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对从新生大鼠大脑中克隆至高纯度的富含小胶质细胞的培养物进行定量形态计量学和细胞类型特异性群体分析。

Quantitative morphometric and cell-type-specific population analysis of microglia-enriched cultures subcloned to high purity from newborn rat brains.

作者信息

Dulka Karolina, Nacsa Kálmán, Lajkó Noémi, Gulya Karoly

机构信息

Department of Cell Biology and Molecular Medicine, University of Szeged, Szeged, Hungary.

出版信息

IBRO Neurosci Rep. 2021 Feb 6;10:119-129. doi: 10.1016/j.ibneur.2021.01.007. eCollection 2021 Jun.

Abstract

Morphological and functional characterizations of cultured microglia are essential for the improved understanding of their roles in neuronal health and disease. Although some studies (phenotype analysis, phagocytosis) can be carried out in mixed or microglia-enriched cultures, in others (gene expression) pure microglia must be used. If the use of genetically modified microglial cells is not feasible, isolation of resident microglia from nervous tissue must be carried out. In this study, mixed primary cultures were established from the forebrains of newborn rats. Secondary microglia-enriched cultures were then prepared by shaking off these cells from the primary cultures, which were subsequently used to establish tertiary cultures by further shaking off the easily detachable microglia. The composition of these cultures was quantitatively analyzed by immunocytochemistry of microglia-, astrocyte-, oligodendrocyte- and neuron-specific markers to determine yield and purity. Microglia were quantitatively characterized regarding morphological and proliferation aspects. Secondary and tertiary cultures typically exhibited 73.3% ± 17.8% and 93.1% ± 6.0% purity for microglia, respectively, although the total number of microglia in the latter was much smaller. One in seven attempts of culturing the tertiary cultures had ~99% purity for microglia. The overall yield from the number of cells plated at DIV0 to the Iba1-positive microglia in tertiary cultures was ~1%. Astrocytic and neuronal contamination progressively decreased during subcloning, while oligodendrocytes were found sporadically throughout culturing. Although the tertiary microglia cultures had a low yield, they produced consistently high purity for microglia; after validation, such cultures are suitable for purity-sensitive functional screenings (gene/protein expression).

摘要

对培养的小胶质细胞进行形态学和功能表征,对于更好地理解它们在神经元健康和疾病中的作用至关重要。尽管一些研究(表型分析、吞噬作用)可以在混合培养物或富含小胶质细胞的培养物中进行,但其他研究(基因表达)则必须使用纯小胶质细胞。如果使用基因改造的小胶质细胞不可行,则必须从神经组织中分离驻留小胶质细胞。在本研究中,从新生大鼠的前脑建立了混合原代培养物。然后通过从原代培养物中摇落这些细胞来制备富含小胶质细胞的二代培养物,随后通过进一步摇落易于分离的小胶质细胞来建立三代培养物。通过对小胶质细胞、星形胶质细胞、少突胶质细胞和神经元特异性标志物进行免疫细胞化学定量分析这些培养物的组成,以确定产量和纯度。从小胶质细胞的形态和增殖方面对其进行了定量表征。二代和三代培养物中小胶质细胞的纯度通常分别为73.3%±17.8%和93.1%±6.0%,尽管后者中小胶质细胞的总数要少得多。培养三代培养物的七次尝试中有一次小胶质细胞的纯度约为99%。从接种在第0天的细胞数量到三代培养物中Iba1阳性小胶质细胞的总产量约为1%。在亚克隆过程中,星形胶质细胞和神经元的污染逐渐减少,而在整个培养过程中偶尔会发现少突胶质细胞。尽管三代小胶质细胞培养物的产量较低,但它们产生的小胶质细胞纯度始终很高;经过验证,这种培养物适用于对纯度敏感的功能筛选(基因/蛋白质表达)。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e0c8/8019997/9a6ef685c0ae/gr1.jpg

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