优化 lncRNA-miRNA 相互作用分析:改良交联和免疫沉淀(M-CLIP)测定

IF 1.6 Q2 MULTIDISCIPLINARY SCIENCES
MethodsX Pub Date : 2024-10-30 DOI:10.1016/j.mex.2024.103028
Revathy Nadhan , Rohini Gomathinayagam , Rangasudhagar Radhakrishnan , Ji Hee Ha , Muralidharan Jayaraman , Danny N. Dhanasekaran
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引用次数: 0

摘要

定义 lncRNA-miRNA 相互作用对于了解它们在细胞信号传导和癌症生物学中的作用至关重要。由于 RNA 本身的不稳定性,捕捉这些相互作用具有挑战性。我们的研究聚焦于长非编码 RNA(lncRNA)UCA1,通过其与 microRNA(miRNA)的相互作用,探索其在卵巢癌进展中的作用。我们假设 UCA1 作为竞争性内源性 RNA(ceRNA),封存 let-7 miRNA,调节 let-7 靶点的表达,从而推动癌症进展。通常,miRNA 与包括 Ago2 蛋白在内的核糖核蛋白复合物结合,而 Ago2 蛋白在介导 miRNA 的活性和稳定性方面起着关键作用。事实证明,分析这些复合物能有效识别 lncRNA 及其 miRNA 伙伴。受以前的 RNA 蛋白交联方法的启发,我们开发了改良交联和免疫沉淀(M-CLIP)测定法,通过免疫沉淀 Ago2 来捕获 UCA1-let-7 miRNA 的相互作用,然后用 qRT-PCR 检测结合的 UCA1 及其相关的 let-7 miRNA。我们的研究结果表明,M-CLIP 法能有效识别 UCA1-let-7 的相互作用,为阐明 UCA1 和类似的 lncRNA 如何通过 miRNA 的螯合作用影响癌症的进展提供了有力的工具。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Optimizing lncRNA-miRNA interaction analysis: Modified crosslinking and immunoprecipitation (M-CLIP) assay

Optimizing lncRNA-miRNA interaction analysis: Modified crosslinking and immunoprecipitation (M-CLIP) assay
Defining lncRNA-miRNA interactions is critical for understanding their roles in cellular signaling and cancer biology. Capturing these interactions is challenging due to the inherent instability of RNAs. Our study focuses on the long non-coding RNA (lncRNA) UCA1, exploring its role in ovarian cancer progression through interactions with microRNAs (miRNAs). We hypothesized that UCA1 acts as a competing endogenous RNA (ceRNA), sequestering let-7 miRNAs to modulate the expression of let-7 targets, thereby driving cancer progression. Typically, miRNAs associate with ribonucleoprotein complexes that include Ago2 protein, pivotal in mediating miRNA activity and stability. Analyzing these complexes has proven effective in identifying lncRNAs and their miRNA partners. Inspired by previous RNA-protein crosslinking methodologies, we developed the Modified Crosslinking and Immunoprecipitation (M-CLIP) assay to capture UCA1-let-7 miRNA interactions through immunoprecipitation of Ago2, followed by qRT-PCR to detect the bound UCA1 and its associated let-7 miRNAs. This method includes:
  • Formaldehyde-based crosslinking followed by cell lysis
  • Immunoprecipitation and isolation of RNAs bound to bait proteins
  • Characterization of bound lncRNA and target miRNAs
Our findings demonstrate the efficacy of the M-CLIP assay in identifying UCA1-let-7 interactions, providing a robust tool to elucidate how UCA1 and similar lncRNAs influence cancer progression through miRNA sequestration.
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来源期刊
MethodsX
MethodsX Health Professions-Medical Laboratory Technology
CiteScore
3.60
自引率
5.30%
发文量
314
审稿时长
7 weeks
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