正常甲状腺功能大鼠培养的垂体前叶细胞对甲状腺素的摄取
Uptake of thyroxine in cultured anterior pituitary cells of euthyroid rats.
作者信息
Everts M E, Docter R, Moerings E P, van Koetsveld P M, Visser T J, de Jong M, Krenning E P, Hennemann G
机构信息
Department of Internal and Nuclear Medicine, Erasmus University Medical School, Rotterdam, The Netherlands.
出版信息
Endocrinology. 1994 Jun;134(6):2490-7. doi: 10.1210/endo.134.6.8194475.
The uptake of [125I]T4 was investigated in cultured anterior pituitary cells isolated from adult fed Wistar rats and cultured for 3 days in medium containing 10% fetal calf serum. Experiments were performed with [125I]T4 (10(5) to 2 x 10(6) cpm; 0.35-7 nM) in medium containing 0.5% or 0.1% BSA. The uptake of [125I]T4 increased with time and showed equilibrium after around 1 h of incubation. The presence of 10 microM unlabeled T4 during incubation decreased the uptake of [125I]T4 by 65-70% at all time intervals. After 24 h of incubation, 1.5% iodide and 3.2% conjugates were detected in the medium, whereas around 20% of cellular radioactivity represented [125I]T3. The 15-min uptake of [125I]T4 was significantly reduced by simultaneous incubation with 100 nM T4 (by 24%; P < 0.05), 100 nM T3 (by 38%; P < 0.001), or 10 microM rT3 (by 32%; P < 0.001), whereas 10 microM tetraiodothyroacetic acid (Tetrac) had no effect. Furthermore, preincubation (30 min) and incubation (15 min) with 10 microM monodansylcadaverine, oligomycin, or monensin reduced the uptake of [125I]T4 by 30%, 50%, and 40%, respectively (all P < 0.001). Substitution of Na+ in the buffer by K+ diminished the uptake of [125I]T4 by 39% (P < 0.005); 2 mM phenylalanine, tyrosine, or tryptophan reduced [125I]T4 uptake by 18% (P < 0.05), 18% (P = NS), and 33% (P < 0.005), respectively. Our data suggest that the pituitary contains a specific carrier-mediated energy-requiring mechanism for [125I]T4 uptake that is partly dependent on the Na+ gradient. In addition, part of [125I]T4 uptake in the pituitary might occur through an amino acid transport system. When expressed per pM of free hormone, the 15-min uptake of [125I]T4 was approximately as high as that of [125I]T3. Because the reduction of [125I]T4 uptake by T4, T3, monodansylcadaverine, oligomycin, and monensin was roughly the same as the previously reported reduction of [125I]T3 uptake by the same compounds, it is further suggested that T4 and T3 share a common carrier in cultured anterior pituitary cells.
在从成年Wistar大鼠分离并在含10%胎牛血清的培养基中培养3天的培养垂体前叶细胞中,研究了[125I]T4的摄取情况。实验使用含0.5%或0.1%牛血清白蛋白(BSA)的培养基中的[125I]T4(10⁵至2×10⁶ cpm;0.35 - 7 nM)进行。[125I]T4的摄取随时间增加,孵育约1小时后达到平衡。孵育期间存在10 μM未标记的T4,在所有时间间隔内,[125I]T4的摄取降低了65 - 70%。孵育24小时后,培养基中检测到1.5%的碘化物和3.2%的结合物,而约20%的细胞放射性代表[125I]T3。与100 nM T4(降低24%;P < 0.05)、100 nM T3(降低38%;P < 0.001)或10 μM反式三碘甲状腺原氨酸(rT3)(降低32%;P < 0.001)同时孵育,显著降低了[125I]T4的15分钟摄取,而10 μM四碘甲状腺乙酸(Tetrac)没有影响。此外,与10 μM单丹磺酰尸胺、寡霉素或莫能菌素预孵育(30分钟)和孵育(15分钟)分别使[125I]T4的摄取降低30%、50%和40%(均P < 0.001)。用K⁺替代缓冲液中的Na⁺使[125I]T4的摄取降低39%(P < 0.005);2 mM苯丙氨酸、酪氨酸或色氨酸分别使[125I]T4摄取降低18%(P < 0.05)、18%(P = 无显著性差异)和33%(P < 0.005)。我们的数据表明垂体含有一种特定的、载体介导的、需要能量的[125I]T4摄取机制,该机制部分依赖于Na⁺梯度。此外,垂体中[125I]T4摄取的一部分可能通过氨基酸转运系统发生。以每皮摩尔游离激素表示时,[125I]T4的15分钟摄取与[125I]T3大致相同。由于T4、T3、单丹磺酰尸胺、寡霉素和莫能菌素对[125I]T4摄取的降低与先前报道的这些化合物对[125I]T3摄取的降低大致相同,进一步表明T4和T3在培养的垂体前叶细胞中共享一个共同载体。
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