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基于多功能纳米抗体的方法在体成像、追踪和重建功能性 Neurexin-1。

Versatile nanobody-based approach to image, track and reconstitute functional Neurexin-1 in vivo.

机构信息

Section on Cellular Communication, Eunice Kennedy Shriver National Institute of Child Health and Human Development, NIH, Bethesda, MD, USA.

Centralized Core Research Facility-Microscopy, All India Institute of Medical Sciences, New Delhi, Delhi, India.

出版信息

Nat Commun. 2024 Jul 18;15(1):6068. doi: 10.1038/s41467-024-50462-2.

Abstract

Neurexins are key adhesion proteins that coordinate extracellular and intracellular synaptic components. Nonetheless, the low abundance of these multidomain proteins has complicated any localization and structure-function studies. Here we combine an ALFA tag (AT)/nanobody (NbALFA) tool with classic genetics, cell biology and electrophysiology to examine the distribution and function of the Drosophila Nrx-1 in vivo. We generate full-length and ΔPDZ ALFA-tagged Nrx-1 variants and find that the PDZ binding motif is key to Nrx-1 surface expression. A PDZ binding motif provided in trans, via genetically encoded cytosolic NbALFA-PDZ chimera, fully restores the synaptic localization and function of Nrx. Using cytosolic NbALFA-mScarlet intrabody, we achieve compartment-specific detection of endogenous Nrx-1, track live Nrx-1 transport along the motor neuron axons, and demonstrate that Nrx-1 co-migrates with Rab2-positive vesicles. Our findings illustrate the versatility of the ALFA system and pave the way towards dissecting functional domains of complex proteins in vivo.

摘要

神经连接蛋白是关键的粘附蛋白,可协调细胞外和细胞内的突触成分。尽管如此,这些多结构域蛋白的丰度低,使得任何定位和结构功能研究都变得复杂。在这里,我们将 ALFA 标签(AT)/纳米抗体(NbALFA)工具与经典遗传学、细胞生物学和电生理学相结合,研究果蝇 Nrx-1 在体内的分布和功能。我们生成全长和 ΔPDZ ALFA 标记的 Nrx-1 变体,并发现 PDZ 结合基序是 Nrx-1 表面表达的关键。通过遗传编码的细胞质 NbALFA-PDZ 嵌合体提供的 PDZ 结合基序,完全恢复了 Nrx 的突触定位和功能。使用细胞质 NbALFA-mScarlet 内体,我们实现了内源性 Nrx-1 的特定区室检测,追踪活 Nrx-1 沿运动神经元轴突的运输,并证明 Nrx-1 与 Rab2 阳性囊泡共迁移。我们的发现说明了 ALFA 系统的多功能性,并为在体内剖析复杂蛋白质的功能结构域铺平了道路。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8389/11258300/15c378dbf2ab/41467_2024_50462_Fig1_HTML.jpg

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