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1 Department of Molecular and Cell Biology, University of California-Berkeley, Berkeley, California 94720, USA
2 Skaggs School of Pharmacy and Pharmaceutical Sciences, University of California–San Diego, La Jolla, California 92093, USA
3 College of Medicine, University of Florida, Gainesville, Florida 32610, USA
(RECEIVED December 11, 2006; FINAL REVISION January 15, 2007; ACCEPTED January 23, 2007)
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Abstract |
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 TOP Abstract IntroductionResults and DiscussionSummary and ConclusionsMaterials and MethodsData depositionAcknowledgmentsReferences |
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Keywords: M11L; poxvirus; apoptosis inhibitor; X-ray crystallography; Bcl-2 homology; fluorescence polarization; immunomodulation
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Introduction |
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TOPAbstractIntroductionResults and DiscussionSummary and ConclusionsMaterials and MethodsData depositionAcknowledgmentsReferences |
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M11L is critical for the virulence of myxoma virus, a member of the leporipoxvirus genus and the causative agent of a lethal rabbit-specific disease known as myxomatosis (Kerr and McFadden 2002). Rabbits infected with an M11L knockout virus develop an attenuated form of disease and ultimately make a full recovery, whereas infection with wild-type virus leads to complete mortality (Opgenorth et al. 1992). This led to the discovery that M11L is also capable of blocking apoptosis in a broad spectrum of mammalian cells, including human cells (Everett et al. 2000, 2002). The M11L protein is a small (166 residue) protein with a C-terminal transmembrane domain that localizes it to the outer mitochondrial membrane, where it exhibits antiapoptotic activity (Everett et al. 2000, 2002). M11L forms a complex with the peripheral benzodiazepine receptor (PBR), and this interaction protects against the loss of mitochondrial membrane potential, a key point in the apoptotic pathway. M11L and F1L also interact with members of the Bak/Bax family of pro-apoptotic regulators to block upstream signals that commit the cell to the death program (Wang et al. 2004; Wasilenko et al. 2005; Fischer et al. 2006; Postigo et al. 2006; Su et al. 2006; Taylor et al. 2006). Although it seems that M11L and F1L are mimicking the function of the Bcl-2 family of antiapoptotic proteins, how they manage to do so without any obvious homology with Bcl-2, has remained a mystery.
The Bcl-2 family of proteins act as gatekeepers for mitochondria-mediated apoptosis (Reed et al. 1998). Members are defined by the presence of at least one of four Bcl-2 homology (BH) motifs (Petros et al. 2004). The family is divided into two separate classes based on their functions: pro-apoptotic and antiapoptotic. The antiapoptotic proteins Bcl-2 and Bcl-xL contain all four BH motifs and are responsible for protecting the integrity of the mitochondrial outer membrane. The pro-apoptotic proteins and their functions can be divided into two classes depending on the BH motifs present. Bax-like proteins (e.g., Bax, Bak), directly responsible for disrupting the membrane, contain the BH1, BH2, and BH3 motifs, while BH3-only proteins, as their name implies, contain only a BH3 motif and promote apoptosis by inhibiting Bcl-2 and Bcl-xL as well as activating Bax. Bcl-2 and Bcl-xL inhibit apoptosis by dimerizing with Bak and Bax (Borner 2003; Sharpe et al. 2004). During apoptosis, BH3-only proteins interfere with the binding of these complexes releasing Bak and Bax, which are then able to form oligomers. The oligomers form a pore in the mitochondrial outer membrane leading to the loss of membrane potential and the release of apoptotic agents from the mitochondria (e.g., cytochrome c and Smac/DIABLO) (Marsden and Strasser 2003). Viral Bcl-2 homologs can act either by binding and sequestering the BH3-only proteins or by directly binding to Bak and Bax, forming complexes that are resistant to BH3-only protein interference (Cuconati and White 2002; Polster et al. 2004). The vBcl-2s are able to accomplish this because of their sequence and structural similarity to Bcl-2/Bcl-xL (Huang et al. 2002), but how viral inhibitors like M11L and F1L accomplish the same feat is unknown.
Sequence alignments show that there is no significant amino acid sequence similarity between M11L and Bcl-2/Bcl-xL. Although secondary structure predictions indicate that, like Bcl-2, M11L is entirely helical, threading analysis (3DPSSM) produced no significant hits. In order to determine exactly how M11L is able to bind Bak and Bax, the structure of M11L was solved. This communication reports the structural features of M11L that facilitate its interaction with Bak and Bax as well as the significance of its overall structure.
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Results and Discussion |
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TOPAbstractIntroductionResults and DiscussionSummary and ConclusionsMaterials and MethodsData depositionAcknowledgmentsReferences |
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143) was produced to remove a predicted C-terminal transmembrane region. M11L143 also expressed in an insoluble form, but when fused to the C terminus of His-tagged maltose binding protein (His6–MBP), it was soluble. Expression levels of the soluble His6–MBP–M11L143 fusion remained low even when expanded codon usage cells (BL21[DE3] Rosetta, Stratagene) were used. In order to increase the yield, an Escherichia coli codon optimized M11L gene was constructed. The codon optimized His6–MBP–M11L143 construct produced significantly higher levels of soluble protein, typically 
28 mg/L of fusion protein which corresponds to 7.5 mg/L of cleaved M11L143.
Consistent with secondary structure predictions, a circular dichroism (CD) spectrum of M11L showed that the protein is folded and helical (Fig. 1). Initial mass spectrometry results indicated that M11L143 contains one intramolecular disulfide (data not shown), which was not entirely unexpected as the protein contains six cysteine residues. To explore whether the disulfide was important for the structure, a CD spectrum was taken in the presence of 1 mM Tris(2-carboxyethyl phosphine) (TCEP), a potent reducing agent. The addition of TCEP had no effect on the overall spectrum, indicating that either the disulfide is not important for the structure/stability of M11L, or that the disulfide is resistant to TCEP, and therefore likely important to the structure (data not shown).
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-RMSD = 0.436 Å). An important crystal contact is made by the interaction of the C-terminal helix of chain B with a surface region on chain A. Likewise, the C-terminal helix of chain A binds the same surface on chain B in an adjacent unit cell. This interaction is critical to the crystal packing, and is discussed in more depth below. An intramolecular disulfide was found between Cys33 and Cys127, despite the crystals being grown in the presence of 1 mM TCEP, suggesting that it is structurally relevant; this is interesting, since most intracellular proteins do not contain disulfides because of the reducing environment in the cytoplasm, although some other examples have been reported (Prinz et al. 1997).
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-helices, the same fold, and they all contain a hydrophobic groove on their surface. Structural alignments of the 138 C atoms of M11L to those of Bcl-2 and Bcl-xL using LSQMAN (Kleywegt 1996) give an RMSD of 2.044 Å and 1.984 Å, respectively. Figure 2C shows an overlay of M11L (shown in yellow) onto Bcl-xL (blue). An alignment based on the overlay of M11L with Bcl-2 and Bcl-xL can be seen in Figure 4.
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-helix and loop region, M11L is still able to make structural interactions with helix 6 and 7, but may not be subject to the same regulation as Bcl-2/Bcl-xL. The NWGR sequence motif found at the beginning of helix 5 in the BH1 domain is highly conserved across all Bcl-2 family members, but it is noticeably absent from M11L (instead of the conserved sequence, M11L contains SPSV in the same position; Fig. 4). In Bcl-2 and Bcl-xL the tryptophan makes extensive contacts with residues in helix 7 and 8, whereas in M11L, the corresponding proline interacts much less with helix 7. Instead, it seems that M11L employs an intramolecular disulfide bond between Cys33 and Cys127 to help hold helix 7 in place. In addition there is a hydrogen bond between Lys80 and a backbone amide found in the loop between helices 6 and 7. These two interactions likely take the place of the interactions lost by the mutation of the conserved tryptophan.
Structural studies of Bcl-2 family proteins have led to a better understanding of how Bax and Bak may function and how various members of the family may interact. All of the members of the Bcl-2 family have the same fold, characterized by an -helical bundle arranged around a single central -helix (Muchmore et al. 1996; Sattler et al. 1997; Suzuki et al. 2000; Petros et al. 2001) . The structure of Bcl-xL also showed that the conserved BH1, BH2, and BH3 domains are all in close spatial proximity and form a shallow hydrophobic groove on the surface (Muchmore et al. 1996). It was proposed, and later confirmed via crystal structures, that this was the site for binding of Bak. When the crystal structure of Bcl-xL and a peptide fragment containing the Bak–BH3 domain was solved, the peptide was found bound in this elongated hydrophobic groove (Sattler et al. 1997). It is thought then that the hydrophobic grooves present on Bcl-2 and Bcl-xL mediate their binding to both Bak and Bax.
Based on similarities between the folds of M11L and Bcl-2 proteins, the hydrophobic groove present on the surface of M11L may be analogous to the groove found in both Bcl-2 and Bcl-xL. This idea is strengthened by a fortuitous crystal contact, in which the C-terminal helix of one molecule is found binding directly into this region of another molecule (Fig. 5). When the M11L structure is aligned with the Bcl-xL/Bak-peptide structure (PDB ID: 1BXL [PDB] ), the helix bound in the M11L structure overlays with the BH3-domain found bound in the Bcl-xL/Bak-peptide structure. However, the groove found on the surface of M11L is wider and slightly more shallow than the groove found in either Bcl-2 or Bcl-xL. This can be explained by the helix that is found bound in the pocket. The groove on M11L is similar in shape to the groove in the Bcl-xL/Bak-peptide structure (Fig. 6). In M11L, Tyr41 protrudes into the groove, creating a bump (Fig. 6A). An analogous large protrusion is not present in Bcl-2 or Bcl-xL, and its effect on binding is unknown at this time. As was found in the Bcl-xL/Bak-peptide structure, there is a hydrophobic pocket that accommodates the highly conserved leucine found in the Bak and Bax BH3 domains (Fig. 6B). In M11L, this pocket is formed by Tyr41, Tyr45, Leu48, Ala82, and Leu86, whereas in Bcl-xL it is formed by Phe97, Tyr101, Leu130, Ala142, and Phe146. The electrostatic distribution around the binding groove in M11L is also very different from that of Bcl-2 and Bcl-xL. As shown in Figure 5, the binding groove of Bcl-xL is immediately lined with Arg100 and Arg103 on one side and Glu129, Arg132, and Arg139 on the other. In contrast, M11L has Lys43 and Asp50 on one side and Arg73 and Asp74 on the other, but these charged residues are further removed from the binding pocket and are unlikely to interact with a bound peptide. The majority of the charge differences are unlikely to affect binding since analysis of Bcl-xL binding to the Bak BH3 domain showed that the only charged residue making an important stabilizing interaction with the peptide was Arg139 (Sattler et al. 1997). There is no homologous residue to Arg139 found in the hydrophobic groove of M11L, so it is unclear how M11L makes up for this loss of binding energy. It was previously reported that M11L contained a putative BH3 domain (Wang et al. 2004). Analysis of this region indicates that the conserved residues are all buried in M11L as they are in Bak and Bcl-xL. It is unclear at this time whether this domain is functional in binding other Bcl-2 proteins or simply important for the overall structure of M11L.
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143 for the peptide. The Kd was determined to be 4.86 ± 0.334 µM. This affinity is 10-fold lower than the affinity of Bak for Bcl-xL (Petros et al. 2000), but it is similar to the affinity of Bak for Bcl-2 (Petros et al. 2001), suggesting that binding to M11L is physiologically relevant. The ability of M11L to bind the peptide confirms that the purified protein is natively folded, and supports the model that M11L acts directly as a structural mimic of the Bcl-2 pro-survival proteins.
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Summary and Conclusions |
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TOPAbstractIntroductionResults and DiscussionSummary and ConclusionsMaterials and MethodsData depositionAcknowledgmentsReferences |
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The discovery that M11L is a Bcl-2 homolog sheds some light on the possible structures of a number of other poxvirus proteins (Table 3). Although it has no sequence homology with M11L, it is likely that F1L and similar proteins are also Bcl-2 homologs. This is further strengthened by the recent structure of the vaccinia virus N1L protein (Aoyagi et al. 2007). N1L has no sequence homology with Bcl-2, but adopts a similar fold and has been shown to bind the BH3 domain from Bak. According to phylogenetic analysis, pox viruses can be broken into four distinct groups (Gubser et al. 2004). Avipoxvirus genus (FPV), Molluscipoxvirus genus (MCV), and the Orthopox genus (OPV) each form separate groups while the Yatapoxvirus, Capripoxvirus, Suipoxvirus, and Leporipoxvirus genera all cluster together (Fig. 8). Interestingly, each of the groups seems to contain its own Bcl-2 homolog. FPVs are the only poxviruses that possess "classic" Bcl-2 sequence homologs, but many of the OPVs, including camelpox, cowpox, variola, and monkeypox, contain a protein that is similar to F1L from the vaccinia virus. In the last group, rabbit fibroma virus has a very close homolog to M11L, while sheeppox, goatpox, lumpy skin disease virus, swinepox, and deerpox all express a more distant relative. It is quite interesting that the poxvirus family, unlike Herpes viruses that express clear Bcl-2 homologs, expresses multiple different proteins with very little homology with Bcl-2, yet they all inhibit apoptosis by binding to Bak, and in some cases to Bax. How many other virus families possess cryptic Bcl-2 homologs is currently unknown. Further structural analysis of both M11L and F1L may lead to the identification of new sequence motifs that can be used to search out these unknown Bcl-2 homologs.
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Materials and Methods |
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TOPAbstractIntroductionResults and DiscussionSummary and ConclusionsMaterials and MethodsData depositionAcknowledgmentsReferences |
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143), was cloned into the pSV272 expression vector (N. Pokala and T.M. Handel, unpubl.) to produce a fusion of M11L to the C terminus of His6–MBP (His6–MBP–M11L143). A tobacco etch virus (TEV) protease site was placed between the MBP and M11L143 to allow for cleavage of the fusion protein, leaving a Gly–Ala on the N terminus of M11L143 (Kapust and Waugh 1999).
Protein expression and purification
The His6–MBP–M11L143 fusion protein was expressed in E. coli BL21(DE3)pLysS cells (Stratagene) by inducing with 1 mM isopropyl-
-D-thiogalactopyranoside (IPTG) at OD600 = 0.6 for 4 h. Cells were harvested and spun down at 6000g at 4°C and resuspended in buffer (50 mM potassium phosphate [pH 8.0], 300 mM NaCl, 20 mM imidazole). Protease inhibitors (Complete: EDTA-free, Roche Diagnostics) were added and the cells were then frozen in liquid nitrogen.
For purification, cells were ruptured using an Emulsiflex C5 (Avestin Inc.) at 12,000 PSI and centrifuged at 25,000g for 20 min at 4°C. The supernatant was run over Ni-NTA resin (Qiagen) and the peak fractions pooled. Pooled protein was then concentrated via ultrafiltration (Centriprep YM-10, Millipore) and cleaved for 1 h at room temperature using a 1:100 molar ratio of TEV protease:M11L-fusion protein. The cleavage reaction was dialyzed against 50 mM potassium phosphate pH 8.0, 300 mM NaCl at 4°C overnight and run over a Ni-Sepharose column (GE Healthcare). The flow-through was concentrated and passed over an S75 gel filtration column (GE Healthcare). The peak fractions were then pooled and concentrated via ultrafiltration (Centriprep YM-3, Millipore). The protein sequence was verified via electrospray mass spectrometry (courtesy of Dr. David King, UC: Berkeley and HHMI).
Selenomethionine-labeled protein was expressed via the method of Van Duyne et al. (1993) and purified as described for native His6–MBP–M11L143 with the addition of 1 mM -mercaptoethanol at all steps up to gel filtration when 1 mM Tris(2-carboxyethyl phosphine) (TCEP) was used instead.
Circular dichroism
M11L143 was dialyzed into 20 mM potassium phosphate (pH 7.5), 100 mM NaCl. Circular dichroism (CD) data was collected on an Aviv 62DS spectropolarimeter (25°C, 1-cm path length).
Crystallization and structure determination
Purified selenomethionine-derivatized M11L143 was dialyzed against 20 mM potassium phosphate (pH 7.4), 100 mM NaCl, and 1 mM TCEP overnight. The protein was then concentrated to 13.5 mg/mL. Crystals were grown via hanging drop vapor diffusion by mixing 1 µL M11L143 with 1 µL of well solution containing 100 mM sodium citrate (pH 5.5), 700 mM ammonium sulfate, and 200 mM KCl. For harvesting, crystals were transferred to a cryoprotectant solution containing well solution plus 30% xylitol before flash freezing in liquid nitrogen.
All data sets were collected on Beamline 8.3.1 at the Advanced Light Source at Lawrence Berkeley National Laboratory (MacDowell et al. 2004). Data were indexed using HKL2000 (Otwinowski et al. 1997), and heavy atom sites were determined from SAD data using Solve (Terwilliger 2004). Heavy atom sites were refined and phases solved using MLPHARE (Collaborative Computational Project 1994) implemented by ELVES (Holton and Alber 2004). Initial density modification was undertaken by RESOLVE (Terwilliger 2004), and manual model building was performed with O (Jones et al. 1991). The model was refined using Refmac5 (Collaborative Computational Project 1994), followed by TLS refinement in Refmac5 (Winn et al. 2001). The model was refined, along with several rounds of manual rebuilding, to a resolution of 2.91 Å, and a final working R-factor of 24.9% and R free of 29.0%. The final model consisted of residues 1–138 of M11L. A total of 90.1% of nonglycine residues are in the most favored regions of Ramachandran space, with 8.3% in additional allowed areas and 1.6% in generously allowed areas (Table 1).
Fluorescence polarization
Unmodified Bak(BH3) peptide (GQVGRQLAIIGDCINR) was obtained from Elim Biopharmaceuticals, Inc. The peptide was derivatized using fluorescein-5-maleimide from Molecular Probes (Invitrogen), purified via reverse-phase HPLC on a C-18 column (Vydac), and verified by electrospray mass spectrometry. Binding experiments were carried out in 120 mM sodium phosphate (pH 7.4), 0.1 mg/mL bovine serum albumin, using a peptide concentration of 10 nM and M11L143 concentrations ranging from 1 nM to 325 mM. Data was collected on a Molecular Devices M5 fluorescence plate reader, and fit nonlinearly to an independent binding site model (Clarke 1996) using KaleidaGraph (Synergy Software).
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Data deposition |
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Footnotes |
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Reprint requests to: Tracy M. Handel, Skaggs School of Pharmacy and Pharmaceutical Sciences, University of California–San Diego, 9500 Gilman Drive MC 0684, La Jolla, CA 92093, USA; e-mail: thandel{at}ucsd.edu; fax: (858) 822-6655.
Article and publication are at http://www.proteinscience.org/cgi/doi/10.1110/ps.062720107.
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Acknowledgments |
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References |
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