Abstract

The proposed research will contribute to solving one of the major remaining problems in lens research: the lack of knowledge about the three-dimensional structure nd the biological functions of alpha- crystallin. this does not only seriously hamper a rational approach towards cataract prevention, but is the more urgent considering the involvement of the alphaB-crystallin subunit as a stress-protein in many important pathological conditions outside the lens. Moreover, because of the structural and probably also functional homologies between alpha- crystallin and the small heat-shock proteins, this proposed research is also of direct relevance for a better insight in the properties of this increasingly important family of proteins. The specific objectives of this proposal, exploiting the possibilities of protein engineering techniques, are twofold: 1. Structural - To make site-directed and deletion/insertion mutants of both the alphaA- and alphaB-subunit of human alpha-crystallin in order to produce subunits, and domains thereof, that can be used for quaternary structure studies and that are suitable to obtain detailed tertiary structure information. To achieve this goal separate domains and site- directed mutants of alphaA- and alphaB-crystallin will be produced in E. coli by expression of the desired cDNA constructs. The influence of the mutations on aggregation will be determined. the recombinant proteins will be purified and used for crystallization studies for subsequent X- ray diffraction analysis. In case of monomeric subunits or domains, use will be made of 2D-NMR spectroscopic studies. 2. Functional - to study the effects of engineered mutants and natural variants of alphaA- and alphaB-crystallin on the biological properties of these proteins, such as: aggregation behavior and stability, membrane binding, protease inhibition, chaperone activity, intracellular translocation and thermoprotection, interaction with actin and intermediate filaments, phosphorylation and mRNA binding. In this manner insight of a fundamentally new type can be obtained about the residues and regions in alpha-crystallin that are involved in these various functional aspects. This goal will be approached by subjecting the domains and mutants to a variety of relevant assays. Where possible and relevant the mouse small heat-shock protein HSP25 will be included in the comparison.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Eye Institute (NEI)
Type
Research Project (R01)
Project #
5R01EY009683-03
Application #
2163364
Study Section
Visual Sciences A Study Section (VISA)
Project Start
1993-09-30
Project End
1996-09-29
Budget Start
1995-09-30
Budget End
1996-09-29
Support Year
3
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
Catholic University Nijmegen
Department
Type
DUNS #
City
Nijmegen
State
Country
Netherlands
Zip Code

  Publications

Smulders, Ronald H P H; van Dijk, Marjon A M; Hoevenaars, Simon et al. (2002) The eye lens protein alphaA-crystallin of the blind mole rat Spalax ehrenbergi: effects of altered functional constraints. Exp Eye Res 74:285-91
Smulders, R H; Kokke, B P; Gijsen, M L et al. (1998) The rodent alphaA-crystallin gene: mutagenesis of a non-consensus 5'-splice site to study alternative splicing in vivo. Mol Biol Rep 25:225-30
Boelens, W C; Croes, Y; de Ruwe, M et al. (1998) Negative charges in the C-terminal domain stabilize the alphaB-crystallin complex. J Biol Chem 273:28085-90
Smulders, R H; van Boekel, M A; de Jong, W W (1998) Mutations and modifications support a 'pitted-flexiball' model for alpha-crystallin. Int J Biol Macromol 22:187-96
Smulders, R H; de Jong, W W (1997) The hydrophobic probe 4,4'-bis(1-anilino-8-naphthalene sulfonic acid) is specifically photoincorporated into the N-terminal domain of alpha B-crystallin. FEBS Lett 409:101-4
Smulders RHPH; Carver, J A; Lindner, R A et al. (1996) Immobilization of the C-terminal extension of bovine alphaA-crystallin reduces chaperone-like activity. J Biol Chem 271:29060-6
Kantorow, M; Horwitz, J; van Boekel, M A et al. (1995) Conversion from oligomers to tetramers enhances autophosphorylation by lens alpha A-crystallin. Specificity between alpha A- and alpha B-crystallin subunits. J Biol Chem 270:17215-20
Smulders, R H; van Geel, I G; Gerards, W L et al. (1995) Reduced chaperone-like activity of alpha A(ins)-crystallin, an alternative splicing product containing a large insert peptide. J Biol Chem 270:13916-24
Smulders, R H; Merck, K B; Aendekerk, J et al. (1995) The mutation Asp69-->Ser affects the chaperone-like activity of alpha A-crystallin. Eur J Biochem 232:834-8
van den IJssel, P R; Overkamp, P; Knauf, U et al. (1994) Alpha A-crystallin confers cellular thermoresistance. FEBS Lett 355:54-6