ABSTRACT
Introducción: El síndrome de X frágil (SXF) es una causa frecuente de retraso mental (RM), se presenta en 1 de 4 000 hombres y en 1 de 8 000 mujeres. A nivel molecular existen principalmente tres tipos de alteraciones: premutación, mutación completa y mosaicos, todas las cuales corresponden a amplificación del trinucleótido CGG localizado en el primer exón del gen FMR1: las premutaciones presentan entre 52 y 200 repetidos; las mutaciones completas, sobre 200 CGG, presentan hipermetilación de la región promotora del gen FMR1 e inhibición de la expresión de la proteína FMRP, causante del RM y dismorfias características de este síndrome. Los mosaicos presentan mutación completa y premutación o metilación parcial del gen FMR1. Los pacientes con SXF son diagnosticados clínicamente según un protocolo de tamizaje que considera 15 características clínicas que entrega un puntaje máximo de 30 puntos en individuos afectados. Objetivo: Definir criterios clínicos específicos para población chilena que ayuden a identificar a los individuos que deban ser sometidos a estudios moleculares confirmatorios de SXF. Pacientes y Método: Se consideraron 99 pacientes varones referidos al INTA por presentar retraso mental y características clínicas sugerentes del SXF; a todos se les realizó evaluación clínica utilizando el protocolo descrito por Buttler y estudio molecular con análisis directo del gen FMR1 por Southern blot. Resultados: 23 de los 99 pacientes estudiados presentaron una mutación en FMR1 y puntaje clínico entre 16 y 27 puntos; los 76 casos restantes con puntajes clínicos entre 10 y 26 puntos, no presentaron mutación en el gen FMR1. Se evaluaron las características clínicas en ambos grupos y se observó que 4 de ellas se asocian significativamente a la mutación, siendo tres de ellas independientes de la edad de los pacientes. Conclusiones: Con estos resultados y a fin de optimizar el estudio molecular directo del gen FMR1, proponemos que el criterio de selección de pacientes sea a través del examen clínico y que todo individuo con puntaje ³ 15 puntos debe ser sometido al estudio molecular.
Subject(s)
Humans , Male , Infant , Child, Preschool , Child , Adolescent , Adult , Genetic Testing , Intellectual Disability/genetics , Fragile X Syndrome/diagnosis , Fragile X Syndrome/genetics , Blotting, Southern , Chile , Trinucleotide Repeat Expansion/genetics , Genetic Markers , Methylation , Molecular Diagnostic Techniques , Mutation/genetics , Sex FactorsABSTRACT
Background: Prader-Willi syndrome (PWS) is a neurogenetic disease characterized by neonatal hypotonia, retarded mental and motor development, hypogonadism, hyperphagia, morbid obesity and dysmorphic facial features. It has an incidence of 1:12.000-15.000 newborns and is caused by abnormalities in genes located in 15q11q13. PWS is one of the most frequent genetic disorders and microdeletion syndromes. It is also the most common cause of obesity from genetic origin and it was the first disease in which imprinting and uniparental disomy were recognized as cause of genetic disorders. Seventy to seventy five percent of PWS cases are due to 15q11q13 deletions, 20-25percent to uniparental disomy and 1percent to mutations in the imprinting center. Aim: To analyze the clinical, genetic and molecular features of patients with PWS, seen at one institution. Patients and methods: Retrospective review of 45 patients (27 males) with PWS seen at the Genetics Outpatient Clinic at INTA. Results: Twenty three (51.1percent) patients had a delection, 13 (28.9percent) patients did not have a deletion. In nine patients, fluorescence in situ hybridization (FISH) study was not performed, therefore the presence of deletion was unknown. The clinical score was 8 points for patients younger than 3 years (n=11) and 11.5 points for patients older than 3 years (n=34); for patients aged 12 months or less, the clinical score was 7 points. Mean clinical score was 11 points for patients with deletion and 10 points for patients without deletion. Conclusions: Most patients with PWS have a deletion; the phenotype depends on age and the clinical score is useful for Chilean patients with PWS .
Subject(s)
Adolescent , Adult , Male , Humans , Female , Infant, Newborn , Infant , Child, Preschool , Child , Prader-Willi Syndrome/diagnosis , Prader-Willi Syndrome/genetics , Retrospective Studies , PhenotypeABSTRACT
Background: Several population studies have shown that patients with neural tube defects (NTD), have a higher frequency of a genetic mutation related with thermolability of the enzyme 5,10-metylentetrahydrofolate reductase (MTHFR). There are regional and ethnic variations in the genotypic or allelic frequency of this mutation and its possible relationship with NTD and others congenital anomalies. Aim: To estimate the frequency of the C677T polymorphism of MTHFR in control women and mothers of spina bifida cases. Patients and Methods: We analyzed 58 blood samples from mothers who had a child diagnosed with spina bifida. A group of 184 healthy mothers matched by age and with no NTD offspring served as controls. We determined the C677T polymorphism on the MTHFR gene by means of PCR and the analysis of the digestion pattern of HinfI restriction enzyme. Results: The genotypic frequencies showed concordance with Hardy-Weinberg equilibrium, in controls (p=0.35), and in mothers of the cases (p=0.95). The odds ratio to the TT genotype compared with the CC genotype (reference category) was estimated as 1.54 (IC 95%: 0,66-3,61), while the odds ratio for the TC genotype compared with CC genotype was 1.06 (IC 95%: 0,48-2,33). Conclusion: No differences in the C677T polymorphism of the MTHFR were observed between mothers who had a child diagnosed with spina bifida and control mothers (Rev Méd Chile 2003; 131: 1399-404).
Subject(s)
Humans , Female , Child , Adolescent , Adult , Middle Aged , Methylenetetrahydrofolate Dehydrogenase (NAD+)/genetics , Polymorphism, Genetic , Spinal Dysraphism/genetics , Alleles , Case-Control Studies , Chile , Genotype , Methylenetetrahydrofolate Dehydrogenase (NAD+)/blood , Mothers , Mutation , Spinal Dysraphism/bloodABSTRACT
Background: The diagnosis of Prader-Willi and Angelman syndromes is difficult, since their phenotypic manifestations are variable and unspecific. The study of the methylation state of DNA in l5(q11-q13) using polymerase chain reaction, called methylation test, allows the diagnosis of most patients with Prader-Willi and Angelman syndromes, irrespective if the underlying molecular alteration is a deletion, uniparental disomy or a punctual imprinting mutation. Aim: To assess the effectiveness of methylation test in the diagnosis of Prader-Willi and Angelman syndromes. Patients and methods : Thirty seven cases with a presumptive diagnosis of Prader-Willi syndrome and 25 with the presumptive diagnosis of Angelman syndrome were studied. Methylation test was done in genomic DNA obtained from peripheral Iymphocytes. Results: Methylation test confirmed the clinical diagnosis in 11 of 37 patients with PraderWilli (30 percent) and 6 of 25 patients with Angelman syndrome (24 percent). Conclusions: Clinical criteria overestimate the diagnosis of Prader-Willi and Angelman syndromes. The initial diagnosis should be confirmed with the methylation test and, if necessary, with FISH that will detect most deletions in the region