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Featured researches published by C. Schlager.


PLOS ONE | 2015

Particulate Matter from Both Heavy Fuel Oil and Diesel Fuel Shipping Emissions Show Strong Biological Effects on Human Lung Cells at Realistic and Comparable In Vitro Exposure Conditions

Sebastian Oeder; Tamara Kanashova; Olli Sippula; Sean C. Sapcariu; Thorsten Streibel; Jose M. Arteaga-Salas; Johannes Passig; M. Dilger; Hanns-Rudolf Paur; C. Schlager; S. Mülhopt; S. Diabate; Carsten Weiss; Benjamin Stengel; R. Rabe; Horst Harndorf; Tiina Torvela; Jorma Jokiniemi; Maija-Riitta Hirvonen; Carsten B. Schmidt-Weber; Claudia Traidl-Hoffmann; Kelly Ann Berube; Anna Julia Wlodarczyk; Zoe Cariad Prytherch; Bernhard Michalke; T. Krebs; André S. H. Prévôt; Michael Kelbg; Josef Tiggesbäumker; Erwin Karg

Background Ship engine emissions are important with regard to lung and cardiovascular diseases especially in coastal regions worldwide. Known cellular responses to combustion particles include oxidative stress and inflammatory signalling. Objectives To provide a molecular link between the chemical and physical characteristics of ship emission particles and the cellular responses they elicit and to identify potentially harmful fractions in shipping emission aerosols. Methods Through an air-liquid interface exposure system, we exposed human lung cells under realistic in vitro conditions to exhaust fumes from a ship engine running on either common heavy fuel oil (HFO) or cleaner-burning diesel fuel (DF). Advanced chemical analyses of the exhaust aerosols were combined with transcriptional, proteomic and metabolomic profiling including isotope labelling methods to characterise the lung cell responses. Results The HFO emissions contained high concentrations of toxic compounds such as metals and polycyclic aromatic hydrocarbon, and were higher in particle mass. These compounds were lower in DF emissions, which in turn had higher concentrations of elemental carbon (“soot”). Common cellular reactions included cellular stress responses and endocytosis. Reactions to HFO emissions were dominated by oxidative stress and inflammatory responses, whereas DF emissions induced generally a broader biological response than HFO emissions and affected essential cellular pathways such as energy metabolism, protein synthesis, and chromatin modification. Conclusions Despite a lower content of known toxic compounds, combustion particles from the clean shipping fuel DF influenced several essential pathways of lung cell metabolism more strongly than particles from the unrefined fuel HFO. This might be attributable to a higher soot content in DF. Thus the role of diesel soot, which is a known carcinogen in acute air pollution-induced health effects should be further investigated. For the use of HFO and DF we recommend a reduction of carbonaceous soot in the ship emissions by implementation of filtration devices.


PLOS ONE | 2016

Metabolic Profiling as Well as Stable Isotope Assisted Metabolic and Proteomic Analysis of RAW 264.7 Macrophages Exposed to Ship Engine Aerosol Emissions: Different Effects of Heavy Fuel Oil and Refined Diesel Fuel.

Sean C. Sapcariu; Tamara Kanashova; M. Dilger; S. Diabate; Sebastian Oeder; Johannes Passig; C. Radischat; Jeroen Buters; Olli Sippula; Thorsten Streibel; Hanns-Rudolf Paur; C. Schlager; S. Mülhopt; Benjamin Stengel; R. Rabe; Horst Harndorf; T. Krebs; Erwin Karg; Thomas Gröger; Carsten Weiss; Gunnar Dittmar; Karsten Hiller; Ralf Zimmermann

Exposure to air pollution resulting from fossil fuel combustion has been linked to multiple short-term and long term health effects. In a previous study, exposure of lung epithelial cells to engine exhaust from heavy fuel oil (HFO) and diesel fuel (DF), two of the main fuels used in marine engines, led to an increased regulation of several pathways associated with adverse cellular effects, including pro-inflammatory pathways. In addition, DF exhaust exposure was shown to have a wider response on multiple cellular regulatory levels compared to HFO emissions, suggesting a potentially higher toxicity of DF emissions over HFO. In order to further understand these effects, as well as to validate these findings in another cell line, we investigated macrophages under the same conditions as a more inflammation-relevant model. An air-liquid interface aerosol exposure system was used to provide a more biologically relevant exposure system compared to submerged experiments, with cells exposed to either the complete aerosol (particle and gas phase), or the gas phase only (with particles filtered out). Data from cytotoxicity assays were integrated with metabolomics and proteomics analyses, including stable isotope-assisted metabolomics, in order to uncover pathways affected by combustion aerosol exposure in macrophages. Through this approach, we determined differing phenotypic effects associated with the different components of aerosol. The particle phase of diluted combustion aerosols was found to induce increased cell death in macrophages, while the gas phase was found more to affect the metabolic profile. In particular, a higher cytotoxicity of DF aerosol emission was observed in relation to the HFO aerosol. Furthermore, macrophage exposure to the gas phase of HFO leads to an induction of a pro-inflammatory metabolic and proteomic phenotype. These results validate the effects found in lung epithelial cells, confirming the role of inflammation and cellular stress in the response to combustion aerosols.


Journal of Aerosol Science | 2016

Toxicity testing of combustion aerosols at the air–liquid interface with a self-contained and easy-to-use exposure system

S. Mülhopt; M. Dilger; S. Diabate; C. Schlager; T. Krebs; Ralf Zimmermann; Jeroen Buters; Sebastian Oeder; Thomas Wäscher; Carsten Weiss; Hanns-Rudolf Paur


Analytica : 26.Internationale Leitmesse für Labortechnik, Analytik, Biotechnologie und Analytica Conference, München, 10.-13.April 2018 | 2018

Systems toxicology of wood smoke

M. Dilger; L. Ramme; Sean C. Sapcariu; S. Mülhopt; C. Schlager; Ahmed Reda; Jürgen Orasche; O. Armant; E. Maser; A. Hartwig; Ralf Zimmermann; Karsten Hiller; S. Diabate; Hanns-Rudolf Paur; Carsten Weiss


Archive | 2017

In Vitro Exposure Systems to Assess the Toxicity of Airborne Substances

T. Krebs; S. Mülhopt; S. Diabate; C. Schlager; Hanns R. Paur; M. Dilger


New Tools and Approaches for Nanomaterial Safety Assessment, Malaga, Spain, February 7 – 9, 2017 | 2017

Effects of Cerium oxide nanoparticle aerosol on human lung cells exposed at the air-liquid-interface

S. Mülhopt; S. Diabate; C. Schlager; M. Dilger; Sivakumar Murugadoss; Carsten Weiss; T. Krebs; Selina Tang; Pete Gooden; Leigh-Anne Koekemoer; Susan Dekkers; Flemming R. Cassee; Hanns-Rudolf Paur


Nanosafety 2017, Saarbrücken, October 11-13, 2017. Hrsg.: E. Arzt | 2017

Lung toxicity testing of aerosols for in-vitro studies at the air-liquid-interface with integrated dose monitoring

S. Mülhopt; S. Diabate; C. Schlager; Dilger Marco; Markus Berger; T. Krebs; Carsten Weiss; Hanns-Rudolf Paur


European Aerosol Conference 2017, Zürich, Schweiz, 27.08.-01.09.2017 | 2017

Toxicity of wood smoke particles in human lung epithelial cells: The role of PAHs, soot and zinc

M. Dilger; Jürgen Orasche; C. Schlager; S. Mühlhopt; Ralf Zimmermann; Hanns-Rudolf Paur; S. Diabate; Carsten Weiss


European Aerosol Conference (EAC), Zurich, Schweiz, Switzerland, 27th August - 1st September 2017 | 2017

Particle mass monitoring by Quartz Crystal Microbalance using electrostatic deposition enhancement

S. Mülhopt; C. Schlager; T. Krebs; M. Berger; Hanns-Rudolf Paur


6th International Symposium on Ultrafine Particles Air Quality and Climate, Brussels, B, May 10-11, 2017 | 2017

Lung Toxicity of Aerosols the Air-Liquid Interface with Integrated Dose Monitoring

S. Mülhopt; S. Diabate; C. Schlager; M. Dilger; Carsten Weiss; T. Krebs; Hanns-Rudolf Paur

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S. Diabate

Karlsruhe Institute of Technology

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S. Mülhopt

Karlsruhe Institute of Technology

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Hanns-Rudolf Paur

Karlsruhe Institute of Technology

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M. Dilger

Karlsruhe Institute of Technology

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Carsten Weiss

Karlsruhe Institute of Technology

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R. Rabe

University of Rostock

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