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机构信息

UMR 8576 CNRS, Unité de Glycobiologie Structurale et Fonctionnelle, Université de Lille, Faculté des Sciences et Technologies, Bât. C9, 59655, Villeneuve d'Ascq, France.

出版信息

Angew Chem Int Ed Engl. 2021 Oct 18;60(43):23084-23105. doi: 10.1002/anie.202101502. Epub 2021 Jul 9.

Abstract

The surging development of bioorthogonal chemistry has profoundly transformed chemical biology over the last two decades. Involving chemical partners that specifically react together in highly complex biological fluids, this branch of chemistry now allows researchers to probe biomolecules in their natural habitat through metabolic labelling technologies. Chemical reporter strategies include metabolic glycan labelling, site-specific incorporation of unnatural amino acids in proteins, and post-synthetic labelling of nucleic acids. While a majority of literature reports mark cell-surface exposed targets, implementing bioorthogonal ligations in the interior of cells constitutes a more challenging task. Owing to limiting factors such as membrane permeability of reagents, fluorescence background due to hydrophobic interactions and off-target covalent binding, and suboptimal balance between reactivity and stability of the designed molecular reporters and probes, these strategies need mindful planning to achieve success. In this review, we discuss the hurdles encountered when targeting biomolecules localized in cell organelles and give an easily accessible summary of the strategies at hand for imaging intracellular targets.

摘要

在过去的二十年中,生物正交化学的蓬勃发展深刻地改变了化学生物学。涉及在高度复杂的生物流体中特异性反应的化学伴侣,这个化学分支现在允许研究人员通过代谢标记技术在其自然栖息地中探测生物分子。化学报告策略包括代谢聚糖标记、蛋白质中特异性非天然氨基酸的掺入以及核酸的后期合成标记。虽然大多数文献报道标记细胞表面暴露的靶标,但在细胞内部实施生物正交连接是一项更具挑战性的任务。由于试剂的膜通透性、疏水性相互作用和非靶标共价结合引起的荧光背景以及设计的分子报告器和探针的反应性和稳定性之间的不平衡等限制因素,这些策略需要精心规划才能取得成功。在这篇综述中,我们讨论了在靶向定位于细胞细胞器的生物分子时遇到的障碍,并对用于成像细胞内靶标的现有策略进行了易于理解的总结。

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