Your search keyword '"Öller, M"' showing total 12 results

1. International Forum on GMP‐grade human platelet lysate for cell propagation: summary

Author

Strunk, D., Lozano, M., Marks, D.C., Loh, Y. S., Gstraunthaler, G., Schennach, H., Rohde, E., Laner‐Plamberger, S., Öller, M., Nystedt, J., Lotfi, R., Rojewski, M., Schrezenmeier, H., Bieback, K., Schäfer, R., Bakchoul, T., Waidmann, M., Jonsdottir‐Buch, S.M., Montazeri, H., Sigurjonsson, O.E., Iudicone, P., Fioravanti, D., Pierelli, L., Introna, M., Capelli, C., Falanga, A., Takanashi, M., Lόpez‐Villar, O., Burnouf, T., Reems, J. A., Pierce, J., Preslar, A.M., and Schallmoser, K.

Published

2018

2. Exosomes differentially modulate the osteogenic and adipogenic induction of bone marrow-derived mesenchymal stem and progenitor cells: OP-028

Author

Gimona, M, Lener, T, Streif, D, Peckl-Schmid, D, Öller, M, Schallmoser, K, Laner-Plamberger, S, and Rohde, E

Published

2013

3. International Forum on GMP-grade human platelet lysate for cell propagation

Author

Strunk, D, Lozano, M, Marks, D, Loh, Y, Gstraunthaler, G, Schennach, H, Rohde, E, Laner-Plamberger, S, Öller, M, Nystedt, J, Lotfi, R, Rojewski, M, Schrezenmeier, H, Bieback, K, Schäfer, R, Bakchoul, T, Waidmann, M, Jonsdottir-Buch, S, Montazeri, H, Sigurjonsson, O, Iudicone, P, Fioravanti, D, Pierelli, L, Introna, M, Capelli, C, Falanga, A, Takanashi, M, López-Villar, O, Burnouf, T, Reems, J, Pierce, J, Preslar, A, Schallmoser, K, Strunk D, Lozano M, Marks DC, Loh YS, Gstraunthaler G, Schennach H, Rohde E, Laner-Plamberger S, Öller M, Nystedt J, Lotfi R, Rojewski M, Schrezenmeier H, Bieback K, Schäfer R, Bakchoul T, Waidmann M, Jonsdottir-Buch SM, Montazeri H, Sigurjonsson OE, Iudicone P, Fioravanti D, Pierelli L, Introna M, Capelli C, Falanga A, Takanashi M, López-Villar O, Burnouf T, Reems JA, Pierce J, Preslar AM, Schallmoser K, Strunk, D, Lozano, M, Marks, D, Loh, Y, Gstraunthaler, G, Schennach, H, Rohde, E, Laner-Plamberger, S, Öller, M, Nystedt, J, Lotfi, R, Rojewski, M, Schrezenmeier, H, Bieback, K, Schäfer, R, Bakchoul, T, Waidmann, M, Jonsdottir-Buch, S, Montazeri, H, Sigurjonsson, O, Iudicone, P, Fioravanti, D, Pierelli, L, Introna, M, Capelli, C, Falanga, A, Takanashi, M, López-Villar, O, Burnouf, T, Reems, J, Pierce, J, Preslar, A, Schallmoser, K, Strunk D, Lozano M, Marks DC, Loh YS, Gstraunthaler G, Schennach H, Rohde E, Laner-Plamberger S, Öller M, Nystedt J, Lotfi R, Rojewski M, Schrezenmeier H, Bieback K, Schäfer R, Bakchoul T, Waidmann M, Jonsdottir-Buch SM, Montazeri H, Sigurjonsson OE, Iudicone P, Fioravanti D, Pierelli L, Introna M, Capelli C, Falanga A, Takanashi M, López-Villar O, Burnouf T, Reems JA, Pierce J, Preslar AM, and Schallmoser K

Published

2018

4. International Forum on GMP-grade human platelet lysate for cell propagation: summary

Author

Strunk, D., primary, Lozano, M., additional, Marks, D.C., additional, Loh, Y. S., additional, Gstraunthaler, G., additional, Schennach, H., additional, Rohde, E., additional, Laner-Plamberger, S., additional, Öller, M., additional, Nystedt, J., additional, Lotfi, R., additional, Rojewski, M., additional, Schrezenmeier, H., additional, Bieback, K., additional, Schäfer, R., additional, Bakchoul, T., additional, Waidmann, M., additional, Jonsdottir-Buch, S.M., additional, Montazeri, H., additional, Sigurjonsson, O.E., additional, Iudicone, P., additional, Fioravanti, D., additional, Pierelli, L., additional, Introna, M., additional, Capelli, C., additional, Falanga, A., additional, Takanashi, M., additional, Lόpez-Villar, O., additional, Burnouf, T., additional, Reems, J. A., additional, Pierce, J., additional, Preslar, A.M., additional, and Schallmoser, K., additional

Published

2017

5. Las orientaciones éticas de los periodistas dentro de la cultura periodística de Ecuador

Author

Oller, Martín, Chavero-Ramírez, Palmira, Cevallos, Patricio, and Carrillo, Julia

Subjects

Cultura Periodística, Ecuador, ética periodística, deontología, autorregulación, profesionalismo - See more at: http://www.gigapp.org/index.php/component/jresearch/?view=publication&task=show&id=1813#sthash.M95PhK26.dpuf, profesionalismo, Political science

Abstract

Este artículo presenta los resultados relacionados con los valores éticos de los periodistas ecuatorianos obtenidos del proyecto Cultura Periodística de Ecuador (CPE). El principal objetivo de este estudio es determinar las orientaciones éticas tradicionales y comunes que comparten los entrevistados, ya que estos principios definen la responsabilidad, las decisiones, la autonomía y el ejercicio profesional de los periodistas. La ética profesional es uno de los principales factores que determina el nivel de profesionalismo de los periodistas y la profesionalización del periodismo; la regulación del mercado mediático –basado en el modelo económico y empresarial de los medios–; la autorregulación de los medios –códigos deontológicos–; el intervencionismo del Estado y la implicación de la sociedad civil en el proceso comunicativo –participación y acceso a la información de los ciudadanos–. En este estudio se realizaron 31 entrevistas en profundidad a periodistas en activo de 6 medios de comunicación nacionales y un análisis contextual de la cultura periodística de Ecuador. Los resultados muestran que los periodistas entrevistados en Ecuador quedan clasificados dentro del contexto periodístico, según las perspectivas propuestas por Plaisance (2005) y Hanitzsch (2007) basadas en las ideologías éticas, como eminentemente absolutistas, tendientes al situacionismo y en menor medida al excepcionismo.

Published

2015

6. Nucleophile Acylierung mit verkappten Acyl-Anionen IV;1α,β-ungesättigte Acyl-Anionen

Author

HERTENSTEIN, U., primary, HÜNIG, S., additional, and ÖLLER, M., additional

Published

1976

7. Nucleophile Acylierung mit verkappten Acyl-Anionen IV;1 α,β-ungesättigte Acyl-Anionen

Author

HERTENSTEIN, U., HÜNIG, S., and ÖLLER, M.

Published

1976

8. International Forum on GMP-grade human platelet lysate for cell propagation

Author

D. Strunk, M. Lozano, D. C. Marks, Y. S. Loh, G. Gstraunthaler, H. Schennach, E. Rohde, S. Laner-Plamberger, M. Öller, J. Nystedt, R. Lotfi, M. Rojewski, H. Schrezenmeier, K. Bieback, R. Schäfer, T. Bakchoul, M. Waidmann, S. M. Jonsdottir-Buch, H. Montazeri, O. E. Sigurjonsson, P. Iudicone, D. Fioravanti, L. Pierelli, M. Introna, C. Capelli, A. Falanga, M. Takanashi, O. López-Villar, T. Burnouf, J. A. Reems, J. Pierce, A. M. Preslar, K. Schallmoser, Strunk, D, Lozano, M, Marks, D, Loh, Y, Gstraunthaler, G, Schennach, H, Rohde, E, Laner-Plamberger, S, Öller, M, Nystedt, J, Lotfi, R, Rojewski, M, Schrezenmeier, H, Bieback, K, Schäfer, R, Bakchoul, T, Waidmann, M, Jonsdottir-Buch, S, Montazeri, H, Sigurjonsson, O, Iudicone, P, Fioravanti, D, Pierelli, L, Introna, M, Capelli, C, Falanga, A, Takanashi, M, López-Villar, O, Burnouf, T, Reems, J, Pierce, J, Preslar, A, and Schallmoser, K

Subjects

0301 basic medicine, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, no keywords for this article, Hematology, General Medicine, platelet, GMP‐grade hPL, blood, 030204 cardiovascular system & hematology

Published

2017

9. Development of a Novel Passive Monitoring Technique to Showcase the 3D Distribution of Tritiated Water (HTO) Vapor in Indoor Air of a Nuclear Facility.

Author

Feng B, Ibesich M, Hainz D, Waidhofer D, Veit-Öller M, Trunner C, Stummer T, Foster M, Nemetz M, Welch JM, Villa M, Sterba JH, Musilek A, Renz F, and Steinhauser G

Subjects

Water, Tritium analysis, Gases, Air Pollutants, Radioactive analysis, Air Pollution, Indoor analysis, Radiation Monitoring methods

Abstract

Tritiated water (HTO), a ubiquitous byproduct of the nuclear industry, is a radioactive contaminant of major concern for environmental authorities. Although understanding spatiotemporal heterogeneity of airborne HTO vapor holds great importance for radiological safety as well as diagnosing a reactor's status, comprehensive HTO distribution dynamics inside nuclear facilities has not been studied routinely yet due to a lack of appropriate monitoring techniques. For current systems, it is difficult to simultaneously achieve high representativeness, sensitivity, and spatial resolution. Here, we developed a passive monitoring scheme, including a newly designed passive sampler and a tailored analytical protocol for the first comprehensive 3D distribution characterization of HTO inside a nuclear reactor facility. The technique enables linear sampling in any environment at a one-day resolution and simultaneous preparation of hundreds of samples within 1 day. Validation experiments confirmed the method's good metrological properties and sensitivity to the HTO's spatial dynamics. The air in TU Wien's reactor hall exhibits a range of 3 H concentrations from 75-946 mBq m -3 in the entire 3D matrix. The HTO release rate estimated by the mass-balance model (3199 ± 306 Bq h -1 ) matches the theoretical calculation (2947 ± 254 Bq h -1 ), suggesting evaporation as the dominant HTO source in the hall. The proposed method provides reliable and quality-controlled 3D monitoring at low cost, which can be adopted not only for HTO and may also inspire monitoring schemes of other indoor pollutants.

Published

2023

10. A Good Manufacturing Practice-grade standard protocol for exclusively human mesenchymal stromal cell-derived extracellular vesicles.

Author

Pachler K, Lener T, Streif D, Dunai ZA, Desgeorges A, Feichtner M, Öller M, Schallmoser K, Rohde E, and Gimona M

Subjects

Adipogenesis drug effects, Adipogenesis physiology, Cell Differentiation drug effects, Cell Engineering methods, Cells, Cultured, Culture Media, Conditioned metabolism, Culture Media, Conditioned pharmacology, Humans, Manufacturing Industry methods, Mesenchymal Stem Cell Transplantation methods, Mesenchymal Stem Cells ultrastructure, Osteogenesis drug effects, Osteogenesis physiology, Practice Guidelines as Topic standards, Reference Standards, Cell Culture Techniques standards, Cell Engineering standards, Extracellular Vesicles transplantation, Manufacturing Industry standards, Mesenchymal Stem Cells cytology

Abstract

Background Aims: Extracellular vesicles (EVs) released by mesenchymal stromal cells (MSCs) may contribute to biological processes such as tissue regeneration, immunomodulation and neuroprotection. Evaluation of their therapeutic potential and application in future clinical trials demands thorough characterization of EV content and production under defined medium conditions, devoid of xenogenic substances and serum-derived vesicles. Addressing the apparent need for such a growth medium, we have developed a medium formulation based on pooled human platelet lysate (pHPL), free from animal-derived xenogenic additives and depleted of EVs., Methods: Depletion of EVs from complete growth medium was achieved by centrifugation at 120 000 g for 3 h, which reduced RNA-containing pHPL EVs to below the detection limit., Results: Bone marrow (BM)-derived MSCs propagated in this medium retained the characteristic surface marker expression, cell morphology, viability and in vitro osteogenic and adipogenic differentiation potential. The proliferation rate was not significantly affected after 48 h but was decreased by 13% after 96 h. EVs collected from BM-MSCs cultured in EV-depleted medium revealed a similar RNA pattern as EVs generated in standard pHPL EV-containing medium but displayed a more clearly defined pattern of proteins characteristic for EVs. Reduction of pHPL content from 10% to 2% or serum-/pHPL-free conditions strongly altered MSC characteristics and RNA content of released EV., Conclusions: The 10% pHPL-based EV-depleted medium is appropriate for purification of exclusively human MSC-derived EVs. With this Good Manufacturing Practice-grade protocol, characterization and establishment of protein and RNA profiles from MSC-derived EVs can now be achieved to identify active components in therapeutic EVs for future clinical application., (Copyright © 2017 International Society for Cellular Therapy. Published by Elsevier Inc. All rights reserved.)

Published

2017

11. Mechanical fibrinogen-depletion supports heparin-free mesenchymal stem cell propagation in human platelet lysate.

Author

Laner-Plamberger S, Lener T, Schmid D, Streif DA, Salzer T, Öller M, Hauser-Kronberger C, Fischer T, Jacobs VR, Schallmoser K, Gimona M, and Rohde E

Subjects

Blood Platelets metabolism, Cell Differentiation, Flow Cytometry, Humans, Mesenchymal Stem Cells metabolism, Blood Platelets cytology, Fibrinogen metabolism, Heparin metabolism, Mesenchymal Stem Cells cytology

Abstract

Background: Pooled human platelet lysate (pHPL) is an efficient alternative to xenogenic supplements for ex vivo expansion of mesenchymal stem cells (MSCs) in clinical studies. Currently, porcine heparin is used in pHPL-supplemented medium to prevent clotting due to plasmatic coagulation factors. We therefore searched for an efficient and reproducible medium preparation method that avoids clot formation while omitting animal-derived heparin., Methods: We established a protocol to deplete fibrinogen by clotting of pHPL in medium, subsequent mechanical hydrogel disruption and removal of the fibrin pellet. After primary culture, bone-marrow and umbilical cord derived MSCs were tested for surface markers by flow cytometry and for trilineage differentiation capacity. Proliferation and clonogenicity were analyzed for three passages., Results: The proposed clotting procedure reduced fibrinogen more than 1000-fold, while a volume recovery of 99.5 % was obtained. All MSC types were propagated in standard and fibrinogen-depleted medium. Flow cytometric phenotype profiles and adipogenic, osteogenic and chondrogenic differentiation potential in vitro were independent of MSC-source or medium type. Enhanced proliferation of MSCs was observed in the absence of fibrinogen but presence of heparin compared to standard medium. Interestingly, this proliferative response to heparin was not detected after an initial contact with fibrinogen during the isolation procedure., Conclusions: Here, we present an efficient, reproducible and economical method in compliance to good manufacturing practice for the preparation of MSC media avoiding xenogenic components and suitable for clinical studies.

Published

2015

12. Lesion-induced accumulation of platelets promotes survival of adult neural stem / progenitor cells.

Author

Kazanis I, Feichtner M, Lange S, Rotheneichner P, Hainzl S, Öller M, Schallmoser K, Rohde E, Reitsamer HA, Couillard-Despres S, Bauer HC, Franklin RJ, Aigner L, and Rivera FJ

Subjects

Adult Stem Cells cytology, Animals, Brain Injuries pathology, Cell Differentiation physiology, Cell Survival physiology, Demyelinating Diseases pathology, Disease Models, Animal, Female, Male, Mice, Inbred C57BL, Neurons cytology, Blood Platelets cytology, Neural Stem Cells cytology, Neurogenesis physiology

Abstract

The presence of neural stem/progenitor cells (NSPCs) in specific areas of the central nervous system (CNS) supports tissue maintenance as well as regeneration. The subependymal zone (SEZ), located at the lateral ventricle's wall, represents a niche for NSPCs and in response to stroke or demyelination becomes activated with progenitors migrating towards the lesion and differentiating into neurons and glia. The mechanisms that underlie this phenomenon remain largely unknown. The vascular niche and in particular blood-derived elements such as platelets, has been shown to contribute to CNS regeneration in different pathological conditions. Indeed, intracerebroventricularly administrated platelet lysate (PL) stimulates angiogenesis, neurogenesis and neuroprotection in the damaged CNS. Here, we explored the presence of platelets in the activated SEZ after a focal demyelinating lesion in the corpus callosum of mice and we studied the effects of PL on proliferating SEZ-derived NSPCs in vitro. We showed that the lesion-induced increase in the size of the SEZ and in the number of proliferating SEZ-resident NSPCs correlates with the accumulation of platelets specifically along the activated SEZ vasculature. Expanding on this finding, we demonstrated that exposure of NSPCs to PL in vitro led to increased numbers of cells by enhanced cell survival and reduced apoptosis without differences in proliferation and in the differentiation potential of NSPCs. Finally, we demonstrate that the accumulation of platelets within the SEZ is spatially correlated with reduced numbers of apoptotic cells when compared to other periventricular areas. In conclusion, our results show that platelet-derived compounds specifically promote SEZ-derived NSPC survival and suggest that platelets might contribute to the enlargement of the pool of SEZ NSPCs that are available for CNS repair in response to injury., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015