC tumors.

Published

2001

48. Identification of an ovarian voltage-activated Na+-channel type: hints to involvement in luteolysis.

Author

Bulling A, Berg FD, Berg U, Duffy DM, Stouffer RL, Ojeda SR, Gratzl M, and Mayerhofer A

Subjects

Animals, Chorionic Gonadotropin pharmacology, Corpus Luteum physiology, Electrophysiology, Female, Granulosa Cells cytology, Granulosa Cells drug effects, Granulosa Cells metabolism, Humans, Lysosomes metabolism, Macaca mulatta genetics, Microscopy, Electron, Molecular Sequence Data, Ovary drug effects, Progesterone biosynthesis, Rats, Sodium Channels drug effects, Tetrodotoxin pharmacology, Ovary physiology, Sodium Channels physiology

Abstract

An endocrine type of voltage-activated sodium channel (eNaCh) was identified in the human ovary and human luteinized granulosa cells (GC). Whole-cell patch-clamp studies showed that the eNaCh in GC is functional and tetrodotoxin (TTX) sensitive. The luteotrophic hormone human CG (hCG) was found to decrease the peak amplitude of the sodium current within seconds. Treatment with hCG for 24-48 h suppressed not only eNaCh mRNA levels, but also mean Na+ peak currents and resting membrane potentials. An unexpected role for eNaChs in regulating cell morphology and function was indicated after pharmacological modulation of presumed eNaCh steady-state activity in GC cultures for 24-48 h using TTX (NaCh blocker) and veratridine (NaCh activator). TTX preserved a highly differentiated cellular phenotype. Veratridine not only increased the number of secondary lysosomes but also led to a significantly reduced progesterone production. Importantly, endocrine cells of the nonhuman primate corpus luteum (CL), which represent in vivo counterparts of luteinized GC, also contain eNaCh mRNA. Although the mechanism of channel activity under physiological conditions is not clear, it may include persistent Na+ currents. As observed in GC in culture, abundant secondary lysosomes were particularly evident in the regressing CL, suggesting a functional link between eNaCh activity and this form of cellular regression in vivo. Our results identify eNaCh in ovarian endocrine cells and demonstrate that their expression is under the inhibitory control of hCG. Activation of eNaChs in luteal cells, due to loss of gonadotropin support, may initiate a cascade of events leading to decreased CL function, a process that involves lysosomal activation and autophagy. These results imply that ovarian eNaChs are involved in the physiological demise of the temporary endocrine organ CL in the primate ovary during the menstrual cycle. Because commonly used drugs, including phenytoin, target NaChs, these results may be of clinical relevance.

Published

2000

49. Continuous in situ electrochemical monitoring of doxorubicin efflux from sensitive and drug-resistant cancer cells.

Author

Yi C and Gratzl M

Subjects

Animals, CHO Cells, Cricetinae, Drug Therapy, Electrochemistry, Humans, Microelectrodes, Molecular Structure, Neoplasms metabolism, Antineoplastic Agents pharmacokinetics, Doxorubicin pharmacokinetics, Drug Resistance, Multiple physiology

Abstract

One of the least well understood problems in cancer chemotherapy is the cross-resistance of certain tumor cells to a series of chemically unrelated drugs. Multidrug resistance (MDR) can be attributed to several different biophysical processes, among them increased drug efflux. This has been found to correlate with overexpression of the cell surface 170-kDa P-glycoprotein that actively excludes cytotoxic drugs against their concentration gradient. To better understand MDR, experimental methods are needed to study drug efflux from cancer cells. Continuous measurement of efflux of nonfluorescent drugs on the same cell culture in situ, or assessing efflux from a few cells or even a single cell, is beyond the capabilities of existing technologies. In this work, a carbon fiber (CF) microelectrode is used to monitor efflux of doxorubicin from a monolayer of two cell lines: an auxotrophic mutant of Chinese hamster ovary cells, AUXB1, and its MDR subline, CHRC5. Because doxorubicin is both fluorescent and electroactive, the results could be validated against existing data obtained optically and with other techniques on the same cell lines, with good agreement found. The electrochemical detection, however, is capable of in situ monitoring with high temporal resolution and is suitable for single-cell studies.

Published

1998

50. Functional importance of synaptobrevin and SNAP-25 during exocytosis of histamine by rat gastric enterochromaffin-like cells.

Author

Höhne-Zell B, Galler A, Schepp W, Gratzl M, and Prinz C

Subjects

Animals, Botulinum Toxins pharmacology, Calcium pharmacology, Cells, Cultured, Enterochromaffin Cells drug effects, Female, Gastric Mucosa cytology, Histamine Release physiology, Histidine Decarboxylase metabolism, Immunoblotting, R-SNARE Proteins, Rats, Rats, Sprague-Dawley, Stomach cytology, Stomach drug effects, Synaptosomal-Associated Protein 25, Tetanus Toxin pharmacology, Tissue Distribution, Enterochromaffin Cells metabolism, Exocytosis physiology, Gastric Mucosa metabolism, Histamine metabolism, Membrane Proteins physiology, Nerve Tissue Proteins physiology

Abstract

Gastric enterochromaffin-like (ECL) cells release histamine upon stimulation with gastrin in a calcium-dependent manner. The intracellular mechanisms and proteins mediating exocytosis of histamine-containing vesicles in ECL cells have not been determined yet. We used immunocytochemistry to show the localization of SNAP-25 (synaptosome-associated protein of 25 kDa) and synaptobrevin VAMP (vesicle-associated membrane protein) in ECL cells of the rat gastric mucosa and in isolated, highly enriched ECL cells, which were identified with an antibody directed against the marker enzyme histidine decarboxylase. Immunoblots of isolated ECL cells demonstrated the presence of SNAP-25, synaptobrevin, synaptophysin, synaptotagmin, and syntaxin. Histamine release from isolated ECL cells permeabilized with 8 microM digitonin (2 min) was stimulated approximately 2.5-fold upon exposure to calcium (30 microM; 10-min incubation). Preincubation with 1 microM tetanus toxin light chain for 15 min attenuated calcium-induced histamine release by 40-50% and almost completely cleaved synaptobrevin. Botulinum neurotoxin A (100 nM) totally blocked calcium-induced histamine release and cleaved SNAP-25. We conclude that synaptobrevin, synaptophysin, synaptotagmin, SNAP-25, and syntaxin are present in gastric ECL cells. Inhibition of histamine secretion by clostridial neurotoxins associated with the cleavage of synaptobrevin and SNAP-25 implicates the functional importance of these proteins in the docking and fusion of histamine vesicles.

Published

1997