Redox environment in stem and differentiated cells: A quantitative approach

Lyublinskaya, O. G.; Ivanova, Ju. S.; Пуговкина, Н. А.; Kozhukharova, Irina; Kovaleva, Z. V.; Shatrova, A. N.; Aksenov, N. D.; Зенин, В. В.; Kaulin, Yu.A.; Gamaley, I. A.; Nikolsky, Nikolay

doi:10.1016/j.redox.2017.04.016

Cited by 63 publications

(43 citation statements)

References 66 publications

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“…To this end, eMSCs were stained with a fluorescein-containing cell-permeable probe 2′, 7′- dichlorodihydrofluorescein diacetate (H 2 DCFDA). H 2 DCFDA becomes fluorescent in the result of the multi-step intracellular oxidation process and is routinely used as a general indicator of the cellular redox-status 46,47 . Fluorescence signal measured with flow cytometer in the cells treated with the aforementioned AOs, excluding Tempol, was lower than that in the control cells (Fig.…”

Section: Resultsmentioning

confidence: 99%

High doses of synthetic antioxidants induce premature senescence in cultivated mesenchymal stem cells

Kornienko

Смирнова

Пуговкина

et al. 2019

Sci Rep

106

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Stress-induced premature senescence program is known to be activated in cells by various genotoxic stressors, and oxidative stress is considered to be the main of those. To this end, many studies discover antioxidants as protective anti-aging agents. In the current study, we examined the effects of different antioxidants (Tempol, resveratrol, NAC, DPI) on the mesenchymal stem cells maintained in normal physiological conditions. We used high, but non-cytotoxic antioxidant doses which are widely used in laboratory practice to protect cells from oxidative damage. We show that these substances induce reversible block of cell proliferation and do not cause any genotoxic effects when applied to the quiescent cells. However, the same doses of the same substances, when applied to the proliferating cells, can induce irreversible cell cycle arrest, DNA strand breaks accumulation and DNA damage response activation. As a consequence, antioxidant-induced DNA damage results in the stress-induced premature senescence program activation. We conclude that high doses of antioxidants, when applied to the proliferating cells that maintain physiological levels of reactive oxygen species, can cause DNA damage and induce premature senescence which suggests to re-estimate believed unconditional anti-aging antioxidant properties.

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Section: Resultsmentioning

confidence: 99%

High doses of synthetic antioxidants induce premature senescence in cultivated mesenchymal stem cells

Kornienko

Смирнова

Пуговкина

et al. 2019

Sci Rep

106

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“…To monitor the extracellular H 2 O 2 concentration in the course of kinetic measurements, Amplex ® Red Hydrogen Peroxide/Peroxidase Assay Kit (Invitrogen) was used in accordance with the procedure described in Ref. [11]. At H 2 O 2 concentration of 5 μM and cell density of 15 000 cells/ml, the decrease in H 2 O 2 concentration in the extracellular medium did not exceed several percent within 10 min after the peroxide addition to cells and therefore was neglected in the analysis of HyPer oxidation.…”

Section: Methodsmentioning

confidence: 99%

Measuring intracellular concentration of hydrogen peroxide with the use of genetically encoded H2O2 biosensor HyPer

Lyublinskaya

Antunes

2019

Redox Biology

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In this study, we propose a method for quantification of average hydrogen peroxide concentration within a living cell that is based on the use of genetically encoded H 2 O 2 biosensor HyPer. The method utilizes flow cytometric measurements of HyPer fluorescence in H 2 O 2 -exposed cells to analyze the biosensor oxidation kinetics. Fitting the experimental curves with kinetic equations allows determining the rate constants of HyPer oxidation/reduction which are used further for the calculation of peroxide concentrations in the cells of interest both in the presence and absence of external H 2 O 2 . Applying this method to K562 cells, we have estimated the gradient as about 390-fold between the extracellular and intracellular level of exogenous H 2 O 2 in cells exposed to the micromole doses of peroxide, as well as the average basal level of H 2 O 2 in the cytosol of undisturbed cells ( ). The method can be extended to other H 2 O 2 -sensitive redox probes or to procedures in which, rather than adding external peroxide, intracellular production of peroxide is triggered, providing a tool to quantitate not only basal average H 2 O 2 concentrations but also the concentration of peroxide build up in the vicinity of redox probes.

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“…Given that ESCs are characterized by low ROS level [33] , it is not surprising that HO-1 is not required for maintaining pluripotency. As such, we were able to establish HO-1 –/– ESCs displaying pluripotent markers ( Fig.…”

Section: Discussionmentioning

confidence: 99%

“…Furthermore, it is well recognized that redox homeostasis regulates stem cell renewal and differentiation [32] . ESCs are characterized by low reactive oxygen species (ROS) level and a low capacity to remove extracellular hydrogen peroxide, assessed by a quantitative redox biology approach [33] . During cardiomyocyte differentiation from ESCs, ROS levels are increased [34] .…”

Section: Introductionmentioning

confidence: 99%

Loss of heme oxygenase-1 accelerates mesodermal gene expressions during embryoid body development from mouse embryonic stem cells

et al. 2018

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Heme oxygenase (HO)-1 is an inducible stress response protein and well known to protect cells and tissues against injury. Despite its important function in cytoprotection against physiological stress, the role of HO-1 in embryonic stem cell (ESC) differentiation remains largely unknown. We showed previously that induced pluripotent stem (iPS) cells that lack HO-1 are more sensitive to oxidant stress-induced cell death and more prone to lose pluripotent markers upon LIF withdrawal. To elucidate the role of HO-1 in ESC differentiation and to rule out the controversy of potential gene flaws in iPS cells, we derived and established mouse HO-1 knockout ESC lines from HO-1 knockout blastocysts. Using wild type D3 and HO-1 knockout ESCs in the 3-dimensional embryoid body (EB) differentiation model, we showed that at an early time point during EB development, an absence of HO-1 led to enhanced ROS level, concomitant with increased expressions of master mesodermal regulator brachyury and endodermal marker GATA6. In addition, critical smooth muscle cell (SMC) transcription factor serum response factor and its coactivator myocardin were enhanced. Furthermore, HO-1 deficiency increased Smad2 in ESCs and EBs, revealing a role of HO-1 in controlling Smad2 level. Smad2 not only mediates mesendoderm differentiation of mouse ESCs but also SMC development. Collectively, loss of HO-1 resulted in higher level of mesodermal and SMC regulators, leading to accelerated and enhanced SMC marker SM α-actin expression. Our results reveal a previously unrecognized function of HO-1 in regulating SMC gene expressions during ESC-EB development. More importantly, our findings may provide a novel strategy in enhancing ESC differentiation toward SMC lineage.

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Redox environment in stem and differentiated cells: A quantitative approach

Cited by 63 publications

References 66 publications

High doses of synthetic antioxidants induce premature senescence in cultivated mesenchymal stem cells

High doses of synthetic antioxidants induce premature senescence in cultivated mesenchymal stem cells

Measuring intracellular concentration of hydrogen peroxide with the use of genetically encoded H2O2 biosensor HyPer

Loss of heme oxygenase-1 accelerates mesodermal gene expressions during embryoid body development from mouse embryonic stem cells

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