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Vol. 14, Issue 3, 1125-1137, March 2003

and
*Unité Mixte Recherche 7009, Centre National de la
Recherche Scientifique/Université Paris VI, Observatoire
Oceanologique de Villefranche sur Mer, 06234, Villefranche sur Mer,
France; and We have used complementary biochemical and in vivo approaches to
study the compartmentalization of M phase-promoting factor (MPF) in
prophase Xenopus eggs and oocytes. We first examined the
distribution of MPF (Cdc2/CyclinB2) and membranous organelles in
high-speed extracts of Xenopus eggs made during mitotic
prophase. These extracts were found to lack mitochondria, Golgi
membranes, and most endoplasmic reticulum (ER) but to contain the bulk
of the pre-MPF pool. This pre-MPF could be pelleted by further
centrifugation along with components necessary to activate it. On
activation, Cdc2/CyclinB2 moved into the soluble fraction. Electron
microscopy and Western blot analysis showed that the pre-MPF pellet
contained a specific ER subdomain comprising "annulate lamellae"
(AL): stacked ER membranes highly enriched in nuclear pores.
Colocalization of pre-MPF with AL was demonstrated by anti-CyclinB2
immunofluorescence in prophase oocytes, in which AL are positioned
close to the vegetal surface. Green fluorescent protein-CyclinB2
expressed in oocytes also localized at AL. These data suggest that
inactive MPF associates with nuclear envelope components just before
activation. This association may explain why nuclei and centrosomes
stimulate MPF activation and provide a mechanism for targeting of MPF
to some of its key substrates.
School of Biological Sciences,
University of Sussex, Falmer, Brighton, BN1 9QG, United Kingdom
Corresponding author. E-mail address:
houliston{at}obs-vlfr.fr.
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