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Small RNA Detection by in Situ Hybridization Methods

机译:原位杂交方法检测小RNA

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Small noncoding RNAs perform multiple regulatory functions in cells, and their exogenous mimics are widely used in research and experimental therapies to interfere with target gene expression. MicroRNAs (miRNAs) are the most thoroughly investigated representatives of the small RNA family, which includes short interfering RNAs (siRNAs), PIWI-associated RNA (piRNAs), and others. Numerous methods have been adopted for the detection and characterization of small RNAs, which is challenging due to their short length and low level of expression. These include molecular biology methods such as real-time RT-PCR, northern blotting, hybridization to microarrays, cloning and sequencing, as well as single cell miRNA detection by microscopy with in situ hybridization (ISH). In this review, we focus on the ISH method, including its fluorescent version (FISH), and we present recent methodological advances that facilitated its successful adaptation for small RNA detection. We discuss relevant technical aspects as well as the advantages and limitations of ISH. We also refer to numerous applications of small RNA ISH in basic research and molecular diagnostics.
机译:小型非编码RNA在细胞中执行多种调节功能,其外源模拟物已广泛用于研究和实验疗法中,以干扰靶基因的表达。 MicroRNA(miRNA)是小RNA家族研究最彻底的代表,其中包括短干扰RNA(siRNA),PIWI相关RNA(piRNA)等。已经采用了许多方法来检测和表征小RNA,由于其长度短且表达水平低,因此具有挑战性。这些方法包括分子生物学方法,例如实时RT-PCR,RNA印迹,与微阵列的杂交,克隆和测序,以及通过显微镜与原位杂交(ISH)进行单细胞miRNA检测。在这篇综述中,我们着重于ISH方法,包括其荧光版本(FISH),并且我们介绍了最近的方法学进展,这些进展促进了其成功地适应小RNA检测。我们讨论了ISH的相关技术方面以及优点和局限性。我们还提到了小RNA ISH在基础研究和分子诊断中的许多应用。

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