Mir-21 Regulation of MARCKS Protein and Mucin Secretion in Airway Epithelial Cells

W. R. Lampe, S. Fang, Q. Yin, A. Crews, Joungjoa Park, K. Adler
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引用次数: 2

Abstract

Hypersecretion of mucus characterizes many inflammatory airway diseases, including asthma, chronic bronchitis, and cystic fibrosis. Excess mucus causes airway obstruction, reduces pulmonary function, and can lead to increased morbidity and mortality. MicroRNAs are small non-coding pieces of RNA which regulate other genes by binding to a complementary sequence in the target mRNA. The microRNA miR-21 is upregulated in many inflammatory conditions and, interestingly, miR-21 has been shown to target the mRNA of Myristoylated Alanine-Rich C Kinase Substrate (MARCKS), a protein that is an important regulator of airway mucin (the solid component of mucus) secretion. In these studies, we determined that exposure of primary, well-differentiated, normal human bronchial epithelial (NHBE) cells to the pro-inflammatory stimulus lipopolysaccharide (LPS) increased expression of both miR-21 and MARCKS in a time-dependent manner. To investigate whether miR-21 regulation of MARCKS played a role in mucin secretion, two separate airway epithelial cell lines, HBE1 (papilloma virus transformed) and NCI-H292 (mucodepidermoid derived) were utilized, since manipulation of miR-21 is performed via transfection of commercially-available miR-21 inhibitors and mimics/activators. Treatment of HBE1 cells with LPS caused concentration-dependent increases in expression of both miR-21 and MARCKS mRNA and protein. The miR-21 inhibitor effectively reduced levels of miR-21 in the cells, coincident with an increase in MARCKS mRNA expression over time as well as enhanced mucin secretion, while the miR-21 mimic/activator increased levels of miR-21, which coincided with a decrease in expression of MARCKS and a decrease in mucin secretion. These results suggest that miR-21 is increased in airway epithelial cells following exposure to LPS, and that miR-21 downregulates expression of MARCKS, which may decrease mucin secretion by the cells. Thus, miR-21 may act as a negative feedback regulator of mucin secretion in airway epithelial cells, and may do so, at least in part, by downregulating expression of MARCKS.
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Mir-21对气道上皮细胞MARCKS蛋白和粘蛋白分泌的调控
粘液分泌过多是许多炎性气道疾病的特征,包括哮喘、慢性支气管炎和囊性纤维化。过多的粘液导致气道阻塞,降低肺功能,并可导致发病率和死亡率增加。MicroRNAs是一种小的非编码RNA片段,通过与靶mRNA中的互补序列结合来调节其他基因。microRNA miR-21在许多炎症条件下上调,有趣的是,miR-21已被证明靶向肉豆蔻酰基化富丙氨酸C激酶底物(MARCKS)的mRNA, MARCKS是气道粘蛋白(粘液的固体成分)分泌的重要调节剂。在这些研究中,我们确定原代、分化良好的正常人支气管上皮(NHBE)细胞暴露于促炎刺激脂多糖(LPS)中,miR-21和MARCKS的表达以时间依赖性的方式增加。为了研究miR-21对MARCKS的调控是否在粘蛋白分泌中发挥作用,我们利用了两种独立的气道上皮细胞系,HBE1(乳头瘤病毒转化)和NCI-H292(粘膜上皮样细胞衍生),因为miR-21的操纵是通过转染市上可用的miR-21抑制剂和模拟物/激活剂进行的。用LPS处理HBE1细胞导致miR-21和MARCKS mRNA和蛋白的表达呈浓度依赖性增加。miR-21抑制剂有效地降低了细胞中miR-21的水平,与随着时间的推移MARCKS mRNA表达的增加以及粘蛋白分泌的增加相一致,而miR-21模拟物/激活物增加了miR-21的水平,这与MARCKS表达的减少和粘蛋白分泌的减少相一致。这些结果表明,暴露于LPS后,miR-21在气道上皮细胞中升高,miR-21下调MARCKS的表达,这可能会减少细胞的粘蛋白分泌。因此,miR-21可能在气道上皮细胞中作为粘蛋白分泌的负反馈调节器,并且可能至少部分地通过下调MARCKS的表达来实现。
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