基于 33 色抗体面板的飞行时间流式细胞仪和全光谱流式细胞仪的比较评估。

IF 1.6 4区 医学 Q4 BIOCHEMICAL RESEARCH METHODS Journal of immunological methods Pub Date : 2024-02-15 DOI:10.1016/j.jim.2024.113641
Antonia Schäfer , Sènan Mickael D'Almeida , Julien Dorier , Nicolas Guex , Jean Villard , Miguel Garcia
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引用次数: 0

摘要

质谱和全谱流式细胞仪是最近出现的新的有前途的单细胞蛋白质组分析工具,可用于破译免疫细胞的广泛多样性及其在人类疾病中的影响。在这项研究中,我们在四名健康人身上使用相同的 33 色抗体面板,评估了质谱流式细胞仪与全谱流式细胞仪的性能。我们的数据显示,使用半自动聚类方法,两种平台在主要免疫细胞群的量化方面总体上高度一致。在比较手动和自动聚类时,我们还发现聚类分配具有很强的相关性。这两项比较显示,在稀有细胞亚群的量化和分配方面存在微小的分歧。我们的研究表明,两种单细胞蛋白质组学技术都能产生高度重叠的结果,这也证明了技术的选择并不是成功评估细胞特征的主要因素,而必须在临床研究的更广泛设计框架中加以考虑。
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Comparative assessment of cytometry by time-of-flight and full spectral flow cytometry based on a 33-color antibody panel

Mass cytometry and full spectrum flow cytometry have recently emerged as new promising single cell proteomic analysis tools that can be exploited to decipher the extensive diversity of immune cell repertoires and their implication in human diseases. In this study, we evaluated the performance of mass cytometry against full spectrum flow cytometry using an identical 33-color antibody panel on four healthy individuals. Our data revealed an overall high concordance in the quantification of major immune cell populations between the two platforms using a semi-automated clustering approach. We further showed a strong correlation of cluster assignment when comparing manual and automated clustering. Both comparisons revealed minor disagreements in the quantification and assignment of rare cell subpopulations. Our study showed that both single cell proteomic technologies generate highly overlapping results and substantiate that the choice of technology is not a primary factor for successful biological assessment of cell profiles but must be considered in a broader design framework of clinical studies.

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来源期刊
CiteScore
4.10
自引率
0.00%
发文量
120
审稿时长
3 months
期刊介绍: The Journal of Immunological Methods is devoted to covering techniques for: (1) Quantitating and detecting antibodies and/or antigens. (2) Purifying immunoglobulins, lymphokines and other molecules of the immune system. (3) Isolating antigens and other substances important in immunological processes. (4) Labelling antigens and antibodies. (5) Localizing antigens and/or antibodies in tissues and cells. (6) Detecting, and fractionating immunocompetent cells. (7) Assaying for cellular immunity. (8) Documenting cell-cell interactions. (9) Initiating immunity and unresponsiveness. (10) Transplanting tissues. (11) Studying items closely related to immunity such as complement, reticuloendothelial system and others. (12) Molecular techniques for studying immune cells and their receptors. (13) Imaging of the immune system. (14) Methods for production or their fragments in eukaryotic and prokaryotic cells. In addition the journal will publish articles on novel methods for analysing the organization, structure and expression of genes for immunologically important molecules such as immunoglobulins, T cell receptors and accessory molecules involved in antigen recognition, processing and presentation. Submitted full length manuscripts should describe new methods of broad applicability to immunology and not simply the application of an established method to a particular substance - although papers describing such applications may be considered for publication as a short Technical Note. Review articles will also be published by the Journal of Immunological Methods. In general these manuscripts are by solicitation however anyone interested in submitting a review can contact the Reviews Editor and provide an outline of the proposed review.
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