APC2 Cullin Protein and APC11 RING Protein Comprise the Minimal Ubiquitin Ligase Module of the Anaphase-promoting Complex

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager


Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Tang, Z.
	Articles by Yu, H.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Tang, Z.
	Articles by Yu, H.

Vol. 12, Issue 12, 3839-3851, December 2001

APC2 Cullin Protein and APC11 RING Protein Comprise the Minimal Ubiquitin Ligase Module of the Anaphase-promoting Complex

Zhanyun Tang,^* Bing Li,^* Rajnish Bharadwaj,^* Haizhen Zhu,^* Engin Özkan, Kevin Hakala,^* Johann Deisenhofer, and Hongtao Yu^*^§

^*Departments of Pharmacology and Biochemistry, and Howard Hughes Medical Institute, The University of Texas Southwestern Medical Center at Dallas, Dallas, Texas 75390-9041

Submitted August 21, 2001; Revised September 16, 2001; Accepted September 24, 2001
Monitoring Editor: Mark J. Solomon

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In mitosis, the anaphase-promoting complex (APC) regulates the onset of sister-chromatid separation and exit from mitosisby mediating the ubiquitination and degradation of the securinprotein and mitotic cyclins. With the use of a baculoviral expressionsystem, we have reconstituted the ubiquitin ligase activity ofhuman APC. In combination with Ubc4 or UbcH10, a heterodimericcomplex of APC2 and APC11 is sufficient to catalyze the ubiquitinationof human securin and cyclin B1. However, the minimal APC2/11 ubiquitinligase module does not possess substrate specificity, becauseit also ubiquitinates the destruction box deletion mutants ofsecurin and cyclin B1. Both APC11 and UbcH10 bind to the C-terminalcullin homology domain of APC2, whereas Ubc4 interacts with APC11directly. Zn²⁺-binding and mutagenesis experiments indicate that APC11 bindsZn²⁺ at a 1:3 M ratio. Unlike the two Zn²⁺ ions of the canonical RING-finger motif, the third Zn²⁺ ion of APC11 is not essential for its ligase activity. Surprisingly,with Ubc4 as the E2 enzyme, Zn²⁺ ions alone are sufficient to catalyze the ubiquitination of cyclinB1. Therefore, the Zn²⁺ ions of the RING finger family of ubiquitin ligases may be directlyinvolved incatalysis.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The orderly progression through mitosis relies on the sequential degradation of several cell cycle regulatory proteins mediatedby the mitotic ubiquitination system (King et al., 1996a; Zachariaeand Nasmyth, 1999; Nasmyth et al., 2000). This system first initiatesthe onset of sister-chromatid separation by ubiquitinating theanaphase inhibitor or securin (Nasmyth et al., 2000). Degradationof the ubiquitinated securin in turn activates the separase, whichthen cleaves a subunit of the cohesin complex, resulting in theloss of sister-chromatid cohesion and the onset of anaphase (Uhlmannet al., 1999, 2000; Waizenegger et al., 2000). The same machineryalso mediates the ubiquitination and destruction of mitotic cyclins,leading to the inactivation of the cdc2 activity and the exitfrom mitosis (King et al., 1996a; Morgan, 1999; Zachariae andNasmyth, 1999).

In this system, a large protein complex, called the anaphase-promoting complex (APC) or cyclosome, functions as the ubiquitinligase (E3) (Irniger et al., 1995; King et al., 1995; Sudakinet al., 1995; Tugendreich et al., 1995). In the presence of theubiquitin-activating enzyme (E1) and certain ubiquitin-conjugatingenzymes (E2s) such as Ubc4 and UbcH10 (called UbcX in Xenopusand E2-C in clams), APC catalyzes the attachment of ubiquitinto the lysine side chains of securin and mitotic cyclins (Kinget al., 1995; Aristarkhov et al., 1996; Yu et al., 1996). Thepolyubiquitinated APC substrates are then targeted to the 26Sproteasome for degradation (Hershko and Ciechanover, 1998).

To ensure that APC substrates are degraded with proper timing, the ubiquitin ligase activity of APC is tightly regulated duringthe cell cycle (King et al., 1996a; Morgan, 1999). Significantprogress has been made toward the understanding of the regulationof APC during the cell cycle. APC is turned on during mitosis,remains active through most of G1, and is rapidly inactivatedat the G1/S transition (Fang et al., 1998; Kramer et al., 1998).The activity profile and substrate specificity of APC can be partiallyexplained by the transient association of two related regulatoryfactors, Cdc20 and Cdh1, at specific stages of the cell cycle(Sigrist and Lehner, 1997; Schwab et al., 1997; Visintin et al.,1997; Fang et al., 1998; Kramer et al., 1998). Cdc20 binds toAPC in mitosis, whereas Cdh1 interacts with APC both in mitosisand the G1 phase (Fang et al., 1998; Kramer et al., 1998). Bindingof either Cdc20 or Cdh1 to APC increases the activity of APC drastically(Fang et al., 1998; Kramer et al., 1998). Although the exact mechanismby which Cdc20 and Cdh1 contribute to the ubiquitination reactionsis unknown, several recent observations suggest that they mightbe directly involved in substrate recruitment (Schwab et al.,1997; Sigrist and Lehner, 1997; Visintin et al., 1997; Burtonet al., 2001; Hilioti et al., 2001; Pfleger et al., 2001).

In contrast to the cell cycle regulation of APC, little is known about the mechanism by which APC catalyzes the ubiquitinationreaction. This is partially due to the fact that the vertebrateAPC contains at least 11 subunits (Yu et al., 1998; Grossbergeret al., 1999; Gmachl et al., 2000). No clues about the biochemicalfunctions of most APC subunits can be inferred from examiningtheir amino acid sequences. However, sequence analysis of APC2and APC11 has revealed homology with proteins involved in otherubiquitination systems, particularly the Skp1-Cullin-F-box (SCF)pathway (Yu et al., 1998; Zachariae et al., 1998; Deshaies, 1999;Ohta et al., 1999; Skowyra et al., 1999; Gmachl et al., 2000).

APC2 contains a region that is similar to a sequence in cullins, and thus is a distant member of the cullin family (Yu etal., 1998; Zachariae et al., 1998). The cullin family of proteinsis essential for the ubiquitination of G1 cyclins, cyclin-dependentkinase inhibitors, and other important regulatory proteins inyeast and mammals (Kipreos et al., 1996; Willems et al., 1996;Feldman et al., 1997; Lyapina et al., 1998; Latres et al., 1999;Tan et al., 1999). A cullin protein in budding yeast, Cdc53p,is a part of the SCF ubiquitin ligase complex, which targets phosphorylatedSic1p and G1 cyclins for degradation in late G1 (Willems et al.,1996; Feldman et al., 1997). Similar SCF complexes containingcullin proteins have been found in mammals; they mediate the degradationof a variety of substrates, including I $kappa$ B and E2F (Marti et al.,1999; Tan et al., 1999). APC11 contains a Zn²⁺-binding motif referred to as the RING-H2 finger and is homologousto Rbx1/Roc1/Hrt1 that physically interacts with Cul1 in mammalsand Cdc53p in yeast (Zachariae et al., 1998; Kamura et al., 1999;Ohta et al., 1999; Seol et al., 1999; Skowyra et al., 1999; Gmachlet al., 2000). Because the Cul1/Rbx1 heterodimeric complex isthe functional core of the SCF ubiquitin ligases, APC2 and APC11,by analogy, might also be directly involved in catalysis (Seolet al., 1999). In fact, it has recently been shown that APC11alone is sufficient to ubiquitinate APC substrates in the presenceof Ubc4 (Gmachl et al., 2000; Leverson et al., 2000). Surprisingly,UbcH10 does not support the ubiquitination reaction mediated byAPC11 (Gmachl et al., 2000; Leverson et al., 2000).

To gain insights into the catalytic mechanism of APC, we have reconstituted the ubiquitin ligase activity of APC. The minimalligase module of APC is the heterodimeric complex of the cullin-relatedprotein APC2 and the RING finger protein APC11. Therefore, APCis a member of the expanding family of cullin-RING finger-basedubiquitin ligases. Although APC11 alone can ubiquitinate APC substrateswith the use of Ubc4 as the E2 enzyme, the APC2/11 complex isrequired to catalyze the ubiquitination of APC substrates in thepresence of UbcH10. Ubc4 interacts directly with APC11, whereasUbcH10 does not. Instead, UbcH10 binds to the C-terminal cullindomain of APC2. We further demonstrate that APC11 contains a thirdZn²⁺-binding site, in addition to the two Zn²⁺ ions of the canonical RING-H2 finger. Interestingly, Zn²⁺ ions alone can catalyze the ubiquitination of APC substrateswith the use of Ubc4 as the E2 enzyme, suggesting that Zn²⁺ ions of the RING finger-containing ubiquitin ligases might bedirectly involved incatalysis.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Protein Expression with Use of Baculoviral System

In addition to the eight human APC subunits (APC1-8) reported previously (Yu et al., 1998), two more subunits were clonedwith the use of polymerase chain reaction (PCR), APC10 and APC11,based on their sequence similarity to the yeast APC subunits.The recombinant baculoviruses were constructed with the Bac-to-Bacsystem (Invitrogen, Carlsbad, CA). Briefly, the human genes encodingAPC subunits (APC1-11), Cdc20, and Cdh1 were amplified by PCRand cloned into the pFastBac, pFastBac-HT, or pFastBac-GST vectorswith the use of suitable restriction sites for the productionof untagged, N-terminal His₆-tagged, or N-terminal GST-taggedproteins. These plasmids were then transformed into the Escherichiacoli strain DH10Bac and the desired bacmids were isolated. Thesebacmids were transfected into adherent Sf9 cells for the packagingof baculoviruses. To limit the number of viruses used in the coinfections,four viruses each harboring two APC genes (APC1/8, APC2/7, APC3/6,and APC4/5) were also made with the use of the pFastBacDual vectorthat contains two independent promoters to transcribe both genessimultaneously. The initial viral stocks were then amplified withtwo successive rounds of infection of Sf9 cells in suspension.The titers of the final viral stocks were typically ~1-5 × 10⁸/ml, as measured with the Rapid Titer kit (CLONTECH, Palo Alto,CA). Small samples were taken during the second round of amplificationand checked for protein production and solubility by immunoblottingwith the relevant antibodies. The production of all 10 APC subunits,Cdc20, and Cdh1 proteins in soluble form was verified by eitherCoomassie staining orimmunoblotting.

For the coinfection experiments, Sf9 or Hi5 insect cells were infected with a Multiplicity of infection of 5-10 for each virusfor 40-50 h. Cells were harvested and lysed by Dounce homogenization.The lysates were cleared by centrifugation at 30,000 × g for 1h. The human APC proteins was then purified via the appropriatetags and assayed for ubiquitin ligase activity or binding to otherproteins. When necessary, the APC proteins were further purifiedby anion exchange and/or gel filtrationchromatography.

Ubiquitination Assay

For the ubiquitination assays involving the intact APC, the $alpha$ -APC3 (Cdc27) beads were incubated with 10 volumes of interphaseXenopus egg extracts for 2 h at 4°C and washed five times withXB (10 mM HEPES, pH 7.7, 100 mM KCl, 0.1 mM CaCl₂, 1 mM MgCl₂,50 mM sucrose) containing 500 mM KCl and 0.5% NP-40 and twicewith XB. The interphase APC beads were then incubated for 1 hat room temperature with human Cdc20 or Cdh1 proteins. After incubation,the APC beads were again washed twice with XB and assayed forubiquitin ligase activity. For the assays with the reconstitutedAPC, 5 µl of Ni²⁺-nitrilotriacetic acid (NTA) beads were incubated with 500 µlof the insect cell lysate containing the appropriate His₆-taggedAPC proteins, washed five times with XB, and assayed for ubiquitinligaseactivity.

Each ubiquitination assay was performed in a volume of 5-10 µl. The reaction mixture contained ATP, 150 µM of bovine ubiquitin,5 µM of the Myc-tagged human securin, or an N-terminal fragmentof human cyclin B1, 5 µM of human E1, 2 µM of Ubc4 or UbcH10,and 2-5 µl of the APC beads. The reactions were incubated at roomtemperature for 1 h, quenched with SDS sample buffer, and analyzedby SDS-PAGE followed by immunoblotting with $alpha$ -Myc.

Cyclin Degradation Assay

The Xenopus egg extracts were prepared as described previously (Murray, 1991). To assay cyclin degradation, the N-terminalfragment of human cyclin B1 (residues 1-102) with a Myc-tag andubiquitin were added to the mitotic extracts at final concentrationsof 100 nM and 150 µM, respectively. Aliquots of the reaction mixturewere quenched by SDS sample buffer at the indicated time, separatedby SDS-PAGE, and blotted with $alpha$ -Myc.

Protein Binding Assay

To assay the binding among APC2, APC11, Ubc4, and UbcH10, one of the binding partners was expressed either in bacteria orinsect cells as His₆-tagged proteins. The other partner was invitro translated in reticulocyte lysate in the presence of [³⁵S]methionine. Purified His₆-tagged proteins were bound to Ni²⁺-NTA beads, incubated with the ³⁵S-labeled proteins, and washed three times with Tris-bufferedsaline containing 0.05% Tween. The ³⁵S-labeled proteins retained on beads were analyzed by SDS-PAGEfollowed by autoradiography. The vectors encoding the APC2 fragmentswere constructed by PCR. The APC11 mutants were made with theuse of the QuikChange site-directed mutagenesis kit (Stratagene,La Jolla,CA).

Zn²⁺-binding Assay

The purified APC2e/11 protein was dialyzed against TNG buffer (10 mM Tris-HCl, pH 8.0, 200 mM NaCl, and 5% glycerol). Theconcentration of APC2e/11 was determined with the use of UV-VISspectroscopy and Bradford assays (Bio-Rad, Hercules, CA). TheZn²⁺ ions bound by APC2e/11 were released by p-hydroxymercuriphenylsulfonicacid. The released Zn²⁺ was then coordinated by 4-2-pyridylazoresorcinol (PAR), and theresulting Zn²⁺-PAR₂ complex absorbed light at 500 nm with an extinction coefficientof 6.6 × 10⁴ M¹ cm¹. Specifically, aliquots of 1 mM p-hydroxymercuriphenylsulfonicacid were successively added to a mixture containing 1.5 µM ofAPC2e/11 and 100 µM of PAR, until a plateau of OD₅₀₀ was reached.The maximum value of OD₅₀₀ divided by the extinction coefficientthen yielded the concentration of Zn²⁺.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Reconstitution of Ubiquitin Ligase Activity of Human APC

To investigate the mechanism of APC, we coinfected Hi5 insect cells with multiple recombinant baculoviruses harboring 10 APCgenes and the cofactors Cdc20 or Cdh1. Because the APC proteinswere His₆-tagged at their N termini, they were purified from theinsect cell lysate with the use of Ni²⁺-NTA beads and assayed for their ubiquitination activity. As shownin Figure 1A, when Hi5 cells were infected with viruses encoding10 APC subunits (APC1-11) and Cdc20, the expressed APC proteinscontained a ubiquitin ligase activity that, in combination withUbcH10, efficiently ubiquitinated human cyclin B1. This activityalso supported ubiquitination of human securin (our unpublisheddata; see below). To determine which subunits were required forthis activity, each virus was omitted individually from the coinfection.Only APC2 and APC11 were required for the ligase activity (Figure1A). Similar results were obtained when the Cdh1 baculovirus wasused in the coinfection instead of Cdc20 (our unpublished data).The fact that omission of APC2 or APC11 alone caused the lossof the reconstituted activity indicated that the purified ligaseactivity was not due to the presence of the endogenous APC frominsect cells.

View larger version (45K):
[in this window]
[in a new window]

Figure 1. Reconstitution of the ubiquitin ligase activity of APC. (A) Hi5 insect cells were coinfected with baculoviruses encoding the indicated APC subunits. The expressed His₆-tagged APC proteins were isolated from the insect cell lysate with the use of the Ni²⁺-NTA beads and assayed for ubiquitin ligase activity in the presence of UbcH10. The reaction mixture was separated on SDS-PAGE and blotted with $alpha$ -Myc to detect the C-terminally Myc-tagged cyclin B1 protein. Omission of the APC2 (lane 3) or APC11 (lane 11) viruses from the coinfection resulted in the loss of ubiquitin ligase activity. (B) Ubiquitin ligase activity of the intact APC. Either UbcH10 (lanes 1-6) or Ubc4 (lanes 7-12) was used as the E2 enzyme. To determine the D-box dependency of APC^Cdc20 and APC^Cdh1, either the wild-type (WT) cyclin B1 (lanes 1-3 and 7-9) or the D-box deletion mutant ( $Delta$ DB) of cyclin B1 (lanes 4-6 and 10-12) was used as substrates. (C) Same as A except that $Delta$ DB-cyclin B1 was used as the substrate instead of the wild-type cyclin B1 protein.

Because Cdc20 and Cdh1 are positive regulators of APC, it was surprising to us that Cdc20 or Cdh1 were not required for theubiquitin ligase activity of the reconstituted APC. We thereforecompared the reconstituted APC activity with that of the intactAPC from Xenopus egg extracts. Nearly all APC substrates containthe destruction box (D-box) or the KEN-box motifs, which are requiredfor the efficient ubiquitination and degradation of these substrates(King et al., 1996b; Pfleger and Kirschner, 2000). Cdc20 and Cdh1have been shown to confer the D-box and KEN-box specificity ofAPC (Burton et al., 2001; Hilioti et al., 2001; Pfleger et al.,2001). The activities of the intact APC^Cdc20 and APC^Cdh1 from Xenopus were assayed with cyclin B1 as the substrate. Asshown in Figure 1B, purified Cdc20 and Cdh1 proteins greatly stimulatedthe ligase activity of the intact interphase Xenopus APC withUbcH10 as the E2 enzyme and wild-type cyclin B1 as substrate.However, neither the intact APC^Cdc20 nor APC^Cdh1 significantly ubiquitinated a D-box deletion mutant of cyclinB1 ( $Delta$ DB-cyclin B1). Similar results were obtained with Ubc4 asthe E2 enzyme, although the patterns of cyclin B-ubiquitin conjugatesformed by the two enzymes were different. Ubc4 appeared to bemore processive than UbcH10 in the presence of either intact APC^Cdc20 or APC^Cdh1.

Because Cdc20 and Cdh1 were not essential for the reconstituted APC activity, we tested whether the ligase activity obtainedwith overexpressed APC proteins conferred D-box specificity, similarto the intact APC. Not surprisingly, the reconstituted human APCubiquitinated $Delta$ DB-cyclin B1 equally efficiently, indicating thatthe reconstituted activity did not possess substrate specificity(Figure 1C). This activity also required the presence of APC2and APC11. Therefore, we reconstituted the minimal ligase activityof APC, which lacked D-box dependency. At present, we do not knowthe exact cause for the lack of D-box dependency of our reconstitutedAPC. However, several factors might contribute to this. First,the reconstituted APC might not have the correct quaternary arrangementof all the relevant subunits. Second, the set of subunits usedto reconstitute the APC is not complete. Additional human APCsubunits are required for the proper function of the reconstitutedAPC. Finally, it is also possible that the high concentrationsof the reconstituted APC and the substrates in our in vitro reactionsmay have eliminated the need for high-affinity interactions betweenAPC and substrates. We are currently investigating thesepossibilities.

Heterodimeric Complex of APC2 and APC11 Is the Minimal Ligase Module of APC

Because both APC2 and APC11 were required for the reconstituted APC activity, we tested whether they interacted with eachother in the absence of the rest of the APC subunits. To characterizethe immediate binding partners of APC11 in the APC complex, theGST-APC11 virus was coinfected with each of the other virusesin a pairwise manner. GST-APC11 and its associated subunits werethen purified with glutathione-Sepharose beads and analyzed bySDS-PAGE followed by Coomassie staining and immunoblotting. Asshown in Figure 2A, APC11 binds tightly to APC2 and weakly toAPC6. The identities of APC2 and APC6 were verified by immunoblotting(our unpublished data). It was not apparent from the GST-APC11pull-down experiment whether GST-APC11 interacts with APC10 becausethe His₆-tagged APC10 (26 kDa) comigrated with proteolytic fragmentsof GST-APC11 on SDS-PAGE (our unpublished data). We thereforeused a His₆-tagged APC10 virus to infect Sf9 cells together withthe GST-APC11 virus. The APC10 protein was then purified withNi²⁺-NTA beads and analyzed by SDS-PAGE. APC10 binds tightly to GST-APC11as revealed by Coomassie staining (Figure 2B) and immunoblottingwith $alpha$ -GST antibody (Figure 2C). Several large proteins containthe so-called DOC domains that are similar in sequence to APC10;some of these proteins also contain cullin homology domains orhomologous to E6-AP C terminus (HECT) domains (Grossberger etal., 1999). E6-AP, the founding member of a family of proteinscontaining HECT domains, mediates the HPV E6-dependent degradationof p53 (Scheffner et al., 1995). It is likely that the DOC domainsof these large multidomain proteins might also be involved inbinding to yet unidentified RING-finger proteins.

View larger version (19K):
[in this window]
[in a new window]

Figure 2. APC11 interacts with APC2 and APC10. (A) GST-APC11 baculovirus was coinfected with APC1/8 (a single baculovirus encoding both APC1 and APC8), APC2/7, APC3/6, APC4/5, or Cdh1 viruses in a pairwise manner into Sf9 cells. GST-APC11 and its interacting proteins were purified on glutathione beads, separated on SDS-PAGE, and stained with Coomassie Blue. GST was added to the lysates of APC1/8, APC2/7, APC3/6, APC4/5, and Cdh1 and used as controls. APC11 interacted strongly with APC2 (lane 3) and weakly with APC6 (lane 5). As determined by mass spectrometry, the band at 55 kDa belonged to $alpha$ / $beta$ -tubulin, which presumably associated nonspecifically with GST-APC11. (B) His₆-tagged APC10 baculovirus was coinfected with the GST-APC11 virus into Sf9 cells. His₆-APC10 and its interacting proteins were purified on Ni²⁺-NTA beads, separated on SDS-PAGE, and stained with Coomassie Blue. As controls, Ni²⁺-beads were added to lysates infected with GST-APC11 alone. The $alpha$ / $beta$ -tubulin proteins again copurified with APC10 and APC11. (C) To verify the interaction between APC10 and APC11, the same samples from B were blotted with $alpha$ -GST, confirming the identity of the GST-APC11 band.

To identify subunits that interact with APC2, the His₆-tagged APC2 virus was used to infect Sf9 cells together with otherviruses. The APC2 protein was then purified with Ni²⁺-NTA beads and analyzed by SDS-PAGE. We confirmed that APC2 interactswith APC11, and found no other strong interactions between APC2and the rest of APC subunits (our unpublished data). Therefore,APC2 and APC11 formed a complex in the absence of the other APCsubunits.

We next tested whether the subcomplex of APC2 and APC11 (APC2/11) was sufficient to support ubiquitination of APC substrates.With the use of UbcH10 as E2, APC2/11 catalyzed the ubiquitinationof human securin, whereas either APC2 or APC11 alone had no activity(Figure 3A). Consistent with previous reports, APC11 alone expressedeither in bacteria or insect cells was sufficient to ubiquitinatehuman securin in the presence of Ubc4 (Figure 3B). Similar datawere obtained with the use of human cyclin B1 as the substrate(our unpublished data). Therefore, APC2/11 represents the minimalligase module of APC, because it supports the ubiquitination ofAPC substrates with the use of either Ubc4 or UbcH10 as E2s.

View larger version (32K):
[in this window]
[in a new window]

Figure 3. Heterodimeric complex of APC2 and APC11 possesses ubiquitin ligase activity. (A) Hi5 cells were either infected with His₆-APC2 (lanes 2 and 7) and His₆-APC11 (lanes 3 and 8) viruses individually, or coinfected with the His₆-APC2 and His₆-APC11 viruses (lanes 4 and 9). The APC2 and APC11 proteins were purified with Ni²⁺-NTA beads and assayed for ubiquitination activity with the use of UbcH10 as the E2 enzyme and wild-type human securin (lanes 1-5) or a D-box deletion mutant ( $Delta$ DB) of securin (lanes 6-10) as the substrates. Bacterial expressed GST-APC11 protein purified with glutathione-agarose beads was also tested for ligase activity (lanes 5 and 10). (B) Same as A except that Ubc4 was used as the E2 enzyme instead of UbcH10.

Ubc4 Interacts with APC11, whereas UbcH10 Binds to APC2

Both Ubc4 and UbcH10 support the ubiquitination reactions catalyzed by APC in an additive manner (Yu et al., 1996). It isunclear which enzyme is the physiological E2 of the APC pathway.Microinjection of a UbcH10 dominant-negative mutant protein intomammalian cells arrested cells in mitosis (Townsley et al., 1997).In addition, mutation of the Schizosaccharomyces pombe homologof UbcH10, UbcP4, caused accumulation of cells in mitosis, similarto mutations of APC subunits (Osaka et al., 1997). These findingssuggest that UbcH10 might be involved in the mitotic degradationsystem in living cells. However, in budding yeast, mutations ofeither the Ubc4/5 family E2s or the UbcH10 homolog Ubc11 did notcause obvious mitotic phenotype (Townsley and Ruderman, 1998).To further clarify this issue, we immunodepleted UbcX, the Xenopushomolog of UbcH10, from the mitotic Xenopus egg extract that containsactive APC and degrades APC substrates with fast kinetics. Asshown in Figure 4A, the $alpha$ -UbcX antibody beads effectively depletedthe UbcX protein from the mitotic extract. Although the mitoticextract depleted with a control antibody degraded cyclin B1 witha half-life of 5-10 min, cyclin B1 was stabilized in the UbcX-depletedextract. Because the concentration of UbcX in mitotic Xenopusextracts was estimated to be 50 nM by semiquantitative immunoblotting(our unpublished data), we added 50 nM of recombinant purifiedUbcX expressed in bacteria back to the UbcX-depleted extract.Addition of the bacterially expressed UbcX restored the abilityof the mitotic extract to degrade cyclin B1. Taken together, UbcXis required for proper degradation of cyclin B1, and possiblyother APC substrates, in Xenopus egg extracts. Unfortunately,we did not have access to an antibody that can immunodeplete Ubc4from these extracts, and thus could not do similar experimentsfor Ubc4.

View larger version (36K):
[in this window]
[in a new window]

Figure 4. Ubc4 binds to the ring protein APC11 whereas UbcH10 binds to the cullin protein APC2. (A) Xenopus homolog of UbcH10, UbcX, was immunodepleted from mitotic Xenopus egg extracts with the use of a polyclonal $alpha$ -UbcX antibody coupled to Affiprep protein A beads (compare lanes 1 and 2). The preimmune serum was used as the control. The kinetics of cyclin B1 degradation was assayed in the control-depleted extract (top), the UbcX-depleted extract (middle), and the UbcX-depleted extract with physiological amount of purified UbcX added back (bottom). (B) Binding assays among Ubc4, UbcH10, APC2, and APC11. Purified His₆-tagged Ubc4 and UbcH10 proteins were immobilized on Ni²⁺-NTA beads and incubated with ³⁵S-labeled APC2 or APC11 proteins. After washing, the ³⁵S-labeled proteins bound to beads were analyzed by SDS-PAGE followed by autoradiography. (C) Sequence alignment of the RING-binding loops of human Ubc4, UbcH7, and UbcH10.

We next examined why APC2 was not required for the ubiquitination reactions of Ubc4. As shown in Figure 4B, UbcH10 interactedstrongly with APC2, whereas it did not bind to APC11. In contrast,Ubc4 associated directly with APC11. It did not exhibit significantbinding toward APC2. This finding explains why APC2 is only requiredfor UbcH10-catalyzed reactions. The two E2s may recognize differentbinding determinants within the APC2/11 ligase module. The factthat UbcH10 did not bind APC11 is consistent with previous structuralstudies on the interactions between the Cbl RING domain and UbcH7,an E2 of the Ubc4 subfamily (Zheng et al., 2000). The two loopsthat are critical for binding to RING domains are conserved betweenUbc4 and UbcH7 (Figure 4C). On the other hand, UbcH10 containsquite divergent amino acid sequences in these two loops. Therefore,Ubc4 and UbcH10 may be recruited to the intact APC with distinctmechanisms: Ubc4 recognize APC11 initially, whereas UbcH10 firstinteracts with APC2. However, it remains possible that, once theyare bound to APC, Ubc4 and UbcH10 occupy a similar site on APCand use a similar mechanism for transferringubiquitin.

Cullin Domain of APC2 Interacts with APC11 and UbcH10

We next mapped the regions within APC2 that interact with APC11 and UbcH10. A series of truncation mutants of APC2 were constructedand tested for binding to APC11 and UbcH10. A C-terminal fragmentof APC2, APC2e, spanning residues 549-822, was sufficient forbinding to APC11 and UbcH10 (Figure 5A). This region almost coincideswith the cullin homology region of APC2 that includes residues512-750 (Yu et al., 1998). Interestingly, even although APC2 andAPC11 formed an active complex when they were coexpressed in insectcells, the full-length APC2 protein did not bind to APC11 in thisassay. This is consistent with the fact that, when APC2 and APC11were expressed individually in insect cells and mixed after purification,no ubiquitin ligase activity was observed. Therefore, the full-lengthAPC2 protein could not form a complex with APC11 post-translationally.However, smaller fragments of APC2 were able to bind to APC11(Figure 5A).

View larger version (33K):
[in this window]
[in a new window]

Figure 5. Cullin domain of APC2 is sufficient for binding to both APC11 and UbcH10. (A) Purified His₆-tagged APC11 and UbcH10 proteins were immobilized on Ni²⁺-NTA beads and incubated with ³⁵S-labeled APC2 or various APC2 truncation mutant proteins. After washing, the proteins retained on beads were analyzed by SDS-PAGE followed by autoradiography. (B) Complex of the cullin domain of APC2 and APC11 possesses ubiquitin ligase activity. A series of APC2 truncation mutants were expressed in insect cells together with APC11. APC proteins were purified with Ni²⁺-NTA beads and assayed for ubiquitination activity. (C) Purified APC2e/11 complex was analyzed by SDS-PAGE followed by Coomassie staining.

Because APC2e binds to both APC11 and UbcH10, we examined whether the APC2e/11 complex was an active ubiquitin ligase. TheAPC fragments were coexpressed with APC11 in insect cells, andassayed for their ability to ubiquitinate cyclin B1 in the presenceof UbcH10. The APC2b and APC2e fragments ubiquitinated cyclinB1 efficiently (Figure 5B); both of these fragments retained theability to bind to APC11 and UbcH10 (Figure 5A). Therefore, acomplex of the cullin domain of APC2 and the RING finger proteinAPC11 is sufficient to catalyze ubiquitination of APC substrates,albeit with decreasedefficiency.

One potential caveat of reconstituting the APC activity in insect cells is that certain insect APC proteins might associatewith the expressed human APC proteins and contribute to the observedligase activity. To rule out this possibility, we purified theAPC2e/11 complex to homogeneity (Figure 5C) and determined thenative size of the APC2e/11 complex by gel filtration chromatographyand dynamic light scattering experiments. APC2e/11 cofractionatedas a single species with an apparent molecular mass of 50 kDaon the gel filtration column (our unpublished data). Based onthe intensity of staining on SDS-PAGE (Figure 5C), we estimatedthat APC2e and APC11 formed a complex of 1:1 stoichiometry. Thecalculated molecular mass of the complex is thus 50 kDa. Basedon the light scattering experiment, the APC2e/11 complex was mono-dispersedwith an apparent molecular mass of 46 kDa. Therefore, it is extremelyunlikely that the APC2e/11 complex contains any insectproteins.

Zn²⁺-binding of APC11 Is Essential for Its Ubiquitin Ligase Activity

Because other RING finger proteins are known to coordinate Zn²⁺ ions, APC11 may also bind Zn²⁺. However, this has not been demonstrated experimentally. We thusperformed a Zn²⁺-binding assay on the purified APC2e/11 complex (Yu and Schreiber,1995). Surprisingly, based on four measurements, we found thatAPC2e/11 bound Zn²⁺ at a molar ratio of 3.2 ± 0.2. Similar results were obtainedwith purified GST-APC11 protein expressed in bacteria. Therefore,it appeared that, in addition to the two Zn²⁺ ions coordinated by the canonical RING finger motif, APC11 containeda third Zn²⁺-binding site (Figure 6A). Sequence alignment of the APC11 andRbx1 proteins from various organisms reveals that three cysteines(Cys 34, Cys 37, and Cys 44 in human APC11) and one histidine(His 58 in human APC11) are conserved among these proteins (Figure6A). These conserved residues do not belong to the canonical RING-H2finger motif, and thus are good candidates for coordinating thethird Zn²⁺ ion.

View larger version (68K):
[in this window]
[in a new window]

Figure 6. One APC11 protein molecule binds three Zn²⁺ ions. (A) Sequence alignment of APC11 and Rbx1 from various organisms (Hs, Homo sapiens; Dm, Drosophila melanogaster; Sc, Saccharomyces cerevisiae; and Sp, S. pombe). The residues that coordinate the two Zn²⁺ ions of the canonical RING finger motif are labeled as open and closed circles, respectively. The residues for coordinating the third Zn²⁺ ion are labeled as open triangles. (B) Autoubiquitination assay of the APC11 mutants. ³⁵S-labeled APC11 mutants were translated in vitro in reticulocyte lysate and incubated with a mixture of ubiquitin, ATP, and E1 in the presence and absence of Ubc4. The reaction mixture was separated on SDS-PAGE followed by autoradiography. The Zn²⁺-coordinating residues are labeled as in A. The mutations that affect Zn²⁺-binding are indicated by +, whereas the mutations that do not affect zinc binding are marked by $-$ .

To determine the residues that coordinate Zn²⁺ ions, all cysteines and histidines of human APC11 were individually mutated toserines and alanines, respectively. Mutations of the Zn²⁺-binding ligands of the RING finger motif markedly reduced theexpression levels of these proteins in bacteria (our unpublisheddata). Similar results were obtained when Cys 34, Cys 37, Cys44, and His 58 were mutated. In contrast, mutations of Cys 7,Cys 33, Cys 54, His 65, and His 72 had no effect on the expressionlevels of the APC11 protein (our unpublished data). These findingsare consistent with the notion that Cys 34, Cys 37, Cys 44, andHis 58 coordinate the third Zn²⁺ ion. It is possible that mutations of the Zn²⁺-binding ligands destabilized the tertiary structure of APC11,resulting in the reduced level of expression of APC11. Obviously,loss of expression of APC11 mutant proteins in bacteria can becaused by factors other than protein folding. Because the APC11mutant proteins that involve the putative Zn²⁺-binding ligands could not be obtained at sufficient purity andquantity, we could not determine whether mutations of these ligandsactually caused the loss of Zn²⁺-binding.

When coexpressed with APC2, the APC11 mutants that did not affect Zn²⁺-binding still possessed ubiquitin ligase activity toward cyclinB1 in the presence of UbcH10 (our unpublished data). Because theAPC11 mutants that perturbed Zn²⁺-binding were not expressed well, we could not compare the ubiquitinligase activities of these mutants with those of the wild typeor mutants that did not affect Zn²⁺-binding. To circumvent this problem, we obtained all APC11 mutantproteins with the use of the in vitro transcription and translationsystem in rabbit reticulocyte lysate. Many RING finger-based ubiquitinligases also autoubiquitinate in the presence of the proper E2enzyme. We therefore tested the autoubiquitination activity ofthe APC11 mutants in the presence of Ubc4. The wild-type APC11protein and the APC11 mutants that did not affect Zn²⁺-binding were ubiquitinated efficiently when Ubc4 was added, basedon the appearance of APC11-ubiquitin conjugates and the percentageof APC11 conjugated to ubiquitin (Figure 6B). Mutations of theeight Zn²⁺-binding ligands of the RING finger motif greatly reduced theautoubiquitination activity of APC11 (Figure 6B). In contrast,mutations of Cys 34, Cys 37, Cys 44, and His 58 that coordinatedthe third Zn²⁺ only slightly reduced the autoubiquitination activity of APC11(Figure 6B). Thus, unlike the two Zn²⁺ ions of the RING-H2 finger motif, the third Zn²⁺ of APC11 might not be involved in catalysis (Figure 6B). ThisZn²⁺ ion may only be important for maintaining the structural integrityof APC11. We also tested the binding of all APC11 mutants to APC2e.None of the mutations affected the binding of APC11 to APC2 (ourunpublished data). Because the N-terminal region of APC11 andRbx1 proteins is conserved and this region is not present in otherRING-finger proteins, we speculate that the N-terminal 20 residuesof APC11 and Rbx1 proteins are involved in binding to APC2 andCul1,respectively.

Zn²⁺ Ions Alone Stimulate Activity of Ubc4 to Ubiquitinate Cyclin B1

Recently, many RING finger proteins have been shown to possess ubiquitin ligase activities. Despite the relatively low sequencehomology outside the RING finger motif, several RING finger proteinsuse the Ubc4/5 family of E2 enzymes in the ubiquitination reactions(Joazeiro et al., 1999; Lorick et al., 1999; Gmachl et al., 2000;Leverson et al., 2000). This suggested to us that the Zn²⁺ ions, the most obvious common feature of these RING finger proteins,might be directly involved in catalysis. Strikingly, we foundthat Zn²⁺ ions alone stimulated the ability of Ubc4 to ubiquitinate cyclinB1 (Figure 7A). Several other divalent cations, such as Cd²⁺, Co²⁺, and Ni²⁺, also enhanced the activity of Ubc4, whereas Mn²⁺, Mg²⁺, Ca²⁺, and Yb³⁺ had no effects (Figure 7, A and B). None of these cations stimulatedthe activity of UbcH10, which did not bind to RING proteins directly(our unpublished data). These findings further support the notionthat Zn²⁺ may be directly responsible for the activity of the RING finger-containingubiquitin ligases.

View larger version (28K):
[in this window]
[in a new window]

Figure 7. Zn²⁺ ions alone stimulate the ubiquitination activity of Ubc4. (A) Various concentrations of Zn²⁺, Cd²⁺, and other divalent cations were added to a reaction mixture containing E1, ubiquitin, Ubc4, ATP, and cyclin B1. Ubiquitination of cyclin B1 was analyzed by immunoblotting with $alpha$ -Myc. (B) Various concentrations of Zn²⁺ and Yb³⁺ were added to a reaction mixture containing E1, ubiquitin, Ubc4, ATP, and cyclin B1. Ubiquitination of cyclin B1 was analyzed by immunoblotting with $alpha$ -Myc. (C) Comparison of the ubiquitin ligase activities of the intact APC^Cdc20, the reconstituted APC, and zinc ions alone. The ligase activity of APC^Cdc20 was plotted against the concentration used in the assay. The activities of the reconstituted APC at 5 µM and zinc ions alone at 100 µM were indicated by closed circle and triangle, respectively.

We next quantitatively compared the activities of the intact APC^Cdc20, the reconstituted APC, and the Zn²⁺ ions alone. Various concentrations of APC^Cdc20 were used in the in vitro ubiquitination assay with the use ofcyclin B1 as the substrate. The ligase activity of APC was measuredby the intensities of the cyclin-ubiquitin conjugates, which werenormalized by the number of ubiquitin molecules in the conjugates(Figure 7C). The activity of the reconstituted APC at 5 µM wassimilar to that of the intact APC^Cdc20 at 90 nM, indicating that the intact APC^Cdc20 was 55 times more active than the reconstituted APC. Zinc ionsat 100 µM exhibited ligase activity comparable to 25 nM of APC^Cdc20. Thus, the activity of zinc ions alone was 4000 weaker than thatof the intactAPC.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

APC as a Member of Cullin-RING Finger Family of Ubiquitin Ligases

Among the three classes of enzymes of the ubiquitin pathway, the ubiquitin ligases are the most divergent, in terms of bothcomposition and function (Hershko and Ciechanover, 1998). Allubiquitination systems use a single ubiquitin-activating enzyme(E1) for the first step of the reaction (Hershko and Ciechanover,1998). Although certain ubiquitin-conjugating enzymes (E2s) areused in different ubiquitination systems, all E2 enzymes are homologousin sequence and contain the ubiquitin-conjugation (UBC) domain(Hershko and Ciechanover, 1998). In contrast, the ubiquitin ligases(E3s) are loosely defined as entities that collaborate with E1and E2 to ligate ubiquitin chains on substrates. They can be unrelatedin amino acid sequence and use distinct biochemical mechanismsforcatalysis.

The E3s identified so far can be divided into three major families. The first family consists of HECT domain-containing proteins(Scheffner et al., 1995). The second family of E3s includes Ubr1,c-Cbl, Mdm2, IAPs, and other RING finger-containing proteins,which appear to contain both the E2-binding domain and the substraterecognition motif in a single polypeptide chain (Joazeiro et al.,1999; Xie and Varshavsky, 1999; Fang et al., 2000; Yang et al.,2000). In contrast, the third group of E3s consists of large proteincomplexes that contain a minimal ligase core of a cullin and RING-H2heterodimer, such as the SCF and the VBC complexes (Deshaies,1999; Kamura et al., 1999). Based on the data presented herein,the minimal ligase module of APC is comprised of APC2 (a distantmember of the cullin family) and APC11 (a RING-H2 finger protein).Therefore, APC belongs to the third group of ubiquitin ligases(Figure 8A).

View larger version (32K):
[in this window]
[in a new window]

Figure 8. (A) APC belongs to the cullin-RING family of ubiquitin ligases. (B) Proposed role of Zn²⁺ in Ubc4-catalyzed ubiquitination reactions. See DISCUSSION for details.

Substrate Recognition by APC and Its Regulation during Cell Cycle

In addition to the fact that APC, SCF, and VBC ligase complexes all contain a cullin-RING finger heterodimeric ligase core,there is another analogy between APC and the other two systems(Figure 8A). The minimal ligase modules of these complexes areconnected to various adaptor proteins that serve to recruit substrates.In the case of SCF complex, the substrate-binding proteins, suchas Cdc4, Grr1, Skp2, and $beta$ -TRCP, contain the F-box motif and interactwith Skp1, which in turn associates with the cullin protein Cdc53or hCul1 (Deshaies, 1999). Likewise, VHL, the substrate receptorof the VBC ligase complex, is tethered to the hCul2/Rbx1 ligasecore through the elongin C protein, which shares structural similaritywith Skp1 (Kamura et al., 1999). The association between VHL andthe elongin BC complex is mediated by the SOCS-box motif of VHL(Kamura et al., 1998). The substrate recognition factors of APCare the WD40 repeat-containing proteins Cdc20 and Cdh1 (Burtonet al., 2001; Hilioti et al., 2001; Pfleger et al., 2001). Wehave observed direct binding between Cdc20 or Cdh1 and the APC2/11ubiquitin ligase core (our unpublished data). However, bindingof Cdc20 or Cdh1 to APC2/11 does not stimulate the ligase activityof APC2/11. Thus, it is unclear which subunit(s) of APC is requiredto anchor Cdc20 or Cdh1 to the ligase core in a functional way.It is also unknown what structural feature of Cdc20 and Cdh1 isrecognized byAPC.

The minimal ligase modules of APC and other cullin-RING type of E3s appear to be constitutively active, at least in vitro(Seol et al., 1999). The regulation of the ubiquitination processesinvolving these enzymes resides in substrate binding. However,APC differs significantly from the SCF and VBC complexes in thespecific mode of regulating substrate binding. Both SCF and VBCcomplexes recognize post-translationally modified substrates:the F-box proteins of SCF complexes bind phosphorylated proteinsubstrates, whereas the VHL protein of the VBC complex recognizesa novel hydroxyproline moiety of the HIF substrate (Skowyra etal., 1997; Ivan et al., 2001; Jaakkola et al., 2001). Therefore,the critical regulation of SCF and VBC pathways is at the levelof the substrates. In contrast, although all APC substrates containspecific sequence motifs, such as the D-box and KEN-box, post-translationalmodifications of the APC substrates are not required for theirefficient ubiquitination. Instead, it is the association of Cdc20or Cdh1 to APC that is tightly regulated during the cell cycle.Dissociation of Cdc20 or Cdh1 from APC during the S, G2, and prophaseof the cell cycle, in essence, serves to inhibit the substratebinding ability and thus the activity of APC (Fang et al., 1998).

Mechanism of Ubiquitin Transfer of APC-catalyzed Reactions

E3-catalyzed ubiquitination reactions may use two distinct mechanisms for conjugating ubiquitin to substrates. In the caseof E6-AP-mediated ubiquitination of p53, Ubc4 (the E2 in the system)first transfers ubiquitin to E6-AP to form an E3-ubiquitin thioester,which then attaches the ubiquitin to the lysine residues of p53(Scheffner et al., 1995). However, this does not seem to be theprevailing mechanism for all ubiquitination reactions. For theSCF complexes, it appears that the ubiquitination reactions donot involve the formation of an E3-ubiquitin thioester (Seol etal., 1999). Instead, the SCF complexes serve as a scaffold tobring together the E2 enzyme Cdc34 and the substrates. The RINGprotein Rbx1 of SCF enhances the ubiquitin transfer activity ofCdc34, and ubiquitin is then transferred directly from the Cdc34thioester tosubstrates.

Aside from the analogy between APC and SCF, there is additional evidence to suggest that APC might also use the latter scaffoldingmechanism for ubiquitin transfer. First, we and others were unableto detect a ubiquitin thioester of any APC subunits so far. Second,in the presence of active APC^Cdc20 or APC^Cdh1, Ubc4 seems to generate cyclin-ubiquitin conjugates of highermolecular weight than those generated by UbcH10 (Figure 1B) (Yuet al., 1996). The E3-thioester model would predict that, no matterwhich E2 is used, the same APC-ubiquitin thioester acts as theintermediate for relaying the ubiquitin to cyclin. The two E2swould then have little influence over the pattern of cyclin-ubiquitinconjugates. Therefore, the fact that Ubc4 and UbcH10 support theformation of cyclin-ubiquitin conjugates with different patternsfavors the scaffolding model. One possible explanation for thehigher molecular weight conjugates catalyzed by Ubc4 might bethat Ubc4 transfers ubiquitin faster than UbcH10. Thus, duringthe residence time of substrate binding to APC, Ubc4 might rechargeand transfer ubiquitin more frequently than UbcH10, thus forminghigher molecular weight conjugates than UbcH10. Finally, all cysteinesof APC11 have been mutated. Except the cysteines coordinatingZn²⁺ ions, mutation of other cysteines does not abolish the ubiquitinligase activity of APC11 with Ubc4 as the E2. Therefore, it isunlikely that an APC-ubiquitin thioester is involved in theseubiquitinationreactions.

Role of Zn²⁺ Ions in Catalysis

The Zn²⁺ ions of the RING finger E3 ligases are clearly essential for maintaining the structural integrity of these proteins.Besides the structural role, are the Zn²⁺ ions of the RING finger proteins also directly involved in catalysis,similar to many Zn²⁺-binding metalloenzymes? Two lines of evidence presented hereinsuggest that this might be the case. First, we found that APC11binds a third Zn²⁺ ion, aside from the two Zn²⁺ ions that form the RING finger motif. Mutations of the residuesthat coordinate the third Zn²⁺ appear to destabilize the structure of APC11. Yet, these APC11mutants still possess E3 ligase activity. In contrast, mutationsof the Zn²⁺-binding residues of the canonical RING motif not only disruptprotein structure but also abrogate the ligase activity of APC11.This suggests that, in addition to the structural role, the twoZn²⁺ ions of the RING motif might be directly involved in catalysis.This notion is further strengthened by the unexpected findingthat Zn²⁺ ions alone can stimulate the ability of Ubc4 to ligate ubiquitinto cyclin B1. Zn²⁺ might facilitate two steps in the ubiquitin ligation reaction(Figure 8B). It might stabilize the oxyanion of the putative tetrahedralintermediate of the reaction. Along this line, it is worth notingthat polycations can stimulate the autoubiquitination activityof Cdc34, and the polycations have been proposed to stabilizethe oxyanion intermediate (Seol et al., 1999; Zachariae and Nasmyth,1999). Zn²⁺ might also promote the release of the active thiol group of theE2 from the tetrahedral intermediate. Consistent with this notion,several cations that can potentially coordinate oxyanions, suchas Cu²⁺ and Yb³⁺, do not have the same effect as Zn²⁺. Obviously, the mechanism by which Zn²⁺ ions at high concentrations catalyze the ubiquitination reactionmay not mimic the mode of action of the RING-containing ubiquitinligases. Further experiments are required to clarify theseissues.

	ACKNOWLEDGMENTS

We thank Marc Kirschner for encouragement at the early stages of this project. We also thank Hui Zou for providing the humansecurin plasmids. This work is supported by the Damon Runyon-WalterWinchell Foundation, the Robert A. Welch Foundation, the BurroughsWellcome Fund, the Packard Foundation, and the National Institutesof Health grant GM-61542.

	FOOTNOTES

^§ Corresponding author. E-mail address: hongtao.yu{at}utsouthwestern.edu.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aristarkhov, A., Eytan, E., Moghe, A., Admon, A., Hershko, A., and Ruderman, J.V. (1996). E2-C, a cyclin-selective ubiquitin carrier protein required for the destruction of mitotic cyclins. Proc. Natl. Acad. Sci. 93, 4294-4299[Abstract/Free Full Text].
Burton, J.L., and Solomon, M.J. (2001). D box and KEN box motifs in budding yeast HSl1p are required APC-mediated degradation and direct binding to Cdc20p and Cdh1p. Genes Dev. 15, 2381-2395[Abstract/Free Full Text].
Deshaies, R.J. (1999). SCF and Cullin/Ring H2-based ubiquitin ligases. Annu. Rev. Cell Dev. Biol. 15, 435-467[Medline].
Fang, S., Jensen, J.P., Ludwig, R.L., Vousden, K.H., and Weissman, A.M. (2000). Mdm2 is a RING finger-dependent ubiquitin protein ligase for itself and p53. J. Biol. Chem. 275, 8945-8951[Abstract/Free Full Text].
Fang, G., Yu, H., and Kirschner, M.W. (1998). Direct binding of CDC20 protein family members activates the anaphase-promoting complex in mitosis and G1. Mol. Cell 2, 163-171[Medline].
Feldman, R., Correll, C.C., Kaplan, K.B., and Deshaies, R.J. (1997). A complex of Cdc4p, Skp1p, and Cdc53p/Cullin catalyzes ubiquitination of the phosphorylated CDK inhibitor Sic1p. Cell 91, 221-230[Medline].
Gmachl, M., Gieffers, C., Podtelejnikov, A.V., Mann, M., and Peters, J.-M. (2000). The RING-H2 finger protein APC11 and the E2 enzyme UBC4 are sufficient to ubiquitinate substrates of the anaphase-promoting complex. Proc. Natl. Acad. Sci. USA 97, 8973-8978[Abstract/Free Full Text].
Grossberger, R., Gieffers, C., Zachariae, W., Podtelejnikov, A.V., Schleiffer, A., Nasmyth, K., Mann, M., and Peters, J.-M. (1999). Characterization of the DOC1/APC10 subunit of the yeast and the human anaphase-promoting complex. J. Biol. Chem. 274, 14500-14507[Abstract/Free Full Text].
Hershko, A., and Ciechanover, A. (1998). The ubiquitin system. Annu. Rev. Biochem. 67, 425-479[Medline].
Hilioti, Z., Chung, Y., Mochizuki, Y., Hardy, C.F., and Cohen-Fix, O. (2001). The anaphase inhibitor Pds1 binds to the APC/C-associated protein Cdc20 in a destruction box-dependent manner. Curr. Biol. 11, 1347-1352[Medline].
Irniger, S., Piatti, S., Michaelis, C., and Nasmyth, K. (1995). Genes involved in sister chromatid separation are needed for B-type cyclin proteolysis in budding yeast. Cell 81, 269-277[Medline].
Ivan, M., Kondo, K., Yang, H., Kim, W., Valiando, J., Ohh, M., Salic, A., Asara, J.M., Lane, W.S., and Kaelin, W.G., Jr. (2001). HIF targeted for VHL-mediated destruction by proline hydroxylation: implications for O₂ sensing. Science 292, 464-468[Abstract/Free Full Text].
Jaakkola, P., et al. (2001). Targeting of HIF to the von Hippel-Lindau ubiquitylation complex by O₂-regulated prolyl hydroxylation. Science 292, 468-472[Abstract/Free Full Text].
Joazeiro, C.A., Wing, S.S., Huang, H., Leverson, J.D., Hunter, T., and Liu, Y.C. (1999). The tyrosine kinase negative regulator c-Cbl as a RING-type, E2-dependent ubiquitin-protein ligase. Science 286, 309-312[Abstract/Free Full Text].
Kamura, T., et al. (1999). Rbx1, a component of the VHL tumor suppressor complex and SCF ubiquitin ligase. Science 284, 657-661[Abstract/Free Full Text].
Kamura, T., Sato, S., Haque, D., Liu, L., Kaelin, W.G., Jr., Conaway, R.C., and Conaway, J.W. (1998). The Elongin BC complex interacts with the conserved SOCS-box motif present in members of the SOCS, ras, WD-40 repeat, and ankyrin repeat families. Genes Dev. 12, 3872-3881[Abstract/Free Full Text].
King, R.W., Deshaies, R.J., Peters, J.-M., and Kirschner, M.W. (1996a). How proteolysis drives the cell cycle. Science 274, 1652-1659[Abstract/Free Full Text].
King, R.W., Glotzer, M., and Kirschner, M.W. (1996b). Mutagenic analysis of the destruction signal of mitotic cyclins and structural characterization of ubiquitinated intermediates. Mol. Biol. Cell 7, 1343-1357[Abstract].
King, R.W., Peters, J.M., Tugendreich, S., Rolfe, M., Hieter, P., and Kirschner, M.W. (1995). A 20S complex containing CDC27 and CDC16 catalyzes the mitosis-specific conjugation of ubiquitin to cyclin B. Cell 81, 279-288[Medline].
Kipreos, E.T., Lander, L.E., Wing, J.P., He, W.W., and Hedgecock, E.M. (1996). Cul-1 is required for cell cycle exit in c-elegans and identifies a novel gene family. Cell 85, 829-839[Medline].
Kramer, E.R., Gieffers, C., Holzl, G., Hengstschlager, M., and Peters, J.-M. (1998). Activation of the human anaphase-promoting complex by proteins of the CDC20/Fizzy family. Curr. Biol. 8, 1207-1210[Medline].
Latres, E., Chiaur, D.S., and Pagano, M. (1999). The human F box protein $beta$ -Trcp associates with the Cul1/Skp1 complex and regulates the stability of $beta$ -catenin. Oncogene 18, 849-854[Medline].
Leverson, J.D., Joazeiro, C.A., Page, A.M., Huang, H., Hieter, P., and Hunter, T. (2000). The APC11 RING-H2 finger mediates E2-dependent ubiquitination. Mol. Biol. Cell 11, 2315-2325[Abstract/Free Full Text].
Lorick, K.L., Jensen, J.P., Fang, S., Ong, A.M., Hatakeyama, S., and Weissman, A.M. (1999). RING fingers mediate ubiquitin-conjugating enzyme (E2)-dependent ubiquitination. Proc. Natl. Acad. Sci. USA 96, 11364-11369[Abstract/Free Full Text].
Lyapina, S.A., Correll, C.C., Kipreos, E.T., and Deshaies, R.J. (1998). Human CUL1 forms an evolutionarily conserved ubiquitin ligase complex (SCF) with SKP1 and an F-box protein. Proc. Natl. Acad. Sci. USA 95, 7451-7456[Abstract/Free Full Text].
Marti, A., Wirbelauer, C., Scheffner, M., and Krek, W. (1999). Interaction between ubiquitin-protein ligase SCF^SKP2 and E2F-1 underlies the regulation of E2F-1 degradation. Nat. Cell Biol. 1, 14-19[Medline].
Morgan, D.O. (1999). Regulation of the APC and the exit from mitosis. Nat. Cell Biol. 1, E47-E53[Medline].
Murray, A.W. (1991). Cell cycle extracts. Methods Cell Biol. 36, 581-605[Medline].
Nasmyth, K., Peters, J.M., and Uhlmann, F. (2000). Splitting the chromosome: cutting the ties that bind sister chromatids. Science 288, 1379-1385[Abstract/Free Full Text].
Ohta, T., Michel, J.J., Schottelius, A.J., and Xiong, Y. (1999). ROC1, a homolog of APC11, represents a family of cullin partners with an associated ubiquitin ligase activity. Mol. Cell 3, 535-541[Medline].
Osaka, F., Seino, H., Seno, T., and Yamao, F. (1997). A ubiquitin-conjugating enzyme in fission yeast that is essential for the onset of anaphase in mitosis. Mol. Cell. Biol. 17, 3388-3397[Abstract].
Pfleger, C.M., and Kirschner, M.W. (2000). The KEN box: an APC recognition signal distinct from the D box targeted by Cdh1. Genes Dev. 14, 655-665[Abstract/Free Full Text].
Pfleger, C.M., Lee, E., and Kirschner, M.W. (2001). Substrate recognition by the Cdc20 and Cdh1 components of the anaphase-promoting complex. Genes Dev. 15, 2396-2407[Abstract/Free Full Text].
Scheffner, M., Nuber, U., and Huibregtse, J.M. (1995). Protein ubiquitination involving an E1-E2-E3 enzyme ubiquitin thioester cascade. Nature 373, 81-83[Medline].
Schwab, M., Lutum, A.S., and Seufert, W. (1997). Yeast Hct1 is a regulator of Clb2 cyclin proteolysis. Cell 90, 683-693[Medline].
Seol, J.H., et al. (1999). Cdc53/cullin and the essential Hrt1 RING-H2 subunit of SCF define a ubiquitin ligase module that activates the E2 enzyme Cdc34. Genes Dev. 13, 1614-1626[Abstract/Free Full Text].
Sigrist, S.J., and Lehner, C.F. (1997). Drosophila fizzy-related down-regulates mitotic cyclins and is required for cell proliferation arrest and entry into endocycles. Cell 90, 671-681[Medline].
Skowyra, D., Craig, K.L., Tyers, M., Elledge, S.J., and Harper, J.W. (1997). F-box proteins are receptors that recruit phosphorylated substrates to the SCF ubiquitin-ligase complex. Cell 91, 209-219[Medline].
Skowyra, D., Koepp, D.M., Kamura, T., Conrad, M.N., Conaway, R.C., Conaway, J.W., Elledge, S.J., and Harper, J.W. (1999). Reconstitution of G1 cyclin ubiquitination with complexes containing SCF^Grr1 and Rbx1. Science 284, 662-665[Abstract/Free Full Text].
Sudakin, V., Ganoth, D., Dahan, A., Heller, H., Hershko, J., Luca, F.C., Ruderman, J.V., and Hershko, A. (1995). The cyclosome, a large complex containing cyclin-selective ubiquitin ligase activity, targets cyclins for destruction at the end of mitosis. Mol. Biol. Cell 6, 185-198[Abstract].
Tan, P., Fuchs, S.Y., Chen, A., Wu, K., Gomez, C., Ronai, Z., and Pan, Z.Q. (1999). Recruitment of a ROC1-CUL1 ubiquitin ligase by Skp1 and HOS to catalyze the ubiquitination of I $kappa$ B $alpha$ . Mol. Cell 3, 527-533[Medline].
Townsley, F.M., Aristarkhov, A., Beck, S., Hershko, A., and Ruderman, J.V. (1997). Dominant-negative cyclin-selective ubiquitin carrier protein E2-C/UbcH10 blocks cells in metaphase. Proc. Natl. Acad. Sci. USA 94, 2362-2367[Abstract/Free Full Text].
Townsley, F.M., and Ruderman, J.V. (1998). Functional analysis of the Saccharomyces cerevisiae UBC11 gene. Yeast 14, 747-757[Medline].
Tugendreich, S., Tomkiel, J., Earnshaw, W., and Hieter, P. (1995). The CDC27HS protein co-localizes with the CDC16HS protein to the centrosome and mitotic spindle and is essential for the metaphase to anaphase transition. Cell 81, 261-268[Medline].
Uhlmann, F., Lottspeich, F., and Nasmyth, K. (1999). Sister-chromatid separation at anaphase onset is promoted by cleavage of the cohesin subunit Scc1. Nature 400, 37-42[Medline].
Uhlmann, F., Wernic, D., Poupart, M.A., Koonin, E.V., and Nasmyth, K. (2000). Cleavage of cohesin by the CD clan protease separin triggers anaphase in yeast. Cell 103, 375-386[Medline].
Visintin, R., Prinz, S., and Amon, A. (1997). CDC20 and CDH1 $---$ A family of substrate-specific activators of APC-dependent proteolysis. Science 278, 460-463[Abstract/Free Full Text].
Waizenegger, I.C., Hauf, S., Meinke, A., and Peters, J.M. (2000). Two distinct pathways remove mammalian cohesin from chromosome arms in prophase and from centromeres in anaphase. Cell 103, 399-410[Medline].
Willems, A.R., Lanker, S., Patton, E.E., Craig, K.L., Nason, T.F., Mathias, N., Kobayashi, R., Wittenberg, C., and Tyers, M. (1996). Cdc53 targets phosphorylated G1 cyclins for degradation by the ubiquitin proteolytic pathway. Cell 86, 453-463[Medline].
Xie, Y., and Varshavsky, A. (1999). The E2-E3 interaction in the N-end rule pathway: the RING-H2 finger of E3 is required for the synthesis of multiubiquitin chain. EMBO J. 18, 6832-6844[Medline].
Yang, Y., Fang, S., Jensen, J.P., Weissman, A.M., and Ashwell, J.D. (2000). Ubiquitin protein ligase activity of IAPs and their degradation in proteasomes in response to apoptotic stimuli. Science 288, 874-877[Abstract/Free Full Text].
Yu, H., King, R.W., Peters, J.-M., and Kirschner, M.W. (1996). Identification of a novel ubiquitin-conjugating enzyme involved in mitotic cyclin degradation. Curr. Biol. 6, 455-466[Medline].
Yu, H., Peters, J.-M., King, R.W., Page, A., Hieter, P., and Kirschner, M.W. (1998). Identification of a cullin homology region in a subunit of the anaphase-promoting complex. Science 279, 1219-1223[Abstract/Free Full Text].
Yu, H., and Schreiber, S.L. (1995). Cloning, Zn²⁺ binding, and structural characterization of the guanine nucleotide exchange factor human Mss4. Biochemistry 34, 9103-9110[Medline].
Zachariae, W., and Nasmyth, K. (1999). Whose end is destruction: cell division and the anaphase-promoting complex. Genes Dev. 13, 2039-2058[Free Full Text].
Zachariae, W., Shevchenko, A., Andrews, P., Galova, M., Stark, M., Mann, M., and Nasmyth, K. (1998). Mass spectrometric analysis of the anaphase-promoting complex from budding yeast: identification of a subunit related to cullins. Science 279, 1216-1219[Abstract/Free Full Text].
Zheng, N., Wang, P., Jeffrey, P.D., and Pavletich, N.P. (2000). Structure of a c-Cbl-UbcH7 complex: RING domain function in ubiquitin-protein ligases. Cell 102, 533-539[Medline].

This article has been cited by other articles: