Sensitive detection of nucleic acids by PNA hybridization directed co-localization of fluorescent beads.

Takehiko Shiraishi, Stijn Deborggraeve, Philippe Büscher, Peter E Nielsen
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引用次数: 16

Abstract

We have designed a pair of biotinylated peptide nucleic acid (PNA) probes targeting two sequences in 18S rRNA (from the parasite Trypanosoma brucei) at a distance of 191 nt (corresponding to maximum distance of ca. 60 nm) from each other. The PNA probes were individually bound to (strept)avidin-coated fluorescent beads, differing in size and color [green beads (1 µm) and red beads (5.9 µm)], thereby allowing distinct detection of each PNA probe by conventional fluorescence microscopy. These two PNA beads showed easily detectable co-localization when simultaneously hybridizing to a target nucleic acid. The assay detected the parasite 18S rRNA down to 1.6 fmol while there was no such co-localization visible with human 18S rRNA not containing the PNA targets. Furthermore, the assay showed positive detection with 1.6 ng of total RNA (corresponding to RNA from ca. 300 parasites). Upon further optimization this method may provide a new tool for a diagnosis of Human African Trypanosomiasis (HAT) and it may more generally have applications within diagnostics for (neglected) infectious diseases.

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利用PNA杂交定向荧光珠共定位的核酸敏感检测方法。
我们设计了一对生物素化肽核酸(PNA)探针,针对来自布鲁氏锥虫(Trypanosoma bruei)的18S rRNA中的两个序列,它们彼此之间的距离为191 nt(最大距离约为60 nm)。PNA探针分别与(strept)亲和素涂覆的荧光珠结合,其大小和颜色不同[绿珠(1µm)和红珠(5.9µm)],从而可以通过常规荧光显微镜对每个PNA探针进行不同的检测。当同时与靶核酸杂交时,这两个PNA珠显示出易于检测的共定位。该实验检测到寄生虫的18S rRNA低至1.6 fmol,而与不含PNA靶点的人类18S rRNA未见共定位。此外,总RNA检测结果为1.6 ng(相当于约300种寄生虫的RNA)。经进一步优化,该方法可为非洲人类锥虫病(HAT)的诊断提供一种新工具,并可能在(被忽视的)传染病的诊断中得到更广泛的应用。
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