Abstract

The goal of this pilot proposal is to develop a system in which the expression of a reporter gene can be conditionally and reversibly inactivated in mammalian cells by regulating alternative splicing. This will be achieved by controlling the activity of an engineered splicing regulatory protein. Members of the SR protein family can function as splicing regulators by binding to alternative exons and enhancing the utilization of upstream splice sites. SR proteins are modular, containing separable RNA binding and splicing activation domains. In fact, the splicing activation domain can retain its function when fused to a heterologous RNA binding protein. Moreover, the splicing activation domain can even function when contained on a separate polypeptide than the RNA binding domain, provided that the two proteins can be physically juxtaposed. This has been achieved by fusing the RNA binding and splicing activation domains to the proteins FKBP and FRB, respectively. FKBP and FRB are two human proteins that do not interact with one another, but can be linked together by the small drug rapamycin (rap), which can simultaneously bind to both proteins. Rap can therefore be used to control the association of the RNA binding domain with the splicing activation domain, and thus regulate the alternative splicing of exons that contain binding sites for the regulator. Here, we propose to use this system to control alternative splicing in tissue culture cells. Specifically we will develop reporter genes in which a constitutively spliced intron disrupts the open reading frame for a reporter gene. Within this intron, we will insert an alternative exon containing in-frame stop codons and binding sites for the splicing regulator. Thus, when the alternative exon is included, no functional reporter will be produced. Experiments are described in each component of the alternative exon is optimized independently. Expression vectors encoding the RNA binding domain-FKBP and splicing activation domain-FRB fusion proteins will be used to test the ability of rap to inactivated expression of the reporter genes. Finally, the induction and decay kinetics of rap-induced alternative splicing will be determined. These experiments will result in the development of a novel system for conditionally and reversibly controlling gene expression. If successful, this system will be extended to conditionally and reversibly inactivate gene expression in transgenic mice. The availability of this method to study genes involved in bone development would significantly enhance our understanding of osteogenesis and will allow experiments to be performed that are not technically possible with the methods available today.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Arthritis and Musculoskeletal and Skin Diseases (NIAMS)
Type
Center Core Grants (P30)
Project #
5P30AR046026-02
Application #
6599985
Study Section
Special Emphasis Panel (ZAR1)
Project Start
2002-06-01
Project End
2003-05-31
Budget Start
Budget End
Support Year
2
Fiscal Year
2002
Total Cost
Indirect Cost

  Institution

Name
University of Connecticut
Department
Type
DUNS #
City
Farmington
State
CT
Country
United States
Zip Code
06030

  Publications

Jacquin, Claire; Koczon-Jaremko, Boguslawa; Aguila, Hector L et al. (2009) Macrophage migration inhibitory factor inhibits osteoclastogenesis. Bone 45:640-9
Chandhoke, Taranpreet K; Huang, Yu-Feng; Liu, Fei et al. (2008) Osteopenia in transgenic mice with osteoblast-targeted expression of the inducible cAMP early repressor. Bone 43:101-9
Liu, Fei; Lee, Sun-Kyeong; Adams, Douglas J et al. (2007) CREM deficiency in mice alters the response of bone to intermittent parathyroid hormone treatment. Bone 40:1135-43
Khosla, Sundeep (2007) Re: ""The 3.6 kb DNA fragment from the rat Col1a1 gene promoter drives the expression of genes in both osteoblast and osteoclast lineage cells"" by Boban et al. (Bone 39:1302-1312, 2006). Bone 40:1671-2;author reply 1673-4
Ardeshirpour, Laleh; Dann, Pamela; Adams, Douglas J et al. (2007) Weaning triggers a decrease in receptor activator of nuclear factor-kappaB ligand expression, widespread osteoclast apoptosis, and rapid recovery of bone mass after lactation in mice. Endocrinology 148:3875-86
He, Jianing; Rosen, Clifford J; Adams, Douglas J et al. (2006) Postnatal growth and bone mass in mice with IGF-I haploinsufficiency. Bone 38:826-35
Lee, Sun-Kyeong; Kadono, Yuho; Okada, Fumihiko et al. (2006) T lymphocyte-deficient mice lose trabecular bone mass with ovariectomy. J Bone Miner Res 21:1704-12
Sher, L B; Harrison, J R; Adams, D J et al. (2006) Impaired cortical bone acquisition and osteoblast differentiation in mice with osteoblast-targeted disruption of glucocorticoid signaling. Calcif Tissue Int 79:118-25
Lee, Sun-Kyeong; Kalinowski, Judith F; Jacquin, Claire et al. (2006) Interleukin-7 influences osteoclast function in vivo but is not a critical factor in ovariectomy-induced bone loss. J Bone Miner Res 21:695-702
Boban, Ivana; Jacquin, Claire; Prior, Katie et al. (2006) The 3.6 kb DNA fragment from the rat Col1a1 gene promoter drives the expression of genes in both osteoblast and osteoclast lineage cells. Bone 39:1302-12

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