Your search keyword '"Sandoval-Jaime C"' showing total 22 results

1. Interpolation of monthly precipitation amounts in mountainous catchments with sparse precipitation networks

Author

Jacquin, Alexandra P, primary and Soto-Sandoval, Jaime C, additional

Published

2013

2. Genetic characterization of a reptilian calicivirus (Cro1)

Author

Sandoval-Jaime Carlos, Parra Gabriel I, Smith Alvin W, Green Kim Y, and Sosnovtsev Stanislav V

Subjects

Reptile calicivirus, Cro1, Complete genome, Vesivirus phylogeny, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Vesiviruses in the family Caliciviridae infect a broad range of animal hosts including mammals, birds, fish, amphibians and reptiles. The vesivirus Cro1 strains were isolated from diseased snakes in the San Diego zoo in 1978 and reported as the first caliciviruses found in reptiles. The goal of this study was to characterize the Cro1 strain 780032I that was isolated in cell culture from a rock rattlesnake (Crotalus lepidus) in the original outbreak. Results We re-amplified the original virus stock in Vero cells, and determined its full-length genome sequence. The Cro1 genome is 8296 nucleotides (nt) in length and has a typical vesivirus organization, with three open reading frames (ORF), ORF1 (5643 nt), ORF2 (2121 nt), and ORF3 (348 nt) encoding a nonstructural polyprotein, the major capsid protein precursor, and a minor structural protein, respectively. Phylogenetic analysis of the full-length genome sequence revealed that the Cro1 virus clustered most closely with the VESV species of the genus Vesivirus, but was genetically distinct (82-83% identities with closest strains). Conclusions This is the first description of a full-length genome sequence from a reptile calicivirus (Cro1). The availability of the Cro1 genome sequence should facilitate investigation of the molecular mechanisms involved in Cro1 virus evolution and host range.

Published

2012

3. Nucleolin-RNA interaction modulates rotavirus replication.

Author

Hernández-Guzmán J, Arias CF, López S, and Sandoval-Jaime C

Subjects

Humans, Virus Replication, Nucleolin metabolism, RNA, Viral genetics, Rotavirus physiology, Rotavirus Infections virology

Abstract

Rotavirus infection is a leading cause of gastroenteritis in children worldwide; the genome of this virus is composed of 11 segments of dsRNA packed in a triple-layered protein capsid. Here, we investigated the role of nucleolin, a protein with diverse RNA-binding domains, in rotavirus infection. Knocking down the expression of nucleolin in MA104 cells by RNA interference resulted in a remarkable 6.3-fold increase in the production of infectious rhesus rotavirus (RRV) progeny, accompanied by an elevated synthesis of viral mRNA and genome copies. Further analysis unveiled an interaction between rotavirus segment 10 (S10) and nucleolin, potentially mediated by G-quadruplex domains on the viral genome. To determine whether the nucleolin-RNA interaction regulates RRV replication, MA104 cells were transfected with AGRO100, a compound that forms G4 structures and selectively inhibits nucleolin-RNA interactions by blocking the RNA-binding domains. Under these conditions, viral production increased by 1.5-fold, indicating the inhibitory role of nucleolin on the yield of infectious viral particles. Furthermore, G4 sequences were identified in all 11 RRV dsRNA segments, and transfection of oligonucleotides representing G4 sequences in RRV S10 induced a significant increase in viral production. These findings show that rotavirus replication is negatively regulated by nucleolin through the direct interaction with the viral RNAs by sequences forming G4 structures.IMPORTANCEViruses rely on cellular proteins to carry out their replicative cycle. In the case of rotavirus, the involvement of cellular RNA-binding proteins during the replicative cycle is a poorly studied field. In this work, we demonstrate for the first time the interaction between nucleolin and viral RNA of rotavirus RRV. Nucleolin is a cellular protein that has a role in the metabolism of ribosomal rRNA and ribosome biogenesis, which seems to have regulatory effects on the quantity of viral particles and viral RNA copies of rotavirus RRV. Our study adds a new component to the current model of rotavirus replication, where cellular proteins can have a negative regulation on rotavirus replication., Competing Interests: The authors declare no conflict of interest.

Published

2024

4. The Capsid Precursor Protein of Astrovirus VA1 Is Proteolytically Processed Intracellularly.

Author

Aguilera-Flores C, López T, Zamudio F, Sandoval-Jaime C, Pérez EI, López S, DuBois R, and Arias CF

Subjects

Caco-2 Cells, Capsid metabolism, Humans, Intracellular Space virology, Trypsin metabolism, Astroviridae Infections virology, Capsid Proteins metabolism, Mamastrovirus physiology, Protein Precursors metabolism

Abstract

Human astrovirus VA1 has been associated with neurological disease in immunocompromised patients, and its recent propagation in cell culture has opened the possibility to study its biology. Unlike classical human astroviruses, VA1 growth was found to be independent of trypsin during virus replication in vitro . In this work, we show that despite its independence on trypsin activation for cell infection, the VA1 capsid precursor protein, of 86 kDa (VP86), is processed intracellularly, and this proteolytic processing is important for astrovirus VA1 infectivity. Antibodies raised against different regions of the capsid precursor showed that the polyprotein can be processed starting at either its amino- or carboxy-terminal end, and they allowed us to identify those proteins of about 33 (VP33) and 38 (VP38) kDa constitute the core and the spike proteins of the mature infectious virus particles, respectively. The amino-terminal end of the spike protein was found to be Thr-348. Whether the protease involved in intracellular cleavage of the capsid precursor is of viral or cellular origin remains to be determined, but the cleavage is independent of caspases. Also, trypsin is able to degrade the capsid precursor but has no effect on VP33 and VP38 proteins when assembled into virus particles. These studies provide the basis for advancement of the knowledge of astrovirus VA1 cell entry and replication. IMPORTANCE Human astrovirus VA1 has been associated with neurological disease in immunocompromised patients. Its recent propagation in cell culture has facilitated the study of its biology. In this work, we show that despite the ability of this virus to grow in the absence of trypsin, a marked feature of human classical astroviruses, the capsid precursor protein of astrovirus VA1 is cleaved intracellularly to yield the mature infectious particles, formed by two polypeptides, VP33 that constitutes the core domain of the virus particle, and VP38 that forms the spike of the virus. These studies provide a platform to advance our knowledge on astrovirus VA1 cell entry and replication.

Published

2022

5. Pooling saliva samples as an excellent option to increase the surveillance for SARS-CoV-2 when re-opening community settings.

Author

Moreno-Contreras J, Espinoza MA, Sandoval-Jaime C, Cantú-Cuevas MA, Madrid-González DA, Barón-Olivares H, Ortiz-Orozco OD, Muñoz-Rangel AV, Guzmán-Rodríguez C, Hernández-de la Cruz M, Eroza-Osorio CM, Arias CF, and López S

Subjects

COVID-19 epidemiology, COVID-19 prevention & control, COVID-19 Nucleic Acid Testing standards, Humans, Mass Screening methods, Mass Screening standards, Quarantine standards, SARS-CoV-2 genetics, SARS-CoV-2 isolation & purification, SARS-CoV-2 pathogenicity, Sensitivity and Specificity, COVID-19 diagnosis, COVID-19 Nucleic Acid Testing methods, Saliva virology

Abstract

In many countries a second wave of infections caused by the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) has occurred, triggering a shortage of reagents needed for diagnosis and compromising the capacity of laboratory testing. There is an urgent need to develop methods to accelerate the diagnostic procedures. Pooling samples represents a strategy to overcome the shortage of reagents, since several samples can be tested using one reaction, significantly increasing the number and speed with which tests can be carried out. We have reported the feasibility to use a direct lysis procedure of saliva as source for RNA to SARS-CoV-2 genome detection by reverse transcription quantitative-PCR (RT-qPCR). Here, we show that the direct lysis of saliva pools, of either five or ten samples, does not compromise the detection of viral RNA. In addition, it is a sensitive, fast, and inexpensive method that can be used for massive screening, especially considering the proximity of the reincorporation of activities in universities, offices, and schools., Competing Interests: The authors have declared that no competing interests exist.

Published

2022

6. Molecular Detection and Characterization of Porcine Epidemic Diarrhea Virus and Porcine Aichivirus C Coinfection in México.

Author

García-Hernández ME, Trujillo-Ortega ME, Alcaraz-Estrada SL, Lozano-Aguirre-Beltrán L, Sandoval-Jaime C, Taboada-Ramírez BI, and Sarmiento-Silva RE

Subjects

Animals, Coinfection epidemiology, Coronavirus Infections epidemiology, Diarrhea virology, Feces virology, Genome, Viral, Kobuvirus classification, Mexico epidemiology, Molecular Diagnostic Techniques, Phylogeny, Porcine epidemic diarrhea virus classification, Sapovirus genetics, Sequence Analysis, Swine, Swine Diseases virology, Coinfection virology, Coronavirus Infections virology, Kobuvirus genetics, Kobuvirus isolation & purification, Porcine epidemic diarrhea virus genetics, Porcine epidemic diarrhea virus isolation & purification

Abstract

Swine enteric viral infections are responsible for substantial economic losses in the pork industry worldwide. Porcine epidemic diarrhea (PEDV) is one of the main causative agents of diarrhea in lactating pigs, and reports of PEDV coinfection with other enteric viruses highlight the importance of viral interactions for disease presentation and outcomes. Using next-generation sequencing (NGS) and sequence analyses from samples taken from piglets with acute diarrhea, we explored the possible interactions between PEDV and other less reported pathogens. PEDV coinfection with porcine kobuvirus (PKV) was detected in 36.4% (27/74) of samples. Full genomes from porcine coronavirus and kobuvirus were obtained, as was a partial porcine sapovirus genome (PSaV). The phylogenetic results show the clustering of these strains corresponding to the geographical relationship. To our knowledge, this is the first full genome and isolation report for porcine kobuvirus in México, as well as the first phylogenetic analysis for porcine sapovirus in the country. The NGS approach provides a better perspective of circulating viruses and other pathogens in affected production units.

Published

2021

7. Astrovirus reverse genetics systems, a story of success.

Author

Sandoval-Jaime C

Subjects

Animals, Astroviridae Infections immunology, Cell Line, Gastroenteritis prevention & control, Gastroenteritis veterinary, Gastroenteritis virology, Humans, Plasmids genetics, Plasmids immunology, Astroviridae genetics, Astroviridae immunology, Astroviridae Infections prevention & control, Astroviridae Infections veterinary, Genome, Viral, Reverse Genetics methods

Abstract

Astroviruses are one of the main causes of gastroenteritis of medical and veterinary relevance worldwide. Recently, these viruses were associated with neurological disease in mammals, including humans. Reverse genetics systems are the most powerful tool to improve our understanding of the virus replication, and eventually to develop safe vaccine candidates. In the present review, it is summarized the current knowledge on the different strategies used to develop reverse genetics systems for mamastroviruses and avastroviruses, and some of the biological answers that have provided are discussed., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

8. Saliva Sampling and Its Direct Lysis, an Excellent Option To Increase the Number of SARS-CoV-2 Diagnostic Tests in Settings with Supply Shortages.

Author

Moreno-Contreras J, Espinoza MA, Sandoval-Jaime C, Cantú-Cuevas MA, Barón-Olivares H, Ortiz-Orozco OD, Muñoz-Rangel AV, Hernández-de la Cruz M, Eroza-Osorio CM, Arias CF, and López S

Subjects

Betacoronavirus genetics, COVID-19 Testing, Clinical Laboratory Techniques, Coronavirus Infections diagnosis, Coronavirus Infections epidemiology, Diagnostic Tests, Routine, Genome, Viral genetics, Humans, Nasopharynx virology, Oropharynx virology, RNA, Viral genetics, RNA, Viral isolation & purification, Real-Time Polymerase Chain Reaction, SARS-CoV-2, Viral Load, Betacoronavirus isolation & purification, Saliva virology, Specimen Handling methods

Abstract

As part of any plan to lift or ease the confinement restrictions that are in place in many different countries, there is an urgent need to increase the capacity of laboratory testing for severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2). Detection of the viral genome through reverse transcription-quantitative PCR (RT-qPCR) is the gold standard for this virus; however, the high demand of the materials and reagents needed to sample individuals, purify the viral RNA, and perform the RT-qPCR has resulted in a worldwide shortage of several of these supplies. Here, we show that directly lysed saliva samples can serve as a suitable source for viral RNA detection that is less expensive and can be as efficient as the classical protocol, which involves column purification of the viral RNA. In addition, it bypasses the need for swab sampling, decreases the risk of the health care personnel involved in the testing process, and accelerates the diagnostic procedure., (Copyright © 2020 American Society for Microbiology.)

Published

2020

9. Development of a novel DNA based reverse genetics system for classic human astroviruses.

Author

Sandoval-Jaime C, Guzmán-Ruiz L, López S, and Arias CF

Subjects

DNA, Complementary genetics, Genetic Vectors, Genome, Viral, Humans, Plasmids, Mamastrovirus genetics, Mamastrovirus growth & development, Reverse Genetics methods

Abstract

Human astroviruses (HAstVs) are a frequent cause of gastroenteritis in young children and immunocompromised patients. The current report describes a new approach to recover genetically defined HAstVs through the use of a reverse genetics system based on a single DNA plasmid. This plasmid, carrying the full-length virus genome under a T7 promoter, is directly transfected into cells expressing T7 RNA polymerase, resulting in the rapid and robust recovery of infectious HAstV. The efficiency of the system was tested with the generation of a chimeric astrovirus having the HAstV serotype 1 replication machinery and the capsid derived from a HAstV serotype 8 virus. This new system provides an efficient and reproducible method to deepen our knowledge of astrovirus biology., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2019

10. Phylogenetic Analysis and Characterization of the Complete Hepatitis E Virus Genome (Zoonotic Genotype 3) in Swine Samples from Mexico.

Author

Sotomayor-González A, Trujillo-Ortega ME, Taboada-Ramírez BI, Sandoval-Jaime C, and Sarmiento-Silva RE

Subjects

Abattoirs, Animals, Animals, Domestic, Bile virology, Feces virology, High-Throughput Nucleotide Sequencing, Liver virology, Mexico, Swine virology, Zoonoses virology, Genome, Viral, Genotype, Hepatitis E veterinary, Hepatitis E virus genetics, Phylogeny, Swine Diseases virology

Abstract

Hepatitis E virus (HEV) is an emerging public health problem with an estimated 20 million infections each year. In Mexico, Orthohepevirus A, genotype 2, has been reported in humans, but genotype 3 has only been reported in swine (zoonotic). No diagnostic tests are publicly available in Mexico, and only partial sequences have been reported from swine samples. Hence, research is necessary to determine circulating strains, understand the features and dynamics of infection on pig farms, determine how to implement surveillance programs, and to assess public health risks. In this study, a next-generation sequencing (NGS) approach was applied to obtain a complete genome of swine HEV. Liver, feces, and bile samples were taken at slaughterhouses and a farm in Mexico. RT-PCR was used to determine positive samples and confirmed by Sanger sequencing. Of the 64 slaughterhouse samples, one bile sample was positive (B1r) (1.56%). Of 21 sample pools from farm animals, 14 were positive (66.66%), representing all stages of production. A complete sequence strain MXCDg3_B1c|_2016 was obtained from the bile of a domestic swine in the fattening stage. In addition, two partial sequences-MXCDg3_H2cons|_2016 (1473 nt) and MXCDg3_C3Acons|_2016 (4777 nt)-were obtained from sampled farm animals. Comparison with all reported genome HEV sequences showed similarity to genotype 3 subgenotype a (G3a), which has been previously reported in acute cases of human hepatitis in the US, Colombia, China, and Japan.

Published

2018

11. Identification of Human Junctional Adhesion Molecule 1 as a Functional Receptor for the Hom-1 Calicivirus on Human Cells.

Author

Sosnovtsev SV, Sandoval-Jaime C, Parra GI, Tin CM, Jones RW, Soden J, Barnes D, Freeth J, Smith AW, and Green KY

Subjects

Animals, CHO Cells, Cats, Cell Adhesion Molecules deficiency, Cell Adhesion Molecules isolation & purification, Cell Membrane chemistry, Cell Membrane genetics, Cricetinae, Cricetulus, Humans, Receptors, Cell Surface deficiency, Receptors, Cell Surface isolation & purification, Receptors, Virus isolation & purification, Vesivirus growth & development, Cell Adhesion Molecules genetics, Cell Adhesion Molecules metabolism, Receptors, Cell Surface genetics, Receptors, Cell Surface metabolism, Receptors, Virus metabolism, Vesivirus physiology, Virus Replication

Abstract

The Hom-1 vesivirus was reported in 1998 following the inadvertent transmission of the animal calicivirus San Miguel sea lion virus to a human host in a laboratory. We characterized the Hom-1 strain and investigated the mechanism by which human cells could be infected. An expression library of 3,559 human plasma membrane proteins was screened for reactivity with Hom-1 virus-like particles, and a single interacting protein, human junctional adhesion molecule 1 (hJAM1), was identified. Transient expression of hJAM1 conferred susceptibility to Hom-1 infection on nonpermissive Chinese hamster ovary (CHO) cells. Virus infection was markedly inhibited when CHO cells stably expressing hJAM were pretreated with anti-hJAM1 monoclonal antibodies. Cell lines of human origin were tested for growth of Hom-1, and efficient replication was observed in HepG2, HuH7, and SK-CO15 cells. The three cell lines (of hepatic or intestinal origin) were confirmed to express hJAM1 on their surface, and clustered regularly interspaced short palindromic repeats/Cas9-mediated knockout of the hJAM1 gene in each line abolished Hom-1 propagation. Taken together, our data indicate that entry of the Hom-1 vesivirus into these permissive human cell lines is mediated by the plasma membrane protein hJAM1 as a functional receptor. IMPORTANCE Vesiviruses, such as San Miguel sea lion virus and feline calicivirus, are typically associated with infection in animal hosts. Following the accidental infection of a laboratory worker with San Miguel sea lion virus, a related virus was isolated in cell culture and named Hom-1. In this study, we found that Hom-1 could be propagated in a number of human cell lines, making it the first calicivirus to replicate efficiently in cultured human cells. Screening of a library of human cell surface membrane proteins showed that the virus could utilize human junctional adhesion molecule 1 as a receptor to enter cells and initiate replication. The Hom-1 virus presents a new system for the study of calicivirus biology and species specificity., (Copyright © 2017 Sosnovtsev et al.)

Published

2017

12. Stress Response and Translation Control in Rotavirus Infection.

Author

López S, Oceguera A, and Sandoval-Jaime C

Subjects

Gene Expression Regulation, Humans, Immunity, Innate, Virus Replication, Host-Pathogen Interactions, Protein Biosynthesis, Rotavirus immunology, Rotavirus pathogenicity, Rotavirus Infections immunology, Rotavirus Infections pathology, Stress, Physiological

Abstract

The general stress and innate immune responses are closely linked and overlap at many levels. The outcomes of these responses serve to reprogram host expression patterns to prevent viral invasions. In turn, viruses counter attack these cell responses to ensure their replication. The mechanisms by which viruses attempt to control host cell responses are as varied as the number of different virus families. One of the most recurrent strategies used by viruses to control the antiviral response of the cell is to hijack the translation machinery of the host, such that viral proteins are preferentially synthesized, while the expression of the stress and antiviral responses of the cell are blocked at the translation level. Here, we will review how rotaviruses, an important agent of acute severe gastroenteritis in children, overcome the stress responses of the cell to establish a productive infectious cycle.

Published

2016

13. Mapping and modeling of a strain-specific epitope in the Norwalk virus capsid inner shell.

Author

Parra GI, Sosnovtsev SV, Abente EJ, Sandoval-Jaime C, Bok K, Dolan MA, and Green KY

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal biosynthesis, Antibodies, Monoclonal chemistry, Antibodies, Viral biosynthesis, Calicivirus, Feline genetics, Calicivirus, Feline metabolism, Capsid chemistry, Capsid immunology, Capsid Proteins genetics, Capsid Proteins immunology, Epitope Mapping, Epitopes genetics, Epitopes immunology, Gene Expression, Mice, Mice, Inbred BALB C, Models, Molecular, Molecular Sequence Data, Norwalk virus genetics, Protein Structure, Tertiary, Sequence Alignment, Single-Chain Antibodies biosynthesis, Antibodies, Viral chemistry, Capsid Proteins chemistry, Epitopes chemistry, Norwalk virus immunology, Single-Chain Antibodies chemistry

Abstract

Noroviruses are diverse positive-strand RNA viruses associated with acute gastroenteritis. Cross-reactive epitopes have been mapped primarily to conserved sequences in the capsid VP1 Shell (S) domain, and strain-specific epitopes to the highly variable Protruding (P) domain. In this work, we investigated a strain-specific linear epitope defined by MAb NV10 that was raised against prototype (Genogroup I.1) strain Norwalk virus (NV). Using peptide scanning and mutagenesis, the epitope was mapped to amino acids 21-32 (LVPEVNASDPLA) of the NV S domain, and its specificity was verified by epitope transfer and reactivity with a recombinant MAb NV10 single-chain variable fragment (scFv). Comparative structural modeling of the NV10 strain-specific and the broadly cross-reactive TV20 epitopes identified two internal non-overlapping sites in the NV shell, corresponding to variable and conserved amino acid sequences among strains, respectively. The S domain, like the P domain, contains strain-specific epitopes that contribute to the antigenic diversity among the noroviruses., (Published by Elsevier Inc.)

Published

2016

14. Nucleolin promotes in vitro translation of feline calicivirus genomic RNA.

Author

Hernández BA, Sandoval-Jaime C, Sosnovtsev SV, Green KY, and Gutiérrez-Escolano AL

Subjects

Animals, Caliciviridae Infections genetics, Caliciviridae Infections metabolism, Caliciviridae Infections virology, Calicivirus, Feline physiology, Cat Diseases genetics, Cats, Cell Line, Host-Pathogen Interactions, Phosphoproteins genetics, RNA, Viral metabolism, RNA-Binding Proteins genetics, Viral Proteins genetics, Viral Proteins metabolism, Virus Replication, Nucleolin, Caliciviridae Infections veterinary, Calicivirus, Feline genetics, Cat Diseases metabolism, Cat Diseases virology, Phosphoproteins metabolism, Protein Biosynthesis, RNA, Viral genetics, RNA-Binding Proteins metabolism

Abstract

Feline calicivirus depends on host-cell proteins for its replication. We previously showed that knockdown of nucleolin (NCL), a phosphoprotein involved in ribosome biogenesis, resulted in the reduction of FCV protein synthesis and virus yield. Here, we found that NCL may not be involved in FCV binding and entry into cells, but it binds to both ends of the FCV genomic RNA, and stimulates its translation in vitro. AGRO100, an aptamer that specifically binds and inactivates NCL, caused a strong reduction in FCV protein synthesis. This effect could be reversed by the addition of full-length NCL but not by a ΔrNCL, lacking the N-terminal domain. Consistent with this, FCV infection of CrFK cells stably expressing ΔrNCL led to a reduction in virus protein translation. These results suggest that NCL is part of the FCV RNA translational complex, and that the N-terminal part of the protein is required for efficient FCV replication., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2016

15. Recovery of murine norovirus and feline calicivirus from plasmids encoding EMCV IRES in stable cell lines expressing T7 polymerase.

Author

Sandoval-Jaime C, Green KY, and Sosnovtsev SV

Subjects

Animals, Calicivirus, Feline genetics, Cell Line, Cricetinae, DNA-Directed RNA Polymerases genetics, Humans, Norovirus genetics, Protein Biosynthesis, Transcription, Genetic, Viral Proteins genetics, Calicivirus, Feline physiology, DNA-Directed RNA Polymerases metabolism, Encephalomyocarditis virus genetics, Internal Ribosome Entry Sites, Norovirus physiology, Plasmids, Reverse Genetics methods, Viral Proteins metabolism

Abstract

Reverse genetics systems constitute one of the most important and powerful tools to study the molecular biology of viruses. We developed a new strategy for the recovery of murine norovirus from a single plasmid in which a bacteriophage T7 RNA polymerase (T7pol) promoter for transcription and an EMCV IRES for efficient translation were engineered immediately upstream of the viral genome. Infectious noroviruses were recovered following transfection of the newly designed plasmid into nonpermissive BHK-21 and HEK293T cell lines that were engineered to express T7pol constitutively. Recovery of the virus did not require the presence of a ribozyme at the 3'-end of the virus genome. The strategy worked also for the efficient recovery of feline calicivirus in these normally nonpermissive cell types. This simplified reverse genetics approach may be broadly applicable to other caliciviruses., (Published by Elsevier B.V.)

Published

2015

16. Genetic characterization of feline calicivirus strains associated with varying disease manifestations during an outbreak season in Missouri (1995-1996).

Author

Prikhodko VG, Sandoval-Jaime C, Abente EJ, Bok K, Parra GI, Rogozin IB, Ostlund EN, Green KY, and Sosnovtsev SV

Subjects

Animals, Asymptomatic Diseases, Caliciviridae Infections pathology, Caliciviridae Infections virology, Calicivirus, Feline isolation & purification, Capsid Proteins genetics, Cats, Cluster Analysis, Disease Outbreaks, Genome, Viral, Missouri epidemiology, Molecular Sequence Data, Mutation, Missense, Phylogeny, RNA, Viral genetics, Sequence Analysis, DNA, Sequence Homology, Caliciviridae Infections veterinary, Calicivirus, Feline classification, Calicivirus, Feline genetics, Cat Diseases pathology, Cat Diseases virology

Abstract

Feline calicivirus (FCV) is a common cause of mild to severe upper respiratory tract disease (URTD) in cats. FCV strain 21223 was isolated from a kitten with severe pneumonia in a disease outbreak with unusually high mortality (35 %) that occurred in a Missouri feline colony in 1995-1996. Phylogenetic analysis of the genome sequence of strain 21223 indicated the emergence of a new FCV strain. Analysis of the full-length genome sequence of a closely related (99.5 % nucleotide identity) strain, 3786, obtained from an asymptomatic animal in the same colony four months later, showed the presence of seven amino acid substitutions, with six of them located in the VP1 capsid sequence encoded by ORF2. Comparative analysis of the E-region sequences (426-521 aa ORF2) presumably involved in virus-host cell receptor interactions did not identify amino acid substitutions unique to the virulent strain. We determined the complete genome sequences of four virus isolates that were collected in regional catteries in the months following the outbreak that were associated with different manifestations of the disease (URTD, chronic stomatitis, and gingivitis). We show that genetically distinct FCV strains were cocirculating in the area, and no apparent correlation could be made between overall sequence and observed disease.

Published

2014

17. Identification of a Broadly Cross-Reactive Epitope in the Inner Shell of the Norovirus Capsid.

Author

Parra GI, Azure J, Fischer R, Bok K, Sandoval-Jaime C, Sosnovtsev SV, Sander P, and Green KY

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal analysis, Antibodies, Monoclonal immunology, Antibodies, Viral analysis, Antibodies, Viral immunology, Capsid chemistry, Capsid Proteins genetics, Capsid Proteins immunology, Capsid Proteins metabolism, Chlorocebus aethiops, Cross Reactions, Enzyme-Linked Immunosorbent Assay, Epitopes genetics, Epitopes immunology, Epitopes metabolism, Genotype, Mice, Mice, Inbred BALB C, Microscopy, Fluorescence, Mutagenesis, Norovirus genetics, Recombinant Proteins biosynthesis, Recombinant Proteins immunology, Recombinant Proteins isolation & purification, Sequence Alignment, Vero Cells, Viral Proteins genetics, Viral Proteins immunology, Viral Proteins metabolism, Capsid metabolism, Norovirus metabolism

Abstract

Noroviruses are major pathogens associated with acute gastroenteritis. They are diverse viruses, with at least six genogroups (GI-GVI) and multiple genotypes defined by differences in the major capsid protein, VP1. This diversity has challenged the development of broadly cross-reactive vaccines as well as efficient detection methods. Here, we report the characterization of a broadly cross-reactive monoclonal antibody (MAb) raised against the capsid protein of a GII.3 norovirus strain. The MAb reacted with VLPs and denatured VP1 protein from GI, GII, GIV and GV noroviruses, and mapped to a linear epitope located in the inner shell domain. An alignment of all available VP1 sequences showed that the putative epitope (residues 52-56) is highly conserved across the genus Norovirus. This broadly cross-reactive MAb thus constitutes a valuable reagent for the diagnosis and study of these diverse viruses.

Published

2013

18. The feline calicivirus leader of the capsid protein is associated with cytopathic effect.

Author

Abente EJ, Sosnovtsev SV, Sandoval-Jaime C, Parra GI, Bok K, and Green KY

Subjects

Animals, Annexin A2 metabolism, Capsid Proteins genetics, Cats, Cell Line, Host-Pathogen Interactions, Point Mutation, Protein Binding, Protein Processing, Post-Translational, Sequence Deletion, Virulence Factors genetics, Calicivirus, Feline pathogenicity, Capsid Proteins metabolism, Cytopathogenic Effect, Viral, Virulence Factors metabolism

Abstract

Open reading frame 2 (ORF2) of the feline calicivirus (FCV) genome encodes a capsid precursor that is posttranslationally processed to release the mature capsid protein (VP1) and a small protein of 124 amino acids, designated the leader of the capsid (LC). To investigate the role of the LC protein in the virus life cycle, mutations and deletions were introduced into the LC coding region of an infectious FCV cDNA clone. Three cysteine residues that are conserved among all vesivirus LC sequences were found to be critical for the recovery of FCV with a characteristic cytopathic effect in feline kidney cells. A cell-rounding phenotype associated with the transient expression of wild-type and mutagenized forms of the LC correlated with the cytopathic and growth properties of the corresponding engineered viruses. The host cellular protein annexin A2 was identified as a binding partner of the LC protein, consistent with a role for the LC in mediating host cell interactions that alter the integrity of the cell and enable virus spread.

Published

2013

19. Multiple antigenic sites are involved in blocking the interaction of GII.4 norovirus capsid with ABH histo-blood group antigens.

Author

Parra GI, Abente EJ, Sandoval-Jaime C, Sosnovtsev SV, Bok K, and Green KY

Subjects

Animals, Antibodies, Monoclonal immunology, Antibodies, Viral immunology, Caliciviridae Infections epidemiology, Capsid Proteins genetics, Disease Outbreaks, Enzyme-Linked Immunosorbent Assay, Epitope Mapping, Genotype, Humans, Maryland epidemiology, Mice, Mice, Inbred BALB C, Norovirus genetics, Norovirus isolation & purification, Protein Binding, ABO Blood-Group System metabolism, Caliciviridae Infections virology, Capsid Proteins metabolism, Norovirus pathogenicity, Protein Interaction Mapping

Abstract

Noroviruses are major etiological agents of acute viral gastroenteritis. In 2002, a GII.4 variant (Farmington Hills cluster) spread so rapidly in the human population that it predominated worldwide and displaced previous GII.4 strains. We developed and characterized a panel of six monoclonal antibodies (MAbs) directed against the capsid protein of a Farmington Hills-like GII.4 norovirus strain that was associated with a large hospital outbreak in Maryland in 2004. The six MAbs reacted with high titers against homologous virus-like particles (VLPs) by enzyme-linked immunoassay but did not react with denatured capsid protein in immunoblots. The expression and self-assembly of newly developed genogroup I/II chimeric VLPs showed that five MAbs bound to the GII.4 protruding (P) domain of the capsid protein, while one recognized the GII.4 shell (S) domain. Cross-competition assays and mutational analyses showed evidence for at least three distinct antigenic sites in the P domain and one in the S domain. MAbs that mapped to the P domain but not the S domain were able to block the interaction of VLPs with ABH histo-blood group antigens (HBGA), suggesting that multiple antigenic sites of the P domain are involved in HBGA blocking. Further analysis showed that two MAbs mapped to regions of the capsid that had been associated with the emergence of new GII.4 variants. Taken together, our data map antibody and HBGA carbohydrate binding to proximal regions of the norovirus capsid, showing that evolutionary pressures on the norovirus capsid protein may affect both antigenic and carbohydrate recognition phenotypes.

Published

2012

20. Nucleolin interacts with the feline calicivirus 3' untranslated region and the protease-polymerase NS6 and NS7 proteins, playing a role in virus replication.

Author

Cancio-Lonches C, Yocupicio-Monroy M, Sandoval-Jaime C, Galvan-Mendoza I, Ureña L, Vashist S, Goodfellow I, Salas-Benito J, and Gutiérrez-Escolano AL

Subjects

Animals, Calicivirus, Feline genetics, Calicivirus, Feline metabolism, Cats, Cell Line, Kidney virology, Norwalk virus genetics, Norwalk virus metabolism, Peptide Hydrolases, Phosphoproteins genetics, RNA Interference, RNA, Messenger genetics, RNA, Messenger metabolism, RNA, Small Interfering, RNA, Viral genetics, RNA, Viral metabolism, RNA-Binding Proteins genetics, Viral Proteins genetics, Nucleolin, 3' Untranslated Regions, Calicivirus, Feline physiology, Phosphoproteins metabolism, RNA-Binding Proteins metabolism, Viral Proteins metabolism, Virus Replication

Abstract

Cellular proteins play many important roles during the life cycle of all viruses. Specifically, host cell nucleic acid-binding proteins interact with viral components of positive-stranded RNA viruses and regulate viral translation, as well as RNA replication. Here, we report that nucleolin, a ubiquitous multifunctional nucleolar shuttling phosphoprotein, interacts with the Norwalk virus and feline calicivirus (FCV) genomic 3' untranslated regions (UTRs). Nucleolin can also form a complex in vitro with recombinant Norwalk virus NS6 and -7 (NS6/7) and can be copurified with the analogous protein from feline calicivirus (p76 or NS6/7) from infected feline kidney cells. Nucleolin RNA levels or protein were not modified during FCV infection; however, as a consequence of the infection, nucleolin was seen to relocalize from the nucleoli to the nucleoplasm, as well as to the perinuclear area where it colocalizes with the feline calicivirus NS6/7 protein. In addition, antibodies to nucleolin were able to precipitate viral RNA from feline calicivirus-infected cells, indicating a direct or indirect association of nucleolin with the viral RNA during virus replication. Small interfering RNA (siRNA)-mediated knockdown of nucleolin resulted in a reduction of the cytopathic effect and virus yield in CrFK cells. Taken together, these results demonstrate that nucleolin is a nucleolar component that interacts with viral RNA and NS6/7 and is required for feline calicivirus replication.

Published

2011

21. Diversity of murine norovirus strains isolated from asymptomatic mice of different genetic backgrounds within a single U.S. research institute.

Author

Barron EL, Sosnovtsev SV, Bok K, Prikhodko V, Sandoval-Jaime C, Rhodes CR, Hasenkrug K, Carmody AB, Ward JM, Perdue K, and Green KY

Subjects

Animals, Cell Line, Fluorescent Antibody Technique, Mice, Norovirus isolation & purification, Phylogeny, Reverse Transcriptase Polymerase Chain Reaction, United States, Academies and Institutes, Norovirus classification, Norovirus genetics

Abstract

Antibody prevalence studies in laboratory mice indicate that murine norovirus (MNV) infections are common, but the natural history of these viruses has not been fully established. This study examined the extent of genetic diversity of murine noroviruses isolated from healthy laboratory mice housed in multiple animal facilities within a single, large research institute- the National Institute of Allergy and Infectious Diseases of the National Institutes of Health (NIAID-NIH) in Bethesda, Maryland, U.S. Ten distinct murine norovirus strains were isolated from various tissues and feces of asymptomatic wild type sentinel mice as well as asymptomatic immunodeficient (RAG 2(-/-)) mice. The NIH MNV isolates showed little cytopathic effect in permissive RAW264.7 cells in early passages, but all isolates examined could be adapted to efficient growth in cell culture by serial passage. The viruses, although closely related in genome sequence, were distinguishable from each other according to facility location, likely due to the introduction of new viruses into each facility from separate sources or vendors at different times. Our study indicates that the murine noroviruses are widespread in these animal facilities, despite rigorous guidelines for animal care and maintenance.

Published

2011

22. Cellular proteins mediate 5'-3' end contacts of Norwalk virus genomic RNA.

Author

Sandoval-Jaime C and Gutiérrez-Escolano AL

Subjects

3' Untranslated Regions genetics, 5' Untranslated Regions genetics, Caco-2 Cells, Genome, Viral, HeLa Cells, Humans, Norwalk virus genetics, Nucleic Acid Conformation, Protein Biosynthesis, RNA, Viral biosynthesis, RNA, Viral genetics, 3' Untranslated Regions metabolism, 5' Untranslated Regions physiology, Norwalk virus metabolism, RNA-Binding Proteins metabolism

Abstract

Long-range RNA-RNA interactions between the 5' and 3' ends are a common feature involved in the regulation of both the initiation of translation and the synthesis of the viral genomic RNAs. These interactions either take place by direct RNA-RNA contacts or can be mediated by proteins. By in silico analysis, we found three possible complementary sequences (CS) between the 5' and the 3' ends of the Norwalk virus genomic RNA. Co-precipitation assays demonstrated that physical contacts between the 5' and the 3' ends of the NV genomic RNA were stabilized by cellular proteins. Mutations and deletions within these regions, that altered the formation of the CS-1 motif disrupted the 5'-3' end contacts, while mutations that restore complementarity of the CS-1 motif, recover the ability to form these contacts. These results suggest that the NV genomic 5'-3' end contacts initially occur by RNA-RNA interactions but are further stabilized by cellular proteins.

Published

2009