Your search keyword '"Madonna, Elisabetta"' showing total 7 results

1. Retrospective analysis of acute HBV infections occurred in 1978–79 and 1994–95 in North-East Italy: increasing prevalence of BCP/pre-core mutants in sub-genotype D3

Author

Bruni, Roberto, Villano, Umbertina, Taffon, Stefania, Equestre, Michele, Madonna, Elisabetta, Chionne, Paola, Candido, Angela, Dettori, Stefano, Pisani, Giulio, Rapicetta, Maria, Bortolotti, Flavia, and Ciccaglione, Anna Rita

Published

2020

2. Hepatitis a virus genotypes and strains from an endemic area of Europe, Bulgaria 2012-2014.

Author

Bruni, Roberto, Taffon, Stefania, Equestre, Michele, Cella, Eleonora, Lo Presti, Alessandra, Costantino, Angela, Chionne, Paola, Madonna, Elisabetta, Golkocheva-Markova, Elitsa, Bankova, Diljana, Ciccozzi, Massimo, Teoharov, Pavel, and Ciccaglione, Anna Rita

Subjects

HEPATITIS A, GENOTYPES, COMMUNICABLE diseases, HEPATITIS A virus, ENTEROVIRUSES, EPIDEMICS, BIOLOGICAL evolution, HEPATITIS viruses, POLYMERASE chain reaction, VIRAL antibodies, CITY dwellers

Abstract

Background: Hepatitis A virus (HAV) infection is endemic in Eastern European and Balkan region countries. In 2012, Bulgaria showed the highest rate (67.13 cases per 100,000) in Europe. Nevertheless, HAV genotypes and strains circulating in this country have never been described. The present study reports the molecular characterization of HAV from 105 patients from Bulgaria.Methods: Anti-HAV IgM positive serum samples collected in 2012-2014 from different towns and villages in Bulgaria were analysed by nested RT-PCR, sequencing of the VP1/2A region and phylogenetic analysis; the results were analysed together with patient and geographical data.Results: Phylogenetic analysis revealed two main sequence groups corresponding to the IA (78/105, 74%) and IB (27/105, 26%) sub-genotypes. In the IA group, a major and a minor cluster were observed (62 and 16 sequences, respectively). Most sequences from the major cluster (44/62, 71%) belonged to either of two strains, termed "strain 1" and "strain 2", differing only for a single specific nucleotide; the remaining sequences (18/62, 29%) showed few (1 to 4) nucleotide variations respect to strain 1 and 2. Strain 2 is identical to the strain previously responsible for an outbreak in the Czech Republic in 2008 and a large multi-country European outbreak caused by contaminated mixed frozen berries in 2013. Most sequences of the IA minor cluster and the IB group were detected in large/medium centers (LMCs). Overall, sequences from the IA major cluster were more frequent in small centers (SCs), but strain 1 and strain 2 showed an opposite relative frequency in SCs and LMCs (strain 1 more frequent in SCs, strain 2 in LMCs).Conclusions: Genotype IA predominated in Bulgaria in 2012-2014 and phylogenetic analysis identified a major cluster of highly related or identical IA sequences, representing 59% of the analysed cases; these isolates were mostly detected in SCs, in which HAV shows higher endemicity than in LMCs. The distribution of viral sequences suggests the existence of some differences between the transmission routes in SCs and LMCs. Molecular characterization of an increased number of isolates from Bulgaria, regularly collected over time, will be useful to explore specific transmission routes and plan appropriate preventing measures. [ABSTRACT FROM AUTHOR]

Published

2017

3. Migration pattern of hepatitis A virus genotype IA in North-Central Tunisia.

Author

Beji-Hamza, Abir, Taffon, Stefania, Mhalla, Salma, Lo Presti, Alessandra, Equestre, Michele, Chionne, Paola, Madonna, Elisabetta, Cella, Eleonora, Bruni, Roberto, Ciccozzi, Massimo, Aouni, Mahjoub, and Ciccaglione, Anna Rita

Subjects

HEPATITIS A transmission, GENOTYPES, GENE flow, NUCLEOTIDE sequencing, REVERSE transcriptase polymerase chain reaction

Abstract

Background: Hepatitis A virus (HAV) epidemiology in Tunisia has changed from high to intermediate endemicity in the last decades. However, several outbreaks continue to occur. The last reported sequences from Tunisian HAV strains date back to 2006. In order to provide an updated overview of the strains currently circulating in Tunisia, a large-scale molecular analysis of samples from hepatitis A cases was performed, the first in Tunisia. Results: Biological samples were collected from patients with laboratory confirmed hepatitis A: 145 sera samples in Tunis, Monastir, Sousse and Kairouan from 2008 to 2013 and 45 stool samples in Mahdia in 2009. HAV isolates were characterised by nested RT-PCR (VP1/2A region) and sequencing. The sequences finally obtained from 81 samples showed 78 genotype IA and 3 genotype IB isolates. A Tunisian genotype IA sequence dataset, including both the 78 newly obtained IA sequences and 51 sequences retrieved from GenBank, was used for phylogenetic investigation, including analysis of migration pattern among six towns. Virus gene flow from Sfax and Monastir was directed to all other towns; in contrast, the gene flows from Sousse, Tunis, Mahdia and Kairouan were directed to three, two, one and no towns, respectively. Conclusions: Several different HAV strains co-circulate in Tunisia, but the predominant genotype still continues to be IA (78/81, 96% isolates). A complex gene flow (migration) of HAV genotype IA was observed, with Sfax and Monastir showing gene flows to all other investigated towns. This approach coupled to a wider sampling can prove useful to investigate the factors underlying the spread of HAV in Tunisia and, thus, to implement appropriate preventing measures. [ABSTRACT FROM AUTHOR]

Published

2015

4. Molecular characterisation of human hepatitis E virus from Italy: comparative analysis of five reverse transcription-PCR assays.

Author

Rosa, Giuseppina La, Fratini, Marta, Muscillo, Michele, Iaconelli, Marcello, Taffon, Stefania, Equestre, Michele, Chionne, Paola, Madonna, Elisabetta, Pisani, Giulio, Bruni, Roberto, and Ciccaglione, Anna Rita

Subjects

HEPATITIS E virus, REVERSE transcriptase polymerase chain reaction, GENETIC polymorphisms, IMMUNOGLOBULIN M, HEPATITIS, PUBLIC health

Abstract

Background Hepatitis E (HEV) is an important public-health concern as a major cause of enterically transmitted hepatitis worldwide. In industrialised countries it is considered rare, and largely confined to travellers returning from endemic areas. However, autochthonous (locally acquired) HEV infection is also emerging in these regions. The infection is caused by different genotypes, depending on whether it is travel-related or autochthonous. Conventional RT-PCR followed by sequencing of PCR products can identify HEV genotype and, depending on the region, the subtype, thus helping in defining the origin of infection and tracing the source of contamination. Methods We re-analysed a collection of serum samples previously confirmed as hepatitis E positive by anti-HEV IgM and IgG assays as well as by Real-Time PCR, with the aim to compare the performances of five different broad range RT-PCR assays that could be provided for molecular characterisation of HEV. This approach is certainly valuable to investigate the molecular epidemiology of acute hepatitis E in countries where co-circulation of different genotypes occurs, like Italy. Results Samples were analyzed by five assays targeting the ORF1, ORF2, and ORF2/3 regions. The sensitivity of these assays varied significantly, depending on the target region. Only 46% of samples tested positive by nested PCR; moreover, no single method was able to detect all positive samples. Most sequences originated from patients who had travelled to endemic areas (genotype 1), while the minority originated from Italian patients with no travel history (genotype 3). Conclusion Broad range methods for molecular characterization of HEV still need to be improved to detect all circulating strains. [ABSTRACT FROM AUTHOR]

Published

2014

5. Diagnosis of HEV infection by serological and real-time PCR assays: a study on acute non-A-C hepatitis collected from 2004 to 2010 in Italy.

Author

Candido, Angela, Taffon, Stefania, Chionne, Paola, Pisani, Giulio, Madonna, Elisabetta, Dettori, Stefano, Hamza, Abir, Valdarchi, Catia, Bruni, Roberto, and Ciccaglione, Anna Rita

Subjects

LIVER diseases, HEPATITIS, GENOMES, NUCLEIC acids, DEVELOPED countries

Abstract

Background: The impact of hepatitis E in developed countries, like Italy, still requires a clear definition. In the present study, we evaluated HEV infection in patients with acute non-A-C hepatitis by an approach comparing data from Real-time PCR and serological assays. Methods: In a first analysis, sera from 52 patients hospitalized with a diagnosis of acute viral non-A-C hepatitis in Italy were tested by in-house Real-Time PCR assay for identification of Hepatitis E Virus (HEV) RNA and by anti-HEV IgM and IgG assays. In a subsequent analysis, selected samples were evaluated by additional IgM tests to confirm diagnosis. Results: Among the 52 samples, 21 showed positive results for all three markers (IgM, IgG and HEV RNA). One patient showed HEV RNA as single marker. Uncertain results were found in 8 samples while the remaining 22 were negative for all markers. Further analysis of the 8 undefined samples by additional IgM tests confirmed HEV infection in 1 patient. Overall, acute HEV infections were reliably identified in 23 (44.2%) out of 52 patients. Conclusions: In the present paper, we performed a study evaluating HEV infection in 52 sporadic non-A-C acute hepatitis cases. All samples were collected from 2004 to 2010 in Italy. By a diagnostic strategy based on genomic and serological assays we identified HEV infections in 23 out of 52 patients (44.2%), a percentage higher than previous estimates. Thus, the actual impact of HEV infections in Italy needs to be further evaluated on a national scale by a diagnostic strategy based on multiple and last generation assays. [ABSTRACT FROM AUTHOR]

Published

2012

6. A cohort study to evaluate persistence of hepatitis B immunogenicity after administration of hexavalent vaccines.

Author

Giambi, Cristina, Bella, Antonino, Barale, Antonella, Montù, Domenico, Marchisio, Maria, Oddone, Maurizio, Zito, Salvatore, Rapicetta, Maria, Chionne, Paola, Madonna, Elisabetta, and Ciofi degli Atti, Marta L.

Subjects

HEPATITIS B, IMMUNOLOGY, HEPATITIS B vaccines, IMMUNIZATION of children, HEPATITIS B virus

Abstract

Background: In 2001, two hexavalent vaccines were licensed in Italy (Hexavac®, Infanrix Hexa®), and since 2002 were extensively used for primary immunization in the first year of life (at 3, 5, 11/12 months of age). In 2005, the market authorization of Hexavac® was precautionary suspended by EMEA, because of doubts on long-term protection against hepatitis B virus. The objectives of this study were to evaluate the persistence of antibodies to anti-HBs, in children in the third year of life, and to investigate the response to a booster dose of hepatitis B vaccine. Methods: Participant children were enrolled concomitantly with the offering of anti-polio booster dose, in the third year of life. Anti-HBs titers were determined on capillary blood samples. A booster dose of hepatitis B vaccine was administered to children with anti-HBs titers < 10 mIU/ml, with the monovalent precursor product of the previously received hexavalent vaccine. HBsAb titers were tested again one month after the booster. Results: Sera from 113 children previously vaccinated with Hexavac®, and from 124 vaccinated with Infanrix Hexa® were tested for anti-HBs. Titers were ≥ 10 mIU/ml in 69% and 96% (p < 0,0001) respectively. The proportion of children with titers ≥ 100 mIU/ml did also significantly differ among groups (27% and 78%; p < 0,0001). Post-booster, 93% of children achieved titers ≥ 10 mIU/ml, with no significant difference by vaccine group. Discussion: Fifteen months after third dose administration, a significant difference in anti-HBs titers was noted in the two vaccine groups considered. Monovalent hepatitis B vaccine administration in 3-year old children induced a proper booster response, confirming that immunologic memory persists in children with anti-HBs titers < 10 mIU/ml. However, long-term persistence of HBV protection after hexavalent vaccines administration should be further evaluated over time. [ABSTRACT FROM AUTHOR]

Published

2008

7. Molecular characterisation of human hepatitis E virus from Italy: comparative analysis of five reverse transcription-PCR assays.

Author

La Rosa G, Fratini M, Muscillo M, Iaconelli M, Taffon S, Equestre M, Chionne P, Madonna E, Pisani G, Bruni R, and Ciccaglione AR

Subjects

Hepatitis E epidemiology, Hepatitis E virus genetics, Humans, Italy epidemiology, Molecular Epidemiology methods, Molecular Sequence Data, RNA, Viral genetics, Sensitivity and Specificity, Sequence Analysis, DNA, Hepatitis E virology, Hepatitis E virus classification, Hepatitis E virus isolation & purification, Reverse Transcriptase Polymerase Chain Reaction methods

Abstract

Background: Hepatitis E (HEV) is an important public-health concern as a major cause of enterically transmitted hepatitis worldwide. In industrialised countries it is considered rare, and largely confined to travellers returning from endemic areas. However, autochthonous (locally acquired) HEV infection is also emerging in these regions. The infection is caused by different genotypes, depending on whether it is travel-related or autochthonous. Conventional RT-PCR followed by sequencing of PCR products can identify HEV genotype and, depending on the region, the subtype, thus helping in defining the origin of infection and tracing the source of contamination., Methods: We re-analysed a collection of serum samples previously confirmed as hepatitis E positive by anti-HEV IgM and IgG assays as well as by Real-Time PCR, with the aim to compare the performances of five different broad range RT-PCR assays that could be provided for molecular characterisation of HEV. This approach is certainly valuable to investigate the molecular epidemiology of acute hepatitis E in countries where co-circulation of different genotypes occurs, like Italy., Results: Samples were analyzed by five assays targeting the ORF1, ORF2, and ORF2/3 regions. The sensitivity of these assays varied significantly, depending on the target region. Only 46% of samples tested positive by nested PCR; moreover, no single method was able to detect all positive samples. Most sequences originated from patients who had travelled to endemic areas (genotype 1), while the minority originated from Italian patients with no travel history (genotype 3)., Conclusion: Broad range methods for molecular characterization of HEV still need to be improved to detect all circulating strains.

Published

2014