Mutations in TBX1 genocopy the 22q11.2 deletion and duplication syndromes: a new susceptibility factor for mental retardation

Torres-Juan, Laura; Rosell, Jordi; Morlà, Montse; Vidal-Pou, Catalina; García-Algas, Fernando; Fuente, Maria-Angeles de la; Juan, M.; Tubau, A.; Bachiller, Daniel; Bernués, Marta; Pérez-Granero, Ángeles; Govea, Nancy; Busquets, Xavier; Heine-Suñer, Damián

doi:10.1038/sj.ejhg.5201819

Cited by 66 publications

(52 citation statements)

References 32 publications

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“…This suggests that the amount of TBX1 protein is crucial for normal development and that either loss or gain of TBX1 can cause DGS phenotypes. Consistent with a role in PA development, Tbx1 is expressed in the pharyngeal arch endoderm, core mesoderm, anterior heart field and head mesenchyme, but is absent in neural crest-derived mesenchyme (Chapman et al, 1996;Torres-Juan et al, 2007;Vitelli et al, 2002a).…”

Section: Introductionmentioning

confidence: 73%

“…Most cases of DGS are caused by deletion of chromosome 22q11.2, which includes the TBX1 gene. However, overexpression of human TBX1 in mice, or mutations that stabilize TBX1 in some DGS patients, also causes the same spectrum of DGS phenotypes (Torres-Juan et al, 2007;Zweier et al, 2007). This indicates that the level of expression of Tbx1 is crucial for PA formation.…”

Section: Discussionmentioning

confidence: 99%

“…Transgenic mice which have an additional human TBX1 gene and patients which have a mutation that stabilizes the TBX1 protein also develop DGS phenotypes (Liao et al, 2004;Torres-Juan et al, 2007;Zweier et al, 2007). This suggests that the amount of TBX1 protein is crucial for normal development and that either loss or gain of TBX1 can cause DGS phenotypes.…”

Section: Introductionmentioning

confidence: 99%

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β-catenin deficiency causes DiGeorge syndrome-like phenotypes through regulation of Tbx1

Huh

Ornitz

2010

Development

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SUMMARYDiGeorge syndrome (DGS) is a common genetic disease characterized by pharyngeal apparatus malformations and defects in cardiovascular, craniofacial and glandular development. TBX1 is the most likely candidate disease-causing gene and is located within a 22q11.2 chromosomal deletion that is associated with most cases of DGS. Here, we show that canonical Wnt-b-catenin signaling negatively regulates Tbx1 expression and that mesenchymal inactivation of b-catenin (Ctnnb1) in mice caused abnormalities within the DGS phenotypic spectrum, including great vessel malformations, hypoplastic pulmonary and aortic arch arteries, cardiac malformations, micrognathia, thymus hypoplasia and mislocalization of the parathyroid gland. In a heterozygous Fgf8 or Tbx1 genetic background, ectopic activation of Wnt-b-catenin signaling caused an increased incidence and severity of DGSlike phenotypes. Additionally, reducing the gene dosage of Fgf8 rescued pharyngeal arch artery defects caused by loss of Ctnnb1. These findings identify Wnt-b-catenin signaling as a crucial upstream regulator of a Tbx1-Fgf8 signaling pathway and suggest that factors that affect Wnt-b-catenin signaling could modify the incidence and severity of DGS.

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Section: Introductionmentioning

confidence: 73%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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β-catenin deficiency causes DiGeorge syndrome-like phenotypes through regulation of Tbx1

Huh

Ornitz

2010

Development

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“…This phenotype has been associated with lack of TBX1 in DiGeorge syndrome patients [9][10][11]42,43 and animal models. 12,13 Despite this, to date only 2 genes have been described as directly regulated by Tbx1.…”

Section: Discussionmentioning

confidence: 99%

Tbx1 Genetically Interacts With the Transforming Growth Factor-β/Bone Morphogenetic Protein Inhibitor Smad7 During Great Vessel Remodeling

Papangeli¹,

Scambler²

2013

Circulation Research

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Rationale: Growth and remodeling of the pharyngeal arch arteries are vital for the development of a mature great vessel system. Dysmorphogenesis of the fourth arch arteries can result in interruption of the aortic arch type B, typically found in DiGeorge syndrome. Tbx1 haploinsufficient embryos, which model DiGeorge syndrome, display fourth arch artery defects during formation of the vessels. Recovery from such defects is a documented yet unexplained phenotype in Tbx1 haploinsufficiency. Objective: To understand the nature of fourth arch artery growth recovery in Tbx1 haploinsufficiency and its underlying genetic control. Methods and Results: We categorized vessel phenotypes of Tbx1 heterozygotes as hypoplastic or aplastic at the conclusion of pharyngeal artery formation and compared these against the frequency of vessel defects scored at the end of great vessel development. The frequency of hypoplastic vessels decreased during embryogenesis, whereas no reduction of vessel aplasia was seen, implying recovery is attributable to remodeling of hypoplastic vessels. We showed that Smad7 , an inhibitory Smad within the transforming growth factor-β pathway, is regulated by Tbx1, is required for arch artery remodeling, and genetically interacts with Tbx1 in this process. Tbx1 and Tbx1 ; Smad7 haploinsufficiency affected several remodeling processes; however, concurrent haploinsufficiency particularly impacted on the earliest stage of vascular smooth muscle cell vessel coverage and subsequent fibronectin deposition. Conditional reconstitution of Smad7 with a Tbx1Cre driver indicated that the interaction between the 2 genes is cell autonomous. Conclusions: Tbx1 acts upstream of Smad7 controlling vascular smooth muscle and extracellular matrix investment of the fourth arch artery.

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“…Of note, mice that are haploinsufficient for TBX1 have several features which have been seen in humans with homologous deletions, in particular, structural cardiac anomalies [Baldini, 2005]. Recently, patients with normal 22q11.2 deletion studies using the commercially available FISH probes (N25 or TUPLE) but with overlapping clinical features of the deletion, have been reported with both gain and loss of function mutations in TBX1 [Yagi et al, 2003;Torres-Juan et al, 2007;Zweir et al, 2007], as well as, atypical or unique 22q11.2 deletions, some of which include TBX1 and others which do not [Kurahashi et al, 1996;O'Donnell et al, 1997;Yamagishi et al, 1998;Amati et al, 1999;McQuaide et al, 1999;Shaikh et al, 2000;GarciaMinaur et al, 2002;McDonald-McGinn et al, 2008]. Nonetheless, with the exception of congenital heart disease and its association with TBX1, to date, there have been no clear genotype-phenotype correlations in the remainder of the patients [McDonald-McGinn et al, 2001b, 2008.…”

mentioning

confidence: 99%

Genetic counseling for the 22q11.2 deletion

McDonald‐McGinn

Zackai

2008

Dev Disabil Res Revs

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Because of advances in palliative medical care, children with the 22q11.2 deletion syndrome are surviving into adulthood. An increase in reproductive fitness will likely follow necessitating enhanced access to genetic counseling for these patients and their families. Primary care physicians/obstetric practitioners are in a unique position to identify previously undiagnosed patients as they reach reproductive age and to refer them for genetic counseling. To date, most deletions are de novo, secondary to homologous recombination between low-copy repeat sequences located within 22q11.2. Nonetheless, both somatic and germ line mosaicism has been observed giving unaffected parents a small risk of recurrence. Once present though there is a 50% chance for a person with this contiguous deletion to have an affected child. With this in mind, a variety of prenatal monitoring techniques, as well as, preimplantation genetic diagnosis are available depending on the specific level of risk.

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Mutations in TBX1 genocopy the 22q11.2 deletion and duplication syndromes: a new susceptibility factor for mental retardation

Cited by 66 publications

References 32 publications

β-catenin deficiency causes DiGeorge syndrome-like phenotypes through regulation of Tbx1

β-catenin deficiency causes DiGeorge syndrome-like phenotypes through regulation of Tbx1

Tbx1 Genetically Interacts With the Transforming Growth Factor-β/Bone Morphogenetic Protein Inhibitor Smad7 During Great Vessel Remodeling

Genetic counseling for the 22q11.2 deletion

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