Your search keyword '"Franchin E"' showing total 11 results

1. SARS-CoV-2 RNA identification in nasopharyngeal swabs: issues in pre-analytics.

Author

Basso D, Aita A, Navaglia F, Franchin E, Fioretto P, Moz S, Bozzato D, Zambon CF, Martin B, Dal Prà C, Crisanti A, and Plebani M

Subjects

Aged, Aged, 80 and over, COVID-19, COVID-19 Testing, Clinical Laboratory Techniques, Coronavirus Envelope Proteins, Coronavirus Infections diagnosis, Diagnostic Tests, Routine, Female, Humans, Male, Middle Aged, Pandemics, Pneumonia, Viral diagnosis, Reproducibility of Results, Reverse Transcriptase Polymerase Chain Reaction, Ribonuclease P genetics, SARS-CoV-2, Temperature, Time Factors, Viral Envelope Proteins genetics, Betacoronavirus chemistry, Nasopharynx virology, RNA, Viral analysis, Specimen Handling methods

Abstract

Objectives: The direct identification of SARS-CoV-2 RNA in nasopharyngeal swabs is recommended for diagnosing the novel COVID-19 disease. Pre-analytical determinants, such as sampling procedures, time and temperature storage conditions, might impact on the end result. Our aim was to evaluate the effects of sampling procedures, time and temperature of the primary nasopharyngeal swabs storage on real-time reverse-transcription polymerase chain reaction (rRT-PCR) results., Methods: Each nasopharyngeal swab obtained from 10 hospitalized patients for COVID-19 was subdivided in 15 aliquots: five were kept at room temperature; five were refrigerated (+4 °C); five were immediately mixed with the extraction buffer and refrigerated at +4 °C. Every day and for 5 days, one aliquot per condition was analyzed (rRT-PCR) for SARS-CoV-2 gene E and RNaseP and threshold cycles (Ct) compared. To evaluate manual sampling, 70 nasopharyngeal swabs were sampled twice by two different operators and analyzed separately one from the other., Results: A total of 6/10 swabs were SARS-CoV-2 positive. No significant time or storage-dependent variations were observed in SARS-CoV-2 Ct. Re-sampling of swabs with SARS-CoV-2 Ct lower than 33 resulted in highly reproducible results (CV=2.9%), while a high variability was observed when Ct values were higher than 33 (CV=10.3%)., Conclusions: This study demonstrates that time and temperature of nasopharyngeal swabs storage do not significantly impact on results reproducibility. However, swabs sampling is a critical step, and especially in case of low viral load, might be a potential source of diagnostic errors.

Published

2020

2. Infection dynamics in a traveller with persistent shedding of Zika virus RNA in semen for six months after returning from Haiti to Italy, January 2016.

Author

Barzon L, Pacenti M, Franchin E, Lavezzo E, Trevisan M, Sgarabotto D, and Palù G

Subjects

Adult, Antibodies, Viral blood, Exanthema virology, Haiti, Humans, Immunoglobulin M blood, Italy, RNA, Viral genetics, RNA, Viral urine, Reverse Transcriptase Polymerase Chain Reaction, Semen virology, Semen Analysis, Sequence Analysis, RNA, Travel, Urine virology, Viral Load, Zika Virus genetics, Zika Virus Infection blood, Zika Virus Infection virology, Fever virology, RNA, Viral blood, Saliva virology, Semen chemistry, Virus Shedding, Zika Virus isolation & purification, Zika Virus Infection diagnosis

Abstract

We describe the dynamics of Zika virus (ZIKV) infection in a man in his early 40s who developed fever and rash after returning from Haiti to Italy, in January 2016. Follow-up laboratory testing demonstrated detectable ZIKV RNA in plasma up to day 9 after symptom onset and in urine and saliva up to days 15 and 47, respectively. Notably, persistent shedding of ZIKV RNA was demonstrated in semen, still detectable at 181 days after onset., Competing Interests: Conflicts of Interest: None declared., (This article is copyright of The Authors, 2016.)

Published

2016

3. Epstein-Barr and cytomegalovirus DNA salivary shedding correlate with long-term plasma HIV RNA detection in HIV-infected men who have sex with men.

Author

Scaggiante R, Andreis S, Basso M, Franchin E, Franzetti M, Del Vecchio C, Torti C, Mengoli C, Cruciani M, Sarmati L, Palù G, and Parisi SG

Subjects

Adult, CD4 Lymphocyte Count, Cytomegalovirus genetics, Cytomegalovirus isolation & purification, Cytomegalovirus Infections blood, Cytomegalovirus Infections virology, DNA, Viral analysis, Epstein-Barr Virus Infections blood, Epstein-Barr Virus Infections complications, Epstein-Barr Virus Infections virology, HIV Infections virology, HIV-1 genetics, Herpesvirus 4, Human genetics, Herpesvirus 4, Human isolation & purification, Humans, Male, Middle Aged, Neoplasms virology, Viral Load, Virus Replication, Cytomegalovirus physiology, HIV Infections complications, HIV-1 isolation & purification, Herpesvirus 4, Human physiology, Homosexuality, Male, RNA, Viral blood, Saliva virology, Virus Shedding

Abstract

The aim of the study was to evaluate cytomegalovirus (CMV) and Epstein-Barr virus (EBV) DNA salivary shedding in HIV-positive men who have sex with men (MSM) and to determine whether viro-immunological parameters and long-term (24 months) plasma HIV RNA (pHIV) detection may predict herpesviruses replication. A total of 193 HIV-positive MSM were consecutively recruited (mean CD4+ cell count 607 cells/mm(3) and mean nadir value 333 cells/mm(3) ); pHIV was analyzed for 24 months prior to saliva sampling: patients were categorized as successfully suppressed (SS) and not suppressed (NS). The EBV viral load was categorized as high viral load (HVL), intermediate (IVL), or low (LVL), CMV DNA as positive or negative. NS patients experienced both herpesviruses detectability more frequently respect to SS patients (P = 0.034); conversely, no salivary shedding was more frequent in SS patients (P = 0.014). HVL EBV was more frequent in NS patients than in SS subjects (P = 0.038 for isolated EBV detection and P = 0.001 when CMV shedding was associated). NS subjects with HVL EBV had a median pHIV of 43,820 copies/ml, significantly higher respect to IVL and LVL patients (P = 0.027 and P = 0.0005, respectively). CMV shedding was mostly associated to EBV shedding. NS patients showed a significantly higher frequency of saliva HVL EBV detection compared to SS patients; moreover, NS patients with HVL EBV had a higher pHIV respect to those with IVL and LVL shedding. Our results suggest that a successful pHIV suppression could reduce the burden of salivary EBV replication and likely the risk of herpesviruses-related cancers., (© 2015 Wiley Periodicals, Inc.)

Published

2016

4. Virological testing of cerebrospinal fluid in children aged less than 14 years with a suspected central nervous system infection: A retrospective study on 304 consecutive children from January 2012 to May 2015.

Author

Parisi SG, Basso M, Del Vecchio C, Andreis S, Franchin E, Bello FD, Pagni S, Biasolo MA, Manganelli R, Barzon L, and Palù G

Subjects

Adenoviridae genetics, Adenoviridae Infections cerebrospinal fluid, Adenoviridae Infections epidemiology, Central Nervous System Infections epidemiology, Central Nervous System Infections virology, Child, Child, Preschool, Cytomegalovirus genetics, Cytomegalovirus Infections cerebrospinal fluid, Cytomegalovirus Infections epidemiology, Encephalitis, Herpes Simplex cerebrospinal fluid, Encephalitis, Herpes Simplex epidemiology, Encephalitis, Varicella Zoster cerebrospinal fluid, Encephalitis, Varicella Zoster epidemiology, Enterovirus genetics, Enterovirus Infections cerebrospinal fluid, Enterovirus Infections epidemiology, Epstein-Barr Virus Infections cerebrospinal fluid, Epstein-Barr Virus Infections epidemiology, Female, Herpes Simplex genetics, Herpesviridae Infections cerebrospinal fluid, Herpesviridae Infections epidemiology, Herpesvirus 3, Human genetics, Herpesvirus 4, Human genetics, Herpesvirus 6, Human genetics, Herpesvirus 7, Human genetics, Herpesvirus 8, Human genetics, Humans, Infant, Newborn, Italy epidemiology, Male, Parechovirus genetics, Parvoviridae Infections cerebrospinal fluid, Parvoviridae Infections epidemiology, Parvovirus B19, Human genetics, Picornaviridae Infections cerebrospinal fluid, Picornaviridae Infections epidemiology, Prevalence, Real-Time Polymerase Chain Reaction, Retrospective Studies, Roseolovirus Infections cerebrospinal fluid, Roseolovirus Infections epidemiology, Virus Diseases epidemiology, Virus Diseases virology, Central Nervous System Infections cerebrospinal fluid, DNA, Viral cerebrospinal fluid, RNA, Viral cerebrospinal fluid, Virus Diseases cerebrospinal fluid

Abstract

Objective: The study aimed to describe the prevalence of HSV DNA, VZV DNA, Enterovirus RNA, Parechovirus RNA, CMV DNA, EBV DNA, adenovirus DNA, HHV-6 DNA, HHV-7 DNA, HHV-8 DNA and Parvovirus B19DNA in children aged less 14 years with a suspected viral infection of the central nervous system in a clinical practice setting., Methods: Between January 2012 and May 2015, cerebrospinal fluids from 304 children were tested with an in-house real-time PCR method., Results: A positive PCR was detected in 64 subjects (21%): the mean number of tests performed in patients who showed a viral infection was 7.5, significantly higher (p = 0.001) with respect to that reported in negative samples (6.4). Enterovirus is the leading virus detected: 12 out of the 37 positive children reported were newborns (85.7% of all the newborns with a positive result). The second most frequently identified virus was HHV-7 (5 positive PCR out of 105 samples tested, 4.8%, if we excluded a child with a concomitant S. pneumoniae isolated), a prevalence significantly higher with respect to VZV (p = 0.02) and to CMV (p = 0.04). HHV-6 was the third most commonly identified aetiology (4.2%). All children were immunocompetent., Significance: Only a minority of children had a specific viral aetiology identified: the rate of HHV-7 positivity suggests a routine testing of these viruses within the diagnostic algorithm in immunocompetent paediatric patients. This approach could help to define the clinical role of this herpesvirus., (Copyright © 2016 European Paediatric Neurology Society. Published by Elsevier Ltd. All rights reserved.)

Published

2016

5. Phylogenetic characterization of Central/Southern European lineage 2 West Nile virus: analysis of human outbreaks in Italy and Greece, 2013-2014.

Author

Barzon L, Papa A, Lavezzo E, Franchin E, Pacenti M, Sinigaglia A, Masi G, Trevisan M, Squarzon L, Toppo S, Papadopoulou E, Nowotny N, Ulbert S, Piralla A, Rovida F, Baldanti F, Percivalle E, and Palù G

Subjects

Amino Acid Substitution, Evolution, Molecular, Genome, Viral, Greece, Humans, Italy, Models, Molecular, Phylogeny, Phylogeography, Sequence Analysis, RNA, West Nile Fever transmission, Disease Outbreaks, RNA, Viral genetics, West Nile Fever epidemiology, West Nile virus classification, West Nile virus genetics

Abstract

In recent years, West Nile virus (WNV) lineage 2 has been spreading and causing disease outbreaks in humans and animals in Europe. In order to characterize viral diversity, we performed full-length genome sequencing of WNV lineage 2 from human samples collected during outbreaks in Italy and Greece in 2013 and 2014. Phylogenetic analysis showed that these WNV lineage 2 genomes belonged to a monophyletic clade derived from a single introduction into Europe of the prototype Hungarian strain. Correlation of phylogenetic data with geospatial information showed geographical clustering of WNV genome sequences both in Italy and in Greece, indicating that the virus had evolved and diverged during its dispersal in Europe, leading to the emergence of novel genotypes, as it adapted to local ecological niches. These genotypes carried divergent conserved amino acid substitutions, which might have been relevant for viral adaptation, as suggested by selection pressure analysis and in silico and experimental modelling of sequence changes. In conclusion, the results of this study provide further information on WNV lineage 2 transmission dynamics in Europe, and emphasize the need for WNV surveillance activities to monitor viral evolution and diversity., (Copyright © 2015 European Society of Clinical Microbiology and Infectious Diseases. Published by Elsevier Ltd. All rights reserved.)

Published

2015

6. Whole genome sequencing and phylogenetic analysis of West Nile virus lineage 1 and lineage 2 from human cases of infection, Italy, August 2013.

Author

Barzon L, Pacenti M, Franchin E, Lavezzo E, Masi G, Squarzon L, Pagni S, Toppo S, Russo F, Cattai M, Cusinato R, and Palu G

Subjects

Base Sequence, Disease Outbreaks, Genome, Humans, Italy epidemiology, Molecular Epidemiology, Phylogeny, West Nile Fever diagnosis, West Nile Fever epidemiology, West Nile Fever virology, RNA, Viral genetics, West Nile Fever genetics, West Nile virus classification, West Nile virus genetics

Abstract

A human outbreak of West Nile virus (WNV) infection caused by WNV lineage 2 is ongoing in northern Italy. Analysis of six WNV genome sequences obtained from clinical specimens demonstrated similarities with strains circulating in central Europe and Greece and the presence of unique amino acid changes that identify a new viral strain. In addition, WNV lineage 1 Livenza, responsible for a large outbreak in north-eastern Italy in 2012, was fully sequenced from a blood donor during this 2013 outbreak.

Published

2013

7. Novel West Nile virus lineage 1a full genome sequences from human cases of infection in north-eastern Italy, 2011.

Author

Barzon L, Pacenti M, Franchin E, Squarzon L, Lavezzo E, Toppo S, Martello T, Cattai M, Cusinato R, and Palù G

Subjects

Genetic Variation, Genotype, Humans, Italy, Molecular Sequence Data, Phylogeny, West Nile virus classification, West Nile virus isolation & purification, Genome, Viral, RNA, Viral genetics, Sequence Analysis, DNA, West Nile Fever virology, West Nile virus genetics

Abstract

During 2008-2009, several human cases of WNV disease caused by an endemic lineage 1a strain were reported in areas surrounding the Po river in north-eastern Italy. Since 2010, cases have been recorded in nearby northern areas, where, in 2011, both lineage 1a and 2 were detected. We describe here two new WNV complete genome sequences from human cases of WNV infection occurring in 2011 in the Veneto Region. Phylogenetic analysis showed that both genome sequences belonged to lineage 1a and were related to WNV strains of the Western Mediterranean subtype. The novel WNV genomes had high nucleotide and amino acid sequence divergence from each other and from the WNV strain circulating in Italy in 2008-2009. The presence of different WNV strains in a relatively small geographical area is a novel finding with unpredictable impact on human disease that requires further investigation., (© 2012 The Authors. Clinical Microbiology and Infection © 2012 European Society of Clinical Microbiology and Infectious Diseases.)

Published

2012

8. Clinical and virological findings in the ongoing outbreak of West Nile virus Livenza strain in northern Italy, July to September 2012.

Author

Barzon L, Pacenti M, Franchin E, Martello T, Lavezzo E, Squarzon L, Toppo S, Fiorin F, Marchiori G, Scotton GP, Russo F, Cattai M, Cusinato R, and Palù G

Subjects

Blood Donors, Follow-Up Studies, Humans, Italy epidemiology, Population Surveillance methods, Real-Time Polymerase Chain Reaction, Sequence Analysis, Viral Load, West Nile Fever epidemiology, West Nile Fever genetics, West Nile virus isolation & purification, Disease Outbreaks, RNA, Viral genetics, West Nile Fever virology, West Nile virus genetics

Abstract

In July-September 2012, one month earlier than in previous years, 13 confirmed human cases of West Nile virus infection were diagnosed in northern Italy, including five with neuroinvasive disease, three with West Nile fever, and five West Nile virus (WNV)-positive blood donors. In nine cases, the presence of the WNV lineage 1a Livenza strain, characterised in 2011, was ascertained. Symptomatic patients had prolonged viruria with high viral load.

Published

2012

9. New endemic West Nile virus lineage 1a in northern Italy, July 2012.

Author

Barzon L, Pacenti M, Franchin E, Lavezzo E, Martello T, Squarzon L, Toppo S, Fiorin F, Marchiori G, Russo F, Cattai M, Cusinato R, and Palu G

Subjects

Endemic Diseases, Humans, Italy epidemiology, Nucleic Acid Amplification Techniques, Phylogeny, Population Surveillance, Sequence Analysis, West Nile Fever epidemiology, West Nile Fever genetics, Blood Donors, RNA, Viral genetics, West Nile Fever virology, West Nile virus genetics

Abstract

We report here the first blood donation positive for West Nile virus (WNV) by nucleic acid amplification testing collected in north-eastern Italy in July 2012.Partial sequencing of the WNV RNA demonstrated identity with a WNV lineage 1a genome identified in the same area in 2011 and divergence from the strain responsible for the outbreak in northern Italy in 2008–09. These data indicate that WNV activity in northern Italy is occurring earlier than expected and that different WNV strains are circulating.

Published

2012

10. Both human immunodeficiency virus cellular DNA sequencing and plasma RNA sequencing are useful for detection of drug resistance mutations in blood samples from antiretroviral-drug-naive patients.

Author

Parisi SG, Boldrin C, Cruciani M, Nicolini G, Cerbaro I, Manfrin V, Dal Bello F, Franchin E, Franzetti M, Rossi MC, Cattelan AM, Romano L, Zazzi M, Andreoni M, and Palù G

Subjects

Adult, Anti-HIV Agents pharmacology, Anti-HIV Agents therapeutic use, DNA, Viral analysis, Female, HIV Infections virology, HIV-1 classification, HIV-1 genetics, Humans, Male, Microbial Sensitivity Tests methods, Middle Aged, RNA, Viral analysis, Sequence Analysis, DNA, Drug Resistance, Viral genetics, HIV Infections drug therapy, HIV-1 drug effects, Leukocytes, Mononuclear virology, Mutation, RNA, Viral blood

Abstract

Genotypic antiretroviral testing is recommended for newly infected drug-naive subjects, and the material of choice is plasma RNA. Since drug resistance mutations (DRMs) may persist longer in cellular DNA than in plasma RNA, we investigated whether the use of peripheral blood mononuclear cell (PBMC) human immunodeficiency virus (HIV) DNA increases the sensitivity of genotypic testing in antiretroviral-drug-naive subjects. We compared the rate of primary drug resistance in plasma RNA and PBMC DNA in 288 HIV type 1-infected drug-naive persons tested at a single clinical virology center from June 2004 to October 2006. Resistance in the plasma compartment to at least one drug was detected for 64 out of 288 (22.2%) naive patients and in the PBMC compartment for 56 (19.4%) patients. Overall, DRMs were found in 80 out of 288 (27.8%) patients. PBMC DNA [corrected] DRMs were present in [corrected] 16 subjects with wild-type virus in their plasma RNA [corrected] Another nine patients had additional DRMs in their PBMC DNA [corrected] with respect to those detected in their [corrected] plasma RNA. On the other hand, extra plasma RNA [corrected] DRMs were detected in [corrected] 24 and 8 subjects with wild-type and drug-resistant virus in their PBMC DNA [corrected] respectively. Resistance to more than one class of antiretroviral drug was detected by plasma and PBMC analysis for 25.0% and 36.2% of the subjects, respectively. Our data support the potential utility of genotypic resistance testing of PBMC DNA in conjunction with the currently recommended plasma RNA analysis.

Published

2007

11. Clinical and virological findings in the ongoing outbreak of West Nile virus Livenza strain in northern Italy, July to September 2012

Author

Barzon, L., Pacenti, M., Franchin, E., Martello, T., Lavezzo, E., Squarzon, L., Stefano Toppo, Fiorin, F., Marchiori, G., Scotton, G. P., Russo, F., Cattai, M., Cusinato, R., and Palù, G.

Subjects

Italy, Population Surveillance, Humans, RNA, Viral, Blood Donors, Viral Load, Real-Time Polymerase Chain Reaction, Sequence Analysis, West Nile virus, West Nile Fever, Disease Outbreaks, Follow-Up Studies

Abstract

In July-September 2012, one month earlier than in previous years, 13 confirmed human cases of West Nile virus infection were diagnosed in northern Italy, including five with neuroinvasive disease, three with West Nile fever, and five West Nile virus (WNV)-positive blood donors. In nine cases, the presence of the WNV lineage 1a Livenza strain, characterised in 2011, was ascertained. Symptomatic patients had prolonged viruria with high viral load.