Your search keyword '"Piu, Pietro"' showing total 6 results

1. Characterization of Enzyme-Linked Immunosorbent Assay (ELISA) for Quantification of Antibodies against Salmonella Typhimurium and Salmonella Enteritidis O-Antigens in Human Sera.

Author

Aruta, Maria Grazia, Lari, Elisa, De Simone, Daniele, Semplici, Bianca, Semplici, Claudia, Dale, Helen, Chirwa, Esmelda, Kadwala, Innocent, Mbewe, Maurice, Banda, Happy, Iturriza-Gomara, Miren, Gordon, Melita, Nyirenda, Tonney, Piu, Pietro, Pizza, Mariagrazia, Berlanda Scorza, Francesco, Grappi, Silvia, Canals, Rocío, and Rossi, Omar

Subjects

SALMONELLA typhimurium, ENZYME-linked immunosorbent assay, SALMONELLA enteritidis, IMMUNOGLOBULINS, VACCINE trials, VACCINE immunogenicity

Abstract

Nontyphoidal Salmonella (NTS) is a leading cause of morbidity and mortality caused by enteric pathogens worldwide in both children and adults, and vaccines are not yet available. The measurement of antigen-specific antibodies in the sera of vaccinated or convalescent individuals is crucial to understand the incidence of disease and the immunogenicity of vaccine candidates. A solid and standardized assay used to determine the level of specific anti-antigens IgG is therefore of paramount importance. In this work, we presented the characterization of a customized enzyme-linked immunosorbent assay (ELISA) with continuous readouts and a standardized definition of EU/mL. We assessed various performance parameters: standard curve accuracy, dilutional linearity, intermediate precision, specificity, limits of blanks, and quantification. The simplicity of the assay, its high sensitivity and specificity coupled with its low cost and the use of basic consumables and instruments without the need of high automation makes it suitable for transfer and application to different laboratories, including resource-limiting settings where the disease is endemic. This ELISA is, therefore, fit for purpose to be used for quantification of antibodies against Salmonella Typhimurium and Salmonella Enteritidis O-antigens in human samples, both for vaccine clinical trials and large sero-epidemiological studies. [ABSTRACT FROM AUTHOR]

Published

2023

2. Characterisation of SARS-CoV-2 Lentiviral Pseudotypes and Correlation between Pseudotype-Based Neutralisation Assays and Live Virus-Based Micro Neutralisation Assays

Author

Hyseni, Inesa, Molesti, Eleonora, Benincasa, Linda, Piu, Pietro, Casa, Elisa, Temperton, Nigel J., Manenti, Alessandro, Montomoli, Emanuele, Hyseni, Inesa, Molesti, Eleonora, Benincasa, Linda, Piu, Pietro, Casa, Elisa, Temperton, Nigel J., Manenti, Alessandro, and Montomoli, Emanuele

Abstract

The recent outbreak of a novel Coronavirus (SARS-CoV-2) and its rapid spread across the continents has generated an urgent need for assays to detect the neutralising activity of human sera or human monoclonal antibodies against SARS-CoV-2 spike protein and to evaluate the serological immunity in humans. Since the accessibility of live virus microneutralisation (MN) assays with SARS-CoV-2 is limited and requires enhanced bio-containment, the approach based on "pseudotyping" can be considered a useful complement to other serological assays. After fully characterising lentiviral pseudotypes bearing the SARS-CoV-2 spike protein, we employed them in pseudotype-based neutralisation assays in order to profile the neutralising activity of human serum samples from an Italian sero-epidemiological study. The results obtained with pseudotype-based neutralisation assays mirrored those obtained when the same panel of sera was tested against the wild type virus, showing an evident convergence of the pseudotype-based neutralisation and MN results. The overall results lead to the conclusion that the pseudotype-based neutralisation assay is a valid alternative to using the wild-type strain, and although this system needs to be optimised and standardised, it can not only complement the classical serological methods, but also allows serological assessments to be made when other methods cannot be employed, especially in a human pandemic context.

Published

2020

3. Influenza D Virus: A Potential Threat for Humans?

Author

Trombetta, Claudia Maria, primary, Marchi, Serena, additional, Manini, Ilaria, additional, Kistner, Otfried, additional, Li, Feng, additional, Piu, Pietro, additional, Manenti, Alessandro, additional, Biuso, Fabrizio, additional, Sreenivasan, Chithra, additional, Druce, Julian, additional, and Montomoli, Emanuele, additional

Published

2020

4. Effect of Repeated Freeze–Thaw Cycles on Influenza Virus Antibodies.

Author

Torelli, Alessandro, Gianchecchi, Elena, Monti, Martina, Piu, Pietro, Barneschi, Irene, Bonifazi, Carolina, Coluccio, Rosa, Ganfini, Luisa, Magra, Luciano Michele La, Marconi, Silvia, Marzucchi, Ginevra, Pace, Ramona, Palladino, Laura, Biagi, Bernardo, Montomoli, Emanuele, and Tripp, Ralph A.

Subjects

VIRAL antibodies, FREEZE-thaw cycles, INFLUENZA A virus, INFLUENZA viruses, VACCINE effectiveness

Abstract

Background: Vaccine effectiveness relies on various serological tests, whose aim is the measurement of antibody titer in serum samples collected during clinical trials before and after vaccination. Among the serological assays required by the regulatory authorities to grant influenza vaccine release there are: Hemagglutination inhibition (HAI), microneutralization (MN), and Single Radial Hemolysis (SRH). Although antibodies are regarded to be relatively stable, limited evidences on the effect of multiple freeze–thaw cycles on the stability of antibodies in frozen serum samples are available so far. In view of this, the present paper aimed to evaluate the impact of multiple freeze–thaw cycles on influenza antibody stability, performing HAI, MN and SRH assays. Methods: Ten serum samples were divided into 14 aliquots each, stored at −20 °C and taken through a total of 14 freeze–thaw cycles to assess influenza antibody stability. Each assay measurement was carried out following internal procedures based on World Health Organization (WHO) guidelines. Results: No statistically significant effect of 14 freeze–thaw cycles on antibody stability, measured through three different assays, was observed. Conclusions: Collectively, these data demonstrated that specific influenza antibody present in serum samples are stable up to 14 freeze–thaw cycles. [ABSTRACT FROM AUTHOR]

Published

2021

5. Serologically-Based Evaluation of Cross-Protection Antibody Responses among Different A(H1N1) Influenza Strains.

Author

Marchi, Serena, Manini, Ilaria, Kistner, Otfried, Piu, Pietro, Remarque, Edmond J., Manenti, Alessandro, Biuso, Fabrizio, Carli, Tommaso, Lazzeri, Giacomo, Montomoli, Emanuele, and Trombetta, Claudia Maria

Subjects

INFLUENZA A virus, H1N1 subtype, ANTIBODY formation, INFLUENZA vaccines, INFLUENZA, SEASONAL influenza

Abstract

After the influenza H1N1 pandemic of 2009, the seasonal A/Brisbane/59/2007 strain was replaced by the A/California/07/2009 strain for the influenza virus vaccine composition. After several seasons with no indications on the occurrence of antigenic drift, A/Michigan/45/2015 was chosen as the H1N1 vaccine strain for the 2017/2018 season. Since the immune response to influenza is shaped by the history of exposure to antigenically similar strains, the potential cross-protection between seasonal human influenza vaccine strains and the emerging pandemic strains was investigated. Human serum samples were tested by hemagglutination inhibition and single radial hemolysis assays against A/Brisbane/59/2007, A/California/07/2009, and A/Michigan/45/2015 strains. Strong cross-reactions between A/California/07/2009 and A/Michigan/45/2015 strains were observed in 2009/2010, most likely induced by the start of the 2009 pandemic, and the subsequent post-pandemic seasons from 2010/2011 onward when A/California/07/2009 became the predominant strain. In the 2014/2015 season, population immunity against A/California/07/2009 and A/Michigan/45/2015 strains increased again, associated with strong cross-reactions. Whereas hemagglutination inhibition assay has a higher sensitivity for detection of new seasonal drift, the single radial hemolysis assay is an excellent tool for determining the presence of pre-existing immunity, allowing a potential prediction on the booster potential of influenza vaccines against newly emerging drifted strains. [ABSTRACT FROM AUTHOR]

Published

2020

6. Influenza D Virus: Serological Evidence in the Italian Population from 2005 to 2017.

Author

Trombetta, Claudia M., Marchi, Serena, Manini, Ilaria, Kistner, Otfried, Li, Feng, Piu, Pietro, Manenti, Alessandro, Biuso, Fabrizio, Sreenivasan, Chithra, Druce, Julian, and Montomoli, Emanuele

Subjects

SENDAI virus, VETERINARY epidemiology, INFLUENZA viruses, POPULATION

Abstract

Influenza D virus is a novel influenza virus, which was first isolated from an ailing swine in 2011 and later detected in cattle, suggesting that these animals may be a primary natural reservoir. To date, few studies have been performed on human samples and there is no conclusive evidence on the ability of the virus to infect humans. The aim of this serological study was to assess the prevalence of antibodies against influenza D virus in human serum samples collected in Italy from 2005 to 2017. Serum samples were analysed by haemagglutination inhibition and virus neutralization assays. The results showed that the prevalence of antibodies against the virus increased in the human population in Italy from 2005 to 2017, with a trend characterized by a sharp increase in some years, followed by a decline in subsequent years. The virus showed the ability to infect and elicit an immune response in humans. However, prevalence peaks in humans appear to follow epidemics in animals and not to persist in the human population. [ABSTRACT FROM AUTHOR]

Published

2020