Fluorescamine staining of nonhistone chromatin proteins as revealed by two-dimensional polyacrylamide gel electrophoresis

Pure [³H]ethyltubulin dimer, containing 1.07 mol of [³H]ethyl groups/110.000 g protein was prepared by reaction of tubulin with acetaldehyde and [³H]sodium borohydride. The derivatized tubulin dimer was shown to be native by the following criteria: (1) the stoichiometry for [³H]GDP binding was similar to that for native tubulin: (2) it repeatedly copolymerized and codepolymerized with native tubulin with constant specific activity. The potential utility for [³H]ethyltubulin in quantitating tubulin in biological samples by isotope dilution, and in studying the relationships between microtubules, rings, and dimers is discussed.