Your search keyword '"Shuster-Meiseles T"' showing total 7 results

1. Correction to Size-resolved Identification, Characterization and Quantification of Primary Biological Organic Aerosol at a European Rural Site.

Author

Bozzetti C, Daellenbach KR, Hueglin C, Fermo P, Sciare J, Kasper-Giebl A, Mazar Y, Abbaszade G, Kazzi ME, Gonzalez R, Shuster-Meiseles T, Flasch M, Wolf R, Křepelová A, Canonaco F, Schnelle-Kreis J, Slowik JG, Zimmermann R, Rudich Y, Baltensperger U, Haddad IE, and Prévôt AS

Published

2016

2. Size-Resolved Identification, Characterization, and Quantification of Primary Biological Organic Aerosol at a European Rural Site.

Author

Bozzetti C, Daellenbach KR, Hueglin C, Fermo P, Sciare J, Kasper-Giebl A, Mazar Y, Abbaszade G, El Kazzi M, Gonzalez R, Shuster-Meiseles T, Flasch M, Wolf R, Křepelová A, Canonaco F, Schnelle-Kreis J, Slowik JG, Zimmermann R, Rudich Y, Baltensperger U, El Haddad I, and Prévôt AS

Subjects

Air Microbiology, Carbohydrates analysis, Carbohydrates chemistry, Gas Chromatography-Mass Spectrometry, Humans, Mass Spectrometry methods, Particulate Matter analysis, Polymerase Chain Reaction, Rural Population, Seasons, Spores, Bacterial genetics, Spores, Fungal genetics, Switzerland, Aerosols analysis, Environmental Monitoring methods

Abstract

Primary biological organic aerosols (PBOA) represent a major component of the coarse organic matter (OMCOARSE, aerodynamic diameter > 2.5 μm). Although this fraction affects human health and the climate, its quantification and chemical characterization currently remain elusive. We present the first quantification of the entire PBOACOARSE mass and its main sources by analyzing size-segregated filter samples collected during the summer and winter at the rural site of Payerne (Switzerland), representing a continental Europe background environment. The size-segregated water-soluble OM was analyzed by a newly developed offline aerosol mass spectrometric technique (AMS). Collected spectra were analyzed by three-dimensional positive matrix factorization (3D-PMF), showing that PBOA represented the main OMCOARSE source during summer and its contribution to PM10 was comparable to that of secondary organic aerosol. We found substantial cellulose contributions to OMCOARSE, which in combination with gas chromatography mass spectrometry molecular markers quantification, underlined the predominance of plant debris. Quantitative polymerase chain reaction (qPCR) analysis instead revealed that the sum of bacterial and fungal spores mass represented only a minor OMCOARSE fraction (<0.1%). X-ray photoelectron spectroscopic (XPS) analysis of C and N binding energies throughout the size fractions revealed an organic N increase in the PM10 compared to PM1 consistent with AMS observations.

Published

2016

3. ROS-generating/ARE-activating capacity of metals in roadway particulate matter deposited in urban environment.

Author

Shuster-Meiseles T, Shafer MM, Heo J, Pardo M, Antkiewicz DS, Schauer JJ, Rudich A, and Rudich Y

Subjects

Aerosols analysis, Air Pollutants analysis, Cells, Cultured, Cities, Environmental Monitoring, Filtration, Greece, Italy, London, Metals analysis, Metals toxicity, Particulate Matter analysis, Transition Elements analysis, Vehicle Emissions analysis, Aerosols toxicity, Air Pollutants toxicity, Particulate Matter toxicity, Reactive Oxygen Species metabolism, Transition Elements toxicity

Abstract

In this study we investigated the possible causal role for soluble metal species extracted from roadway traffic emissions in promoting particulate matter (PM)-induced reactive oxygen species (ROS) production and antioxidant response element (ARE) promoter activation. To this end, these responses have been evaluated in alveolar macrophage and epithelial lung cells that have been exposed to 'Unfiltered', 'Filtered' and 'Filtered+Chelexed' water extracts of PM samples collected from the roadway urban environments of Thessaloniki, Milan and London. Except for Thessaloniki, our results demonstrate that filtration resulted in a minor decrease in ROS activity of the fine PM fraction, suggesting that ROS activity is attributed mainly to water-soluble PM species. In contrast to ROS, ARE activity was mediated predominantly by the water-soluble component of PM present in both the fine and coarse extracts. Further removal of metals by Chelex treatment from filtered water extracts showed that soluble metal species are the major factors mediating ROS and ARE activities of the soluble fraction, especially in the London PM extracts. Finally, utilizing step-wise multiple-regression analysis, we show that 87% and 78% of the total variance observed in ROS and ARE assays, respectively, is accounted for by changes in soluble metal concentration. Using a statistical analysis we find that As, Zn and Fe best predict the ROS-generating/ARE-activating capacity of the near roadway particulate matter in the pulmonary cells studied. Collectively, our findings imply that soluble metals present in roadside PM are potential drivers of both pro- and anti-oxidative effects of PM in respiratory tract., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2016

4. Impact of urban air pollution on the allergenicity of Aspergillus fumigatus conidia: Outdoor exposure study supported by laboratory experiments.

Author

Lang-Yona N, Shuster-Meiseles T, Mazar Y, Yarden O, and Rudich Y

Subjects

Hypersensitivity epidemiology, Spores, Fungal, Air Microbiology, Air Pollution statistics & numerical data, Allergens analysis, Aspergillus fumigatus growth & development, Environmental Exposure statistics & numerical data

Abstract

Understanding the chemical interactions of common allergens in urban environments may help to decipher the general increase in susceptibility to allergies observed in recent decades. In this study, asexual conidia of the allergenic mold Aspergillus fumigatus were exposed to air pollution under natural (ambient) and controlled (laboratory) conditions. The allergenic activity was measured using two immunoassays and supported by a protein mass spectrometry analysis. The allergenicity of the conidia was found to increase by 2-5 fold compared to the control for short exposure times of up to 12h (accumulated exposure of about 50 ppb NO2 and 750 ppb O3), possibly due to nitration. At higher exposure times, the allergenicity increase lessened due to protein deamidation. These results indicate that during the first 12h of exposure, the allergenic potency of the fungal allergen A. fumigatus in polluted urban environments is expected to increase. Additional work is needed in order to determine if this behavior occurs for other allergens., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2016

5. Low cytotoxicity of inorganic nanotubes and fullerene-like nanostructures in human bronchial epithelial cells: relation to inflammatory gene induction and antioxidant response.

Author

Pardo M, Shuster-Meiseles T, Levin-Zaidman S, Rudich A, and Rudich Y

Subjects

Antioxidants analysis, Antioxidants metabolism, Cell Line, Cell Survival drug effects, Cytokines analysis, Cytokines genetics, Cytokines metabolism, Disulfides toxicity, Gene Expression drug effects, Humans, Molybdenum toxicity, Particulate Matter metabolism, Silicon Dioxide toxicity, Soot toxicity, Tungsten toxicity, Epithelial Cells drug effects, Fullerenes toxicity, Nanotubes toxicity

Abstract

The cytotoxicity of tungsten disulfide nano tubes (INT-WS2) and inorganic fullerene-like molybdenum disulfide (IF-MoS2) nanoparticles (NPs) used in industrial and medical applications was evaluated in comparison to standard environmental particulate matter. The IF-MoS2 and INT-WS2 reside in vesicles/inclusion bodies, suggestive of endocytic vesicles. In cells representing the respiratory, immune and metabolic systems, both IF-MoS2 and INT-WS2 NPs remained nontoxic compared to equivalent concentrations (up to 100 μg/mL in the medium) of silica dioxide (SiO2), diesel engine-derived and carbon black NPs, which induced cell death. Associating with this biocompatibility of IF-MoS2\INT-WS2, we demonstrate in nontransformed human bronchial cells (NL-20) relative low induction of the pro-inflammatory cytokines IL-1β, IL-6, IL-8, and TNF-α. Moreover, IF-MoS2 and INT-WS2 activated antioxidant response as measured by the antioxidant response element (ARE) using a luciferase reporter, and induced Nrf2-mediated Phase II detoxification genes. Collectively, our findings suggest that the lower cytotoxicity of IF-MoS2 and INT-WS2 NPs does not reflect general biological inertness. Rather, compared to other NP's, it likely results from decreased pro-inflammatory activation, but a comparable significant capacity to induce protective antioxidant/detoxification defense mechanisms.

Published

2014

6. TiO2 nanoparticles induce insulin resistance in liver-derived cells both directly and via macrophage activation.

Author

Gurevitch D, Shuster-Meiseles T, Nov O, Zick Y, Rudich A, and Rudich Y

Subjects

Animals, Blotting, Western, Cell Line, Tumor, Culture Media, Conditioned, Glycogen biosynthesis, Insulin metabolism, Rats, Real-Time Polymerase Chain Reaction, Signal Transduction, Insulin Resistance, Liver drug effects, Macrophage Activation, Metal Nanoparticles toxicity, Titanium toxicity

Abstract

Upon exposure, TiO(2) nanoparticles (NPs) have been recovered in internal organs such as the liver, and are proposed to cause cellular/organ dysfunction, particularly in the liver and lungs. We hypothesized that despite being considered "inert" as bulk material, TiO(2) NPs may impair insulin responses in liver-derived cells, either indirectly by inflammatory activation of macrophages, and/or by directly interfering with insulin signaling. Using qRT-PCR and conditioned medium (CM) approaches, we show that exposure to TiO(2) NPs activates macrophages' expression of TNF-α, IL-6, IL-8, IL-1α and IL-1β and the resulting CM induces insulin resistance in Fao cells. Furthermore, direct exposure of Fao cells to TiO(2) results in activation of the stress kinases JNK and p38MAP kinase, and in induction of insulin resistance at the signaling and metabolic levels. Collectively, our findings provide a proof-of-concept for the ability of man-made NPs to induce insulin resistance in liver-derived cells, an endocrine abnormality underlying some of the most common human diseases.

Published

2012

7. A novel domain mediates insulin-induced proteasomal degradation of insulin receptor substrate 1 (IRS-1).

Author

Boura-Halfon S, Shuster-Meiseles T, Beck A, Petrovich K, Gurevitch D, Ronen D, and Zick Y

Subjects

Animals, Apoptosis drug effects, CHO Cells, Cricetinae, Cricetulus, Cytoprotection drug effects, Mice, Mutant Proteins chemistry, Mutant Proteins metabolism, Phosphorylation drug effects, Phosphoserine metabolism, Protein Structure, Tertiary, Protein Transport drug effects, Proto-Oncogene Proteins c-mdm2 metabolism, Rats, Sequence Deletion, Signal Transduction drug effects, Structure-Activity Relationship, Ubiquitination drug effects, Insulin pharmacology, Insulin Receptor Substrate Proteins chemistry, Insulin Receptor Substrate Proteins metabolism, Proteasome Endopeptidase Complex metabolism, Protein Processing, Post-Translational drug effects

Abstract

Insulin receptor substrate-1 (IRS-1) plays a pivotal role in insulin signaling, therefore its degradation is exquisitely regulated. Here, we show that insulin-stimulated degradation of IRS-1 requires the presence of a highly conserved Ser/Thr-rich domain that we named domain involved in degradation of IRS-1 (DIDI). DIDI (amino acids 386-430 of IRS-1) was identified by comparing the intracellular degradation rate of several truncated forms of IRS-1 transfected into CHO cells. The isolated DIDI domain underwent insulin-stimulated Ser/Thr phosphorylation, suggesting that it serves as a target for IRS-1 kinases. The effects of deletion of DIDI were studied in Fao rat hepatoma and in CHO cells expressing Myc-IRS-1(WT) or Myc-IRS-1(Δ386-430). Deletion of DIDI maintained the ability of IRS-1(Δ386-434) to undergo ubiquitination while rendering it insensitive to insulin-induced proteasomal degradation, which affected IRS-1(WT) (80% at 8 h). Consequently, IRS-1(Δ386-434) mediated insulin signaling (activation of Akt and glycogen synthesis) better than IRS-1(WT). IRS-1(Δ386-434) exhibited a significant greater preference for nuclear localization, compared with IRS-1(WT). Higher nuclear localization was also observed when cells expressing IRS-1(WT) were incubated with the proteasome inhibitor MG-132. The sequence of DIDI is conserved more than 93% across species, from fish to mammals, as opposed to approximately 40% homology of the entire IRS-1. These findings implicate DIDI as a novel, highly conserved domain of IRS-1, which mediates its cellular localization, rate of degradation, and biological activity, with a direct impact on insulin signal transduction.

Published

2010