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Ефремов Роман Гербертович

Московский институт электроники и математики им. А.Н. Тихонова

Профиль на hse.ru ↗ тел.: +7 (495) 916-88-76 | 15129 | +7 (903) 743-16-56
Публикаций
127
Языков
2
Наград
5
Конференций
3
Профиль Публикации (127) Курсы (4)

Профессиональные интересы

Вычислительная биологиякомпьютерная биологиямолекулярное моделированиеструктура и динамика биомолекулбиофизика

Должности

  • ПрофессорМосковский институт электроники и математики им. А.Н. Тихонова, Департамент прикладной математики

Био

  • · Начал работать в НИУ ВШЭ в 2013 году.
  • · Научно-педагогический стаж: 42 года.

Образование

  • 2007 · Ученое звание: Профессор
  • 2000 · Доктор физико-математических наук
  • 1986 · Кандидат физико-математических наук
  • 1983 · Специалитет: Московский инженерно-физический институт, специальность «Дозиметрия и защита», квалификация «Инженер-физик»

Награды и поощрения

  • · Участие в научных советах и обществах: член Ученого Совета ИБХ РАН; член трех специализированных диссертационных советов (ИБХ РАН, МГУ, ГУ НИИ БМХ РАМН); член Американского химического общества; член Биофизического общества (США).
  • · Надбавка за публикацию в журнале из Списка А (и приравненном к нему научном издании) (2025–2026, 2024–2025, 2023–2024)
  • · Надбавка за публикацию в международном рецензируемом научном издании (2022–2023, 2021–2022, 2019–2021)
  • · Надбавка за статью в зарубежном рецензируемом журнале (2014–2016)
  • · Надбавка за статью в зарубежном рецензируемом научном издании (2016–2018)

Гранты и проекты

  • 2016 · Грант Российского научного фонда «Компьютерный анализ структурно-функциональных аспектов олигомеризации трансмембранных доменов рецепторов сигнальных систем клетки», 2014-2016 гг., руководитель.
  • 2016 · Грант Российского научного фонда «Молекулярные технологии управления нейросигнализацией», 2014-2016 гг., отв. соисполнитель.
  • 2017 · Грант Программы Президиума РАН «Молекулярная и клеточная биология», тема: «Молекулярное моделирование пептидов и белков в мембранах как фундаментальная основа для рационального конструирования новых биологически активных соединений», 2013-2017 гг., руководитель.
  • 2014 · Грант Программы Президиума РАН № 27 «Основы фундаментальных исследований нанотехнологий и наноматериалов», тема: «Новые вычислительные технологии мультимасштабного моделирования мезоскопических биомембранных систем: от понимания фундаментальных принципов структурно-динамического поведения – к созданию наноструктур для биомедицинских приложений», 2012-2014 гг., руководитель.
  • 2015 · Грант РФФИ «Коллективные молекулярные движения, кластеры и флуктуации в гидратированных липидных бислоях и их роль в структурно-динамическом поведении клеточных мембран», 2013-2015 гг., руководитель.
  • 2018 · Грант РФФИ «Клеточные мембраны как стохастические динамические системы: от атомистического моделирования – к рациональному конструированию новых мембранных материалов», 2016-2018 гг., руководитель.

Конференции (3)

Показать все
  • · 2016: Актуальные вопросы биологической физики и химии БФФХ-2016 (Севастополь). Доклад: Оценка влияния среды на димеризацию трансмембранных доменов гликофорина А в компьютерном эксперименте
  • · 2016: Khujand Symposium on Computational Materials and Biological Sciences 2016 (Худжанд). Доклад: Helix-helix interactions in membranes: focus on lipids
  • · 2014: Dushanbe Symposium on Computational Materials and Biological Sciences DSCMBS-2014 (Душанбе). Доклад: The adaptable lipid matrix promotes transmembrane helices association in membranes

Идентификаторы исследователя

Публикации (127)

Impact of external amino acids on fluorescent protein chromophore biosynthesis revealed by molecular dynamics and mutagenesis studies

2020 · ARTICLE · en

The precise positioning of catalytic amino acids against the substrate in an enzyme active site is a crucial factor in biocatalysis. Biosynthesis of the chromophores of fluorescent proteins (FPs) is an autocatalytic process that must conform to these requirements. Here, we show that, in addition to the internal amino acid residues in the proximity of the chromophore, chromophore biosynthesis is influenced by the remote amino acids exposed on the outer surface of the β-barrel structure of the FP. It has been shown earlier that chromophore biosynthesis of the red FP from Zoanthus sp. (zoan2RFP) proceeds via an immature green state. At the same time, the green state is the final stage of chromophore biosynthesis of green FP (zoanGFP), which is highly homologous to zoan2RFP. It was also shown that a single N66D substitution in the chromophore-forming sequence of zoanGFP might trigger the synthesis of the red chromophore. However, in this case, the synthesis of the red chromophore is incomplete and occurs only at elevated temperatures. Here, we tried to uncover additional structural determinants that govern the biosynthesis of the red chromophore. A comparison of zoanGFP and zoan2RFP revealed intrabarrel amino acid differences at five positions. Exhaustive substitutions of these five positions in zoanGFP-N66D gave rise to zoanGFPmut with the same intrabarrel amino acid composition as zoan2RFP. zoanGFPmut showed only partial green-to-red chromophore transformation at elevated temperatures. To elucidate the extra factors that can affect red chromophore biosynthesis, we performed comparative molecular dynamics simulations of zoan2RFP and zoanGFPmut. The simulations revealed several external amino acids that might influence the arrangement and flexibility of the chromophore-surrounding amino acid residues in these proteins. Mutagenesis experiments confirmed the crucial role of these residues in red chromophore biosynthesis. The obtained zoanGFPmut2 exhibited complete green-to-red transformation, suggesting that the mutated amino acids exposed on the surface of the β-barrel contribute to red chromophore biosynthesis.

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Antibacterial activity of cardiotoxin-like basic polypeptide from cobra venom

2020 · ARTICLE · en

Antibacterial activity of the three-finger toxins from cobra venom, including cytotoxin 3 from N. kaouthia, cardiotoxin-like basic polypeptide A5 from N. naja (CLBP), and alpha-neurotoxin from N. oxiana venom, was investigated. All toxins failed to influence Gram-negative bacteria. The most pronounced activity against Bacillus subtilis was demonstrated by CLBP. The latter is ascribed to the presence of additional Lys-residues within the membrane-binding motif of this toxin.

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Tuning Scorpion Toxin Selectivity: Switching From KV1.1 to KV1.3

2020 · ARTICLE · en

Voltage-gated potassium channels (KVs) perform vital physiological functions and are targets in different disorders ranging from ataxia and arrhythmia to autoimmune diseases. An important issue is the search for and production of selective ligands of these channels. Peptide toxins found in scorpion venom named KTx excel in both potency and selectivity with respect to some potassium channel isoforms, which may present only minute differences in their structure. Despite several decades of research the molecular determinants of KTx selectivity are still poorly understood. Here we analyze MeKTx13-3 (Kalium ID: α-KTx 3.19) from the lesser Asian scorpion Mesobuthus eupeus, a high-affinity KV1.1 blocker (IC50 ~2 nM); it also affects KV1.2 (IC50 ~100 nM), 1.3 (~10 nM) and 1.6 (~60 nM). By constructing computer models of its complex with KV1.1–1.3 channels we identify specific contacts between the toxin and the three isoforms. We then perform mutagenesis to disturb the identified contacts with KV1.1 and 1.2 and produce recombinant MeKTx13-3_AAAR, which differs by four amino acid residues from the parent toxin. As predicted by the modeling, this derivative shows decreased activity on KV1.1 (IC50 ~550 nM) and 1.2 (~200 nM). It also has diminished activity on KV1.6 (~1500 nM) but preserves KV1.3 affinity as measured using the voltage-clamp technique on mammalian channels expressed in Xenopus oocytes. In effect, we convert a selective KV1.1 ligand into a new specific KV1.3 ligand. MeKTx13-3 and its derivatives are attractive tools to study the structure-function relationship in potassium channel blockers.

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Sevanol and Its Analogues: Chemical Synthesis, Biological Effects and Molecular Docking

2020 · ARTICLE · en

Among acid-sensing ion channels (ASICs), ASIC1a and ASIC3 subunits are the most widespread and prevalent in physiological and pathophysiological conditions. They participate in synaptic plasticity, learning and memory, as well as the perception of inflammatory and neurological pain, making these channels attractive pharmacological targets. Sevanol, a natural lignan isolated from Thymus armeniacus, inhibits the activity of ASIC1a and ASIC3 isoforms, and has a significant analgesic and anti-inflammatory effect. In this work, we described the efficient chemical synthesis scheme of sevanol and its analogues, which allows us to analyze the structure–activity relationships of the different parts of this molecule. We found that the inhibitory activity of sevanol and its analogues on ASIC1a and ASIC3 channels depends on the number and availability of the carboxyl groups of the molecule. At the structural level, we predicted the presence of a sevanol binding site based on the presence of molecular docking in the central vestibule of the ASIC1a channel. We predicted that this site could also be occupied in part by the FRRF-amide peptide, and the competition assay of sevanol with this peptide confirmed this prediction. The intravenous (i.v.), intranasal (i.n.) and, especially, oral (p.o.) administration of synthetic sevanol in animal models produced significant analgesic and anti-inflammatory effects. Both non-invasive methods of sevanol administration (i.n. and p.o.) showed greater efficacy than the invasive (i.v.) method, thus opening new horizons for medicinal uses of sevanol.

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Dimeric states of transmembrane domains of insulin and IGF-1R receptors: Structures and possible role in activation

2020 · ARTICLE · en

Despite the biological significance of insulin signaling, the molecular mechanisms of activation of the insulin receptor (IR) and other proteins from its family remain elusive. Current hypothesis on signal transduction suggests ligand-triggered structural changes in the extracellular domain followed by transmembrane (TM) domains closure and dimerization leading to trans-autophosphorylation and kinase activity in intracellular segments of the receptor. Using NMR spectroscopy, we detected dimerization of isolated TM segments of IR in DPC micelles and observed multiple signals of NH groups of protein backbone possibly corresponding to several dimer conformations. Taking available experimental data as constraints, several atomistic models of dimeric TM domains of IR and insulin-like growth factor 1 (IGF-1R) receptors were elaborated. Molecular dynamics simulations of IR ectodomain revealed noticeable collective movements potentially responsible for closure of the C-termini of FnIII-3 domains and spatial approaching of TM helices upon insulin-induced receptor activation. In addition, we demonstrated that the intracellular part of the receptor does not impose restrictions on the positioning of TM helices in the membrane. Finally, we used two independent structure prediction methods to generate a series of dimer conformations followed by their cluster analysis and dimerization free energy estimation to select the best dimer models. Biological relevance of the later was further tested via comparison of the hydrophobic organization of TM helices for both wild-type receptors and their mutants. Based on these data, the ability of several segments from other proteins to functionally replace IR and/or IGF-1R TM domains was explained.

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Transmembrane peptides as inhibitors of protein-protein interactions: an efficient strategy to target cancer cells?

2020 · ARTICLE · en

Cellular functions are regulated by extracellular signals such as hormones, neurotransmitters, matrix ligands, and other chemical or physical stimuli. Ligand binding on its transmembrane receptor induced cell signaling and the recruitment of several interacting partners to the plasma membrane. Nowadays, it is well-established that the transmembrane domain is not only an anchor of these receptors to the membrane, but it also plays a key role in receptor dimerization and activation. Indeed, interactions between transmembrane helices are associated with specific biological activity of the proteins as cell migration, proliferation, or differentiation. Overexpression or constitutive dimerization (due notably to mutations) of these transmembrane receptors are involved in several physiopathological contexts as cancers. The transmembrane domain of tyrosine kinase receptors as ErbB family proteins (implicated in several cancers as HER2 in breast cancer) or other receptors as Neuropilins has been described these last years as a target to inhibit their dimerization/activation using several strategies. In this review, we will focus on the strategy which consists in using peptides to disturb in a specific manner the interactions between transmembrane domains and the signaling pathways (induced by ligand binding) of these receptors involved in cancer. This approach can be extended to inhibit other transmembrane protein dimerization as neuraminidase-1 (the catalytic subunit of elastin receptor complex), Discoidin Domain Receptor 1 (a tyrosine kinase receptor activated by type I collagen) or G-protein coupled receptors (GPCRs) which are involved in cancer processes.

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Transmembrane peptides as a new strategy to inhibit neuraminidase-1 activation

2020 · ARTICLE · en

Сиалидазы или нейраминидазы вовлечены в развитие ряда патологических состояний у человека: нейродегенративных, сердечно-сосудистых и инфекционных заболеваний. Накопленные данные показывают, что ингибирование нейраминидаз, таких как сиалидаза NEU1, может представлять фармакологический интерес, и специфичные ингибиторы NEU1 также будут полезны для понимания биологических функций этой сиалидазы. В настоящей работе мы создали интерферирующие пептиды, нацеленный на димеризацию трансмембранного домена, ранее обнаруженную для данного белка, и таким образом модулирующий сиалидазную активность. Рассмотрели две стратегии доставки интерферирующего пептид в клетки: добавление TAT-последовательности, либо встраивание в детергентные мицеллы. Вместе с этим, данные молекулярного моделирования и спектроскопии ЯМР в мембраноподобном окружении показали, что предлагаемый интерферирующий пептид способен взаимодействовать с трансмембранным сегментом NEU1 и таким образом нарушать димеризацию, приводя к значительному снижению сиалидазной активности в плазматической мембране. В заключение, мы предлагаем новые селективные ингибиторы человеческой NEU1, которые представляют особый интерес при изучении функции этой сиалидазы.

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Atomistic mechanism of the constitutive activation of PDGFRA via its transmembrane domain

2019 · ARTICLE · en

Single-point mutations in the transmembrane (TM) region of receptor tyrosine kinases (RTKs) can lead to abnormal ligand-independent activation. We use a combination of computational modeling, NMR spectroscopy and cell experiments to analyze in detail the mechanism of how TM domains contribute to the activation of wild-type (WT) PDGFRA and its oncogenic V536E mutant. Using a computational framework, we scan all positions in PDGFRA TM helix for identification of potential functional mutations for the WT and the mutant and reveal the relationship between the receptor activity and TM dimerization via different interfaces. This strategy also allows us design a novel activating mutation in the WT (I537D) and a compensatory mutation in the V536E background eliminating its constitutive activity (S541G). We show both computationally and experimentally that single-point mutations in the TM region reshape the TM dimer ensemble and delineate the structural and dynamic determinants of spontaneous activation of PDGFRA via its TM domain. Our atomistic picture of the coupling between TM dimerization and PDGFRA activation corroborates the data obtained for other RTKs and provides a foundation for developing novel modulators of the pathological activity of PDGFRA.

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Specific refolding pathway of viscumin A chain in membrane-like medium reveals a possible mechanism of toxin entry into cell.

2019 · ARTICLE · en

How is a water-soluble globular protein able to spontaneously cross a cellular membrane? It is commonly accepted that it undergoes significant structural rearrangements on the lipid-water interface, thus acquiring membrane binding and penetration ability. In this study molecular dynamics (MD) simulations have been used to explore large-scale conformational changes of the globular viscumin A chain in a complex environment – comprising urea and chloroform/methanol (CHCl3/MeOH) mixture. Being well-packed in aqueous solution, viscumin A undergoes global structural rearrangements in both organic media. In urea, the protein is “swelling” and gradually loses its long-distance contacts, thus resembling the “molten globule” state. In CHCl3/MeOH, viscumin A is in effect turned “inside out”. This is accompanied with strengthening of the secondary structure and surface exposure of hydrophobic epitopes originally buried inside the globule. Resulting solvent-adapted models were further subjected to Monte Carlo simulations with an implicit hydrophobic slab membrane. In contrast to only a few point surface contacts in water and two short regions with weak protein-lipid interactions in urea, MD-derived structures in CHCl3/MeOH reveal multiple determinants of membrane interaction. Consequently it is now possible to propose a specific pathway for the structural adaptation of viscumin A with respect to the cell membrane – a probable first step of its translocation into cytoplasmic targets.

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Kalium 2.0, a comprehensive database of polypeptide ligands of potassium channels

2019 · ARTICLE · en

Potassium channels are the most diverse group of ion channels in humans. They take vital parts in numerous physiological processes and their malfunction gives rise to a range of pathologies. In addition to small molecules, there is a wide selection of several hundred polypeptide ligands binding to potassium channels, the majority of which have been isolated from animal venoms. Until recently, only scorpion toxins received focused attention being systematically assembled in the manually curated Kalium database, but there is a diversity of well-characterized potassium channel ligands originating from other sources. To address this issue, here we present the updated and improved Kalium 2.0 that covers virtually all known polypeptide ligands of potassium channels and reviews all available pharmacological data. In addition to an expansion, we have introduced several new features to the database including posttranslational modification annotation, indication of ligand mode of action, BLAST search, and possibility of data export.

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Курсы (4)