Glucose deprivation increases nuclear DNA repair protein Ku and resistance to radiation induced oxidative stress in human cancer cells

Li, Jie; Ayene, Roashan; Ward, Kathleen; Dayanandam, Eswarkumar; Ayene, Iraimoudi S.

doi:10.1002/cbf.1541

Cited by 20 publications

(17 citation statements)

References 41 publications

(64 reference statements)

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“…The intracellular non protein thiol (NPSH) was determined by DTNB assay as described previously (Li et al, 2009). Cells in the dish with the desired medium were rinsed twice and the attached cells were mixed with 1 ml of ice cold 50 mM SSA buffer.…”

Section: Methodsmentioning

confidence: 99%

“…This modification of the Active Motif nuclear extract preparation is necessary to avoid the reversal of HEDS mediated oxidation of protein thiols including Ku protein thiols by DTT (Ayene et al 2002). The nuclear proteins were prepared by membrane disruption using Active Motif hypotonic buffer, detergent and complete lysis buffer and centrifugation as per the manufacturer’s instructions (Li et al, 2009). The nuclear proteins were stored at −80°C.…”

Section: Methodsmentioning

confidence: 99%

“…In cancer cells, this question has intensified with direct evidence that steady-state concentrations of glucose are significantly reduced in solid tumors (Aronen et al, 2000; Izuishi et al, 2000; Rajendran et al, 2004). Unlike cells in normal tissue, where glucose deprivation is injurious, cancer cells in solid tumors can often adapt to glucose-deprivation induced oxidative stress by mechanisms that also permit them to acquire therapeutiuc resistance (Kato et al, 2002; Lee 2001; Li et al, 2009; Park et al, 2007; Wyld et al, 2002; Yun et al, 2005). While the effects of glucose deprivation have received significant attention, the specific role of glucose deprivation without the confounding effects of other nutrient, growth factors and oxygen depletion on the cellular control of thiol homeostasis and its subsequent effects on protein function, cell survival and response to free radicals induced oxidative stress have not been demonstrated in either cancer or normal cells.…”

Section: Introductionmentioning

confidence: 99%

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A bioactive probe of the oxidative pentose phosphate cycle: Novel strategy to reverse radioresistance in glucose deprived human colon cancer cells

Ward

Zhang

et al. 2013

Toxicology in Vitro

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The specific effects of glucose deprivation on oxidative pentose phosphate cycle (OPPC) function, thiol homeostasis, protein function and cell survival remain unclear due to lack of a glucose-sensitive chemical probe. Using p53 wild type and mutant human colon cells, we determined the effects of hydroxyethyl disulfide (HEDS) on NADPH, GSH, GSSG, total glutathione, total non-protein and protein thiol levels, the function of the DNA repair protein Ku, and the susceptibility to radiation-induced free radicals under normal glucose or glucose-deprived conditions. HEDS is rapidly detoxified in normal glucose but triggered a p53-independent metabolic stress in glucose depleted state that caused loss of NADPH, protein and non protein thiol homeostasis and Ku function, and enhanced sensitivity of both p53 wild type and mutant cells to radiation induced oxidative stress. Additionally, high concentration of HEDS alone induced cell death in p53 wild type cells without significant effect on p53 mutant cells. HEDS offers a useful tool to gain insights into how glucose metabolism affects OPPC dependent stress-induced cellular functions and injury, including in tumor cells, where our findings imply a novel therapeutic approach to target glucose deprived tumor. Our work introduces a novel probe to address cancer metabolism and ischemic pathology.

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Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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A bioactive probe of the oxidative pentose phosphate cycle: Novel strategy to reverse radioresistance in glucose deprived human colon cancer cells

Ward

Zhang

et al. 2013

Toxicology in Vitro

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“…Some other proteins related to DNA damage were also downregulated in HUVEC treated with 400 mol/L elaidic acid, such as XRCC 5 (spot (23)), PSME 3 (spot (3)), and SAE 1 (spot (20)). XRCC 5 , a subunit of the Ku heterodimer protein, played a major role in cellular resistance to radiation [52]. However, the expression of P53 was increased ( Figure 5); this indicated that the DNA damage level was increased.…”

Section: Effect Of Elaidicmentioning

confidence: 99%

Potential Pathways Involved in Elaidic Acid Induced Atherosclerosis in Human Umbilical Vein Endothelial Cells

Liang

et al. 2017

Journal of Chemistry

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Researches have demonstrated that trans-fatty acids are related to the progression of atherosclerosis, but the underlying mechanism is not clear till now. In the presented study, two-dimensional electrophoresis based proteomics was used to discover the role of elaidic acid in atherosclerosis. In human umbilical vein endothelial cells (HUVEC), twenty-two and twenty-three differentially expressed proteins were identified in low (50 mol/L) and high (400 mol/L) concentration elaidic acid simulated groups, respectively, comparing with the control group. The expressions of some selected proteins (PSME 3 , XRCC 5 , GSTP 1 , and GSTO 1 ) were validated by qRT-PCR analysis. Western blotting analysis further confirmed that elaidic acid downregulated the expression of PSME 3 and XRCC 5 . Moreover, P53, the downstream protein of PSME 3 , was further investigated. Results demonstrated that a variety of proteins, many of which were related to oxidative stress, apoptosis, and DNA damage, were involved in the elaidic acid induced atherosclerosis. Furthermore, P53 was demonstrated to regulate the atherosclerosis through cell cycle arrest and apoptosis pathway.

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“…We have recently demonstrated in a series of publications that GSH recycling (GSH → GSSG (oxidized GSH) → GSH), which is dependent on several GSH dependent pathways, is required for the metabolic conversion of hydroxyethyldisulfide (HEDS) into mercaptoethanol (ME) (Ayene, Biaglow, Kachur, Stamato, & Koch, 2008; Ayene, et al, 2000; Ayene, et al, 2002; Biaglow, et al, 2003; Biaglow, et al, 2000; Biaglow, et al, 2006; Biaglow, et al, 1998; Li, Ayene, Ward, Dayanandam, & Ayene, 2009; Li, et al, 2013; Li, Zhang, Ward, Prendergast, & Ayene, 2012; Tuttle, et al, 2007). Unlike all the previous assays that measured just the glutathione level, a functional assay for glutathione such as HEDS metabolism will measure the “GSH dependent antioxidant capacity” of cells, a process that requires “glutathione recycling” by oxidative pentose phosphate cycle (OPPC) in conjunction with other GSH dependent pathways (Ayene, et al, 2002; Biaglow, et al, 2003; Lushchak, 2012).…”

Section: Introductionmentioning

confidence: 99%

A bioactive probe for glutathione-dependent antioxidant capacity in breast cancer patients: Implications in measuring biological effects of arsenic compounds

Zhang

Jefferson

et al. 2014

Journal of Pharmacological and Toxicological Methods

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Introduction Glutathione, a major cellular non-protein thiol (NPSH), serves a central role in repairing damage induced by cancer drugs, pollutants and radiation and in the detoxification of several cancer chemotherapeutic drugs and toxins. Current methods measure glutathione levels only, which require cellular extraction, rather than the glutathione recycling dependent antioxidant activity in intact cells. Here, we present a novel method using a bioactive probe of the oxidative pentose phosphate cycle, termed the OxPhos™ test, to quantify glutathione recycling dependent antioxidant activity in whole blood and intact human and rodent cells without the need for the isolation and cytoplasm extraction of cells. Methods OxPhos™ test kit (Rockland Immunochemicals, USA), which uses hydroxyethyldisulfide (HEDS) as a probe for the oxidative pentose phosphate cycle, was used in these studies. The results with OxPhos™ test kit in human blood and intact cells were compared with total thiol and high pressure liquid chromatography/electrochemical detection of HEDS metabolism. Results The OxPhos™ test measured glutathione-dependent antioxidant activity both in intact human and rodent cells and breast cancer patient’s blood with a better correlation coefficient and biological variability than the thiol assay. Additionally, human blood and mammalian cells treated with various arsenicals showed a concentration-dependent decrease in activity. Discussion The results demonstrate the application of this test for measuring the antioxidant capacity of blood and the effects of environmental pollutants/toxins. It opens up new avenues for an easy and reliable assessment of glutathione-dependent antioxidant capacity in various diseases such as stroke, blood borne diseases, infection, cardiovascular disease and other oxidative stress related diseases and as a prognostic indicator of chemotherapy response and toxicity. The use of this approach in pharmacology/toxicology including screening drugs that improve the glutathione-dependent antioxidant capacity and not just the glutathione level is clinically relevant since mammalian cells require glutathione dependent pathways for antioxidant activity.

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Glucose deprivation increases nuclear DNA repair protein Ku and resistance to radiation induced oxidative stress in human cancer cells

Cited by 20 publications

References 41 publications

A bioactive probe of the oxidative pentose phosphate cycle: Novel strategy to reverse radioresistance in glucose deprived human colon cancer cells

A bioactive probe of the oxidative pentose phosphate cycle: Novel strategy to reverse radioresistance in glucose deprived human colon cancer cells

Potential Pathways Involved in Elaidic Acid Induced Atherosclerosis in Human Umbilical Vein Endothelial Cells

A bioactive probe for glutathione-dependent antioxidant capacity in breast cancer patients: Implications in measuring biological effects of arsenic compounds

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