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小鼠骨骼中绿色荧光蛋白(GFP)表达的组织学分析。

Histological analysis of GFP expression in murine bone.

作者信息

Jiang Xi, Kalajzic Zana, Maye Peter, Braut Alen, Bellizzi Justin, Mina Mina, Rowe David W

机构信息

Department of Genetics and Development Biology, University of Connecticut Health Center, Farmington, CT 06030, USA.

出版信息

J Histochem Cytochem. 2005 May;53(5):593-602. doi: 10.1369/jhc.4A6401.2005.

Abstract

The power for appreciating complex cellular interactions during embryonic development using green fluorescent protein (GFP) as a visual histological marker has not been applied to adult tissues due to loss of GFP signal during paraffin embedding and a high autofluorescent background, particularly in section of bone and bone marrow. Here we demonstrate that the GFP signal is well preserved in frozen sections of adult decalcified bone. Using a tape-transfer system that preserves histological relationships, GFP expression can be related to standard histological stains used in bone biology research. The choice of a dual-filter cube and a strong GFP signal makes it possible to readily distinguish at least four different GFP colors that are distinctly different from the autofluorescent background. An additional advantage of the frozen sections is better preservation of immunological epitopes that allow colocalization of an immunostained section with an endogenous GFP and a strong lacZ signal emanating from a beta-gal marker gene. We present an approach for recording multiple images from the same histological section that allows colocalization of a GFP signal with subsequent stains and procedures that destroy GFP. Examples that illustrate the flexibility for dual imaging of various fluorescent signals are described in this study. The same imaging approach can serve as a vehicle for archiving, retrieving, and sharing histological images among research groups.

摘要

利用绿色荧光蛋白(GFP)作为可视化组织学标记来解析胚胎发育过程中复杂细胞相互作用的技术,由于在石蜡包埋过程中GFP信号丢失以及自发荧光背景较高(尤其是在骨和骨髓切片中),尚未应用于成体组织。在此,我们证明GFP信号在成体脱钙骨的冰冻切片中保存良好。使用一种能保持组织学关系的胶带转移系统,GFP表达可与骨生物学研究中使用的标准组织学染色相关联。双滤光片立方体的选择以及强烈的GFP信号使得能够轻松区分至少四种与自发荧光背景明显不同的GFP颜色。冰冻切片的另一个优点是更好地保存了免疫表位,这使得免疫染色切片能够与内源性GFP以及来自β-半乳糖苷酶标记基因的强烈lacZ信号共定位。我们提出了一种从同一组织学切片记录多张图像 的方法,该方法允许GFP信号与后续染色以及破坏GFP的程序共定位。本研究描述了说明各种荧光信号双重成像灵活性的示例。相同的成像方法可作为各研究组之间存档、检索和共享组织学图像的工具。

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