The identity and nuclear uptake of a cytosolic binding protein for 3-methylcholanthrene

The ability of 3-methylcholanthrene to interact noncovalently with rat liver cytosolic proteins was studied using Sephadex G200 chromatography. A specific 3-methylcholanthrene binding fraction from Sephadex G200 chromatography, termed peak B, when incubated with rat liver nuclei was able to translocate 3-methylcholanthrene into the nucleus. This translocation occurred faster and was quantitatively greater than the binding of 3-methylcholanthrene in buffer to nuclei. In addition, the nuclear uptake of peak B was increased by prewarming, suggesting that a heat-sensitive activation step may occur prior to the translocation process. However, no evidence was found on sucrose gradients for any conformational change in the protein fraction studied here. The translocation to the nucleus was temperature and time dependent. An examination of the characteristics of this 3-methylcholanthrene binding protein using Sephacryl S200 column chromatography showed a small number of high-affinity, saturable, binding sites to be present. These had an apparent dissociation constant, K_d, of 2.8 nm and a binding capacity of 770 fmol/mg of cytosolic protein. The selectivity of this protein was examined by competition studies and, in general, polycyclic hydrocarbons competed for the binding site, except for anthracene and phenanthrene. Of the inducers studied, 5,6-benzoflavone was a strong competitor. No competition was found with 12-O-tetradecanoyl phorbol-13-acetate, 2,6-ditertbutyl-p-cresol, β-retinyl acetate, or a number of steroids, except for 17β-estradiol which exhibited moderate binding. Peak B had a sedimentation coefficient of 4.2 S when analyzed on a linear sucrose gradient. Chromatography of peak B on a calibrated Sephacryl S200 column gave a molecular weight corresponding to 44,600 ± 4000.