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USF1和USF2介导Mash-2和缺氧对人滋养层细胞分化及CYP19基因表达的抑制作用。

USF1 and USF2 mediate inhibition of human trophoblast differentiation and CYP19 gene expression by Mash-2 and hypoxia.

作者信息

Jiang Bing, Mendelson Carole R

机构信息

Department of Biochemistry, The University of Texas Southwestern Medical Center, Dallas, Texas 75390-9038, USA.

出版信息

Mol Cell Biol. 2003 Sep;23(17):6117-28. doi: 10.1128/MCB.23.17.6117-6128.2003.

Abstract

In the human placental syncytiotrophoblast, C(19) steroids are converted to estrogens by aromatase P450, product of the CYP19 gene. When human cytotrophoblasts, which lack the capacity to express aromatase, are cultured in 20% O(2), they spontaneously fuse to form a multinuclear syncytiotrophoblast and CYP19 expression is markedly induced. On the other hand, when cytotrophoblasts are cultured in 2% O(2), syncytiotrophoblast differentiation and induction of CYP19 expression are prevented. We previously observed that expression of the transcription factor Mash-2 (mammalian achaete/scute homologue 2), which is elevated in human cytotrophoblasts and maintained at elevated levels by hypoxia, declines with syncytiotrophoblast differentiation. Overexpression of Mash-2 prevents syncytiotrophoblast differentiation and induction of CYP19 expression. In the present study, we observed that unexpectedly immunoreactive Mash-2 protein was localized predominantly to the cytoplasm of human cytotrophoblasts. Elevated cytoplasmic levels of Mash-2 were maintained when trophoblasts were cultured in 2% O(2) and declined to undetectable levels upon culture in 20% O(2). Previously, we found that Mash-2 inhibited CYP19 promoter activity through sequences within a 350-bp region upstream and within placenta-specific exon I.1 containing three E boxes (E1 at -325 bp, 5'-CACTTG-3'; E2 at -58 bp, 5'-CACATG-3'; and E3 at +26 bp, 5'-CACGTG-3'). In this study, we found that trophoblast nuclear protein binding to these E boxes declined with syncytiotrophoblast differentiation in 20% O(2) and was induced by hypoxia; however, Mash-2 did not appear to bind to any of these E boxes. On the other hand, the basic helix-loop-helix leucine zipper transcription factors upstream stimulatory factors 1 and 2 (USF1 and USF2) did bind to E2 and E3 but not E1. Nuclear levels of USF1 and USF2 and DNA-binding activity declined with syncytiotrophoblast differentiation and were maintained at elevated levels by hypoxia and overexpression of Mash-2, whereas USF1 mRNA levels were unaffected. Finally, USF1 overexpression in cultured human trophoblasts markedly inhibited endogenous CYP19 expression, differentiation of cultured human trophoblast cells, and CYP19 promoter activity. These findings suggest that increased protein levels and DNA binding of USF1 and USF2 mediate the inhibitory effects of hypoxia and of Mash-2 on CYP19 gene expression in human placenta.

摘要

在人胎盘合体滋养层细胞中,C(19)类固醇通过CYP19基因产物芳香化酶P450转化为雌激素。当缺乏芳香化酶表达能力的人细胞滋养层细胞在20% O(2)中培养时,它们会自发融合形成多核合体滋养层细胞,且CYP19表达被显著诱导。另一方面,当细胞滋养层细胞在2% O(2)中培养时,合体滋养层细胞分化及CYP19表达的诱导受到抑制。我们之前观察到,转录因子Mash-2(哺乳动物achaete/scute同源物2)在人细胞滋养层细胞中表达升高,并在缺氧条件下维持在较高水平,其表达会随着合体滋养层细胞分化而下降。Mash-2的过表达可阻止合体滋养层细胞分化及CYP19表达的诱导。在本研究中,我们意外地观察到,具有免疫反应性的Mash-2蛋白主要定位于人细胞滋养层细胞的细胞质中。当滋养层细胞在2% O(2)中培养时,Mash-2的细胞质水平升高,而在20% O(2)中培养时则降至检测不到的水平。此前,我们发现Mash-2通过胎盘特异性外显子I.1内及上游350 bp区域内包含三个E盒(-325 bp处的E1,5'-CACTTG-3';-58 bp处的E2,5'-CACATG-3';+26 bp处的E3,5'-CACGTG-3')的序列抑制CYP19启动子活性。在本研究中,我们发现,在20% O(2)中,滋养层细胞核蛋白与这些E盒的结合随着合体滋养层细胞分化而下降,并在缺氧时被诱导;然而,Mash-2似乎不与这些E盒中的任何一个结合。另一方面,碱性螺旋-环-螺旋转录因子上游刺激因子1和2(USF1和USF2)确实与E2和E3结合,但不与E1结合。USF1和USF2的核水平及DNA结合活性随着合体滋养层细胞分化而下降,并在缺氧和Mash-2过表达时维持在较高水平,而USF1 mRNA水平不受影响。最后,在培养的人滋养层细胞中过表达USF1显著抑制内源性CYP19表达、培养的人滋养层细胞分化及CYP19启动子活性。这些发现表明,USF1和USF2蛋白水平的增加及DNA结合介导了缺氧和Mash-2对人胎盘中CYP19基因表达的抑制作用。

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