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利用同步辐射 X 射线荧光和 STED 超分辨率显微镜对原代神经元中的金属和蛋白质进行相关的纳米成像:实验验证。

Correlative nano-imaging of metals and proteins in primary neurons by synchrotron X-ray fluorescence and STED super resolution microscopy: Experimental validation.

机构信息

Univ. Bordeaux, CNRS, LP2I Bordeaux, UMR 5797, Chemical Imaging and Speciation, F-33170 Gradignan, France.

出版信息

J Neurosci Methods. 2022 Nov 1;381:109702. doi: 10.1016/j.jneumeth.2022.109702. Epub 2022 Sep 5.

DOI:10.1016/j.jneumeth.2022.109702
PMID:36064068
Abstract

BACKGROUND

It is becoming increasingly clear that biological metals such as iron, copper or zinc are involved in synaptic functions, and in particular in the mechanisms of synaptogenesis and subsequent plasticity. Understanding the role of metals on synaptic functions is a difficult challenge due to the very low concentration of these elements in neurons and to the submicrometer size of synaptic compartments.

NEW METHOD

To address this challenge we have developed a correlative nano-imaging approach combining metal and protein detection. First, stimulated emission depletion (STED) microscopy, a super resolution optical microscopy technique, is applied to locate fluorescently labeled proteins. Then, synchrotron radiation induced X-ray fluorescence (SXRF) is performed on the same regions of interest, e.g. synaptic compartments.

RESULTS

We present here the principle scheme that allows this correlative nano-imaging and its experimental validation. We applied this correlative nano-imaging to the study of the physiological distribution of metals in synaptic compartments of primary rat hippocampal neurons. We thus compared the nanometric distribution of metals with that of synaptic proteins, such as PSD95 or cytoskeleton proteins.

COMPARISON WITH EXISTING METHOD(S): Compared to correlative imaging approaches currently used to characterize synaptic structures, such as electron microscopy correlated with optical fluorescence, our approach allows for ultra-sensitive detection of trace metals using highly focused synchrotron radiation beams.

CONCLUSION

We provide proof-of-principle for correlative imaging of metals and proteins at the synaptic scale and discuss the present limitations and future developments in this area.

摘要

背景

越来越明显的是,生物金属如铁、铜或锌参与突触功能,特别是在突触发生和随后的可塑性的机制中。由于神经元中这些元素的浓度非常低,以及突触隔室的亚微米尺寸,理解金属对突触功能的作用是一个具有挑战性的难题。

新方法

为了解决这个挑战,我们开发了一种结合金属和蛋白质检测的相关纳米成像方法。首先,受激发射损耗(STED)显微镜是一种超分辨率光学显微镜技术,用于定位荧光标记的蛋白质。然后,在同一感兴趣区域(例如突触隔室)上进行同步辐射诱导的 X 射线荧光(SXRF)。

结果

我们在这里介绍了允许这种相关纳米成像的原理方案及其实验验证。我们将这种相关的纳米成像应用于研究原代大鼠海马神经元突触隔室中金属的生理分布。因此,我们将金属的纳米分布与 PSD95 或细胞骨架蛋白等突触蛋白进行了比较。

与现有方法的比较

与目前用于表征突触结构的相关成像方法(例如电子显微镜与光学荧光相关)相比,我们的方法允许使用高度聚焦的同步辐射束对痕量金属进行超灵敏检测。

结论

我们提供了在突触尺度上对金属和蛋白质进行相关成像的原理证明,并讨论了该领域目前的限制因素和未来的发展方向。

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