Your search keyword '"DiNunno, Nadia"' showing total 4 results

1. Infectious parvovirus B19 circulates in the blood coated with active host protease inhibitors.

Author

Lee, Hyunwook, Assaraf, Ruben, Subramanian, Suriyasri, Goetschius, Dan, Bieri, Jan, DiNunno, Nadia M., Leisi, Remo, Bator, Carol M., Hafenstein, Susan L., and Ros, Carlos

Abstract

The lack of a permissive cell culture system has limited high-resolution structures of parvovirus B19 (B19V) to virus-like particles (VLPs). In this study, we present the atomic resolution structure (2.2 Å) of authentic B19V purified from a patient blood sample. There are significant differences compared to non-infectious VLPs. Most strikingly, two host protease inhibitors (PIs), inter-alpha-trypsin inhibitor heavy chain 4 (ITIH4) and serpinA3, were identified in complex with the capsids in all patient samples tested. The ITIH4 binds specifically to the icosahedral fivefold axis and serpinA3 occupies the twofold axis. The protein-coated virions remain infectious, and the capsid-associated PIs retain activity; however, upon virion interaction with target cells, the PIs dissociate from the capsid prior to viral entry. Our finding of an infectious virion shielded by bound host serum proteins suggests an evolutionarily favored phenomenon to evade immune surveillance and escape host protease activity.This study presents the first high-resolution structure of infectious parvovirus B19, purified from a patient. Two acute phase reactants, serpinA3, and ITIH4, bind to the capsid, suggesting B19V utilizes host proteins during viremia for survival and function. [ABSTRACT FROM AUTHOR]

Published

2024

2. Infectious parvovirus B19 circulates in the blood coated with active host protease inhibitors.

Author

Lee, Hyunwook, Assaraf, Ruben, Subramanian, Suriyasri, Goetschius, Dan, Bieri, Jan, DiNunno, Nadia M., Leisi, Remo, Bator, Carol M., Hafenstein, Susan L., and Ros, Carlos

Abstract

The lack of a permissive cell culture system has limited high-resolution structures of parvovirus B19 (B19V) to virus-like particles (VLPs). In this study, we present the atomic resolution structure (2.2 Å) of authentic B19V purified from a patient blood sample. There are significant differences compared to non-infectious VLPs. Most strikingly, two host protease inhibitors (PIs), inter-alpha-trypsin inhibitor heavy chain 4 (ITIH4) and serpinA3, were identified in complex with the capsids in all patient samples tested. The ITIH4 binds specifically to the icosahedral fivefold axis and serpinA3 occupies the twofold axis. The protein-coated virions remain infectious, and the capsid-associated PIs retain activity; however, upon virion interaction with target cells, the PIs dissociate from the capsid prior to viral entry. Our finding of an infectious virion shielded by bound host serum proteins suggests an evolutionarily favored phenomenon to evade immune surveillance and escape host protease activity.This study presents the first high-resolution structure of infectious parvovirus B19, purified from a patient. Two acute phase reactants, serpinA3, and ITIH4, bind to the capsid, suggesting B19V utilizes host proteins during viremia for survival and function. [ABSTRACT FROM AUTHOR]

Published

2024

3. A human monoclonal antibody binds within the poliovirus receptor-binding site to neutralize all three serotypes.

Author

Charnesky, Andrew J., Faust, Julia E., Lee, Hyunwook, Puligedda, Rama Devudu, Goetschius, Daniel J., DiNunno, Nadia M., Thapa, Vaskar, Bator, Carol M., Cho, Sung Hyun, Wahid, Rahnuma, Mahmood, Kutub, Dessain, Scott, Chumakov, Konstantin M., Rosenfeld, Amy, and Hafenstein, Susan L.

Subjects

MONOCLONAL antibodies, POLIOVIRUS, SEROTYPES, BINDING sites, CAPSIDS

Abstract

Global eradication of poliovirus remains elusive, and it is critical to develop next generation vaccines and antivirals. In support of this goal, we map the epitope of human monoclonal antibody 9H2 which is able to neutralize the three serotypes of poliovirus. Using cryo-EM we solve the near-atomic structures of 9H2 fragments (Fab) bound to capsids of poliovirus serotypes 1, 2, and 3. The Fab-virus complexes show that Fab interacts with the same binding mode for each serotype and at the same angle of interaction relative to the capsid surface. For each of the Fab-virus complexes, we find that the binding site overlaps with the poliovirus receptor (PVR) binding site and maps across and into a depression in the capsid called the canyon. No conformational changes to the capsid are induced by Fab binding for any complex. Competition binding experiments between 9H2 and PVR reveal that 9H2 impedes receptor binding. Thus, 9H2 outcompetes the receptor to neutralize poliovirus. The ability to neutralize all three serotypes, coupled with the critical importance of the conserved receptor binding site make 9H2 an attractive antiviral candidate for future development. Cross-neutralizing activity of monoclonal antibodies against poliovirus serotypes is less commonly reported. In this study, the authors use high-resolution cryo-EM to reveal that a cross-neutralizing human antibody neutralizes all three poliovirus serotypes by interacting with the receptor-binding region, called the canyon. [ABSTRACT FROM AUTHOR]

Published

2023

4. Identification of a pocket factor that is critical to Zika virus assembly.

Author

DiNunno, Nadia M., Goetschius, Daniel J., Narayanan, Anoop, Majowicz, Sydney A., Moustafa, Ibrahim, Bator, Carol M., Hafenstein, Susan L., and Jose, Joyce

Subjects

ZIKA virus, MOIETIES (Chemistry), HYDROPHOBIC interactions, ATOMIC structure, ANTIVIRAL agents, BILAYER lipid membranes, MEMBRANE lipids

Abstract

Zika virus (ZIKV) is an emerging mosquito borne flavivirus and a major public health concern causing severe disease. Due to the presence of a lipid membrane and structural heterogeneity, attaining an atomic resolution structure is challenging, but important to understand virus assembly and life cycle mechanisms that offer distinct targets for therapeutic intervention. We here use subvolume refinement to achieve a 3.4 Å resolution structure and identify two distinct lipid moieties. The first arises from the inner leaflet and is coordinated by hydrophobic residues of the M and E transmembrane helices that form a binding pocket not previously characterized. The second lipid arises from the outer leaflet coordinate between two E protein helices. Structure-based mutagenesis identifies critical hydrophobic interactions and their effect on the virus life cycle. Results show that lipids play an essential role in the ZIKV assembly pathway revealing a potential target of lipid based antiviral drug development. Here, the authors provide a 3.4 Å resolution structure of mature Zika virus (ZIKV) and identify two lipid moieties, coordinated by hydrophobic residues of the M and E transmembrane helices and between two helices of E protein, that play an essential role in the ZIKV assembly pathway. [ABSTRACT FROM AUTHOR]

Published

2020