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Fluorescence resonance energy transfer(FRET)for DNA biosensors:FRET pairs and Forster distances for various dye-DNA conjugates

机译:DNA生物传感器的荧光共振能量转移(FRET):各种染料-DNA共轭物的FRET对和Forster距离

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Fluorescence resonance energy transfer(FRET)between the extrinsic dye labels Cyanine 3(Cy3),Cyanine 5(Cy5),Carboxytetramethyl Rhodamine(TAMRA),Iowa Black Fluorescence Quencher(IabFQ),and Iowa Black RQ(IabRQ)has been studied.The Forster distances for these FRET-pairs in single-and double-stranded DNA conjugates have been determined.In particular,it should be noted that the quantum yield of the donors Cy3 and TAMRA varies between single-and double-stranded DNA.While this alters the Forster distance for a donor-acceptor pair,this also allows for detection of thermal denaturation events with a single non-intercalating fluorophore.The utility of FRET in the development of nucleic acid biosensor technology is illustrated by using TAMRA and IabRQ as a FRET pair in selectivity experiments.The differential quenching of TAMRA fluorescence by IabRQ in solution has been used to discriminate between 0 and 3 base pair mismatches at 60 deg C for a 19 base sequence.At room temperature,the quenching of TAMRA fluorescence was not an effective indicator of the degree of base pair mismatch.There appears to be a threshold of duplex stability at room temperature which occurs beyond two base pair mismatches and reverses the observed trend in TAMRA fluorescence prior to that degree of mismatch.When this experimental system is transferred to a glass surface through covalent coupling and organosilane chemistry,the observed trend in TAMRA fluorescence at room temperature is similar to that obtained in bulk solution,but without a threshold of duplex stability.In addition to quenching of fluorescence by FRET,it is believed that several other quenching mechanisms are occurring at the surface.
机译:研究了外在染料标记Cyanine 3(Cy3),Cyanine 5(Cy5),Carboxytetramethyl Rhodamine(TAMRA),Iowa Black荧光猝灭剂(IabFQ)和Iowa Black RQ(IabRQ)之间的荧光共振能量转移(FRET)。已经确定了单链和双链DNA缀合物中这些FRET对的Forster距离。尤其应注意,供体Cy3和TAMRA的量子产率在单链和双链DNA之间有所不同。供体-受体对的Forster距离,这也允许使用单个非插入式荧光团检测热变性事件。通过使用TAMRA和IabRQ作为FRET对来说明FRET在核酸生物传感器技术开发中的实用性IabRQ在溶液中对TAMRA荧光的差异猝灭已用于区分19碱基序列在60℃下0到3个碱基对错配。在室温下, TAMRA荧光不是碱基对错配程度的有效指标,室温下似乎存在双链体稳定性阈值,该阈值超出两个碱基对错配发生,并在该错配度之前逆转了观察到的TAMRA荧光趋势。通过共价偶联和有机硅烷化学将该实验体系转移到玻璃表面,室温下TAMRA荧光的观察趋势与本体溶液中观察到的趋势相似,但没有双链稳定性阈值。此外,通过FRET猝灭荧光据信,在表面上还发生了其他几种淬火机理。

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