Abstract

The heterozygous deletion of a chromosomal region of human 22q11 is the genetic basis for several developmental defects with variable clinical severity. The clinical presentations may fit the diagnostic criteria for DiGeorge syndrome (DGS), Velocardiofacial syndrome (VCFS) or be very mild or complex. As the deletion is the unifying molecular element of these apparently diverse clinical entities, we will refer to these as the deletion 22q11 (del22q11) syndrome. Congenital heart disease, craniofacial anomalies, thymic and parathyroid aplasia and mental retardation are common findings in this syndrome. The 22q11 deletion, with an estimated incidence of 1:4000 live births, is one of the most frequent human chromosomal deletions associated with an abnormal phenotype. Almost twenty genes have been identified so far in the deleted region. However, a number of fundamental biological questions remains to be answered about the del22q11 syndrome: a) Is this a single or multiple gene disorder? b) Are any of the genes so far isolated from the deleted region relevant for the phenotype? c) What are the developmental pathways affected by the del22q11? To answer these questions, we propose to generate a panel of mouse embryonic stem (ES) cell lines carrying deletions, balancing duplications and single gene disruptions within the murine region homologous to the de122q11 region. These will be obtained using standard homologous recombination and a newly developed Cre-loxP strategy. Deletions will be designed to mimic the human mutations. The ES cell lines will be injected into mouse blastocysts to obtain the germ line transmission of the mutations. The phenotypic effects of deficiencies, single gene disruptions and combinations of these will be tested in vivo. This should allow us to perform a detailed genotype phenotype correlation study. Finally, the phenotype-generating deficiencies will be complemented in vivo to identify critical gene(s). This will be achieved using engineered balancer chromosomes or by reintroduction of genomic segments using standard mouse transgenic technologies. With this approach we will be able to dissect the del22q11 syndrome genetically and obtain mouse mutants which will be used to study the development of tissues and organs affected by this syndrome.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
2R01HL051524-04
Application #
2855377
Study Section
Mammalian Genetics Study Section (MGN)
Program Officer
Wang, Lan-Hsiang
Project Start
1996-05-05
Project End
2004-04-30
Budget Start
1999-05-01
Budget End
2000-04-30
Support Year
4
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Baylor College of Medicine
Department
Genetics
Type
Schools of Medicine
DUNS #
074615394
City
Houston
State
TX
Country
United States
Zip Code
77030

  Publications

Vitelli, Francesca; Huynh, Tuong; Baldini, Antonio (2009) Gain of function of Tbx1 affects pharyngeal and heart development in the mouse. Genesis 47:188-95
Xu, Huansheng; Baldini, Antonio (2007) Genetic pathways to mammalian heart development: Recent progress from manipulation of the mouse genome. Semin Cell Dev Biol 18:77-83
Huynh, Tuong; Chen, Li; Terrell, Phillip et al. (2007) A fate map of Tbx1 expressing cells reveals heterogeneity in the second cardiac field. Genesis 45:470-5
Dastjerdi, Akbar; Robson, Lesley; Walker, Rebecca et al. (2007) Tbx1 regulation of myogenic differentiation in the limb and cranial mesoderm. Dev Dyn 236:353-63
Zhang, Zhen; Huynh, Tuong; Baldini, Antonio (2006) Mesodermal expression of Tbx1 is necessary and sufficient for pharyngeal arch and cardiac outflow tract development. Development 133:3587-95
Vitelli, Francesca; Zhang, Zhen; Huynh, Tuong et al. (2006) Fgf8 expression in the Tbx1 domain causes skeletal abnormalities and modifies the aortic arch but not the outflow tract phenotype of Tbx1 mutants. Dev Biol 295:559-70
Xu, Huansheng; Cerrato, Fabiana; Baldini, Antonio (2005) Timed mutation and cell-fate mapping reveal reiterated roles of Tbx1 during embryogenesis, and a crucial function during segmentation of the pharyngeal system via regulation of endoderm expansion. Development 132:4387-95
Zhang, Zhen; Cerrato, Fabiana; Xu, Huansheng et al. (2005) Tbx1 expression in pharyngeal epithelia is necessary for pharyngeal arch artery development. Development 132:5307-15
Xu, Huansheng; Morishima, Masae; Wylie, John N et al. (2004) Tbx1 has a dual role in the morphogenesis of the cardiac outflow tract. Development 131:3217-27
Morishima, Masae; Yanagisawa, Hiromi; Yanagisawa, Masashi et al. (2003) Ece1 and Tbx1 define distinct pathways to aortic arch morphogenesis. Dev Dyn 228:95-104

Showing the most recent 10 out of 21 publications