Heiligenstein Xavier, Lucas Miriam S
CryoCapCell, Le Kremlin-Bicêtre, Paris, France.
Scientific Center for Light and Electron Microscopy (ScopeM), ETH Zurich, Zurich, Switzerland.
Front Cell Dev Biol. 2022 Jun 30;10:866472. doi: 10.3389/fcell.2022.866472. eCollection 2022.
Sample preparation is the novel bottleneck for high throughput correlative light and electron microscopy (CLEM). Protocols suitable for both imaging methods must therefore balance the requirements of each technique. For fluorescence light microscopy, a structure of interest can be targeted using: 1) staining, which is often structure or tissue specific rather than protein specific, 2) dye-coupled proteins or antibodies, or 3) genetically encoded fluorescent proteins. Each of these three methods has its own advantages. For ultrastructural investigation by electron microscopy (EM) resin embedding remains a significant sample preparation approach, as it stabilizes the sample such that it withstands the vacuum conditions of the EM, and enables long-term storage. Traditionally, samples are treated with heavy metal salts prior to resin embedding, in order to increase imaging contrast for EM. This is particularly important for volume EM (vEM) techniques. Yet, commonly used contrasting agents (e.g., osmium tetroxide, uranyl acetate) tend to impair fluorescence. The discovery that fluorescence can be preserved in resin-embedded specimens after mild heavy metal staining was a game changer for CLEM. These so-called in-resin fluorescence protocols present a significant leap forward for CLEM approaches towards high precision localization of a fluorescent signal in (volume) EM data. Integrated microscopy approaches, combining LM and EM detection into a single instrument certainly require such an "all in one" sample preparation. Preserving, or adding, dedicated fluorescence prior to resin embedding requires a compromise, which often comes at the expense of EM imaging contrast and membrane visibility. Especially vEM can be strongly hampered by a lack of heavy metal contrasting. This review critically reflects upon the fundamental aspects of resin embedding with regard to 1) specimen fixation and the physics and chemistry underlying the preservation of protein structure with respect to fluorescence and antigenicity, 2) optimization of EM contrast for transmission or scanning EM, and 3) the choice of embedding resin. On this basis, various existing workflows employing in-resin fluorescence are described, highlighting their common features, discussing advantages and disadvantages of the respective approach, and finally concluding with promising future developments for in-resin CLEM.
样本制备是高通量相关光电子显微镜(CLEM)的新瓶颈。因此,适用于两种成像方法的方案必须平衡每种技术的要求。对于荧光光学显微镜,可以使用以下方法靶向感兴趣的结构:1)染色,其通常是结构或组织特异性的,而非蛋白质特异性的;2)染料偶联蛋白或抗体;或3)基因编码的荧光蛋白。这三种方法各有其优点。对于通过电子显微镜(EM)进行的超微结构研究,树脂包埋仍然是一种重要的样本制备方法,因为它能稳定样本,使其能够承受EM的真空条件,并便于长期保存。传统上,在树脂包埋之前,样本要用重金属盐处理,以增加EM成像的对比度。这对于体积电子显微镜(vEM)技术尤为重要。然而,常用的造影剂(如四氧化锇、醋酸铀)往往会损害荧光。轻度重金属染色后,树脂包埋标本中的荧光可以保留,这一发现改变了CLEM的局面。这些所谓的树脂内荧光方案代表了CLEM方法在(体积)EM数据中对荧光信号进行高精度定位方面的重大飞跃。将光学显微镜(LM)和电子显微镜(EM)检测集成到一台仪器中的综合显微镜方法当然需要这样一种“一体化”的样本制备。在树脂包埋之前保留或添加专用荧光需要做出妥协,这通常会以牺牲EM成像对比度和膜可见性为代价。特别是vEM可能会因缺乏重金属造影而受到严重阻碍。本综述批判性地反思了树脂包埋的基本方面,涉及1)标本固定以及与荧光和抗原性相关的蛋白质结构保存的物理和化学原理,2)透射或扫描电子显微镜的EM对比度优化,以及3)包埋树脂的选择。在此基础上,描述了各种现有的采用树脂内荧光的工作流程,突出了它们的共同特征,讨论了各自方法的优缺点,最后总结了树脂内CLEM未来有前景的发展方向。
