Jain Chandni V, Jessmon Philip, Kilburn Brian A, Jodar Meritxell, Sendler Edward, Krawetz Stephen A, Armant D Randall
Department of Physiology, Wayne State University School of Medicine, Detroit, Michigan, United States of America.
Department of Obstetrics and Gynecology, Wayne State University School of Medicine, Detroit, Michigan, United States of America.
PLoS One. 2016 Oct 4;11(10):e0163913. doi: 10.1371/journal.pone.0163913. eCollection 2016.
The growth factor HBEGF is upregulated post-transcriptionally in the low O2 environment of the human placenta during the first 10 weeks of pregnancy. We have examined the possible roles of HBEGF turnover and micro-RNA (miRNA) in its regulation by O2 in human first trimester trophoblast.
HTR-8/SVneo trophoblast cells were cultured at 2% or 20% O2. The cells were transfected with a dual luciferase reporter construct (psiCHECK-2) containing no insert (control), the HBEGF 3' untranslated region (3'UTR), or sub-regions of the 3'UTR, as well as with siRNA for DGCR8. RNA was extracted from trophoblast cells cultured at 2% O2 for 0-4 h for next-generation sequencing. HBEGF was quantified by ELISA. HBEGF, DGCR8, and β-actin were examined by western blotting.
Protein turnover studies, using 10 μg/ml cyclohexamide, 1 μg/ml lactocystin, or 100 μg/ml MG132, demonstrated faster HBEGF degradation at 20% O2 than 2% O2, mediated by the proteasome. However, proteasome inhibition failed to initiate HBEGF accumulation at 20% O2. Reporter assays, comparing to empty vector, demonstrated that the intact HBEGF 3' UTR inhibited expression (0.26), while fragments containing only its flanking regions increased reporter activity (3.15; 3.43). No differential expression of miRNAs was found in trophoblast cells cultured at 2% and 20% O2. Nevertheless, HBEGF upregulation at 2% O2 was blocked when the miRNA-processing protein DGCR8 was silenced, suggesting a role for miRNA.
Our findings suggest involvement of flanking regions of the 3'UTR in activating HBEGF protein synthesis in response to 2% O2, possibly through a miRNA-mediated mechanism.
在怀孕的前10周,人胎盘低氧环境中生长因子肝素结合表皮生长因子(HBEGF)在转录后水平上调。我们研究了HBEGF周转和微小RNA(miRNA)在人早孕期滋养层细胞中受氧调节过程中的可能作用。
将HTR-8/SVneo滋养层细胞分别在2%或20%氧气浓度下培养。用不含插入片段(对照)、HBEGF 3'非翻译区(3'UTR)或3'UTR亚区域的双荧光素酶报告构建体(psiCHECK-2)以及针对DGCR8的小干扰RNA(siRNA)转染细胞。从在2%氧气浓度下培养0至4小时的滋养层细胞中提取RNA用于下一代测序。通过酶联免疫吸附测定(ELISA)对HBEGF进行定量。通过蛋白质免疫印迹法检测HBEGF、DGCR8和β-肌动蛋白。
使用10μg/ml放线菌酮、1μg/ml乳胞素或100μg/ml MG132进行的蛋白质周转研究表明,在20%氧气浓度下,蛋白酶体介导的HBEGF降解比在2%氧气浓度下更快。然而,蛋白酶体抑制未能在20%氧气浓度下引发HBEGF积累。与空载体相比,报告基因检测表明完整的HBEGF 3'UTR抑制表达(0.26),而仅包含其侧翼区域的片段增加报告基因活性(3.15;3.43)。在2%和20%氧气浓度下培养的滋养层细胞中未发现miRNA的差异表达。然而,当miRNA加工蛋白DGCR8沉默时,2%氧气浓度下HBEGF的上调被阻断,提示miRNA起作用。
我们的研究结果表明,3'UTR的侧翼区域可能通过miRNA介导的机制参与响应2%氧气浓度激活HBEGF蛋白合成。
