Wolfram Syndrome (Diabetes Insipidus, Diabetes, Optic Atrophy, and Deafness)

d’Annunzio, Giuseppe; Minuto, Nicola; D’Amato, Elena; Toni, Teresa De; Lombardo, Fortunato; Pasquali, Lorenzo; Lorini, Renata

doi:10.2337/dc08-0178

Cited by 45 publications

(41 citation statements)

References 11 publications

Supporting

Mentioning

Contrasting

Unclassified

Order By: Relevance

“…Mortality occurs in approximately 65% of patients before the age of 35, 59 primarily caused by central respiratory and renal failure, as well as brain stem atrophy. 62 While generally considered a rare disease in most countries, for example in the UK the prevalence is 1/770,000, 59 with a carrier frequency of 1/354, 63 some countries like Japan and Lebanon have higher incidences. 61,64 The nuclear gene responsible for this syndrome which spans 33.4 kb of genomic DNA was identified by two separate groups in 1998 and named WFS1.…”

Section: Hyperactivation Of the Uprmentioning

confidence: 99%

Stress hypERactivation in the β-cell

Fonseca

Urano²,

Burcin

et al. 2010

Islets

View full text Add to dashboard Cite

Section: Hyperactivation Of the Uprmentioning

confidence: 99%

Stress hypERactivation in the β-cell

Fonseca

Urano²,

Burcin

et al. 2010

Islets

View full text Add to dashboard Cite

“…To date, over 200 distinct mutations in WFS1 have been identified in WS individuals from different ethnic backgrounds, and these include a variety of missense, nonsense, and frameshift insertion/ deletion mutations [3,5,6,[13][14][15][16][17][18][19][20][21][22].…”

Section: Introductionmentioning

confidence: 99%

Identification of Novel Wsf1 Mutations in a Sicilian Child with Wolfram Syndrome

Pizzolanti¹

2014

J Genet Syndr Gene Ther

View full text Add to dashboard Cite

Wolfram Syndrome (WS) is a rare hereditary disease with autosomal recessive inheritance with incomplete penetrance. It is characterized by diabetes mellitus associated with progressive optic atrophy. The diagnosis is essentially clinical and mutation analysis is used to confirm the diagnosis. In the present study we describe the clinical and molecular features of a diabetic child carrying two novel WFS1 mutations. The Sicilian proband and his non-affected family were studied. Ophthalmologic examination included: visual acuity determination and funduscopy, optical coherent tomography, retinal fluorangiography, perimetry and electroretinogram. Molecular methods: automatic sequencing of PCR amplified WFS1 gene fragments and qRT-PCR analysis of WFS1 transcripts. 3 WSF1 mutations have been identified in the proband. One allele carries 2 paternally inherited mutations (c.1332 C>G and c.1631C>G) in exon-8, never annotated before, in heterozygosis with one "de novo" classic mutation (c.505 G>A) in exon-5. In addition, we report an unexpected molecular feature: higher WFS1 mRNA levels in the proband compared to the father. Milan, Italy) following manifacturer's instructions. A neuroblastoma cell line (LAN5) used as a positive control. WFS1 expression was analysed by real-time quantitative RT-PCR (qRT-PCR) in individual samples and WFS1 mRNA levels were quantified in comparison to β-actin mRNA expression. WFS1 PCR primers were purchased from Quiagen (Quantitect Primer Hs_WFS1_1_SG QT00082663) the amplicon size was 117 bp (Suppl. Figure 1); β-actin primers were obtained from RealTimePrimers.com (Elkins Park, PA, USA) with the following sequences: F 5'-GGACTTCGAGCAAGAGATGG-3'; R 5'-AGCACTGTGTTGGCGTACAG-3'; the amplicon size was 234 bp. All reactions were performed using the LightCycler 1.0 (Roche Diagnostics GMbH, Germany). Briefly, 2 g of total RNA was retrotranscribed using the ImProm-II™ Reverse Transcription System (Promega, Milan, Italy). Each RNA was combined with 1l of oligo16dT (Promega Milan, Italy) and thermally denatured at 70°C for 5 minutes and then chilled on ice. As a final step, the template-oligodT combination was added to the reaction mix (4 l ImProm-II™ 1X Reaction Buffer, 1l ImProm-II™ Reverse Transcriptase, 3.2 l Magnesium Chloride 3 mM, 1 l dNTPs mix 10 mM and 1 l Recombinant RNasin Ribonuclease Inhibitor 1u/l) and nuclease-free water was added to 20 l of final volume on ice. Following an initial annealing at 25°C for 5 minutes, the reaction was incubated at 42°C for one hour. In order to heat-inactivate the ImProm-II Reverse Transcriptase the reaction mix was finally incubated at 70°C for 15 minutes. Journal of Genetic Syndromes & Gene TherapyReal-time PCR was performed using 2 l of cDNA diluited 1:5, plus 10 l of Quantitech master mix (Qiagen), 2 l of Quantitect Primer Hs_WFS1_1_SG or β-actin primers, and nuclease-free water to 20 l of final volume. A standard reference curve was performed in parallel using RNAs extracted from LAN5 cell line serially 1:2 diluited starting from 100 ng reaction...

show abstract

“…Hasta el momento se han descrito más de 200 mutaciones distintas del gen WFS1. La mayoría de las mutaciones son únicas para un individuo o una familia, por lo que su naturaleza privada hace muy difícil el delinear una clara relación genotipo-fenotipo 32,56,57 . Las mutaciones se distribuyen aleatoriamente en toda la secuencia codificante del gen, pero hasta el 80% de las mutaciones reportadas hasta la fecha se encuentran en el exón 8 25,26,30,31,37,[56][57][58][59] .…”

Section: Discussionunclassified

“…La mayoría de las mutaciones son únicas para un individuo o una familia, por lo que su naturaleza privada hace muy difícil el delinear una clara relación genotipo-fenotipo 32,56,57 . Las mutaciones se distribuyen aleatoriamente en toda la secuencia codificante del gen, pero hasta el 80% de las mutaciones reportadas hasta la fecha se encuentran en el exón 8 25,26,30,31,37,[56][57][58][59] . En este estudio, el 60% de los pacientes (n = 3) cuentan con diagnóstico molecular y se trata de tres hermanos (los tres hombres del estudio) que presentan dos mutaciones en estado heterocigoto: la primera, heredada del padre, es una transición de guanina por citocina en el codón 177 que cambia una arginina por una prolina en el exón 5, y la segunda es una deleción de herencia materna de 16 pb (P451fsX515) en el exón 8 que cambia el marco de lectura y genera un codón de terminación prematura en la secuencia normal de la proteína.…”

Section: Discussionunclassified

Diabetes mellitus y atrofia óptica: estudio del síndrome de Wolfram

Rivas-Gómez

Reza-Albarrán

2017

GMM

View full text Add to dashboard Cite

Wolfram Syndrome (Diabetes Insipidus, Diabetes, Optic Atrophy, and Deafness)

Cited by 45 publications

References 11 publications

Stress hypERactivation in the β-cell

Stress hypERactivation in the β-cell

Identification of Novel Wsf1 Mutations in a Sicilian Child with Wolfram Syndrome

Diabetes mellitus y atrofia óptica: estudio del síndrome de Wolfram

Contact Info

Product

Resources

About