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Method for multiplex cellular detection of mRNAs using quantum dot fluorescent in situ hybridization

机译:利用量子点荧光原位杂交技术对mRNA进行多重细胞检测的方法

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摘要

The photostability and narrow emission spectra of non-organic quantum dot fluorophores (QDs) make them desirable candidates for fluorescent in situ hybridization (FISH) to study the expression of specific mRNA transcripts. We developed a novel method for direct QD labeling of modified oligonucleotide probes through streptavidin and biotin interactions, as well as protocols for their use in multiple-label FISH. We validated this technique in mouse brainstem sections. The subcellular localization of the vesicular monoamine transporter (Vmat2) mRNA corresponds when using probes labeled with two different QDs in the same hybridization. We developed protocols for combined direct QD FISH and QD immunohistochemical labeling within the same neurons as well as for simultaneous study of the subcellular distribution of multiple mRNA targets. We demonstrated increased sensitivity of FISH using QDs in comparison with organic fluorophores. These techniques gave excellent histological results both for multiplex FISH and combined FISH and immunohistochemistry. This approach can facilitate the ultrasensitive simultaneous study of multiple mRNA and protein markers in tissue culture and histological section.
机译:非有机量子点荧光团(QD)的光稳定性和窄发射光谱使其成为荧光原位杂交(FISH)研究特定mRNA转录本表达的理想候选物。我们开发了一种通过链霉亲和素和生物素相互作用直接对修饰的寡核苷酸探针进行QD标记的新方法,以及将其用于多标签FISH的协议。我们在小鼠脑干部分中验证了此技术。当在同一杂交中使用带有两个不同QD标记的探针时,相应的水泡单胺转运蛋白(Vmat2)mRNA的亚细胞定位。我们开发了用于在同一神经元内进行直接QD FISH和QD免疫组化组合标记以及同时研究多个mRNA靶标的亚细胞分布的方案。我们证明了与有机荧光团相比,使用QD可以提高FISH的灵敏度。这些技术为多重FISH以及FISH与免疫组织化学的结合提供了出色的组织学结果。这种方法可以促进组织培养和组织学切片中多种mRNA和蛋白质标记物的超灵敏同时研究。

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