Abstract

This proposal is based on the hypothesis that the Insulin-like Growth Factors (IGF-I and IGF-II) are essential to the regulation of embryonic and fetal growth and development. We postulate that the IGFs, IGF receptors, and IGF binding proteins (IGFBPs) are expressed from early in embryogenesis, and that the time of onset and control of expression of these proteins differs depending on the stage of cellular maturation. Furthermore, because the IGFs have diverse biologic effects, we believe that all IGF in utero actions have not been defined. The goals of this proposal therefore, are to determine the time of inset of IGF, IGF receptor and IGFBP expression; to elucidate the factors that regulate IGFs in utero; and to define IGF actions and mechanisms of action important to development. Specifically, we will determine the ontogeny and sites of expression of the IGFs, IGF receptors and IGFBPs from pre-implantation embryogenesis through neonatal life in rats and mice (Spec.
Aim 1). To define the regulation IGF, IGF receptor and IGFBP expression during in utero and neonatal development (Spec.
Aim 2), we will assess the factors that modulate in vitro expression in embryonal carcinoma cell lines and in cultured fetal and neonatal rat fibroblasts. We also will evaluate in vivo expression of IGFs, IGF receptors and IGFBPs in tissues of fetal rats subjected to perturbations that result in intrauterine growth retardation and to the administration of substances found to alter the expression of these proteins in vitro. To determine the factors that stimulate IGF transcription (Spec.
Aim 3), we will study the regulation of expression of fusion genes linking IGF 5' genomic flanking elements to reporter genes in stably transfected cultured cells and transgenic mice. Using a number of transgenes designed to alter IGF expression, we will study in utero actions and mechanisms of action of IGFs in cultured stably transfected cells (Spec.
Aim 4) and transgenic mice (Spec.
aim 5). To investigate IGF actions, we will: a) create IGF-I expression in embryonic and fetal- derived cells that do not normally express IGF-I using transgenes that fuse either the metallothionein promoter or the mIGF-II genomic 5' flanking region to an IGF-IA gene, b) generate in utero IGF-I overexpression in transgenic mice using the fusion of MIGF-II 5' flanking IGFs and in transgenic mice using fusion genes that express anti-sense IGF transcripts or ribozymes that specifically cleave IGF transcripts. To examine the mechanisms of IGF-I's actions, we will: a) examine changes in the expression of IGF receptors and IGFBPs as a consequence of each of the above alterations in IGF expression, b) test IGF-I's potential autocrine actions, using transgenes expressing mutant IGF-I molecules that are not secreted either because they have amino acid (KDEL) trailer sequence targeting the endoplasmic reticulum or because they lack a signal peptide, and c) determine the effect of IGFBP-1 expression on IGF actions by study of cultured cells and transgenic mice made to express transgenes encoding hBP-1 and an anti-sense hBP-1 transcript (Spec.
Aim 6).

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Eunice Kennedy Shriver National Institute of Child Health & Human Development (NICHD)
Type
Research Project (R01)
Project #
5R01HD008299-19
Application #
3310848
Study Section
Endocrinology Study Section (END)
Project Start
1977-06-01
Project End
1996-05-31
Budget Start
1992-06-01
Budget End
1993-05-31
Support Year
19
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

Name
University of North Carolina Chapel Hill
Department
Type
Schools of Medicine
DUNS #
078861598
City
Chapel Hill
State
NC
Country
United States
Zip Code
27599

  Publications

Hu, Qichen; Lee, Seong Yong; O'Kusky, John R et al. (2012) Signalling through the type 1 insulin-like growth factor receptor (IGF1R) interacts with canonical Wnt signalling to promote neural proliferation in developing brain. ASN Neuro 4:
Liu, Wen; D'Ercole, Joseph A; Ye, Ping (2011) Blunting type 1 insulin-like growth factor receptor expression exacerbates neuronal apoptosis following hypoxic/ischemic injury. BMC Neurosci 12:64
Lehtinen, Maria K; Zappaterra, Mauro W; Chen, Xi et al. (2011) The cerebrospinal fluid provides a proliferative niche for neural progenitor cells. Neuron 69:893-905
Ye, Ping; Hu, Qichen; Liu, Hedi et al. (2010) beta-catenin mediates insulin-like growth factor-I actions to promote cyclin D1 mRNA expression, cell proliferation and survival in oligodendroglial cultures. Glia 58:1031-41
Moy, S S; Nadler, J J; Young, N B et al. (2009) Social approach in genetically engineered mouse lines relevant to autism. Genes Brain Behav 8:129-42
Liu, Wen; Ye, Ping; O'Kusky, John R et al. (2009) Type 1 insulin-like growth factor receptor signaling is essential for the development of the hippocampal formation and dentate gyrus. J Neurosci Res 87:2821-32
Joseph D'Ercole, A; Ye, Ping (2008) Expanding the mind: insulin-like growth factor I and brain development. Endocrinology 149:5958-62
Zhang, Jihui; Moats-Staats, Billie M; Ye, Ping et al. (2007) Expression of insulin-like growth factor system genes during the early postnatal neurogenesis in the mouse hippocampus. J Neurosci Res 85:1618-27
Zhang, Jihui; Liu, Wen; Ye, Ping et al. (2007) Pitfalls of PCR-based strategy for genotyping cre-loxP mice. Biotechniques 42:281, 283
Simmons, J G; Ling, Y; Wilkins, H et al. (2007) Cell-specific effects of insulin receptor substrate-1 deficiency on normal and IGF-I-mediated colon growth. Am J Physiol Gastrointest Liver Physiol 293:G995-1003

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