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Dissecting Torsin/cofactor function at the nuclear envelope: a genetic study

机译:剖析核膜上的都灵/辅因子功能:一项遗传研究

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摘要

The human genome encodes four Torsin ATPases, the functions of which are poorly understood. In this study, we use CRISPR/Cas9 engineering to delete all four Torsin ATPases individually and in combination. Using nuclear envelope (NE) blebbing as a phenotypic measure, we establish a direct correlation between the number of inactivated Torsin alleles and the occurrence of omega-shaped herniations within the lumen of the NE. A similar, although not identical, redundancy is observed for LAP1 and LULL1, which serve as regulatory cofactors for a subset of Torsin ATPases. Unexpectedly, deletion of Tor2A in a TorA/B/3A-deficient background results in a stark increase of bleb formation, even though Tor2A does not respond to LAP1/LULL1 stimulation. The robustness of the observed phenotype in Torsin-deficient cells enables a structural analysis via electron microscopy tomography and a compositional analysis via immunogold labeling. Ubiquitin and nucleoporins were identified as distinctively localizing components of the omega-shaped bleb structure. These findings suggest a functional link between the Torsin/cofactor system and NEuclear pore complex biogenesis or homeostasis and establish a Torsin-deficient cell line as a valuable experimental platform with which to decipher Torsin function.
机译:人类基因组编码四种Torsin ATPase,其功能尚不清楚。在这项研究中,我们使用CRISPR / Cas9工程技术单独或组合删除所有四个Torsin ATPase。使用核包膜(NE)起泡作为一种表型措施,我们建立灭活的Torsin等位基因的数量与NE腔内的ω型疝的发生之间的直接相关性。对于LAP1和LULL1,可以观察到相似但不相同的冗余,它们充当Torsin ATPase子集的调节辅助因子。出乎意料的是,即使Tor2A对LAP1 / LULL1的刺激没有反应,在TorA / B / 3A缺失的背景下Tor2A的缺失也会导致气泡形成的急剧增加。在Torsin缺陷型细胞中观察到的表型的鲁棒性使得可以通过电子显微镜断层扫描进行结构分析,并通过免疫金标记进行成分分析。泛素和核孔蛋白被确定为Ω形气泡结构的独特定位成分。这些发现暗示了Torsin /辅因子系统与NE /核孔复合物的生物发生或体内平衡之间的功能联系,并建立了Torsin缺陷型细胞系,作为破译Torsin功能的有价值的实验平台。

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