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一种快速、通用的协议,可用于对幼虫整个身体中转基因表达进行 3D 可视化。

A quick and versatile protocol for the 3D visualization of transgene expression across the whole body of larval .

机构信息

Leibniz Institute for Neurobiology, Combinatorial NeuroImaging Core Facility (CNI), Magdeburg, Germany.

Department of Genetics of Learning and Memory, Leibniz Institute for Neurobiology, Magdeburg, Germany.

出版信息

J Neurogenet. 2021 Sep;35(3):306-319. doi: 10.1080/01677063.2021.1892096. Epub 2021 Mar 10.

DOI:10.1080/01677063.2021.1892096
PMID:33688796
Abstract

Larval are used as a genetically accessible study case in many areas of biological research. Here we report a fast, robust and user-friendly procedure for the whole-body multi-fluorescence imaging of larvae; the protocol has been optimized specifically for larvae by systematically tackling the pitfalls associated with clearing this small but cuticularized organism. Tests on various fluorescent proteins reveal that the recently introduced monomeric infrared fluorescent protein (mIFP) is particularly suitable for our approach. This approach comprises an effective, low-cost clearing protocol with minimal handling time and reduced toxicity in the reagents employed. It combines a success rate high enough to allow for small-scale screening approaches and a resolution sufficient for cellular-level analyses with light sheet and confocal microscopy. Given that publications and database documentations typically specify expression patterns of transgenic driver lines only within a given organ system of interest, the present procedure should be versatile enough to extend such documentation systematically to the whole body. As examples, the expression patterns of transgenic driver lines covering the majority of neurons, or subsets of chemosensory, central brain or motor neurons, are documented in the context of whole larval body volumes (using nsyb-Gal4, IR76b-Gal4, APL-Gal4 and mushroom body Kenyon cells, or OK371-Gal4, respectively). Notably, the presented protocol allows for triple-color fluorescence imaging with near-infrared, red and yellow fluorescent proteins.

摘要

幼虫被广泛应用于生物学研究的各个领域,作为一种具有遗传可操作性的研究模型。本研究报告了一种用于幼虫整体多荧光成像的快速、稳健且用户友好的方法;该方案是专门针对幼虫进行优化的,通过系统地解决与清除这个小而角质化生物体相关的难题。对各种荧光蛋白的测试表明,最近引入的单体近红外荧光蛋白(mIFP)特别适合我们的方法。该方法包括一种有效的、低成本的清除方案,处理时间短,所用试剂的毒性低。它的成功率足够高,足以进行小规模的筛选方法,分辨率足以进行基于光片和共聚焦显微镜的细胞水平分析。由于出版物和数据库文档通常仅在特定感兴趣的器官系统内指定转基因驱动线的表达模式,因此本程序应该足够通用,可以系统地将此类文档扩展到整个身体。例如,以幼虫整体体积为背景,记录了覆盖大多数神经元或化学感觉神经元、中枢脑神经元或运动神经元亚群的转基因驱动线的表达模式(分别使用 nsyb-Gal4、IR76b-Gal4、APL-Gal4 和蘑菇体 Kenyon 细胞或 OK371-Gal4)。值得注意的是,所提出的方案允许进行近红外、红色和黄色荧光蛋白的三色荧光成像。

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