The expression of genes involved in myometrial contractility changes during ex situ culture of pregnant human uterine smooth muscle tissue.

Q3 Medicine Journal of Smooth Muscle Research Pub Date : 2017-01-01 DOI:10.1540/jsmr.53.73
Marina Ilicic, Trent Butler, Tamas Zakar, Jonathan W Paul
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引用次数: 14

Abstract

Background: Ex situ analyses of human myometrial tissue has been used to investigate the regulation of uterine quiescence and transition to a contractile phenotype. Following concerns about the validity of cultured primary cells, we examined whether myometrial tissue undergoes culture-induced changes ex situ that may affect the validity of in vitro models.

Objectives: To determine whether human myometrial tissue undergoes culture-induced changes ex situ in Estrogen receptor 1 (ESR1), Prostaglandin-endoperoxide synthase 2 (PTGS2) and Oxytocin receptor (OXTR) expression. Additionally, to determine whether culture conditions approaching the in vivo environment influence the expression of these key genes.

Methods: Term non-laboring human myometrial tissues were cultured in the presence of specific treatments, including; serum supplementation, progesterone and estrogen, cAMP, PMA, stretch or NF-κB inhibitors. ESR1, PTGS2 and OXTR mRNA abundance after 48 h culture was determined using quantitative RT-PCR.

Results: Myometrial tissue in culture exhibited culture-induced up-regulation of ESR1 and PTGS2 and down-regulation of OXTR mRNA expression. Progesterone prevented culture-induced increase in ESR1 expression. Estrogen further up-regulated PTGS2 expression. Stretch had no direct effect, but blocked the effects of progesterone and estrogen on ESR1 and PTGS2 expression. cAMP had no effect whereas PMA further up-regulated PTGS2 expression and prevented decline of OXTR expression.

Conclusion: Human myometrial tissue in culture undergoes culture-induced gene expression changes consistent with transition toward a laboring phenotype. Changes in ESR1, PTGS2 and OXTR expression could not be controlled simultaneously. Until optimal culture conditions are determined, results of in vitro experiments with myometrial tissues should be interpreted with caution.

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妊娠人子宫平滑肌组织离位培养过程中子宫肌收缩性相关基因的表达变化。
背景:人子宫肌组织的非原位分析已被用于研究子宫静止和向收缩表型过渡的调节。考虑到培养原代细胞的有效性,我们检查了子宫肌组织是否经历了可能影响体外模型有效性的培养诱导的非原位变化。目的:探讨培养诱导的人子宫肌组织雌激素受体1 (ESR1)、前列腺素内过氧化物合成酶2 (PTGS2)和催产素受体(OXTR)表达是否发生原位改变。此外,确定接近体内环境的培养条件是否会影响这些关键基因的表达。方法:在特定处理下培养足月非分娩人子宫肌组织,包括;血清补充,孕酮和雌激素,cAMP, PMA,拉伸或NF-κB抑制剂。采用定量RT-PCR检测培养48 h后ESR1、PTGS2和OXTR mRNA的丰度。结果:培养肌组织中ESR1和PTGS2表达上调,OXTR mRNA表达下调。黄体酮阻止培养诱导的ESR1表达增加。雌激素进一步上调PTGS2的表达。拉伸对大鼠无直接影响,但可阻断孕酮和雌激素对ESR1和PTGS2表达的影响。cAMP没有影响,而PMA进一步上调PTGS2表达,阻止了OXTR表达的下降。结论:培养的人子宫肌组织经历了培养诱导的基因表达变化,与向劳动表型的过渡一致。ESR1、PTGS2和OXTR的表达变化不能同时得到控制。在确定最佳培养条件之前,子宫肌组织体外实验的结果应谨慎解释。
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来源期刊
Journal of Smooth Muscle Research
Journal of Smooth Muscle Research Biochemistry, Genetics and Molecular Biology-Physiology
CiteScore
2.30
自引率
0.00%
发文量
7
审稿时长
10 weeks
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