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敲低与卡尼综合征相关的基因PRKAR1A会干扰成骨细胞的分化。

Knockdown of PRKAR1A, the gene responsible for Carney complex, interferes with differentiation in osteoblastic cells.

作者信息

Zhang Mei, Manchanda Parmeet K, Wu Dayong, Wang Qianben, Kirschner Lawrence S

机构信息

Departments of Molecular, Virology, Immunology, and Medical Genetics (M.Z., P.K.M., L.S.K.) and Molecular and Cellular Biochemistry (D.W., Q.W.) and Division of Endocrinology, Diabetes, and Metabolism (L.S.K.), The Ohio State University, Columbus, Ohio 43210.

出版信息

Mol Endocrinol. 2014 Mar;28(3):295-307. doi: 10.1210/me.2013-1152. Epub 2014 Feb 7.

Abstract

PRKAR1A is the gene encoding the type 1A regulatory subunit of protein kinase A, and it is the cause of the inherited human tumor syndrome Carney complex. Data from our laboratory has demonstrated that Prkar1a loss causes tumors in multiple cell lineages, including neural crest cells and osteoblasts. We have proposed that one mechanism by which tumorigenesis occurs is through the failure of terminal differentiation. In the present study, we directly test the effects of Prkar1a reduction on osteogenic differentiation in mouse and human cells in vitro. We found that Prkar1a levels noticeably increased during osteoblastic differentiation, indicating a positive correlation between the expression of Prkar1a and osteogenic potential. To validate this hypothesis, we generated stable Prkar1a knockdown in both mouse and human cells. These cells displayed significantly suppressed bone nodule formation and decreased expression of osteoblast markers such as osteocalcin and osteopontin. These observations imply that the antiosteogenic effect of Prkar1a ablation is not species or cell line specific. Furthermore, because Runt-related transcription factor-2 (Runx2) is a key mediator of osteoblast differentiation, we reasoned that the function of this transcription factor may be inhibited by Prkar1a knockdown. Chromatin immunoprecipitation and luciferase assays demonstrated that Prkar1a ablation repressed DNA binding and function of Runx2 at its target genes. Additionally, we determined that this effect is likely due to reductions in the Runx2-cooperating transcription factors forkhead box O1 and activating transcription factor 4. Taken together, this study provides direct evidence that ablation of Prkar1a interferes with signaling pathways necessary for osteoblast differentiation.

摘要

PRKAR1A是编码蛋白激酶A 1A型调节亚基的基因,它是遗传性人类肿瘤综合征卡尼综合征的病因。我们实验室的数据表明,Prkar1a缺失会导致多种细胞谱系发生肿瘤,包括神经嵴细胞和成骨细胞。我们提出肿瘤发生的一种机制是终末分化失败。在本研究中,我们直接测试了Prkar1a表达降低对小鼠和人类细胞体外成骨分化的影响。我们发现,在成骨细胞分化过程中,Prkar1a水平显著升高,表明Prkar1a的表达与成骨潜能呈正相关。为了验证这一假设,我们在小鼠和人类细胞中均构建了稳定的Prkar1a基因敲低模型。这些细胞显示出骨结节形成明显受到抑制,成骨细胞标志物如骨钙素和骨桥蛋白的表达降低。这些观察结果表明,Prkar1a缺失的抗成骨作用不具有物种或细胞系特异性。此外,由于Runx2相关转录因子2(Runx2)是成骨细胞分化的关键调节因子,我们推测该转录因子的功能可能会受到Prkar1a基因敲低的抑制。染色质免疫沉淀和荧光素酶分析表明,Prkar1a缺失会抑制Runx2在其靶基因上的DNA结合和功能。此外,我们确定这种效应可能是由于Runx2协同转录因子叉头框O1和激活转录因子4的减少所致。综上所述,本研究提供了直接证据,表明Prkar1a缺失会干扰成骨细胞分化所需的信号通路。

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