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Genetically Encoded Photocontrol of Protein Localization in Mammalian Cells

机译:基因编码的哺乳动物细胞中蛋白质定位的光控制。

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Precise photochemical control of protein function can be achieved through the site-specific introduction of caging groups. Chemical and enzymatic methods, including in vitro translation and chemical ligation, have been used to photocage proteins in vitro. These methods have been extended to allow the introduction of caged proteins into cells by permeabilization or microinjection, but cellular delivery remains challenging. Since lysine residues are key determinants for nuclear localization sequences, the target of key post-translational modifications (including ubiquitination, methylation, and acetylation), and key residues in many important enzyme active sites, we were interested in photocaging lysine to control protein localization, post-translational modification, and enzymatic activity. Photochemical control of these important functions mediated by lysine residues in proteins has not previously been demonstrated in living cells. Here we synthesized 1 and evolved a pyrrolysyl-tRNA synthetase/tRNA pair to genetically encode the incorporation of this amino acid in response to an amber codon in mammalian cells. To exemplify the utility of this amino acid, we caged the nuclear localization sequences (NLSs) of nucleoplasmin and the tumor suppressor p53 in human cells, thus mislocalizing the proteins in the cytosol. We triggered protein nuclear import with a pulse of light, allowing us to directly quantify the kinetics of nuclear import.
机译:蛋白质功能的精确光化学控制可通过特定位置引入笼基来实现。化学和酶促方法,包括体外翻译和化学连接,已用于体外光笼蛋白。这些方法已经扩展到允许通过透化或显微注射将笼中的蛋白质引入细胞中,但是细胞递送仍然具有挑战性。由于赖氨酸残基是核定位序列的关键决定因素,关键的翻译后修饰(包括泛素化,甲基化和乙酰化)的目标以及许多重要酶活性位点中的关键残基,因此我们对将赖氨酸进行光切以控制蛋白质的定位感兴趣,翻译后修饰和酶活性。以前尚未在活细胞中证明蛋白质中赖氨酸残基介导的这些重要功能的光化学控制。在这里,我们合成了1,并开发了一个吡咯基-tRNA合成酶/ tRNA对,以遗传方式编码此氨基酸的掺入,以响应哺乳动物细胞中的琥珀密码子。为了举例说明这种氨基酸的效用,我们将核纤蛋白和肿瘤抑制因子p53的核定位序列(NLSs)固定在人细胞中,从而使蛋白质在细胞溶胶中定位不正确。我们用光脉冲触发了蛋白质核输入,从而使我们能够直接定量核输入的动力学。

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