The cytoskeleton of digitonin-treated rat hepatocytes.

Fiskum, Gary; Craig, Susan W.; Decker, Glenn L.; Lehninger, Albert L.

doi:10.1073/pnas.77.6.3430

Cited by 218 publications

(145 citation statements)

References 24 publications

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“…To prevent the potential reverse transport of dopamine and thus "trap" cytosolic dopamine inside the cell, cultures were continuously exposed to the DAT inhibitor, mazindol. Cytosolic dopamine was then extracted using a mild, selective permeabilization of the plasma membrane with the steroid glycoside, digitonin (Fiskum et al, 1980). Using this digitonin-based permeabilization technique we extracted the cytosolic dopamine fraction from rat postnatal VM neurons transduced with VMAT2 overexpressing or VMAT2 silencing lentiviral vectors.…”

Section: 4mentioning

confidence: 99%

Vesicular monoamine transporter 2 regulates the sensitivity of rat dopaminergic neurons to disturbed cytosolic dopamine levels

Vergo¹,

Johansen²,

Leist³

et al. 2007

Brain Research

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A B S T R A C TAn abnormal accumulation of cytosolic dopamine resulting in reactive oxygen species and dopamine-quinone products may play an important role in the rather selective degeneration of substantia nigra pars compacta (SNc) dopaminergic neurons in Parkinson's disease. The neuronal-specific vesicular monoamine transporter (VMAT2), responsible for uptake of dopamine into vesicles, has been shown to play a central role both in intracellular dopamine homeostasis and sequestration of dopaminergic neurotoxins. Direct or indirect enhancement of VMAT2 activity could therefore have neuroprotective effects by decreasing cytosolic dopamine levels. Here, we demonstrate that transfection of VMAT2 in the dopaminergic cell line, PC12, increases intracellular dopamine content, augments potassium-induced dopamine release and attenuates cell death induced by the cytosolic dopamine enhancer, methamphetamine, suggesting an enhancement in vesicular dopamine storage. In rat ventral mesencephalic cultures highly enriched for dopaminergic neurons, lentiviral delivery of recombinant VMAT2 using a neuronal-specific promoter also resulted in elevated intracellular dopamine content and neurotransmitter release after depolarization. The opposite was seen after downregulation of VMAT2 using virally delivered shRNAs. Furthermore, using this VMAT2 knockdown model, we are the first to report a direct link between enhanced cytoplasmic dopamine levels, measured following mild permeabilization of the plasma membrane using digitonin, and neurite degeneration in primary dopaminergic neurons. In conclusion, our data support the hypothesis that an increase in vesicular sequestration of dopamine by modulation of VMAT2 activity could restore neuronal function and enhance dopaminergic cell survival in conditions of dysregulated dopamine homeostasis such as Parkinson's disease.

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Section: 4mentioning

confidence: 99%

Vesicular monoamine transporter 2 regulates the sensitivity of rat dopaminergic neurons to disturbed cytosolic dopamine levels

Vergo¹,

Johansen²,

Leist³

et al. 2007

Brain Research

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“…Mitochondrial and cytoplasmic enzyme fractions were separated by a digitonin method as described in Fiskum et al (13). Individual embryos were incubated in a 500-nl drop of enzyme extraction buffer (12), supplemented with 0.001% digitonin, for 2 min.…”

Section: Media-mentioning

confidence: 99%

Mitochondrial Malate-Aspartate Shuttle Regulates Mouse Embryo Nutrient Consumption

Lane

Gardner

2005

Journal of Biological Chemistry

107

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Pyruvate has been considered the sole substrate that can support development of the mouse zygote to the two-cell stage, with lactate able to support development from the two-cell stage. This study has determined for the first time that mitochondrial reducing equivalent shuttles regulate metabolism in the early embryo. Activity of the malate-aspartate shuttle was found to be essential for the metabolism of lactate in the two-cell embryo. Furthermore, the inability of the mouse zygote to use lactate as an energy source was a result of a lack of malate-aspartate shuttle activity. The mRNA for the four enzymes for shuttle activity were detected at all stages of development. It was determined that aspartate was a rate-limiting factor in the activity of the malate-aspartate shuttle in mouse zygotes probably due to the high K m of the cytoplasmic aspartate aminotransferase. Addition of high concentrations of exogenous aspartate to the culture medium enabled mouse zygotes to utilize lactate in the absence of pyruvate and develop normally to the blastocyst stage as well as produce normal viable offspring. This study determined that the malateaspartate shuttle is a key regulator of embryo metabolism and therefore viability and is the first report that mouse zygotes can develop normally to term in the absence of pyruvate.Studies on the preimplantation mouse embryo have indicated that the zygote has an absolute requirement for pyruvate to complete the first cleavage division (1-3). Significantly, lactate is only able to support development from the two-cell stage (4), and glucose could support development from the eight-cell stage (5). Interestingly, mouse zygotes can metabolize both pyruvate and lactate (6, 7) even though cleavage only occurs in the presence of pyruvate. While this has been documented for more than 30 years, there is no explanation for this unusual pattern of metabolism at the zygote nor is it known what changes occur in the embryo that enable the two-cell embryo to use lactate to support development.Energy metabolism in cells is compartmentalized to either the cytoplasm or the mitochondria. Pyruvate is transported into the mitochondria by specific transport proteins and is metabolized within the mitochondria. In contrast, lactate is converted to pyruvate within the cytosol with the concomitant conversion of NAD ϩ to NADH. Cells must maintain a balance of metabolic intermediates between the cytosol and the mitochondria to enable lactate metabolism to continue. An inability to maintain this balance results in impairment of either mitochondrial and/or cytoplasmic metabolism. In addition to many enzymes existing in either the cytoplasm or mitochondria, the pyridine nucleotides (NAD ϩ , NADH, NADP ϩ , and NADPH) are also compartmentalized between the cytoplasm and the mitochondria. Intact mitochondria are impermeable to NADH (8). Therefore to transfer NADH across the mitochondrial membrane for oxidation and ATP production and for the regeneration of cytoplasmic NAD ϩ , there is an indirect pathway involving th...

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“…Protein extracts were prepared by selective plasma membrane permeabilization with digitonin to allow for separation of cytoplasmic, mitochondrial, and nuclear+membrane components according to a published protocol (Fiskum et al, 1980). Brie¯y, cells were washed in isotonic sucrose buer (250 mM sucrose, 10 mM KCl, 1.5 mM MgCl 2 , 1 mM EDTA, 1 mM EGTA, 10 mM HEPES, pH 7.1, plus protease inhibitors 1 mg/ml leupeptin, 2 mg/ml aprotinin, and 0.5 mM PMSF) and subsequently incubated for 1 min at room temperature in 100 ml of the same buer to which 0.05% digitonin has been added, followed by 10 min of centrifugation at 48C.…”

Section: Immuno Blot Analysismentioning

confidence: 99%

Characterization of distinct consecutive phases in non-genotoxic p53-induced apoptosis of Ewing tumor cells and the rate-limiting role of caspase 8

et al. 2000

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To dissect the p53-dependent apoptotic pathway, events following induction of temperature sensitive (ts) p53val138 were studied in a Ewing tumor cell line. Transcriptional deregulation of p53 targets ®rst observable after 1 h at 328C preceded activation of caspases and the break-down of mitochondrial respiratory activity. Activation of caspases was ®rst observed 4 h after p53 induction. Using peptide inhibitors we identi®ed activation of caspase 8 upstream of caspases-9 and -3. Although the caspase 8 speci®c inhibitor z-IETD.fmk did not aect translocation of BAX to the mitochondrial membrane and cytochrome C release it almost completely blocked cleavage of the prototype caspase substrate PARP and DNA fragmentation while enforcing mitochondrial depolarization and production of reactive oxygene species (ROS). Activation of caspase 8 did not involve death-domain receptor signaling. Expression of BCL2 only partially suppressed caspase activation but blocked apoptosis. Replacement of the Nterminus of p53val138 by the related VP16 transactivation domain created a ts p53 with a tanscriptional activity indistinguishable from p53val138 until the time of caspase activation. However, the VP16 ± p53 fusion failed to trigger caspases and subsequent induction of the ROS producing gene pig3 paralleled by complete loss of apoptotic activity. These results indicate that p53-dependent transcriptional deregulation, triggering of the caspase cascade and the mitochondrial break-down occur in a timely ordered sequence coordinated by the genuine p53 amino terminus and suggest caspase 8 and PIG3 as key regulatory elements in this process. Oncogene (2000) 19, 4096 ± 4107.

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The cytoskeleton of digitonin-treated rat hepatocytes.

Cited by 218 publications

References 24 publications

Vesicular monoamine transporter 2 regulates the sensitivity of rat dopaminergic neurons to disturbed cytosolic dopamine levels

Vesicular monoamine transporter 2 regulates the sensitivity of rat dopaminergic neurons to disturbed cytosolic dopamine levels

Mitochondrial Malate-Aspartate Shuttle Regulates Mouse Embryo Nutrient Consumption

Characterization of distinct consecutive phases in non-genotoxic p53-induced apoptosis of Ewing tumor cells and the rate-limiting role of caspase 8

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