Your search keyword '"Nesmeyanova, Valentina S."' showing total 8 results

1. Phage Display Revealed the Complex Structure of the Epitope of the Monoclonal Antibody 10H10.

Author

Shanshin, Daniil V., Borisevich, Sophia S., Shaprova, Olga N., Nesmeyanova, Valentina S., Bondar, Alexander A., Porozov, Yuri B., Khamitov, Edward M., Kolosova, Evgeniia A., Shelemba, Arseniya A., Ushkalenko, Nikita D., Protopopova, Elena V., Sergeev, Artemiy A., Loktev, Valery B., and Shcherbakov, Dmitriy N.

Subjects

RECOMBINANT proteins, FLAVIVIRAL diseases, MOLECULAR dynamics, AMINO acid sequence, TICK-borne encephalitis, FLAVIVIRUSES

Abstract

The annual number of reported human cases of flavivirus infections continues to increase. Measures taken by local healthcare systems and international organizations are not fully successful. In this regard, new approaches to treatment and prevention of flavivirus infections are relevant. One promising approach is to use monoclonal antibody preparations. The mouse mAb 10H10 is capable of interacting with viruses belonging to the genus Orthoflavivirus which are pathogenic to humans. ELISA and molecular modeling data can indicate that mAb 10H10 recognizes the fusion loop region of E protein. The KD of interaction between the mAb 10H10 and recombinant analogs of the E protein of the tick-borne encephalitis (TBEV), Zika (ZIKV) and dengue (DENV) viruses range from 1.5 to 4 nM. The aim of this study was to map the epitope of this antibody using phage display technology. After three rounds of biopanning, 60 individual phage clones were chosen. The amino acid sequences of the selected peptides were conveniently divided into five groups. Based on the selected peptides, bacteriophages were obtained carrying peptides on the surfaces of the pIII and pVIII proteins, which were tested for binding to the antibody in ELISA. Thus, the epitope of the mAb 10H10 is the highly conserved region 98-DRGWGNXXGLFGK-110 of the flavivirus E protein. The structures of the complexes of the identified peptides with the antibody paratope are proposed using the molecular docking and dynamics methods. [ABSTRACT FROM AUTHOR]

Published

2024

2. SARS-CoV-2 RBD Conjugated to Polyglucin, Spermidine, and dsRNA Elicits a Strong Immune Response in Mice.

Author

Volosnikova, Ekaterina A., Merkuleva, Iuliia A., Esina, Tatiana I., Shcherbakov, Dmitry N., Borgoyakova, Mariya B., Isaeva, Anastasiya A., Nesmeyanova, Valentina S., Volkova, Natalia V., Belenkaya, Svetlana V., Zaykovskaya, Anna V., Pyankov, Oleg V., Starostina, Ekaterina V., Zadorozhny, Alexey M., Zaitsev, Boris N., Karpenko, Larisa I., Ilyichev, Alexander A., and Danilenko, Elena D.

Subjects

SARS-CoV-2, DOUBLE-stranded RNA, IMMUNE response

Abstract

Despite the rapid development and approval of several COVID vaccines based on the full-length spike protein, there is a need for safe, potent, and high-volume vaccines. Considering the predominance of the production of neutralizing antibodies targeting the receptor-binding domain (RBD) of S-protein after natural infection or vaccination, it makes sense to choose RBD as a vaccine immunogen. However, due to its small size, RBD exhibits relatively poor immunogenicity. Searching for novel adjuvants for RBD-based vaccine formulations is considered a good strategy for enhancing its immunogenicity. Herein, we assess the immunogenicity of severe acute respiratory syndrome coronavirus 2 RBD conjugated to a polyglucin:spermidine complex (PGS) and dsRNA (RBD-PGS + dsRNA) in a mouse model. BALB/c mice were immunized intramuscularly twice, with a 2-week interval, with 50 µg of RBD, RBD with Al(OH)3, or conjugated RBD. A comparative analysis of serum RBD-specific IgG and neutralizing antibody titers showed that PGS, PGS + dsRNA, and Al(OH)3 enhanced the specific humoral response in animals. There was no significant difference between the groups immunized with RBD-PGS + dsRNA and RBD with Al(OH)3. Additionally, the study of the T-cell response in animals showed that, unlike adjuvants, the RBD-PGS + dsRNA conjugate stimulates the production of specific CD4+ and CD8+ T cells in animals. [ABSTRACT FROM AUTHOR]

Published

2023

3. Natural IgG against S-Protein and RBD of SARS-CoV-2 Do Not Bind and Hydrolyze DNA and Are Not Autoimmune.

Author

Timofeeva, Anna M., Sedykh, Sergey E., Ermakov, Evgeny A., Matveev, Andrey L., Odegova, Eva I., Sedykh, Tatiana A., Shcherbakov, Dmitry N., Merkuleva, Iuliia A., Volosnikova, Ekaterina A., Nesmeyanova, Valentina S., Tikunova, Nina V., and Nevinsky, Georgy A.

Subjects

DNA antibodies, VITRONECTIN, COVID-19, SARS-CoV-2, AUTOIMMUNE diseases, DESMOGLEINS, VIRAL antibodies, AUTOANTIBODIES

Abstract

Since the onset of the COVID-19 pandemic, numerous publications have appeared describing autoimmune pathologies developing after a coronavirus infection, with several papers reporting autoantibody production during the acute period of the disease. Several viral diseases are known to trigger autoimmune processes, and the appearance of catalytic antibodies with DNase activity is one of the earliest markers of several autoimmune pathologies. Therefore, we analyzed whether IgG antibodies from blood plasma of SARS-CoV-2 patients after recovery could bind and hydrolyze DNA. We analyzed how vaccination of patients with adenovirus Sputnik V vaccine influences the production of abzymes with DNase activity. Four groups were selected for the analysis, each containing 25 patients according to their relative titers of antibodies to S-protein: with high and median titers, vaccinated with Sputnik V with high titers, and a control group of donors with negative titers. The relative titers of antibodies against DNA and the relative DNase activity of IgGs depended very much on the individual patient and the donor, and no significant correlation was found between the relative values of antibodies titers and their DNase activity. Our results indicate that COVID-19 disease and vaccination with adenoviral Sputnik V vaccine do not result in the development or enhancement of strong autoimmune reactions as in the typical autoimmune diseases associated with the production of anti-DNA and DNA hydrolyzing antibodies. [ABSTRACT FROM AUTHOR]

Published

2022

4. Antibodies to the Spike Protein Receptor-Binding Domain of SARS-CoV-2 at 4–13 Months after COVID-19.

Author

Kolosova, Evgeniia A., Shaprova, Olga N., Shanshin, Daniil V., Nesmeyanova, Valentina S., Merkuleva, Iuliia A., Belenkaya, Svetlana V., Isaeva, Anastasiya A., Nikitin, Artem O., Volosnikova, Ekaterina A., Nikulina, Yuliya A., Nikonorova, Marina A., Shcherbakov, Dmitry N., and Elchaninova, Svetlana A.

Subjects

PROTEIN domains, COVID-19, SARS-CoV-2, ENZYME-linked immunosorbent assay, ANTIBODY titer

Abstract

Identification of factors behind the level and duration of persistence of the SARS-CoV-2 antibodies in the blood is assumed to set the direction for studying humoral immunity mechanisms against COVID-19, optimizing the strategy for vaccine use, antibody-based drugs, and epidemiological control of COVID-19. Objective: This study aimed to study the relationship between clinical and demographic characteristics and the level of IgG antibodies to the RBD of SARS-CoV-2 spike protein after COVID-19 in the long term. Residents of the Altai Region of Western Siberia of Russia, Caucasians, aged from 27 to 93 years (median 53.0 years), who recovered from COVID-19 between May 2020 and February 2021 (n = 44) took part in this prospective observational study. The titer of IgG antibodies to the RBD of SARS-CoV-2 spike protein was measured repeatedly in the blood at 4–13 months from the beginning of the clinical manifestation of COVID-19 via the method of enzyme-linked immunosorbent assay. The antibody titer positively correlated with age (p = 0.013) and COVID-19 pneumonia (p = 0.002) at 20–40 and 20–24 weeks from the onset of COVID-19 symptoms, respectively. Age was positively associated with antibody titer regardless of history of COVID-19 pneumonia (beta regression coefficient p = 0.009). The antibody titer decreased in 15 (34.1%) patients, increased in 10 (22.7%) patients, and did not change in 19 (43.2%) patients from the baseline to 48–49 weeks from the onset of COVID-19 symptoms, with seropositivity persisting in all patients. Age and COVID-19 pneumonia are possibly associated with higher IgG antibodies to the spike protein RBD of SARS-CoV-2 following COVID-19 in the long term. Divergent trends of anti-RBD IgG levels in adults illustrate inter-individual differences at 4–13 months from the onset of COVID-19 symptoms. [ABSTRACT FROM AUTHOR]

Published

2022

5. Are Hamsters a Suitable Model for Evaluating the Immunogenicity of RBD-Based Anti-COVID-19 Subunit Vaccines?

Author

Merkuleva, Iuliia A., Shcherbakov, Dmitry N., Borgoyakova, Mariya B., Isaeva, Anastasiya A., Nesmeyanova, Valentina S., Volkova, Natalia V., Aripov, Vazirbek S., Shanshin, Daniil V., Karpenko, Larisa I., Belenkaya, Svetlana V., Kazachinskaia, Elena I., Volosnikova, Ekaterina A., Esina, Tatiana I., Sergeev, Alexandr A., Titova, Kseniia A., Konyakhina, Yulia V., Zaykovskaya, Anna V., Pyankov, Oleg V., Kolosova, Evgeniia A., and Viktorina, Olesya E.

Subjects

HAMSTERS, IMMUNE response, VACCINE immunogenicity, HUMORAL immunity, VACCINE effectiveness, LABORATORY animals

Abstract

Currently, SARS-CoV-2 spike receptor-binding-domain (RBD)-based vaccines are considered one of the most effective weapons against COVID-19. During the first step of assessing vaccine immunogenicity, a mouse model is often used. In this paper, we tested the use of five experimental animals (mice, hamsters, rabbits, ferrets, and chickens) for RBD immunogenicity assessments. The humoral immune response was evaluated by ELISA and virus-neutralization assays. The data obtained show hamsters to be the least suitable candidates for RBD immunogenicity testing and, hence, assessing the protective efficacy of RBD-based vaccines. [ABSTRACT FROM AUTHOR]

Published

2022

6. Self-Assembled Particles Combining SARS-CoV-2 RBD Protein and RBD DNA Vaccine Induce Synergistic Enhancement of the Humoral Response in Mice.

Author

Borgoyakova, Mariya B., Karpenko, Larisa I., Rudometov, Andrey P., Volosnikova, Ekaterina A., Merkuleva, Iuliia A., Starostina, Ekaterina V., Zadorozhny, Alexey M., Isaeva, Anastasiya A., Nesmeyanova, Valentina S., Shanshin, Daniil V., Baranov, Konstantin O., Volkova, Natalya V., Zaitsev, Boris N., Orlova, Lyubov A., Zaykovskaya, Anna V., Pyankov, Oleg V., Danilenko, Elena D., Bazhan, Sergei I., Shcherbakov, Dmitry N., and Taranin, Alexander V.

Subjects

DNA vaccines, HUMORAL immunity, COMBINED vaccines, SARS-CoV-2, COVID-19 vaccines, IMMUNOGLOBULINS

Abstract

Despite the fact that a range of vaccines against COVID-19 have already been created and are used for mass vaccination, the development of effective, safe, technological, and affordable vaccines continues. We have designed a vaccine that combines the recombinant protein and DNA vaccine approaches in a self-assembled particle. The receptor-binding domain (RBD) of the spike protein of SARS-CoV-2 was conjugated to polyglucin:spermidine and mixed with DNA vaccine (pVAXrbd), which led to the formation of particles of combined coronavirus vaccine (CCV-RBD) that contain the DNA vaccine inside and RBD protein on the surface. CCV-RBD particles were characterized with gel filtration, electron microscopy, and biolayer interferometry. To investigate the immunogenicity of the combined vaccine and its components, mice were immunized with the DNA vaccine pVAXrbd or RBD protein as well as CCV-RBD particles. The highest antigen-specific IgG and neutralizing activity were induced by CCV-RBD, and the level of antibodies induced by DNA or RBD alone was significantly lower. The cellular immune response was detected only in the case of DNA or CCV-RBD vaccination. These results demonstrate that a combination of DNA vaccine and RBD protein in one construct synergistically increases the humoral response to RBD protein in mice. [ABSTRACT FROM AUTHOR]

Published

2022

7. Comparative Immunogenicity of the Recombinant Receptor-Binding Domain of Protein S SARS-CoV-2 Obtained in Prokaryotic and Mammalian Expression Systems.

Author

Merkuleva, Iuliia A., Shcherbakov, Dmitry N., Borgoyakova, Mariya B., Shanshin, Daniil V., Rudometov, Andrey P., Karpenko, Larisa I., Belenkaya, Svetlana V., Isaeva, Anastasiya A., Nesmeyanova, Valentina S., Kazachinskaia, Elena I., Volosnikova, Ekaterina A., Esina, Tatiana I., Zaykovskaya, Anna V., Pyankov, Oleg V., Borisevich, Sophia S., Shelemba, Arseniya A., Chikaev, Anton N., and Ilyichev, Alexander A.

Subjects

PROTEIN S, PROTEIN domains, IMMUNE response, SARS-CoV-2, HUMORAL immunity, TITERS

Abstract

The receptor-binding domain (RBD) of the protein S SARS-CoV-2 is considered to be one of the appealing targets for developing a vaccine against COVID-19. The choice of an expression system is essential when developing subunit vaccines, as it ensures the effective synthesis of the correctly folded target protein, and maintains its antigenic and immunogenic properties. Here, we describe the production of a recombinant RBD protein using prokaryotic (pRBD) and mammalian (mRBD) expression systems, and compare the immunogenicity of prokaryotic and mammalian-expressed RBD using a BALB/c mice model. An analysis of the sera from mice immunized with both variants of the protein revealed that the mRBD expressed in CHO cells provides a significantly stronger humoral immune response compared with the RBD expressed in E.coli cells. A specific antibody titer of sera from mice immunized with mRBD was ten-fold higher than the sera from the mice that received pRBD in ELISA, and about 100-fold higher in a neutralization test. The data obtained suggests that mRBD is capable of inducing neutralizing antibodies against SARS-CoV-2. [ABSTRACT FROM AUTHOR]

Published

2022

8. Structure- and Interaction-Based Design of Anti-SARS-CoV-2 Aptamers.

Author

Mironov V, Shchugoreva IA, Artyushenko PV, Morozov D, Borbone N, Oliviero G, Zamay TN, Moryachkov RV, Kolovskaya OS, Lukyanenko KA, Song Y, Merkuleva IA, Zabluda VN, Peters G, Koroleva LS, Veprintsev DV, Glazyrin YE, Volosnikova EA, Belenkaya SV, Esina TI, Isaeva AA, Nesmeyanova VS, Shanshin DV, Berlina AN, Komova NS, Svetlichnyi VA, Silnikov VN, Shcherbakov DN, Zamay GS, Zamay SS, Smolyarova T, Tikhonova EP, Chen KH, Jeng US, Condorelli G, de Franciscis V, Groenhof G, Yang C, Moskovsky AA, Fedorov DG, Tomilin FN, Tan W, Alexeev Y, Berezovski MV, and Kichkailo AS

Subjects

Humans, Molecular Docking Simulation, Molecular Dynamics Simulation, SARS-CoV-2, SELEX Aptamer Technique, Spike Glycoprotein, Coronavirus, Aptamers, Nucleotide chemistry, COVID-19

Abstract

Aptamer selection against novel infections is a complicated and time-consuming approach. Synergy can be achieved by using computational methods together with experimental procedures. This study aims to develop a reliable methodology for a rational aptamer in silico et vitro design. The new approach combines multiple steps: (1) Molecular design, based on screening in a DNA aptamer library and directed mutagenesis to fit the protein tertiary structure; (2) 3D molecular modeling of the target; (3) Molecular docking of an aptamer with the protein; (4) Molecular dynamics (MD) simulations of the complexes; (5) Quantum-mechanical (QM) evaluation of the interactions between aptamer and target with further analysis; (6) Experimental verification at each cycle for structure and binding affinity by using small-angle X-ray scattering, cytometry, and fluorescence polarization. By using a new iterative design procedure, structure- and interaction-based drug design (SIBDD), a highly specific aptamer to the receptor-binding domain of the SARS-CoV-2 spike protein, was developed and validated. The SIBDD approach enhances speed of the high-affinity aptamers development from scratch, using a target protein structure. The method could be used to improve existing aptamers for stronger binding. This approach brings to an advanced level the development of novel affinity probes, functional nucleic acids. It offers a blueprint for the straightforward design of targeting molecules for new pathogen agents and emerging variants., (© 2022 Wiley-VCH GmbH.)

Published

2022