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用细胞穿透肽功能化的铑嵌入剂靶向DNA错配。

Targeting DNA mismatches with rhodium intercalators functionalized with a cell-penetrating peptide.

作者信息

Brunner Jens, Barton Jacqueline K

机构信息

Division of Chemistry and Chemical Engineering, California Institute of Technology, Pasadena, California 91125, USA.

出版信息

Biochemistry. 2006 Oct 10;45(40):12295-302. doi: 10.1021/bi061198o.

DOI:10.1021/bi061198o
PMID:17014082
Abstract

Cell-penetrating peptides are widely used to deliver cargo molecules into cells. Here we describe the synthesis, characterization, DNA binding, and cellular uptake studies of a series of metal-peptide conjugates containing oligoarginine as a cell-penetrating peptide. d-Octaarginine units are appended onto a rhodium intercalator containing the sterically expansive chrysenequinone diimine (chrysi) ligand to form Rh(chrysi)(phen)(bpy)(3+)-tethered oligoarginine conjugates, where the peptide is attached to the ancillary bpy ligand; some conjugates also include a fluorescein or thiazole orange tag. These complexes bind and with photoactivation selectively cleave DNA neighboring single-base mismatches. The presence of the oligoarginines is found to increase the nonspecific binding affinity of the complexes for both matched and mismatched DNA, but for these conjugates, photocleavage remains selective for the mismatched site, as assayed using both gel electrophoresis and mass spectrometry experiments. Significantly, the rhodium complex does not interfere with the delivery properties of the cell-penetrating peptide. Confocal microscopy experiments show rapid nuclear localization of the metal-peptide conjugates containing the tethered fluorescein. Mass spectrometry experiments confirm the association of the rhodium with the HeLa cells. These results provide a strategy for targeting mismatch-selective metal complexes inside cell nuclei.

摘要

细胞穿透肽被广泛用于将货物分子递送至细胞内。在此,我们描述了一系列以寡聚精氨酸作为细胞穿透肽的金属-肽缀合物的合成、表征、DNA结合及细胞摄取研究。将d-八聚精氨酸单元连接到含有空间位阻较大的苝醌二亚胺(chrysi)配体的铑嵌入剂上,形成Rh(chrysi)(phen)(bpy)(3+)-连接的寡聚精氨酸缀合物,其中肽连接到辅助bpy配体上;一些缀合物还包含荧光素或噻唑橙标签。这些配合物能结合并通过光活化选择性切割邻近单碱基错配的DNA。发现寡聚精氨酸的存在会增加配合物对匹配和错配DNA的非特异性结合亲和力,但对于这些缀合物,通过凝胶电泳和质谱实验测定,光切割对错配位点仍具有选择性。值得注意的是,铑配合物不会干扰细胞穿透肽的递送特性。共聚焦显微镜实验显示含有连接荧光素的金属-肽缀合物能快速定位于细胞核。质谱实验证实铑与HeLa细胞有关联。这些结果为在细胞核内靶向错配选择性金属配合物提供了一种策略。

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