Ordering of ceramide formation, caspase activation, and mitochondrial changes during CD95- and DNA damage–induced apoptosis
Annemiek D. Tepper, Evert de Vries, Wim J. van Blitterswijk, Jannie Borst
Annemiek D. Tepper, Evert de Vries, Wim J. van Blitterswijk, Jannie Borst
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Article

Ordering of ceramide formation, caspase activation, and mitochondrial changes during CD95- and DNA damage–induced apoptosis

Abstract

To evaluate the role of ceramide (Cer) in apoptosis signaling, we examined Cer formation induced by CD95, etoposide, or γ-radiation (IR) in relation to caspase activation and mitochondrial changes in Jurkat T cells. The Cer response to all three stimuli was mapped in between caspases sensitive to benzoyloxycarbonyl-VAD-fluoromethylketone (zVAD-fmk) and acetyl-DEVD-aldehyde (DEVD-CHO). Cer production was independent of nuclear fragmentation but associated with the occurrence of other aspects of the apoptotic morphology. Caspase-8 inhibition abrogated Cer formation and apoptosis induced by CD95 but did not affect the response to etoposide or IR, placing CD95-induced Cer formation downstream from caspase-8 and excluding a role for caspase-8 in the DNA damage pathways. CD95 signaling to the mitochondria required caspase-8, whereas cytochrome c release in response to DNA damage was caspase-independent. These results indicate that the caspases required for the Cer response to etoposide and IR reside at or downstream from the mitochondria. Bcl-2 overexpression abrogated the Cer response to etoposide and IR and reduced CD95-induced Cer accumulation. We conclude that the Cer response to DNA damage fully depends on mitochondrion-dependent caspases, whereas the response to CD95 partially relies on these caspases. Our data imply that Cer is not instrumental in the activation of inducer caspases or signaling to the mitochondria. Rather, Cer formation is associated with the execution phase of apoptosis.

Authors

Annemiek D. Tepper, Evert de Vries, Wim J. van Blitterswijk, Jannie Borst

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Figure 1

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Etoposide and IR induce Cer formation and apoptosis. Jurkat T cells (J16...
Etoposide and IR induce Cer formation and apoptosis. Jurkat T cells (J16) labeled until equilibrium with [14C]serine were exposed to etoposide (10 μg/ml) or IR (30 Gy), or left untreated (medium). At the indicated times, Cer levels and apoptosis were determined. (a) TLC separation of Cer from dihydroceramide. Apoptosis is expressed as percentage of nuclei with subdiploid DNA content. (b) Time course of changes in Cer levels induced by etoposide or IR. Cer data are expressed as -fold increase relative to control and are representative of three experiments. The inset shows Cer levels (expressed relative to total radioactivity in phosphatidylserine and phosphatidylethanolamine) at shorter time points. Cer, ceramide; IR, γ-radiation.