Introduction

What are Minibinders?

These mini proteins target the interaction between ACE2 and SARS-CoV-2 spike protein ^[1]. The mini binders are small proteins designed to bind to the SARS-CoV-2 spike protein with a greater affinity than ACE2 ^[1]. These mini binders reduce the viral burden of SARS-CoV-2 in mice ^[2]. Minibinders were de novo designed to mimic the ACE2 helix, but have a lower dissociation constant, yielding a greater affinity for the spike protein ^[1]. The binding region between (PDB: 8K4U) makes it seem like binding region is telling how these proteins were designed. Taking a closer look at the SARS-CoV-2 disease pathway shows where the minibinders target the interaction between ACE2 and SARS-CoV-2 spike protein.

Figure 1. Image of the individual helices of AHB2, LCB1, and LCB3, respectively, bound to the RBD of the spike protein.

SARS-CoV-2 Disease Pathway

Minibinders mimic the pathway of the SARS-CoV-2 virus attachment to the cell surface receptors. In the standard process, the SARS-CoV-2 surface spike proteins ACE2. This anchors to the host for viral entry ^[3]. When the spike protein binds to the ACE2 receptor, the cell membrane-associated protease, TMPRSS2, activates the spike protein, promoting viral entry ^[4]. The activated spike protein then cleaves itself into S1 and S2 subunits ^[4]. The S1 subunit contains a receptor binding domain that recognizes and binds to ACE2 ^[4]. The S2 subunit undergoes a conformational change which permits viral entry ^[4]. The S2 domain has a fusion peptide (FP) domain that will help regulate membrane fusion by disrupting and connecting the host cell’s membrane ^[4]. The S2 domain is also composed of HR1 and HR2 subunits, which are heptapeptide sequences involved in the entry of SARS-CoV-2. HR1 is located at the C-terminal domain of a hydrophobic FP, and HR2 is located at the N-terminal of the transmembrane domain ^[4]. In this conformational change, the S2 subunit inserts its FP domain into the host cell's membrane. Once the host cell’s membrane is penetrated, this triggers an interaction with the HR2 domain and HR1 trimer, forming the 6-helical bundle. The bundle brings the viral envelope and cell membrane in close enough distance for viral fusion and ultimately viral entry ^[4]. Once inside, the virus translates viral proteins, eliciting an immune response and spreading the viral particles throughout the body ^[4]. See also: Coronavirus Disease 2019 (COVID-19)

Minibinders block SARS- CoV-2 Acceptor Binding

The primary goal of the mini binders is to prevent the spike proteins from binding to ACE2, blocking viral membrane attachment ^[2]. Because the mini binders have a greater binding affinity than ACE2 for the spike protein, they prevent viral entry and infection ^[5]. Targeting this specific interaction between the SARS-CoV-2 spike protein and ACE2 are potential targets for future therapeutics to treat the virus ^[4]. There is a demand for more treatments for SARS-CoV-2. These minibinders pose an advantage to other therapeutics, such as antibodies, because they are much smaller in size and more stable ^[1]. As for vaccines, constantly updating and modifying them drains finances and time. The faster and more cost-appropriate answer is in the minibinders ^[1].

Expectations of this page

The focus of this page is on the design of mini binders and how they effectively prevent the entry of the viral SARS-CoV-2 spike protein. To explain inhibition by the minibinders, we will initially describe the structure of the spike protein and its interaction with ACE2. We will then explain the helical design of minibinders and how they block spike protein function. Laying the foundation for the mini binders, we will then take a look at how the mini binders are designed to obtain the best possible helical structure. With that, then it is finally time to look at the receptor binding domain between the various mini binders and their interactions with the spike protein.

SARS-COV-2 Spike Protein

Figure 2. Spike protein shown in "B-Factor"; depicting mobility and flexibility of different portions. Depicted in red are the most mobile, whilst dark blue are the least mobile. The 2 red portions depict RBDs, which correspond to 1-up and 2-up conformational states.

The (PDB: 7QUS) of SARS-COV-2 is a symmetric trimer featuring 3 spike glycoprotein chains (UNIPROT: P0DTC2). Each monomer of the spike is called a spike glycoprotein, and the total assembly contains 2 main parts: The (PDB: 7V78) and (PDB: 7V78) subunits^[4]. However, the native spike protein does not exist in this state prior to infection. The protein is actually inactive initially, but is later activated by proteases cleaving the inactive S protein into its two active subunits^[4]. For more information about the cleaving of the native protein by furin, please reference SARS-CoV-2_protein_S_priming_by_furin. The S1 subunit contains : N-Terminal domain (NTD; blue), C-Terminal Domain (CTD; red), and the Receptor Binding Domain (RBD; bisque) (PDB: 7V7A). The RBD is responsible for (PDB: 8K4U) on the surface of the target cell, as well as neutralizing antibodies. The NTD, CTD, and their relevant interfaces actually play much larger roles in the binding of the spike protein to ACE2 than the RBD does due to their larger surface areas^[4]. The S2 subunit is responsible for viral fusion and entry. Once bound to ACE2, and after the different domains in S2 have anchored to the membrane as well as delivered the viral envelope, the S2 subunit then changes conformation from the pre-hairpin to (PDB: 6M3W) conformation^[4]. The S2 subunit contains a fusion peptide domain (FP), heptapeptide repeat sequences 1 and 2 (HR1 & HR2), TM domain, and cytoplasmic fusion domain (CT). Full information about the location and structures of these domains within the S2 subunit can be found in references 1 and 3^[4][6]. For the purpose of this article about the minibinders, attention will be directed to the S1 subunit and its binding properties with ACE2. An animation and explanation of the fusion mechanism can be found in SARS-CoV-2_spike_protein_fusion_transformation. Throughout the entire process, the spike protein has 3 main conformations. An (PDB: 7QUS) conformation; an active, "open" conformation; and a 6M3W) conformation mentioned previously^[4][7][6]. In the closed conformation, the RBDs of each monomer are tucked inwards, preventing interaction. In the open conformation, however, 1 or more of these RBDs can be in the "up" conformation, meaning they are exposed and able to interact within the extracellular space. Mainly, there exits a "" (PDB: 7V78) and "" (PDB: 7V7A) conformation in this phase^[7][6]. Depicted in Figure 1, the RBDs of the spike protein have the highest mobility, which further support the many conformational changes in which they are involved. Most of the depictions of the minibinders bound to the spike protein show the spike protein in the 2-up conformation.

See also: SARS-CoV-2_protein_S, Spike protein, SARS-CoV-2_spike_protein_mutations (About the spike protein in further detail)

ACE2

(PDB: 1R4L) is a carboxypeptidase present on cell surfaces that is responsible for the degradation of angiotensin II. It is a critical enzyme in the suppression of the renin-angiotensin system. This improves both cardiovascular and renal systems, as well as abates acute respiratory distress syndrome (ARDS). It does the 2 former via the RAS System's role in the regulation of blood pressure, renal function, water homeostasis, electrolyte balance, and/or inflammation^[8]. The critical role that this enzyme plays in the regulation of this system is what results in the adverse symptomology observed in victims of the SARS-COV-2 virus. The ACE2 receptor is considered the only essential receptor in the SARS-COV-2 viral mechanism, and thus the collateral debilitation of ACE2 results in the adverse respiratory effects including ARDS, pulmonary edema, destruction of alveolar structures, and others^[8]. This relationship was further proven when ACE-2 deficient mice had developed these effects at higher rates compared to the wild type^[9]. Further information can be found in Angiotensin-Converting_Enzyme.

As mentioned previously, all of the S1 subunit domains play important roles in the (PDB: 8K4U). The surface area of the NTD and CTD are particularly important, along with the direct interactions observed in the RBD. Whilst ACE2 is not the focus of this article, understanding its role in the infection pathway of COVID 19, as well as how it binds to the spike protein will assist in understanding the design and functional processes of the minibinders.

Minibinders

Design

AHB2 is a Series A Helix Binder which is a miniprotein that binds specifically to the alpha helix of the protein. LCB1 and LCB3 are long chain bases that are longer in length which allow for more contact between the RBD, increasing the binding affinity. These mini binders, AHB2 and LCB1, were designed de novo with the intention to mimic the binding of ACE2 to the spike protein ^[1]. Using Rotamer Interaction Field (RIF) docking, the proteins were able to make the most efficient bonding using the ACE2 spike protein binding interface ^[1]. Using Site Saturation Mutagenesis (SSM), every residue in the minibinder’s helix scaffold was substituted with each of the 20 amino acids, one at a time, computationally choosing the best sequence ^[10]. Forming SSM libraries,experimental tests were run on each of the libraries to converge on a small number of closely related sequences ^[10]. From these libraries, one of these was selected for each design, AHB2 or LCB1-LCB8^[1]. AHB2 was designed using an ACE2 helix scaffold, while LCB1 and LCB3 were designed completely from scratch, attempting to make the best possible helix with the greatest affinity for the spike protein receptors . Although LCB1 was designed before LCB3, LCB3 was less effective at neutralizing the viral response with a high IC₅₀ Value ^[1] . These minibinders are small proteins, modeled similarly to the ACE2 and SARS-CoV-2 spike protein. There were two strategies utilized. One strategy included directly incorporating the ACE2 helix of the RBD and creating more interactions, increasing the binding affinity of the minibinders ^[1]. The other strategy was designing the minibinders completely from scratch, completely dependent on the RBD ^[1]. AHB2 utilized the first method, incorporating the ACE2 helix, while LCB1 and LCB3 utilized the second method ^[1] .

Potency of the minibinders

Examining the IC₅₀ values of the various mini binders gives quantitative data to the effectiveness of the proteins in preventing an immune response. The highest IC₅₀ was AHB2 (15.5 nM), followed by LCB3 (40.1 pM) LCB1 (23.5 pM) ^[1]. The higher IC₅₀ indicates a larger concentration of mini binder required to inhibit the biological process. Both LCB1 and LCB3 proved to be significantly more effective than AHB2, LCB1 and LCB3 were within 3-fold of the most potent anti-Spike monoclonal antibodies described to date ^[1].

Structure

These minibinders were designed to form stronger connections to the spike protein RBD than ACE2^[1]. This section highlights some important residue connections with the RBD that give the minibinders higher affinities for the spike protein than ACE2.

ACE2 binds to the spike protein RBD using . The minibinders are smaller than ACE2, but still form strong connections to the spike protein. This means the minibinders interact with the RBD residues more efficiently than ACE2 giving them a higher affinity for the spike protein ^[1]. AHB2 was designed to mimic ACE2 while making better use of the RBD residues giving it a higher affinity for the spike protein with an IC₅₀ value of 15.5 nM^[1] (). LCB1 was designed from scratch to bind the most efficiently to the RBD residues giving it the highest affinity with the lowest IC₅₀ value of 23.5 pM^[1] (). LCB3 was designed after LCB1 with the goal of making the minibinder even more efficient, however it ended up having a lower affinity than LCB1 with a higher IC₅₀ value of 40.1 pM^[1] ().

The Glutamine-493 residue on the spike protein is an important residue in showing the differences in strength between ACE2 and the minibinders ^[1]. ACE2 does not make use of this residue when . The nearest residues of ACE2, Gln35 and Lys31, do not form any interaction on Gln493 of the spike protein. The AHB2 minibinder, instead forms a on the Gln493 of the spike protein residue of the spike protein with its Glu41, increasing affinity to the spike protein. LCB1 forms on Gln493 of the spike protein using its Asp17 and Arg14 residues, giving it the highest affinity based on the Gln493 residue. However, these interactions are not required. LCB1 forms with the Gln493 residue of the RDB previously mentioned, yet it still has a higher affinity to the RBD than AHB2.

Similarly, LCB1 forms with both the Lys417 and Arg403 of the spike protein from its Asp30 residue. This is a very strong interaction, further contributing to the high affinity of LCB1 to the spike protein^[1]. ACE2, however, forms only with the Lys417 from its Asp30 residue.

Implications

Results from mice study

The effectiveness of the most potent minibinder was examined in mice. LCB1 was administered to the mice via nasal delivery. As expected, compared to control mini protein, the LCB1 was significantly more effective at reducing the viral burden, diminishing the immune cell infiltration, and inflammation ^[2]. The virus was not detected in the lungs 4-7 days post-infection, and the spleen, heart, and brain had viral RNA at very low concentrations ^[2].

Benefits of minibinders over other therapeutics

The size of these mini binders is a large reason why they are so effective. The minibinders have a 20-fold more potential for nebulization compared with antibodies, and the molecular weight of the minibinders is 5% of a full antibody molecule ^[1]. When the LCB1 wasa attached to a human IgG domain to enhance bioavailability, staying in the body longer, LCB1 was less effective ^[2]. This is likely due to the increase in size when bound to the antibody. The high stability of the mini binders allows them to be administered as a gel via nebulization ^[1]. Future directions of mini binders are to increase the efficiency of the process to obtain a sequence for pathogen neutralizing designs more promptly ^[1]. Given that there are only a small number of antibody therapies and vaccines approved for treatment of SARS-CoV-2, minibinders as potential therapeutics may lay the foundation for similar minibinders designs as treatments for other viruses.