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Título : Large deletions and point mutations involving the dedicator of cytokinesis 8 (DOCK8) in the autosomal-recessive form of hyper-IgE syndrome
Creador: Engelhardt KR
Nivel de acceso: Open access
Palabras clave : Genes Recesivos - genética - niño
Estudio de Asociación del Genoma Completo - métodos - niño
Factores de Intercambio de Guanina Nucleótido - genética - niño
Haplotipos - genética - niño
Homocigoto
Síndrome de Job - genética - child
Síndrome de Job - inmunologia - child
Síndrome de Job - patología - child
Mutación Puntual - genética - child
Polimorfismo de Nucleótido Simple - genética - child
Eliminación de Secuencia - genética - child
Linfocitos T - inmunologia - niño
Genes, Recessive - genetics - child
Genome-Wide Association Study - methods - child
Guanine Nucleotide Exchange Factors - genetics - child Haplotypes - genetics - child
Homozygote
Job Syndrome - genetics - child
Job Syndrome - immunology - child
Job Syndrome - pathology - child
Lymphocyte Activation - genetics - child
Lymphocyte Activation - immunology - child
Point Mutation genetics - child
Polymorphism, Single Nucleotide - genetics - child
Sequence Deletion - genetics - child
T-Lymphocytes - immunology - child
Síndrome autosómico recesivo hiperactivo-IgE, gen humano, mutación, DOCK8, inmunodeficiencia primaria, molusco contagioso, infección recurrente, Células TT, Células TH17, eosinófilos, Regulación de IgE, variaciones de número de copia, deleciones genómicas
Autosomal recessive hyper-IgE syndrome, human gene mutation, DOCK8, primary immunodeficiency, molluscum contagiosum, recurrent infection, T cells, TH17 cells, eosinophils, IgE regulation, copy number variations, genomic deletions
Descripción : The genetic etiologies of the hyper-IgE syndromes are diverse. Approximately 60% to 70% of patients with hyper-IgE syndrome have dominant mutations in STAT3, and a single patient was reported to have a homozygous TYK2 mutation. In the remaining patients with hyper-IgE syndrome, the genetic etiology has not yet been identified. OBJECTIVES: We aimed to identify a gene that is mutated or deleted in autosomal recessive hyper-IgE syndrome. METHODS: We performed genome-wide single nucleotide polymorphism analysis for 9 patients with autosomal-recessive hyper-IgE syndrome to locate copy number variations and homozygous haplotypes. Homozygosity mapping was performed with 12 patients from 7 additional families. The candidate gene was analyzed by genomic and cDNA sequencing to identify causative alleles in a total of 27 patients with autosomal-recessive hyper-IgE syndrome. RESULTS: Subtelomeric biallelic microdeletions were identified in 5 patients at the terminus of chromosome 9p. In all 5 patients, the deleted interval involved dedicator of cytokinesis 8 (DOCK8), encoding a protein implicated in the regulation of the actin cytoskeleton. Sequencing of patients without large deletions revealed 16 patients from 9 unrelated families with distinct homozygous mutations in DOCK8 causing premature termination, frameshift, splice site disruption, and single exon deletions and microdeletions. DOCK8 deficiency was associated with impaired activation of CD4+ and CD8+T cells. CONCLUSION: Autosomal-recessive mutations in DOCK8 are responsible for many, although not all, cases of autosomal-recessive hyper-IgE syndrome. DOCK8 disruption is associated with a phenotype of severe cellular immunodeficiency characterized by susceptibility to viral infections, atopic eczema, defective T-cell activation and T(h)17 cell differentiation, and impaired eosinophil homeostasis and dysregulation of IgE
Colaborador(es) u otros Autores: McGhee S
Winkler S
Sassi A
Woellner C
Lopez-Herrera G
Chen A
Kim HS
Lloret MG
Schulze I
Thiel J
Pfeifer D
Veelken H
Niehues T
Siepermann K
Weinspach S
Reisli I
Keles S
Genel F
Kutukculer N
Camcioğlu Y
Somer A
Karakoc-Aydiner E
Barlan I
Gennery A
Metin A
Degerliyurt A
Pietrogrande MC
Yeganeh M
Baz Z
Al-Tamemi S
Klein C
Puck JM
Holland SM
McCabe ER
Grimbacher B
Chatila TA.
Fecha de publicación : 2009
Tipo de publicación: Artículo
Formato: pdf
Identificador del Recurso : 10.1016/j.jaci.2009.10.038
Fuente: J Allergy Clin Immunol 124(6):1289-1302
URI : http://repositorio.pediatria.gob.mx:8180/handle/20.500.12103/2573
Idioma: eng
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