SARS-CoV-2 can recruit a haem metabolite to evade antibody immunity

Protein expression and purification

DNA fragments encoding SARS-CoV-2 S1 (Uniprot ID: P0DTC2; residues 1-530), NTD (1-310), RBD (319-541), SARS-CoV-1 S1 (Uniprot ID: P59594; residues 1-518), HCoV NL63 (Uniprot ID: Q6Q1S2; residues 1-618), HCoV OC43 (isolate LRTI_238, NCBI accession code KX344031; residues 1-619) were codon-optimized for expression in human cells and cloned control of the cytomegalovirus promoter for production of the recombinant proteins carrying a C-terminal extension containing human rhinovirus 14 3C protease recognition site followed by a TwinStrep tag. The signal peptide from immunoglobulin kappa gene product (METDTLLLWVLLLWVPGSTGD) was used to direct secretion of the RBD construct. The vector for production of the His₆-tagged stabilized trimeric SARS-CoV-2 has been described (18). Expression constructs encoding heavy and light chains of P008_056 Fab were made by inserting the respective coding sequences into pHLsec (38), including a sequence encoding a hexa-histidine (His₆) tag on the heavy chain fragment C terminus.

With exception of trimeric stabilized SARS-CoV-2 spike ectodomain, the proteins were produced by transient transfection of Expi293 (Thermo Fisher Scientific) cells with endotoxin-free preparations of the corresponding DNA constructs using ExpiFectamine293 (Thermo Fisher Scientific). The cells were maintained in shake flasks in FreeStyle293 (Thermo Fisher Scientific) medium at 37°C in humidified 5% CO₂ atmosphere. To produce SARS-CoV-2 S1 NTD fragment for crystallography, cell culture medium was supplemented with 5 μM kifunensine (Sigma-Aldrich) to suppress complex glycosylation (39). Conditioned medium containing recombinant product was harvested twice, 4 and 8 days post-transfection, or once, for production of the NTD and P008_056 Fab, 5 days post-transfection. For production of the trimeric SARS-CoV-2 spike ectodomain, Expi293 transfected with the pcDNA3-based expression construct (18) were selected with 250 μg/ml geneticin. Stably transfected cells, grown to a density of 3.5 million per ml at 37°C, were shifted to 32°C for 3 days prior to harvesting conditioned medium to enhance secretion of the viral glycoprotein (40).

TwinStrep-tagged proteins were captured on Strep-Tactin XT (IBA LifeSciences) affinity resin. Following extensive washes in TBSE (150 mM NaCl, 1 mM ethylenediaminetetraacetic acid (EDTA), 25 mM Tris-HCl, pH 8.0), the proteins were eluted in 1xBXT buffer (IBA LifeSciences). His₆-tagged proteins were captured on HisTrap Excel (Sigma-Aldrich) resin and eluted with 300 mM imidazole in phosphate buffered saline. For the use in crystallography, SARS-CoV-2 S1 NTD was digested with Endo Hf (New England Biolabs) and rhinoviral 3C protease to trim glycans and to remove the C-terminal twin Strep tag; Endo Hf was depleted by absorption to amylose resin (New England Biolabs). The proteins were further purified by size exclusion chromatography through a Superdex 200 16/600 column (GE Healthcare) in HBSE (150 mM NaCl, 1 mM EDTA, 20 mM Hepes-NaOH, pH 8.0) and concentrated by ultrafiltration using a Vivaspin-20 with 10-kDa cut-off (Sartorius). To deplete biliverdin from SARS-CoV-2 S1, recombinant protein eluted from Strep-Tactin XT resin was supplemented with 0.5 M sodium acetate, pH 5.2 and subjected to size exclusion chromatography through a Superdex 200 16/600 column in 200 mM sodium acetate, pH 5.2; fractions containing S1 were pooled and dialyzed overnight against HBSE buffer. Light absorbance spectra of recombinant proteins were acquired using Jasco V-550 UV/VIS spectrophotometer.

Mass spectrometry

Recombinant SARS-CoV-2 S1 (3.5 mg/ml, 500 μl), denatured by addition of 1% (w/v) sodium dodecyl sulfate, was extracted with 500 μl n-butanol. Organic phase containing green pigment was allowed to evaporate under vacuum, and dry residue was re-dissolved in 20 μl water. Liquid chromatography-tandem mass spectrometry was performed as described previously (41). LC-MS/MS analysis was conducted using a Dionex UltiMate LC system (Thermo Scientific) with a ZIC-pHILIC column (150 mm × 4.6 mm, 5 μm particle, Merck Sequant). A 15-min elution gradient of 80% Solvent A (20 mM ammonium carbonate in Optima HPLC grade water, Sigma-Aldrich) to 20% Solvent B (acetonitrile Optima HPLC grade, Sigma-Aldrich) was used, followed by a 5-min wash of 95:5 Solvent A to Solvent B and 5-min re-equilibration. Other parameters were as follows: flow rate, 300 μl/min; column temperature, 25°C; injection volume, 10 μl; autosampler temperature, 4°C. Metabolites were detected across a mass range of 70-1050 m/z using a Q Exactive Orbitrap instrument (Thermo Scientific) with heated electrospray ionization and polarity switching mode at a resolution of 70,000 (at 200 m/z). MS parameters were as follows: spray voltage 3.5 kV for positive mode and 3.2 kV for negative mode; probe temperature, 320°C; sheath gas, 30 arbitrary units; auxiliary gas, 5 arbitrary units. Parallel reaction monitoring was used at a resolution of 17,500 to confirm the identification of biliverdin; collision energy was set at 30 in high-energy collisional dissociation mode. Data was recorded using Xcalibur 3.0.63 software and analyzed using Free Style 1.6 and Tracefinder 4.1 software (Thermo Scientific) according to the manufacturer’s workflows.

SPR

Experiments were performed on a Biacore S200 (Cytiva); S1 protein, diluted to 50 μg/ml in 10 mM sodium acetate, pH 5.0, was immobilized on a CM5 sensor chip (Cytiva product code BR100530) using amine coupling chemistry. Immobilization levels were typically 4,000 response units. Analyte binding was studied in running buffer comprising 150 mM NaCl, 50 mM HEPES-NaOH, pH 8.0 or 50 mM BisTris-HCl, pH 5.0, 0.05% Tween-20, and 1% dimethyl sulfoxide (DMSO). Biliverdin, bilirubin, haem, and protoporphyrin were obtained from Sigma-Aldrich (product codes 3089, 14370, 51280, and P8293, respectively). Generally, analyte stock solutions were prepared in DMSO prior to dilution in running buffer, maintaining the final DMSO concentration of 1%. The final analyte concentration was verified by spectrophotometry, using the following molar extinction coefficients: biliverdin 39,900 (at a wavelength of 388 nm), bilirubin 53,846 (460 nm), haem 58,440 (385 nm), and protoporphyrin IX 107,000 (407 nm). Alternatively, biliverdin, which is highly soluble at pH>7, was dissolved directly in running buffer to omit DMSO from the experiment. The presence of DMSO did not affect the measured K_d of the S1-biliverdin interaction (Table S1). All experiments were conducted using a CM5-kinetics-multicycle template at 25°C. Flow rate was 30 μl/min with a contact time of 180 s, followed by a dissociation time of 10 min; three start-ups were performed at the beginning of each experiment. Solvent correction was deemed unnecessary for the assays that contained DMSO. Biliverdin displayed very fast association precluding detailed kinetics analyses due to mass transfer effects. Data were analyzed using the 1:1 binding model in the Biacore S200 Evaluation software to estimate equilibrium binding constants (K_d).

Protein thermostability assay

Biliverdin-depleted SARS-CoV-2 NTD (corresponding to spike residues 1-310) was diluted to 1 mg/ml in 150 mM NaCl, 20 mM HEPES-NaOH, pH 8.0 and supplemented with biliverdin from a 5-mM stock prepared in 100 mM Tris-HCl, pH8.0 where appropriate. Melting curves were recorded using 20−95 °C 1.5 °C/min temperature ramps on a Promethius NT.48 instrument (Nanotemper). Melting points were determined from inflection points of fluorescence intensity ratios (350 and 330 nm) using first derivative analysis (fig. S3K).

Cryo-electron microscopy

Four μl stabilized trimeric SARS-CoV-2 spike ectodomain (0.6 mg/ml final concentration in TBSE supplemented with 0.1% n-octyl glucoside) with 25 μM biliverdin or 0.2 mg/ml P008_056 Fab, was applied onto glow-discharged 200-mesh copper holey carbon R2/2 grids (Quantifoil) for 1 min, under 100% humidity at 20°C, before blotting for 3-4 s and plunge-freezing in liquid ethane using Vitrobot Mark IV (Thermo Fisher Scientific). The data were collected on Titan Krios microscopes operating at 300 keV (Thermo Fisher Scientific). Single particles of spike-biliverdin were imaged using a Falcon III direct electron detector (Thermo Fisher Scientific). A total of 15,962 movies were recorded with a calibrated pixel size of 1.09 Å and a total electron exposure of 33 e^-/Ų, spread over 30 frames in single electron counting mode. The spike-Fab complex was imaged on a GIF Quantum K2 detector with a post-column energy filter (Gatan), selecting a 20-eV window, in single electron counting mode. A total of 17,010 movies were collected with a pixel size of 1.38 Å and total electron exposure of 51 e^-/Ų spread over 40 frames. Both datasets were acquired with a defocus range of -1.6 to -4 μm (Table S2).

Cryo-EM image processing and real-space refinement

Micrograph movies were aligned with dose weighting applied using MotionCor2 (42), and the contrast transfer function (CTF) parameters were estimated from the frame sums with Gctf (43). Images exhibiting ice contamination or poor CTF estimation were discarded at this stage, leaving 15,803 (biliverdin complex) and 16,619 (Fab complex) movies for further processing. An initial set of particles, autopicked with Laplacian-of-Gaussian function in Relion-3.1 (44), was used to generate 2D class averages that served as templates for picking both datasets with Gautomatch (https://www.mrc-lmb.cam.ac.uk/kzhang/). Particles (1,209,334 and 2,505,265 for spike-biliverdin and spike-Fab, respectively) were extracted from weighted frame sums, binned 4-fold, and subjected to reference-free 2D classification in cryoSPARC-2 (45). 371,422 spike-biliverdin and 709,127 spike-Fab particles belonging to well-defined classes containing trimeric spike were selected for further processing (figs S4A, S11A). An initial 3D model was generated using ab initio procedure in cryoSPARC-2. Selected particles, re-extracted with 2-fold binning, were subjected to 3D classification into 11 (spike-biliverdin) and 16 (spike-Fab) classes in Relion-3.1. Particles belonging to selected 3D classes were re-extracted without binning and used in 3D reconstruction followed by CTF refinement (beam tilt and per-particle defocus) and Bayesian polishing in Relion-3.1. The final 3D reconstructions were done using non-uniform refinement procedure in cryoSPARC-2. Resolution is reported according to the gold-standard Fourier shell correlation (FSC), using the 0.143 criterion (46, 47) (figs S4C-D and S12C-D, Table S2). To aid in model building process, the maps were filtered and sharpened using deepEMhancer (48) or using density modification procedure in Phenix (49). An additional spike-Fab reconstruction was obtained using multibody refinement in Relion-3.1 accounting for two rigid bodies (one spanning the Fab moiety plus the associated NTD, and the second encompassing the rest of the structure) was used for illustration purposes (Fig. 4A).

For the 3RBD-down spike model, coordinates from protein databank entry 6ZGE (18) were docked into the cryo-EM map in Chimera (50). Residues 14-319 were replaced with the NTD crystal structure for each of the chains along with the associated biliverdin molecules. The model was manually adjusted in Coot (51) and refined using phenix.real_space_refine (version 1.19rc5-4047) (52). The model was then docked into the cryo-EM map of asymmetric 1RBD-up reconstruction and one RBD refitted to the extended position in Chimera; the model was manually adjusted in Coot and refined using phenix.real_space_refine. For the spike-Fab model, 3RBD-down spike model was fitted to the map using Chimera; the RBD of chain A was fitted in to the extended position, which is less well defined, and the NTD of chain C was extensively remodeled. The protein data bank was searched for similar structures using the sequence of the Fab chains; 6APC (53) and 6PHB (54) were selected as templates for the heavy and light chains of the Fab respectively, variable and constant sub-domains were fitted individually using either phenix.dock_in_map (55) and/or fitted in Chimera. The Fab fragments were manually adjusted to match the sequence of P0008_056 antibody and fitted to the cryo-EM map. The constant domains of the Fab are less well resolved in the map and minimal adjustments were made to these domains. The whole structure was subjected to automatic flexible fitting using Namdinator v2.13 (56) and then phenix.real_space_refine before another round of manual rebuilding in Coot and a final round of phenix.real_space_refine. Biliverdin (BLA) ligand geometry definition file was generated by Grade (Global Phasing) and model quality was assessed using Molprobity (57).

Crystal Structure of the NTD in complex with biliverdin

Protein construct (spanning SARS-CoV-2 S1 residues 1-310) at 10 mg/ml was supplemented with 90 μM biliverdin before mixing with crystallization mother liquor in a 1:1 ratio. Plate-like crystals grew to 80-120 μm in two dimensions and ~10-20 μm in the third dimension in conditions containing 24% PEG 3350 (w/v) and 0.25 M NaSCN by hanging drop vapor diffusion over 1-2 weeks at 18°C. Crystals were cryoprotected by the addition of PEG 400 to a final concentration of 30% (v/v) to the drop solution and frozen by plunging in liquid nitrogen. X-ray diffraction data were collected at the PX1 beamline, Swiss Light Source, using wavelength 1 Å, 100% transmission, a 40-μm beam, 0.1-s exposure and 0.5° rotation per image. Data were indexed, scaled and merged using XDS (58) and Aimless (59) via Xia2 (60). SARS-CoV-2 spike NTD (residues 14-290; PDB ID 6ZGE) (18) was used as a model for molecular replacement and yielded a solution containing one NTD per asymmetric unit, with a log likelihood gain of 490 and translation function Z-score of 22.7, in space group C222₁ using Phaser (61) within the Phenix package (55). The initial molecular replacement solution was subjected to morph model in Phenix before commencing with rounds of manual fitting in Coot (51) and refinement using phenix.refine (version 1.19rc4-4035) (55). First, the protein chain was fitted and extended where possible, and refined, then glycosylation moieties were added where visualized in the positive Fo-Fc density, followed by conceivable PEG and water molecules. The electron density around the disulphide bonds suggested that they were labile and as such were modeled as alternative conformations between oxidized and reduced where appropriate and the occupancy refined between these states. The stability of the disulphide bonds could have been affected by trace amounts of DTT introduced during the treatment of the protein with 3C protease and EndoH. The R_free and R_work were 21.5 and 18.5%, respectively, before a biliverdin molecule was fitted into the prominent positive difference density; rings A, B and C are defined very well in the density, ring D appears to be marginally less well defined. The final refinement included four Translation/Libration/Screw groups (residues 14-67, 68-202, 203-278, 279-319) that had been segmented by the TLSMD server (62). Ligand geometry definitions were generated by Grade (Global Phasing). The final model consists of spike residues 14-319, one biliverdin molecule, seven N-linked glycans (attached to asparagine residues at positions 17, 61, 122, 149, 165, 234, and 282), 10 PEG moieties, and 351 water molecules and has reasonable geometry and fit to the electron density (Table S3, fig. S5B). Model quality was assessed using Molprobity (63). The alignment of the sarbecoviral spike sequences with the NTD secondary structures (fig. S7) was formatted using ESPript3 server (https://espript.ibcp.fr/ESPript/ESPript/) (64).

Human sera

Following written informed consent, serum samples from staff and patients of the Imperial College Healthcare NHS Trust (ICHNT) and the Wellington Hospital diagnosed with SARS-CoV-2 infection were donated to the Communicable Diseases Research Tissue Bank (CDRTB) of the Section of Virology, Department of Infectious Disease, Imperial College London. The use of these sera was approved by the CDRTB Steering Committee in accordance with the responsibility delegated by the National Research Ethics Service (South Central Ethics Committee Oxford – C, NRES references 15/SC/0089 and 20/SC/0226). The median time from onset of symptoms (or positive RT-PCR test in the case of asymptomatic infection) was 29 (0-94) days. Additionally, serum or plasma samples were obtained from University College London Hospitals (UCLH) COVID-19 patients testing positive for SARS-CoV-2 infection by RT-qPCR and sampled between March 2020 and April 2020 (23). The sera were collected a median of 21 (9-31) days post onset of symptoms. Patient sera were from residual samples prior to discarding, in accordance with Royal College Pathologists guidelines and the UCLH Clinical Governance for assay development and approved by HRA (IRAS reference 284088). All serum or plasma samples were heat-treated at 56°C for 30 min prior to testing by flow cytometry.

IgG capture assay

WT (depleted of biliverdin by chromatography under acidic conditions) and mutant SARS-CoV-2 S1 proteins (4.1 mg/ml; 100 μl) were conjugated to horseradish peroxidase (HRP) using the Lynx rapid HRP conjugation kit (BioRad). Following quenching and dilution in conjugate stabilizer (Clintech, Guildford, UK; product code #MI20080), half of each conjugate was supplemented with 10 μM biliverdin. Nunc 96-well, U8 MaxiSorp plates (Fisher Scientific) were coated overnight at 4°C with AffiniPure rabbit anti-human IgG antibody (Stratech; product code #309-005-008) diluted to 5 μg/ml in coating buffer (Clintech; product code #643005). Following a 3-hours incubation at 37°C, and a 1 hour incubation at room temperature, the wells were washed with washing buffer (Clintech; product code #20024) and incubated for 4 hours in blocking solution (Clintech; product code #MI20011). The wells were air-dried and stored desiccated at 4°C until use. For ELISA, 100-μl serum samples, each diluted 1:100 in diluent buffer (Clintech, product code #2040), were added to the coated wells and incubated stationary at 37°C for 1 hour. To detect S1-specific IgGs, the wells were washed with washing buffer (Clintech) and aspirated to dryness, following which 100 μl of S1-HRP fusion conjugate diluted in conjugate diluent (Clintech; product code #100171) to a previously defined optimum concentration (1:1,500) were added and incubated for one hour at 37°C. The wells were then washed as before and developed for 30 min at 37°C using tetramethylbenzidine substrate (Clintech; product code #2030b), quenched by the addition of 50 μl stop solution (Clintech; product code #20031). The resulting optical densities (ODs) were acquired using a SpectraMax M2 reader (Molecular Devices).

The IgG capture ELISA data was modeled with a Bayesian linear model, using the gamma likelihood function: Gamma(μ, Scale). The linear model took the form of log(μ) = intercept[Sample] + offset[Protein], where the intercept[Sample] term allows varying intercepts across samples (to account for the repeated measurements of each serum sample across conditions, assumed to be distributed as Gamma(μ_intercept, scale_intercept)), and the offset[Protein] term accounts for variation attributable to different protein coatings. Pairwise contrasts were drawn from the posterior distribution to construct credible intervals for the difference in OD values between different protein coatings. Priors: offset[Protein]∼Normal(-3,0.2), scale∼Exponential(5), μ_intercept∼Normal(1,0.2), scale_intercept∼Exponential(5). Monte Carlo settings: 10,000 iterations, 4 chains, adapt_delta = 0.95, sampler = NUTS.

Flow cytometry

Serum antibody binding to full-length SARS-CoV-2 S expressed on HEK293T cells was performed using a recently described method (23). Briefly, HEK293T cells were transfected with an expression vector (pcDNA3) carrying codon-optimized genes encoding either the wild-type SARS-CoV-2 S (UniProt ID: P0DTC2) or N121Q SARS-CoV-2 S, using GeneJuice (EMD Millipore). Two days after transfection, cells were trypsinized and transferred into V-bottom 96-well plates (20,000 cells/well). Cells were incubated with sera (diluted 1:50 in PBS) for 30 min, with or without addition of 10 μM biliverdin throughout the staining period. They were then washed with FACS buffer (PBS, 5% BSA, 0.05% sodium azide) and stained with FITC anti-IgG (clone HP6017, Biolegend), APC anti-IgM (clone MHM-88, Biolegend) and PE anti-IgA (clone IS11-8E10, Miltenyi Biotech) for 30 min (all antibodies diluted 1:200 in FACS buffer). Samples were run on a Ze5 analyzer (Bio-Rad) running Bio-Rad Everest software v2.4 and analyzed using FlowJo v10 (Tree Star Inc.) analysis software. To calculate the effect of biliverdin, the mean fluorescence intensity (MFI) of positively stained cells only was used in each condition. The MFI data was modeled with a Bayesian linear model, using the gamma likelihood function: Gamma(μ, Scale). The linear model took the form of log(μ) = intercept[Sample] + offset[Protein], where the intercept[Sample] term allows varying intercepts across samples (to account for the repeated measurements of each serum sample across conditions, assumed to be distributed as Normal(μ_intercept,σ_intercept)), and the offset[Protein] term accounts for variation attributable to different protein coatings. Pairwise contrasts were drawn from the posterior distribution to construct credible intervals for the difference in MFI values between samples ±biliverdin. Priors: offset[Protein]∼Normal(0,400), scale∼Exponential(0.1), μ_intercept∼Normal(2500,200), σ_intercept∼Exponential(0.01). Monte Carlo settings: 10,000 iterations, 4 chains, adapt_delta = 0.95, sampler = NUTS.

The same procedure was performed to assess monoclonal IgG binding to cell surface SARS-CoV-2 spike with the following alterations: Transfection was performed with PEI-Max (1 mg/ml, Polysciences), FACS wash buffer (FWB) containing PBS supplemented with 1% BSA. Monoclonal IgGs were serially diluted 10-fold from 50 μg/ml prior to mixing with transfected cells. Antibody binding was detected with APC anti-IgG (Biolegend) diluted 1:200 in FWB buffer. Samples were run on a NovoCyte 96-well plate flow cytometer and analyzed using FlowJo v10 (Tree Star) analysis software. Three buffer only samples and secondary antibody alone conditions were used to define the spike-positive gate.

Monoclonal human antibodies

The following IgGs COVA1-26, COVA1-23, COVA2-38, COVA2-17, COVA1-20, COVA2-26, COVA1-22, COVA3-07, COVA2-03, COVA1-18,COVA1-12, COVA1-16, COVA2-01, COVA2-02, COVA2-04, COVA2-07, COVA2-11, COVA2-15, COVA2-29, COVA2-39, COVA2-44, COVA2-46, COVA2-10, COVA2-25, COVA2-30 have been reported (11). Cloning and characterization of human IgGs P008_056, P003_027, P008_039, P008_051, P008_052, P003_014, P008_057, P008_100, P008_081, P008_017, P008_087, P054_021, P008_007, P003_055, and P008_108 is described elsewhere (14).

ELISA with monoclonal IgGs

The assays were performed in a similar manner to the previously described protocol for serum samples (23, 65, 66). Briefly, high-binding ELISA plates (Corning, product code 3690) were coated with 3 μg/ml (25 μl per well) SARS-CoV2 WT S1 antigen (purified with or without acid treatment) or N121Q S1 in PBS, either overnight at 4 °C or for 2 h at 37 °C. Wells were washed with PBS supplemented with 0.05% Tween-20 (PBS-T) and blocked with 100 μl 2% casein in PBS for 1 h at room temperature. The wells were emptied and 25 μl of 2% (w/v) casein in PBS was added per well. This solution was supplemented with biliverdin at 10 μM where indicated. Serial dilutions of IgGs were prepared in separate 96-well plate (Greiner Bio-One) in 2% casein, and then 25 μl of each serial dilution added to the ELISA assay plates and incubated for 2 h at room temperature. Wells were washed with PBS-T. Secondary antibody was added and incubated for 1 h at room temperature. IgG binding was detected using goat-anti-human-Fc conjugated to alkaline phosphatase (1:1,000; Jackson, product code 109-055-098). Wells were washed with PBS-T, and alkaline phosphatase substrate (Sigma-Aldrich) was added and read at 405 nm. Area under the curve values were calculated using GraphPad Prism.

Pseudotype infectivity assay

Simian immunodeficiency (SIV) particles were used to assess effects of H207A, R190K and N121Q mutations on the function of SARS-CoV-2 spike. HEK293T cells, seeded one day earlier in 10-cm dishes in complete Dulbecco’s modified Eagle’s medium (DMEM, supplemented with 10% (v/v) fetal bovine serum, FBS), were co-transfected with 17 μg SIVMAC239-GFP, an env- and nef- defective provirus construct expressing a GFP reporter (67), and 4 μg pcDNA-SARS-CoV-2-del19, encoding SARS-CoV-2 spike with or without mutations in the biliverdin binding pocket. To improve pseudotyping efficiency, the constructs encoded a truncation of the spike C-terminal 19 amino acid residues (68). Viral pseudotypes were harvested 48 hours post-transfection, clarified by low-speed centrifugation at 300×g for 5 min and filtered through a 0.45-μm filter. The stocks of viruses pseudotyped with the spike variants were diluted to an equal reverse transcriptase activity (69). Six 5-fold serially diluted virus stocks were inoculated in quadruplicate in 96-well plates onto Huh7 and Vero cells, modified to overexpress ACE2 from a lentiviral vector, seeded one day before infection in 96-well plates. At 48 hours post-infection, fluorescent cells were counted using the Ensight plate reader (Perkin Elmer). Infectivity was calculated from values falling into a linear dilution range by dividing the number of infected cells in a well for the amount of reverse transcriptase activity associated to the virus inoculum, expressed in mU.

Pseudotype neutralization assay

HIV-1 particles pseudotyped with SARS-Cov-2 spike were produced in a T75 flask seeded the day before with 3 million HEK293T/17 cells (American Type Culture Collection; catalog code CRL-11268) in 10 ml complete DMEM, supplemented with 10% (v/v) FBS, 100  IU/ml penicillin and 100 μg/ml streptomycin. Cells were transfected using 60 μg of PEI-Max (Polysciences) with a mix of three plasmids: 9.1  μg HIV-1 luciferase reporter vector (65), 9.1  μg HIV-1 p8.91 packaging construct (70) and 1.4  μg WT SARS-CoV-2 spike expression vector (23) or its N121Q mutant version. Supernatants containing pseudotyped virions were harvested 48 h post-transfection, filtered through a 0.45-μm filter and stored at -80°C. Neutralization assays were conducted by serial dilution of monoclonal IgGs at the indicated concentrations in DMEM (10% (v/v) FBS and 1% penicillin–streptomycin) and incubated with pseudotyped virus for 1 h at 37°C in 96-well plates. HeLa cells stably expressing ACE-2 (provided by J.E. Voss, Scripps Institute) (71) were then added to the assay (10,000 cells per 100 μl per well). After 48-72 h luminescence was assessed as a proxy of infection by lysing cells with the Bright-Glo luciferase kit (Promega), using a Glomax plate reader (Promega). Measurements were performed in duplicate and used to calculate 50% inhibitory concentrations (IC₅₀) in GraphPad Prism software.

SARS-CoV-2 infectivity assay

SARS-CoV-2 strain BetaCoV/England/02/2020 (obtained from Public Health England) was propagated and quantified as described previously (72). VeroE6 cells were grown in DMEM (supplemented with 10% FBS) at 37°C and 5% CO₂ in 96-well imaging plates (Greiner #655090). SARS-CoV-2 (0.5 plaque forming units per cell) was added to DMEM with 2 or 10% (v/v) FBS with or without 100 μM biliverdin and added to the cells. At 22 hours post-infection, cells were fixed, permeabilized and stained for SARS-CoV-2 N protein using Alexa488-labeled CR3009 antibody (73) and 4′,6-diamidino-2-phenylindole (DAPI). The plate was imaged using the high-content screening Opera Phenix microscope (Perkin Elmer) with a 5x lens. Harmony software (Perkin Elmer) was used to delineate the whole well area and to determine the total intensities of the Alexa488 (SARS-CoV-2 N protein) and DAPI (which stains DNA) signals per said whole well area during image acquisition. Background-subtracted Alexa488 intensities were normalized to the untreated control condition.

SARS-CoV2 neutralization assay

Vero E6 (Cercopithecus aethiops derived epithelial kidney cells, provided by Prof. Wendy Barclay, Imperial College London) cells were grown in DMEM, supplemented with GlutaMAX (Thermo Fisher Scientific), 10% (v/v) FBS, and 20 μg/ml gentamicin, and incubated at 37°C in 5% CO₂ atmosphere. SARS-CoV-2 Strain England 2 (England 02/2020/407073) was obtained from Public Health England. The virus was propagated by infecting Vero E6 cells in T75 flasks (60-70% confluent), at a multiplicity of infection 0.005 in 3 ml of DMEM, supplemented with GlutaMAX and 10% (v/v) FBS. Cells were incubated for 1 hour at 37°C before adding 15 ml of the same medium. Supernatant was harvested 72 hours post-infection following visible cytopathic effect, and filtered through a 0.22-μm filter, aliquoted and stored at -80C. The infectious virus titer was determined by plaque assay in Vero E6 cells.

Neutralization assays were performed as previously described (65). Cells were seeded at a concentration of 20,000 cells/100 μl per well in 96-well plates and allowed to adhere overnight. Serial dilutions of monoclonal antibodies were prepared with DMEM media (supplemented with 2% FBS, 100  IU/ml penicillin and 100 μg/ml streptomycin, Thermo Fisher Scientific) and incubated with SARS-CoV-2 for 1 hour at 37°C. Biliverdin was added to the virus at a final concentration of 25 μM before addition to the antibody. The media was removed from the pre-plated Vero-E6 cells and the serum-virus mixtures were added to the Vero E6 cells and incubated at 37°C for 24 hours. These virus/serum mixtures were aspirated and cells fixed with 150 μl of 4% formaldehyde at room temperature for 30 min and then topped up to 300 μl with PBS. The cells were washed once with PBS and permeabilised with 0.1% Triton-X100 in PBS at room temperature for 15 min. The cells were washed twice with PBS and blocked using 3% milk in PBS at room temperature for 15 min. The blocking solution was removed cells were incubated with 2 μg/ml SARS-CoV-2 nuclear protein-specific murinized-CR3009 antibody in PBS supplemented with 1% milk at room temperature for 45 min. The cells were washed twice with PBS and horse anti-mouse-IgG-conjugated to HRP was added (1:2,000 in 1% milk in PBS, Cell Signaling Technology; product code S7076) at room temperature for 45 min. The cells were washed twice with PBS, developed using 3,3′,5,5′-tetramethylbenzidine substrate for 30 min and quenched using 2 M sulfuric acid prior to reading at 450 nm. Measurements were performed in duplicate.