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DNA Mimics for the Rapid Identification of Microorganisms by Fluorescence in situ Hybridization (FISH)

机译:DNA模仿物通过荧光原位杂交(FISH)快速鉴定微生物

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摘要

Fluorescence in situ hybridization (FISH) is a well-established technique that is used for a variety of purposes, ranging from pathogen detection in clinical diagnostics to the determination of chromosomal stability in stem cell research. The key step of FISH involves the detection of a nucleic acid region and as such, DNA molecules have typically been used to probe for the sequences of interest. However, since the turn of the century, an increasing number of laboratories have started to move on to the more robust DNA mimics methods, most notably peptide and locked nucleic acids (PNA and LNA). In this review, we will cover the state-of-the-art of the different DNA mimics in regard to their application as efficient markers for the presence of individual microbial cells, and consider their potential advantages and pitfalls. Available PNA probes are then reassessed in terms of sensitivity and specificity using rRNA databases. In addition, we also attempt to predict the applicability of DNA mimics in well-known techniques attempting to detect in situ low number of copies of specific nucleic acid sequences such as catalyzed reporter deposition (CARD) and recognition of individual genes (RING) FISH.
机译:荧光原位杂交(FISH)是一项成熟的技术,可用于多种目的,从临床诊断中的病原体检测到干细胞研究中确定染色体稳定性。 FISH的关键步骤涉及核酸区域的检测,因此,DNA分子通常已用于探测目标序列。然而,自本世纪初以来,越来越多的实验室开始转向更强大的DNA模拟方法,最著名的是肽和锁核酸(PNA和LNA)。在这篇综述中,我们将介绍各种不同的DNA模拟物的最新技术,这些模拟物是作为单个微生物细胞存在的有效标记物而应用的,并考虑了它们的潜在优势和陷阱。然后使用rRNA数据库对可用的PNA探针的敏感性和特异性进行重新评估。另外,我们还尝试预测DNA模仿物在众所周知的技术中的适用性,这些技术试图原位检测特定核酸序列的低拷贝数,例如催化的报道分子沉积(CARD)和单个基因的识别(RING)FISH。

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