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An enzymatically-sensitized sequential and concentric energy transfer relay self-assembled around semiconductor quantum dots

机译:一个enzymatically-sensitized顺序和同心能量传递接力自组装在半导体量子点

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The ability to control light energy within de novo nanoscale structures and devices will greatly benefit their continuing development and ultimate application. Ideally, this control should extend from generating the light itself to its spatial propagation within the device along with providing defined emission wavelength (s), all in a stand-alone modality. Here we design and characterize macromolecular nanoassemblies consisting of semiconductor quantum dots (QDs), several differentially dye-labeled peptides and the enzyme luciferase which cumulatively demonstrate many of these capabilities by engaging in multiple-sequential energy transfer steps. To create these structures, recombinantly-expressed luciferase and the dye-labeled peptides were appended with a terminal polyhistidine sequence allowing for controlled ratio-metric self-assembly around the QDs via metal-affinity coordination. The QDs serve to provide multiple roles in these structures including as central assembly platforms or nanoscaffolds along with acting as a potent energy harvesting and transfer relay. The devices are activated by addition of coelenterazine H substrate which is oxidized by luciferase producing light energy which sensitizes the central 625 nm emitting QD acceptor by bioluminescence resonance energy transfer (BRET). The sensitized QD, in turn, acts as a relay and transfers the energy to a first peptide-labeled Alexa Fluor 647 acceptor dye displayed on its surface. This dye then transfers energy to a second red-shifted peptide-labeled dye acceptor on the QD surface through a second concentric Forster resonance energy transfer (FRET) process. Alexa Fluor 700 and Cy5.5 are both tested in the role of this terminal FRET acceptor. Photophysical analysis of spectral profiles from the resulting sequential BRET-FRET-FRET processes allow us to estimate the efficiency of each of the transfer steps. Importantly, the efficiency of each step within this energy transfer cascade can be controlled to some extent by the number of enzymes/peptides displayed on the QD. Further optimization of the energy transfer process(es) along with potential applications of such devices are finally discussed.
机译:在全程控制光能量的能力纳米结构和设备将极大地他们的持续发展和最终受益应用程序。从生成光本身的空间在和传播提供定义的发射波长(s),所有一个独立的方法。描述高分子nanoassemblies组成的半导体量子点(量子点),几个不同dye-labeled肽累计的酶荧光素酶展示许多这样的能力参与多个连续能量转移步骤。recombinantly-expressed荧光素酶和dye-labeled肽是附加的终端允许polyhistidine序列ratio-metric自组装的控制量子点通过metal-affinity协调。在这些服务提供多个角色结构包括中央组装平台或nanoscaffolds充当强大的能量收集和传输中继。通过添加设备被激活coelenterazine H氧化的底物荧光素酶生产光能量中央625海里排放QD处于敏感状态受体的生物荧光共振能量转移(BRET)。作为一个继电器和传输能量peptide-labeled Alexa萤石647受体染料显示在其表面。能量peptide-labeled第二个有红移的通过第二个染料QD表面受体同心福斯特共振能量转移(烦恼)的过程。这个终端担心这两个测试的作用受体。概要文件从生成的顺序让我们估计BRET-FRET-FRET流程每个转换步骤的效率。重要的是,在每一步的效率这种能量转移级联可以控制某种程度上酶的数量/肽显示在QD。能量传递过程(es)和潜力这类设备最终的应用程序进行了讨论。

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