Whole Blood Aggregometry in Mice

Siobhan Branfield, Yashieta Somani, A. Valance Washington, Barbara Manfredi
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Abstract

Aggregometry plays a crucial role in both clinical diagnostics and research within hematology, serving as a fundamental tool for understanding platelet function and its implications in physiological and pathological processes. In research, aggregometry provides insights into platelet aggregation dynamics and aids in understanding the underlying mechanisms of hemostasis, thrombosis, and related disorders. Light transmission aggregometry (LTA) and lumi-aggregometry, as well as whole blood aggregometry, are commonly employed methods. While LTA and lumi-aggregometry allow for specific platelet function assessment under controlled conditions, whole blood aggregometry provides a more physiologically relevant approach by evaluating platelet aggregation within the context of whole blood.

Although both methodologies offer unique advantages, whole blood aggregometry allows for preservation of the native cellular environment, simplicity, and potential for better clinical correlation. In a clinical setting, with human blood samples, protocols are established for both LTA and whole blood aggregometry as they are frequently used diagnostic tools. A protocol for LTA and lumi-aggregometry in murine models has been described; however, to date, there is no standardized protocol for whole blood aggregometry in murine models accessible to hematology researchers. This article aims to outline a simple, basic protocol for murine whole blood aggregometry, offering an alternative method to the commonly used LTA aggregometry in research settings. Standardizing whole blood aggregometry protocols in murine models could enhance experimental reliability and facilitate translational research efforts in hematology. © 2024 Wiley Periodicals LLC.

Basic Protocol 1: Whole blood aggregometry in mice

Support Protocol: Phenylhydrazine-induced anemia in wild-type mice

Basic Protocol 2: Hematocrit percentage in mice

小鼠全血聚集测定法
聚集测定法在血液学的临床诊断和研究中发挥着至关重要的作用,是了解血小板功能及其在生理和病理过程中的影响的基本工具。在研究中,聚集测定法可深入了解血小板聚集动力学,有助于理解止血、血栓形成和相关疾病的内在机制。透光聚集测定法(LTA)和发光聚集测定法以及全血聚集测定法是常用的方法。透光聚集测定法和荧光聚集测定法可在受控条件下进行特定的血小板功能评估,而全血聚集测定法通过评估全血中的血小板聚集情况提供了一种更贴近生理的方法。虽然这两种方法都具有独特的优势,但全血聚集测定法可保留原生细胞环境,操作简单,并具有更好的临床相关性。在临床环境中,由于 LTA 和全血聚集测定法都是常用的诊断工具,因此在采集人体血液样本时都会制定相应的方案。已经介绍了在小鼠模型中进行 LTA 和 Lumi-aggregometry 测量的方案;但迄今为止,血液学研究人员还没有在小鼠模型中进行全血聚集测量的标准化方案。本文旨在概述小鼠全血聚集测定的简单基本方案,为研究环境中常用的 LTA 聚集测定提供一种替代方法。小鼠模型全血聚集测定法的标准化可提高实验的可靠性,促进血液学领域的转化研究工作。© 2024 Wiley Periodicals LLC.基本方案 1:小鼠全血聚集测定法辅助方案:苯肼诱导的野生型小鼠贫血 基本方案 2:小鼠血细胞比容百分比。
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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