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SUPPLEMENTARY MATERIAL Extracts deriving from olive mill waste water and their effects on the liver of the goldfish Carassius auratus fed with hyperocholesterolemic diet Alessio Alescia, Nicola Ciceroa,*, Andrea Salvoa, Deborah Palombierib, Daniele Zacconea, Giacomo Dugoa, Maurizio Brunoc, Rossella Vadalàa, Eugenia Rita Laurianoa, and Simona Pergolizzia a Department of Environmental Sciences, Territorial, Food and Health Security (S.A.S.T.A.S.), Viale F. Stagno d’Alcontres 31, University of Messina, 98166 Messina, Italy b Department of Biological and Environmental Sciences, Viale Stagno d’Alcontres 31, University of Messina, 98166 Messina, Italy c Dipartimento di Scienze e Tecnologie Biologiche Chimiche e Farmaceutiche (STEBICEF), Università di Palermo, Viale delle Scienze, Parco d’Orleans II - 90128 Palermo, Italy Tissue preparation, histology and immunohistochemistry 15-20 goldfish (Carassius auratus) were used for the present study. The fishes were purchased from a business and kept in 8-liter aquaria under the experimental conditions of the laboratory for 30 days. They are then divided into four groups: the first group was fed with a cholesterol 10% enriched diet; the second group received a curative treatment, with a hypercholesterolemic diet and polyphenols, administered only in the last 15 days of treatment; the third group was fed with hypercholesterolemic diet with additional administration of polyphenol extracts from Olea europaea as a preventative treatment; finally, the fourth group normal-fed, was used as control. At the end of the experiment, the fishes were anesthetized with Ethyl 3-aminobenzoate methanesulfonate (MS) and we proceeded with the removal of organs of interest: liver. The samples were processed according to the techniques of sustainable construction preparations for light microscopy. They were then fixed in immunofix® (Bio-Optica, Milano, Italia) for two hours and dehydrated in ascending series of alcohols up to immersion in xylene. It was done with subsequent inclusion in Bioplast® (Bio-Optica, Milano, Italia) and microtome rotary cutting, resulting sections with a thickness of about 3-5 micrometers. The sections thus obtained were placed on glass slide and left in the oven for 48 hours. Then a morphological analysis was carried out by performing twotoned histological staining: hematoxylin-eosin, and histochemical staining: Periodic acid Schiff reaction, May Grunwald-Giemsa and Sirius Red. And even to confirmed this results , the research has made use of immunohistochemical techniques, testing CYP1A, S100 and α-Smooth with optic and confocal microscope for observation. Panel S1. H/E, 100x. a) Normal group; b) Hypercholesterolemic group: the epatocytes are irregular, it is evident cellular ballooning and lipid droplets, and centrilobular veins are alterated; c) Preventive group: it is evident the presence of lipocromics pigments; d) Curative group: histology tend to normal; PAS, 100x. e) Normal group; f) Hypercholesterolemic group; g) Preventive group; h) Curative group. Panel S2. Sirius Red, 100x. a) Normal group; b) Hypercholesterolemic group: the collagen is more present around centrilobular veins and in the gaps between hepatocytes, to prove a fibrotic condition; c) Preventive group; d) Curative group: in this group it s possible to observe a decreasing concentration of collagen to demonstrate positive effects of polyphenols. Panel S3. CYP1A, 100X. a) Normal group; b) Hypercholesterolemic group : it is evident the marking around centilobular veins and in some hepatocytes; c) Preventive group ; d) Curative group: the marking is absent to explain beneficial effect of polyphenols. Panel S4. May Grunwald-Giemsa, 100x. a) Normal group; b) Hypercholesterolemic group : there are many granulocytes to prove immune response to oxidative stress cholesterol-induced. c) Preventive group; d) Curative group: it is possible to observe a reduction of the number of granulocytes in response to effect of polyphenols. S-100, 100x. e) Normal group; f) Hypercholesterolemic group: the granulocytes are marking positively because they present a specific protein, calprotectin, that plays a role in flogosys and in immune response; g) Preventive group; h) Curative group: the reduction of granulocytes shows a morphological condition that tend to normal. Panel S5. α – SMOOTH ACTINE. Peroxidase, 100x. a) Normal group; b) Hypercholesterolemic group: alteration of centrilobular veins demonstrate presence of a inflammatory condition marked with specific antibody of smooth muscle of endothelium; c) Preventive group; d) Curative group. Fluorescence, 100x. e) Normal group; f) Hypercholesterolemic group; g) Preventive group; h) Curative group. This results confirm data obtained with peroxidase, explaining and proving alteration of veins to response to oxidative stress cholesterol-induced at level of smooth muscle of endothelium in centrilobular veins.