Abstract

Tissues of the eye depend on families of specialized proteins. In the lens, the major proteins the crystallins. We have shown that in humans and other species, crystallins have arisen by a process called Gene Recruitement. Proteins such as enzymes and stress proteins have been recruited to serve an additionl structural role in lens transparency. The origins and functions of many classes of crystallins have been elucidated. Currently we are investigating the last major group for which a function is unknown. These are the related beta(b) and gamma (g) crystallins. Non-lens relatives of these proteins with stress and cancer related functions have been identified. This includes a novel gene expressed in non-lens eye tissues. This """"""""new gamma"""""""" (gN) has a gene structure that combines features of both b and g gene families. gN expression has been detected in retina by Northern blot and gN protein has been detected by 2D gels and mass spec in mouse lens. Recombinant gN is in crystalliization studies. We have shown that gS-crystallin is the major bg-crystallin in the adult human lens. In mouse, the gS gene is the locus of the Opj cataract. The Opj mice provide evidence for a role of gS in control of lens fiber cell structure. Recombinant wild type and mutant proteins for gS have been produced for functional studies. The mutant protein in Opj contains a temperature-sensitive destablizing mutation. Around mouse body temperature one domain unfolds and causes the protein to become insoluble. Recombinant protein is being used in both x-ray crystallographic and NMR structure studies. To separate the issues of mis-folded protein and loss-of-function in the Opj cataract, homologous recombination, """"""""knock-out"""""""" mice for the gS gene have been created. A homozygous -/- line for crygs is now being studied. The loss of function phenotype includes defects in both epithelial and fiber cells similar to some of the (more serious) defects in the Opj mice. gS crystallin appears to have a role in control of normal cell morphology and fiber cell maturation. In some species enzymes have been recruited as crystallins. We have produced recombinant protein for one of these, eta-crystallin, which is a retinaldehyde dehydrogenase that acts as a major crystallin in elepant shrews (macroscelids). A crystal structure has been determined in collaboration with the Birkbeck College group. This structure shows that the NAD(H) cofactor is avidly bound in the crystallized protein. This is consistent with the idea that eta-crystallin may have a protective role in the lens, sequestering NADH has a UV filter to reduce glare and protect against damage from bright sunlight.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Intramural Research (Z01)
Project #
1Z01EY000255-14
Application #
6659572
Study Section
(MSF)
Project Start
Project End
Budget Start
Budget End
Support Year
14
Fiscal Year
2002
Total Cost
Indirect Cost

  Institution

Name
U.S. National Eye Institute
Department
Type
DUNS #
City
State
Country
United States
Zip Code

  Publications

Aravind, Penmatsa; Wistow, Graeme; Sharma, Yogendra et al. (2008) Exploring the limits of sequence and structure in a variant betagamma-crystallin domain of the protein absent in melanoma-1 (AIM1). J Mol Biol 381:509-18
Nag, Nabanita; Peterson, Katherine; Wyatt, Keith et al. (2007) Endogenous retroviral insertion in Cryge in the mouse No3 cataract mutant. Genomics 89:512-20
Purkiss, Andrew G; Bateman, Orval A; Wyatt, Keith et al. (2007) Biophysical properties of gammaC-crystallin in human and mouse eye lens: the role of molecular dipoles. J Mol Biol 372:205-22
Smith, Amber A; Wyatt, Keith; Vacha, Jennifer et al. (2006) Gene duplication and separation of functions in alphaB-crystallin from zebrafish (Danio rerio). FEBS J 273:481-90
Vihtelic, Thomas S; Fadool, James M; Gao, James et al. (2005) Expressed sequence tag analysis of zebrafish eye tissues for NEIBank. Mol Vis 11:1083-100
Wu, Zhengrong; Delaglio, Frank; Wyatt, Keith et al. (2005) Solution structure of (gamma)S-crystallin by molecular fragment replacement NMR. Protein Sci 14:3101-14
Fan, Jianguo; Fariss, Robert N; Purkiss, Andrew G et al. (2005) Specific interaction between lens MIP/Aquaporin-0 and two members of the gamma-crystallin family. Mol Vis 11:76-87
Wistow, Graeme; Wyatt, Keith; David, Larry et al. (2005) gammaN-crystallin and the evolution of the betagamma-crystallin superfamily in vertebrates. FEBS J 272:2276-91
Evans, P; Wyatt, K; Wistow, G J et al. (2004) The P23T cataract mutation causes loss of solubility of folded gammaD-crystallin. J Mol Biol 343:435-44
Wallace, B A; Wien, Frank; Miles, Andrew J et al. (2004) Biomedical applications of synchrotron radiation circular dichroism spectroscopy: identification of mutant proteins associated with disease and development of a reference database for fold motifs. Faraday Discuss 126:237-43; discussion 245-54

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