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重新审视固定和包埋技术,以优化组织中树突状细胞亚群的检测。

Revisiting fixation and embedding techniques for optimal detection of dendritic cell subsets in tissues.

机构信息

Transgene S.A., Illkirch Graffenstaden, France (NA, FS, RR)Novartis Institutes for Biomedical Research, Basel, Switzerland (NA)Fisher Scientific, Illkirch Graffenstaden., France (FS).

Transgene S.A., Illkirch Graffenstaden, France (NA, FS, RR)Novartis Institutes for Biomedical Research, Basel, Switzerland (NA)Fisher Scientific, Illkirch Graffenstaden., France (FS)

出版信息

J Histochem Cytochem. 2014 Sep;62(9):661-71. doi: 10.1369/0022155414539963. Epub 2014 May 29.

DOI:10.1369/0022155414539963
PMID:24874853
Abstract

Organ-specific cell types are maintained by tissue homeostasis and may vary in nature and/or frequency in pathological situations. Moreover, within a cell lineage, some sub-populations, defined by combinations of cell-surface markers, may have specific functions. Dendritic cells are the epitome of such a population as they may be subdivided into discrete sub-groups with defined functions in specific compartments of various organs. Technically, to study the distribution of DC sub-populations, it involves performing multiparametric immunofluorescence on well-conserved organ structures. However, immunodetection may be impacted by protein cross-linking and antigenic epitope masking by the use of 10% neutral-buffered formalin. To circumvent this and to preserve a good morphological tissue structure, we evaluated alternative fixatives such as Periodate Lysine Paraformaldehyde or Tris Zinc fixatives in combination with other embedding techniques. The cryosection protocols were adapted for optimal antigen detection but offered a poor morphological preservation. We therefore developed a new methodology based on Tris Zinc fixative, gelatin-sucrose embedding and freezing. Using multiple DC markers, we demonstrate that this treatment is an optimal protocol for cell-surface marker detection on high-quality tissue sections.

摘要

组织特异性细胞类型由组织内稳态维持,在病理情况下其性质和/或频率可能会有所不同。此外,在细胞谱系内,一些亚群通过细胞表面标志物的组合来定义,可能具有特定的功能。树突状细胞就是这种群体的典型代表,因为它们可以根据在特定器官的特定隔室中的功能分为离散的亚群。从技术上讲,要研究 DC 亚群的分布,需要对保存完好的器官结构进行多参数免疫荧光染色。然而,由于使用 10%中性缓冲福尔马林进行蛋白交联和抗原表位掩蔽,免疫检测可能会受到影响。为了避免这种情况并保持良好的组织形态结构,我们评估了替代固定剂,如过碘酸钠赖氨酸多聚甲醛或三锌固定剂,并结合了其他包埋技术。冷冻切片方案经过优化以实现最佳抗原检测,但提供的形态保存效果不佳。因此,我们开发了一种基于三锌固定剂、明胶-蔗糖包埋和冷冻的新方法。使用多种 DC 标志物,我们证明该处理方法是在高质量组织切片上进行细胞表面标志物检测的最佳方案。

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