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SYTO 13 是一种荧光染料,可与核酸结合,用于体外系统中微粒的检测。

Use of SYTO 13, a fluorescent dye binding nucleic acids, for the detection of microparticles in in vitro systems.

机构信息

Division of Rheumatology and Immunology, Department of Medicine, Duke University, Durham, North Carolina, USA.

出版信息

Cytometry A. 2010 Mar;77(3):294-301. doi: 10.1002/cyto.a.20833.

Abstract

Microparticles (MPs) are small membrane-bound vesicles that are released from activated or dying cells by a blebbing process. These particles contain nuclear and cytoplasmic components and represent unique biomarkers for disease. The small size of particles, however, limits detection using flow cytometry with either light scatter or staining for surface markers. Because MPs contain DNA and RNA, we have explored the use of SYTO 13, a member of the class of SYTO dyes, for particle detection. SYTO 13 is cell permeable and has a high fluorescent yield when bound to DNA or RNA. In this study, we compared detection of MPs using either light scatter or SYTO 13 staining, testing the hypothesis that, with fluorescence detection with SYTO 13, problems of "noise" with light scatter are reduced and the range of MP sizes detected is increased. In these experiments, particles were obtained from lymphoid cell lines treated in vitro to undergo apoptosis. As these results showed, STYO 13 allowed the detection of 1.5-2.9 times as many particles as did light scatter. The increased sensitivity was observed with three different cell lines and was independent of inducing stimulus. Treatment of fixed and permeabilized MPs with DNase and RNase showed that SYTO 13 binding resulted from interaction with both DNA and RNA. Together, these findings indicate that the nucleic acid content of MPs provides the basis for their detection in in vitro systems and suggests the utility of fluorescent dyes like SYTO 13 for more sensitive quantitative assays.

摘要

微粒(MPs)是通过起泡过程从激活或死亡的细胞中释放出来的小膜结合囊泡。这些颗粒包含核和细胞质成分,是疾病的独特生物标志物。然而,颗粒的小尺寸限制了使用流式细胞术通过光散射或表面标记染色进行检测。由于 MPs 含有 DNA 和 RNA,我们已经探索了使用 SYTO 13(SYTO 染料类的成员)进行颗粒检测。SYTO 13 可穿透细胞,与 DNA 或 RNA 结合时具有高荧光产率。在这项研究中,我们比较了使用光散射或 SYTO 13 染色检测 MPs,检验了这样一个假设,即使用 SYTO 13 进行荧光检测,可以减少光散射的“噪声”问题,并增加检测到的 MPs 尺寸范围。在这些实验中,从体外处理以诱导细胞凋亡的淋巴样细胞系中获得颗粒。结果表明,与光散射相比,SYTO 13 允许检测到 1.5-2.9 倍的颗粒。这种增强的灵敏度在三种不同的细胞系中均观察到,且与诱导刺激无关。用 DNase 和 RNase 处理固定和透化的 MPs 表明,SYTO 13 结合是由于与 DNA 和 RNA 的相互作用。总之,这些发现表明 MPs 的核酸含量为体外系统中它们的检测提供了基础,并表明像 SYTO 13 这样的荧光染料在更灵敏的定量测定中的实用性。

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