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在体内胚胎脊髓神经元中,微管的存在对于新生轴突的生成并非必需。

Microtubules are not required to generate a nascent axon in embryonic spinal neurons in vivo.

机构信息

Centre for Developmental Neurobiology, Institute of Psychiatry, Psychology and Neuroscience, King's College London, London, UK.

The Francis Crick Institute, London, UK.

出版信息

EMBO Rep. 2022 Nov 7;23(11):e52493. doi: 10.15252/embr.202152493. Epub 2022 Oct 4.

Abstract

Our understanding of the cell behaviours and cytoskeletal requirements of axon formation is largely derived from in vitro models but how these relate to axon formation in vivo is not clear. In vitro, neurons progress through a well-defined multineurite stage to form an axon and both actin and microtubules cooperate to drive the first steps in neurite and axon morphogenesis. However, these steps are not recapitulated in vivo, and it is not clear whether the underlying cell biological mechanisms may differ also. Here, we investigate the mechanisms that regulate axon formation in embryonic zebrafish spinal neurons in vivo. We find microtubule organising centres are located distant from the site of axon initiation, and microtubule plus-ends are not enriched in the axon during axon initiation. Focal F-actin accumulation precedes axon formation, and we find that nocodazole-treated neurons with no detectable microtubules are still able to form nascent axonal protrusions that are approximately 10-μm long, dilated and relatively long-lived. We suggest spinal axon formation in vivo is fundamentally different from axon formation in in vitro models.

摘要

我们对轴突形成的细胞行为和细胞骨架需求的理解主要来自于体外模型,但这些模型与体内的轴突形成如何相关还不清楚。在体外,神经元经历一个明确的多突阶段以形成轴突,肌动蛋白和微管共同协作,推动神经突和轴突形态发生的最初步骤。然而,这些步骤在体内并没有被重复,也不清楚潜在的细胞生物学机制是否也不同。在这里,我们研究了体内斑马鱼胚胎脊髓神经元中调节轴突形成的机制。我们发现微管组织中心远离轴突起始部位,并且在轴突起始时,微管的正极末端没有在轴突中富集。轴突起始前,局部 F-肌动蛋白聚集,我们发现,用诺考达唑处理的神经元,尽管检测不到微管,但仍能形成大约 10-μm 长、扩张且相对长寿命的新生轴突突起。我们认为,体内的脊髓轴突形成与体外模型中的轴突形成在根本上是不同的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e11e/9638849/d249c16417e0/EMBR-23-e52493-g007.jpg

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