Ubiquitination as a Priming Process of PKC [alpha]and PKC [epsilon] Degradation in the [alpha]T3-1 Gonadotrope Cell Line

Background/Aim: Protein kinase C (PKC) is a family of isoenzymes playing a key role in the regulation of gonadotrope cell functions. Specific PKC isoforms are activated and downregulated differentially by gonadotropin-releasing hormone (GnRH) and the phorbol ester TPA. In the present study, focusing mainly on PKC [epsilon], the mechanisms underlying the proteasome-dependent downregulation of GnRH-activated PKC [epsilon] and TPA-sensitive PKC [alpha] and [epsilon] isoenzymes were investigated in [alpha]T3-1 gonadotrope cells. Methods/Results: In pull-down assays involving the use of glutathione-agarose affinity beads conjugated with a GST-fusion protein containing ubiquitin-associated domains of Rad23 that bind very likely to K48-linked polyubiquitinated proteins, TPA induced rapid (within 15 min) and sustained (up to 4 h) PKC [alpha] and PKC [epsilon] polyubiquitination. However, GnRH selectively elicited receptor-dependent polyubiquitination of PKC [epsilon], but not that of PKC [alpha]. The GnRH-evoked PKC [epsilon] polyubiquitination was a strong, fast process (taking place as early as 10 min) which decreased progressively with time (but was still detectable after 4 h of treatment). In addition, no apparent association between PKC [epsilon] and the lysosomal compartment was observed upon performing double-labeling immunofluorescence and confocal microscopy, after either 10 min or 1 hour of stimulation by GnRH or the phorbol ester. Conclusion: In [alpha]T3-1 gonadotrope cells, polyubiquitination is therefore the event triggering GnRH-evoked PKC [epsilon] desensitization as well as TPA-induced PKC [alpha] and PKC [epsilon] downregulations; it precedes the respective isoenzyme's degradation by the proteasome complex. Copyright © 2008 S. Karger AG, Basel [PUBLICATION ABSTRACT]