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一种用于杂交后基于图像的基因表达平行定量和基因分型的优化流程。

An optimised pipeline for parallel image-based quantification of gene expression and genotyping after hybridisation.

作者信息

Dobrzycki Tomasz, Krecsmarik Monika, Bonkhofer Florian, Patient Roger, Monteiro Rui

机构信息

MRC Molecular Haematology Unit, MRC Weatherall Institute of Molecular Medicine, John Radcliffe Hospital, University of Oxford, Oxford OX3 9DS, UK.

BHF Centre of Research Excellence, Weatherall Institute of Molecular Medicine, John Radcliffe Hospital, University of Oxford, Oxford OX3 9DS, UK.

出版信息

Biol Open. 2018 Apr 9;7(4):bio031096. doi: 10.1242/bio.031096.

Abstract

Advances in genome engineering have resulted in the generation of numerous zebrafish mutant lines. A commonly used method to assess gene expression in the mutants is hybridisation (ISH). Because the embryos can be distinguished by genotype after ISH, comparing gene expression between wild-type and mutant siblings can be done blinded and in parallel. Such experimental design reduces the technical variation between samples and minimises the risk of bias. This approach, however, requires an efficient method of genomic DNA extraction from post-ISH fixed zebrafish samples to ascribe phenotype to genotype. Here we describe a method to obtain PCR-quality DNA from 95-100% of zebrafish embryos, suitable for genotyping after ISH. In addition, we provide an image analysis protocol for quantifying gene expression of ISH-probed embryos, adaptable for the analysis of different expression patterns. Finally, we show that intensity-based image analysis enables accurate representation of the variability of gene expression detected by ISH and that it can complement quantitative methods like qRT-PCR. By combining genotyping after ISH and computer-based image analysis, we have established a high-confidence, unbiased methodology to assign gene expression levels to specific genotypes, and applied it to the analysis of molecular phenotypes of newly generated mutants.

摘要

基因组工程的进展已导致产生了众多斑马鱼突变品系。评估突变体中基因表达的一种常用方法是原位杂交(ISH)。由于在ISH后胚胎可以通过基因型进行区分,因此可以在不知情的情况下并行比较野生型和突变体同胞之间的基因表达。这种实验设计减少了样本之间的技术差异,并将偏差风险降至最低。然而,这种方法需要一种从ISH后固定的斑马鱼样本中高效提取基因组DNA的方法,以便将表型归因于基因型。在这里,我们描述了一种从95%-100%的斑马鱼胚胎中获得适合PCR的DNA的方法,适用于ISH后的基因分型。此外,我们提供了一种图像分析方案,用于量化ISH检测的胚胎的基因表达,适用于分析不同的表达模式。最后,我们表明基于强度的图像分析能够准确呈现ISH检测到的基因表达变异性,并且它可以补充qRT-PCR等定量方法。通过结合ISH后的基因分型和基于计算机的图像分析,我们建立了一种高可信度、无偏差的方法,将基因表达水平分配给特定基因型,并将其应用于新产生突变体的分子表型分析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1fed/5936060/cf0a96f622de/biolopen-7-031096-g1.jpg

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