Unique interstitial miRNA signature drives fibrosis in a murine model of autosomal dominant polycystic kidney disease.

Ameya Patil, William E Sweeney, Cynthia G Pan, Ellis D Avner
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引用次数: 4

Abstract

Aim: To delineate changes in miRNA expression localized to the peri-cystic local microenvironment (PLM) in an orthologous mouse model of autosomal dominant polycystic kidney disease (ADPKD) (mcwPkd1(nl/nl) ).

Methods: We profiled miRNA expression in the whole kidney and laser captured microdissection (LCM) samples from PLM in mcwPkd1(nl/nl) kidneys with Qiagen miScript 384 HC miRNA PCR arrays. The three times points used are: (1) post-natal (PN) day 21, before the development of trichrome-positive areas; (2) PN28, the earliest sign of trichrome staining; and (3) PN42 following the development of progressive fibrosis. PN21 served as appropriate controls and as the reference time point for comparison of miRNA expression profiles.

Results: LCM samples revealed three temporally upregulated miRNAs [2 to 2.75-fold at PN28 and 2.5 to 4-fold (P ≤ 0.05) at PN42] and four temporally downregulated miRNAs [2 to 2.75 fold at PN28 and 2.75 to 5-fold (P ≤ 0.05) at PN42]. Expression of twenty-six miRNAs showed no change until PN42 [six decreased (2.25 to 3.5-fold) (P ≤ 0.05) and 20 increased (2 to 4-fold) (P ≤ 0.05)]. Many critical miRNA changes seen in the LCM samples from PLM were not seen in the contralateral whole kidney.

Conclusion: Precise sampling with LCM identifies miRNA changes that occur with the initiation and progression of renal interstitial fibrosis (RIF). Identification of the target proteins regulated by these miRNAs will provide new insight into the process of fibrosis and identify unique therapeutic targets to prevent or slow the development and progression of RIF in ADPKD.

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在常染色体显性多囊肾病小鼠模型中,独特的间质miRNA特征驱动纤维化。
目的:研究常染色体显性多囊肾病(ADPKD)小鼠模型(mcwPkd1(nl/nl))中定位于囊周局部微环境(PLM)的miRNA表达的变化。方法:采用Qiagen miScript 384 HC miRNA PCR阵列对mcwPkd1(nl/nl)肾脏PLM的全肾和激光捕获显微解剖(LCM)样品进行miRNA表达谱分析。使用的三个时间点是:(1)产后(PN)第21天,三色阳性区域发育之前;(2) PN28,三色染色最早的标志;(3)进展性纤维化后PN42的变化。PN21作为适当的对照,并作为比较miRNA表达谱的参考时间点。结果:LCM样品显示3个暂时上调的mirna [PN28为2 ~ 2.75倍,PN42为2.5 ~ 4倍(P≤0.05)]和4个暂时下调的mirna [PN28为2 ~ 2.75倍,PN42为2.75 ~ 5倍(P≤0.05)]。26个mirna的表达没有变化,直到PN42[6个减少(2.25 ~ 3.5倍)(P≤0.05),20个增加(2 ~ 4倍)(P≤0.05)]。在PLM的LCM样本中观察到的许多关键miRNA变化在对侧全肾中未见。结论:LCM精确取样可识别miRNA在肾间质纤维化(RIF)发生和发展过程中的变化。鉴定由这些mirna调控的靶蛋白将为纤维化过程提供新的见解,并确定独特的治疗靶点,以防止或减缓ADPKD中RIF的发生和进展。
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