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一种用于海胆幼虫和幼体的共聚焦显微镜观察和三维图像重建的简单快速染色方法。

An easy and rapid staining method for confocal microscopic observation and reconstruction of three-dimensional images of echinoderm larvae and juveniles.

机构信息

Research Center for Marine Biology, Graduate School of Life Sciences, Tohoku University, Aomori, Japan.

Spectrography and Bioimaging Facility, National Institute for Basic Biology Core Research Facilities, National Institute for Basic Biology, Aichi, Japan.

出版信息

Dev Growth Differ. 2021 Dec;63(9):478-487. doi: 10.1111/dgd.12758. Epub 2021 Nov 21.

DOI:10.1111/dgd.12758
PMID:34747504
Abstract

The morphologies of the internal organs of echinoderm larvae and juveniles are difficult to study using conventional optical microscopes because of their structural complexity and opaqueness. This paper describes an easy and rapid protocol involving Nile blue staining followed by benzyl alcohol/benzyl benzoate (BABB) clearing to overcome this limitation. This method was developed for a three-dimensional (3D) analysis of the internal structures of advanced larvae and juveniles of echinoderms (the sea lily Metacrinus rotundus, the sea urchin Hemicentrotus pulcherrimus, and the sand dollar Scaphechinus mirabilis) and is suitable for obtaining serial optical images by confocal microscopy without the use of specific antibodies or special reagents for labeling. Nile blue is an easy-to-use stain that offers several advantages for confocal microscopy such as it can stain various tissues with strong fluorescent signals without substantial bleaching during observation. We found that the strong fluorescence signal of Nile blue quickly yielded clear high-resolution optical section images for 3D reconstruction. BABB clearing rendered opaque larvae highly transparent. The clearing procedure was also easy and quick. During the process, agarose embedding prior to staining and clearing was found to be critical for handling the samples of less than 500-μm length and stabilizing their orientations. To conclude, the protocol described is useful for performing a rapid and accurate 3D morphological analysis of echinoderm larvae and juveniles.

摘要

由于其结构的复杂性和不透明性,用传统的光学显微镜很难研究棘皮动物幼虫和幼体的内部器官形态。本文描述了一种简单而快速的方法,涉及尼罗蓝染色,然后用苄醇/苯甲酸苄酯(BABB)清除,以克服这一限制。该方法是为了对棘皮动物(海百合 Metacrinus rotundus、海胆 Hemicentrotus pulcherrimus 和沙钱 Scaphechinus mirabilis)的高级幼虫和幼体的内部结构进行三维(3D)分析而开发的,适合通过共聚焦显微镜获得连续的光学图像,而无需使用特殊的抗体或特殊的标记试剂。尼罗蓝是一种易于使用的染色剂,它为共聚焦显微镜提供了几个优点,例如可以用强荧光信号染色各种组织,在观察过程中不会有明显的漂白。我们发现,尼罗蓝的强荧光信号很快产生了清晰的高分辨率光学切片图像,用于 3D 重建。BABB 清除使不透明的幼虫变得高度透明。该清除过程也很简单快捷。在这个过程中,我们发现,在染色和清除之前进行琼脂糖包埋对于处理小于 500-μm 长度的样本和稳定它们的方向非常重要。总之,所描述的方案对于棘皮动物幼虫和幼体的快速、准确的 3D 形态分析是有用的。

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