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Electroporated recombinant proteins as tools for in vivo functional complementation imaging and chemical biology

机译:电穿孔重组蛋白作为体内功能互补成像和化学生物学的工具

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摘要

Delivery of native or chemically modified recombinant proteins into mammalian cells shows promise for functional investigations and various technological applications, but concerns that sub-cellular localization and functional integrity of delivered proteins may be affected remain high. Here, we surveyed batch electroporation as a delivery tool for single polypeptides and multi-subunit protein assemblies of the kinetochore, a spatially confined and well-studied subcellular structure. After electroporation into human cells, recombinant fluorescent Ndc80 and Mis12 multi-subunit complexes exhibited native localization, physically interacted with endogenous binding partners, and functionally complemented depleted endogenous counterparts to promote mitotic checkpoint signaling and chromosome segregation. Farnesylation is required for kinetochore localization of the Dynein adaptor Spindly. In cells with chronically inhibited farnesyl transferase activity, in vitro farnesylation and electroporation of recombinant Spindly faithfully resulted in robust kinetochore localization. Our data show that electroporation is well-suited to deliver synthetic and chemically modified versions of functional proteins, and, therefore, constitutes a promising tool for applications in chemical and synthetic biology.
机译:将天然或化学修饰的重组蛋白递送至哺乳动物细胞显示出功能研究和各种技术应用的前景,但人们担心,亚细胞定位和所递送蛋白的功能完整性可能会受到影响。在这里,我们调查了分批电穿孔作为动粒的单个多肽和多亚基蛋白质组装体的递送工具,该单个多肽和多亚基蛋白质组装体是在空间上受限且经过充分研究的亚细胞结构。在电穿孔进入人体细胞后,重组荧光Ndc80和Mis12多亚基复合物表现出天然定位,与内源性结合伴侣发生物理相互作用,并在功能上补充了耗尽的内源性对应物,从而促进了有丝分裂检查点信号传导和染色体分离。 Dynein接头Spindly的线粒体定位需要法尼基化。在具有长期抑制法呢基转移酶活性的细胞中,重组的Spindly的体外法呢基化和电穿孔忠实地导致了稳健的线粒体定位。我们的数据表明,电穿孔非常适合提供功能蛋白的合成和化学修饰版本,因此,构成了在化学和合成生物学中应用的有前途的工具。

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