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2. Evaluation of human gene variants detection in amplicon pools by the GS-FLX parallel

Author

BORDONI R, BONNAL R, RIZZI E, CARRERA P, BENEDETTI S, CREMONESI L, STENIRRI S, COLOMBO A, MONTRASIO C, BONALUMI S, ALBERTINI A, ROSSI BERNARDI L, DE BELLIS G., FERRARI , MAURIZIO, Bordoni, R, Bonnal, R, Rizzi, E, Carrera, P, Benedetti, S, Cremonesi, L, Stenirri, S, Colombo, A, Montrasio, C, Bonalumi, S, Albertini, A, ROSSI BERNARDI, L, Ferrari, Maurizio, and DE BELLIS, G.

Published
2008

3. Integrated Strategy for Fast and Automated Molecular Characterization of Genes Involved in Craniosynostosis

Author

Stenirri S, Restagno G, Ferrero GB, Alaimo G, Sbaiz L1, Gomez A1, Mari C1C, Genitori L, Cremonesi L., FERRARI , MAURIZIO, Stenirri, S, Restagno, G, Ferrero, Gb, Alaimo, G, Sbaiz, L1, Gomez, A1, Mari, C1c, Genitori, L, Ferrari, Maurizio, and Cremonesi, L.

Subjects
Pathology, medicine.medical_specialty, Clinical Biochemistry, Apert syndrome, Craniosynostoses, Biology, Polymerase Chain Reaction, Craniosynostosis, Cranial vault, medicine, Humans, Receptor, Fibroblast Growth Factor, Type 3, Receptor, Fibroblast Growth Factor, Type 2, Child, Chromatography, High Pressure Liquid, Oligonucleotide Array Sequence Analysis, Autoanalysis, Biochemistry (medical), Crouzon syndrome, Dysostosis, Infant, medicine.disease, Molecular Diagnostic Techniques, Child, Preschool, Mutation, Pfeiffer syndrome, Plagiocephaly, Electronics
Abstract

Background: Craniosynostosis, the premature fusion of 1 or more sutures of the skull, is a common congenital defect, with a prevalence of 1 in 2500 live births. Untreated progressive craniosynostosis leads to inhibition of brain growth and increased intracranial and intraorbital pressure. The heterogeneity of clinical phenotypes and the overlap of the various associated syndromes render the correct diagnosis of the different craniosynostoses particularly difficult. Methods: To identify 10 common mutations in the genes for fibroblast growth factor receptors 2 and 3 (FGFR2 and FGFR3), we developed a microelectronic microchip assay that exploited the PCR multiplexing format and coupled it with serial addressing and probe hybridization on the same pad. For the molecular characterization of patients who tested negative in the microchip screening, we also developed conditions for denaturing HPLC (DHPLC) analysis of the most mutated regions of FGFR2 and FGFR3 and the entire coding region of the TWIST1 gene. Results: In our cohort of 159 patients with various craniosynostosis syndromes, mutations were found in 100% of patients with Apert syndrome, 83.3% with Pfeiffer syndrome, 72.7% with Crouzon syndrome, 50.0% with Saethre-Chotzen syndrome, 27.7% with plagiocephaly, 31.8% with brachicephaly, 20% of complex cases, and 6.9% of mixed cases. No mutations were found in syndromic cases. Conclusions: The combined microchip-DHPLC strategy allows rapid and specific molecular diagnosis of craniosynostosis and is an effective tool for the medical and surgical management of these common congenital anomalies in a newborn or an infant with a developmental defect of the cranial vault.

Published
2007

14. Three new familial hemiplegic migraine mutants affect P/Q-type Ca(2+) channel kinetics.

Author

Kraus, R L, Sinnegger, M J, Koschak, A, Glossmann, H, Stenirri, S, Carrera, P, and Striessnig, J

Abstract

Missense mutations in the pore-forming human alpha(1A) subunit of neuronal P/Q-type Ca(2+) channels are associated with familial hemiplegic migraine. We studied the functional consequences on P/Q-type Ca(2+) channel function of three recently identified mutations, R583Q, D715E, and V1457L after introduction into rabbit alpha(1A) and expression in Xenopus laevis oocytes. The potential for half-maximal channel activation of Ba(2+) inward currents was shifted by > 9 mV to more negative potentials in all three mutants. The potential for half-maximal channel inactivation was shifted by > 7 mV in the same direction in R583Q and D715E. Biexponential current inactivation during 3-s test pulses was significantly faster in D715E and slower in V1457L than in wild type. Mutations R583Q and V1457L delayed the time course of recovery from channel inactivation. The decrease of peak current through R583Q (30.2%) and D715E (30. 1%) but not V1457L (18.7%) was more pronounced during 1-Hz trains of 15 100-ms pulses than in wild type (18.2%). Our data demonstrate that the mutations R583Q, D715E, and V1457L, like the previously reported mutations T666M, V714A, and I1819L, affect P/Q-type Ca(2+) channel gating. We therefore propose that altered channel gating represents a common pathophysiological mechanism in familial hemiplegic migraine.

Published
2000

17. Molecular diagnostics by microelectronic microchips

Author

Pierangelo Bonini, Barbara Foglieni, Stefania Stenirri, Laura Cremonesi, Maurizio Ferrari, Ferrari, Maurizio, Cremonesi, L, Bonini, Pa, Stenirri, S, and Foglieni, B.

Subjects
business.industry, Computer science, Nanotechnology, Biosensing Techniques, DNA, Bioinformatics, Molecular diagnostics, Dna amplification, Polymerase Chain Reaction, Pathology and Forensic Medicine, Molecular Diagnostic Techniques, Microsystem, Microchip Analytical Procedures, Electrochemistry, Genetics, Miniaturization, Animals, Humans, RNA, Molecular Medicine, Microelectronics, Mutation detection, Sequence variation, business, Molecular Biology
Abstract

Molecular diagnostics is being revolutionized by the development of highly advanced technologies for DNA and RNA testing. One of the most important challenges is the integration of microelectronics to microchip-based nucleic acid technologies. The specific characteristics of these microsystems make the miniaturization and automation of any step of a molecular diagnostic procedure possible. This review describes the application of microelectronics to all the processes involved in a genetic test, particularly to sample preparation, DNA amplification and sequence variation detection.

Published
2005
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18. HIF1A and MIF as potential predictive mRNA biomarkers of pre-eclampsia: a longitudinal prospective study in high risk population

Author

Maurizio Ferrari, Silvia Galbiati, Vincenza Causarano, Massimo Candiani, Nadia Soriani, Laura Cremonesi, Maddalena Smid, Luca Valsecchi, Stefania Stenirri, Alessandro Ambrosi, Annalisa Inversetti, Galbiati, S, Inversetti, A, Causarano, V, Stenirri, S, Soriani, N, Ambrosi, Alessandro, Valsecchi, L, Candiani, Massimo, Cremonesi, L, Ferrari, Maurizio, and Smid, M.

Subjects
Risk, medicine.medical_specialty, pre-eclampsia, Clinical Biochemistry, Population, chemistry.chemical_compound, Pre-Eclampsia, Pregnancy, Internal medicine, medicine, Humans, Longitudinal Studies, Prospective Studies, RNA, Messenger, Endothelial dysfunction, education, Macrophage Migration-Inhibitory Factors, education.field_of_study, Eclampsia, business.industry, hypoxia, Biochemistry (medical), high risk population, longitudinal study, General Medicine, Hypoxia (medical), Endoglin, Hypoxia-Inducible Factor 1, alpha Subunit, medicine.disease, predictive mRNA markers, Intramolecular Oxidoreductases, Vascular endothelial growth factor, Endocrinology, HIF1A, chemistry, inflammation, Immunology, Female, Macrophage migration inhibitory factor, medicine.symptom, business, Biomarkers
Abstract

Pre-eclampsia (PE) is a hypertensive multisystem disorder, causing significant fetal-maternal mortality and morbidity worldwide. This study aims to define possible longitudinal predictive mRNA markers involved in the main pathogenic pathways of PE: inflammation [macrophage migration inhibitory factor (MIF)], hypoxia and oxidative stress [hypoxia inducible factor 1-α subunit (HIF1A) and β-site APP-cleaving enzyme-2 (BACE2)] and endothelial dysfunction [endoglin (ENG), fms-related tyrosine kinase-1 (FLT1) and vascular endothelial growth factor (VEGF)].Peripheral blood was collected from 33 singleton pregnancies characterized by a high cardiovascular profile risk sampled consecutively at 6–16; 17–23; 24–30; 31–34; ≥35 weeks followed by the Obstetrics and Gynecology Unit of the San Raffaele Hospital in Milan. A real-time quantitative PCR reaction was performed on plasma RNA.Of the 33 women enrolled, nine developed PE. Until 23 weeks HIF1A was significantly higher in women who later developed PE compared to women who did not (p=0.049 and p=0.012 in the first and second blood collection). In the third time interval MIF (p=0.0005), FLT1 (p=0.024), ENG (p=0.0034) and BACE2 (p=0.044) appeared to be significantly increased while HIF1A was elevated even from 24 week onwards but not reaching the statistical significance. In the fourth time interval ENG mRNA still remained increased (p=0.037).HIF1A, marker of hypoxia and oxidative stress, and MIF, marker of inflammation, seemed to be the most promising RNA markers, suggesting that hypoxia, principally, and inflammation may play an important role in PE pathogenesis.

Published
2015

19. Identification of an 18 bp deletion in the TWIST1 gene by CO-amplification at lower denaturation temperature-PCR (COLD-PCR) for non-invasive prenatal diagnosis of craniosynostosis: first case report

Author

Maurizio Ferrari, Gabriella Restagno, Silvia Galbiati, Stefania Stenirri, Laura Cremonesi, Luca Sbaiz, Marco Barberis, Galbiati, S, Stenirri, S, Sbaiz, L, Barberis, M, Cremonesi, L, Restagno, G, and Ferrari, Maurizio

Subjects
Protein Denaturation, DNA Mutational Analysis, Molecular Sequence Data, Clinical Biochemistry, Prenatal diagnosis, Biology, Polymerase Chain Reaction, Craniosynostosis, Craniosynostoses, chemistry.chemical_compound, Pregnancy, Prenatal Diagnosis, medicine, Humans, Allele, Alleles, Sequence Deletion, COLD-PCR, Genetics, Fetus, Base Sequence, Twist-Related Protein 1, Biochemistry (medical), Nuclear Proteins, General Medicine, medicine.disease, Molecular biology, Cold Temperature, medicine.anatomical_structure, chemistry, Mutation, Chorionic villi, Female, DNA
Abstract

Background: Non-invasive prenatal diagnosis has found application in a limited number of genetic diseases due to the difficulty in detecting a few copies of fetal mutated sequences in the presence of a large excess of wild-type maternal alleles, even in the case of single-base mutations. Methods: We developed conditions for the enrichment of fetal mutated alleles in maternal plasma based on CO-amplification at lower denaturation temperature-PCR (COLD-PCR). In particular, we applied a full COLD-PCR protocol to the identification of a p.A87_G92del mutation in the TWIST1 gene causing craniosynostosis in a couple at risk for the disease. Results: The use of the COLD-PCR protocol coupled with direct sequencing enabled correct identification of the fetal paternally inherited mutated allele, in accordance with the result obtained on DNA extracted from chorionic villi. Conclusions: COLD-PCR proved to be a simple and powerful tool for the identification of minority mutated alleles even in the case of a moderately large deletion (18 bp) and confirmed to be very suitable for non-invasive prenatal diagnosis of a variety of genetic diseases.

Published
2014
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20. Further considerations concerning non-invasive prenatal diagnosis of craniosynostosis based on the identification of an 18 bp deletion in the TWIST1 gene by COLD-PCR

Author

Stefania Stenirri, Maurizio Ferrari, Laura Cremonesi, Marco Barberis, Luca Sbaiz, Silvia Galbiati, Gabriella Restagno, Galbiati, S, Stenirri, S, Sbaiz, L, Barberis, M, Cremonesi, L, Restagno, and Ferrari, Maurizio

Subjects
Clinical Biochemistry, Prenatal diagnosis, Craniosynostoses, Biology, Polymerase Chain Reaction, Craniosynostosis, law.invention, Twist transcription factor, Pregnancy, law, Prenatal Diagnosis, medicine, Humans, Nuclear protein, Polymerase chain reaction, Sequence Deletion, COLD-PCR, Genetics, Twist-Related Protein 1, Biochemistry (medical), Nuclear Proteins, General Medicine, medicine.disease, Cold Temperature, Female, Identification (biology)
Published
2014

21. Unilateral Vitelliform Phenotype in Autosomal Recessive Bestrophinopathy

Author

Maria Lucia Cascavilla, Maurizio Battaglia Parodi, Lea Querques, Stefania Stenirri, Giuseppe Querques, Francesco Bandello, Cascavilla, Ml, Querques, Giuseppe, Stenirri, S, Parodi, Mb, Querques, L, and Bandello, Francesco

Subjects
Proband, medicine.medical_specialty, genetic structures, Consanguinity, BEST1 gene, Severity of Illness Index, Cellular and Molecular Neuroscience, Chloride Channels, Ophthalmology, medicine, Electroretinography, Humans, Age of Onset, Bestrophins, Fluorescein Angiography, Child, Eye Proteins, business.industry, General Medicine, Macular dystrophy, Phenotype, eye diseases, Sensory Systems, Fundus autofluorescence, Vitelliform Macular Dystrophy, Electrooculography, Mutation, Female, business, Novel mutation, Autosomal recessive bestrophinopathy, Tomography, Optical Coherence
Abstract

Aims: It was the aim of this study to report on a patient in whom a novel mutation in the BEST1 gene was responsible for unilateral vitelliform phenotype in autosomal recessive bestrophinopathy (ARB). Methods: An 8-year-old young girl (proband) with unilateral vitelliform phenotype underwent a complete ophthalmologic examination at baseline (time of diagnosis) and 2 years later. Genomic DNA was extracted to look for BEST1 gene mutations in the patient and her parents. Results: Fundus autofluorescence imaging and spectral-domain optical coherence tomography showed unchanged findings in the right eye over the 2-year follow-up period. Conversely, both fundus autofluorescence imaging and spectral-domain optical coherence tomography showed a partial reabsorption of the hyper-autofluorescent/hyper-reflective subretinal material in the left macula over the 2-year follow-up period. On BEST1 gene analysis, the patient presented a novel mutation c.535_537delAAC (p.Asn179del) in homozygous condition; interestingly, despite the absence of parents' consanguinity, both the father and mother showed the same novel mutation in heterozygous condition. Conclusion: This case of unilateral vitelliform phenotype further supports the notion that ARB represents a disease spectrum in terms of severity, age at onset and heritability. Copyright (C) 2012 S. Karger AG, Basel Aims: It was the aim of this study to report on a patient in whom a novel mutation in the BEST1 gene was responsible for unilateral vitelliform phenotype in autosomal recessive bestrophinopathy (ARB). Methods: An 8-year-old young girl (proband) with unilateral vitelliform phenotype underwent a complete ophthalmologic examination at baseline (time of diagnosis) and 2 years later. Genomic DNA was extracted to look for BEST1 gene mutations in the patient and her parents. Results: Fundus autofluorescence imaging and spectral-domain optical coherence tomography showed unchanged findings in the right eye over the 2-year follow-up period. Conversely, both fundus autofluorescence imaging and spectral-domain optical coherence tomography showed a partial reabsorption of the hyper-autofluorescent/hyper-reflective subretinal material in the left macula over the 2-year follow-up period. On BEST1 gene analysis, the patient presented a novel mutation c.535_537delAAC (p.Asn179del) in homozygous condition; interestingly, despite the absence of parents' consanguinity, both the father and mother showed the same novel mutation in heterozygous condition. Conclusion: This case of unilateral vitelliform phenotype further supports the notion that ARB represents a disease spectrum in terms of severity, age at onset and heritability. Copyright (C) 2012 S. Karger AG, Basel

Published
2012

22. Study of FTMT and ABCA4 genes in a patient affected by age-related macular degeneration: identification and analysis of new mutations

Author

M. Setaccioli, Laura Cremonesi, Maurizio Ferrari, Stefania Stenirri, Ermanna Rovida, Paolo Santambrogio, Maria Pia Manitto, Benedetta Gaia Erba, Sonia Levi, Stenirri, S, Santambrogio, P, Setaccioli, M, Erba, Bg, Pia Manitto, M, Rovida, E, Ferrari, Maurizio, Levi, SONIA MARIA ROSA, and Cremonesi, L.

Subjects
Models, Molecular, Clinical Biochemistry, DNA Mutational Analysis, ABCA4, Mitochondrion, medicine.disease_cause, Cohort Studies, Mitochondrial Proteins, Exon, Macular Degeneration, medicine, Missense mutation, Humans, Protein Structure, Quaternary, Gene, Aged, 80 and over, Mutation, biology, Base Sequence, Biochemistry (medical), MITOCHONDRIAL FERRITIN, General Medicine, Molecular biology, Protein Structure, Tertiary, Ferritins, biology.protein, ATP-Binding Cassette Transporters, Female, Haploinsufficiency
Abstract

"BACKGROUND: Age-related macular degeneration (AMD) is a multifactorial disease for which an involvement of alterations in the retinal ABC transporter gene (ABCA4) is still debated. Oxidative stress in retinal pigment epithelial cells has been postulated to contribute to the pathogenesis of the disease. Mitochondrial ferritin (FtMt), an iron-sequestering protein, is expressed in cell types characterized by high metabolic activity and oxygen consumption, including human retina, suggesting a role in protecting mitochondria from iron-dependent oxidative damage. Based on these findings we wanted to investigate whether mutations in this gene could be found in AMD patients.. . METHODS: Mutational scanning of the FTMTgene was performed in a cohort of 50 patients affected by age-related macular degeneration. The ABCA4 gene was also scanned in one patient carrying an FtMt mutation. In silico analyses were carried out on the identified variants. The recombinant form of FtMt variant was expressed in Escherichia coli and biochemically characterized.. . RESULTS: One patient was found to be heterozygous for two previously unreported genetic changes: a complex FtMt mutation (c.437_450delinsCT: delAGGACATCAAGAAGinsCT) and a missense p.Leu973Phe (c.2919G>T) mutation in exon 20 of ABCA4. Computational analyses predicted a severe structural impairment for FtMt variant and a mild destabilizing effect for ABCA4. E. coli expression of recombinant FtMt variant yielded a highly insoluble protein that could not be renatured under in vitro conditions suitable for wild-type ferritins.. . CONCLUSIONS: Our findings suggest that the FtMt mutation may determine a condition similar to haploinsufficiency resulting in a reduced protection from iron-dependent oxidative stress in mitochondria.. . "

Published
2011

23. CACNA1A gene non-synonymous single nucleotide polymorphisms and common migraine in Italy: a case-control association study with a micro-array technology

Author

Giorgio Binelli, Paola Carrera, Alberto Bernardi, Simona Balan, Stefania Stenirri, Stefania Canova, Stefania Battistini, G. Arnetoli, Stefano Gerola, Maria Nicolodi, Maurizio Ferrari, Gerola, S, Battistini, S, Stenirri, S, Nicolodi, M, Arnetoli, G, Canova, S, Binelli, G, Bernardi, A, Balan, S, Ferrari, M, and Carrera, P

Subjects
Adult, Male, Migraine without Aura, medicine.medical_specialty, CACNA1A gene, Clinical Biochemistry, Migraine with Aura, Single-nucleotide polymorphism, Polymorphism, Single Nucleotide, Case control association, Common migraine, Gene Frequency, Genotype, medicine, Humans, Genetic Predisposition to Disease, Genetic variability, Oligonucleotide Array Sequence Analysis, Genetics, business.industry, Biochemistry (medical), General Medicine, Micro array, Middle Aged, Surgery, Italy, Case-Control Studies, Female, Calcium Channels, business, Non synonymous
Published
2009

24. Are microarrays useful in the screening of ABCA4 mutations in Italian patients affected by macular degenerations?

Author

Rosario Brancato, Laura Cremonesi, Georgia Alaimo, Maurizio Ferrari, Stefania Stenirri, Maria Pia Manitto, Stenirri, S, Alaimo, G, Manitto, Mp, Brancato, R, Ferrari, Maurizio, and Cremonesi, L.

Subjects
Microarray, Clinical Biochemistry, ABCA4, medicine.disease_cause, Macular Degeneration, Medicine, Humans, Allele, Gene, Genotyping, Chromatography, High Pressure Liquid, Oligonucleotide Array Sequence Analysis, Genetics, Mutation, biology, business.industry, Biochemistry (medical), General Medicine, medicine.disease, Stargardt disease, Italy, biology.protein, ATP-Binding Cassette Transporters, DNA microarray, business
Abstract

Background: Recessive Stargardt disease is due to mutations in the retina-specific ABC transporter gene. Established strategies for molecular characterization of this gene include direct detection by a microarray interrogating approximately 500 DNA variations and a scanning denaturing HPLC methodology. Methods: Because 11 mutations were reported to account for approximately 50% of molecular defects in the Italian population, we evaluated an alternative open microchip-based assay for a fast and simplified level 1 screening for these mutations. Results: This approach allowed the characterization of both mutated alleles in 4% and one mutated allele in 43% of cases when applied to a cohort of 47 Stargardt patients. In the same patients, further investigation by denaturing HPLC for complete characterization identified both mutated alleles in 51% and one mutated allele in 19% of cases, allowing the detection of 38 different mutations, five of which had never been described. Notably, new mutations account for a high proportion (13%) of molecular defects in our patient cohort. Conclusions: This finding raises the question about the choice of the optimal diagnostic strategy for complete genotyping of the ABCA4 gene, as new mutations could not be identified by any direct detection technology, irrespective of the total number of variations screened.

Published
2008

25. De novo deletion removes a conserved motif in the C-terminus of ABCA4 and results in cone-rod dystrophy

Author

Maria Pia Manitto, Stefania Stenirri, Rosario Brancato, Laura Cremonesi, Maurizio Ferrari, Isabella Fermo, Elisabetta Martina, Stefania Battistella, Stenirri, S, Battistella, S, Fermo, I, Manitto, Mp, Martina, E, Brancato, R, Ferrari, Maurizio, and Cremonesi, L.

Subjects
Male, Heterozygote, Adolescent, Eye Diseases, genetic structures, Molecular Sequence Data, Clinical Biochemistry, ABCA4, ATP-binding cassette transporter, Exon, Retinal Rod Photoreceptor Cells, Retinitis pigmentosa, medicine, Humans, Amino Acid Sequence, Gene, Chromatography, High Pressure Liquid, Genetics, biology, Biochemistry (medical), Intron, Dystrophy, Sequence Analysis, DNA, General Medicine, medicine.disease, Molecular biology, eye diseases, Protein Structure, Tertiary, Stargardt disease, Mutation, Retinal Cone Photoreceptor Cells, biology.protein, ATP-Binding Cassette Transporters, sense organs, Gene Deletion
Abstract

Background: Mutations in the retina-specific ABC transporter (ABCA4) gene are associated with different types of macular degeneration, including Stargardt disease, cone-rod dystrophy, Fundus flavimaculatus, Retinitis pigmentosa and probably age-related macular degeneration. Methods: Screening for mutations in the ABCA4 gene was performed using denaturing high-performance liquid chromatography and direct sequencing. Results: We describe the identification of a new de novo 44-bp deletion in an Italian patient affected by cone-rod dystrophy. The mutation, located in intron 48 of the ABCA4 gene, is predicted to cause exon 49 skipping, resulting in loss of the C-terminus of the ABCA4 protein. Interestingly, exon 49 also codes for a highly conserved VFVNFA motif, which has been demonstrated to be essential for the activity of ABCA1, another gene of the ABC transporter family. The presence of CT repeats at the breakpoints might have facilitated the generation of the deletion through a slippage mispairing mechanism. Conclusions: The new 6730-16del44 deletion is the first de novo mutation associated with cone-rod dystrophy and may contribute to a better understanding of the role of ABCA4 mutations in macular dystrophies.

Published
2006
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26. Denaturing HPLC profoling of the ABCA4 gene for reliable detection of allelic variations

Author

Maurizio Ferrari, Rosario Brancato, Elisabetta Martina, Laura Cremonesi, Stefania Stenirri, Silvia Galbiati, Maria Pia Manitto, Isabella Fermo, Rita Paroni, Rando Allikmets, Nadia Soriani, Stefania Battistella, Stenirri S, 1. 4. 5., Fermo, I, Battistella, S, Galbiati, S, Soriani, N, Paroni, R, Manitto, Mp, Martina, E, Brancato, R, Allikmets, R, Ferrari, Maurizio, and Cremonesi, L.

Subjects
Genetics, Denaturing hplc, Electrophoresis, Polymorphism, Genetic, biology, Genotype, Biochemistry (medical), Clinical Biochemistry, ABCA4, Phenotype, Exon, Macular Degeneration, Settore BIO/10 - Biochimica, Mutation, biology.protein, Humans, ATP-Binding Cassette Transporters, Allele, Gene, Temperature gradient gel electrophoresis, Alleles, Chromatography, High Pressure Liquid, Retrospective Studies
Abstract

Background: Mutations in the retina-specific ABC transporter (ABCA4) gene have been associated with several forms of macular degenerations. Because the high complexity of the molecular genotype makes scanning of the ABCA4 gene cumbersome, we describe here the first use of denaturing HPLC (DHPLC) to screen for ABCA4 mutations. Methods: Temperature conditions were designed for all 50 exons based on effective separation of 83 samples carrying 86 sequence variations and 19 mutagenized controls. For validation, samples from 23 previously characterized Stargardt patients were subjected to DHPLC profiling. Subsequently, samples from a cohort of 30 patients affected by various forms of macular degeneration were subjected to DHPLC scanning under the same conditions. Results: DHPLC profiling not only identified all 132 sequence alterations previously detected by double-gradient denaturing gradient gel electrophoresis but also identified 5 sequence alterations that this approach had missed. Moreover, DHPLC scanning of an additional panel of 30 previously untested patients led to the identification of 26 different mutations and 29 polymorphisms, accounting for 203 sequence variations on 29 of the 30 patients screened. In total, the DHPLC approach allowed us to identify 16 mutations that had never been reported before. Conclusions: These results provide strong support for the use of DHPLC for molecular characterization of the ABCA4 gene.

Published
2004

27. Denaturing HPLC analysis of DNA deletions and insertions

Author

Maurizio Ferrari, Mario Cazzola, Paolo Arosio, Isabella Fermo, Stefania Stenirri, Rita Paroni, Laura Cremonesi, Cremonesi, L, Stenirri, S, Fermo, I, Paroni, R, Ferrari, Maurizio, Cazzola, M, and Arosio, P.

Subjects
Cystic Fibrosis Transmembrane Conductance Regulator, ABCA4, Gene mutation, Nucleic Acid Denaturation, Polymerase Chain Reaction, chemistry.chemical_compound, Genetics, Humans, Nucleotide, Cation Transport Proteins, Gene, Chromatography, High Pressure Liquid, Genetics (clinical), Denaturing hplc, chemistry.chemical_classification, biology, DNA, Amplicon, Rod Cell Outer Segment, Molecular biology, Mutagenesis, Insertional, chemistry, Ferritins, biology.protein, ATP-Binding Cassette Transporters, Chromosome Deletion, 5' Untranslated Regions, Nucleic Acid Amplification Techniques, Heteroduplex
Abstract

Denaturing HPLC (DHPLC) is a useful technique for the fast screening of known and unknown heterozygous gene mutations. Most DNA mutations causing genetic disorders consist of nucleotide substitutions, but insertions and deletions occur, albeit less frequently. The heteroduplexes with insertions/deletions have gaps that may affect molecular stability differently from the mismatches caused by substitutions. Therefore, gaps and mismatches may be distinguished by DHPLC analysis, which is based on the differential thermal stability of amplicons with different characteristics. To verify this hypothesis, we examined 12 DNA samples containing insertions and deletions of different sizes (one to 29 residues) from four different genes (ABCA4, CFTR, FTL, and SLC11A3). We found that all of them were detected by DHPLC runs at 50°C, which is considered a non-denaturing temperature, as well as by runs at the temperature optimized for mismatch recognition. The finding confirms that gaps reduce heteroduplex stability more than mismatches, and indicates that DHPLC analysis at low temperature may be applied to distinguish DNA deletions/insertions from substitutions. Hum Mutat 22:98–102, 2003. © 2003 Wiley-Liss, Inc.

Published
2003

28. Deciphering Variability of PKD1 and PKD2 in an Italian Cohort of 643 Patients with Autosomal Dominant Polycystic Kidney Disease (ADPKD).

Author

Carrera P, Calzavara S, Magistroni R, den Dunnen JT, Rigo F, Stenirri S, Testa F, Messa P, Cerutti R, Scolari F, Izzi C, Edefonti A, Negrisolo S, Benetti E, Alibrandi MT, Manunta P, Boletta A, and Ferrari M

Subjects
Adolescent, Adult, Alleles, Base Sequence, Cohort Studies, Female, Gene Frequency, Humans, Italy epidemiology, Kidney diagnostic imaging, Kidney pathology, Magnetic Resonance Imaging, Male, Middle Aged, Mutation, Missense, Pedigree, Polycystic Kidney, Autosomal Dominant epidemiology, Polycystic Kidney, Autosomal Dominant pathology, Polymorphism, Genetic, Young Adult, Polycystic Kidney, Autosomal Dominant genetics, TRPP Cation Channels genetics
Abstract

Autosomal Dominant Polycystic Kidney Disease (ADPKD) is the most common hereditary kidney disease. We analysed PKD1 and PKD2, in a large cohort of 440 unrelated Italian patients with ADPKD and 203 relatives by direct sequencing and MLPA. Molecular and detailed phenotypic data have been collected and submitted to the PKD1/PKD2 LOVD database. This is the first large retrospective study in Italian patients, describing 701 variants, 249 (35.5%) already associated with ADPKD and 452 (64.5%) novel. According to the criteria adopted, the overall detection rate was 80% (352/440). Novel variants with uncertain significance were found in 14% of patients. Among patients with pathogenic variants, in 301 (85.5%) the disease is associated with PKD1, 196 (55.7%) truncating, 81 (23%) non truncating, 24 (6.8%) IF indels, and in 51 (14.5%) with PKD2. Our results outline the high allelic heterogeneity of variants, complicated by the presence of variants of uncertain significance as well as of multiple variants in the same subject. Classification of novel variants may be particularly cumbersome having an important impact on the genetic counselling. Our study confirms the importance to improve the assessment of variant pathogenicity for ADPKD; to this point databasing of both clinical and molecular data is crucial.

Published
2016
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29. HIF1A and MIF as potential predictive mRNA biomarkers of pre-eclampsia: a longitudinal prospective study in high risk population.

Author

Galbiati S, Inversetti A, Causarano V, Stenirri S, Soriani N, Ambrosi A, Valsecchi L, Candiani M, Cremonesi L, Ferrari M, and Smid M

Subjects
Biomarkers metabolism, Female, Humans, Longitudinal Studies, Pre-Eclampsia diagnosis, Pregnancy, Prospective Studies, RNA, Messenger genetics, RNA, Messenger metabolism, Risk, Hypoxia-Inducible Factor 1, alpha Subunit genetics, Intramolecular Oxidoreductases genetics, Macrophage Migration-Inhibitory Factors genetics, Pre-Eclampsia genetics
Abstract

Background: Pre-eclampsia (PE) is a hypertensive multisystem disorder, causing significant fetal-maternal mortality and morbidity worldwide. This study aims to define possible longitudinal predictive mRNA markers involved in the main pathogenic pathways of PE: inflammation [macrophage migration inhibitory factor (MIF)], hypoxia and oxidative stress [hypoxia inducible factor 1-α subunit (HIF1A) and β-site APP-cleaving enzyme-2 (BACE2)] and endothelial dysfunction [endoglin (ENG), fms-related tyrosine kinase-1 (FLT1) and vascular endothelial growth factor (VEGF)]., Methods: Peripheral blood was collected from 33 singleton pregnancies characterized by a high cardiovascular profile risk sampled consecutively at 6-16; 17-23; 24-30; 31-34; ≥35 weeks followed by the Obstetrics and Gynecology Unit of the San Raffaele Hospital in Milan. A real-time quantitative PCR reaction was performed on plasma RNA., Results: Of the 33 women enrolled, nine developed PE. Until 23 weeks HIF1A was significantly higher in women who later developed PE compared to women who did not (p=0.049 and p=0.012 in the first and second blood collection). In the third time interval MIF (p=0.0005), FLT1 (p=0.024), ENG (p=0.0034) and BACE2 (p=0.044) appeared to be significantly increased while HIF1A was elevated even from 24 week onwards but not reaching the statistical significance. In the fourth time interval ENG mRNA still remained increased (p=0.037)., Conclusions: HIF1A, marker of hypoxia and oxidative stress, and MIF, marker of inflammation, seemed to be the most promising RNA markers, suggesting that hypoxia, principally, and inflammation may play an important role in PE pathogenesis.

Published
2015
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30. Further considerations concerning non-invasive prenatal diagnosis of craniosynostosis based on the identification of an 18 bp deletion in the TWIST1 gene by COLD-PCR.

Author

Galbiati S, Stenirri S, Sbaiz L, Barberis M, Cremonesi L, Restagno G, and Ferrari M

Subjects
Female, Humans, Pregnancy, Cold Temperature, Craniosynostoses diagnosis, Nuclear Proteins genetics, Polymerase Chain Reaction methods, Prenatal Diagnosis, Sequence Deletion genetics, Twist-Related Protein 1 genetics
Published
2014
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31. Study of FTMT and ABCA4 genes in a patient affected by age-related macular degeneration: identification and analysis of new mutations.

Author

Stenirri S, Santambrogio P, Setaccioli M, Erba BG, Pia Manitto M, Rovida E, Ferrari M, Levi S, and Cremonesi L

Subjects
ATP-Binding Cassette Transporters chemistry, ATP-Binding Cassette Transporters metabolism, Aged, 80 and over, Base Sequence, Cohort Studies, Female, Ferritins chemistry, Ferritins metabolism, Humans, Macular Degeneration metabolism, Mitochondrial Proteins chemistry, Mitochondrial Proteins metabolism, Models, Molecular, Protein Structure, Quaternary, Protein Structure, Tertiary, ATP-Binding Cassette Transporters genetics, DNA Mutational Analysis, Ferritins genetics, Macular Degeneration genetics, Mitochondrial Proteins genetics, Mutation
Abstract

Background: Age-related macular degeneration (AMD) is a multifactorial disease for which an involvement of alterations in the retinal ABC transporter gene (ABCA4) is still debated. Oxidative stress in retinal pigment epithelial cells has been postulated to contribute to the pathogenesis of the disease. Mitochondrial ferritin (FtMt), an iron-sequestering protein, is expressed in cell types characterized by high metabolic activity and oxygen consumption, including human retina, suggesting a role in protecting mitochondria from iron-dependent oxidative damage. Based on these findings we wanted to investigate whether mutations in this gene could be found in AMD patients., Methods: Mutational scanning of the FTMTgene was performed in a cohort of 50 patients affected by age-related macular degeneration. The ABCA4 gene was also scanned in one patient carrying an FtMt mutation. In silico analyses were carried out on the identified variants. The recombinant form of FtMt variant was expressed in Escherichia coli and biochemically characterized., Results: One patient was found to be heterozygous for two previously unreported genetic changes: a complex FtMt mutation (c.437_450delinsCT: delAGGACATCAAGAAGinsCT) and a missense p.Leu973Phe (c.2919G>T) mutation in exon 20 of ABCA4. Computational analyses predicted a severe structural impairment for FtMt variant and a mild destabilizing effect for ABCA4. E. coli expression of recombinant FtMt variant yielded a highly insoluble protein that could not be renatured under in vitro conditions suitable for wild-type ferritins., Conclusions: Our findings suggest that the FtMt mutation may determine a condition similar to haploinsufficiency resulting in a reduced protection from iron-dependent oxidative stress in mitochondria.

Published
2012
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32. Unilateral vitelliform phenotype in autosomal recessive bestrophinopathy.

Author

Cascavilla ML, Querques G, Stenirri S, Battaglia Parodi M, Querques L, and Bandello F

Subjects
Age of Onset, Bestrophins, Child, Electrooculography, Electroretinography, Female, Fluorescein Angiography, Humans, Phenotype, Severity of Illness Index, Tomography, Optical Coherence, Vitelliform Macular Dystrophy diagnosis, Chloride Channels genetics, Eye Proteins genetics, Mutation, Vitelliform Macular Dystrophy genetics
Abstract

Aims: It was the aim of this study to report on a patient in whom a novel mutation in the BEST1 gene was responsible for unilateral vitelliform phenotype in autosomal recessive bestrophinopathy (ARB)., Methods: An 8-year-old young girl (proband) with unilateral vitelliform phenotype underwent a complete ophthalmologic examination at baseline (time of diagnosis) and 2 years later. Genomic DNA was extracted to look for BEST1 gene mutations in the patient and her parents., Results: Fundus autofluorescence imaging and spectral-domain optical coherence tomography showed unchanged findings in the right eye over the 2-year follow-up period. Conversely, both fundus autofluorescence imaging and spectral-domain optical coherence tomography showed a partial reabsorption of the hyper-autofluorescent/hyper-reflective subretinal material in the left macula over the 2-year follow-up period. On BEST1 gene analysis, the patient presented a novel mutation c.535_537delAAC (p.Asn179del) in homozygous condition; interestingly, despite the absence of parents' consanguinity, both the father and mother showed the same novel mutation in heterozygous condition., Conclusion: This case of unilateral vitelliform phenotype further supports the notion that ARB represents a disease spectrum in terms of severity, age at onset and heritability., (Copyright © 2012 S. Karger AG, Basel.)

Published
2012
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33. CACNA1A gene non-synonymous single nucleotide polymorphisms and common migraine in Italy: a case-control association study with a micro-array technology.

Author

Gerola S, Battistini S, Stenirri S, Nicolodi M, Arnetoli G, Canova S, Binelli G, Bernardi A, Balan S, Ferrari M, and Carrera P

Subjects
Adult, Case-Control Studies, Female, Gene Frequency, Humans, Italy, Male, Middle Aged, Oligonucleotide Array Sequence Analysis, Calcium Channels genetics, Genetic Predisposition to Disease, Migraine with Aura genetics, Migraine without Aura genetics, Polymorphism, Single Nucleotide
Published
2009
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34. Dual-color microchip electrophoresis with single-photon avalanche diodes: application to mutation detection.

Author

Stenirri S, Cretich M, Rech I, Restelli A, Ghioni M, Cova S, Ferrari M, Cremonesi L, and Chiari M

Subjects
DNA analysis, DNA genetics, Electrophoresis, Microchip methods, DNA Mutational Analysis methods, Electrophoresis, Microchip instrumentation, Mutation genetics, Photons
Abstract

A novel microchip electrophoresis instrument based on single-photon avalanche diodes was used for the molecular characterization of mutations in disease genes. The identification of the main mutation causing cystic fibrosis, named DeltaF508, by the Amplification Refractory Mutation System was used to validate the technology. In our implemented protocol the wild-type and mutant allele-specific primers are labeled with Cy5 and Cy5.5, respectively. The protocol enables the amplification of the DNA sample in a single PCR. The genotype was deduced from the fluorescence of the amplicons run in the CE microchip. Validation on 15 DNA samples from either homozygous wild-type or heterozygous and homozygous mutated control subjects proved the complete reliability of the system, thus confirming its high diagnostic potential.

Published
2008
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35. Evaluation of human gene variant detection in amplicon pools by the GS-FLX parallel Pyrosequencer.

Author

Bordoni R, Bonnal R, Rizzi E, Carrera P, Benedetti S, Cremonesi L, Stenirri S, Colombo A, Montrasio C, Bonalumi S, Albertini A, Bernardi LR, Ferrari M, and De Bellis G

Subjects
Genetic Diseases, Inborn genetics, Genetic Variation genetics, Humans, Mutation genetics, Neoplasms genetics, Polymorphism, Single Nucleotide genetics, Genomics methods, Sequence Analysis, DNA methods
Abstract

Background: A new priority in genome research is large-scale resequencing of genes to understand the molecular basis of hereditary disease and cancer. We assessed the ability of massively parallel pyrosequencing to identify sequence variants in pools. From a large collection of human PCR samples we selected 343 PCR products belonging to 16 disease genes and including a large spectrum of sequence variations previously identified by Sanger sequencing. The sequence variants included SNPs and small deletions and insertions (up to 44 bp), in homozygous or heterozygous state., Results: The DNA was combined in 4 pools containing from 27 to 164 amplicons and from 8,9 to 50,8 Kb to sequence for a total of 110 Kb. Pyrosequencing generated over 80 million base pairs of data. Blind searching for sequence variations with a specifically designed bioinformatics procedure identified 465 putative sequence variants, including 412 true variants, 53 false positives (in or adjacent to homopolymeric tracts), no false negatives. All known variants in positions covered with at least 30x depth were correctly recognized., Conclusion: Massively parallel pyrosequencing may be used to simplify and speed the search for DNA variations in PCR products. Our results encourage further studies to evaluate molecular diagnostics applications.

Published
2008
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37. Are microarrays useful in the screening of ABCA4 mutations in Italian patients affected by macular degenerations?

Author

Stenirri S, Alaimo G, Manitto MP, Brancato R, Ferrari M, and Cremonesi L

Subjects
Chromatography, High Pressure Liquid, Humans, Italy, Macular Degeneration metabolism, ATP-Binding Cassette Transporters genetics, Macular Degeneration genetics, Mutation, Oligonucleotide Array Sequence Analysis
Abstract

Background: Recessive Stargardt disease is due to mutation in the retina-specific ABC transporter gene. Established strategies for molecular characterization of this gene include direct detection by a microarray interrogating approximately 500 DNA variations and a scanning denaturing HPLC methodology., Methods: Because 11 mutations were recorded to account for approximately 50% of molecular defects in the Italian population, we evaluated an alternative open microchip-based assay for a fast and simplified level 1 screening for these mutations., Results: This approach allowed the characterization of both mutated alleles in 4% and one mutated allele in 43% of cases when applied to a cohort of 47 Stargardt patients. In the same patients, further investigation by denaturing HPLC for complete characterization identified both mutated allele in 51% and one mutated allele in 19% of cases, allowing the detection of 38 different mutations, five of which had never been described. Notably, new mutations account for a high proportion (13%) of molecular defects in our patient cohort., Conclusion: The findings raises the question about the choice of the optimal diagnostic strategy for complete genotyping of the ABCA4 gene, as new mutations could not be identified by any direct detection technology, irrespective of the total number of variations screened.

Published
2008
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38. De novo deletion removes a conserved motif in the C-terminus of ABCA4 and results in cone-rod dystrophy.

Author

Stenirri S, Battistella S, Fermo I, Manitto MP, Martina E, Brancato R, Ferrari M, and Cremonesi L

Subjects
Adolescent, Amino Acid Sequence, Chromatography, High Pressure Liquid methods, Heterozygote, Humans, Male, Molecular Sequence Data, Protein Structure, Tertiary, Sequence Analysis, DNA, ATP-Binding Cassette Transporters genetics, Eye Diseases genetics, Gene Deletion, Mutation, Retinal Cone Photoreceptor Cells pathology, Retinal Rod Photoreceptor Cells pathology
Abstract

Background: Mutations in the retina-specific ABC transporter (ABCA4) gene are associated with different types of macular degeneration, including Stargardt disease, cone-rod dystrophy, Fundus flavimaculatus, Retinitis pigmentosa and probably age-related macular degeneration., Methods: Screening for mutations in the ABCA4 gene was performed using denaturing high-performance liquid chromatography and direct sequencing., Results: We describe the identification of a new de novo 44-bp deletion in an Italian patient affected by cone-rod dystrophy. The mutation, located in intron 48 of the ABCA4 gene, is predicted to cause exon 49 skipping, resulting in loss of the C-terminus of the ABCA4 protein. Interestingly, exon 49 also codes for a highly conserved VFVNFA motif, which has been demonstrated to be essential for the activity of ABCA1, another gene of the ABC transporter family. The presence of CT repeats at the breakpoints might have facilitated the generation of the deletion through a slippage mispairing mechanism., Conclusions: The new 6730-16del44 deletion is the first de novo mutation associated with cone-rod dystrophy and may contribute to a better understanding of the role of ABCA4 mutations in macular dystrophies.

Published
2006
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39. Single-nucleotide polymorphism and mutation identification by the nanogen microelectronic chip technology.

Author

Ferrari M, Cremonesi L, Bonini P, Foglieni B, and Stenirri S

Subjects
Base Sequence, Humans, Molecular Diagnostic Techniques, Molecular Sequence Data, Nucleic Acid Conformation, DNA Mutational Analysis instrumentation, DNA Mutational Analysis methods, Mutation, Nanotechnology, Oligonucleotide Array Sequence Analysis instrumentation, Oligonucleotide Array Sequence Analysis methods, Polymorphism, Single Nucleotide
Abstract

The present chapter describes a microarray technology developed by Nanogen Inc., for the identification of DNA variations based on the use of microelectronics. The NMW 1000 NanoChip Molecular Biology Workstation allows the active deposition and concentration of charged biotinylated molecules on designated test sites. The DNA at each pad is then hybridized with specific oligonucleotide probes, complementary to normal or mutant sequences, that labeled with Cy3 or Cy5 dyes, respectively. The array is imaged, and fluorescence signals are scanned, monitored, and quantified by highly developed, digital image-processing procedures. The experimental steps to be performed for the development and execution of a microchip assay are described. Attention is focused on the fundamental aspects of probe design, and guidelines and useful suggestions are given. Protocols for sample preparation, addressing, reporting, and data analysis are also detailed.

Published
2005
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40. Denaturing HPLC profiling of the ABCA4 gene for reliable detection of allelic variations.

Author

Stenirri S, Fermo I, Battistella S, Galbiati S, Soriani N, Paroni R, Manitto MP, Martina E, Brancato R, Allikmets R, Ferrari M, and Cremonesi L

Subjects
Alleles, Chromatography, High Pressure Liquid methods, Electrophoresis methods, Genotype, Humans, Macular Degeneration genetics, Mutation, Phenotype, Polymorphism, Genetic, Retrospective Studies, ATP-Binding Cassette Transporters genetics
Abstract

Background: Mutations in the retina-specific ABC transporter (ABCA4) gene have been associated with several forms of macular degenerations. Because the high complexity of the molecular genotype makes scanning of the ABCA4 gene cumbersome, we describe here the first use of denaturing HPLC (DHPLC) to screen for ABCA4 mutations., Methods: Temperature conditions were designed for all 50 exons based on effective separation of 83 samples carrying 86 sequence variations and 19 mutagenized controls. For validation, samples from 23 previously characterized Stargardt patients were subjected to DHPLC profiling. Subsequently, samples from a cohort of 30 patients affected by various forms of macular degeneration were subjected to DHPLC scanning under the same conditions., Results: DHPLC profiling not only identified all 132 sequence alterations previously detected by double-gradient denaturing gradient gel electrophoresis but also identified 5 sequence alterations that this approach had missed. Moreover, DHPLC scanning of an additional panel of 30 previously untested patients led to the identification of 26 different mutations and 29 polymorphisms, accounting for 203 sequence variations on 29 of the 30 patients screened. In total, the DHPLC approach allowed us to identify 16 mutations that had never been reported before., Conclusions: These results provide strong support for the use of DHPLC for molecular characterization of the ABCA4 gene.

Published
2004
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41. Denaturing HPLC analysis of DNA deletions and insertions.

Author

Cremonesi L, Stenirri S, Fermo I, Paroni R, Ferrari M, Cazzola M, and Arosio P

Subjects
5' Untranslated Regions genetics, ATP-Binding Cassette Transporters genetics, Cation Transport Proteins genetics, Cystic Fibrosis Transmembrane Conductance Regulator genetics, DNA chemistry, DNA genetics, Ferritins genetics, Humans, Nucleic Acid Amplification Techniques methods, Nucleic Acid Denaturation genetics, Polymerase Chain Reaction methods, Rod Cell Outer Segment, Ferroportin, Chromatography, High Pressure Liquid methods, Chromosome Deletion, DNA analysis, Mutagenesis, Insertional genetics
Abstract

Denaturing HPLC (DHPLC) is a useful technique for the fast screening of known and unknown heterozygous gene mutations. Most DNA mutations causing genetic disorders consist of nucleotide substitutions, but insertions and deletions occur, albeit less frequently. The heteroduplexes with insertions/deletions have gaps that may affect molecular stability differently from the mismatches caused by substitutions. Therefore, gaps and mismatches may be distinguished by DHPLC analysis, which is based on the differential thermal stability of amplicons with different characteristics. To verify this hypothesis, we examined 12 DNA samples containing insertions and deletions of different sizes (one to 29 residues) from four different genes (ABCA4, CFTR, FTL, and SLC11A3). We found that all of them were detected by DHPLC runs at 50 degrees C, which is considered a non-denaturing temperature, as well as by runs at the temperature optimized for mismatch recognition. The finding confirms that gaps reduce heteroduplex stability more than mismatches, and indicates that DHPLC analysis at low temperature may be applied to distinguish DNA deletions/insertions from substitutions., (Copyright 2003 Wiley-Liss, Inc.)

Published
2003
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42. Molecular diagnostics by microelectronic microchips.

Author

Ferrari M, Stenirri S, Bonini P, and Cremonesi L

Subjects
Gene Expression Profiling, Humans, Molecular Diagnostic Techniques, Oligonucleotide Array Sequence Analysis methods
Abstract

Molecular diagnostics is being revolutionized by the completion of the human genome project and by the development of highly advanced technologies for DNA testing. One of the most important challenges is the introduction of high throughput systems such as DNA chips into diagnostic laboratories. DNA microchips are small devices permitting rapid analysis of genetic information, exploiting miniaturization of all components and automation of operational procedures. The most important biochip applications include gene expression and genetic variation identification and both may improve human molecular diagnostics. Here we review several approaches developed to allow rapid detection of many single nucleotide polymorphisms and mutations in large population samples. Among these, the use of microelectronics seems to best fit with the needs of molecular diagnostics.

Published
2003
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43. Familial hemiplegic migraine: a ion channel disorder.

Author

Carrera P, Stenirri S, Ferrari M, and Battistini S

Subjects
Humans, Mutation, Calcium Channels genetics, Migraine with Aura genetics, Trinucleotide Repeats
Abstract

At present, little information is available on the genetics of common migraines, most likely to be considered a multifactorial disease. Recently, the CACNA1A gene encoding the brain-specific P/Q type calcium channel alpha(1) subunit, has been cloned and mutations in this gene, located on chromosome 19p13, have been shown to be involved in familial hemiplegic migraine (FHM), a rare autosomal dominantly inherited subtype of migraine with aura. Being part of the migraine spectrum, FHM represents a good model to study the genetics of more common forms of migraine. Different classes of mutations within the CACNA1A gene have been associated with different diseases, thus identifying a new member among 'channelopathies'. Variable clinical expression and genetic heterogeneity of FHM will be discussed.

Published
2001
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