3-Hydroxykynurenine-mediated Modification of Human Lens Proteins

  • Staniszewska M
  • Nagaraj R
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Abstract

Tryptophan can be oxidized in the eye lens by both enzymatic and non-enzymatic mechanisms. Oxidation products, such as kynurenines, react with proteins to form yellow-brown pigments and cause covalent crosslinking. We generated a monoclonal antibody against 3-hydroxykynurenine (3OHKYN)-modified keyhole limpet hemocyanin and characterized it using 3OHKYN-modified amino acids and proteins. This monoclonal antibody reacted with 3OHKYN-modified N-acetyl lysine, N-acetyl histidine, N-acetyl arginine and N-acetyl cysteine. Among the several tryptophan oxidation products tested, 3OHKYN produced the highest concentration of antigen when reacted with human lens proteins. A major antigen from the reaction of 3OHKYN and N-acetyl lysine was purified by reversed phase HPLC, which was characterized by spectroscopy and identified as 2-amino-3-hydroxyl-[(5S)-5-acetamino-5-carboxypentyl amino]-oxo-benzene butanoic acid. Enzyme digested cataractous lens proteins displayed 3 O H K Y N-d e r i v e d m o d i f i c a t i o n s. Immunohistochemistry revealed 3OHKYN modifications in proteins associated with the lens fiber cell plasma membrane. The low molecular products (<10,000 Da) isolated from normal lenses after reaction with glucosidase followed by incubation with proteins generated 3OHKYN-derived products. Human lens epithelial cells incubated with 3OHKYN showed intense immunoreactivity. We also investigated the effect of glycation on tryptophan oxidation and kynurenine-mediated modification of lens proteins. The results showed that glycation products failed to oxidize tryptophan or generate kynurenine modifications in proteins. Our studies indicate that 3OHKYN modifies lens proteins independent of glycation to form products that may contribute to protein aggregation and browning during cataract formation.

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Staniszewska, M. M., & Nagaraj, R. H. (2005). 3-Hydroxykynurenine-mediated Modification of Human Lens Proteins. Journal of Biological Chemistry, 280(23), 22154–22164. https://doi.org/10.1074/jbc.m501419200

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