key: cord-0936228-i2b9yul2
authors: Slezak, Tomasz; Kossiakoff, Anthony A.
title: Engineered ultra-high affinity synthetic antibodies for SARS-CoV-2 neutralization and detection
date: 2021-03-26
journal: J Mol Biol
DOI: 10.1016/j.jmb.2021.166956
sha: addee83bc63c291478b0311f2f0e06a4ca542963
doc_id: 936228
cord_uid: i2b9yul2

The Covid-19 pandemic is a centenarial global catastrophe. Similar events are likely to be recurring with more frequency in the future. The inability to control the virus’ impact is caused by many factors, but the lack of a technology infrastructure to detect and impede the virus at an early stage are principal shortcomings. Using phage display mutagenesis, we have generated a cohort of high performance antibody fragments (Fabs) that can be used in a sensitive point of care (POC) assay and are potent inhibitors (IC(50)- 0.5 nM) to viral entry into cells. The POC assay is based on a split-enzyme (β-lactamase) complementation strategy that detects virus particles at low nM levels. We have shown that this assay is equally effective for detecting other viruses like Ebola and Zika. Importantly, its components can be freeze dried and stored, but becomes fully active when rehydrated.

The COVID- pandemic caused by the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) has become a global health and economic calamity. Unfortunately, at the onset of the pandemic, few methods and reagents were available to mount a timely response to the threat. The rate at which new viral infections like CoV-19 proliferate across populations makes it virtually impossible to respond effectively in real time without having specific infrastructure in place. The current standard for detection is through nucleic acid-based assays that involve utilization of polymerase chain reaction (PCR) 1 . While highly reliable, these have been shown to be impractical in rapid large scale systematic testing. Thus, there have been attempts to develop more rapid point of care (POC) approaches to detect low abundance viral antigens without the requirement of sophisticated instrumentation that the PCR based tests require. Clearly, what is needed is a set of detection assay formats that are well vetted by regulatory agencies so that when other pandemic threats are identified in their nascent state, there is a roadmap for how to assemble a rapid chain of responses.

With this in mind, we describe here the development of a sensitive and robust point of care (POC) viral detection assay. As with other protein antigen assays, the main component is a set of high performance antibody-based reagents used for antigen detection. Importantly, the same antibodies used for detection might also bind to epitopes that would lead to virus neutralization. It has been established that the viral entry of SARS-CoV-2 into cells is initiated by the receptor binding domain (RBD) of the trimeric spike protein of the virus binding to angiotensin-converting enzyme 2 (ACE2) 2 . Blocking this interaction is thought to be the most promising approach to neutralize the virus. For our applications, high affinity Fabs against the receptor binding domain (RBD) of the spike protein (S-protein) were generated by phage display mutagenesis technology. The Fabs are based on the Herceptin Fab scaffold that has been engineered for stability and expression 3 . The principal epitope for Fab binding was found to be aligned with the ACE2 binding site on the RBD since it can be used as an effective viral inhibitor of cell entry. In this regard, using affinity maturation, we were able to generate a set of ultra high affinity binders that targeted this epitope with sub-nanomolar neutralization capabilities.

Most POC assays rely on some type of ELISA format for the detection readout 4 . In contrast, the detection assay described here involves a split-enzyme complementation readout, which can have orders of magnitude better signal to noise discrimination than classical ELISA methods 4 . The split-enzyme used in this complementation assay is based on the reconstitution of two fragments of β-lactamase to produce a fluorogenic signal. It is a variant of a traditional sandwich assay, the N and C-terminal fragments of β-lactamase are attached independently to different Fabs that recognize two distinct epitopes and thus, can bind simultaneously to the RBD target. Further, the complementation constructs containing the enzyme fragments are designed to be modular so that Fabs generated to other virus targets can be interchanged in a plug and play fashion. For instance, the same system detects Ebola and Zika antigens alongside SARS-CoV-2 antigen detection by simply adding the appropriate Fabs for the target of interest 3 . Thus, the assay can be quickly recapitulated depending only on the step to generate Fabs to the desired target antigen. Other attributes built into our POC detection assay is that it can be packaged in a kit, which can be stored and rapidly activated without losing sensitivity.

Our objective was to generate a cohort of high performance synthetic Fabs to the receptor binding domain (RBD) of SARS-CoV-2 that could be used for sensitive enzymecomplementation detection assays and for possible viral neutralization purposes. To generate Fabs that fill these criteria, we undertook a phage display mutagenesis campaign using the receptor binding domain (RBD) of SARS-CoV-2 as the target antigen. The RBD is highly glycosylated and thus was expressed in mammalian cells. Exploiting its high level of glycosylation, the protein was biotinylated through its carbohydrate groups with EZ-Link Hydrazide Biotins (Thermo) to facilitate immobilization onto streptavidin-coated paramagnetic beads during the phage display biopanning procedure. Five rounds of phage display selection were performed with a high diversity (10 10 ) synthetic library 5 using previously published protocols 6; 7 . To obtain high affinity binders, the concentration of the RBD antigen was systematically reduced, starting from 500 nM during the first round and ending with 1 nM in round 5. To acquire binders with a slow dissociation rate, additional selection pressure with longer washes during biopanning was applied. Phage ELISA was performed on 192 clones resulting in identifying 5 unique high affinity variants: RBD1-RBD5 with RBD1 having the highest ELSIA signal [ Figure S1 ].

A key component of developing the split-enzyme complementation assay involves having a pair of high affinity Fabs that can bind simultaneously. An anticipated challenge was that since the SARS-CoV-2 RBD is heavily glycosylated, the available surface space to accommodate Fabs with non-overlapping epitopes would be reduced significantly. Having the high affinity RBD1 Fab in hand from the first selection, we sought to generate a second set of Fabs that bound to the RBD through independent epitopes. To obtain these Fabs, we employed an epitope masking strategy that involved adding the RBD1 Fab as a competitor during a second biopanning campaign. To do so, five rounds of selection with 1 μM RBD1 added as a competitor were performed starting with a 200 nM antigen concentration in round 1 and ending with an antigen concentration of 1 nM in round 5. After phage ELISA, positive clones were sequenced resulting in two unique sequences: sRBD6 and sRBD7, as well as the previously selected RBD5, indicating that this Fab from the original selection also had an independent epitope compared to RBD1

[ Table S1 ]. From this set, we chose sRBD7 to pair with RBD1 from the first selection to carry forward for the development of the complementation assay.

The binding affinities of RBD1 and sRBD7 were determinate by Surface Plasmon Resonance (SPR) showing they had similar binding constant (K D ) of ~3 nM. However, their binding kinetics were quite different, where sRBD7 had almost an order of magnitude slower dissociation rate [ Figure 1 ]. This reflects the success of the additional stringency placed on the biopanning conditions used for its selection.

We have observed that epitope binning experiments based on protein ELISAs have to be interpreted with caution since Fabs that share a relatively small amount of epitope overlap can appear to be independent. To better quantify the independent epitopes, we performed epitope binning experiments by SPR. This confirmed that RBD1 and sRBD7 do bind to two distinct epitopes [ Figure S2 ]. Further, although a full kinetic evaluation of RBD1 binding to the full SARS-CoV-2 spike protein could not be done due to a paucity of available protein, high affinity binding was confirmed based on a single injection SPR analysis (K D~ 3 nM), which showed a similar binding profile to that observed for its binding to the RBD [ Figure S3 ].

Although the RBD1 has a high affinity (3 nM) and displays good kinetics, for the purposes of the complementation and neutralization assays, we decided to further improve its dissociation rate. Therefore, we initiated an affinity maturation campaign by designing and constructing phage display libraries to introduce higher diversity in CDR-H1. The choice of CDR-H1 was somewhat arbitrary since we did not have direct evidence to the extent of its engagement with the antigen; nevertheless, our experience has been that the heavy chain CDRs have a higher propensity to be involved antigen binding compared to light chain CDRs. We designed a combination of "tailored" and "hard" randomization strategies incorporated into six CDR-H1 positions. To that end, two sub-libraries were created, where in the first library mutated positions were bias to hydrophobic and aromatic amino acids, while the second library involved including all possible amino acids into the six positions. To ensure the improvement of Fab off-rates, additional selection pressure was applied during the biopanning. Three rounds of selection were performed with the RBD concentration being decreased accordingly, from 10 nM to 20 pM. Each round was additionally supplemented with four consecutives 30-minute washing steps to strongly bias towards slow dissociation of the selected candidates.

After round 3, 96 clones were picked and tested in phage ELISA leading to the identification of 19 sequence unique Fabs. Sequence alignment of these unique CDR-H1 variants showed no randomization at position 1 and a very limited randomization at position 5 and 6 compared to original RBD1 CDR-H1. High diversity at position 2, 3 and 4, with a preference for His at position 2 was observed [ Figure 2A ]. The binding analysis showed the 10-100-fold affinity improvement of matured CDR-H1 variants compared to the parent RBD1 Fab [Table S2 ]. Based on the overall binding kinetics, the affinity matured RBD1.5 variant (designated as mRBD1.5) had an affinity (K D ) of 42 pM, where both the association and dissociation rates were improved by two orders of magnitude in comparison to WT RBD1 [ Figure 2B and 2C].

Previously we developed a sensitive protein complementation assay that was successfully applied for the detection of Ebola and Zika virus proteins 3 . The system involves the use of the well established proximity-driven activity reconstitution of a TEM1 -lactamase (BL) split-enzyme system 8 . In this assay, the two separate fragments, BFL1 (residues 26-196) and BFL2 (residues 198-220), are attached respectively to the two target molecules whose proximity is being evaluated. The assay system employed here does not involve linking the BFL fragments directly to the target molecule, but attaches these fragments to Fabs that are themselves directed against two distinct epitopes of the target, in this case the RBD of SARS-CoV-2. However, we have found that direct fusion constructs containing Fabs with linkers comprising the BFP fragments are difficult to express and tend to aggregate 3 . Therefore, to circumvent these problems, we developed an alternative approach that exploits the high affinity (100 pM) between engineered forms of protein-G (pG) and a Fab's constant domain [ Figure 4A ]. These engineered components are referred to as pGA1 (for protein G) and Fab LRT (for the Fab). In this assay, the two separate fragments of the BL (BLF1 and BLF2) are attached through a linker to engineered protein pGA1 9 .

Thus, using the ultra-high affinity of Fab LRT scaffold 3 to protein pGA1, we were able to generate the pair of RBD1-BLF2 and sRBD7-BLF1 by premixing them separately to a final concentration of 250 nM. Conceptually, this non-wash assay requires simultaneous binding of the two Fab LRT pairs to the target RBD protein [ Figure 3B ]. Without knowledge of the RBD1 and sRBD7 epitope positions on the RBD, we decided to use a Gly-Ser linker of 15 residues between the protein pGA1-BLF (1 and 2) constructs. Titrating with increasing RBD concentration resulted in a detectable fluorescent signal at 30 nM, which increased linearly over the range from 30 to 125 nM with a distinct maximum at 250 nM [ Figure 3C ]. A reduction of the signal is observed at RBD excess, presumably caused by a breakdown of the stoichiometry at high antigen concentration due to the hook effect. To establish how the assay is influenced by the affinity levels of the Fab, we replaced the RBD1 Fab (K D ~3 nM) with the mRBD1.5 Fab (K D ~42 pM) coupled to BLF2, while keeping sRBD7 attached to BLF1. This resulted in about ~4-fold improvement in detection ( Fig.   S4 ]. Control experiments involving attaching the two BLF fragments to either Fab RBD1 or sRBD7 resulted in no detectable signal when added in the presence of 250 nM RBD. This indicates that productive enzyme complementation requires the two Fabs to bind simultaneously to the same RBD molecule [ Figure S5 ].

Next, we tested if the complementation system could be used for detection of full trimeric S-protein, since the RBD Fab epitopes are unknown and might not be accessible in a context of a full-length S-protein. Notably, the S-protein was readily detected with a higher sensitivity with a detectable concentration starting at 7 nM with a distinct maximum at 125 nM [ Figure S6 ]. A similar control experiment to the one above, where each Fab was premixed with both components (i.e. RBD1-BLF1, RBD1-BLF2) showed that measurable signal was not produced in this format [ Fig. S7 ]. Thus, as was the case for the RBD domain alone, triggering a signal requires the Fabs to bind to two independent epitopes on the same trimeric S-protein configuration.

One of the key features we wished to instill in our point-of-care assay for ease of storage was the ability to preserve the functionality of the components upon reconstitution from a freeze-dried form. To that end, single Fabs, RBD1-BLF2 and sRBD7-BLF1 at 500 nM were lyophilized overnight. Upon reconstitution no aggregation was observed and the Fabs' binding properties were unchanged [ Figure S8A ]. Moreover, the pGA1-FAB LRT complementation assay performed equally well as the control (not lyophilized) when the sample was supplemented with a protein carrier (BSA) as part of the freeze-drying procedure. Lack of BSA supplementation led to 40% signal reduction [ Figure S8B ].

To determine the potential level of virus neutralization, the Fabs were tested in a plaque reduction assay that measures the cell survival afforded by the Fabs. This is a stringent assay that is the gold standard currently in use 10 . RBD1 showed a dose-dependent SARS-CoV-2 infection neutralization with an IC 50 of 4.8 nM [ Figure 4B ]. Conversely, as expected, sRBD7 showed no virus neutralization capacity [ Figure 4B ], since it recognizes a different epitope than RBD1.

Additionally, we anticipated that neutralization could be further increased by converting the RBD1 Fab into a bivalent IgG type format. As an alternative approach to introducing bivalency, we tested the Protein pGA1 dimer with 52 Gly-Ser linker with two LRT grafted 3 RBD1 Fabs. This resulted in 2.5-times improvement in viral neutralization (IC 50 = 1.9 nM) [ Figure 4C ]. Additionally, the affinity matured fab, mRBD1.15, had over 10-times improved neutralization capabilities (IC 50 = 0.48 nM) in a monovalent form [ Figure 4D ]. These findings suggest a potential for the development of anti-viral drugs based on Fabs that bind tightly to the RBD.

We have described the generation and validation of a cohort of Fabs produced by phage display mutagenesis (Table S1) An additional challenge for generating antibodies to the RBD is that the S-protein is heavily glycosylated, presumably to help the virus evade the immune system 12 Phage display selection produced four Fab binders (RBD1-4), which shared the same epitope. Of these binders, RBD1, had superior binding properties, as judged by ELISA and SPR (K D -3 nM). A competition assay with soluble ACE2 showed that this epitope is associated with the ACE2-RBD interface [ Figure S9 ]. To assess the ability of RBD1 to neutralize the viral activity of SARS-CoV-2, a Plaque reduction assay was performed 10 . This is a stringent assay that measures the percentage of cell survival as a function of Fab concentration. Serial additions of the RBD1 resulted in a clear dose dependent cell survival response with an IC 50 of 4.8 nM [ Figure 4B ].

Notably, using the monovalent RBD1 Fab alone displayed comparable neutralization potency with other reported IgG antibodies having bivalent formats [14] [15] [16] . We next decided to evaluate whether further improvement could be achieved by converting RBD1 into a format mimicking IgG bivalency. This was done by employing an engineered construct we had previously developed that effectively couples two Fabs together through a linker of adjustable length 3 [ Figure 3A ]. An important consideration for the linker length was to ensure the linked Fabs could bind on different S-proteins on the viral coat since there is only a single accessible RBD available for Fab binding per spike. As a compromise between limiting the linker length, while ensuring that it was long enough to facilitate the two RBD1 Fabs to bind across spikes (~160 Å apart 17 ), a 52 residue Gly-Ser linker was employed. The viral neutralization potential of this bivalent construct was evaluated in the plaque reduction assay and showed a 2.5-fold improvement (IC 50 -1.9 nM) in cell protection over the monovalent RBD1 Fab ( Figure 4C ). Because these assays have to be run at a special containment facility and consequently are low throughput, we were not able to systematically test different linker lengths to further optimize the bivalent effects of the construct.

While the RBD1 Fab had potent neutralization properties, we sought to further improve it through an affinity maturation process. From the affinity maturation phage display selection, 19 unique clones were isolated and reformatted into protein format. The affinities and kinetics of these Fabs showed marked reductions in K D and dissociation rates; for instance, affinity matured Fab, mRBD1.5 had a 100-fold improved affinity and off-rate compared to the parent RBD1; a number of the other affinity matured Fabs showed affinity increases in the range of 50fold [Table S2 ]. Notably, a number of these Fabs exhibited extremely slow off-rates which were at the limits of what can be measured by SPR accurately, so their affinities may be underestimated.

To establish whether these higher affinities would translate into more effective inhibitors of viral entry, the plaque reduction assay was performed using mRBD1.15 (K D -100 pM). Indeed, this Fab displayed a 10-fold greater neutralization capacity (EC 50 -0.48 nM) than the RBD1 parent (EC 50 -4.8 nM). Although there were several affinity matured Fabs with higher affinities (mRBD1.5-42 pM, mRBD1.9-62 pM), these were not tested because at affinities below 1 nM, the dynamic range of the assay is significantly reduced. Likewise, improved neutralization that may have been produced by converting these Fabs into a bivalent format could not be evaluated for similar reasons.

The second goal of the project was to develop a sensitive high throughput point-of-care (POC) detection system to identify virus infection. To accomplish this, we employed an assay built upon our previously developed and deployed split-enzyme complementation assay for the detection of Ebola and Zika virus based on the split β-lactamase system 3 . This complementation format is a variation of a classical sandwich assay and has superior target specificity and sensitivity compared to traditional ELISA assays 4 . Having established this proof of concept, we endeavored to repurpose the detection platform for detecting SARS-CoV-2.

For the complementation assay to detect the RBD, we used RBD1 from the first selection and sRBD7, which was obtained using an epitope masking strategy ensuring it bound to an orthogonal epitope to RBD1. Connecting these Fabs to the β-lactamase fragments using the pGA1-Fab LRT constructs resulted in detection with excellent signal-to-noise of the RBD domain at a concentration of 30 nM [ Figure 3C ]. We next tested the sensitivity in the context of the full S-protein. In this format, possible interference due to glycosylation or other steric shielding involving the trimeric nature of the S-protein could be assessed. For instance, in the full trimeric S-protein, the RBD would be displayed in two conformational states, one copy in the open position making it accessible for ACE2 binding and two copies in the down position, which presumably covers this binding site. We anticipated that RBD1 would bind to the open state since its mode of neutralization involves direct epitope competition with ACE2. Notably, the epitope for sRBD7 is also available since adding the two Fabs with their associated β-lactamase fragments leads to enzyme reconstitution and activity. Importantly, the detection level is more sensitive in the context of the full S-protein leading to appreciable signal over noise discrimination at 7 nM concentration of the S-protein [ Figure S6 ]. Thus, we postulate that using the affinity matured mRBD1.5 version would lead to a further increase in detection sensitivity.

The linker lengths on the BLFs are too short to accommodate complementation between An additional enhancement is the assay's portability that provides for the POC aspects of its utility. The objective was to establish a kit where all the reagents could be packaged and stored on the shelf, to be reconstituted when needed upon rehydration. To accomplish this, we tested whether the Fab and pGA1 linkers with the associated enzyme fragments could be lyophilized and reconstituted with no loss in functionality. Figure S8 shows that these components are not affected by lyophilization and are as active after reconstitution as their counterparts which were not lyophilized. Thus, it will be possible to package an assay like this into a kit that is cheap, storable and readily useable in the field.

To put this work into context, we undertook this project with the full appreciation that the tools and reagents that we produced would not make an immediate impact during the current pandemic. However, the strategies devised and applied here provide a blueprint for quickly responding to future challenges, which will unfortunately occur. As in the case of many efforts to respond to the Cov-19 pandemic in real time, this work was accomplished during a lab shutdown with minimal research material and staff. Nevertheless, exploiting our phage display mutagenesis pipeline, we generated a set of high performance inhibitors to viral entry. Further, repurposing an assay platform that was previously developed for detecting Ebola and Zika infections, we were able to quickly incorporate a set of high performance Fab binders into a detection platform that could be utilized for sensitive virus detection in an easily used kit format.

We thank the Wilson and Hubbell labs from the University of Chicago for providing the RBD protein and Wells lab from the UCSF for ACE2 protein. We acknowledge the assistance and advice of S. Mukherjee, E. Davydova and A. Prominski. We thank G. Randall (University of Chicago) for performing the virus plaque reduction assay at the BCL3 facility at Argonne National Laboratory. We acknowledge support from NIH GM082545 (AAK).

The sequences of the constructs used are provided in Table S3 . The RBD protein was produced in mammalian cells (gifted by Wilson and Hubbell labs from the University of Chicago).

Proteins for the split enzyme proximity assay were cloned into pHFT2 vector 18 with the strategy described previously 3 . Selected Fabs were cloned from phage into Sph1 sites of pSFV4 expression vector using an Infusion HD cloning kit (Takara Bio) according to the protocol. All selected Fab CDR sequences are provided in Table S1 . The Fab LRT scaffold was grafted into Fab light chain at aa positions 123-127 (SQLKS -> LRT) using quick change site-directed mutagenesis. For the proximity assay, pGA1-BLF fusions were expressed and purified as described previously 3 . Briefly, proteins were expressed in BL21 (DE3) overnight in 20°C post induction with 1 mM IPTG at OD 600 = 0.6. Cells were sonicated in buffer A containing 50 mM Tris-HCl, pH 8.0, 150 mM NaCl and 10% glycerol. The insoluble His-tagged pGA1-BLF fusions were extracted from the cell pellets by 6M Gua-HCl in buffer A with 0.3 mM TCEP and purified on TALON resin (Takara Bio) using a denaturation-condition protocol and on-column renaturations reached by six washes of the column with serially diluted 6M Gua-HCl, followed by the final wash in buffer A alone.

Proteins were eluted from the column with 100 mM imidazole in buffer A. Fusion proteins were stored on ice and never frozen.

To obtain high affinity binders, five rounds of selection were performed using phage display selection protocol previously described in 6; 19 . RBD protein was biotinylated via glycoproteins with EZ-Link Hydrazide Biotin (Thermo Scientific) as recommended in order to immobilize onto streptavidin-coated paramagnetic beads (Promega and Dynabeads M0270, Invitrogen). In the first round of selection, 500 nM of RBD was immobilized on 200 l SA magnetic beads (Promega) and was incubated with 1 mL phage library (10 11 cfu) for 1 hour at room temperature with gentle shaking. The beads were washed three times to remove nonspecific phage and added to log phase E. coli XL-1 blue cells (Stratagene) and incubated for 20 minutes at room temperature. Then, media containing 100 g/mL ampicillin and 10 9 p.f.u./mL of M13K07 helper phage (NEB) was added for overnight phage amplification at 37°C. For all subsequent rounds, the amplified phage was precipitated in 20% PEG/2.5 M NaCl for 20 minutes on ice.

Before each round, the phage pool was negatively selected against empty paramagnetic beads for 30 minutes with shaking to eliminate nonspecific binders. The final concentration of antigen was dropped systematically from 500 to 1 nM from the first to the fifth round (2 nd round: 200 nM, 3 rd round: 50 nM, 4 th round 10 nM and 5 th round 1 nM). After phage binding, the beads were subjected to five washing rounds. Last two washes steps were 20 and 25 minutes respectively. This additional selection pressure was supposed to remove all low affinity binders. The bound phages were eluted using 0.1 M glycine, pH 2.6 and neutralized with TRIS-HCl, pH 8. Then, the phage eluate was used for E. coli infection and phage amplification as described above. Additional selection to generate non-overlapping epitope with sRBD1 was performed. Selection protocol was as described above with addition of 1 of sRBD1 in every step to ensure binding to a different epitope. The final concentration of antigen was dropped gradually from 200 to 1 nM from the first to the fifth round (2 nd round: 50 nM, 3 rd round: 20 nM, 4 th round 10 nM and 5 th round 1 nM). After round 4 th and 5 th phages were plated on ampicillin plates and 96 single colonies were picked for single-point phage ELISA assays. The promising clones demonstrating high ELISA signal and low non-specific binding were sequenced and reformatted into a pSFV4 expressing vector as described in Protein expression and purification.

The ELISA protocol was described previously 20 . Briefly, 50 nM of RBD was directly immobilized on high binding experimental wells (Greiner Bio) and BSA was immobilized in control wells, followed by extensive blocking with BSA. After 15 minutes incubation with phage, the wells were extensively washed three times and incubated with Protein L-HRP (Thermo Scientific, 1:5000 dilution in HBST) for 20 minutes. The plates were again washed and developed with TMB substrate (Thermo Scientific) and quenched with 10% H 3 PO 4 , followed by the absorbance at A 450 determination.

Phage libraries of RBD1 for affinity maturation were created using the strategy previously published 21 . To that end, a stop codon was introduced in CDR-H1 with quick-change mutagenesis.

Two phage libraries with "hard" and "tailored" randomization strategies were created with the phosphorylated oligos. ssDNA containing stop codon introduced in the middle of CDR-H1 was isolated from phage (using QIAprep Spin M13 Kit, Qiagen) and used in a Kunkel mutagenesis protocol 22 

All Surface plasmon resonance (SPR) analyses were performed on a MASS-1 (Bruker). All targets were immobilized via a 6x His-tag to a Ni-NTA sensor chip. Fabs in twofold dilutions were run as analytes at 30 l/min flow rate at 20°C. Sensograms were corrected through double referencing and 1:1 binding model fit was done using Sierra Analyzer (Bruker). For epitope binning experiments, after injection of a saturating concentration of the RBD1 Fab, an equal molar mixture of sRBD7 fab was injected and increase in Response Unit (RU) was observed.

Viral detection protocol using non-wash pGA1-FAB LRT protein complementation assay was previously described 3 

Vero E6 cells (ATCC) were infected under biosafety level 3 conditions with SARS-CoV-2 (nCoV/Washington/1/2020, kindly provided by the National Biocontainment Laboratory, Galveston, TX). The neutralization assay was performed as previously described 23 with some modifications. Briefly, the Fabs were serially diluted 4-fold and mixed with 400 PFU of SARS-CoV-2

for one hour at 37ºC, then used to infect Vero E6 cells for three days. Cells were fixed with 3.7%

formalin and stained with 0.25% crystal violent. Crystal violet-stained cells were then quantified by absorbance at (595 nm) with a Tecan m200 microplate reader. The 50% neutralization titer was then calculated using GraphPad Prism. Graphical abstract

 Fab-based reagents with SARS-CoV-2 neutralization capabilities  Sensitive high throughput point-of-care virus detection kit  Multiple epitope binders to spike protein  Plug and play detection system with stable shelf life.

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