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通过花菁染料对荧光寿命变化来检测转录因子结合

Sensing of transcription factor binding via cyanine dye pair fluorescence lifetime changes.

作者信息

Bogdanov Alexei A, Metelev Valeriy, Zhang Surong, Kumar Anand T N

机构信息

The Laboratory of Molecular Imaging Probes S6-434, Department of Radiology, University of Massachusetts Medical School, 55 Lake Ave North, Worcester, MA 01655, USA.

出版信息

Mol Biosyst. 2012 Aug;8(8):2166-73. doi: 10.1039/c2mb25057h. Epub 2012 Jun 19.

Abstract

We designed and synthesized sensors for imaging transcription factor-DNA interactions using a complementary pair of 21-base pair long oligonucleotides (ODNs) carrying two internucleoside phosphate-linked cyanine fluorophores that can either engage in Förster's resonance energy transfer (FRET) with fluorescence emission or assemble into a ground state quenched dimer with short fluorescence lifetimes (FL). Cyanine fluorophores were linked to ODNs within the NF-κB binding site. These sensors were tested in the presence of recombinant p50 and p65 NF-κB proteins or constitutively NF-κB activating HeLa cell lysates. By using a coherent light excitation source we followed changes in fluorescence lifetime of the donor (Cy5.5) at the donor's excitation and emission light wavelengths, as well as the acceptor (800CW or Cy7 cyanine fluorophores) in FRET mode. We observed increases in the donor lifetime in both emitting (0.08-0.15 ns) and non-emitting quenched (0.21 ns) sensors in response to protein binding. The measurements of lifetimes in FRET mode in quenched pair-carrying ODN duplex sensors showed significant differences in FL of the acceptor cyanine fluorophore between NF-κB-containing and NF-κB-free samples but not in control sensors with ODN sequences that have decreased binding affinity to NF-κB. We anticipate that the observed effects will be instrumental for developing sensors enabling non-invasive imaging in cells that undergo activation of NF-κB.

摘要

我们设计并合成了用于成像转录因子 - DNA相互作用的传感器,该传感器使用一对互补的21个碱基对长的寡核苷酸(ODN),其携带两个通过核苷间磷酸连接的花菁荧光团,这些荧光团既可以通过荧光发射参与Förster共振能量转移(FRET),也可以组装成具有短荧光寿命(FL)的基态猝灭二聚体。花菁荧光团连接在NF-κB结合位点内的ODN上。这些传感器在重组p50和p65 NF-κB蛋白或组成型NF-κB激活的HeLa细胞裂解物存在的情况下进行了测试。通过使用相干光激发源,我们跟踪了供体(Cy5.5)在其激发和发射光波长处的荧光寿命变化,以及FRET模式下受体(800CW或Cy7花菁荧光团)的荧光寿命变化。我们观察到,响应于蛋白质结合,发射型(0.08 - 0.15 ns)和非发射型猝灭型(0.21 ns)传感器中的供体寿命均增加。在携带猝灭对的ODN双链体传感器中进行的FRET模式下的寿命测量显示含NF-κB和不含NF-κB的样品之间受体花菁荧光团的FL存在显著差异,但与对NF-κB结合亲和力降低的ODN序列的对照传感器中没有差异。我们预计,观察到的这些效应将有助于开发能够在经历NF-κB激活的细胞中进行非侵入性成像的传感器。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ac91/3544408/de052ff7e420/nihms388296f1.jpg

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