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A nanobody-based system using fluorescent proteins as scaffolds for cell-specific gene manipulation

机译:基于纳米抗体的系统,使用荧光蛋白作为细胞特异性基因操纵的支架

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摘要

Fluorescent proteins are commonly used to label cells across organisms, but the unmodified forms cannot control biological activities. Using GFP-binding proteins derived from Camelid antibodies, we co-opted GFP as a scaffold for inducing formation of biologically active complexes, developing a library of hybrid transcription factors that control gene expression only in the presence of GFP or its derivatives. The modular design allows for variation in key properties such as DNA specificity, transcriptional potency, and drug dependency. Production of GFP controlled cell-specific gene expression and facilitated functional perturbations in the mouse retina and brain. Further, retrofitting existing transgenic GFP mouse and zebrafish lines for GFP-dependent transcription enabled applications such as optogenetic probing of neural circuits. This work establishes GFP as a multifunctional scaffold and opens the door to selective manipulation of diverse GFP-labeled cells across transgenic lines. This approach may also be extended to exploit other intracellular products as cell-specific scaffolds in multicellular organisms.
机译:荧光蛋白通常用于跨生物标记细胞,但未修饰的形式无法控制生物活性。使用来源于骆驼科动物抗体的GFP结合蛋白,我们选择GFP作为诱导生物活性复合物形成的支架,开发了仅在GFP或其衍生物存在时控制基因表达的杂交转录因子文库。模块化设计允许改变关键特性,例如DNA特异性,转录潜能和药物依赖性。 GFP的产生控制着细胞特异性基因的表达,并促进了小鼠视网膜和大脑的功能扰动。此外,对现有的转基因GFP小鼠和斑马鱼品系进行改造,以实现GFP依赖性转录,从而实现了诸如神经回路的光遗传学探测等应用。这项工作将GFP建立为多功能支架,并为跨转基因品系的各种GFP标记细胞的选择性操作打开了大门。该方法也可以扩展为利用其他细胞内产物作为多细胞生物中的细胞特异性支架。

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