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首页> 外文期刊>Journal of Immunological Methods >Optimized lymphocyte isolation methods for analysis of chemokine receptor expression.
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Optimized lymphocyte isolation methods for analysis of chemokine receptor expression.

机译:优化的淋巴细胞分离方法,用于分析趋化因子受体的表达。

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Manipulations typically used to isolate enriched lymphocyte populations from peripheral blood can impact on the measured levels of chemokine receptors. Optimum sensitivity and accurate discrimination of receptor-expressing cell subsets therefore requires cell isolation methods that minimally affect expression levels. We used flow cytometry to examine the effects of different protocols for processing and staining T lymphocytes on chemokine receptor expression. Our results confirm that FACS analysis of some chemokine receptors is compromised after standard methods (such as Ficoll density separation). While the optimal method was typically to stain cells prior to lysing whole blood, this may not be practical in many experimental conditions. In general, we found that staining cells at 37C following Ficoll separation yielded excellent results. However, the precise method used will depend on which receptor is being measured. We used the optimal methods to compare the expression of chemokine receptors on naive and memory T-cell subsets using 8-color flow cytometry.
机译:通常用于从外周血中分离富集的淋巴细胞群体的操作会影响趋化因子受体的测定水平。因此,表达受体的细胞亚群的最佳灵敏度和准确判别需要最小化影响表达水平的细胞分离方法。我们使用流式细胞仪来检查处理和染色T淋巴细胞对趋化因子受体表达的不同协议的影响。我们的结果证实,采用标准方法(例如Ficoll密度分离)后,某些趋化因子受体的FACS分析受到损害。尽管最佳方法通常是在裂解全血之前对细胞进行染色,但在许多实验条件下可能并不可行。通常,我们发现Ficoll分离后在37℃对细胞染色产生了极好的结果。但是,使用的精确方法将取决于要测量的受体。我们使用了最佳方法,使用8色流式细胞术比较了天然和记忆T细胞亚群上趋化因子受体的表达。

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