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Dual pyrene-labeled pyrrolidinyl peptide nucleic acid as an excimer-to-monomer switching probe for DNA sequence detection

机译:双pyr标记的吡咯烷基肽核酸作为用于DNA序列检测的准分子对单体转换探针

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The unique ability of pyrene to form excimers with distinct emission characteristic from monomer offers an attractive means to signal the interactions between biomolecules. In this work, dual pyrene-labeled pyrrolidinyl peptide nucleic acid probe with a d-prolyl-2- aminocyclopetanecarboxylic acid α,β-dipeptide backbone (acpcPNA) was designed as an excimer-to-monomer switching probe for DNA sequence detection. In single stranded state, the excimer emission at 470 nm was mainly observed in the fluorescence spectrum. In the presence of DNA target, the hybridization resulted in separation of the two pyrene units, therefore the spectrum displayed increased monomer emission at 380 nm with concomitant decreased excimer emission. Switching ratio, which is defined as the ratio of the monomer to excimer in the double stranded form [F_(380)/F_(470)(ds)] divided by the same value obtained from the single stranded form [F _(380)/F_(470)(ss)], was used to describe the performance of the probes. Switching ratios in the range of 5-30 were observed with various dual pyrene-labeled acpcPNA probes bearing pyrenebutyryl label attached five-base apart. Practically no excimer-to-monomer switching behavior was observed with DNA targets carrying a single mismatched base as shown by the small switching ratios of ~1.
机译:of形成具有与单体不同的发射特性的受激准分子的独特能力提供了一种有吸引力的方式来指示生物分子之间的相互作用。在这项工作中,具有d-脯氨酰基-2-氨基环戊烷羧酸α,β-二肽主链(acpcPNA)的双pyr标记的吡咯烷基肽核酸探针被设计为用于DNA序列检测的准分子对单体转换探针。在单链状态下,主要在荧光光谱中观察到470nm的准分子发射。在存在DNA靶标的情况下,杂交导致两个pyr单元分离,因此光谱显示在380 nm处单体发射增加,同时受激准分子发射降低。转换比,定义为双链形式[F_(380)/ F_(470)(ds)]的单体与准分子的比率除以从单链形式[F _(380)获得的相同值/ F_(470)(ss)]用于描述探针的性能。用带有分开的五个碱基的pyr标记的各种双pyr标记的acpcPNA探针观察到了5-30的转换比。实际上,对于带有单个错配碱基的DNA靶,没有观察到准分子对单体的转换行为,如〜1的小转换比所示。

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