Degroot L J, Torresani J, Carrayon P, Tirard A
Acta Endocrinol (Copenh). 1976 Oct;83(2):293-304. doi: 10.1530/acta.0.0830293.
Triiodothyronine (T3) may bind directly to receptors present in liver cell nuclei, or may be transported into nuclei by receptor protein(s) present in the cytosol. To evaluate these possibilities, T3 binding was studied in vitro using liver cell nuclei isolated from rats exposed in vivo to very low (H), normal (N),or high levels of T3 (H + T3), and using nuclei incubated in vitro with added cytosol proteins. Ka for T3 was 0.075 +/- 0.05 x 10(10) M-1 in N, 0.1 + 0.04 in H, and 0.094 + 0.04 in H + T3, and pg T3 bound/100 mug DNA were 47 +/- 17, 31 +/- 14, and 29 +/- 8 in the three groups. The data indicate no difference in binding capacity between the groups related to prior in vivo exposure to T3, and that T3 may bind directly to empty nuclear receptor sites. Rat liver cytosol proteins added to the in vitro incubation medium always depressed T3 uptake by nuclei. Bovine serum albumin had a similar effect. Large amounts of rat serum proteins depressed uptake, but low levels augmented T3 binding through an unknown mechanism. It is probable that free T3 in serum is in equilibrium with free T3 in the cytosol and nucleus, and binds directly to nuclear receptor proteins without mediation by a cytosol receptor protein.
三碘甲状腺原氨酸(T3)可能直接与存在于肝细胞核中的受体结合,或者可能通过存在于细胞质中的受体蛋白转运到细胞核中。为了评估这些可能性,使用从体内暴露于极低(H)、正常(N)或高水平T3(H + T3)的大鼠分离的肝细胞核,以及使用在体外与添加的细胞质蛋白一起孵育的细胞核,在体外研究了T3结合。在N组中,T3的Ka为0.075±0.05×10(10) M-1,在H组中为0.1 + 0.04,在H + T3组中为0.094 + 0.04,三组中每100μg DNA结合的T3 pg数分别为47±17、31±14和29±8。数据表明,与先前体内暴露于T3相关的各组之间的结合能力没有差异,并且T3可能直接与空的核受体位点结合。添加到体外孵育培养基中的大鼠肝脏细胞质蛋白总是会降低细胞核对T3的摄取。牛血清白蛋白有类似的作用。大量的大鼠血清蛋白会降低摄取,但低水平的大鼠血清蛋白会通过未知机制增强T3结合。血清中的游离T3可能与细胞质和细胞核中的游离T3处于平衡状态,并直接与核受体蛋白结合,而无需细胞质受体蛋白的介导。
