Wilber J F, Xu A H
Division of Endocrinology, University of Maryland Medical System, Baltimore 21201-1595.
Thyroid. 1998 Oct;8(10):897-901. doi: 10.1089/thy.1998.8.897.
Mechanisms of triiodothyronine (T3) negative regulation of the human thyrotropin-releasing hormone (TRH) gene were investigated with a chimeric construct of the 5' flanking region fused to a luciferase reporter gene, transfected into human neuroblastoma cells (HTB-11). Maximum negative regulation was achieved with constructs containing bases -242 to +54. Four sequences in this region exhibited homology with half sites of thyroid hormone response elements (TRE) (AGGTCA). The most important site was a sequence with an overlapping TRE/CRE, involving bases -53 to -60 (TGACCTCA). Potential combinatorial interactions of thyroid hormone receptors and CREB at this site were explored. Modest promoter stimulation was achieved with dibutyryl cyclic adenosine monophosphate (cAMP) (10(-3) M) plus IBMX (0.5 mM). Stimulation was greatly enhanced (+820%) by cotransfection of a constitutively activated protein kinase A (pPKA) construct. Cotransfection with pCREB increased stimulation further to 1350% above control. Stimulation of pPKA and pCREB interfered with stimulation by unliganded TRbeta1, and co-transfected pPKA and pCREB blocked T3 negative inhibition by TRbeta1-T3 complexes. When this site was mutated by polymerase chain reaction (PCR) mutagenesis, the mutant construct failed to respond to unliganded TRbeta1, and stimulation by pPKA and/or pCREB was inhibited markedly, from 12.5- to 2.1-fold, p < 0.001. Moreover, TRbeta1-T3 complexes failed to show any inhibition of the mutated promoter. These results suggest that negative regulation is achieved by inhibition of CREB stimulation of the TRH promoter at this overlapping TRE/CRE site. The two cosuppressors, NCoR and SMRT, were able to augment stimulation of the TRH promoter by unliganded TRbeta1 and enhance the magnitude of T3 inhibition. The potential role of the TRH gene and the pathophysiology of thyroid hormone resistance was investigated with three mutant TRbeta1 constructs. Thyroid hormone resistance was found to be expressed at the level of TRH gene regulation, due to lowered inhibition by mutant TRbeta1-T3 complexes and by their dominant negative effects on wild-type TRbeta1-T3 inhibition. TRH gene expression has been identified in the heart. Cardiac TRH mRNA was not regulated by T3, in contrast to HTB-11 cells, but cardiac TRH mRNA density could be augmented by glucocorticoids and by testosterone. TRH receptors were identified using Scatchard blots that showed a kilodalton of 1.4 nM and a bmax of 10 pmol/mg protein. TRH-R mRNA was identified also by reverse transcription polymerase chain reaction (RT-PCR). Enhanced ventricular contractility by TRH was demonstrated in both an open-chested dog preparation and in ex vivo ventricular myocytes, using video edge cinematography. Under controlled conditions, myocyte shortening was 13.3%, and TRH (10(-6) M) caused muscle shortening to increase 140%, (p < 0.005). TRH gene expression was demonstrated exclusively in Leydig cells of the testis. High affinity binding sites were identified in testicular membranes with a kilodalton of 1.6 x 10(-6) M. TRH was able to inhibit LH and HCG-activated testosterone secretion significantly. Thus, one paracrine role of TRH in the testis may be to serve as inhibitory modulator of gonadotropin-stimulated testosterone secretion.
利用与荧光素酶报告基因融合的5'侧翼区嵌合构建体,转染到人神经母细胞瘤细胞(HTB - 11)中,研究了三碘甲状腺原氨酸(T3)对人促甲状腺激素释放激素(TRH)基因的负调控机制。含有碱基-242至+54的构建体实现了最大程度的负调控。该区域的四个序列与甲状腺激素反应元件(TRE)(AGGTCA)的半位点具有同源性。最重要的位点是一个具有重叠TRE/CRE的序列,涉及碱基-53至-60(TGACCTCA)。探讨了甲状腺激素受体和CREB在该位点的潜在组合相互作用。用二丁酰环磷酸腺苷(cAMP)(10⁻³ M)加异丁基甲基黄嘌呤(IBMX)(0.5 mM)可实现适度的启动子刺激。通过共转染组成型激活的蛋白激酶A(pPKA)构建体,刺激作用大大增强(增加820%)。与pCREB共转染进一步将刺激作用提高到比对照高1350%。pPKA和pCREB的刺激干扰了未结合配体的TRβ1的刺激,共转染的pPKA和pCREB阻断了TRβ1 - T3复合物对T3的负抑制作用。当通过聚合酶链反应(PCR)诱变使该位点发生突变时,突变构建体对未结合配体的TRβ1无反应,并且pPKA和/或pCREB的刺激作用明显受到抑制,从12.5倍降至2.1倍,p < 0.001。此外,TRβ1 - T3复合物对突变的启动子没有任何抑制作用。这些结果表明,通过在这个重叠的TRE/CRE位点抑制CREB对TRH启动子的刺激来实现负调控。两种共抑制因子NCoR和SMRT能够增强未结合配体的TRβ1对TRH启动子的刺激作用,并增强T3抑制的程度。用三种突变的TRβ1构建体研究了TRH基因的潜在作用和甲状腺激素抵抗的病理生理学。发现甲状腺激素抵抗在TRH基因调控水平表达,这是由于突变的TRβ1 - T3复合物的抑制作用降低以及它们对野生型TRβ1 - T3抑制的显性负效应。已在心脏中鉴定出TRH基因表达。与HTB - 11细胞不同,心脏TRH mRNA不受T3调控,但糖皮质激素和睾酮可增加心脏TRH mRNA密度。使用Scatchard印迹法鉴定了TRH受体,其解离常数为1.4 nM,最大结合容量为10 pmol/mg蛋白质。还通过逆转录聚合酶链反应(RT - PCR)鉴定了TRH - R mRNA。在开胸犬制备模型和离体心室肌细胞中,利用视频边缘摄影术证明TRH可增强心室收缩力。在对照条件下,心肌细胞缩短率为13.3%,TRH(10⁻⁶ M)使肌肉缩短增加140%,(p < 0.005)。TRH基因表达仅在睾丸的Leydig细胞中得到证实。在睾丸膜中鉴定出高亲和力结合位点,解离常数为1.6×10⁻⁶ M。TRH能够显著抑制促黄体生成素(LH)和人绒毛膜促性腺激素(HCG)激活的睾酮分泌。因此,TRH在睾丸中的一个旁分泌作用可能是作为促性腺激素刺激的睾酮分泌的抑制性调节剂。
