Properties of triiodothyronine-binding proteins in liver cytosol of rat

Abstract

The electrophoretic mobility and the sedimentation coefficient were determined in partially purified preparations of both rat liver cytosol and serum triiodothyronine (T₃)-binding proteins. Crude cytosol and serum, each labeled with [¹²⁵I]T₃, were filtered through a Sephadex G-100 column. The cytosol yielded a single T₃-binding peak, whereas three binding components were recognized in the serum. Protamine sulfate precipitated the cytosol T₃-binding protein, but had no effect on the serum T₃-binders. The cytosol protein and the three binding proteins from serum were analyzed by polyacrylamide gel electrophoresis and sucrose density gradient centrifugation. The cytosol binder migrated as a single peak on gel electrophoresis with an R_f of 0.53, whereas the serum proteins had R_fs between 0.27–0.33. The sedimentation coefficient of the cytosol protein was 6.3 S, whereas it was 4.1 S for the major binding protein of the serum. These data indicate that: (i) preliminary purification by gel chromatography is a useful step for better characterization of the T₃-binding proteins of the cytosol and serum; (ii) the cytosol binder is an acidic protein with completely different properties from those of the serum T₃-binding proteins.