A broadly applicable method for quantifying cardiomyocyte cell division identifies proliferative events following myocardial infarction.

IF 4.3 Q1 BIOCHEMICAL RESEARCH METHODS

Cell Reports Methods Pub Date : 2024-09-16 Epub Date: 2024-09-09 DOI:10.1016/j.crmeth.2024.100860

Samantha K Swift, Alexandra L Purdy, Tyler Buddell, Jerrell J Lovett, Smrithi V Chanjeevaram, Anooj Arkatkar, Caitlin C O'Meara, Michaela Patterson

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引用次数: 0

Abstract

Cardiomyocyte proliferation is a challenging metric to assess. Current methodologies have limitations in detecting the generation of new cardiomyocytes and technical challenges that reduce widespread applicability. Here, we describe an improved cell suspension and imaging-based methodology that can be broadly employed to assess cardiomyocyte cell division in standard laboratories across a multitude of model organisms and experimental conditions. We highlight additional metrics that can be gathered from the same cell preparations to enable additional relevant analyses to be performed. We incorporate additional antibody stains to address potential technical concerns of miscounting. Finally, we employ this methodology with a dual-thymidine analog-labeling approach to a post-infarction murine model, which allowed us to robustly identify unique cycling events, such as cardiomyocytes undergoing multiple rounds of cell division.

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一种广泛适用的量化心肌细胞分裂的方法可识别心肌梗死后的增殖事件。

心肌细胞增殖是一项具有挑战性的评估指标。目前的方法在检测新心肌细胞的生成方面存在局限性，技术上的挑战也降低了其广泛适用性。在此，我们介绍了一种改进的细胞悬浮和成像方法，该方法可广泛应用于标准实验室评估多种模式生物和实验条件下的心肌细胞分裂。我们强调了可从相同的细胞制备中收集的其他指标，以便进行更多相关分析。我们加入了额外的抗体染色，以解决潜在的计数错误技术问题。最后，我们将这种方法与双胸苷类似物标记法一起用于梗死后的小鼠模型，这使我们能够有力地识别独特的循环事件，如经历多轮细胞分裂的心肌细胞。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Cell Reports Methods Chemistry (General), Biochemistry, Genetics and Molecular Biology (General), Immunology and Microbiology (General)

CiteScore

3.80

自引率

0.00%

发文量

审稿时长

111 days