Abstract

Vitamin A is an essential nutrient required not only for vision but also for the proper differentiation of many cell types in the body. This proposal seeks to define and study the molecular apparatus of the intestinal absorptive cell that carries out the necessary metabolism and movement of vitamin A during its transit of that cell during absorption. Particular elements under study are the enterocyte-specific retinol-binding protein, cellular retinol-binding protein II [CRBP(II)], a brush-border retinyl ester hydrolase, a brush-border retinol transporter, microsomal retinal reductase, and microsomal lecithin-retinol acyltransferase (LRAT).
The specific aims are to: 1.) Purify the brush-border retinyl ester hydrolase for physical and biochemical characterization and for production of antiserum for radioimmunoassay and immunolocalization. Its ontogeny and distribution along the gastrointestinal tract in rat and other species will be determined. Its physiological role will be tested by comparing its properties to the abilities of rat everted gut sacs and the human intestinal Caco-2 cell line to utilize retinyl esters. 2.) Characterize retinol transport in both rat everted gut sacs and the Caco-2 cell. Possible coupling of the putative retinol transporter with both the brush border retinyl ester hydrolase and with CRBP(II) will be tested. Evidence for specific uptake mechanisms for retinol bound to several retinol binding proteins will be sought. 3.) Purify and characterize microsomal retinal reductase and produce antiserum for immunolocalization. Its physiological function will be tested by comparing its developmental pattern and the stereospecificity of its reduction of retinal to the abilities/properties observed for everted gut sacs and Caco-2 cells. 4.) Purify and characterize LRAT and produce antiserum for radioimmunoassay and for immunolocalization, with particular reference to the localization of retinal reductase. Possible channeling of retinoid from the reductase to LRAT will be tested. The source of substrate lecithin will be examined by testing the potential role of phospholipid transfer proteins as substrate carrier.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
2R01DK032642-09
Application #
3231020
Study Section
Nutrition Study Section (NTN)
Project Start
1983-08-01
Project End
1996-11-30
Budget Start
1992-01-15
Budget End
1992-11-30
Support Year
9
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

Name
Vanderbilt University Medical Center
Department
Type
Schools of Medicine
DUNS #
004413456
City
Nashville
State
TN
Country
United States
Zip Code
37212

  Publications

Everts, Helen B; Sundberg, John P; King Jr, Lloyd E et al. (2007) Immunolocalization of enzymes, binding proteins, and receptors sufficient for retinoic acid synthesis and signaling during the hair cycle. J Invest Dermatol 127:1593-604
He, Quanhua; Alexeev, Dmitriy; Estevez, Maureen E et al. (2006) Cyclic nucleotide-gated ion channels in rod photoreceptors are protected from retinoid inhibition. J Gen Physiol 128:473-85
Swift, Larry L; Kakkad, Bharati; Boone, Cordelia et al. (2005) Microsomal triglyceride transfer protein expression in adipocytes: a new component in fat metabolism. FEBS Lett 579:3183-9
Swift, Larry L; Jovanovska, Aneta; Kakkad, Bharati et al. (2005) Microsomal triglyceride transfer protein expression in mouse intestine. Histochem Cell Biol 123:475-82
Everts, Helen B; Sundberg, John P; Ong, David E (2005) Immunolocalization of retinoic acid biosynthesis systems in selected sites in rat. Exp Cell Res 308:309-19
Li, Xiao-Hong; Kakkad, Bharati; Ong, David E (2004) Estrogen directly induces expression of retinoic acid biosynthetic enzymes, compartmentalized between the epithelium and underlying stromal cells in rat uterus. Endocrinology 145:4756-62
Everts, Helen B; King Jr, Lloyd E; Sundberg, John P et al. (2004) Hair cycle-specific immunolocalization of retinoic acid synthesizing enzymes Aldh1a2 and Aldh1a3 indicate complex regulation. J Invest Dermatol 123:258-63
Li, Xiao-Hong; Ong, David E (2003) Cellular retinoic acid-binding protein II gene expression is directly induced by estrogen, but not retinoic acid, in rat uterus. J Biol Chem 278:35819-25
Rexer, Brent N; Ong, David E (2002) A novel short-chain alcohol dehydrogenase from rats with retinol dehydrogenase activity, cyclically expressed in uterine epithelium. Biol Reprod 67:1555-64
Kuppumbatti, Y S; Rexer, B; Nakajo, S et al. (2001) CRBP suppresses breast cancer cell survival and anchorage-independent growth. Oncogene 20:7413-9

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