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海葵属的 SABER-FISH

SABER-FISH in Hydractinia.

机构信息

University of Galway, Galway, Ireland.

出版信息

Methods Mol Biol. 2024;2784:77-85. doi: 10.1007/978-1-0716-3766-1_5.

Abstract

In situ hybridization allows the detection of nucleic acid sequences in fixed cells and tissues. The gelatinous nature of cnidarians and Hydractinia demands extensive and exhausting protocols to detect RNA transcripts with traditional methods (e.g., colorimetric in situ hybridization). Signal amplification by exchange reaction (SABER) fluorescence in situ hybridization (FISH) enables simplifying and multiplex imaging of RNA targets in a rapid and cost-effective manner. In one enzymatic reaction, SABER-FISH uses a strand-displacing polymerase and catalytic DNA hairpin to generate FISH probes with adjustable signal amplification, allowing highly sensitive detection of nucleic acids and reducing the number of required probes. Here I describe the methodology to detect transcripts within the cells of Hydractinia by SABER-FISH in whole-mount samples.

摘要

原位杂交允许在固定的细胞和组织中检测核酸序列。刺胞动物和水螅的凝胶状性质需要广泛而费力的传统方法(例如,比色原位杂交)来检测 RNA 转录本。通过交换反应进行信号放大的荧光原位杂交(FISH)以快速且经济有效的方式简化和多重成像 RNA 靶标。在一个酶反应中,SABER-FISH 使用链置换聚合酶和催化 DNA 发夹以产生具有可调信号放大的 FISH 探针,从而能够高度灵敏地检测核酸并减少所需探针的数量。在这里,我描述了通过 SABER-FISH 在全培养样本中检测水螅细胞内转录本的方法。

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