Your search keyword '"Orsini, Paola"' showing total 6 results

1. Design and MinION testing of a nanopore targeted gene sequencing panel for chronic lymphocytic leukemia.

Author

Orsini P, Minervini CF, Cumbo C, Anelli L, Zagaria A, Minervini A, Coccaro N, Tota G, Casieri P, Impera L, Parciante E, Brunetti C, Giordano A, Specchia G, and Albano F

Subjects

Aged, DNA Mutational Analysis instrumentation, DNA Mutational Analysis methods, Female, Humans, Male, Middle Aged, Leukemia, Lymphocytic, Chronic, B-Cell genetics, Nanopores, Neoplasm Proteins genetics

Abstract

We report a customized gene panel assay based on multiplex long-PCR followed by third generation sequencing on nanopore technology (MinION), designed to analyze five frequently mutated genes in chronic lymphocytic leukemia (CLL): TP53, NOTCH1, BIRC3, SF3B1 and MYD88. For this purpose, 12 patients were selected according to specific cytogenetic and molecular features significantly associated with their mutational status. In addition, simultaneous analysis of the targets genes was performed by molecular assays or Sanger Sequencing. Data analysis included mapping to the GRCh37 human reference genome, variant calling and annotation, and average sequencing depth/error rate analysis. The sequencing depth resulted on average higher for smaller amplicons, and the final breadth of coverage of the panel was 94.1%. The error rate was about 6% and 2% for insertions/deletions and single nucleotide variants, respectively. Our gene panel allows analysis of the prognostically relevant genes in CLL, with two PCRs per patient. This strategy offers an easy and affordable workflow, although further advances are required to improve the accuracy of the technology and its use in the clinical field. Nevertheless, the rapid and constant development of nanopore technology, in terms of chemistry advances, more accurate basecallers and analysis software, offers promise for a wide use of MinION in the future.

Published

2018

2. Nanopore sequencing approach for immunoglobulin gene analysis in chronic lymphocytic leukemia.

Author

Minervini, Crescenzio Francesco, Cumbo, Cosimo, Redavid, Immacolata, Conserva, Maria Rosa, Orsini, Paola, Zagaria, Antonella, Anelli, Luisa, Coccaro, Nicoletta, Tota, Giuseppina, Impera, Luciana, Parciante, Elisa, Tarantini, Francesco, Giordano, Annamaria, Specchia, Giorgina, Musto, Pellegrino, and Albano, Francesco

Subjects

NANOPORES, IMMUNOGLOBULINS, CHRONIC lymphocytic leukemia, DATA analysis, THERAPEUTICS

Abstract

The evaluation of the somatic hypermutation of the clonotypic immunoglobulin heavy variable gene has become essential in the therapeutic management in chronic lymphocytic leukemia patients. European Research Initiative on Chronic Lymphocytic Leukemia promotes good practices and standardized approaches to this assay but often they are labor-intensive, technically complex, with limited in scalability. The use of next-generation sequencing in this analysis has been widely tested, showing comparable accuracy and distinct advantages. However, the adoption of the next generation sequencing requires a high sample number (run batching) to be economically convenient, which could lead to a longer turnaround time. Here we present data from nanopore sequencing for the somatic hypermutation evaluation compared to the standard method. Our results show that nanopore sequencing is suitable for immunoglobulin heavy variable gene mutational analysis in terms of sensitivity, accuracy, simplicity of analysis and is less time-consuming. Moreover, our work showed that the development of an appropriate data analysis pipeline could lower the nanopore sequencing error rate attitude. [ABSTRACT FROM AUTHOR]

Published

2021

3. Nanopore Sequencing in Blood Diseases: A Wide Range of Opportunities.

Author

Minervini, Crescenzio Francesco, Cumbo, Cosimo, Orsini, Paola, Anelli, Luisa, Zagaria, Antonella, Specchia, Giorgina, and Albano, Francesco

Subjects

BLOOD diseases, NANOPORES, PATHOLOGY, NUCLEOTIDE sequencing, INDIVIDUALIZED medicine

Abstract

The molecular pathogenesis of hematological diseases is often driven by genetic and epigenetic alterations. Next-generation sequencing has considerably increased our genomic knowledge of these disorders becoming ever more widespread in clinical practice. In 2012 Oxford Nanopore Technologies (ONT) released the MinION, the first long-read nanopore-based sequencer, overcoming the main limits of short-reads sequences generation. In the last years, several nanopore sequencing approaches have been performed in various "-omic" sciences; this review focuses on the challenge to introduce ONT devices in the hematological field, showing advantages, disadvantages and future perspectives of this technology in the precision medicine era. [ABSTRACT FROM AUTHOR]

Published

2020

4. TP53 gene mutation analysis in chronic lymphocytic leukemia by nanopore MinION sequencing.

Author

Minervini, Crescenzio Francesco, Cumbo, Cosimo, Orsini, Paola, Brunetti, Claudia, Anelli, Luisa, Zagaria, Antonella, Minervini, Angela, Casieri, Paola, Coccaro, Nicoletta, Tota, Giuseppina, Impera, Luciana, Giordano, Annamaria, Specchia, Giorgina, and Albano, Francesco

Subjects

P53 protein, CHRONIC lymphocytic leukemia, PROTEIN expression, GENE expression, GENETIC mutation, NANOPORES

Abstract

Background: The assessment of TP53 mutational status is becoming a routine clinical practice for chronic lymphocytic leukemia patients (CLL). A broad spectrum of molecular techniques has been employed so far, including both direct Sanger sequencing and next generation sequencing. Oxford Nanopore Technologies recently released the MinION an USB-interfaced sequencer. In this paper we report our experience, with the MinION technology for the detection of the TP53 gene mutation in CLL patients. Twelve CLL patients at diagnosis were included in this study. All except one patient showed the TP53 gene deletion in Fluorescence in situ hybridization experiments. Patients were investigated for TP53 mutation by Sanger and by MinION sequencing. Analysis by Sanger was performed according with the IARC protocol. Analysis by MinION was performed adopting a strategy based on long template PCR, read error correction, and post variant calling filtering. Results: Due to the high error rate of nanopore technology, sequence data were both used directly and before correction with two different in silico methods: ALEC and nanocorrect. A mean error rate of 15 % was detected before correction that was reduced to 4-5 % after correction. Analysis by Sanger sequencing was able to detect four patients mutated for TP53. MinION analysis detected one more mutated patient previously not detected from Sanger. Conclusion: In our hands, the Nanopore technology shows correlation with Sanger sequencing but more sensitive, manageable and less expensive, and therefore has proven to be a useful tool for TP53 gene mutation detection. [ABSTRACT FROM AUTHOR]

Published

2016

5. Nanopore Targeted Sequencing for Rapid Gene Mutations Detection in Acute Myeloid Leukemia.

Author

Cumbo, Cosimo, Minervini, Crescenzio Francesco, Orsini, Paola, Anelli, Luisa, Zagaria, Antonella, Minervini, Angela, Coccaro, Nicoletta, Impera, Luciana, Tota, Giuseppina, Parciante, Elisa, Conserva, Maria Rosa, Spinelli, Orietta, Rambaldi, Alessandro, Specchia, Giorgina, and Albano, Francesco

Subjects

NANOPORES, ACUTE myeloid leukemia, MOLECULAR biology, GENES, SEQUENCE analysis

Abstract

Acute myeloid leukemia (AML) clinical settings cannot do without molecular testing to confirm or rule out predictive biomarkers for prognostic stratification, in order to initiate or withhold targeted therapy. Next generation sequencing offers the advantage of the simultaneous investigation of numerous genes, but these methods remain expensive and time consuming. In this context, we present a nanopore-based assay for rapid (24 h) sequencing of six genes (NPM1, FLT3, CEBPA, TP53, IDH1 and IDH2) that are recurrently mutated in AML. The study included 22 AML patients at diagnosis; all data were compared with the results of S5 sequencing, and discordant variants were validated by Sanger sequencing. Nanopore approach showed substantial advantages in terms of speed and low cost. Furthermore, the ability to generate long reads allows a more accurate detection of longer FLT3 internal tandem duplications and phasing double CEBPA mutations. In conclusion, we propose a cheap, rapid workflow that can potentially enable all basic molecular biology laboratories to perform detailed targeted gene sequencing analysis in AML patients, in order to define their prognosis and the appropriate treatment. [ABSTRACT FROM AUTHOR]

Published

2019

6. Mutational analysis in BCR-ABL1 positive leukemia by deep sequencing based on nanopore MinION technology.

Author

Minervini, Crescenzio F., Cumbo, Cosimo, Orsini, Paola, Anelli, Luisa, Zagaria, Antonella, Impera, Luciana, Coccaro, Nicoletta, Brunetti, Claudia, Minervini, Angela, Casieri, Paola, Tota, Giuseppina, Russo Rossi, Antonella, Specchia, Giorgina, and Albano, Francesco

Subjects

*GENETIC mutation, *LEUKEMIA, *PRELEUKEMIA, *NANOPORES, LEUKEMIA genetics

Abstract

We report a third-generation sequencing assay on nanopore technology (MinION) for detecting BCR - ABL1 KD mutations and compare the results to a Sanger sequencing(SS)-based test in 24 Philadelphia-positive (Ph +) leukemia cases. Our data indicates that MinION is markedly superior to SS in terms of sensitivity, costs and timesaving, and has the added advantage of determining the clonal configuration of multiple mutations. We demonstrate that MinION is suitable for employment in the hematology laboratory for detecting BCR - ABL1 KD mutation in Ph + leukemias. [ABSTRACT FROM AUTHOR]

Published

2017