Your search keyword '"Amato, Felice"' showing total 19 results

1. GENOTYPE PREDICTS THE RESPONSE TO THERAPY IN CHILDREN WITH CONGENITAL CHLORIDE DIARRHEA

Author

G. Terrin, AMATO, FELICE, P. Heinz Erian, G. Cardillo, R. Cacace, M. G. Martin, R. Tomaiuolo, A. Passariello, G. Castaldo, R. Troncone, BERNI CANANI, ROBERTO, Terrin, G., Amato, Felice, Heinz Erian, P., Cardillo, G., Cacace, R., Martin, M. G., Tomaiuolo, R., Passariello, A., Castaldo, G., Troncone, R., and BERNI CANANI, Roberto

Published

2010

2. Corrigendum: Age-Related Differences in the Expression of Most Relevant Mediators of SARS-CoV-2 Infection in Human Respiratory and Gastrointestinal Tract

Author

Roberto Berni Canani, Marika Comegna, Lorella Paparo, Gustavo Cernera, Cristina Bruno, Caterina Strisciuglio, Immacolata Zollo, Antonietta Gerarda Gravina, Erasmo Miele, Elena Cantone, Nicola Gennarelli, Rita Nocerino, Laura Carucci, Veronica Giglio, Felice Amato, Giuseppe Castaldo, Berni Canani, Roberto, Comegna, Marika, Paparo, Lorella, Cernera, Gustavo, Bruno, Cristina, Strisciuglio, Caterina, Zollo, Immacolata, Gravina, Antonietta Gerarda, Miele, Erasmo, Cantone, Elena, Gennarelli, Nicola, Nocerino, Rita, Carucci, Laura, Giglio, Veronica, Amato, Felice, and Castaldo, Giuseppe

Subjects

neuropilin-1, angiotensin-converting enzyme 2, transmembrane serine protease-2, healthy subjects, Pediatrics, Perinatology and Child Health, COVID-19, healthy subject, Pediatrics, RJ1-570

Abstract

[This corrects the article DOI: 10.3389/fped.2021.697390.].

Published

2021

3. Cystic Fibrosis Patients with F508del/Minimal Function Genotype: Laboratory and Nutritional Evaluations after One Year of Elexacaftor/Tezacaftor/Ivacaftor Treatment

Author

Vincenzo Carnovale, Filippo Scialò, Monica Gelzo, Paola Iacotucci, Felice Amato, Federica Zarrilli, Assunta Celardo, Giuseppe Castaldo, Gaetano Corso, Carnovale, Vincenzo, Scialò, Filippo, Gelzo, Monica, Iacotucci, Paola, Amato, Felice, Zarrilli, Federica, Celardo, Assunta, Castaldo, Giuseppe, Corso, Gaetano, Carnovale, V., Scialo, F., Gelzo, M., Iacotucci, P., Amato, F., Zarrilli, F., Celardo, A., Castaldo, G., and Corso, G.

Subjects

lipid profile, inflammation, protein metabolism, General Medicine, cystic fibrosis, CFTR modulators, cystic fibrosi, CFTR modulator

Abstract

The last ten years have been characterized by an enormous step forward in the therapy and management of patients with Cystic Fibrosis (CF), thanks to the development and combination of Cystic Fibrosis Transmembrane Receptor (CFTR) correctors and potentiators. Specifically, the last approved triple combination elexacaftor/tezacaftor/ivacaftor has been demonstrated to improve lung function in CF patients with both homozygous Phe508del and Phe508del/minimal function genotypes. Here we have assessed the effect of elexacaftor/tezacaftor/ivacaftor in patients carrying the Phe508del/minimal function genotype (n = 20) after one year of treatments on liver function and nutrient absorption with a focus on lipid metabolism. We show that weight, BMI, and albumin significantly increase, suggesting a positive impact of the treatment on nutrient absorption. Furthermore, cholesterol levels as a biomarker of lipid metabolism increased significantly after one year of treatment. Most importantly, we suggest that these results were not dependent on the diet composition, possibly indicating that the drug improves the hepatic synthesis and secretion of proteins and cholesterol.

Published

2022

4. Age-Related Differences in the Expression of Most Relevant Mediators of SARS-CoV-2 Infection in Human Respiratory and Gastrointestinal Tract

Author

Roberto Berni Canani, Marika Comegna, Lorella Paparo, Gustavo Cernera, Cristina Bruno, Caterina Strisciuglio, Immacolata Zollo, Antonietta Gerarda Gravina, Erasmo Miele, Elena Cantone, Nicola Gennarelli, Rita Nocerino, Laura Carucci, Veronica Giglio, Felice Amato, Giuseppe Castaldo, Berni Canani, R., Comegna, M., Paparo, L., Cernera, G., Bruno, C., Strisciuglio, C., Zollo, I., Gravina, A. G., Miele, E., Cantone, E., Gennarelli, N., Nocerino, R., Carucci, L., Giglio, V., Amato, F., Castaldo, G., Berni Canani, Roberto, Comegna, Marika, Paparo, Lorella, Cernera, Gustavo, Bruno, Cristina, Strisciuglio, Caterina, Zollo, Immacolata, Gravina, Antonietta Gerarda, Miele, Erasmo, Cantone, Elena, Gennarelli, Nicola, Nocerino, Rita, Carucci, Laura, Giglio, Veronica, Amato, Felice, and Castaldo, Giuseppe

Subjects

0301 basic medicine, transmembrane serine protease-2, healthy subject, Pediatrics, TMPRSS2, RJ1-570, Virus, 03 medical and health sciences, 0302 clinical medicine, angiotensin-converting enzyme 2, Medicine, 030212 general & internal medicine, Respiratory system, Gastrointestinal tract, business.industry, Correction, COVID-19, Brief Research Report, Small intestine, neuropilin-1, 030104 developmental biology, medicine.anatomical_structure, Expression (architecture), healthy subjects, Pediatrics, Perinatology and Child Health, Immunology, Angiotensin-converting enzyme 2, business, Respiratory tract

Abstract

Background: Clinical features of severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) infection seem to differ in children compared to that in adults. It has been hypothesized that the lower clinical severity in children could be influenced by differential expression of the main host functional receptor to SARS-CoV-2, the angiotensin-converting enzyme 2 (ACE2), but data are still conflicting. To explore the origin of age-dependent clinical features of coronavirus disease 2019 (COVID-19), we comparatively evaluated the expression in children and adult subjects of the most relevant mediators of the SARS-CoV-2 infection: ACE2, angiotensin-converting enzyme 1 (ACE1), transmembrane serine protease-2 (TMPRSS2), and neuropilin-1 (NRP1), at upper respiratory tract and small intestine level.Methods: The expression of ACE2, ACE1, TMPRSS2, and NRP1 in nasal epithelium and in small intestine epithelium was investigated by quantitative real-time PCR analysis.Results: We found no differences in ACE2, ACE1, and TMPRSS2 expression in the nasal epithelium comparing children and adult subjects. In contrast, nasal epithelium NRP1 expression was lower in children compared to that in adults. Intestinal ACE2 expression was higher in children compared to that in adults, whereas intestinal ACE1 expression was higher in adults. Intestinal TMPRSS2 and NRP1 expression was similar comparing children and adult subjects.Conclusions: The lower severity of SARS-CoV-2 infection observed in children may be due to a different expression of nasal NRP1, that promotes the virus interaction with ACE2. However, the common findings of intestinal symptoms in children could be due to a higher expression of ACE2 at this level. The insights from these data will be useful in determining the treatment policies and preventive measures for COVID-19.

Published

2021

5. Lung Microbiome in Cystic Fibrosis

Author

Monica Gelzo, Giuseppe Castaldo, Andrea Bianco, Federica Zarrilli, Lucio Pastore, Marika Comegna, Gustavo Cernera, Felice Amato, Filippo Scialò, Scialo, Filippo, Amato, Felice, Cernera, Gustavo, Gelzo, Monica, Zarrilli, Federica, Comegna, Marika, Pastore, Lucio, Bianco, Andrea, Castaldo, Giuseppe, Scialo, F., Amato, F., Cernera, G., Gelzo, M., Zarrilli, F., Comegna, M., Pastore, L., Bianco, A., and Castaldo, G.

Subjects

0301 basic medicine, Lung microbiome, Mucociliary clearance, microbiome, Disease, Respiratory physiology, Review, Cystic fibrosis, General Biochemistry, Genetics and Molecular Biology, lung, cystic fibrosis, 03 medical and health sciences, 0302 clinical medicine, Medicine, In patient, Microbiome, CFTR, lcsh:Science, Ecology, Evolution, Behavior and Systematics, cystic fibrosi, Lung, business.industry, Paleontology, respiratory system, medicine.disease, respiratory tract diseases, 030104 developmental biology, medicine.anatomical_structure, 030228 respiratory system, Space and Planetary Science, Immunology, lcsh:Q, business

Abstract

The defective mucociliary clearance due to CFTR malfunctioning causes predisposition to the colonization of pathogens responsible for the recurrent inflammation and rapid deterioration of lung function in patients with cystic fibrosis (CF). This has also a profound effect on the lung microbiome composition, causing a progressive reduction in its diversity, which has become a common characteristic of patients affected by CF. Although we know that the lung microbiome plays an essential role in maintaining lung physiology, our comprehension of how the microbial components interact with each other and the lung, as well as how these interactions change during the disease’s course, is still at an early stage. Many challenges exist and many questions still to be answered, but there is no doubt that manipulation of the lung microbiome could help to develop better therapies for people affected by CF.

Published

2020

6. Butyrate modulating effects on pro-inflammatory pathways in human intestinal epithelial cells

Author

Giuseppe Castaldo, Antonio Calignano, Ausilia Elce, Felice Amato, Roberto Berni Canani, Riccardo Troncone, Federica Zarrilli, Elce, A., Amato, Felice, Zarrilli, F., Calignano, Antonio, Troncone, Riccardo, Castaldo, Giuseppe, and BERNI CANANI, Roberto

Subjects

0301 basic medicine, Microbiology (medical), inflammation, membrane carrier, short chain fatty acids, Colon, Anti-Inflammatory Agents, Inflammation, Butyrate, Real-Time Polymerase Chain Reaction, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Immune system, Mediator, Intestine, Small, Gene expression, medicine, Humans, Immunologic Factors, inflammation, membrane carrier, short chain fatty acids, Receptor, Cells, Cultured, biology, Gene Expression Profiling, Epithelial Cells, Molecular biology, Cell biology, Butyrates, 030104 developmental biology, Histone, biology.protein, 030211 gastroenterology & hepatology, medicine.symptom, Energy source

Abstract

Butyrate acts as energy source for intestinal epithelial cells and as key mediator of several immune processes, modulating gene expression mainly through histone deacetylation inhibition. Thanks to these effects, butyrate has been proposed for the treatment of many intestinal diseases. Aim of this study was to investigate the effect of butyrate on the expression of a large series of target genes encoding proteins involved in pro-inflammatory pathways. We performed quantitative real-time-PCR analysis of the expression of 86 genes encoding proteins bearing to pro-inflammatory pathways, before and after butyrate exposure, in primary epithelial cells derived from human small intestine and colon. Butyrate significantly down-regulated the expression of genes involved in inflammatory response, among which nuclear factor kappa beta, interferon-gamma, Toll like 2 receptor and tumour necrosis factor-alpha. Further confirmations of these data, including studies at protein level, would support the use of butyrate as effective therapeutic strategy in intestinal inflammatory disorders.

Published

2017

7. Twelve Novel Mutations in the SLC26A3 Gene in 17 Sporadic Cases of Congenital Chloride Diarrhea

Author

Sabrina Cardile, Vincenza Pezzella, Licia Lugli, Giuseppe Castaldo, Ausilia Elce, Roberto Berni Canani, Sonia Giordano, Manuela Scorza, Marika Comegna, Claudio Romano, Renato Liguori, Giuseppe Cardillo, Laura Lucaccioni, Felice Amato, Amato, Felice, Cardillo, Giuseppe, Liguori, Renato, Scorza, Manuela, Comegna, Marika, Elce, Ausilia, Giordano, Sonia, Lucaccioni, Laura, Lugli, Licia, Cardile, Sabrina, Romano, Claudio, Pezzella, Vincenza, Castaldo, Giuseppe, and BERNI CANANI, Roberto

Subjects

Diarrhea, Genetic Markers, 0301 basic medicine, Genotype, Genotyping Techniques, Congenital chloride diarrhea, In silico, SLC26A3, 03 medical and health sciences, 0302 clinical medicine, medicine, Humans, Missense mutation, Chloride-Bicarbonate Antiporters, Genetic Testing, Gene, Genetics, biology, Gastroenterology, medicine.disease, 030104 developmental biology, Sulfate Transporters, Case-Control Studies, Mutation, chloride losing diarrhea, diarrhea anion exchanger, genotype, member 3 of solute carrier family 26, mutations, splicing effect, Metabolism, Inborn Errors, Pediatrics, Perinatology and Child Health, RNA splicing, biology.protein, Gastroenterology, chloride losing diarrhea, diarrhea anion exchanger, mutations, SLC26A3, splicing effect, 030211 gastroenterology & hepatology, Minigene

Abstract

Objectives: We aimed to improve the knowledge of pathogenic mutations in sporadic cases of congenital chloride diarrhea (CCD) and emphasize the importance of functional studies to define the effect of novel mutations. Methods: All member 3 of solute carrier family 26 (SLC26A3) coding regions were sequenced in 17 sporadic patients with CCD. Moreover, the minigene system was used to analyze the effect of 2 novel splicing mutations. Results: We defined the SLC26A3 genotype of all 17 patients with CDD and identified 12 novel mutations. Using the minigene system, we confirmed the in silico prediction of a complete disruption of splicing pattern caused by 2 of these novel mutations: the c.971þ3_971þ4delAA and c.735þ4_c.735þ7delAGTA. Moreover, several prediction tools and a structure-function prediction defined the pathogenic role of 6 novel missense mutations. Conclusions: We confirm the molecular heterogeneity of sporadic CDD adding 12 novel mutations to the list of known pathogenic mutations. Moreover, we underline the importance, for laboratories that offer molecular diagnosis and genetic counseling, to perform fast functional analysis of novel mutations

Published

2017

8. Genotype–phenotype correlation and functional studies in patients with cystic fibrosis bearing CFTR complex alleles

Author

Giuseppe Castaldo, Ausilia Elce, Natalia Cirilli, Marika Comegna, Antonella Miriam Di Lullo, Manuela Scorza, Adriano Angioni, Valeria Raia, Paola Iacotucci, Valentina Maria Sofia, Anna Perfetti, Roberta Cimino, Rosaria Casciaro, Carla Colombo, Felice Amato, Vincenzo Carnovale, Vincenzina Lucidi, Manuela Seia, Donatello Salvatore, Marco Lucarelli, Vito Terlizzi, Serena Quattrucci, Federica Zarrilli, Terlizzi, Vito, Castaldo, Giuseppe, Salvatore, Donatello, Lucarelli, Marco, Raia, Valeria, Angioni, Adriano, Carnovale, Vincenzo, Cirilli, Natalia, Casciaro, Rosaria, Colombo, Carla, DI LULLO, ANTONELLA MIRIAM, Elce, Ausilia, Iacotucci, Paola, Comegna, Marika, Scorza, Manuela, Lucidi, Vincenzina, Perfetti, Anna, Cimino, Roberta, Quattrucci, Serena, Seia, Manuela, Sofia, Valentina Maria, Zarrilli, Federica, and Amato, Felice

Subjects

Male, 0301 basic medicine, Cystic Fibrosis, [L997F, Cystic Fibrosis Transmembrane Conductance Regulator, Compound heterozygosity, medicine.disease_cause, Cystic fibrosis, nasal brushing, 0302 clinical medicine, Genotype, [I148T, 3199del6bp], R117L], [R74W, V201M, D1270N], gating activity, Child, Genetics (clinical), Mutation, Homozygote, Middle Aged, Cystic fibrosis transmembrane conductance regulator, Phenotype, Child, Preschool, Female, cystic fibrosis, genotype phenotype correlation, CFTR mutations, complex alleles, functional characterization, gating activity, chloride transport, Adult, Heterozygote, medicine.medical_specialty, Adolescent, Biology, Young Adult, 03 medical and health sciences, Molecular genetics, Genetics, medicine, Humans, Genetic Predisposition to Disease, Allele, Alleles, Genetic Association Studies, Heterozygote advantage, medicine.disease, Molecular biology, digestive system diseases, Nasal Mucosa, 030104 developmental biology, 030228 respiratory system, Immunology, biology.protein

Abstract

BACKGROUND: The effect of complex alleles in cystic fibrosis (CF) is poorly defined for the lack of functional studies. OBJECTIVES: To describe the genotype-phenotype correlation and the results of either in vitro and ex vivo studies performed on nasal epithelial cells (NEC) in a cohort of patients with CF carrying cystic fibrosis transmembrane conductance regulator (CFTR) complex alleles. METHODS: We studied 70 homozygous, compound heterozygous or heterozygous for CFTR mutations: p.[Arg74Trp;Val201Met;Asp1270Asn], n=8; p.[Ile148Thr;Ile1023_Val1024del], n=5; p.[Arg117Leu;Leu997Phe], n=6; c.[1210-34TG[12];1210-12T[5];2930C>T], n=3; p.[Arg74Trp;Asp1270Asn], n=4; p.Asp1270Asn, n=2; p.Ile148Thr, n=6; p.Leu997Phe, n=36. In 39 patients, we analysed the CFTR gating activity on NEC in comparison with patients with CF (n=8) and carriers (n=4). Finally, we analysed in vitro the p.[Arg74Trp;Val201Met;Asp1270Asn] complex allele. RESULTS: The p.[Ile148Thr;Ile1023_Val1024del] caused severe CF in five compound heterozygous with a class I-II mutation. Their CFTR activity on NEC was comparable with patients with two class I-II mutations (mean 7.3% vs 6.9%). The p.[Arg74Trp;Asp1270Asn] and the p.Asp1270Asn have scarce functional effects, while p.[Arg74Trp;Val201Met;Asp1270Asn] caused mild CF in four of five subjects carrying a class I-II mutation in trans, or CFTR-related disorders (CFTR-RD) in three having in trans a class IV-V mutation. The p.[Arg74Trp;Val201Met;Asp1270Asn] causes significantly (pT] and a class I-II mutation had mild CF or CFTR-RD (gating activity: 18.5-19.0%). CONCLUSIONS: The effect of complex alleles partially depends on the mutation in trans. Although larger studies are necessary, the CFTR activity on NEC is a rapid contributory tool to classify patients with CFTR dysfunction.

Published

2016

9. Two CFTR mutations within codon 970 differently impact on the chloride channel functionality

Author

Ilaria Musante, Valeria Tomati, Giuseppe Castaldo, Luis J. V. Galietta, Emanuela Caci, Cesare Braggion, Felice Amato, Marika Comegna, Antonella Miriam Di Lullo, Elke De Wachter, Vito Terlizzi, Paolo Scudieri, Eef Vanderhelst, Francesca Manzoni, Sabrina Maietta, Amato, Felice, Scudieri, Paolo, Musante, Ilaria, Tomati, Valeria, Caci, Emanuela, Comegna, Marika, Maietta, Sabrina, Manzoni, Francesca, Di Lullo, Antonella Miriam, De Wachter, Elke, Vanderhelst, Eef, Terlizzi, Vito, Braggion, Cesare, Castaldo, Giuseppe, Galietta, Luis J. V., Clinical sciences, Physiotherapy, Human Physiology and Anatomy, Pediatrics, and Pneumology

Subjects

chloride channel, Cystic Fibrosis, RNA Splicing, Mutant, Cystic Fibrosis Transmembrane Conductance Regulator, medicine.disease_cause, Transfection, Cystic fibrosis, 03 medical and health sciences, Genetic, Genetics, medicine, Missense mutation, Humans, Point Mutation, Genetics(clinical), CFTR, airway epithelium, cystic fibrosis, RNA splicing, Codon, HEK293 Cells, Phenotype, cystic fibrosi, Genetics (clinical), 030304 developmental biology, 0303 health sciences, Mutation, biology, 030305 genetics & heredity, Potentiator, medicine.disease, Molecular biology, Cystic fibrosis transmembrane conductance regulator, Chloride channel, biology.protein

Abstract

Pharmacological rescue of mutant cystic fibrosis transmembrane conductance regulator (CFTR) in cystic fibrosis (CF) depends on the specific defect caused by different mutation classes. We asked whether a patient with the rare p.Gly970Asp (c.2909G>A) mutation could benefit from CFTR pharmacotherapy since a similar missense mutant p.Gly970Arg (c.2908G>C) was previously found to be sensitive to potentiators in vitro but not in vivo. By complementary DNA transfection, we found that both mutations are associated with defective CFTR function amenable to pharmacological treatment. However, analysis of messenger RNA (mRNA) from patient's cells revealed that c.2908G>C impairs RNA splicing whereas c.2909G>A does not perturb splicing and leads to the expected p.Gly970Asp mutation. In agreement with these results, nasal epithelial cells from the p.Gly970Asp patient showed significant improvement of CFTR function upon pharmacological treatment. Our results underline the importance of controlling the effect of CF mutation at the mRNA level to determine if the pharmacotherapy of CFTR basic defect is appropriate.

Published

2018

10. Genetic Diseases That Predispose to Early Liver Cirrhosis

Author

Ausilia Elce, Felice Amato, Renato Liguori, Federica Zarrilli, Giuseppe Castaldo, Manuela Scorza, Manuela, Scorza, Ausilia, Elce, Zarrilli, Federica, Renato, Liguori, Amato, Felice, and Castaldo, Giuseppe

Subjects

medicine.medical_specialty, Cirrhosis, Hepatology, medicine.diagnostic_test, business.industry, Liver Cirrhosi, HEMOCHROMATOSIS, Review Article, medicine.disease, Bioinformatics, Pathophysiology, AAT, Molecular analysis, Liver biopsy, Molecular genetics, Medicine, lcsh:Diseases of the digestive system. Gastroenterology, lcsh:RC799-869, business, cystic fibrosi, Wilson disease

Abstract

Inherited liver diseases are a group of metabolic and genetic defects that typically cause early chronic liver involvement. Most are due to a defect of an enzyme/transport protein that alters a metabolic pathway and exerts a pathogenic role mainly in the liver. The prevalence is variable, but most are rare pathologies. We review the pathophysiology of such diseases and the diagnostic contribution of laboratory tests, focusing on the role of molecular genetics. In fact, thanks to recent advances in genetics, molecular analysis permits early and specific diagnosis for most disorders and helps to reduce the invasive approach of liver biopsy.

Published

2014

11. An Update on Laboratory Diagnosis of Liver Inherited Diseases

Author

Felice Amato, Ausilia Elce, Federica Zarrilli, Giuseppe Castaldo, Sonia Giordano, Manuela Scorza, Zarrilli, Federica, Ausilia, Elce, Manuela, Scorza, Sonia, Giordano, Amato, Felice, and Castaldo, Giuseppe

Subjects

Pathology, medicine.medical_specialty, Wilson’s disease, lcsh:Medicine, Review Article, Degeneration (medical), Disease, Cystic fibrosis, General Biochemistry, Genetics and Molecular Biology, cystic fibrosis, Liver disease, Hepatolenticular Degeneration, alpha 1-Antitrypsin Deficiency, Liver inherited diseases, Wilson’s disease, hepatolenticular degeneration, hereditary hemochromatosis, alpha-1 antitrypsin deficiency, cystic fibrosis, medicine, Humans, Hemochromatosis, alpha-1 antitrypsin deficiency, Alpha 1-antitrypsin deficiency, General Immunology and Microbiology, alpha 1 antitrypsin deficiency, cystic fibrosis, genetic counseling, genetic disorder, genotype, hemochromatosis, molecular diagnosis, Wilson disease, Clinical Laboratory Techniques, business.industry, lcsh:R, Liver inherited diseases, General Medicine, hereditary hemochromatosis, medicine.disease, Wilson's disease, Liver, Hereditary hemochromatosis, business

Abstract

Liver inherited diseases are a group of genetically determined clinical entities that appear with an early chronic liver involvement. They include Wilson’s disease (hepatolenticular degeneration), hereditary hemochromatosis, and alpha-1-antitrypsin deficiency. In addition, cystic fibrosis, although it is not specifically a liver disease, may cause a severe liver involvement in a significant percentage of cases. For all these pathologies, the disease gene is known, and molecular analysis may contribute to the unequivocal diagnosis. This approach could avoid the patient invasive procedures and limit complications associated with a delay in diagnosis. We review liver inherited diseases on the basis of the genetic defect, focusing on the contribution of molecular analysis in the multistep diagnostic workup.

Published

2013

12. An 'ex vivo model' contributing to the diagnosis and evaluation of new drugs in cystic fibrosis

Author

G. Ilardi, Elena Cantone, A. M. Di Lullo, Giuseppe Castaldo, Manuela Scorza, Maurizio Iengo, Marika Comegna, Valeria Raia, Luigi Maiuri, Felice Amato, DI LULLO, ANTONELLA MIRIAM, Scorza, M, Amato, Felice, Comegna, Marika, Raia, Valeria, Maiuri, L, Ilardi, Gennaro, Cantone, E, Castaldo, Giuseppe, and Iengo, Maurizio

Subjects

Pathology, medicine.medical_specialty, Cystic Fibrosis, Cystic Fibrosis Transmembrane Conductance Regulator, Butyrate, medicine.disease_cause, Cystic fibrosis, 03 medical and health sciences, 0302 clinical medicine, Genotype, Medicine, Humans, CFTR, 030223 otorhinolaryngology, Cystic Fibrosi, Gene, Cells, Cultured, Mutation, business.industry, Nasal brushing, CF, Rhinology, medicine.disease, Transmembrane protein, Nasal Mucosa, General Energy, Otorhinolaryngology, 030220 oncology & carcinogenesis, RNA splicing, Cancer research, business, Ex vivo, Mutations

Abstract

Cystic fibrosis (CF) is an autosomal recessive disease caused by mutations in the cystic fibrosis transmembrane regulator (CFTR) gene. About 2000 mutations have been described so far. We setup an ex vivo model of human nasal epithelial cells (HNECs) to study CF patients testing the effect of novel mutations and molecular therapies. We performed sampling (by brushing), followed by culture and analysis of HNECs using a series of molecular techniques. We performed 50 brushings from CF patients and controls. Using cultured cells, we: i) demonstrated the widely heterogeneous CFTR expression in patients and in controls; ii) defined the splicing effect of a CFTR mutation; iii) assessed the CFTR gating activity in patients bearing different mutations; iv) demonstrated that butyrate significantly enhances CFTR expression. Based on our data, we can conclude: 1) HNEC brushing is performed without anaesthesia and is well tolerated in all CF patients (children and adults); 2) HNECs can be preserved for up to 48 hours before culture allowings multicentre studies; 3) HNECs culture can be considered a suitable model to study the molecular effects of new CFTR gene mutations and/or uncertain meaning specific mutations of carriers; 4) an ex vivo model of HNECs may be used to evaluate, before human use, the effect of new drugs on patients' cells bearing specific CFTR mutations; 5) the methodology is adequate for a quantitative measurement, by fluorescence, of the CFTR gating activity of the HNECs from patients with different genotypes identifying: a) CF patients bearing two severe mutations with an activity10% (compared to controls - 100%); b) CF patients bearing at least a mild mutation with an activity of 10-20%; c) CF carriers (heterozygous subjects) with an activity between 40-70%.La fibrosi cistica (FC) è una malattia autosomica recessiva causata da mutazioni nel gene CFTR (Cystic Fibrosis Transmembrane conductance Regulator). Finora sono state descritte circa 2000 mutazioni, ma per la maggior parte di esse è difficile definirne l’effetto senza complesse procedure in vitro. Abbiamo effettuato il campionamento (mediante brushing), la cultura e l’analisi di cellule epiteliali nasali umane (HNEC) utilizzando una serie di tecniche che possono aiutare a testare l’effetto delle mutazioni CFTR. Abbiamo eseguito 50 brushing da pazienti FC e controlli, e in 45 casi si è ottenuta una coltura positiva. Utilizzando cellule in coltura: i) abbiamo dimostrato l’espressione ampiamente eterogenea del CFTR nei pazienti e nei controlli; ii) abbiamo definito l’effetto di splicing di una mutazione sul gene CFTR; iii) abbiamo valutato l’attività di gating di CFTR in pazienti portatori di differenti mutazioni; iv) abbiamo dimostrato che il butirrato migliora in modo significativo l’espressione di CFTR. I dati provenienti dal nostro studio sperimentale dimostrano che l’uso del modello ex-vivo di cellule epiteliali nasali è un importante e valido strumento di ricerca e di diagnosi nella studio della FC e può anche essere mirato alla sperimentazione ed alla verifica di nuovi farmaci. In definitiva, in base ai nostri dati è possibile esprimere le seguenti conclusioni: 1) il prelievo delle cellule epiteliali nasali mediante brushing è applicabile senza alcuna anestesia ed è ben tollerato da tutti i pazienti affetti da FC (bambini e adulti), è scarsamente invasivo e facilmente ripetibile, è anche in grado di ottenere una sufficiente quantità di HNECs rappresentative, ben conservate, idonee allo studio della funzionalità di CFTR; 2) la conservazione delle cellule prelevate è possibile fino a 48 ore prima che si provveda all’allestimento della coltura e ciò permette di avviare studi multicentrici con prelievi in ogni sede e quindi di ottenere una ampia numerosità campionaria; 3) la coltura di cellule epiteliali nasali può essere considerata un modello adatto a studiare l’effetto molecolare di nuove mutazioni del gene CFTR e/o mutazioni specifiche di pazienti “carriers” dal significato incerto; 4) il modello ex-vivo delle HNECs consente inoltre di valutare, prima dell’impiego nell’uomo, l’effetto di farmaci (potenziatori e/o correttori) sulle cellule di pazienti portatori di mutazioni specifiche di CFTR; tali farmaci possono modulare l’espressione genica del canale CFTR aprendo così nuove frontiere terapeutiche e migliori prospettive di vita per pazienti affetti da una patologia cronica come la Fibrosi Cistica; 5) la metodologia da noi istituita risulta essere idonea alla misura quantitativa, mediante fluorescenza, dell’attività di gating del canale CFTR presente nelle membrane delle cellule epiteliali nasali prelevate da pazienti portatori di differenti genotipi; in tal modo è possibile individuare: a) pazienti FC portatori di 2 mutazioni gravi con un’attività10% (in rapporto ai controlli -100%), b) soggetti FC portatori contemporaneamente di una mutazione grave e di una lieve con un’attività tra 10-30%, c) i cosiddetti portatori “carriers”- eterozigoti - con un’attività tra 40-70%. In conclusione la possibilità di misurare l’attività del canale CFTR in HNECs fornisce un importante contributo alla diagnosi di FC, mediante individuazione di un “cut-off diagnostico”, ed anche alla previsione della gravità fenotipica della malattia; quindi quanto rilevabile dalla misura del suddetto canale permette di prospettare per il futuro la possibilità di valutare meglio i pazienti per i quali il test del sudore ha dato risultati ambigui (borderline o negativi). La metodica da noi sperimentata consente anche di monitorare i pazienti durante il trattamento farmacologico, valutando in tal modo i reali effetti delle nuove terapie.

Published

2016

13. A Novel DHPLC-Based Procedure for the Analysis of COL1A1 and COL1A2 Mutations in Osteogenesis Imperfecta

Author

Felice Amato, Mariangela Iorio, Rosaria Ingino, Francesco Salvatore, Giuseppe Castaldo, Antonella Fuccio, Rossella Tomaiuolo, Mirella Filocamo, Ausilia Elce, Fuccio, Antonella, Iorio, Mariangela, Amato, Felice, Elce, A, Ingino, R, Filocamo, M, Castaldo, Giuseppe, Salvatore, Francesco, and Tomaiuolo, Rossella

Subjects

Genotype, RNA Splicing, DNA Mutational Analysis, osteogenesis imperfecta, Biology, medicine.disease_cause, COL1A1 COL1A2 mutations, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Collagen Type I, Pathology and Forensic Medicine, law.invention, Exon, Gene Frequency, law, medicine, Humans, Gene, Chromatography, High Pressure Liquid, Preimplantation Diagnosis, Polymerase chain reaction, Genetics, Mutation, Base Sequence, Intron, Regular Article, Sequence Analysis, DNA, dHPLC, Molecular biology, Collagen Type I, alpha 1 Chain, Molecular Diagnostic Techniques, RNA splicing, Molecular Medicine, COL1A1 COL1A2 mutation, Minigene

Abstract

Approximately 90% of patients with osteogenesis imperfecta (OI) exhibit dominant COL1A1 or COL1A2 mutations; however, molecular analysis is difficult because these genes span 51 and 52 exons, respectively. We devised a PCR-denaturing high-performance liquid chromatography (DHPLC) procedure to analyze the COL1A1 or COL1A2 coding regions and validated it using 130 DNA samples from individuals without OI, 25 DNA samples from two cells to investigate the procedure's potential for preimplantation diagnosis, and DNA samples from 10 patients with OI. Three novel intronic variants in vitro were expressed using a minigene assay to assess their effects on splicing. The procedure is rapid, inexpensive, and reproducible. Analysis of samples from individuals without OI revealed six novel and some known polymorphisms useful for linkage diagnosis because of high heterozygosity. Analysis of two-cell samples confirmed the known genotype in 24 of 25 experiments; DNA failed to amplify in only one case. No incidence of allele dropout was recorded. DHPLC revealed six novel mutations, three of which were intronic, in all patients with OI, and these results were confirmed by means of COL1A1 and COL1A2 direct sequencing. Expression of intronic mutations demonstrated that variant 804 + 2_804 + 3delTG in intron 11 disrupts normal splicing, thereby leading to formation of two alternative products. Variants c.3046-4_3046-5dupCT (COL1A1) and c.891 + 77A>T (COL1A2) did not affect splicing. The described DHPLC protocol combined with the minigene assay may contribute to molecular diagnosis in OI. Moreover, this protocol will aid in counseling about prenatal and preimplantation diagnosis.

Published

2011

14. Exploitation of a very small peptide nucleic acid as a new inhibitor of miR-509-3p involved in the regulation of cystic fibrosis disease-gene expression

Author

Stefano D'Errico, Giuseppe De Rosa, Gennaro Piccialli, Carmine Marco Morgillo, Bruno Catalanotti, Felice Amato, Rossella Tomaiuolo, Giuseppe Castaldo, Laura Mayol, Giorgia Oliviero, Ausilia Elce, Fabrizia Nici, Nicola Borbone, Amato, Felice, Tomaiuolo, Rossella, Nici, Fabrizia, Borbone, Nicola, Ausilia, Elce, Catalanotti, Bruno, D'Errico, Stefano, Morgillo, CARMINE MARCO, DE ROSA, Giuseppe, Mayol, Laura, Piccialli, Gennaro, Oliviero, Giorgia, and Castaldo, Giuseppe

Subjects

Peptide Nucleic Acids, Article Subject, Cystic Fibrosis, Ultraviolet Rays, lcsh:Medicine, Electrophoretic Mobility Shift Assay, Biology, Molecular Dynamics Simulation, Nucleic Acid Denaturation, General Biochemistry, Genetics and Molecular Biology, chemistry.chemical_compound, Cell Line, Tumor, microRNA, Humans, Gene, Regulation of gene expression, General Immunology and Microbiology, Peptide nucleic acid, Circular Dichroism, lcsh:R, RNA, General Medicine, MicroRNAs, chemistry, Biochemistry, Gene Expression Regulation, Nucleic acid, Spectrophotometry, Ultraviolet, Fluorescein-5-isothiocyanate, Heteroduplex, Research Article

Abstract

Computational techniques, and in particular molecular dynamics (MD) simulations, have been successfully used as a complementary technique to predict and analyse the structural behaviour of nucleic acids, including peptide nucleic acid- (PNA-) RNA hybrids. This study shows that a 7-base long PNA complementary to the seed region of miR-509-3p, one of the miRNAs involved in the posttranscriptional regulation of the CFTR disease-gene of Cystic Fibrosis, and bearing suitable functionalization at its N- and C-ends aimed at improving its resistance to nucleases and cellular uptake, is able to revert the expression of the luciferase gene containing the 3′UTR of the gene in A549 human lung cancer cells, in agreement with the MD results that pointed at the formation of a stable RNA/PNA heteroduplex notwithstanding the short sequence of the latter. The here reported results widen the interest towards the use of small PNAs as effective anti-miRNA agents.

Published

2013

15. Enhanced frequency of CFTR gene variants in couples who are candidates for assisted reproductive technology treatment

Author

Ausilia Elce, Giuseppe Castaldo, Marsia Fausto, Felice Amato, Rossella Tomaiuolo, Giuseppe De Placido, A. Ranieri, Carlo Alviggi, Ida Strina, Tomaiuolo, Rossella, Fausto, Marsia, Elce, A, Strina, Ida, Ranieri, A, Amato, Felice, Castaldo, Giuseppe, DE PLACIDO, Giuseppe, and Alviggi, Carlo

Subjects

Infertility, Male, assisted reproductive technology (ART), Genotype, Reproductive Techniques, Assisted, Clinical Biochemistry, Population, Cystic Fibrosis Transmembrane Conductance Regulator, Genetic Counseling, Bioinformatics, Cystic fibrosis, Male infertility, cystic fibrosis, Andrology, CFTR gene, Vas Deferens, Gene Frequency, Male Urogenital Diseases, medicine, Humans, education, cystic fibrosi, Alleles, Azoospermia, education.field_of_study, Polymorphism, Genetic, biology, business.industry, Biochemistry (medical), Female infertility, General Medicine, Oligospermia, Sequence Analysis, DNA, mutations, medicine.disease, Cystic fibrosis transmembrane conductance regulator, Haplotypes, biology.protein, mutation, polymorphisms, business

Abstract

Background: An increased frequency of (cystic fibrosis transmembrane conductance regulator) CFTR mutations has been detected in some types of male infertility. The aim of this study was to shed light on the link between CFTR mutations and infertility. Methods: We sequenced the CFTR gene in 294 subjects (190 males) affected by infertility of different origin who underwent assisted reproductive technology (ART). As a control group, we studied 1000 (353 males) unrelated, unselected subjects from the general population of southern Italy. Results: The frequency of CFTR mutations, some of which are detected only by gene sequencing, and of the IVS8 poly(TG)12-poly(T)5-V470 haplotype was significantly higher in obstructive [congenital bilateral absence of vasa defer-entes (CBAVD, five cases)] and secretory (23 cases) azoospermic patients than in the general population. Some patients, primarily those with CBAVD, were compound heterozygous for two mutations. Interestingly, the frequency of the TG12-T5-V470 variant haplotype was significantly higher in severe oligospermic patients (88 cases) and in patients with tubal sterility (74 cases) compared with the general population. Finally, neither the frequency of CFTR mutations nor the frequency of the TG12-T5 variants differed between patients with mild oligospermia (74 cases) and patients with ovulatory sterility (30 cases) compared with the general population. Conclusions: All subjects affected by obstructive or secretory azoospermia should undergo molecular analysis and counselling for CF using gene scanning which has a high detection rate and also reveals rare CFTR mutations. Molecular analysis seems to be less mandatory in other types of male/female infertility. Furthermore, we found that the CFTR TG12-T5-V470 variant haplotype was associated with both severe oligospermia and tubal infertility, thereby implicating the CFTR protein in both spermatogenesis and tubal functionality.

Published

2011

16. Epigenetic effects of butyrate in children with congenital chloride diarrhea: an in-vivo and in-vitro study

Author

Terrin G, Elce A, Castaldo G, Pedrolli A, Centenari C, Cardillo G, Tomaiuolo R, Amato F, Passariello A, Di Costanzo M, Troncone R, and Berni Canani R, Terrin, G., Elce, A., Castaldo, G., Tomaiuolo, R., Cardillo, G., Amato, Felice, Pedrolli, A., Centenari, C., Passariello, A., Di Costanzo, M., Troncone, Riccardo, BERNI CANANI, Roberto, Terrin, G, Elce, A, Castaldo, G, Pedrolli, A, Centenari, C, Cardillo, G, Tomaiuolo, R, Amato, F, Passariello, A, Di Costanzo, M, Troncone, R, and and Berni Canani, R

Published

2011

17. BUTYRATE MODULATES EPITHELIAL DRA EXPRESSION IN CHILDREN WITH CONGENITAL CHLORIDE DIARRHEA

Author

Terrin, Gianluca, Elce, A., Castaldo, G., Pedrolli, A., Centenari, C., Cardillo, G., Amato, F., Tomaiuolo, R., Passariello, A., Di Costanzo, M., Cosenza, L., Salvatore, F., Troncone, R., Berni Canani, R., Terrin, G., Elce, A., Castaldo, G., Pedrolli, A., Centenari, C., Cardillo, G., Amato, Felice, Tomaiuolo, R., Passariello, A., Di Costanzo, M., Cosenza, L., Salvatore, F., Troncone, R., BERNI CANANI, Roberto, Terrin, G, Elce, A, Castaldo, G, Pedrolli, A, Centenari, C, Cardillo, G, Amato, F, Tomaiuolo, R, Passariello, A, Di Costanzo, M, Cosenza, L, Salvatore, F, Troncone, R, and Berni Canani, R

Published

2011

18. Editorial Comment to p.Leu636Pro mutation is associated with cystic fibrosis transmembrane conductance regulator-related disorders (congenital bilateral absence of vas deferens)

Author

Giuseppe Castaldo, Felice Amato, Castaldo, Giuseppe, and Amato, Felice

Subjects

Male, medicine.medical_specialty, Pathology, Cystic Fibrosis, Cystic fibrosis transmembrane conductance regulator, CFTR related disorders, congenital bilateral absence of vas deferens, genetic analysis, male infertility, biology, business.industry, Urology, Vas deferens, Cystic Fibrosis Transmembrane Conductance Regulator, Cystic fibrosis transmembrane conductance regulator, Congenital bilateral absence, Vas Deferens, Endocrinology, medicine.anatomical_structure, Male Urogenital Diseases, Internal medicine, Mutation (genetic algorithm), medicine, biology.protein, Humans, business

Published

2015

19. The implication of MBL deficient haplotypes in acute coronary syndrome

Author

Tomaiuolo, R., Bellia, C., Di Micco, P., Ausilia Elce, Amato, F., Lo Sasso, B., Zarrilli, F., Ciaccio, M., Castaldo, G., Tomaiuolo, Rossella, Bellia, C, Di Micco, P, Elce, A, Amato, Felice, Lo Sasso, B, Zarrilli, F, Ciaccio, M, Castaldo, Giuseppe, Bellia, Chiara, Di Micco, Pierpaolo, Elce, Ausilia, Lo Sasso, Bruna, Zarrilli, Federica, and Ciaccio, Marcello

Subjects

haplotype, Settore BIO/12 - Biochimica Clinica E Biologia Molecolare Clinica, Physiology, Physiology (medical), mannose binding lectin 2, mannose binding lectin 2, DNA, acute coronary syndrome, genetic polymorphism, haplotype, genetic polymorphism, DNA, Cardiology and Cardiovascular Medicine, acute coronary syndrome