key: cord-0690994-p7d99tmt authors: Somasundaram, Rajeswari; Choraria, Ankit; Antonysamy, Michael title: An approach towards development of monoclonal IgY antibodies against SARS CoV-2 spike protein (S) using phage display method: A review date: 2020-06-03 journal: Int Immunopharmacol DOI: 10.1016/j.intimp.2020.106654 sha: 7dbda65d4f485c827d902b939170904dbed2cfce doc_id: 690994 cord_uid: p7d99tmt The present state of diagnostic and therapeutic developmental race for vaccines against the SARS CoV-2 (nCOVID-19) focuses on prevention and control of this global pandemic which also represents a critical challenge to the global health community. Although development of novel vaccines can prevent the SARS CoV-2 infections, it is still impeded by several other factors and therefore novel approaches towards treatment and management of this disease is the urgent need. Passive immunotherapy plays a vital role as a possible alternative to meet this challenge and among various antibody sources, chicken egg yolk antibodies (IgY) can be used as an alternative to mammalian antibodies which have been previously studied against SARS CoV outbreak in China. In this review, we discuss the strategies for the use of chicken egg yolk (IgY) antibodies in the development of rapid diagnosis and immunotherapy against SARS CoV-2. Also, IgY antibodies have previously been used against various respiratory bacterial and viral infections in humans and animals. Compared to mammalian antibodies (IgG), chicken egg yolk antibodies (IgY) have greater binding affinity to specific antigens, ease of extraction and lower production costs, hence possessing remarkable pathogen-neutralizing activity of pathogens in respiratory and lungs. We provide an overall importance for the use of monoclonal chicken egg yolk antibodies (IgY) using phage display method describing their potential passive immunotherapeutic application for the treatment and prevention of SARS CoV-2 infection which is simple, fast and safe way of approach for treating patients effectively. will be a good candidate for developing antiviral drugs, vaccines and that generating high specific antibodies to recognize this domain would be much more valuable. Some of the reported studies with SARS CoV shows that immunization of mice with recombinant spike protein (S) can protect them from infection effectively [7, 8] . Therefore, generating monoclonal antibodies that are specifically to recognize the spike protein (S) is the need of the hour. However, we have to overcome the difficulties in generating highly specific monoclonal antibodies from the traditional way of antibody generation [9] , phage display method of monoclonal antibody generation would be safe and effective procedure because of the in vitro process of antibody generation by cloning the specific repertoires and subsequent screening and isolation of monoclonal antibodies from the antibody libraries [10, 11] . Although there are many ways of recombinant antibody generation, the single-chain variable fragments (scFv) of the whole antibody will be an effective region that can be generated in phage display system [12] [13] [14] . Antibody production in chickens is the simplest, easier and efficient way of generating monoclonal antibodies using phage display library selection for scFv gene constructs with higher affinity against targetted pathogens [15, 16] . Also, it has been reported that monospecific scFv antibodies generated using phage display technology has high neutralizing effect against SARS CoV infection that have been generated from non-immunized individuals and convalescent SARS infected individuals [17, 18] . This review focuses to show that the monoclonal IgY scFv antibodies raised against SARS CoV-2 spike protein (S) isolated from chickens using phage display technology would be a potential model for large scale production of high-affinity antibodies effectively. The SARS-CoV-2 (nCOVID-19) are enveloped viruses with round or pleiomorphic structure of approximately 80 to 120 nm in diameter containing positive single-stranded RNA genome of 30kb size [19, 20] . The RNA genome is complexed with basic nucleocapsid protein (N) to form a helical viral protein and these are spike proteins (S) which are the Type-I glycoprotein that forms the peplomers on the virion surface giving it a crown-like structure [ Fig.1 ]. The membrane protein (M) which spans three time the viral membrane has a short Nterminal ectodomain and a cytoplasmic tail. The small membrane protein (E) is found to be highly hydrophobic in nature [21] and this spans twice the viral membrane has both N and C terminals on the interior part of the virion [22] . There are still many other minor proteins present in the viral structure yet undetected and the genomes of all the coronaviruses were found to have similar stuctural characteristics [23] . For all coronaviruses, the structural proteins are encoded in order of S-E-M-N within the one third of the genome and each group of coronaviruses encodes a group of unique small proteins while these are non-essential proteins and have been found to serve as accessory proteins to interact or interfere with the host innate immune responses which has not been demonstrated for any of these proteins [24, 25] . Untranslated regions of coronaviruses (UTRs) on both 5' and 3' ends of the genome were believed to interact with the host and control the RNA replication process and the viral transcription has been reviewed in recent studies [26] . Transmembrane spike (S) protein of the coronavirus mediates host cell entry. S protein is a glycoprotein that forms homotrimers [27] . Each monomer is about 180 kDa. Because it is surface-exposed on part of the virus and easily accessible for neutralizing antibodies, it becomes a potential drug target and interest of several structural studies. SARS-CoV-2 S protein is capable of triggering protease-independent and receptor-dependent syncytium formation; this enhances virus spreading through cell-cell fusion and the rapid progress of the diseases [28, 29] . The functional domains of S protein are distributed among the two subunits, the receptor-binding domain (RBD) is in the S1 subunit [ Fig.1 ]. SARS CoV and SARS CoV-2 interact directly with human angiotensin-converting enzyme 2 (hACE2) through domain B (S B ). The cryoelectron microscopy structures of the SARS-CoV-2 S ectodomain trimer reveal that it adopts multiple S B conformations as like SARS-CoV [30] [31] [32] . The S proteins of SARS CoV-2 share the amino acid similarity of about 76% and 97% with SARS CoV, and RaTG13 (bat coronavirus-BatCoV RaTG13) respectively. Interestingly, the RBD has only 74% and 90.1% similarity with SARS CoV, and RaTG13 respectively [33] . This partially explains the difference in the binding affinity of these viruses towards their respective host targets and the efficient transmission. In most of the coronavirus, these two subunits are non-covalently bound in the prefusion conformation [34] [35] [36] . Additionally, the S protein structure is covered with N-linked glycans, this perhaps helps to maintain its integrity and acts as a shield to escape the host immune system [37, 38] . The neutralizing antibodies have to slot in between the glycans to attach with the spike protein. S protein is the main target for neutralizing antibodies and vaccine design which plays a vital role in studying the viral entry, determination of virulence, understanding the range of hosts, a pseudotype system with S protein of SARS-CoV-2 [30, 40] . Though there is considerable homology between S protein of SARS CoV and SARS CoV-2, polyclonal rabbit anti-SARS S1 antibodies T62 did not completely neutralize the SARS-CoV-2 and there is less affinity of binding with SARS-CoV-2 S protein [40] . Previous studies postulated that major immuneepitopes for anti-SARS S1 antibody T62 may lie in the region of RBD. Moreover, the experiment with convalescent sera from SARS and COVID-19 patients has shown only moderate cross-neutralization and the sera from SARS-CoV infected individual targets S B site of the SARS-CoV-2 S protein [41] . Few studies had reported the lack of cross-reactivity among these S B -directed antibodies [42, 43] . Most of SARS-CoV neutralizing antibodies target the S B domain and several of them recognize the receptor binding domain regions and prevent receptor engagement [44] [45] [46] . This suggests that those previously recovered from SARS-CoV infection may not be fully protected against SARS-CoV-2 infection, and vice versa. The more proper understanding of the S protein and its accessible antigenic regions will help to develop more effective antibodies or drugs to fight against SARS-CoV-2 effectively. Antibodies are also called as immunoglobulins, which are associated with the humoral immune response [47] . Producing antibodies from mammals involves stress to animals, such as immunization, blood collection and sometimes sacrifice [48] . An alternative for the mammalian antibodies is the IgY antibody which is being purified from eggs of immunized birds (mostly hens and ducks). Looking closely, into the functions, IgY antibodies are similar to that of mammalian IgG's [49] and are transported from the blood serum to the yolk plasma [50] . Chicken egg yolk antibodies (IgY) from hyperimmunized eggs against tetanus toxin had the ability to neutralize the lethality in in vivo experiments [51] . These neutralizing antibodies from chickens were later termed as IgY in 1969 [52] . Chicken egg yolk antibodies (IgY) were considered to be the largest source of major nutrients and the chicken eggs also contains various other biological substances in it that forms the basic unit of life [53, 54] . In recent years, the use of 3R's (Reducing, Refining and Reusing) has been well accepted by industries producing antibodies and IgY clearly defines the use of 3R's, which has allowed the production of IgY antibodies for research, diagnostic and therapeutic purposes. IgY antibodies are highly effective in neutralizing the bacterial and viral diseases of respiratory system, causing no side effects [54] . The response of immunoglobulins in chickens to the highly conserved mammalian proteins is robust showing higher affinity, thereby potentially targeting broad spectrum of epitopes on protein immunogens [55] . Molecular weight of IgY is around 180kDa and is slightly greater than IgG (150kDa) as the IgY heavy chain has an additional constant domain and higher amounts of carbohydrates [56] . Hinge region is absent in the heavy chain of IgY. Sequence analysis of IgY and IgG showed that CH3 and CH4 domains of IgY are closely related to CH2 and CH3 domains of IgG [57] . Irrespective of IgY being a protein molecule, it shows resistant to heat at temperatures ranging from 30-70°C and is active at pH 3-11 [58] . The isoelectric point (pI) of IgY is between 5.4-7.6 and are stable for a period of 10 years at 4°C, at room temperature for 6 months and for 1 month at 37°C, without loss of any activity. Since antibodies from chickens are harvested from egg yolks, chickens show higher advantages to conventional mammalian species such as rabbits, goats and sheep. Chickens are able to produce 100-150 mg of antibodies per yolk, of which 5-10% is the specific antibody [59] [60] . A chicken can lay up to 300-325 eggs every year which yields 20-30gms of IgY production. The administration of preformed antibodies or immunoglobulins to treat various infectious diseases is known as passive immunization therapy [63] [64] [65] and transferring of such pathogen specific derived antibodies to non-immune subjects by oral, intravenous and systemic route of passive immunization. Owing to such immediate, short-term development of immunity, continuous and mass production of highly specific antibodies can be produced by hyperimmunization of chickens with target antigens will be the need of the hour [66] for large scale production of antibodies ensuring higher purity and constant supply of antibodies [67] . Intranasal route of passive immunotherapy proves to be highly promising and effective in treating many viral infections because it binds directly to the virus, acts rapidly to neutralize the virus and one such has also been reported with the use of IgY antibodies against SARS CoV outbreak in china [68] [69] [70] . In recent years the use of monoclonal chicken IgY antibodies derived from phage display technology has been widely studied and promising results of producing neutralizing antibodies has been observed by different research groups. It was in 1985 when George smith first used this technology, which used an expression vector, having a capability of presenting the foreign amino acid sequences, which could bind to the antibody [71] . This technology was considered as an alternative to the conventional production of monoclonal antibodies using hybridoma technology. The major advantage of using PDT is that the generation of scFv/ Fab fragments specific to a particular antigen can be performed within few weeks [72] . The immunoglobulin repertoire of chickens is ideally suited for phage display, as it is generated from a single set of V H and V L germ line sequence [73] . The phage display system is considered as a fast and valuable technique for monoclonal antibody production against broad viral infections [74] . In the conventional monoclonal antibody production through hybridoma technology, the lymphocytes are isolated, immortalized by hybridization with myeloma cells which paves a way for in vitro cloning in eukaryotic cell culture system. Whereas in the phage display technology, the prokaryotic system is used for cloning the cells. confirmed that the epitope (S protein) is a suitable candidate for development of vaccine and for rapid detection of viral infections [78] . It has also been stated that using the biotin-tagged phage conjugated with streptavidin coated quantum dot has the ability to detect as few as 10 cells/ml [78, 79] . IgY antibodies purified from ostrich eggs can aid in development of antibody vaccines for corona virus, SARS-CoV and MERS-CoV [80] . For selection of phage display systems, moreover E. coli filamentous bacteriophages, such as the M13 phages are commonly used [81] . Most commonly, for construction of library, the following steps are widely preferred, i. Preparation of primary library or amplification of the existing one ii. Exposing phage particles to target (cell surface proteins/vascular endothelium) iii. Removing non-specific binders (washing/perfusion) iv. Recovery of the target bound by elution or direct bacterial infection v. Amplification of recovered phages. vi. Repeating step (i) until highest binding population is reached, bio-panning is repeated. Currently, there are various ongoing clinical trials which involves different drugs leading to the discovery of potential vaccine or the potential drug to treat SARS CoV-2 pandemic which would then lead to the rapid development of vaccine and its application as a powerful means in preventing the global pandemic situation. Inspite of these, vaccine developments are little slower compared to the human transmission of SARS CoV-2 infection there is still an urgent need and necessity for vaccine development [82] . Also, it is clear that the epidemic situation became pandemic and it is appearing to be transformed likely to a flu-like seasonal infection from human to human transmission which is still rapidly co-existing with human hosts for long time. These scFv regions are cloned and expressed into vectors (E.coli) for generating antigenspecific IgY antibodies expressing the antibody library and it is constructed [83] [84] [85] which ensures that the antibody library constructs are not diversified during amplification [86, 87] . It has also been reported thar recent studies with production of IgY monoclonal antibodies designed based on ezymatic methods for assembling scFv IgY antibodies [88] . This method of chicken IgY monoclonal antibody production against SARS CoV-2 spike protein (S) would be more standardized, reproducible and suitable for large scale production of antigen specific antibodies (anti-SARS CoV-2 IgY antibodies) which inhibits the antigen (SARS CoV-2) to the binding receptor (ACE2) present on the human cell membrane and thereby leading to prevention of viral entry or replication in the host cell effectively [Fig:4 ]. Additionally this technology offers lesser methodological variablities when compared to that of bacterial diplay technology [89] and also ensures that the expressed scFv antibody targets are structurally and functionally correct with higher capability of target antigen binding for effective neutralization [90] . Currently, immune and naïve derived antibody libraries from avian sources using phage display method can be easily established and the distinctive immunological benefits of chicken antibodies enables development of highly specific unique antibodies creating an efficient immunotherapeutic and diagnostic tool that allows the capture of distinct conformational structural changes of immunoglobulin molecules pertaining to their protein structures. Development of chicken monoclonal IgY antibodies using phage display technology for its promising applications in diagnosis and therapeutic use widely to treat various pathogenic infections especially viral diseases like the current pandemic SARS CoV-2 infection. Still, there is need for numerous areas of research required for the development and use of high-affinity monoclonal IgY antibodies. Immunization of these developed antibodies can be performed effectively to reduce the immunogenecity of the developed antigen-specific monoclonal IgY antibodies against SARS CoV-2 as a parameter that should be considered in using these antibodies in use as immunodiagnostic and immunotherapeutic mode of treatments and humanization of monoclonal IgY antibodies has been reported to be successful tool as immunotherapeutic administration [91, 92] . Additionally, various studies has been reported that the use of chimeric scFv chicken IgY antibodies can be extended further to other mammalian species in veterinary applications and the more recent use of chicken IgY monoclonal antibodies seems to have more potential in immunotherapy [93, 94] . Hence, molecular characterization also allows researchers to determine and correlate target specific parameters of scFv IgY genes in relation to its properties like thermal stability, aggregation capacity, solubility, binding efficacy and its expression stability [95, 96] . The residual changes of scFv IgY antibodies facilitates the bioconjugation chemistries of chicken scFv IgY immunoglobulin when it reacts with certain chemicals like chelating agents and prodrugs used in certain immunotherapeutic treatments [97] . Therefore, these approaches and reported studies reinforces that the need of future research in contribution to better understanding and knowledge of chicken IgY monoclonal antibodies against specific antigens like SARS CoV-2 explained here can be developed further from the molecular level to the large scale production of antibodies with their effective applications thereof effectively. It has been proven that antibody receptors that are specifically engineered to a target antigen with combined specific sites were used in human therapy and reported to be effective with these single-chain antigen binding molecules [98] . Also, chicken immunoglobulin fragments like chFcR/L receptor molecules were identified to be the first member of this avian antibody family which plays a vital role in mammalian immune system that makes it a significant and important tool in immunoregulatory family and additionally exploring these specific mechanisms would be certainly contributing a new perspective on antibody small molecule receptor interactions [99] . Further analysis provides evidences that some of the major shifts in the mode of Fc, scFv receptor binding regions during immunoglobulin evolutions undergoes various structural changes which may lead to develop novel functions during the evolution of immunoglobulins in mammals [100] . The development of chicken IgY monoclonal antibodies using phage display method against various target pathogens have been reported to be effective in enriching the target specific scFv IgY antibodies from the phage displayed antibody libraries [100] . Also, it is noted that the feasiblity and effectiveness in generating highly specific scFv IgY monoclonal antibodies using phage display method in chickens is significantly potential and the ability in generating mass production of these highly specific monoclonal scFv IgY antibodies will facilitate the investigations of their ability to quantitative and qualitative response to the target pathogen contributing to be a valuable tool in immunotherapeuti applications [101] . Further to this, these IgY antibodies were even developed against snake venoms which has the potential to replace equine antibodies because they do not cause any adverse effects upon therapeutic administration [102] . Recently, it has also been reported that anti-ZIKV-E IgY antibodies has been a potential target for development of vaccine and immunodiagnostic assays which were derived from the antibody libraries and these scFv antibody fragments effectively played a vital role in inhibition and detection assays [103, 104] . To face the current global pandemic situation of SARS CoV-2, it is the need of the hour to have better diagnostic and therapeutic modes for overcoming this health problem. Hence, production of highly specific monoclonal antibodies using chicken egg yolk antibodies (IgY) by phage display method against SARS CoV-2 will be an effective platform which holds much effective clinical and scientific advantages [105] [106] [107] . The use of monoclonal IgY antibodies promises the need for effective and continuous research to improve further in various aspects and development of monoclonal IgY antibodies using phage display system will combine the benefits of both mammalian monoclonal antibodies (IgG) and avain antibodies (IgY). Also chicken monoclonal IgY antibodies proved to be more specific when compared to polyclonal antibodies in recognizing a single unique epitope. Thus, the identified epitope of SARS CoV-2 spike protein (S) will be an effective potential candidate for antibody based vaccine development as immunotherapeutic agent in preventing and treating the infection and thereby playing a vital role in both scientific and clinical applications. It is foreseen that chicken scFv IgY antibodies developed against SARS CoV-2 spike protein (S) using phage disply technology can be a potential model for effective mass production of high-affinity monoclonal IgY antibodies to treat this disease with standardized preparation for its effective use in long term. All authors contributed equally and have read and approved the complete manuscript. There are no funding support and no conflict of interest to report. 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Highlights: 1. Production of highly specific chicken egg yolk (IgY) monoclonal antibodies using phage display method against SARS CoV-2 will be an effective platform which holds much effective clinical and scientific advantages.2. This method holds higher specificity, consistency and reproducibility.3. Highly scalable manufacturing and lower cross-reactive due to the absence of invariable regions. Dr.Rajeswari Somasundaram, Department of Microbiology, PSG College of Arts & Science,