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H C57BL6 genetic backgrounds had been employed in all of the experiments. The mice have been housed in plastic cages using a 12 h light/12 h dark cycle and free access to meals and water. The study mice have been euthanized with isoflurane, and the Animal Care and Use committee from the Sheba Healthcare Center, Tel-Hashomer, authorized all animal protocols. Diets Two industrial diets had been made use of: a non-purified, low-fat diet plan along with a semi-purified high-fat eating plan. To enrich the diet program with -carotene, we made use of powder on the alga Dunaliella bardawil containing six -carotene, comprised of 50 order SU-11274 all-trans and 50 9-cis isomers . In order to prepare the feed, 0.25 L of distilled hot water was mixed with 14 g of gelatin till the option was clear. Then, 1 kg of powdered feed and Dunaliella powder have been thoroughly mixed with the warm gelatin remedy. Just after solidification, the feed was divided into tablets and stored at -20C within the freezer; the feed was replaced each other day to minimize the oxidation and degradation of its ingredients. Study design and style Exp.1: Ten, 12-week-old male LDLR-/- mice have been allocated into two groups, five animals per group. The control group was fed a typical eating plan with no supplementations. The Dunaliella group was fed a diet regime fortified using the algal powder. Following four weeks of treatment, the mice had been injected with thioglycolate followed by the isolation of peritoneal macrophages. Exp.two: Ten, 12-week-old male LDLR-/- mice had been allocated into two groups, 5 animals per group. The control group was fed a high fat diet with no supplementations. The Dunaliella group was fed a high fat diet regime fortified together with the algal powder. Just after six weeks of remedy, the mice have been injected with thioglycolate followed by the isolation of peritoneal macrophages. Peritoneal macrophage production Mouse peritoneal macrophages were isolated as described previously. These isolated macrophages were counted and seeded at 1.5106 cells per ml. Tissue culture The cells were grown in DMEM 4.five g/L glucose containing ten FCS, 50 U/ml penicillin and 50 g/ml streptomycin. Two cell lines have been employed: Raw264.7, mouse macrophage cell line, enriched with 2 mM glutamine, purchased from ATCC; and Hepa1-6, mouse hepatoma cell line, enriched with 4 mM glutamine, purchased from ATCC. 3 / 15 Macrophage Foam Cell Inhibition by 9-Cis -Carotene For BCMO1 activity, the cells had been seeded in a one hundred mm plates, at 6106 cells per plate. Forty-eight hours following seeding, the cells have been treated with -carotene for 24 hours and analyzed for the presence of retinol. BCMO1 protein levels have been determined by western blot analysis. RAW 264.7 macrophage cells had been treated for 24 hours with car, 2 M of 9-cis -carotene or all-trans -carotene. The outcomes represent one of 5 independent experiments. Retinol, retinal and retinoic acid have been dissolved in DMSO having a final concentration of 0.five DMSO in the cell medium. -carotene was dissolved in hexane, and the concentration was determined by 450 nm absorbance, followed by the addition of tween40 in acetone to a total concentration of 0.1 tween within the cell medium. Finally, the solvents had been evaporated and also the residue was solubilized within the medium. The Dunaliella extraction was BMS-833923 supplier carried out by dissolving the alga powder in absolute ethanol, with all the addition of an identical volume of hexane and 1 mL of DDW. Right after 30 seconds of vortex spinning, the extract was centrifuged for five minutes at 2,000 g, and also the upper phase was separated for carotenoid concentration determination. Western.H C57BL6 genetic backgrounds were utilized in all the experiments. The mice have been housed in plastic cages with a 12 h light/12 h dark cycle and absolutely free access to food and water. The study mice have been euthanized with isoflurane, and the Animal Care and Use committee on the Sheba Health-related Center, Tel-Hashomer, authorized all animal protocols. Diets Two commercial diets had been applied: a non-purified, low-fat diet regime and a semi-purified high-fat diet regime. To enrich the diet with -carotene, we used powder of the alga Dunaliella bardawil containing 6 -carotene, comprised of 50 all-trans and 50 9-cis isomers . In an effort to prepare the feed, 0.25 L of distilled hot water was mixed with 14 g of gelatin till the solution was clear. Then, 1 kg of powdered feed and Dunaliella powder were thoroughly mixed with all the warm gelatin answer. Just after solidification, the feed was divided into tablets and stored at -20C in the freezer; the feed was replaced just about every other day to lessen the oxidation and degradation of its ingredients. Study style Exp.1: Ten, 12-week-old male LDLR-/- mice were allocated into two groups, 5 animals per group. The handle group was fed a common diet regime with no supplementations. The Dunaliella group was fed a eating plan fortified with all the algal powder. Right after four weeks of treatment, the mice have been injected with thioglycolate followed by the isolation of peritoneal macrophages. Exp.2: Ten, 12-week-old male LDLR-/- mice have been allocated into two groups, 5 animals per group. The handle group was fed a higher fat diet with no supplementations. The Dunaliella group was fed a higher fat diet plan fortified together with the algal powder. Just after six weeks of treatment, the mice have been injected with thioglycolate followed by the isolation of peritoneal macrophages. Peritoneal macrophage production Mouse peritoneal macrophages have been isolated as described previously. These isolated macrophages have been counted and seeded at 1.5106 cells per ml. Tissue culture The cells were grown in DMEM four.five g/L glucose containing ten FCS, 50 U/ml penicillin and 50 g/ml streptomycin. Two cell lines had been made use of: Raw264.7, mouse macrophage cell line, enriched with 2 mM glutamine, bought from ATCC; and Hepa1-6, mouse hepatoma cell line, enriched with four mM glutamine, purchased from ATCC. three / 15 Macrophage Foam Cell Inhibition by 9-Cis -Carotene For BCMO1 activity, the cells had been seeded inside PubMed ID:http://jpet.aspetjournals.org/content/124/1/16 a 100 mm plates, at 6106 cells per plate. Forty-eight hours just after seeding, the cells have been treated with -carotene for 24 hours and analyzed for the presence of retinol. BCMO1 protein levels have been determined by western blot analysis. RAW 264.7 macrophage cells have been treated for 24 hours with car, two M of 9-cis -carotene or all-trans -carotene. The results represent 1 of five independent experiments. Retinol, retinal and retinoic acid had been dissolved in DMSO having a final concentration of 0.five DMSO within the cell medium. -carotene was dissolved in hexane, and also the concentration was determined by 450 nm absorbance, followed by the addition of tween40 in acetone to a total concentration of 0.1 tween within the cell medium. Ultimately, the solvents had been evaporated and also the residue was solubilized within the medium. The Dunaliella extraction was carried out by dissolving the alga powder in absolute ethanol, together with the addition of an identical volume of hexane and 1 mL of DDW. Following 30 seconds of vortex spinning, the extract was centrifuged for five minutes at two,000 g, and also the upper phase was separated for carotenoid concentration determination. Western.

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Author: HMTase- hmtase