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DETECTION OF NUCLEIC ACIDS USING G-QUARTETS

机译:用G-Quetet检测核酸

摘要

Oligonucleotides which form G-quartet structures have been found to be useful in fluorescence assays to detect a selected nucleic acid sequence. When one end of the5 oligonucleotide is labeled with a donor fluorophore and the other end is labeled with an acceptor dye, the folding of the molecule in the G-quartet structure brings the donor-acceptor pair into close proximity, allowing an interaction between the two labels which results in quenching of donor fluorescence or a change in other fluorescence properties which are the result of the interaction of two dyes in close proximity. The G-quartet structure unfolds upon10 hybridization to its complementary sequence, increasing the distance between the two dye labels. This results in decreased donor quenching or a change in another proximity-related fluorescence parameter. The associated increase in donor fluorescence intensity or the change in another fluorescence parameter may be monitored as an indication of the presence of a selected nucleic acid sequence. Alternatively, in some cases a decrease in acceptor15 fluorescence may be monitored as an indication of the presence of the selected nucleic acid sequence when the acceptor is also a fluorophore. Figure 1
机译:已经发现形成G-四重结构的寡核苷酸可用于 荧光检测以检测选定的核酸序列。当一端5个寡核苷酸用供体荧光团标记,另一端用 受体染料,分子在G四方结构中的折叠带来了供体-受体 配对非常接近,从而允许两个标签之间发生相互作用,从而导致 供体荧光的猝灭或其他荧光特性的变化 两种染料相互作用的结果。 G四重奏结构在10杂交至其互补序列,增加了两种染料之间的距离 标签。这导致供体猝灭减少或另一个邻近相关的改变 荧光参数。相关的供体荧光强度增加或变化 可以监测另一种荧光参数,以指示是否存在 选择的核酸序列。或者,在某些情况下,受体的减少可以监测15个荧光以指示所选核酸的存在 当受体也是荧光团时的序列。 图1

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