Metallobiochemistry of ultratrace levels of bismuth in the rat II. Interaction of 205+206Bi3+ with tissue,intracellular and molecular components |
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| Affiliation: | 1. Center for Advanced Studies and Technology (C.A.S.T.), “G. d''Annunzio” University of Chieti-Pescara, Via Luigi Polacchi 11, Chieti, I-66100, Italy;2. Department of Physics, Università Degli Studi di Milano, Via Celoria 16, Milano, I-20133, Italy;3. LASA, Department of Physics, Università Degli Studi di Milano and INFN-Milano, Via F.lli Cervi 201, Segrate, MI, I-20090, Italy;4. Institute of Clinical Immunotherapy and Advanced Biological Treatments, Piazza Pierangeli 1, Pescara, Italy;5. Rectorate of Leonardo da Vinci Telematic University, Largo San Rocco 11 Torrevecchia, Teatina, CH, Italy;6. Department of Medicine and Aging Sciences, “G. d’Annunzio” University of Chieti-Pescara, via Luigi Polacchi 11, Chieti, I-66100, Italy;1. Istituto Zooprofilattico Sperimentale del Piemonte, Liguria e Valle d’Aosta, Chemistry Department, CReAA, via Bologna 148, Turin, Italy;2. ASL BI Local Veterinary Service Veterinary Biella, BI, Italy;1. Research Laboratory Education, Motricité, Sport et Santé, EM2S, LR19JS01, High Institute of Sport and Physical Education of Sfax, University of Sfax, 3000, Tunisia;2. Laboratory of Biochemistry, CHU Habib Bourguiba, University of Sfax, 3000, Tunisia;1. Univ. Grenoble Alpes, CEA, IRIG, 38000, Grenoble, France;2. Univ. Grenoble Alpes, INSERM U1055, Laboratory of Fundamental and Applied Bioenergetics (LBFA), and Environmental and System Biology (BEeSy), 38000, Grenoble, France;1. Centro de Pesquisa Clínica e Epidemiológica, Hospital Universitário, Universidade de São Paulo, São Paulo, Brazil;2. Department of Clinical, Toxicological and Bromatological Analyzes. ASTox - Laboratory of Analytical and Systems Toxicology, Faculty of Pharmaceutical Sciences of Ribeirão Preto, Universidade de São Paulo, São Paulo, Brazil;3. Department of Nutrition, School of Public Health, Faculdade de Saúde Pública, Universidade de São Paulo, Brazil;4. Faculdade de Medicina, Universidade Federal de Minas Gerais, Belo Horizonte, Minas Gerais, Brazil;5. Universidade Federal de São Paulo, São Paulo, Brazil;6. Thyroid Unit, Division of Endocrinology and Metabolism, Department of Medicine, Faculdade de Medicina de Marília, São Paulo, Brazil;7. Universidade Federal do Espírito Santo, Espírito Santo, Brazil;1. Saint-Petersburg Research Institute of Ear, Throat, Nose and Speech, St. Petersburg, Russia;2. I.I. Mechnikov North-Western State Medical University, St. Petersburg, Russia;3. K.A. Raukhfus Children''s City Multidisciplinary Clinical Center for High Medical Technologies, St. Petersburg, Russia;4. First Pavlov State Medical University of Saint Petersburg, St. Petersburg, Russia;5. National Center of Morphological Diagnostic, St. Petersburg, Russia;6. Institute of General Pathology and Pathophysiology, Moscow, Russia;7. I.M. Sechenov First Moscow State Medical University (Sechenov University), Moscow, Russia;8. K.G. Razumovsky Moscow State University of Technologies and Management, Moscow, Russia;9. Yaroslavl State University, Yaroslavl, Russia |
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| Abstract: | BackgroundKnowledge on Bi metabolism in laboratory animals refers to studies at “extreme” exposures, i.e. pharmacologically relevant high-doses (mg kg−1 b.w.) in relation to its medical use, or infinitesimal doses (pg kg−1b.w.) concerning radiobiology protection and radiotherapeutic purposes. There are no specific studies on metabolic patterns of environmental exposure doses (ultratrace level, μg kg−1 b.w.), becoming in this context Bi a “heavy metal fallen into oblivion”. We previously reported the results of the metabolic fate of ultratrace levels of Bi in the blood of rats [1]. In reference to the same study here we report the results of the retention and tissue binding of Bi with intracellular and molecular components.MethodsAnimals were intraperitoneally injected with 0.8 μg Bi kg−1 b.w. as 205+206Bi(NO)3, alone or in combination with 59Fe for the radiolabeling of iron proteins. The use of 205+206Bi radiotracer allowed the determination of Bi down to pg fg−1 in biological fluids, tissues, subcellular fractions, and biochemical components isolated by differential centrifugation, size exclusion chromatography, solvent extraction, precipitation, immunoprecipitation and dialysis.Main findingsAt 24 h post injection the kidney contained by far the highest Bi concentration (10 ng g−1 wt.w.) followed by the thymus, spleen, liver, thyroid, trachea, femur, lung, adrenal gland, stomach, duodenum and pancreas (0.1 to 1.3 ng g−1 wt.w.). Brain and testis showed smaller but consistently significant concentrations of the element (0.03 ng g−1 wt.w). Urine was the predominant route of excretion. Intracellularly, liver, kidney, spleen, testis, and brain cytosols displayed the highest percentages (35%–58%) of Bi of homogenates. Liver and testis nuclei were the organelles with the highest Bi content (24 % and 27 %). However, when the recovered Bi of the liver was recorded as percent of total recovered Bi divided by percent of total recovered protein the lysosomes showed the highest relative specific activity than in other fractions. In the brain subcellular fractions Bi was incorporated by neuro-structures with the protein and not lipidic fraction of the myelin retaining 18 % of Bi of the total homogenate. After the liver intra-subcellular fractionation: (i) 65 % of the nuclear Bi was associated with the protein fraction of the nuclear membranes and 35 % with the bulk chromatin bound to non-histone and DNA fractions; (ii) about 50 % of the mitochondrial Bi was associated with inner and outer membranes being the other half recovered in the intramitochondrial matrix; (iii) in microsomes Bi showed a high affinity (close to 90 %) for the membranous components (rough and smooth membranes); (iv) In the liver cytosol three pools of Bi-binding proteins (molecular size > 300 kDa, 70 kDa and 10 kDa) were observed with ferritin and metallothionein–like protein identified as Bi-binding biomolecules. Three similar protein pools were also observed in the kidney cytosol. However, the amount of Bi, calculated in percent of the total cytosolic Bi, were significantly different compared to the corresponding pools of the liver cytosol.ConclusionsAt the best of our knowledge the present paper represents the first in vivo study, on the basis of an environmental toxicology approach, aiming at describing retention and binding of Bi in the rat at tissue, intracellular and molecular levels. |
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| Keywords: | Bismuth Radioisotopes Environmental toxicology Metabolic pattern Rat tissues |
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