Your search keyword '"Giunti, L"' showing total 210 results

201. Promoter methylation and expression analysis of MGMT in advanced pediatric brain tumors.

Author

Sardi I, Cetica V, Massimino M, Buccoliero AM, Giunti L, Genitori L, and Aricò M

Subjects

Adolescent, Antineoplastic Agents, Alkylating therapeutic use, Brain Neoplasms drug therapy, Brain Neoplasms pathology, Child, Child, Preschool, DNA Modification Methylases biosynthesis, DNA Repair Enzymes biosynthesis, Dacarbazine analogs & derivatives, Dacarbazine therapeutic use, Disease-Free Survival, Female, Humans, Immunohistochemistry, Infant, Male, Neoplasm Recurrence, Local drug therapy, Neoplasm Recurrence, Local genetics, Neoplasm Recurrence, Local pathology, RNA, Messenger analysis, Reverse Transcriptase Polymerase Chain Reaction, Temozolomide, Tumor Suppressor Proteins biosynthesis, Brain Neoplasms genetics, DNA Methylation genetics, DNA Modification Methylases genetics, DNA Repair Enzymes genetics, Drug Resistance, Neoplasm genetics, Promoter Regions, Genetic genetics, Tumor Suppressor Proteins genetics

Abstract

Insufficient response to oral temozolomide (TMZ) in children with brain tumor may depend on the repair-action of inducible O6-methylguanine-DNA methyltransferase (MGMT). To investigate the clinical relevance of MGMT expression, we analyzed MGMT levels by qRT-PCR and immunohistochemistry, and the methylation of gene promoter in patients with relapsed or refractory brain tumor, enrolled in an off-label trial with oral temozolomide. The drug was administered at the dose of 200 mg/m(2)/day in patients with no prior cranio-spinal irradiation, and 180 mg/m(2)/day in those with previous radiotherapy and/or high-dose chemotherapy followed by autologous hematopoietic stem cell rescue. Nine patients with recurrent ependymoma (n=3), low grade glioma (n=3), glioblastoma (n=1), relapsed medulloblastoma (n=2) were enrolled in the study. Median absolute MGMT mRNA expression level standardized for GAPDH was 1.06 (range -0.453 to 3.932). The median relative expression level (RQ=2(-ddC)) was 4.29 (range 1.585 to 12.228). By immunohistochemistry, the score was 2+ in 6 of the 9 tumor samples, and 1+ in 3, while none was MGMT negative. Methylation of MGMT promoter was detected in only one ependymoma sample. The heterogeneous PFS in our patients treated with second line TMZ, indicates that MGMT expression alone is insufficient to predict the response to TMZ, presumably because of the DNA repair mechanisms involved.

Published

2009

202. Pediatric brain tumors: mutations of two dioxygenases (hABH2 and hABH3) that directly repair alkylation damage.

Author

Cetica V, Genitori L, Giunti L, Sanzo M, Bernini G, Massimino M, and Sardi I

Subjects

Adolescent, AlkB Homolog 2, Alpha-Ketoglutarate-Dependent Dioxygenase, AlkB Homolog 3, Alpha-Ketoglutarate-Dependent Dioxygenase, Alkylation, Brain Neoplasms pathology, Case-Control Studies, Child, Child, Preschool, Female, Humans, Infant, Male, Neoplasm Recurrence, Local genetics, RNA, Messenger genetics, Reverse Transcriptase Polymerase Chain Reaction, Spinal Neoplasms genetics, Spinal Neoplasms secondary, Brain Neoplasms genetics, DNA Damage genetics, DNA Repair genetics, DNA Repair Enzymes genetics, Dioxygenases genetics, Mutation genetics

Abstract

Alkylating agents, commonly used for brain tumor therapy, induce DNA and RNA lesions that, if not repaired, drive cells to apoptosis. Thus, cellular mechanisms that are responsible for nucleic acid repair are possibly involved in drug resistance. This work analyzes hABH2 and hABH3, two human Fe(II)-dependent dioxygenases in pediatric brain tumors that are treated with alkylating agents. We analyzed 25 brain tumor samples for hABH2 and hABH3 mutations; a subset of samples was tested for quantitative expression with Real-Time PCR. Sequencing analysis showed two new mutations in two glioma patients, one of hABH2 coding sequence (I141 V) and the other of hABH3 (D189 N). The mutation at codon 189 falls in a crucial region of the protein. All subjects analyzed by Real-Time PCR showed an enhanced expression of the two genes, particularly of hABH2. This is the first study of hABH2 and hABH3 in pediatric brain tumors; further molecular investigations of their mutations and expression may help determine their role in response to chemotherapy.

Published

2009

203. Type A microsatellite instability in pediatric gliomas as an indicator of Turcot syndrome.

Author

Giunti L, Cetica V, Ricci U, Giglio S, Sardi I, Paglierani M, Andreucci E, Sanzo M, Forni M, Buccoliero AM, Genitori L, and Genuardi M

Subjects

Adolescent, Child, Child, Preschool, DNA analysis, DNA Mismatch Repair genetics, Female, Humans, Infant, Male, Pedigree, Syndrome, Biomarkers, Tumor genetics, Central Nervous System Neoplasms genetics, Colorectal Neoplasms, Hereditary Nonpolyposis genetics, Glioma genetics, Microsatellite Instability

Abstract

Microsatellite instability (MSI) is present in hereditary conditions due to mismatch repair (MMR) gene mutations. Following MSI analysis, tumor samples are classified into MSS (stable), MSI-L (low instability), and MSI-H (high instability) based on the fraction of unstable loci. Another MSI-based classification takes into account the size difference between mutant alleles in tumor DNA compared to wild-type alleles; two types of MSI, A and B, are recognized using this approach, type A being characterized by smaller, more subtle allelic shifts compared to type B. Biallelic mutations of MMR genes are associated with pediatric cancers, including glial tumors, in Turcot syndrome type 1 (TS1). However, most TS1-associated gliomas so far analyzed did not display MSI. We investigated the frequency of MSI in a series of 34 pediatric gliomas of different grade using a panel of five mononucleotide quasimonomorphic markers. Subtle qualitative changes were observed for the majority of markers in two glioblastomas (5.9% of the total series and 33.3% of glioblastomas). In both cases, family histories were compatible with TS1, and mutations of the PMS2 and MLH1 genes were identified. In one family, the MSI patterns were compared between the glioblastoma and a colon cancer from an affected relative, showing a clear qualitative difference, with the former displaying type A and the latter type B instability, respectively. These results were confirmed using additional microsatellite markers, indicating that knowledge of the association between TS1-related glial tumors and subtle type A MSI is important for full ascertainment of TS1 patients and appropriate counselling.

Published

2009

204. Clonality analysis of pediatric multiple tumors: two case reports and laboratory investigation.

Author

Giunti L, Bernini G, Forni M, Tucci F, Wheeler E, and Sardi I

Subjects

Adult, Antineoplastic Combined Chemotherapy Protocols therapeutic use, Autopsy, Base Sequence, Child, DNA Primers, DNA, Mitochondrial genetics, Fatal Outcome, Humans, Infant, Male, Neoplasms blood, Neoplasms pathology, Polymerase Chain Reaction, Polymorphism, Genetic, Polymorphism, Single Nucleotide, Sequence Deletion, Neoplasms genetics

Abstract

We examined the possibility of using microsatellite and mitochondrial DNA polymorphisms as markers to detect the clonal origin of tumor cells found in the same patient. We considered two children with complex tumor diseases: one with supratentorial primitive neuroectodermal tumors (PNET) and a hepatic rhabdoid tumor and another with brain and abdominal rhabdoid tumors. In the first patient we found an mtDNA cytosine insertion both in the normal tissue and in the primary tumor, whereas in the hepatic tumor we detected an insertion of 2 cytosine. In the second child, who had a constitutional mutation of hSNF5/INI-1, we identified the same mtDNA pattern both in normal tissue and in the abdominal tumor but not in the brain tumor, which presented three different mtDNA polymorphisms. Thus, we demonstrated the same clonal origin for tumors in the first patient and different clonal origins of the tumors in the second patient. At times it is very difficult to discriminate two neoplastic lesions or metastatic diseases by using only histopathologic techniques. Molecular examination of clonality is a useful tool to obtain information about the origin of synchronous and/or metachronous tumors found in the same patient.

Published

2006

205. [Epigenetic study of Rett's syndrome as an adequate model for autistic disorders].

Author

Iurov IIu, Vorsanova SG, Voinova-Ulas VIu, Villard L, Demidova IA, Giunti L, Guivabyccu-Uzielli ML, Budilov AV, Beresheva AK, Novikov PV, and Iurov IuV

Subjects

Child, DNA Mutational Analysis, Dosage Compensation, Genetic, Female, Humans, Methyl-CpG-Binding Protein 2, Mothers, Mutation, Missense genetics, Pedigree, Point Mutation genetics, Polymerase Chain Reaction, Receptors, Androgen genetics, Software, Chromosomal Proteins, Non-Histone genetics, Chromosomes, Human, X genetics, DNA-Binding Proteins genetics, Repressor Proteins genetics, Rett Syndrome genetics

Abstract

Rett's syndrome (RTT) is a severe hereditary disorder of the nervous system. MECP2 gene mutations are considered as a primary cause of the disease. In the present study, we have found MECP2 mutations in 33 (84.6%) out of 39 RTT females. We have also studied X-inactivation patterns in 70 girls with RTT. A frequency of skewed X-inactivation was 37% (26 patients), being significantly higher (p < 0.001) than that in the controls. The investigation of inactivated X chromosome origin revealed that about 33% pairs had preferentially the inactivated maternal X chromosome. An abnormal type of chromosome X inactivation was observed in all RTT females. Thus, we conclude that skewed X-inactivation may be considered as a common feature of RTT. There is unambiguous evidence that epigenetic alterations in RTT are associated with MECP2 mutations. MeCP2 protein also appears to be involved in transcriptional regulation of chromosome X genes. RTT in females without MECP2 mutations is related to the epigenetic alterations. We suggest X chromosome inactivation study in RTT females and their mothers to be informative for investigation of genetic processes in RTT girls, even in case MECP2 mutations have not been found. RTT could be considered as an appropriate model for studying epigenetic abnormalities in relation to autistic spectrum disorders.

Published

2005

206. Double incompatibility at human alpha fibrinogen and penta E loci in paternity testing.

Author

Nutini AL, Mariottini A, Giunti L, Torricelli F, and Ricci U

Subjects

Female, Humans, Male, Mutation, Polymorphism, Genetic, Sequence Analysis, DNA, Fibrinogen genetics, Tandem Repeat Sequences genetics

Abstract

We present a paternity testing case in which a double incompatibility was found for two short tandem repeat (STR) markers, human fibrinogen alpha (FGA) and Penta E. Analysis of the trio (mother, father, and daughter) included the amplification with a battery of 15 autosomal short tandem repeats (STR) by using a commercially available PowerPlex 16 System kit, and the detection with an ultraviolet-automatic sequencer. The biological paternity was confirmed with 12 additional markers. Reanalysis of the trio for the same markers with different primers was carried out by using an infrared automated sequencer and infrared-fluorescent primers. High paternity index confirmed that the observed inconsistencies were due to a double mutation, which was confirmed by sequence analysis at FGA and Penta E loci. Amplification and detection results obtained by the infrared-protocol showed consistent results with those obtained by ultraviolet-protocol and a commercially available kit. This has been our first case of double mutation at FGA and Penta E in a paternity testing. The use of our approach, based on two amplification and detection formats and on the sequence analysis, confirmed the observed meiotic paternal mutations.

Published

2003

207. Loss of heterozygosity and p53 polymorphism Pro72Arg in a young patient with medulloblastoma.

Author

Sardi I, Giunti L, Donati P, Lacitignola L, Tucci F, Sardo L, Giovannucci Uzielli ML, and Bernini G

Subjects

Cerebellar Neoplasms therapy, Child, Chromosomes, Human, Pair 17, Diagnosis, Differential, Female, Headache etiology, Humans, Magnetic Resonance Imaging, Medulloblastoma therapy, Nausea etiology, Vomiting etiology, Cerebellar Neoplasms genetics, Genes, p53 genetics, Loss of Heterozygosity, Medulloblastoma genetics, Polymorphism, Genetic

Abstract

Differently from conventional primary neuroectodermal tumors (PNETs), molecular features of undifferentiated lesions have been poorly studied. Medulloblastoma and PNET neoplasms showed a high incidence of loss of heterozygosity (LOH) on chromosome 17p13, in the region of tumor suppressor gene p53. Recent studies have shown a significant correlation between the presence of p53 Arg72Pro polymorphism and several undifferentiated carcinomas. We performed molecular analysis in an anaplastic tumor of posterior fossa in a patient with a constitutional maternal translocation [46,XX,t(5;19)] and a history of headache, nausea and vomiting. We identified the presence of LOH at 17p13 and Pro72Arg polymorphism in tumor DNA. These molecular findings helped us better characterize this undifferentiated tumor and led to a more aggressive therapy.

Published

2003

208. Analysis of 13 tetrameric short tandem repeat loci in a population of Tuscany (Central Italy) performed by means of an automated infrared sequencer.

Author

Ricci U, Sani I, Giunti L, Guarducci S, Coviello S, and Giovannucci Uzielli ML

Subjects

Gene Frequency, Genetics, Population, Humans, Italy, Spectrophotometry, Infrared methods, Sequence Analysis, DNA methods, Tandem Repeat Sequences genetics, White People genetics

Abstract

Allele frequencies for the 13 STRs of the Combined DNA Index System (CODIS) core were obtained from a sample of 188 unrelated individuals living in the area of Florence, Prato and Pistoia (Tuscany, Central Italy).

Published

2002

209. Infrared fluorescent automated detection of thirteen short tandem repeat polymorphisms and one gender-determining system of the CODIS core system.

Author

Ricci U, Sani I, Guarducci S, Biondi C, Pelagatti S, Lazzerini V, Brusaferri A, Lapini M, Andreucci E, Giunti L, and Giovannucci Uzielli ML

Subjects

Automation, DNA analysis, Humans, Indoles chemistry, Infrared Rays, Molecular Structure, Nucleic Acid Amplification Techniques, Reproducibility of Results, Sensitivity and Specificity, Templates, Genetic, Fluorescent Dyes chemistry, Minisatellite Repeats, Paternity, Polymorphism, Genetic, Sequence Analysis, DNA methods

Abstract

We used an infrared (IR) automated fluorescence monolaser sequencer for the analysis of 13 autosomal short tandem repeat (STR) systems (TPOX, D3S1358, FGA, CSF1PO, D5S818, D7S820, D8S1179, TH01, vWA, D13S317, D16S359, D18S51, D21S11) and the X-Y homologous gene amelogenin system. These two systems represent the core of the combined DNA index systems (CODIS). Four independent multiplex reactions, based on the polymerase chain reaction (PCR) technique and on the direct labeling of the forward primer of every primer pair, with a new molecule (IRDye800), were set up, permitting the exact characterization of the alleles by comparison with ladders of specific sequenced alleles. This is the first report of the whole analysis of the STRs of the CODIS core using an IR automated DNA sequencer. The protocol was used to solve paternity/maternity tests and for population studies. The electrophoretic system also proved useful for the correct typing of those loci differing in size by only 2 bp. A sensibility study demonstrated that the test can detect an average of 10 pg of undegraded human DNA. We also performed a preliminary study analyzing some forensic samples and mixed stains, which suggested the usefulness of using this analytical system for human identification as well as for forensic purposes.

Published

2000

210. Direct sequencing of long polymerase chain reaction fragments.

Author

Iannelli F, Giunti L, and Pozzi G

Subjects

DNA genetics, DNA, Bacterial chemistry, DNA, Bacterial genetics, Escherichia coli chemistry, Escherichia coli genetics, Polymerase Chain Reaction, Reproducibility of Results, Streptococcus pneumoniae chemistry, Streptococcus pneumoniae genetics, DNA chemistry, Sequence Analysis, DNA methods

Abstract

Direct sequencing of polymerase chain reaction (PCR)-generated templates is a commonly used technique in molecular biology laboratories. We describe an improved method for direct sequencing of PCR fragments longer than 20 kb obtained with a commercial mixture of Taq and Pwo DNA polymerases. The sequencing protocol was optimized for an automated infrared DNA sequencer, consistently yielding long reads (500-600 bases).

Published

1998