Modulation of intracellular GSH in THP-1 cells during oxidative stress induced by AAPH

Brown, Erin

January 2006

The human monocyte-derived THP-1 cell line was incubated with 10mM AAPH in Earle’s Balanced Salt Solution at 37°C for up to 24 hours. Protein hydroperoxide formation occurred after an 8 hour lag phase which corresponded to glutathione loss observed in the cells. SDS-Page analysis confirmed protein degradation occurred after 6 hours. Cell viability measured by the MTT reduction assay also dropped after 8 hours. Reduction of intracellular glutathione levels using BSO caused reduction of the lag phase seen in protein hydroperoxide formation. Cell viability of BSO-treated cells was lower than control cells, indicating the initiation of apoptotic events. Flow cytometry analysis showed no difference between BSO-treated and control cells, indicating that GSH levels do not have an effect on the type of cell death observed in AAPH-induced oxidative damage on THP-1 cells. These results confirmed previous data in the lab suggesting THP-1 cells undergo AAPH-induced necrosis as a result of cellular damage, including the loss of GSH and the formation of protein hydroperoxides.

monocyte-derived THP-1 cell

incubated

AAPH

modulation

Modulation of intracellular GSH in THP-1 cells during oxidative stress induced by AAPH

Brown, Erin

January 2006

The human monocyte-derived THP-1 cell line was incubated with 10mM AAPH in Earle’s Balanced Salt Solution at 37°C for up to 24 hours. Protein hydroperoxide formation occurred after an 8 hour lag phase which corresponded to glutathione loss observed in the cells. SDS-Page analysis confirmed protein degradation occurred after 6 hours. Cell viability measured by the MTT reduction assay also dropped after 8 hours. Reduction of intracellular glutathione levels using BSO caused reduction of the lag phase seen in protein hydroperoxide formation. Cell viability of BSO-treated cells was lower than control cells, indicating the initiation of apoptotic events. Flow cytometry analysis showed no difference between BSO-treated and control cells, indicating that GSH levels do not have an effect on the type of cell death observed in AAPH-induced oxidative damage on THP-1 cells. These results confirmed previous data in the lab suggesting THP-1 cells undergo AAPH-induced necrosis as a result of cellular damage, including the loss of GSH and the formation of protein hydroperoxides.

monocyte-derived THP-1 cell

incubated

AAPH

modulation

Experimental Approach for Drug Profiling of Calcitriol in Yeast

Jagadeesan, Sasi Kumar

January 2016

Vitamin D regulation is associated with several human disorders and contributes to various cellular mechanisms. Calcitriol (commercially available as Rocaltrol), an active Vitamin D metabolite, is known as a neuro-protective and anti-cancer drug but most importantly helps maintaining the calcium homeostasis inside the human body. The effectiveness of calcitriol to perform as an effective therapeutic agent is counteracted by its calcemic effects. In order to obtain better therapeutic results, synthetic calcitriol analogs without these calcemic effects have been recently developed but they are not yet cost-effective and their production is time-consuming. In order to determine the best active form of calcitriol that could provide higher chemotherapeutic activity without these calcemic effects, calcitriol mode of action was studied using yeast as a model system. In order to achieve this, we analyzed the calcitriol effects on yeast cellular growth based on calcium intake levels. In this work, we also assessed yeast strains with gene deletions of selected calcium transporter genes to understand the calcitriol metabolism. For the aim of understanding hypercalcemic effects of calcitriol, we developed a hypothesis based on calcitriol interactions with oxygen. Interestingly, use of an anaerobic model validated the oxygen interactions with calcitriol that might possibly cause calcemic effects on patients. Anaerobically grown yeast treated with calcitriol showed significantly less intracellular calcium levels when imaged under indo-1 calcium binding fluorescence dye as compared to calcitriol treated yeast grown under aerobic conditions. Finally, we predict that calcitriol might control free radical generation within the yeast system based on experiments with AAPH and UV- irradiation.

calcitriol

calcium interactions

AAPH

UV-irradiation

Hypercalcemic effects

Yeast system

Effects of polyphenolic-rich bark extracts of Burkea africana and Syzygium cordatum on oxidative stress

Cordier, Werner

23 November 2012

Free radicals have been implicated in the progression of various diseases, such as cancers and cardiomyopathies. When the body is overburdened with free radicals and endogenous antioxidants become depleted, oxidative stress ensues with resultant damage to biomolecules. During oxidative stress high levels of reactive oxygen species are generated, cellular viability decreases, and apoptosis and lipid peroxidation are induced. Supplementation with exogenous supplements rich in antioxidants, such as herbal remedies containing polyphenols, could result in increased protection against oxidative stress. The aim of the study was to assess the effect of Burkea africana and Syzygium cordatum in a cellular oxidative stress model for the potential development of an antioxidant supplement. Crude aqueous and methanolic extracts were prepared by solvent maceration, while a polyphenolic-rich extract was created through liquid-liquid extraction. Polyphenolic content and antioxidant activity was assessed in cell-free systems. Polyphenolic content was determined through the Folin-Ciocalteau and aluminium trichloride methods, while antioxidant activity was assessed by the Trolox Equivalence Antioxidant Capacity and 1,1-diphenyl-2-picrylhydrazyl radical assays. Identification of phytochemical classes was done through thin layer chromatography and biochemical reactions. Inherent cytotoxicity of samples was determined in four cell cultures (3T3-L1 pre-adipocytes, C2C12 myoblasts, normal human dermal fibroblasts and U937 macrophage-like cells) using the neutral red uptake assay. The effect on oxidative stress was assessed in 2,2`-azobis-(2-methylpropionamidine) dihydrochloride-exposed U937 macrophage-like cells with regards to reactive oxygen species generation, cytotoxicity, apoptosis, lipid peroxidation and GSH depletion. Both B. africana and S. cordatum showed enrichment of polyphenols from the aqueous extract, to methanolic extract, to polyphenolic-rich extract. Antioxidant activity showed the same trend, which correlated well with the increased concentration of polyphenols, such as catechin, gallic acid and myricetin. Samples indicated toxicity in the 3T3-L1 and C2C12 cell lines, though no toxicity was noted in the U937 cell line and normal human dermal fibroblast cultures. Free radical-induced generation of reactive oxygen species, cytotoxicity, lipid peroxidation and apoptosis was successfully reduced by crude extracts of B. africana and the polyphenolic-rich extracts of both plants between concentrations of 10 and 20 ìg/ml. The crude extracts of S. cordatum were mostly ineffective in reducing these parameters, even though cell viability was increased. B. africana pre-treatment decreased reduced glutathione concentrations significantly in a dose-dependent manner, while the methanolic and polyphenolic-rich extract of S. cordatum increased concentrations moderately. Polyphenolic-rich extracts of B. africana and S. cordatum had the most potent decrease in oxidative stress-related parameters in the present study, which could be attributed to the polyphenolic content and antioxidant activity. Limited cytotoxicity was apparent in two of the four cell lines tested; further isolation and purification needs to be carried out to assess the bioactive constituents which do not elicit a toxic response. Further investigation through the use of quantitative structure–activity relationship modeling could give more insight on conformational and chemical changes that need to be brought about to modify the bioactive phytochemicals for reduced cytotoxicity, but increased antioxidant activity. Copyright / Dissertation (MSc)--University of Pretoria, 2013. / Pharmacology / unrestricted

Syzygium cordatum

Reactive oxygen species

Polyphenols

Oxidative stress

Lipid peroxidation

Glutathione

Aaph

Antioxidant

Apoptosis

Burkea africana

UCTD