JC-1: alternative excitation wavelengths facilitate mitochondrial membrane potential cytometry

Perelman, Alexander; Wachtel, Chaim; Cohen, Meital; Haupt, Sara; Shapiro, Howard M.; Tzur, Amit

doi:10.1038/cddis.2012.171

Cited by 449 publications

(371 citation statements)

References 15 publications

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“…The mitochondrial membrane potential (DCm) in NSCs and NCs was measured by staining with the lipophilic cation JC-1. 23 As expected, long-term FR elevated the DCm in NCs (Fig. 3A, right panel).…”

Section: Long-term Fr Enhanced Mitochondrial Oxidative Phosphorylatiosupporting

confidence: 81%

A comparison of radiation-induced mitochondrial damage between neural progenitor stem cells and differentiated cells

et al. 2017

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Mitochondria play a key role in maintaining cellular homeostasis during stress responses, and mitochondrial dysfunction contributes to carcinogenesis, aging, and neurologic disease. We here investigated ionizing radiation (IR)-induced mitochondrial damage in human neural progenitor stem cells (NSCs), their differentiated counterparts and human normal fibroblasts. Long-term fractionated radiation (FR) with low doses of X-rays for 31 d enhanced mitochondrial activity as evident by elevated mitochondrial membrane potential (DCm) and mitochondrial complex IV (cytochrome c oxidase) activity to fill the energy demands for the chronic DNA damage response in differentiated cells. Subsequent reduction of the antioxidant glutathione via continuous activation of mitochondrial oxidative phosphorylation caused oxidative stress and genomic instability in differentiated cells exposed to longterm FR. In contrast, long-term FR had no effect on the mitochondrial activity in NSCs. This cell type showed efficient DNA repair, no mitochondrial damage, and resistance to long-term FR. After high doses of acute single radiation (SR) (> 5 Gy), cell cycle arrest at the G2 phase was observed in NSCs and human fibroblasts. Under this condition, increase in mitochondria mass, mitochondrial DNA, and intracellular reactive oxygen species (ROS) levels were observed in the absence of enhanced mitochondrial activity. Consequently, cellular senescence was induced by high doses of SR in differentiated cells.In conclusion, we demonstrated that mitochondrial radiation responses differ according to the extent of DNA damage, duration of radiation exposure, and cell differentiation.

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Section: Long-term Fr Enhanced Mitochondrial Oxidative Phosphorylatiosupporting

confidence: 81%

A comparison of radiation-induced mitochondrial damage between neural progenitor stem cells and differentiated cells

et al. 2017

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“…A polarized mitochondrial membrane draws additional dye into the mitochondrial membrane from the medium and reduces the fluorescence intensity of the suspension. Whereas if there is depolarization or any damage to the mitochondrial membrane potential dyes is released dye into the medium, increasing the overall fluorescence (Perelman et al 2012). Our results confirmed the anticancer potential of the tested compounds on Hep2 cells by increasing the fluorescence intensity, which was a direct confirmation of the mitochondrial damage and change in the mitochondrial membrane potential as the possible mechanism for the anticancer property of the tested compounds.…”

Section: Discussionsupporting

confidence: 82%

Synthesis and evaluation of selected 1,3,4-oxadiazole derivatives for in vitro cytotoxicity and in vivo anti-tumor activity

et al. 2016

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The oxadiazole moiety is known for its anticancer activity through its antiangiogenic and mitostatic potential. Taking this as a cue, the present study was designed to investigate the anti-cancer potential of selected oxadiazole derivatives. Twelve 1,3,4-oxadiazole derivatives (AMK OX-1 to AMK OX-12) were synthesized and were tested for IC 50 values through brine shrimp lethality assay and MTT assay on HeLa and A549 cell lines. Four compounds, AMK OX-8, 9, 11 and 12 showed potential cytotoxicity activity with low IC 50 value. These compounds produced considerable cytotoxic effect on Hep-2 and A549 cancer cell lines. However, they were found to be comparatively safer to normal cell lines, viz., V-79 cell lines than to the tested cancer cell lines, such as HeLa, A 549, and Hep2 cell lines. The mechanism of cytotoxicity was evaluated through nuclear staining and DNA ladder assay. Although DNA ladder assay showed DNA fragmentation (apoptotic phenomenon) in Hep-2 cells treated with only AMK OX-12, the staining procedures using acridine orange, ethidium bromide and propidium iodide showed apoptotic bodies in cells treated with AMK OX-8, 9 and 12 also. In JCI staining on isolated mitochondria of Hep2 cells, AMK OX-8, 9-11 and 12 displayed increasing fluorescence intensity with time which confirmed involvement of mitochondrial pathway and intrinsic pathway of apoptosis. All four compounds were found to be safe in acute oral toxicity study in Swiss albino mice. These derivatives were effective in reducing tumor size and weight in the in vivo DLA-induced solid tumor model. They were found to be significantly effective in reducing tumor volume and tumor weight.

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“…47 Briefly, JC-1 was added to reach a final concentration of 5 mg/ml and incubated for 20 min, and then the cells were washed twice with medium and imaged under a fluorescence microscope.…”

Section: Mitochondrial Membrane Potential Assay (Jc-1)mentioning

confidence: 99%

Autophagy impairment with lysosomal and mitochondrial dysfunction is an important characteristic of oxidative stress-induced senescence

et al. 2016

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Macroautophagy/autophagy has profound implications for aging. However, the true features of autophagy in the progression of aging remain to be clarified. In the present study, we explored the status of autophagic flux during the development of cell senescence induced by oxidative stress. In this system, although autophagic structures increased, the degradation of SQSTM1/p62 protein, the yellow puncta of mRFP-GFP-LC3 fluorescence and the activity of lysosomal proteolytic enzymes all decreased in senescent cells, indicating impaired autophagic flux with lysosomal dysfunction. The influence of autophagy activity on senescence development was confirmed by both positive and negative autophagy modulators; and MTOR-dependent autophagy activators, rapamycin and PP242, efficiently suppressed cellular senescence through a mechanism relevant to restoring autophagic flux. By time-phased treatment of cells with the antioxidant N-acetylcysteine (NAC), the mitochondria uncoupler carbonyl cyanide m-chlorophenyl hydrazone (CCCP) and ambroxol, a reagent with the effect of enhancing lysosomal enzyme maturation, we found that mitochondrial dysfunction plays an initiating role, while lysosomal dysfunction is more directly responsible for autophagy impairment and senescence. Interestingly, the effect of rapamycin on autophagy flux is linked to its role in functional revitalization of both mitochondrial and lysosomal functions. Together, this study demonstrates that autophagy impairment is crucial for oxidative stressinduced cell senescence, thus restoring autophagy activity could be a promising way to retard senescence.

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JC-1: alternative excitation wavelengths facilitate mitochondrial membrane potential cytometry

Cited by 449 publications

References 15 publications

A comparison of radiation-induced mitochondrial damage between neural progenitor stem cells and differentiated cells

A comparison of radiation-induced mitochondrial damage between neural progenitor stem cells and differentiated cells

Synthesis and evaluation of selected 1,3,4-oxadiazole derivatives for in vitro cytotoxicity and in vivo anti-tumor activity

Autophagy impairment with lysosomal and mitochondrial dysfunction is an important characteristic of oxidative stress-induced senescence

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