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accessMichaelis-like complex of SARS-CoV-2 main protease visualized by room-temperature X-ray crystallography
aNeutron Scattering Division, Oak Ridge National Laboratory, 1 Bethel Valley Road, Oak Ridge, TN 37831, USA, bNational Virtual Biotechnology Laboratory, US Department of Energy, Washington, DC 20585, USA, cSecond Target Station, Oak Ridge National Laboratory, 1 Bethel Valley Road, Oak Ridge, TN 37831, USA, and dLaboratory of Chemical Physics, National Institute of Diabetes and Digestive and Kidney Diseases, National Institutes of Health, DHHS, Bethesda, MD 20892-0520, USA
*Correspondence e-mail: kovalevskyay@ornl.gov
SARS-CoV-2 emerged at the end of 2019 to cause an unprecedented pandemic of the deadly respiratory disease COVID-19 that continues to date. The viral main protease (Mpro) is essential for SARS-CoV-2 replication and is therefore an important drug target. Understanding the catalytic mechanism of Mpro, a cysteine protease with a catalytic site comprising the noncanonical Cys145–His41 dyad, can help in guiding drug design. Here, a 2.0 Å resolution room-temperature X-ray is reported of a Michaelis-like complex of Mpro harboring a single inactivating mutation C145A bound to the octapeptide Ac-SAVLQSGF-CONH2 corresponding to the nsp4/nsp5 autocleavage site. The peptide substrate is unambiguously defined in subsites S5 to S3′ by strong electron density. Superposition of the Michaelis-like complex with the neutron structure of substrate-free Mpro demonstrates that the catalytic site is inherently pre-organized for catalysis prior to substrate binding. Induced fit to the substrate is driven by P1 Gln binding in the predetermined subsite S1 and rearrangement of subsite S2 to accommodate P2 Leu. The Michaelis-like complex structure is ideal for in silico modeling of the SARS-CoV-2 Mpro catalytic mechanism.
Keywords: SARS-CoV-2; 3CL protease; main protease; catalytic mechanism; C145A mutant; enzyme–substrate complex; room-temperature X-ray crystallography.
PDB reference: room-temperature X-ray of SARS-CoV-2 main protease C145A mutant in complex with the substrate Ac-SAVLQSGF-CONH2, 7n89
1. Introduction
Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) causes the deadly coronavirus disease 2019 (COVID-19) that engulfed the globe in a pandemic in early 2020 and remains a significant health threat despite the availability of several vaccines and antiviral therapies (Gavor et al., 2020![[Gavor, E., Choong, Y. K., Er, S. Y., Sivaraman, H. & Sivaraman, J. (2020). Trends Immunol. 41, 1006-1022.]](../../../../../../logos/arrows/iucrj_arr.gif "Gavor, E., Choong, Y. K., Er, S. Y., Sivaraman, H. & Sivaraman, J. (2020). Trends Immunol. 41, 1006-1022.")
; Meo et al., 2021; Doroftei et al., 2021; Bidram et al., 2021). The main protease of SARS-CoV-2 (3CLpro or Mpro) is virally encoded and its precise function is essential for virus replication. Mpro cleaves two polyproteins, pp1a and pp1ab (∼450 and ∼790 kDa, respectively), into individual functional proteins that build the virus genome replication/transcription machinery (Wu et al., 2020; Xu et al., 2020). Mpro is a cysteine protease (Tong, 2002) that hydrolyses scissile peptide bonds at 11 specific locations, including its own release as the nonstructural protein nsp5 (termed autoprocessing), in the polyprotein precursors. The substrate specificity of Mpro and its active-site architecture are dissimilar relative to human Thus, Mpro is considered an important drug target for the design and development of specific antivirals with potentially minimal nonspecific binding to human proteins (Liu et al., 2020; Jin et al., 2020; Ton et al., 2020; Suárez & Díaz, 2020; Acharya et al., 2020; Pathak et al., 2021), including the possibility of designing pan-coronavirus antivirals (Ullrich & Nitsche, 2020).
Mpro is a homodimer, with each protomer composed of three distinct domains (Zhang et al., 2020; Jin et al., 2020; Anand et al., 2002). The catalytic domains I (residues 1–101) and II (residues 102–200) have antiparallel β-barrel structures that resemble the chymotrypsin fold. The helical domain III (residues 201–306) comprises five α-helices and promotes dimerization through interactions with specific residues of domains I and II (Chou et al., 2004; Barrila et al., 2006; Tsai et al., 2010). The catalytic site of Mpro is noncanonical; it has a catalytic Cys145–His41 dyad believed to be assisted by a conserved (catalytic) water molecule (Wang et al., 2020), instead of the more common (Ser)Cys–His–Asp(Glu) triads found in other cysteine (and serine) (Gorbalenya & Snijder, 1996). The Mpro cleavage sites are characterized by a preference for Gln and Leu/Phe at substrate positions P1 and P2, respectively (Fan et al., 2004; Goetz et al., 2007). Substrate specificity is conserved in most coronavirus Mpro cleavage sites (Lai et al., 2006). Based on the crystal structures of the closely related SARS-CoV Mpro inactive mutant H41A in complex with an 11-amino-acid peptide substrate (Xue et al., 2008) and SARS-CoV Mpro inactive mutant C145A containing a ten-residue C-terminal prosequence (Muramatsu et al., 2016), the Mpro active-site cavity located on the protein surface can accommodate up to nine substrate residues in positions P5 through P4′ in the corresponding substrate-binding subsites S5 through S4′.
To date, most of the SARS-CoV-2 Mpro X-ray crystal structures deposited in the Protein Data Bank (PDB) and associated studies have focused on the design of protease inhibitors. Conversely, there is an apparent lack of structural studies into the catalytic mechanism of SARS-CoV-2 Mpro. Lee et al. (2020) have recently reported capturing a covalent acyl-enzyme intermediate using native enzyme and a product complex using the inactive C145A mutant. In both structures, the C-terminal residues of one protomer extend into the active site of the other protomer, thus mimicking autocleavage of its C-terminus. Consequently, a Michaelis-like complex structure of SARS-CoV-2 Mpro bound to a discrete peptide substrate remains unidentified. This paper reports a room-temperature X-ray of SARS-CoV-2 Mpro C145A mutant (Mpro/C145A) in complex with the octapeptide Ac-SAVLQSGF-CONH2 corresponding to the nsp4/nsp5 autocleavage site (henceforth referred to as Mpro/C145A–substrate), at 2.0 Å resolution and pH 6.5. The peptide substrate spans residues from P5 through P3′ and is chemically protected by acetylation at the N-terminus and amidation at the C-terminus. The octapeptide binds asymmetrically in the Mpro active-site cavity such that the five groups P5–P1 bind to the nonprime substrate-binding subsites S5 through S1 and the three groups P1′–P3′ bind to the prime substrate-binding subsites S1′ through S3′. We hypothesize that this substrate mode of binding is the reason behind our success in producing crystals of such a complex. We previously reported enzyme kinetics measurements for a FRET substrate based on the same nsp4/nsp5 autocleavage site (kcat = 0.28 s−1 and Km = 170 µM; Kneller, Galanie et al., 2020).
2. Materials and methods
2.1. General information
Crystallization reagents and supplies were purchased from Hampton Research, Aliso Viejo, California, USA. Crystallographic supplies for crystal mounting and X-ray diffraction data collection at room temperature were purchased from MiTeGen, Ithaca, New York, USA. The Ac-SAVLQSGF-CONH2 peptide used in this study was custom-synthesized by Biomatik Corp., Kitchener, Ontario, Canada.
2.2. Expression and purification of Mpro/C145A
A DNA insert encoding a 6×His tag followed by a TEV protease cleavage site and SARS CoV-2 Mpro (306 amino acids) bearing an active-site C145A mutation was cloned into the pJ414 vector (ATUM) and transformed into Escherichia coli BL21(DE3) cells (Agilent). The last residue in the TEV protease recognition sequence (ENLYFQG/S) was chosen to be a serine, such that upon cleavage the Mpro/C145A construct starts with the native N-terminal Ser1 residue. Cells were grown in Luria–Bertani medium, and the Mpro/C145A fusion protein was expressed using established protocols. The fusion protein was purified under native conditions by lysis and Ni–NTA in 20 mM Tris–HCl pH 8, 150 mM NaCl, 1 mM TCEP, 20 mM imidazole. This step was followed by on a Superose 12 column (16 × 60 cm, Cytiva) to remove minor high-molecular-weight contaminants and to exchange the buffer to 25 mM Tris–HCl pH 8, 100 mM NaCl, 0.5 mM EDTA, 1 mM DTT, 20 mM imidazole, which is suitable for cleavage by TEV protease at a molar ratio of 75:1 fusion protein:TEV protease. TEV protease was prepared as described by Lucast et al. (2001). Upon completion of the cleavage and adjustment of the EDTA concentration to 0.25 mM, Mpro/C145A was collected in the flowthrough from the Ni–NTA column, concentrated and then subjected again to isocratic fractionation on Superose 12 in 25 mM Tris pH 7.6, 150 mM NaCl, 1 mM TCEP. Peak fractions were combined, concentrated and aliquots of the protein were stored at − 20 C. Purity was verified both by SDS–PAGE and electrospray ionization mass spectrometry.
2.3. Crystallography of the Mpro/C145A–substrate complex
We have previously published detailed methods for crystallizing high-quality Mpro crystals using the sitting-drop vapor-diffusion methodology (Kneller, Galanie et al., 2020; Kneller, Phillips, Kovalevsky et al., 2020). Crystallization conditions for the Mpro/C145A mutant were discovered by automated high-throughput screening at the Hauptman–Woodward Medical Research Institute (Luft et al., 2003). The protein was concentrated to 6 mg ml−1. Initially, flower-like crystal aggregates unsuitable for room-temperature X-ray diffraction grew using a sample of 270 µl protein solution mixed with 1.6 mg lyophilized peptide in 20% PEG 3350, 0.1 M bis-Tris pH 7.0. Subsequently, the protein was mixed in a 1:5 molar ratio with peptide from a 50 mM stock in 100% DMSO and used for crystallization with 20% PEG 3350, 0.1 M bis-Tris pH 6.5. This condition produced a final pH in the crystallization drop of 6.5 as measured by a microelectrode. Drops were seeded using a cat whisker and flower-shaped aggregates grew with thicker `petal' substituents after one week of incubation at 14°C. A single crystal from the aggregate was harvested and mounted on loops and capillary setups for room-temperature diffraction.
2.4. Room-temperature X-ray diffraction data collection and structure refinement
Room-temperature X-ray diffraction data were collected on a Rigaku HighFlux HomeLab instrument equipped with a MicroMax-007 HF X-ray generator, Osmic VariMax optics and a Dectris EIGER R 4M hybrid photon-counting detector. Data were integrated using the CrysAlisPro software suite (Rigaku, The Woodlands, Texas, USA) and were reduced and scaled using AIMLESS (Evans & Murshudov, 2013) from the CCP4 suite (Winn et al., 2011). The Mpro/C145A–substrate structure was solved by using PDB entry 6wqf (Kneller, Phillips, O'Neill et al., 2020) with Phaser (McCoy et al., 2007) from CCP4. The model was iteratively refined using phenix.refine from the Phenix suite (Liebschner et al., 2019) and Coot (Emsley et al., 2010; Casañal et al., 2020) aided by MolProbity (Chen, Arendall et al., 2010) for geometry validation. Final data-collection and are given in Supplementary Table S1.
3. Results and discussion
3.1. Binding of peptide substrate
In Mpro/C145A–substrate, a substrate occupies each of the two active-site grooves in the Mpro homodimer structure (Fig. 1). There is unambiguous electron density for all residues except for the P3′ Phe side chain. Interactions between Mpro and substrate are nearly identical in both protomers; hence, subsequent details of our analysis will focus on protomer A. Main-chain interactions between the peptide and Mpro are consistent with adding a β-strand to the antiparallel β-sheets flanking the scissile bond [Fig. 2(a)]. There are eight hydrogen bonds between the main chains of the peptide substrate and Mpro, which involve residues Thr190, Glu166, His164, Ser144, Gly143 and Thr26. In the catalytic site, P1 Gln is driven into the S1 subsite via a 2.7 Å hydrogen bond to the His163 imidazole and a water-mediated interaction with Asn142, whereas its main-chain carbonyl O atom is centered into the characteristic oxyanion hole [Fig. 2(b)]. The bulky hydrophobic P2 Leu side chain fills its respective hydrophobic S2 subsite, whereas the smaller P4 Ala juts into the shallow S4 pocket capped by the flexible S5 loop. P2′ Gly contributes to substrate binding via backbone hydrogen-bond interactions with Thr26, whereas P1′ Ser makes no hydrogen bonds to Mpro, as is the case for P5 Ser. The P5 Ser, P3 Val, P2′ Ser and P3′ Phe side chains face the solvent space between crystallographic symmetry-related molecules, with the P3′ Phe phenyl ring being dynamic and poorly defined in the electron-density maps.
![[Figure 1]](mf5056fig1thm.gif) | Figure 1 Mpro/C145A–substrate complex. Mpro/C145A (protomer A is shown as a purple cartoon and protomer B as an orange surface) was co-crystallized with an octapeptide (green sticks and surface) corresponding to the nsp4/nsp5 autocleavage site. The top inset shows the peptide in protomer B in conventional orientation, while the bottom inset shows protomer A rotated by 180°. Fo − Fc omit difference electron-density maps for each peptide are contoured at 3σ. |
![[Figure 2]](mf5056fig2thm.gif) | Figure 2 Mpro/C145A–substrate interactions for induced fit of substrate. (a) Main-chain hydrogen-bond interactions between Mpro and the peptide substrate (shown as orange and green C atoms, respectively). Hydrogen bonds are shown as dotted lines. Distances are in Å. (b) Hydrogen-bond interactions between peptide P1 Gln with the S1 subsite and the catalytic site. Water molecules are shown as red spheres. (c) Superposition of Mpro/C145A–substrate with the substrate-free Mpro neutron (light blue; PDB entry 7jun) showing the scissile bond in relation to the catalytic Cys145–His41 zwitterion. Superposition was by a least-squares fit to Cα atoms of protomer A. (d) Induced fit of Mpro/C145A to the peptide substrate by the rearrangements of side chains in the S2 and S4 subsite. |
The C-terminal residues of Mpro flank the last helix in domain III. Here, residues 302–306 constitute a flexible loop (Kneller, Phillips, O'Neill et al., 2020) and are typically disordered in crystal structures of SARS-CoV-2 Mpro to the extent that some crystallographers choose not to model the C-terminus (Dai et al., 2020; Zhang et al., 2020). In this context, it is noteworthy that electron density for the C-terminal residues up to the very last Gln306 amine is clearly observed in Mpro/C145A–substrate (Supplementary Fig. S1). When the C-terminal residues of Mpro/C145A–substrate and the product complex reported by Lee et al. (2020) are superimposed, the main-chain atoms align with an r.m.s.d. of 0.7 Å for residues 303–306 (Supplementary Fig. S2), demonstrating that the C-terminus of Mpro is pre-organized to bind into the active site during Mpro autoprocessing.
3.2. Comparison with substrate-free Mpro
Superposition of Mpro/C145A–substrate and our recently determined substrate-free neutron crystallographic structure of wild-type SARS-CoV-2 Mpro (PDB entry 7jun; Kneller, Phillips, Weiss et al., 2020) offers unique insights into catalysis because the Cys145–His41 dyad was observed as a zwitterionic species with the Cys145 thiolate Sγ atom 3.8 Å away from His41 Nɛ2, already primed for proteolysis [Fig. 2(c)]. When the two structures are superimposed, the Cys145 thiolate is positioned 1.8 Å away from the scissile-bond carbonyl C atom with an ideal distance and orientation for a nucleophilic attack. The scissile-bond amide N atom is positioned 2.7 Å away from the Nɛ2 hydrogen on the catalytic His41, which does not significantly change its position in the complex, poised for proton transfer to the amino-terminus that is created in the cleavage reaction. The Mpro/C145A–substrate structure therefore underscores the suggestion that the zwitterionic catalytic dyad is present prior to substrate binding (Kneller, Phillips, Weiss et al., 2020) instead of requiring reorganization of the catalytic site to facilitate proton transfer from Cys145 to His41 in the catalytically resting (nonreactive) state (i.e. a protonated Cys145 thiol and singly protonated His41 imidazole) to create the reactive zwitterionic species (Paasche et al., 2014; Ramos-Guzmán et al., 2020; Díaz & Suárez, 2021).
In subsite S1, Glu166 accommodates P1 Gln by moving ∼0.9 Å away from the substrate and simultaneously rotating to form a 2.8 Å hydrogen bond to His172 that is absent in substrate-free Mpro. This conformational change of the Glu166 side chain is due to the binding of a ligand to the active site and is consistent with the changes observed in Mpro–inhibitor complexes (Kneller, Galanie et al., 2020; Dai et al., 2020). Meanwhile, the Asn142 side chain flips ∼180° and shifts 2.6 Å from its position in the substrate-free structure to produce water-mediated contacts with P1 Gln. This comparison indicates that the catalytic dyad is already pre-organized and primed for catalysis in the substrate-free structure, requiring minimal rearrangements to initiate the peptide-hydrolysis reaction. Induced fit of the peptide substrate to Mpro is achieved primarily through the continuation of β-sheet structures and key rearrangements of the large side chains Met165, Met49 and Gln189 from their positions in substrate-free Mpro to create subsites S2 and S4 [Fig. 2(d)]. The substrate P2 Leu forms the S2 subsite by a >3 Å steric swing of the Met49 side chain located on the short S2 helix (residues 46–50). P2 Leu also acts in consortium with the methyl C atom of P4 Ala to produce the shallow S4 subsite by initiating a new rotational isomer for Met165 and shifting the position of the S4 β-hairpin loop by as much as 1.5 Å. The peptide residue arrangement is stabilized by Gln189 rotating to hydrogen-bond to the main-chain NH of P3 Val. P5 Ser does not interact directly with Mpro. However, the hydroxymethyl side chain might act to nullify repulsion of the Gln189 backbone by intramolecular hydrogen bonding to the carbonyl of P3 Val. The active site around P4 and P5 expands by >1.5 Å from the substrate-free structure to accommodate the substrate, as measured by the Cα distances between Pro168/168′ and Thr190/190′. Interestingly, the S2 subsite helix of the complex shows only minor distal expansion, unlike in Mpro–inhibitor complexes where the S2 subsite helix can shift by >1.5 Å (Jin et al., 2020; Kneller, Galanie et al., 2020). Similarly, the S5 loop (residues 189–194) is only minimally disturbed by the substrate, shifting by <1.0 Å.
3.3. Comparison with SARS-CoV Mpro/H41A
It is instructive to compare our room-temperature Mpro/C145A–substrate structure from SARS-CoV-2 with a low-temperature structure of the SARS-CoV main protease H41A mutant, Mpro/H41A, soaked with an 11-amino-acid peptide substrate spanning the same nsp4/nsp5 autocleavage site (Xue et al., 2008; Fig. 3; PDB entry 2q6g). The peptide substrate in both structures bows into the active site by conforming to the antiparallel β-sheets flanking the catalytic site. Overall, the orientations of the substrate residues in both protomers are in agreement or can be explained by a lack of electron density, with one exception. The Cγ atoms of P2 Leu deviate by ∼1 Å, which is coordinated with the rotational isomer differences observed for the Met49 and Met165 side chains. In the SARS-CoV Mpro/H41A–substrate complex, the substrate pushes the catalytic Cys145 side chain away from the scissile bond towards the vacated space left by the H41A mutation to a position where the S atom is 4.5 Å from the scissile carbonyl C atom. Mpro possesses 96% sequence identity between SARS-CoV and SARS-CoV-2. The nearest mutation to the active site in SARS-CoV-2 Mpro, A46S, does not introduce appreciable differences despite minor differences in the S2 subsite helix.
![[Figure 3]](mf5056fig3thm.gif) | Figure 3 Comparison of substrate-bound Mpro/C145A from SARS-CoV-2 (PDB entry 7n89) with Mpro/H41A from SARS-CoV (PDB entry 2q6g). (a) Protomer A in Mpro/C145A–substrate from SARS-CoV-2 (orange protein, green substrate) superimposed on the SARS-CoV Mpro/H41A–substrate complex (cyan protein, slate substrate). Superposition was by a least-squares fit of Cα atoms of protomer B in PDB entry 2q6g to protomer A in PDB entry 7n89. (b) Protomer B in Mpro/C145A–substrate from SARS-CoV-2 (orange protein, green substrate) superimposed on the SARS-CoV Mpro/H41A–substrate complex. Superposition was by a least-squares fit of Cα atoms of protomer A in PDB entry 2q6g to protomer B in PDB entry 7n89. |
4. Conclusion
We describe details of the structure of SARS-CoV-2 Mpro bearing an active-site C145A mutation in complex with an octapeptide substrate corresponding to the natural nsp4/nsp5 junction sequence which Mpro autoprocesses prior to its C-terminal junction (nsp5/nsp6 site) during its maturation from the polyprotein precursor (Hsu et al., 2005; Chen, Jonas et al., 2010; Muramatsu et al., 2013). Substrate affinity is driven primarily by P1 Gln hydrogen-bonding interactions and P2 Leu induced-fit rearrangement, with assistance from secondary-structure main-chain interactions. Superposition of the substrate complex with the substrate-free Mpro neutron structure reinforces the suggestion that the substrate-free Mpro structure is innately pre-organized to attack the scissile bond upon a substrate-binding event. We also suggest that our structure is an ideal starting point for in silico modeling and simulations looking into understanding Mpro–substrate relationships due to specificity and the absence of cryo-artifacts. These results bring timely insights into the nature of catalysis to expedite structure/mechanism-based drug design.
Supporting information
PDB reference: room-temperature X-ray of SARS-CoV-2 main protease C145A mutant in complex with the substrate Ac-SAVLQSGF-CONH2, 7n89
Supplementary Table and Figures. DOI: https://doi.org/10.1107/S2052252521010113/mf5056sup1.pdf
Acknowledgements
This research used resources at Oak Ridge National Laboratory's Center for Structural Molecular Biology (CSMB), a DOE Office of Science User Facility, supported by the Office of Biological and Environmental Research. This research used resources of the Spallation Neutron Source Second Target Station Project at Oak Ridge National Laboratory (ORNL). ORNL is managed by UT-Battelle LLC for DOE's Office of Science, the single largest supporter of basic research in the physical sciences in the United States. We thank Dr Hugh M. O'Neill from ORNL for assistance during expression and purification of the protein. We thank Annie Aniana for excellent technical assistance, John Lloyd and the NIDDK core facility for Author contributions were as follows. DWK, LC and AK conceived the study, QZ and JML constructed, expressed and purified Mpro/C145A, DWK crystallized the protein and DWK and AK collected and processed the X-ray data and refined the structure. The manuscript was written with the contribution of all authors. All authors have given approval to the final version of the manuscript.
Funding information
This research was supported by the DOE Office of Science through the National Virtual Biotechnology Laboratory (NVBL), a consortium of DOE national laboratories focused on response to COVID-19, with funding provided by the Coronavirus CARES Act. This work was also supported by the Intramural Research Program of the National Institute of Diabetes and Digestive and Kidney Diseases, NIH.
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