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将生长素诱导降解系统与基于CRISPR/Cas9的基因组编辑相结合,用于条件性耗尽内源性黑腹果蝇蛋白质。

Combining the auxin-inducible degradation system with CRISPR/Cas9-based genome editing for the conditional depletion of endogenous Drosophila melanogaster proteins.

作者信息

Bence Melinda, Jankovics Ferenc, Lukácsovich Tamás, Erdélyi Miklós

机构信息

Institute of Genetics, Biological Research Centre of the Hungarian Academy of Sciences, Szeged, Hungary.

Brain Research Institute, University of Zürich, Switzerland.

出版信息

FEBS J. 2017 Apr;284(7):1056-1069. doi: 10.1111/febs.14042. Epub 2017 Mar 8.

DOI:10.1111/febs.14042
PMID:28207183
Abstract

Inducible protein degradation techniques have considerable advantages over classical genetic approaches, which generate loss-of-function phenotypes at the gene or mRNA level. The plant-derived auxin-inducible degradation system (AID) is a promising technique which enables the degradation of target proteins tagged with the AID motif in nonplant cells. Here, we present a detailed characterization of this method employed during the adult oogenesis of Drosophila. Furthermore, with the help of CRISPR/Cas9-based genome editing, we improve the utility of the AID system in the conditional elimination of endogenously expressed proteins. We demonstrate that the AID system induces efficient and reversible protein depletion of maternally provided proteins both in the ovary and the early embryo. Moreover, the AID system provides a fine spatiotemporal control of protein degradation and allows for the generation of different levels of protein knockdown in a well-regulated manner. These features of the AID system enable the unraveling of the discrete phenotypes of genes with highly complex functions. We utilized this system to generate a conditional loss-of-function allele which allows for the specific degradation of the Vasa protein without affecting its alternative splice variant (solo) and the vasa intronic gene (vig). With the help of this special allele, we demonstrate that dramatic decrease of Vasa protein in the vitellarium does not influence the completion of oogenesis as well as the establishment of proper anteroposterior and dorsoventral polarity in the developing oocyte. Our study suggests that both the localization and the translation of gurken mRNA in the vitellarium is independent from Vasa.

摘要

诱导性蛋白质降解技术相较于经典遗传学方法具有显著优势,经典遗传学方法在基因或mRNA水平产生功能缺失表型。植物源生长素诱导降解系统(AID)是一种很有前景的技术,它能够在非植物细胞中降解带有AID基序标签的靶蛋白。在此,我们详细描述了该方法在果蝇成虫卵子发生过程中的应用。此外,借助基于CRISPR/Cas9的基因组编辑技术,我们提高了AID系统在条件性消除内源性表达蛋白方面的效用。我们证明,AID系统在卵巢和早期胚胎中均能有效且可逆地耗尽母源提供的蛋白。而且,AID系统能够对蛋白质降解进行精细的时空控制,并能以良好调控的方式产生不同程度的蛋白质敲低。AID系统的这些特性使得具有高度复杂功能的基因的离散表型得以揭示。我们利用该系统产生了一个条件性功能缺失等位基因,该等位基因能够特异性降解Vasa蛋白,而不影响其可变剪接变体(单独形式)和vasa内含子基因(vig)。借助这个特殊的等位基因,我们证明,卵黄发生区Vasa蛋白的显著减少并不影响卵子发生的完成以及发育中卵母细胞前后极性和背腹极性的建立。我们的研究表明,卵黄发生区中gurken mRNA的定位和翻译均独立于Vasa。

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