探测细胞增殖:染料选择注意事项

4区 生物学 Q4 Biochemistry, Genetics and Molecular Biology Methods in cell biology Pub Date : 2024-01-01 Epub Date: 2024-04-04 DOI:10.1016/bs.mcb.2024.02.012
Kah Teong Soh, Joseph D Tario, Katharine A Muirhead, Paul K Wallace
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引用次数: 0

摘要

广义上讲,细胞追踪染料是一种荧光化合物,能与细胞上或细胞内的成分稳定结合,从而追踪标记细胞的命运。它们的染色应该明亮均匀,不会影响细胞功能。为了监测细胞增殖,每次细胞分裂时,细胞追踪染料的强度应在子细胞之间平均减弱。这些染料可分为两类。蛋白质活性染料通过与细胞内蛋白质发生共价但非选择性反应来标记细胞。羧基荧光素二乙酸琥珀酰亚胺酯(CFSE)是普通蛋白质标记的原型。膜插层染料通过在质膜内进行非选择性和非共价分区来标记细胞。PKH 膜染料是亲脂性化合物的典范,其化学性质允许它们保留在生物膜内,如果使用得当,不会影响细胞的生长、活力或增殖。在此,我们提供了使用这两类染料标记细胞系和外周血单核细胞的注意事项。我们列举了优化实验的实例,以及染色程序的关键环节,以帮助降低常见风险。值得注意的是,我们提供了用蛋白质染料和膜追踪染料标记对数生长细胞系的数据,以比较 6 天内染料的损失率。我们发现,双重染色的细胞与相应的单一染色细胞的染料损失率相同。然而,蛋白活性染料导致的荧光强度下降比膜活性染料更快,这表明存在额外的不依赖于分裂的染料损失。
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Probing cell proliferation: Considerations for dye selection.

Broadly speaking, cell tracking dyes are fluorescent compounds that bind stably to components on or within the cells so the fate of the labeled cells can be followed. Their staining should be bright and homogeneous without affecting cell function. For purposes of monitoring cell proliferation, each time a cell divides the intensity of cell tracking dye should diminish equally between daughter cells. These dyes can be grouped into two different classes. Protein reactive dyes label cells by reacting covalently but non-selectively with intracellular proteins. Carboxyfluorescein diacetate succinimidyl ester (CFSE) is the prototypic general protein label. Membrane intercalating dyes label cells by partitioning non-selectively and non-covalently within the plasma membrane. The PKH membrane dyes are examples of lipophilic compounds whose chemistry allows for their retention within biological membranes without affecting cellular growth, viability, or proliferation when used properly. Here we provide considerations based for labeling cell lines and peripheral blood mononuclear cells using both classes of dyes. Examples from optimization experiments are presented along with critical aspects of the staining procedures to help mitigate common risks. Of note, we present data where a logarithmically growing cell line is labeled with both a protein dye and a membrane tracking dye to compare dye loss rates over 6days. We found that dual stained cells paralleled dye loss of the corresponding single stained cells. The decrease in fluorescence intensity by protein reactive dyes, however, was more rapid than that with the membrane reactive dyes, indicating the presence of additional division-independent dye loss.

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来源期刊
Methods in cell biology
Methods in cell biology 生物-细胞生物学
CiteScore
3.10
自引率
0.00%
发文量
125
审稿时长
3 months
期刊介绍: For over fifty years, Methods in Cell Biology has helped researchers answer the question "What method should I use to study this cell biology problem?" Edited by leaders in the field, each thematic volume provides proven, state-of-art techniques, along with relevant historical background and theory, to aid researchers in efficient design and effective implementation of experimental methodologies. Over its many years of publication, Methods in Cell Biology has built up a deep library of biological methods to study model developmental organisms, organelles and cell systems, as well as comprehensive coverage of microscopy and other analytical approaches.
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