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首页> 外文期刊>The Biochemical Journal >Targeting protein function: the expanding toolkit for conditional disruption
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Targeting protein function: the expanding toolkit for conditional disruption

机译:靶向蛋白质功能:有条件中断的扩展工具包

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摘要

A major objective in biological research is to understand spatial and temporal requirements for any given gene, especially in dynamic processes acting over short periods, such as catalytically driven reactions, subcellular transport, cell division, cell rearrangement and cell migration. The interrogation of such processes requires the use of rapid and flexible methods of interfering with gene function. However, many of the most widely used interventional approaches, such as RNAi or CRISPR (clusteredregularly interspaced short palindromic repeats)-Cas9 (CRISPR-associated 9), operate at the level of the gene or its transcripts, meaning that the effects of gene perturbation are exhibited over longer time frames than the process under investigation. There has been much activity over the last fewyears to address this fundamental problem. In the present review, we describe recent advances in disruption technologies acting at the level of the expressed protein, involving inducible methods of protein cleavage, (in)activation, protein sequestrationor degradation. Drawing on examples from model organisms we illustrate the utility of fast-acting techniques and discuss how different components of the molecular toolkit can be employed to dissect previously intractable biochemical processes and cellular behaviours.
机译:生物学研究中的一个主要目标是了解对任何给定基因的空间和时间要求,特别是在短时间的动态过程中,例如催化驱动的反应,亚细胞输送,细胞分裂,细胞重排和细胞迁移。这些过程的询问需要利用干扰基因功能的快速和灵活的方法。然而,许多最广泛使用的介入方法,例如RNAi或CRISPR(Clusteredregulary interspaced短语重复)-CAS9(CIRSPR相关的9),在基因或其转录物的水平下运行,这意味着基因扰动的影响在较长的时间范围内比调查的过程展出。在最后的少年上有很多活动来解决这一基本问题。在本综述中,我们描述了在表达蛋白水平的中断技术的最近进展,涉及诱导蛋白质切割的诱导方法,(in)活化,蛋白质螯合剂降解。从模型生物体的实例上绘制我们的示例,说明了快速作用技术的效用,并讨论了分子工具包的不同组分如何用于筛选以前顽固的生物化学过程和细胞行为。

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