10 results on '"Marco Milioli"'
Search Results
2. A Hybrid In Silico/In Vitro Target Fishing Study to Mine Novel Targets of Urolithin A and B: A Step Towards a Better Comprehension of Their Estrogenicity
- Author
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Margherita Interlandi, Angela Falco, Paola Puccini, Benedetta Riccardi, Chiara Dall'Asta, Abdelrahman Mohamed, Martin Frotscher, Daniele Del Rio, Marco Milioli, Luca Dellafiora, and Gianni Galaverna
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0301 basic medicine ,Models, Molecular ,17-Hydroxysteroid Dehydrogenases ,In silico ,Cell ,Computational biology ,Molecular Dynamics Simulation ,Ligands ,Estradiol Dehydrogenases ,03 medical and health sciences ,chemistry.chemical_compound ,Molecular level ,Coumarins ,medicine ,Humans ,Computer Simulation ,Estrogen Sulfotransferase ,Enzyme Inhibitors ,Beneficial effects ,030109 nutrition & dietetics ,Cell-Free System ,Chemistry ,Proteins ,In vitro ,Urolithin ,Molecular Docking Simulation ,030104 developmental biology ,medicine.anatomical_structure ,MCF-7 Cells ,Sulfotransferases ,Food Science ,Biotechnology ,Ellagic acid - Abstract
Scope Urolithin A and B are gut metabolites of ellagic acid and ellagitannins associated with many beneficial effects. Evidence in vitro pointed to their potential as estrogenic modulators. However, both molecular mechanisms and biological targets involved in such activity are still poorly characterized, preventing a comprehensive understanding of their bioactivity in living organisms. This study aimed at rationally identifying novel biological targets underlying the estrogenic-modulatory activity of urolithins. Methods and results The work relies on an in silico/in vitro target fishing study coupling molecular modeling with biochemical and cell-based assays. Estrogen sulfotransferase and 17β-hydroxysteroid dehydrogenase are identified as potentially subject to inhibition by the investigated urolithins. The inhibition of the latter undergoes experimental confirmation either in a cell-free or cell-based assay, validating computational outcomes. Conclusions The work describes target fishing as an effective tool to identify unexpected targets of food bioactives detailing the interaction at a molecular level. Specifically, it described, for the first time, 17β-hydroxysteroid dehydrogenase as a target of urolithins and highlighted the need of further investigations to widen the understanding of urolithins as estrogen modulators in living organisms.
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- 2020
3. Primary pulmonary arterial hypertension: Protocol to assess comprehensively in the rat the response to pharmacologic treatments
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Francesco De Logu, Romina Nassini, Deborah Novelli, Marcello Trevisani, Silvia Cantoni, Fabrizio Facchinetti, Ilaria Russo, Lidia Staszewsky, Sabina Ceriani, Marco Milioli, Serge Masson, Francesca Fumagalli, Teresa Letizia, Monica Salio, Daria De Giorgio, Giuseppe Ristagno, Roberto Latini, Roberta Massafra, and Davide Olivari
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medicine.medical_specialty ,Randomization ,Clinical Biochemistry ,Disease ,010501 environmental sciences ,01 natural sciences ,03 medical and health sciences ,chemistry.chemical_compound ,Dose finding ,Right ventricular systolic pressure ,Heart histology ,Internal medicine ,Medicine ,lcsh:Science ,Alanine transaminase ,030304 developmental biology ,0105 earth and related environmental sciences ,ComputingMethodologies_COMPUTERGRAPHICS ,Protocol (science) ,0303 health sciences ,Creatinine ,Monocrotaline ,business.industry ,Sample size ,Primary pulmonary arterial hypertension ,Medicine and Dentistry ,Morphometric analysis of pulmonary arteries ,Medical Laboratory Technology ,Cardiac biomarkers ,Blood pressure ,chemistry ,Echocardiography ,Cardiology ,Ventricular pressure ,lcsh:Q ,business - Abstract
Graphical abstract, The identification of new treatments for primary pulmonary arterial hypertension (PAH) is a critical unmet need since there is no a definitive cure for this disease yet. Due to the complexity of PAH, a wide set of methods are necessary to assess the response to a pharmacological intervention. Thus, a rigorous protocol is crucial when experimental studies are designed. In the present experimental protocol, a stepwise approach was followed in a monocrotaline-induced PAH model in the rat, moving from the dose finding study of treatment compounds to the recognition of the onset of disease manifestation, in order to identify when to start a curative treatment. A complete multidimensional evaluation of treatment effects represented the last step. The primary study endpoint was the change in right ventricular systolic pressure after 14 days of treatment; echocardiographic and biohumoral markers together with heart and pulmonary arterial morphometric parameters were considered as secondary efficacy and/or safety endpoints and for the evaluation of the biologic coherence in the different results.
- Published
- 2020
4. Monocrotaline-induced pulmonary arterial hypertension: Time-course of injury and comparative evaluation of macitentan and Y-27632, a Rho kinase inhibitor
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Francesco De Logu, Giuseppe Ristagno, Roberta Affatato, Fabrizio Facchinetti, Marco Milioli, Sabina Ceriani, Ilaria Russo, Silvia Cantoni, Roberto Latini, Davide Olivari, Marcello Trevisani, Teresa Letizia, Monica Salio, Francesca Fumagalli, Romina Nassini, Lidia Staszewsky, Serge Masson, Daria De Giorgio, and Deborah Novelli
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0301 basic medicine ,Endothelin Receptor Antagonists ,Male ,Pyridines ,Idiopathic Pulmonary Hypertension ,Heart Ventricles ,Vasodilation ,Pharmacology ,Pulmonary Artery ,03 medical and health sciences ,chemistry.chemical_compound ,0302 clinical medicine ,medicine.artery ,Medicine ,Animals ,Rats, Wistar ,Rho-associated protein kinase ,Protein Kinase Inhibitors ,Macitentan ,Pulmonary Arterial Hypertension ,Sulfonamides ,rho-Associated Kinases ,Monocrotaline ,Hypertrophy, Right Ventricular ,business.industry ,Endothelin receptor antagonist ,Hemodynamics ,medicine.disease ,Pulmonary hypertension ,Amides ,030104 developmental biology ,Pyrimidines ,chemistry ,Rho kinase inhibitor ,Pulmonary artery ,business ,030217 neurology & neurosurgery - Abstract
Novel pharmacological approaches are needed to improve outcomes of patients with idiopathic pulmonary hypertension. Rho-associated protein kinase (ROCK) inhibitors have shown beneficial effects in preclinical models of pulmonary arterial hypertension (PAH), because of their role in the regulation of pulmonary artery vasoconstrictor tone and remodeling. We compared a ROCK inhibitor, Y-27632, for the first time with the dual endothelin receptor antagonist, macitentan, in a monocrotaline-induced rat pulmonary hypertension model. Different methods (echocardiography, hemodynamics, histology of right ventricle and pulmonary vessels, and circulating biomarkers) showed consistently that 100 mg/kg daily of Y-27632 and 10 mg/kg daily of macitentan slowed the progression of PAH both at the functional and structural levels. Treatments started on day 14 after monocrotaline injection and lasted 14 days. The findings of all experimental methods show that the selective ROCK inhibitor Y-27632 has more pronounced effects than macitentan, but a major limitation to its use is its marked peripheral vasodilating action.
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- 2019
5. Comparative Evaluation of Two Different Modalities of Oral Delivery of Macitentan in Experimental Pulmonary Hypertension
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Fabrizio Facchinetti, M. Cont, A. Fioni, Fiorella Pastore, Marco Milioli, Stefano Cavalli, Silvia Cantoni, Gino Villetti, and F. Dardi
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medicine.medical_specialty ,chemistry.chemical_compound ,Modalities ,chemistry ,business.industry ,Medicine ,business ,Intensive care medicine ,medicine.disease ,Pulmonary hypertension ,Comparative evaluation ,Macitentan - Published
- 2019
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6. Downregulation of SLC7A7 Triggers an Inflammatory Phenotype in Human Macrophages and Airway Epithelial Cells
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Maria Di Lascia, Amelia Barilli, Valeria Dall'Asta, Rossana Visigalli, Paola Puccini, Bianca Maria Rotoli, Benedetta Riccardi, Filippo Ingoglia, and Marco Milioli
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0301 basic medicine ,lcsh:Immunologic diseases. Allergy ,Chemokine ,THP-1 Cells ,medicine.medical_treatment ,Immunology ,Interleukin-1beta ,Inflammation ,arginine ,Respiratory Mucosa ,Proinflammatory cytokine ,03 medical and health sciences ,0302 clinical medicine ,medicine ,Immunology and Allergy ,Humans ,Interleukin 8 ,Gene Silencing ,RNA, Small Interfering ,Renal Aminoacidurias ,Amino Acid Metabolism, Inborn Errors ,Chemokine CCL5 ,innate immunity ,Original Research ,A549 cell ,Innate immune system ,biology ,Chemistry ,Tumor Necrosis Factor-alpha ,Fusion Regulatory Protein 1, Light Chains ,Macrophages ,NF-kappa B ,Amino Acid Transport System y+L ,Cell biology ,030104 developmental biology ,Cytokine ,Phenotype ,A549 Cells ,inflammation ,030220 oncology & carcinogenesis ,Mutation ,biology.protein ,LPI ,Tumor necrosis factor alpha ,medicine.symptom ,lcsh:RC581-607 ,cytokine and chemokines - Abstract
Lysinuric protein intolerance (LPI) is a recessively inherited aminoaciduria caused by mutations of SLC7A7, the gene encoding y+LAT1 light chain of system y+L for cationic amino acid transport. The pathogenesis of LPI is still unknown. In this study, we have utilized a gene silencing approach in macrophages and airway epithelial cells to investigate whether complications affecting lung and immune system are directly ascribable to the lack of SLC7A7 or, rather, mediated by an abnormal accumulation of arginine in mutated cells. When SLC7A7/y+LAT1 was silenced in human THP-1 macrophages and A549 airway epithelial cells by means of short interference RNA (siRNA), a significant induction of the expression and release of the inflammatory mediators IL1β and TNFα was observed, no matter the intracellular arginine availability. This effect was mainly regulated at transcriptional level through the activation of NFκB signaling pathway. Moreover, since respiratory epithelial cells are the important sources of chemokines in response to pro-inflammatory stimuli, the effect of IL1β has been addressed on SLC7A7 silenced A549 cells. Results obtained indicated that the downregulation of SLC7A7/y+LAT1 markedly strengthened the stimulatory effect of the cytokine on CCL5/RANTES expression and release without affecting the levels of CXCL8/IL8. Consistently, also the conditioned medium of silenced THP-1 macrophages activated airway epithelial cells in terms of CCL5/RANTES expression due to the presence of elevated amount of proinflammatory cytokines. In conclusion, our results point to a novel thus far unknown function of SLC7A7/y+LAT1, that, under physiological conditions, besides transporting arginine, may act as a brake to restrain inflammation.
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- 2018
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7. An innovative method based on quick, easy, cheap, effective, rugged, and safe extraction coupled to desorption electrospray ionization-high resolution mass spectrometry for screening the presence of paralytic shellfish toxins in clams
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Monica Mattarozzi, Marco Milioli, Maria Careri, Federica Bianchi, and Antonella Cavazza
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Spectrometry, Mass, Electrospray Ionization ,Electrospray ,Time Factors ,Bacterial Toxins ,Chemical Fractionation ,Quechers ,01 natural sciences ,Analytical Chemistry ,Limit of Detection ,medicine ,Animals ,Shellfish ,Detection limit ,Microbial toxins ,Desorption electrospray ionization ,Chromatography ,010405 organic chemistry ,Chemistry ,010401 analytical chemistry ,Chemical fractionation ,Extraction (chemistry) ,Reproducibility of Results ,medicine.disease ,Bivalvia ,0104 chemical sciences ,Shellfish poisoning ,Safety ,Food Analysis - Abstract
The capabilities of desorption electrospray ionization-high resolution mass spectrometry (DESI-HRMS) were tested for screening the presence of some paralytic shellfish toxins in clams. A quick, easy, cheap, effective, rugged, and safe (QuEChERS) approach is proposed for sample clean-up. QuEChERS extraction was optimized by using a full factorial design followed by the multicriteria method of the desirability functions. Quantitation limits in the microgram per kilogram range proved reliability of the method for the detection of the investigated toxins in accordance to the rules laid down by European legislation. The optimized QuEChERS-DESI-HRMS based-method allowed for a rapid reliable screening of the investigated compounds at levels of interest, thus being useful for high-throughput analyses.
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- 2016
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8. Investigation of different sample pre-treatment routes for liquid chromatography–tandem mass spectrometry detection of caseins and ovalbumin in fortified red wine
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Monica Mattarozzi, Maria Careri, Chiara Bignardi, Marco Milioli, Lisa Elviri, and Claudio Corradini
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Pre treatment ,Wine ,Chromatography ,biology ,Chemistry ,Sample (material) ,Size-exclusion chromatography ,Mass spectrometry ,Winery ,Ovalbumin ,Liquid chromatography–mass spectrometry ,biology.protein ,Food Science ,Biotechnology - Abstract
Different sample treatment protocols for the liquid chromatography–electrospray-tandem mass spectrometry (LC–ESI-MS/MS) analysis of potential residuals of ovalbumin and caseins added to red wines were developed. In particular, attention was paid to the simultaneous detection and quantitation of fining agent residues, i.e. ovalbumin, α- and β-casein, in wine samples. The different sample treatment methods were compared in terms of protein recovery. The use of denaturing agents combined with size exclusion concentration and purification allowed to obtain a reproducible (RDS
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- 2014
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9. Quantitative proteomics analysis of platelet-derived microparticles reveals distinct protein signatures when stimulated by different physiological agonists
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Maria Careri, Simone Sidoli, Marco Milioli, María Ibáñez-Vea, Martin R. Larsen, and Giuseppe Palmisano
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Blood Platelets ,Proteomics ,Agonist ,Spectrometry, Mass, Electrospray Ionization ,Proteome ,medicine.drug_class ,Population ,Quantitative proteomics ,Biophysics ,Cell Communication ,Biochemistry ,Phosphates ,Thrombin ,Platelet degranulation ,Cell-Derived Microparticles ,Tandem Mass Spectrometry ,medicine ,Cluster Analysis ,Humans ,Platelet ,Platelet activation ,Databases, Protein ,education ,Cytoskeleton ,education.field_of_study ,Chemistry ,Proteins ,Platelet Activation ,Actins ,Cell biology ,Adenosine Diphosphate ,Collagen ,medicine.drug - Abstract
Platelet-derived MPs (PMPs) are a heterogeneous population of microvesicles released from platelets upon activation and apoptosis. Different platelet activations may affect PMP protein profiles and roles in intercellular communication. Here, we performed a quantitative proteomics study to characterize the protein content of PMPs generated by four differentially activated platelet samples. We selected known physiological agonists for platelet activation such as ADP, thrombin and collagen. Thrombin, which is mostly used to generate PMPs in vitro, was set as control. Platelets were activated by following a known agonist strength scale in which ADP was the weakest activation and thrombin and collagen stimulations were the strongest ones. Our proteomic analysis allowed the quantification of 3383 proteins, of which 428 membrane and 131 soluble proteins were found as significantly different in at least one of the analyzed conditions. Activation with stronger agonists led to the enrichment of proteins related to platelet activation in PMPs. In addition, proteins involved in platelet degranulation and proteins from the electron transport chain were less abundant in PMPs when stronger activation was used. Collectively, our data describe the most detailed characterization of PMPs after platelet physiological activation. Furthermore, we show that PMP protein content is highly dependent on the type of physiological agonist involved in platelet stimulation. Biological significance Platelet-derived MPs (PMPs) are a population of vesicles generated upon platelet activation by various stimuli known to be involved in several physiological and pathological processes. This manuscript investigates the protein profile of PMPs obtained by performing four different activation protocols using mass spectrometry-based quantitative proteomics. By following a known physiological agonist strength scale our findings suggest a biological link between agonist strength and proteins associated to platelet mediated processes such as activation and degranulation. These data may provide new insights for understanding PMP biological role and formation.
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- 2015
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10. Rapid desorption electrospray ionization-high resolution mass spectrometry method for the analysis of melamine migration from melamine tableware
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Federica Bianchi, Maria Careri, C. Cavalieri, Monica Mattarozzi, and Marco Milioli
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Electrospray ,Desorption electrospray ionization ,Chromatography ,Chemistry ,Analytical chemistry ,Plastic materials ,Context (language use) ,Orbitrap ,Analytical Chemistry ,law.invention ,chemistry.chemical_compound ,law ,Desorption ,Melamine ,Alert system - Abstract
Migration of melamine into foods from melamine tableware has been object of recent Rapid Alert System for Food and Feed (RASFF) notifications. In this context, a rapid and sensitive desorption electrospray ionization-high resolution mass spectrometry (DESI-HRMS) method was developed and validated for the determination of melamine migration from plastic materials. The migration test was performed using acetic acid 3% ( w / v ) as food simulant. Evaluation of DESI parameters in terms of choice of support, motion profile, geometrical configuration and operating conditions coupled to the use of an orbitrap mass analyzer allowed to achieve significant improvements in terms of selectivity and accuracy obtaining detection and quantitation limits at low microgram per kilogram level. A LC–ESI-MS method was also developed for confirmatory purposes. Both methods were applied to 44 melamine tableware samples available on Italian market in order to assess their compliance with the law. Different concentration levels ranging from 0.00773±0.0006 to 3.0±0.1 mg/kg were found after the third exposure to the simulant in new and used tableware with two samples out of 44 being characterized by a melamine release higher than the legal limit, i.e. 2.5 mg/kg. A two tailed t -test allowed to assess the good agreement between the quantitative results obtained applying the DESI-MS method with those provided by LC–ESI-MS, thus proving reliability of DESI-HRMS as rapid technique for the study of melamine release from plastic materials.
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- 2012
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