大量裂解过程会改变目标细胞群的数量。

IF 2.5 4区 生物学 Q3 BIOCHEMICAL RESEARCH METHODS Cytometry Part A Pub Date : 2024-05-09 DOI:10.1002/cyto.a.24848
Laura G. Rico, Roser Salvia, Michael D. Ward, Jordi Petriz
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引用次数: 0

摘要

要通过流式细胞术(FCM)实现高灵敏度细胞测量(5 个细胞),必须考虑获得细胞的最低数量,而传统的免疫分型方案无法达到这些数量。大量裂解(BL)试验是一种标准化的红细胞裂解方法,可分析高灵敏度可测量残留疾病(MRD)检测所需的数百万个细胞。然而,这种方法与大量细胞丢失有关,而且在使用这种方法时可能会高估或低估罕见细胞。本研究的目的是评估批量裂解方案,并将其与最小样本扰动(MSP)方案进行比较,据报道,后者能更好地保留原生细胞状态,避免因清洗步骤造成大量细胞丢失。为此,我们首先在新鲜外周血中加入稳定表达 EGFP 的 K562 细胞,以已知的 EGFP 阳性细胞占白细胞的百分比生成 MRD 模型。然后用 BL 和 MSP 方案制备样本,并用 FCM 进行分析。在确定和评估的所有 K562 细胞百分比中,与 MSP 样本相比,即使 K562 细胞百分比较低,也能检测到 BL 样本中的 K562 群体显著减少。与 MSP 样本相比,在 BL 样本中也观察到非坏死细胞显著减少。总之,评估 BL 方案对获得最终计数的潜在影响是非常有意义的,尤其是在高估或低估目标细胞的情况下,例如在可测量残留疾病的情况下。由于传统的流式细胞术或最小样本扰动检测无法获得高灵敏度测量所需的最低数量,因此可能需要大力改进批量裂解溶液试剂。
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Bulk lysis procedures alter target cell population counts

To achieve high-sensitivity cell measurements (<1 in 105 cells) by flow cytometry (FCM), the minimum number of acquired cells must be considered and conventional immunophenotyping protocols fall short of these numbers. The bulk lysis (BL) assay is a standardized erythrocyte lysing approach that allows the analysis of the millions of cells required for high-sensitivity measurable residual disease (MRD) detection. However, this approach has been associated with significant cell loss, along with potential over or underestimates of rare cells when using this method. The aim of this study was to evaluate bulk lysis protocols and compare them with minimal sample perturbation (MSP) protocols, which are reported to better preserve the native cellular state and avoid significant cell loss due to washing steps. To achieve this purpose, we first generated an MRD model by spiking fresh peripheral blood with K562 cells, stably expressing EGFP, at known percentages of EGFP positive cells to leukocytes. Samples were then prepared with BL and MSP protocols and analyzed using FCM. For all percentages of K562 cells established and evaluated, a significant decrease of this population was detected in BL samples compared with MSP samples, even at low K562 cell percentages. Significant decreases for non-necrotic cells were also observed in BL samples relative to MSP samples. In conclusion, the evaluation of the potential effects of BL protocols in obtaining the final count is of great interest, especially for over- or under-estimation of target cells, as in the case of measurable residual disease. Since conventional flow cytometry or minimal sample perturbation assays fall short in obtaining the minimum numbers required to reach high sensitivity measurements, significant efforts may be needed to improve bulk lysis solution reagents.

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来源期刊
Cytometry Part A
Cytometry Part A 生物-生化研究方法
CiteScore
8.10
自引率
13.50%
发文量
183
审稿时长
4-8 weeks
期刊介绍: Cytometry Part A, the journal of quantitative single-cell analysis, features original research reports and reviews of innovative scientific studies employing quantitative single-cell measurement, separation, manipulation, and modeling techniques, as well as original articles on mechanisms of molecular and cellular functions obtained by cytometry techniques. The journal welcomes submissions from multiple research fields that fully embrace the study of the cytome: Biomedical Instrumentation Engineering Biophotonics Bioinformatics Cell Biology Computational Biology Data Science Immunology Parasitology Microbiology Neuroscience Cancer Stem Cells Tissue Regeneration.
期刊最新文献
Issue Information - TOC Volume 105A, Number 12, December 2024 Cover Image Autofluorescence lifetime flow cytometry rapidly flows from strength to strength. Flow cytometry-based method to detect and separate Mycoplasma hyorhinis in cell cultures. The consequence of mismatched buffers in purity checks when spectral cell sorting
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