POSTTRANSLATIONAL ARGINYLATION IN THE BOVINE LENS

This study demonstrates post-translational arginylation of bovine serum albumin and endogenous lens proteins by bovine lens arginyl-tRNA: protein transferase. This reaction has been proposed to be the first step in marking specific proteins for degradation by the non-lysosomal. ATP-dependent, ubiquitin-mediated proteolytic pathway. The transferase was obtained by the method used for isolation of the same enzyme from reticulocytes (Ferber and Ciechanover, 1987, Nature326, 808-811). Incorporation of [3H]Arg was linear for at least 2 hr at 37°C. The amount of incorporation was directly proportional to the amount of lens enzyme or substrate added. Arginylation was ATP-dependent. A requirement for tRNA was demonstrated by inhibition upon pretreatment of the enzyme preparation with nuclease to hydrolyse endogenous tRNA, and restoration of activity upon replacement of tRNA. [3H]Leu, [3H]Lys and [3H]His were not incorporated, demonstrating specificity of the reaction for arginine. This is the first demonstration of post-translational modification of proteins by arginylation in the lens. © 1991.