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1 Department of Pharmacology and Cancer Biology, Duke University Medical Center, Durham, NC 27710
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0 |+ V8 K* A8 y. q) b2 Department of Molecular Genetics, University of Texas M.D. Anderson Cancer Center, Houston, TX 77030
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w4 ]: B. @( ]" ^; b0 ?3 Department of Pathology, Stanford University School of Medicine, Stanford, CA 94305
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4 Department of Microbiology and Immunology, Stanford University School of Medicine, Stanford, CA 94305
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/ {! ~. V7 J* f. X- L0 C v! x5 Cancer Research UK, Clare Hall Laboratories, South Mimms, Herts EN6 3LD, England, UK, k8 J5 W' B3 S( Z7 w( C
5 B5 m% Y8 W/ N* U4 SDegradation of specific protein substrates by the anaphase-promoting complex/cyclosome (APC) is critical for mitotic exit. We have identified the protein Xenopus nuclear factor 7 (Xnf7) as a novel APC inhibitor able to regulate the timing of exit from mitosis. Immunodepletion of Xnf7 from Xenopus laevis egg extracts accelerated the degradation of APC substrates cyclin B1, cyclin B2, and securin upon release from cytostatic factor arrest, whereas excess Xnf7 inhibited APC activity. Interestingly, Xnf7 exhibited intrinsic ubiquitin ligase activity, and this activity was required for APC inhibition. Unlike other reported APC inhibitors, Xnf7 did not associate with Cdc20, but rather bound directly to core subunits of the APC. Furthermore, Xnf7 was required for spindle assembly checkpoint function in egg extracts. These data suggest that Xnf7 is an APC inhibitor able to link spindle status to the APC through direct association with APC core components.
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Abbreviations used in this paper: APC, anaphase-promoting complex/cyclosome; CRS, cytoplasmic retention sequence; CSF, cytostatic factor; IAP, inhibitor of apoptosis; RRL, rabbit reticulocyte lysate; Xnf7, Xenopus nuclear factor 7.
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- L6 I7 l$ {1 h4 X2 eIntroduction
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Key events in mitosis such as sister chromatid separation and inactivation of the cyclin-dependent kinase Cdc2 are regulated by the anaphase-promoting complex/cyclosome (APC), a large multisubunit ubiquitin ligase that promotes ubiquitylation and proteasomal degradation of its substrates (Zachariae and Nasmyth, 1999; Harper et al., 2002; Peters, 2002). Although the APC was originally identified as a cyclin B ubiquitin ligase (Irniger et al., 1995; King et al., 1995; Sudakin et al., 1995), it has since been shown to ubiquitylate numerous cell cycle regulatory proteins including cyclin A, securin, Xkid1, Cdc20, Plk1, and Ase1, as well as regulatory proteins involved in other cellular processes such as transcription and development (Hershko and Ciechanover, 1998; Peters, 2002).
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5 p) G- p" {9 l# h+ d, aThe APC is present throughout the cell cycle, but its activity is highly regulated. It is active from prometaphase until late G1, and inactive in S phase and G2 when cyclin B accumulates. Activation of the APC is controlled in part by phosphorylation of at least three of its subunits (Cdc16, Cdc23, and Cdc27) by the mitotic kinases Cdk1/cyclin B and Plk1 (Kotani et al., 1998; Rudner and Murray, 2000; Golan et al., 2002). However, the relative importance of these two kinases in the direct phosphorylation of the APC remains unclear, as data suggesting both kinases (Golan et al., 2002), only Plk1 (Kotani et al., 1998), or only Cdk1 (Rudner and Murray, 2000; Kraft et al., 2003) directly phosphorylate the APC have yet to be reconciled. APC activation is also controlled by the binding of activators, the WD40-repeat–containing proteins Cdc20 and Cdh1. In somatic cells, Cdc20 and Cdh1 binding to the APC is regulated, resulting in a peak in APCCdc20 activity in anaphase and APCCdh1 activity in G1 (Fang et al., 1998b; Zachariae et al., 1998; Kramer et al., 2000). Until recently, it was thought that Cdh1 was not expressed in the early Xenopus laevis embryo, and that only APCCdc20 was active (Lorca et al., 1998). A recent paper suggests, however, that Cdh1 is present in stage VI oocytes, and that it might have a role during the first meiotic cell cycle (Papin et al., 2004). Although the widely accepted model for the role of Cdc20/Cdh1in APC activation defines these proteins as essential for substrate recognition (Burton and Solomon, 2001; Pfleger et al., 2001; Schwab et al., 2001), several recent studies have shown that the core subunits of the APC, rather than Cdc20/Cdh1, are directly responsible for substrate recognition (Meyn et al., 2002; Passmore et al., 2003; Yamano et al., 2004) and that Cdc20/Cdh1 are required for activation of the APC in a still undefined manner.0 Z& u% k0 r9 E3 F, E4 \" f4 i
: x8 E, [+ s# C' l4 tTight regulation of the APC is critical to ensure the appropriate sequential destruction of APC substrates during the cell cycle. For example, cyclin A is degraded during prometaphase, and securin, Xkid1, and cyclin B are destroyed at the metaphase–anaphase transition (Funabiki and Murray, 2000; den Elzen and Pines, 2001; Geley et al., 2001). During anaphase and telophase, APCCdh1 is activated and mediates the destruction of Plk1, Ase1, and Cdc20 (Juang et al., 1997; Shirayama et al., 1998). The precise sequence of degradative events that must occur to ensure the proper timing of mitosis suggests that additional factors control the timing of APC-mediated ubiquitylation. One such factor is Emi1 (early mitotic inhibitor 1), an inhibitor of the APC that binds directly to Cdc20 to prevent premature APC activation (Reimann et al., 2001). Another recently reported APC inhibitor, XErp1 (Xenopus Emi1 related protein 1), also prevents premature APCCdc20 activation, although the mechanism of inhibition remains unknown (Schmidt et al., 2005).; J5 p/ k9 K6 y7 t
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APCCdc20 activity is also regulated by the spindle checkpoint, a mechanism that is critical for the maintenance of genomic stability and acts by delaying sister chromatid separation until all chromosomes are properly attached to the mitotic spindle (Amon, 1999; Shah and Cleveland, 2000; Yu, 2002). Upon activation of the checkpoint at unattached kinetochores, checkpoint protein complexes containing BubR1, Bub3, and Mad2 bind to and inhibit the APC activator Cdc20 (Fang et al., 1998a; Hwang et al., 1998; Sudakin et al., 2001; Tang et al., 2001; Fang, 2002). Recent studies show that not only are the spindle checkpoint proteins and Cdc20 spatially regulated but that spindle checkpoint components are required to recruit the APC to kinetochores, suggesting that the APC could be regulated directly by the spindle checkpoint (Acquaviva et al., 2004; Vigneron et al., 2004).# f$ X9 e6 y+ V4 _. [! d; F6 P6 B
* d @7 G4 C; }: V* [' F0 ~ gMuch of our knowledge of cell cycle progression has emerged from studies in model systems, including yeast and X. laevis. Here, we have used the Xenopus egg extract, in which APC regulation has been extensively analyzed. Unfertilized Xenopus eggs are arrested in metaphase of meiosis II due to the stabilization of cyclin B by an activity known as cytostatic factor (CSF; Tunquist and Maller, 2003). Crushing the eggs by centrifugation releases intracellular Ca2 stores, activating calcium/calmodulin-dependent protein kinase II and triggering APC activation and degradation of cyclin B (Lorca et al., 1993). However, preparing extracts in the presence of EGTA prevents the activation of calcium/calmodulin-dependent protein kinase II, allowing high levels of cyclin B to remain and arresting extracts in meiosis. These CSF-arrested extracts can then be released from their meiotic state by addition of Ca2 , leading to activation of the APC and progression into interphase.& `6 d; T" c3 X1 T, ~6 ~
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In performing experiments designed to identify novel cyclin B2 interactors from Xenopus egg extracts that might regulate its function, we have uncovered an additional APC inhibitor, Xenopus nuclear factor 7 (Xnf7). Xnf7 was originally cloned during a screen for proteins that accumulate in embryonic nuclei during the midblastula transition (Reddy et al., 1991). Xnf7 is a maternally expressed protein found in oocyte nuclei. After release into the cytoplasm during maturation, where it remains throughout the early embryonic cell divisions, it reenters nuclei at the midblastula transition. El-Hodiri et al. (1997b) demonstrated that Xnf7 plays a role in dorso-ventral patterning of the Xenopus embryo, but no specific molecular function has been shown to account for this phenotype.
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1 X- r% {9 x! C! GHere, we demonstrate that Xnf7 has the unexpected ability to inhibit APC function. Although we isolated Xnf7 via its affinity for cyclin B2, Xnf7 appears to have universal effects on APC-dependent ubiquitylation. Immunodepletion of Xnf7 from CSF-arrested egg extracts accelerates the degradation of cyclin B1, cyclin B2, and securin upon addition of Ca2 , thereby accelerating the transition to interphase. Moreover, we demonstrate that Xnf7 itself has intrinsic ubiquitin ligase activity, and that this activity is required for inhibition of the APC. Unlike previously identified inhibitors of APCCdc20 (e.g., Mad2 and Emi1), Xnf7 does not inhibit APCCdc20 activity via direct binding to Cdc20, but rather appears to act independently of Cdc20 via association with a core APC subunit. We also find that Xnf7 is required for the spindle assembly checkpoint in egg extracts. Collectively, our data suggest that Xnf7 inhibits APC activation in a manner distinct from known APC regulators, likely via interaction with a core APC subunit.
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Results
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Xnf7 binds to the cyclin B2 cytoplasmic retention sequence (CRS)
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( g4 d; t u( y: P; ^0 Z3 {( TPrevious work from our laboratory and others has demonstrated that the subcellular localization of cyclins B1 and B2 is controlled by a region of the cyclin proteins known as the CRS (Pines and Hunter, 1994). However, the CRSs of these two cyclins differ significantly. The cyclin B1 CRS contains a Crm1-binding nuclear export sequence that promotes nuclear export of cyclin B1 throughout interphase and is inactivated by phosphorylation to allow nuclear accumulation at the onset of mitosis (Yang et al., 1998; Hagting et al., 1999). In contrast, the cyclin B2 CRS lacks a classical nuclear export sequence and may serve to anchor cyclin B2 in the cytoplasm (Jackman et al., 1995). The cyclin B2 CRS, when injected into Xenopus oocytes, has also been reported to promote formation of monopolar rather than bipolar spindles, suggesting that this region might interact with proteins important for spindle polarity (Yoshitome et al., 1998). Therefore, we sought to purify novel factors interacting with the cyclin B2 CRS. Upon passage of Xenopus egg extract over a column of immobilized recombinant cyclin B2 CRS protein (amino acids 94 to 204), we observed a prominent band of 80 kD bound specifically to the cyclin B2 CRS (Fig. 1 A). Analysis by mass spectrometry identified this band as Xnf7., P' g( B6 X2 w) y. f
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Depletion of Xnf7 accelerates the ubiquitylation of APC substrates and mitotic exit4 N" o9 a/ q9 M* X! g* [. H5 m) o0 C
% w3 K. m" A6 k" X" WGiven the previously reported effects of the cyclin B2 CRS on spindle polarity, we sought to determine if Xnf7 had a discernible role in spindle formation. Toward this end, we produced anti-Xnf7 antibodies for immunodepletion from Xenopus egg extracts. Affinity-purified Xnf7 antibodies recognized a protein of 80 kD in Xenopus XTC lysates and Xenopus interphase and CSF-arrested egg extracts, whereas preimmune IgG did not (Fig. 1 B). Antibodies also recognized recombinant Xnf7 and in vitro translated Xnf7, but did not detect a protein in unprogrammed rabbit reticulocyte lysate (RRL; Fig. 1 C).
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8 ~+ e1 b$ @2 W" mImmunodepletion of Xnf7 from interphase or CSF extracts was accomplished with three sequential depletions (Fig. 1 D). The absence of Xnf7 had no detectable effect on bipolar spindle formation, cyclin B2 localization, or DNA replication (unpublished data). However, we found that CSF extracts immunodepleted of Xnf7 behaved in an unexpected manner. Specifically, when Xnf7-depleted CSF extracts were released into interphase by Ca2 , we found that they transited from the CSF-arrested state to interphase considerably more rapidly than mock-depleted (control) extracts, reforming interphase nuclei 40–50 min after Ca2 addition compared with 60–80 min in control extracts (unpublished data). (Note that to start with a high level of Cdc2/cyclin B activity and monitor its decline, extracts were first incubated at room temperature for 30 min before Ca2 was added.) Consistent with this observation, depletion of Xnf7 accelerated the degradation of cyclin B1, cyclin B2, and securin (Fig. 1, E and F). The extracts shown in Fig. 1 (E and F) are distinct, and the timing of exit from CSF arrest shown here is representative of the timing observed in numerous experiments. Although the absolute timing of exit differed between extracts, the relative rates of exit under different treatment conditions remained constant.: g- q( c- y; y6 y+ S/ c
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Because CSF extracts are arrested in metaphase of meiosis II, and therefore have characteristics distinct from extracts that mimic the first embryonic M phase (Tunquist and Maller, 2003), we sought to determine whether depletion of Xnf7 accelerated exit from an extract prepared so as to recapitulate the first embryonic mitosis or if this acceleration was unique to the meiotic cell cycle. To this end, we prepared CSF extracts, immediately added Ca2 (without prior room temperature incubation, thereby promoting a more rapid release from the arrest), and monitored meiotic exit and exit from the following mitosis. As expected, Xnf7-depleted extracts progressed to interphase more rapidly than control extracts, degrading cyclin B by 10 min (compared with 20 min; Fig. 2 A) and reforming nuclei at 20 min (compared with 30 min; unpublished data). Once in the subsequent mitosis, cyclin B degradation (Fig. 2 B, 140 min) and nuclear reformation (Fig. 2 C, 160 min) in depleted extracts proceeded ahead of control extracts, suggesting that Xnf7 affects mitotic exit as well as meiotic exit. We also observed that depletion of Xnf7 from CSF extracts did not cause spontaneous release from CSF arrest without the addition of Ca2 (Fig. 2 D), nor did the depletion of Xnf7 from interphase extracts induce spontaneous degradation of mitotic substrates (Fig. 2 E). Therefore, Xnf7 is not required for maintenance of the CSF arrest. Moreover, depletion of Xnf7 appeared to alter the rate of cyclin B degradation rather than the lag time until initiation of degradation in that both Xnf7-depleted and mock-depleted extracts appeared to initiate degradation immediately after Ca2 addition to CSF extracts.
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After finding that immunodepletion of Xnf7 accelerates the degradation of all APC substrates examined, we wanted to determine whether this effect was specific to APC substrates or if the absence of Xnf7 affected the degradation of other proteins, perhaps causing a global acceleration of proteasome-mediated degradation. To evaluate the effect of Xnf7 immunodepletion on the degradation of a non-APC substrate, we examined an inhibitor of apoptosis (IAP), a protein that does not exhibit distinct cell cycle–regulated turnover. IAPs are E3 ubiquitin ligases that can autoubiquitylate in vivo, marking themselves for destruction by the 26S proteasome (Yang et al., 2000). IAP autoubiquitylation and accelerated proteasomal degradation can be triggered by binding the proapoptotic protein reaper (Holley et al., 2002). Examination of IAP protein levels in control and Xnf7-depleted extracts supplemented with reaper revealed that IAP was degraded at nearly the same rate in the presence or absence of Xnf7 (Fig. 3 A), suggesting that the acceleration of degradation in the absence of Xnf7 was not universal and was likely specific to APC substrates. Together, these data indicated that either Xnf7 or associated codepleted proteins acted to suppress APC activation.; t8 G2 ?' n; ?) p: x" z# E
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To determine if removal of Xnf7 itself, rather than associated proteins, contributed to accelerated APC activation, we examined the effect of anti-Xnf7 antibody addition to extracts. Before Ca2 addition, we treated CSF extracts with preimmune IgG, anti-Xnf7 antibodies, or anti-Xnf7 antibodies blocked with recombinant Xnf7 protein. Extracts treated with anti-Xnf7 antibodies exited meiosis more rapidly (as observed by microscopy) and degraded cyclin B more rapidly than extracts treated with preimmune IgG. Moreover, the effects of the anti-Xnf7 antibodies were neutralized by treatment with recombinant Xnf7 (Fig. 3 B, left; unpublished data). Note that addition of anti-Xnf7 antibodies did not alter the amount of Xnf7 in the extract (Fig. 3 B, right). Together with the effects of immunodepletion, these data suggested that Xnf7 protein antagonized APC-mediated substrate degradation. To address this issue further, we tested the ability of recombinant wild-type Xnf7 (Xnf7WT) protein to restore the "normal" timing of meiotic exit in extracts from which Xnf7 had been immunodepleted.
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# I" x5 @- f. o- V; RAfter depletion, CSF extracts were treated with buffer or Xnf7WT for 30 min at room temperature before Ca2 addition. As expected, Xnf7-depleted extracts degraded cyclin B more rapidly than control extracts (Fig. 3 C). Addition of recombinant Xnf7 to depleted extracts restored the normal timing of APC-mediated substrate degradation, slowing cyclin B degradation to a rate similar to that observed in mock-depleted extracts. These data reinforce our conclusion that Xnf7 protein has an inhibitory effect on APC-mediated substrate degradation. Because addition of recombinant Xnf7WT could complement the inhibitory activity of the endogenous protein, we reasoned that the addition of excess recombinant Xnf7WT to egg extracts might delay or even prevent exit from CSF arrest. To examine the effect of increasing the Xnf7 concentration in the extract, we added buffer or Xnf7WT to CSF extracts before Ca2 addition. Although the control extract reformed interphase nuclei 30 min after Ca2 addition, Xnf7WT addition caused a meiotic arrest. Accordingly, cyclin B was destroyed by 12 min after Ca2 addition in control extract, and was stabilized by addition of Xnf7WT (Fig. 3 D). These results implicate Xnf7 as an APC regulator and suggest that it is the removal of Xnf7, not a codepleting protein, that leads to accelerated APC-mediated substrate degradation and mitotic exit./ V& L) `6 F7 h8 Q
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To further confirm that Xnf7 inhibited mitotic exit at the level of ubiquitylation of APC substrates, not at the level of degradation by the 26S proteasome, we repeated the experiment described in the previous paragraph in the presence of methyl-ubiquitin to "trap" cyclin B in its ubiquitylated form. Although cyclin B ubiquitylation peaked at 10–12 min in the control extract, Xnf7WT addition delayed this peak (Fig. 3 E, 16–20 min). Moreover, cyclin B was eventually destroyed in the control extract (presumably due to ubiquitylation with endogenous ubiquitin following the action of deubiquitylating enzymes) but was stabilized by the addition of Xnf7WT.
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* ~: \2 z; i% B" a% U! kXnf7 is a ubiquitin ligase& V: T6 |, K- M/ D2 G
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In analyzing the Xnf7 sequence, Reddy et al. (1991) noted the presence of two putative zinc-binding domains and speculated that Xnf7 might be a transcription factor. However, as one zinc-binding region contains a consensus sequence typical of RING domains found in ubiquitin ligases, we suspected that Xnf7 might function as a ubiquitin ligase (Fig. 4 A). Accordingly, we performed in vitro ubiquitylation assays using purified E1, E2 (UbcH5a), ubiquitin, and recombinant Xnf7 as the only source of E3 activity. In addition to testing Xnf7WT, we constructed Xnf7 RING finger mutants in which conserved cysteine residues that coordinate zinc binding were replaced by alanine. Xnf7 mutant 3 (Xnf7m3) contained a mutation at position 3 of the RING finger (C160A) and Xnf7 mutant 36 (Xnf7m36) contained mutations at positions 3 and 6 (C160A and C168A; Fig. 4 A). As with many ubiquitin ligases in vitro, Xnf7WT was able to autoubiquitylate, converting the single electrophoretic form of Xnf7 into a polyubiquitylated form (Fig. 4 B). Mutation of the RING finger inhibited this activity. We note that Xnf7 was not able to ubiquitylate cyclin B or securin proteins directly (unpublished data), and that Xnf7 cannot use UbcH10, the ubiquitin-conjugating enzyme that functions with the APC, as a source of E2 in the autoubiquitylation reaction (Fig. 4 C, left). Note that all E2 enzymes were functional in E2-thioester assays (Fig. 4 C, right; unpublished data).
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Given that Xnf7 has intrinsic ubiquitin ligase activity, we sought to determine whether or not this activity was required for its effects on mitotic exit. We therefore compared the effects of Xnf7WT or Xnf7m36 addition to extracts. As previously shown in Fig. 3 D, addition of excess Xnf7WT prevented cyclin B degradation and mitotic exit. Addition of Xnf7m36 did not stabilize cyclin B; rather, cyclin B was degraded (Fig. 4 D), demonstrating that Xnf7's ligase activity is required for its effects on mitotic exit. Indeed, addition of excess Xnf7m36 actually accelerated cyclin B degradation relative to buffer-treated control extracts, suggesting that this mutant protein may act in a dominant-negative fashion to antagonize the effects of endogenous Xnf7 (Fig. 4 E). In the presence of methyl-ubiquitin, cyclin B ubiquitylation peaked at 12–16 min after Ca2 addition in the Xnf7m36-treated extract, whereas Xnf7WT addition slowed ubiquitylation of cyclin B, delaying the peak until 20 min (Fig. 4 F). As expected, cyclin B was destroyed eventually in the Xnf7m36-treated extract but was stabilized by Xnf7WT.
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' E9 |* y4 g' {4 q! u8 G& nXnf7 inhibits the APC0 d* C% u' e2 H4 b. b2 C! Q
/ f% P# B! i( a0 h7 o QTo determine if the inhibitory effect of Xnf7 was exerted directly on the APC, APC was immunopurified from mitotic egg extracts using anti-Cdc27 antibodies and treated with recombinant Xnf7WT. APC inhibitors Mad2 and Emi1 have been shown previously to inhibit the APC in this manner via their interactions with Cdc20 (Fang et al., 1998a; Reimann et al., 2001). As shown in Fig. 5 A, addition of Cdc20 to APC immunoprecipitates activated the APC, promoting ubiquitylation of cyclin B. Preincubation of Cdc20 with MBP-Emi1 significantly inhibited the APC; however, preincubation with recombinant Xnf7WT or Xnf7m36 had no discernible effect.+ I% T/ o: D e
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Because we had clearly observed an effect of Xnf7 on APC function in extracts (containing a full complement of cellular components) and Xnf7's enzymatic activity was required for its effect on mitotic exit (Fig. 4, D and F), we reasoned that the inhibitory effect of Xnf7 on the APC might be evident only under conditions that would allow Xnf7 to function as a ubiquitin ligase. (Note that the in vitro Xnf7 ubiquitylation assay was performed using UbcH5a and that the purified APC assay contained only UbcH10. Xnf7 does not function as a ligase with UbcH10 [Fig. 4 C, left].) To this end, UbcH5a was added during the incubation of Xnf7 with APC immunoprecipitates to create conditions permissive for Xnf7's enzymatic activity. Whereas Xnf7WT alone failed to inhibit the APC (Fig. 5 B, lane 2), Xnf7WT incubated under ubiquitylating conditions did, indeed, inhibit the purified APC (Fig. 5 B, lane 3). In contrast, Xnf7m36 protein did not inhibit the APC (Fig. 5 B, lane 4), consistent with a requirement for Xnf7's enzymatic activity in its direct inhibition of the APC. The presence of Xnf7 in the assay did not prevent Cdc20 from binding to the APC (unpublished data).$ f1 {# J6 K8 t3 D$ E
4 w1 e a+ m$ x8 C9 |Xnf7 interacts with a core subunit of the APC
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Given the inhibitory effects of Xnf7 on the activity of the APC, we sought to determine how Xnf7 might be exerting its effects. To investigate the potential association of Xnf7 with the APC, we separated CSF extracts on 10–40% sucrose gradients and examined the sedimentation of Xnf7, APC subunits Apc2 and Cdc27/Apc3, and the APC activator Cdc20. Xnf7 was found mainly in lower molecular mass fractions of 100–250 kD (Fig. 6 A, fractions 2–7) along with Cdc20 (Fig. 6 A, fractions 2–6), but peaked again with the 1.5-MD APC complex in fraction 11, where APC subunits Apc2 and Cdc27/Apc3 also sedimented (Fig. 6 A). Although a considerable amount of Xnf7 did not cosediment with APC components, Xnf7 immunoprecipitations from selected cosedimenting fractions (Fig. 6 A, *) revealed that Cdc27/Apc3 coimmunoprecipitated with Xnf7 from APC-containing fractions but that Cdc20 did not coimmunoprecipitate (Fig. 6 B), even in fractions where they were both abundantly represented. Similarly negative results were obtained when fractions were immunoprecipitated with anti-Cdc20 antibodies and immunoblotted with anti-Xnf7 antibodies (unpublished data). These data strongly suggest that Xnf7 acts in a manner distinct from previously reported APC regulators, most likely through direct interaction with a core APC subunit. That being said, we note that Xnf7 coimmunoprecipitated equally well with Cdc27 from CSF extracts before and after Ca2 addition, suggesting that Xnf7 functions other than binding (possibly ubiquitin ligase activity) are required for Xnf7-mediated APC inhibition (Fig. 6 C).
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9 I5 e% U: o2 vXnf7 is required for the spindle assembly checkpoint7 [$ o& e$ `6 X) ?, a# I
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Given the ability of Xnf7 to inhibit the APC and the previously reported localization of Xnf7 to the mitotic spindle (Li et al., 1994), we sought to determine if Xnf7 might play a role in the spindle assembly checkpoint. As described by Minshull et al. (1994), Xenopus extracts can be induced to undergo a spindle checkpoint arrest after the addition of high concentrations of demembranated sperm chromatin and nocodazole. To determine if Xnf7 might play a role in spindle checkpoint function, CSF extracts were preincubated with preimmune IgG or anti-Xnf7 antibodies for 15 min to functionally inhibit Xnf7. After incubation with high concentrations of sperm chromatin and nocodazole, Ca2 was added. Although control extracts lacking nocodazole did not arrest, extracts containing nocodazole and preimmune IgG established a spindle checkpoint and therefore failed to degrade cyclin B (Fig. 7). In contrast, addition of anti-Xnf7 antibodies effectively overrode the spindle checkpoint, allowing cyclin B degradation and rapid reformation of interphase nuclei, even in the presence of nocodazole. These data demonstrate that Xnf7 is required for spindle assembly checkpoint function in Xenopus egg extracts and suggest that Xnf7 may provide a link between spindle status and the core APC machinery.
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]! n7 V, T9 o+ [: cActivation of the APC is controlled in part by Cdc20/Cdh1 as well as their upstream regulators, including BubR1, Bub3, Mad2, and Emi1 (Zachariae and Nasmyth, 1999; Peters, 2002). Here, we have identified Xnf7 as a novel inhibitor of APC function unlikely to act via Cdc20. In addition, we have shown that Xnf7 itself is a ubiquitin ligase and that its ligase activity is required for its effects on APC-dependent ubiquitylation. Because Xnf7 cosedimented and coimmunoprecipitated with Cdc27, it is attractive to speculate that Xnf7 modifies either Cdc27 function or the function of other associated core APC subunits. Furthermore, we have shown that Xnf7 is required for spindle assembly checkpoint function in Xenopus egg extracts, suggesting that Xnf7 could be part of a mechanism for direct regulation of the APC by the spindle checkpoint (a model recently proposed by Acquaviva et al. [2004]).
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6 v4 d+ _0 [/ H+ a0 JIdentification of Xnf7 as a cyclin B2–interacting protein2 y2 Y7 Y' j9 P+ b9 g2 o: _
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Although we identified Xnf7 as a cyclin B2–interacting protein, we have shown that Xnf7 also affects the degradation of cyclin B1 and securin, and, given its inhibitory effect on the APC, is likely to affect other APC substrates as well. Because Xnf7 is phosphorylated by Cdc2/cyclin B and mitogen-activated protein kinase during oocyte maturation (Reddy et al., 1991; El-Hodiri et al., 1997a), we speculate that the specific interaction with cyclin B2 might reflect an enzyme–substrate interaction due to phosphorylation of Xnf7 by Cdc2/cyclin B2.' |( W$ U, d( `6 a- D8 i7 e
# N9 L; K' g* Q' Q" @2 aRegulation of APC activation5 R r4 I/ ]0 W8 O+ b: { ?) X
6 e5 C8 T1 N* ^. tActivation of the APC is controlled not only by the binding of activating proteins Cdc20 and Cdh1 but is also regulated by phosphorylation of its subunits by mitotic kinases including Cdc2/cyclin B, Plk1, and PKA (for review see Castro et al., 2005). One way in which mitotic phosphorylation of APC subunits promotes its activation is by facilitating the binding of Cdc20 (Kramer et al., 2000). In budding yeast, mutation of Cdk1 sites in APC subunits Cdc16, Cdc23, and Cdc27 inhibits APC phosphorylation, reduces Cdc20 binding, and delays mitotic exit, suggesting that phosphorylation of the APC is essential for its activation (Rudner and Murray, 2000). However, it is clear that the absence of APC subunit phosphorylation during interphase does not render the APC impervious to activation in that APC from interphase extracts can be activated in vitro by Cdc20 or Cdh1 (Fang et al., 1998b) or in vivo by overexpression of either activator at any stage in the cell cycle (Visintin et al., 1997). Thus, multiple mechanisms are likely to cooperate to ensure that the APC is not activated prematurely. Our data suggest that Xnf7 participates in one such mechanism., W; |/ r: |- P3 t' G7 {# Q
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Xnf7's ligase activity is required for its inhibition of the APC
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/ s' R0 M: a, i1 W' A" x" LConsistent with its role as an inhibitor of APC activity, excess Xnf7 was able to slow degradation of APC substrates and concomitantly delay mitotic exit. Intriguingly, this function of Xnf7 required that it be active as a ubiquitin ligase. Moreover, in our studies using mitotic APC immunoprecipitates to investigate direct inhibition of the APC, inhibition by Xnf7 required the presence of Xnf7WT in conditions permissive for Xnf7's enzymatic activity (E1, UbcH5a, and ubiquitin). It is not yet clear whether this reflects a requirement for Xnf7 autoubiquitylation in its ability to regulate the APC or the necessity for ubiquitylation of a substrate in the APC immunoprecipitates. Although it is formally possible that Xnf7 could promote ubiquitin-dependent degradation of APC components, the level of APC subunits examined has not been found to vary throughout the cell cycle. However, because ubiquitylation can modify substrate function without targeting it for degradation, it is possible that Xnf7 inhibits APC function by ubiquitylation of an APC subunit. Indeed, several ubiquitin ligases have been reported to modify substrate localization and/or protein–protein interactions through monoubiquitylation of targets (Hicke, 2001). With regard to the possibility that either autoubiquitylation or ubiquitylation of APC components might be important for Xnf7 function, it is interesting to note that Xnf7 binding to the APC appeared to be equal before and after release from CSF arrest (when the APC is differentially active). Moreover, direct association of Xnf7 with the APC was not measurably altered by the spindle checkpoint (unpublished data). These observations strongly suggest that binding alone is not sufficient for Xnf7-mediated inhibition of the APC. It is attractive to speculate that Xnf7's E3 ligase activity may be cell cycle regulated, and thus responsible for its cell cycle–specific actions. Alternatively, or additionally, cell cycle–specific modification of Xnf7 itself (e.g., phosphorylation or autoubiquitylation) may be required for it to effectively inhibit the APC., A8 A6 n6 T: [' l, x+ H% q; B3 m
- _5 d! t. O, F; j- ~Recently, it was reported that the core subunits of the APC, rather than Cdc20/Cdh1, are directly responsible for substrate recognition (Carroll and Morgan, 2002; Meyn et al., 2002; Passmore et al., 2003; Yamano et al., 2004). Given our finding that Xnf7 inhibits the APC via association with core APC subunits, it is plausible that this novel APC inhibitor exerts its effects by interfering with substrate recognition, perhaps through ubiquitylation of an APC subunit. Ideally, we would like to address this issue directly by determining if Xnf7 can ubiquitylate proteins present in the anti-Cdc27 precipitate. Unfortunately, this approach has been hampered thus far by the high level of ubiquitylation associated with the APC itself.
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Although we have identified a role for Xnf7 in regulating APC activation, previously reported data have implicated Xnf7 as a regulator of dorsal–ventral polarity establishment in Xenopus (El-Hodiri et al., 1997b). Because ubiquitin ligases may have multiple substrates and therefore participate in several signaling pathways, it is possible that these two roles of Xnf7 are entirely distinct. However, it is interesting to note that reduction-of-function APC mutations in Caenorhabditis elegans can disrupt establishment of anterior–posterior polarity (Rappleye et al., 2002). Thus, Xnf7 could potentially regulate polarity establishment in Xenopus via its effects on the APC.8 R1 m' A- e a. @# D
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Collectively, the data reported here strongly support a role for Xnf7 in regulating APC activation and suggest that Xnf7 participates in the spindle checkpoint. Interestingly, it has recently been reported that the APC colocalizes with spindle checkpoint protein complexes at unattached kinetochores and that the spindle checkpoint machinery is required for the recruitment of the APC to these sites (Acquaviva et al., 2004). These data suggest that the APC can be regulated directly by the spindle checkpoint. Given our finding that Xnf7 is required for spindle checkpoint function in egg extracts, it is attractive to speculate that Xnf7 might be involved in such a mechanism. Future identification of direct Xnf7 ubiquitin ligase substrates should help to elucidate the mechanism of Xnf7-mediated APC inhibition while helping to further define the links between spindle function and APC activation.# V/ }; R6 D/ C
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Materials and methods8 J0 d" N" u5 t- L2 D! v* k
/ O, J% \3 p; [+ y# URecombinant protein expression% t V3 O- _, f& J7 r: \! A7 B
6 W$ }8 Z' S) `Wild-type Xnf7 was subcloned into the EcoRI and NcoI sites of pGexKG. Xnf7 RING-finger mutants Xnf7m3 (C160A) and Xnf7m36 (C160A and C168A) were prepared using the QuikChange Site-Directed Mutagenesis Kit (Stratagene). To prepare pGexKG-Xnf7C, Xnf7 (257–609 aa) was PCR amplified and subcloned into the EcoRI and NcoI sites of pGex-KG. GST fusion proteins expressed in bacteria were purified on glutathione-Sepharose by standard protocols. Proteins were cleaved with thrombin and dialyzed against Xnf7 buffer (XB-Xnf7: 100 mM KCl, 25 mM sucrose, 10 mM Hepes, 1 mM MgCl2, and 1 mM DTT, pH 7.8). Uncleaved GST-Xnf7C was dialyzed against PBS.+ [% D/ X, B b# L& Q4 r
; K% y9 }& b; u7 ^4 [CRS affinity chromatography
& n2 Y0 J7 \9 {. c0 K$ N: u! k% R( ?& S" \) ]! ~( W9 N1 ]5 [
Glutathione-Sepharose coupled to GST, GST-cyclin B1 CRS, or GST-cyclin B2 CRS (Yang et al., 1998) were incubated with egg extracts. Bound material was biotinylated, resolved by SDS-PAGE, transferred to nitrocellulose, and probed with HRP-streptavidin. For Coomassie blue staining, bound material was washed and resolved by SDS-PAGE. The 80-kD band of interest was analyzed by mass spectrometry at Harvard Microchemistry.6 S0 ?, l v5 F* c& L
7 l F0 ~8 H; C, t8 O; z" VAntibodies and immunodepletions7 h9 E9 B9 p* \ v
0 A* A, ?4 X- P5 R( SRabbit polyclonal antibodies raised against Xnf7C were affinity purified on glutathione-Sepharose covalently coupled to GST-Xnf7C with dimethyl pimelimidate. Other antibodies used were as follows: anti–cyclin B1 and anti–cyclin B2 (Hochegger et al., 2001), anti-APC2 (a gift from G. Fang, Stanford University, Stanford, CA), anti-ubiquitin (Santa Cruz Biotechnology, Inc.), anti-Cdc27 (Santa Cruz Biotechnology, Inc.) for immunoprecipitation, anti-Cdc27 (Transduction Laboratories) for immunoblotting, and anti-Cdc20 (Santa Cruz Biotechnology, Inc.).
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. t y3 y r7 `+ T/ B: J8 }. lFor immunodepletions, purified anti-Xnf7 antibodies or preimmune IgG coupled to protein A–Sepharose were washed in XB-CSF (100 mM KCl, 50 mM sucrose, 10 mM Hepes, pH 7.7, 5 mM EGTA, 2 mM MgCl2, and 100 μM CaCl2) or ELB (250 mM sucrose, 50 mM KCl, 10 mM Hepes, pH 7.7, 2.5 mM MgCl2, and 1 mM dithiothreitol), incubated with extracts (0.2 μl beads/μl extract, 30 min at 4°C), and removed by centrifugation (10,000 rpm, 1 min at 4°C).: ~! W% N7 a. k' s: \$ K
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Degradation assays
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Xenopus egg extracts were prepared as described previously (Murray, 1991). Degradation assays were performed in CSF extracts by adding CaCl2 to 0.6 mM to initiate anaphase. Human securin (a gift from J. Pines, Wellcome Trust/Cancer Research UK, Cambridge, UK) was translated in vitro in the presence of 35S-methionine/cysteine. Aliquots were removed and analyzed by SDS-PAGE followed by autoradiography (35S-securin) or immunoblotting (cyclin B). In all degradation assays, the same amount of protein was loaded in each gel lane. For interphase extracts, 35S-labeled cyclin B1 or IAP was added, and aliquots were analyzed as 35S-securin. To stimulate IAP autoubiquitylation, Drosophila melanogaster reaper was added to extracts (37.5 μM final) with 100 μM zVAD-fmk (BIOMOL Research Laboratories).
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0 r8 V( t4 u; T$ p) _1 _For antibody addition to extracts, Xnf7 antibodies and preimmune IgG were concentrated to 3 μg/μl. Blocked Xnf7 antibodies were prepared by incubating with GST-Xnf7C. After antibody addition (0.3 μg antibody/μl extract), extracts were incubated at 23°C for 15 min before addition of CaCl2. For Xnf7 protein addition, buffer, Xnf7WT, or Xnf7m36 was added (0.06 μg protein/μl extract), followed by 15 min incubation at 23°C before addition of CaCl2. Methyl-ubiquitin (3 μg/μl final) and 35S-labeled Xenopus cyclin B1 fragment (1–126 aa) were added in the indicated experiments. For Xnf7 protein addition to depleted extracts, buffer or Xnf7WT was added (0.09 μg protein/μl extract), followed by 30 min incubation at 23°C before CaCl2 addition.
9 I" O/ r7 j- g' {# T& h* I0 d) Y7 J0 }6 Y
Spindle assembly checkpoints were formed as described previously (Minshull et al., 1994). DNA was stained with Hoechst 33258 and nuclear morphology was examined using a microscope (model Axioskop; Carl Zeiss MicroImaging, Inc.) with a 40x Plan-Neofluar objective (NA 0.75) or a 100x Plan-Apochromat objective (NA 1.4). Images were captured using a Pentamax cooled charge-coupled device camera (Princeton Instruments) interfaced with MetaMorph software (Universal Imaging Corp.).
. L4 [4 K2 P5 `& x1 l1 j6 R: w" Q/ |0 j0 t! n
Xnf7 ubiquitylation assay
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5 f7 I# ~& A/ z' P' M7 b& u% E4 μg Xnf7WT, Xnf7m3, or Xnf7m36 were incubated (2 h at 37°C) with 50 ng of rabbit E1, 1 μg UbcH5a, 10 μg ubiquitin, and 3 mM ATP brought to 50 μl with buffer (25 mM Hepes, pH 7.5, 10 mM NaCl, 3 mM MgCl2, 10 mM DTT, and 0.05% Triton X-100). Reactions were stopped with SDS sample buffer, resolved by SDS-PAGE, and analyzed by immunoblotting.1 s5 v i7 n7 s4 g6 H" w
. c; G6 g4 N0 GE2-Thioester assay
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Z6 r- t* a( I9 x0 N, W8 p. F* G2 μg of each E2 were incubated (30 min at 37°C) with 0.5 μg of rabbit E1, 40 μg ubiquitin, 10 mM ATP, and 10 mM MgCl2 in a 10-μl total volume. Reactions stopped with SDS sample buffer were resolved on 4–20% Tris-HCl SDS-PAGE gels and visualized by silver stain.0 {6 l2 ^- F) Q' z/ |5 L6 Y8 q X$ N
. i3 [9 g4 K1 w2 D' d# \In vitro APC assay
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/ E# `9 E/ o# p9 x$ k" i9 y5 CAnti-Cdc27 antibodies coupled to protein A Dynabeads were washed in ELB and incubated (2.5 h at 4°C) with mitotic extracts. APC beads were washed with 500 mM KCl, 20 mM Hepes, pH 7.7, and 0.5% NP-40 followed by 20 mM Hepes, pH 7.7. Beads were incubated (1 h at 23°C) with RRL or in vitro translated human Cdc20 that had been preincubated with buffer, 6 μM MBP, 6 μM MBP-Emi1, or 2–5 μM Xnf7WT or Xnf7m36. The incubation also included 80 ng of rabbit E1, 120 ng UbcH5a, 10 μg of bovine ubiquitin, 3 mM ATP, and 3 mM MgCl2 where indicated. Beads were washed with 20 mM Hepes, pH 7.7, and assayed for cyclin ubiquitylation activity with 1.25 μg/μl of bovine ubiquitin, 60 ng/μl E1, 40 ng/μl UbcH10, an energy regenerating system, 2 μl of 35S-labeled in vitro translated Xenopus cyclin B1 fragment (1–126 aa) as a substrate, and 3 μl APC beads. Reactions were incubated at 23°C for 1 h, quenched with SDS sample buffer, analyzed by SDS-PAGE and autoradiography, and quantitated by Phosphorimager. O) D+ i3 r4 g% h- [- y
9 }( H5 G) Z; V8 G0 q. D( qSucrose gradient centrifugation
+ g1 L& S/ p& }3 M- Z( V F. s4 k% z4 m5 q, T8 I' B
CSF extract diluted 1:3 in XB-CSF without sucrose was cleared at 40,000 rpm and resolved on a 12-ml 10–40% wt/vol sucrose gradient by centrifugation in an SW40 rotor (30,000 rpm, 18 h at 4°C). 20 0.5-ml fractions were collected and analyzed by SDS-PAGE and immunoblotting.
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/ v6 C4 q# `( _: {; R) qWe thank Guowei Fang for anti-Xenopus APC2 antibodies and Jon Pines for the human securin construct. We are also grateful to Adam Eldridge for helpful discussions and to Christopher Freel for assistance with figure preparation.6 h2 F8 T3 I8 K6 K! ~4 S: `
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This research was supported by a grant from the National Institutes of Health to S. Kornbluth (RO1 GM067225). J.B. Casaletto is a predoctoral fellow of the Howard Hughes Medical Institute.- u2 c6 ?* \- V- Q
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发表于 2009-4-25 09:59
