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用于量化兽医物种中精子刺激的中性粒细胞中嗜中性粒细胞胞外陷阱形成细胞的核分割组织流式细胞术检测

Tissue Cytometry Assay with Nuclear Segmentation for Quantifying NETotic Cells in Neutrophils Stimulated by Spermatozoa in Veterinary Species.

作者信息

Rivera-Concha Rodrigo, León Marion, Ponce-Rojas Nikol, Prado-Sanhueza Aurora, Uribe Pamela, Taubert Anja, Hermosilla Carlos, Sánchez Raúl, Zambrano Fabiola

机构信息

Center of Excellence in Translational Medicine-Scientific and Technological Bioresource Nucleus (CEMT-BIOREN), Edificio Biociencias de la Salud, Faculty of Medicine, Universidad de La Frontera, Avenida Alemania 0458, Temuco 4810296, Chile.

Medical Sciences Research Laboratory, Ph.D. Program in Medical Sciences, Faculty of Medicine, Universidad de La Frontera, Montevideo 870, Temuco 4811322, Chile.

出版信息

Animals (Basel). 2025 Sep 19;15(18):2742. doi: 10.3390/ani15182742.

Abstract

Upon activation, neutrophils perform three distinct functions: phagocytosis, degranulation of antimicrobial substances into the extracellular medium, and release of neutrophil extracellular traps. Determination of the nuclear area expansion of neutrophils activated to release neutrophil extracellular traps has become critical in demonstrating early neutrophil activation and has become standard. Here, we demonstrate an automated method for measuring nuclear area expansion in two different mammalian species: canine and bovine. For both species, neutrophils were isolated from peripheral blood and co-incubated with fresh spermatozoa for up to 120 min for canine neutrophil-spermatozoa and recently thawed cryopreserved spermatozoa up to 240 min for bovine neutrophil-spermatozoa. Fluorescence images were acquired using a TissueFAXS microscope and then analyzed using StrataQuest v.7.0 software. The images show the release of neutrophil extracellular traps upon activation with spermatozoa for both species, as evidenced by the co-localization of neutrophil elastase and DNA staining. Neutrophil nuclei were expanded as early as 15 min and were detected at up to 120 min in both species. Analysis by nuclei segmentation showed that the data sets generated for both species were reliable and consistent with previously published methods. The method was developed as an automated alternative for measuring the area expansion of neutrophil nuclei in different species.

摘要

激活后,中性粒细胞执行三种不同的功能:吞噬作用、将抗菌物质脱颗粒到细胞外介质中以及释放中性粒细胞胞外陷阱。测定被激活以释放中性粒细胞胞外陷阱的中性粒细胞的核面积扩张,已成为证明中性粒细胞早期激活的关键指标,并已成为标准方法。在此,我们展示了一种自动测量两种不同哺乳动物物种(犬和牛)核面积扩张的方法。对于这两个物种,均从外周血中分离出中性粒细胞,并分别与新鲜精子共同孵育长达120分钟(犬中性粒细胞 - 精子)和与最近解冻的冷冻保存精子共同孵育长达240分钟(牛中性粒细胞 - 精子)。使用TissueFAXS显微镜采集荧光图像,然后使用StrataQuest v.7.0软件进行分析。图像显示,两种物种的中性粒细胞在与精子激活后均释放了中性粒细胞胞外陷阱,中性粒细胞弹性蛋白酶和DNA染色的共定位证明了这一点。两种物种的中性粒细胞核早在15分钟时就开始扩张,并且在长达120分钟时均可检测到。通过细胞核分割分析表明,为两种物种生成的数据集是可靠的,并且与先前发表的方法一致。该方法是作为一种自动替代方法开发的,用于测量不同物种中性粒细胞核的面积扩张。

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