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SpiroZin2 优于 FluoZin-3,可用于监测囊泡 Zn,从而跟踪溶酶体 Zn 池。

Superiority of SpiroZin2 Versus FluoZin-3 for monitoring vesicular Zn allows tracking of lysosomal Zn pools.

机构信息

Department of Biochemistry and BioFrontiers Institute, University of Colorado, Boulder, CO, 80303, USA.

Department of Chemistry, Massachusetts Institute of Technology, Cambridge, MA, 02139-4307, USA.

出版信息

Sci Rep. 2018 Oct 9;8(1):15034. doi: 10.1038/s41598-018-33102-w.

Abstract

Small-molecule fluorescent probes are powerful and ubiquitous tools for measuring the concentration and distribution of analytes in living cells. However, accurate characterization of these analytes requires rigorous evaluation of cell-to-cell heterogeneity in fluorescence intensities and intracellular distribution of probes. In this study, we perform a parallel and systematic comparison of two small-molecule fluorescent vesicular Zn probes, FluoZin-3 AM and SpiroZin2, to evaluate each probe for measurement of vesicular Zn pools. Our results reveal that SpiroZin2 is a specific lysosomal vesicular Zn probe and affords uniform measurement of resting Zn levels at the single cell level with proper calibration. In contrast, FluoZin-3 AM produces highly variable fluorescence intensities and non-specifically localizes in the cytosol and multiple vesicular compartments. We further applied SpiroZin2 to lactating mouse mammary epithelial cells and detected a transient increase of lysosomal free Zn at 24-hour after lactation hormone treatment, which implies that lysosomes play a role in the regulation of Zn homeostasis during lactation. This study demonstrates the need for critical characterization of small-molecule fluorescent probes to define the concentration and localization of analytes in different cell populations, and reveals SpiroZin2 to be capable of reporting diverse perturbations to lysosomal Zn.

摘要

小分子荧光探针是测量活细胞中分析物浓度和分布的强大且普遍的工具。然而,要准确描述这些分析物,需要严格评估荧光强度的细胞间异质性和探针在细胞内的分布。在这项研究中,我们对两种小分子荧光囊泡锌探针(FluoZin-3 AM 和 SpiroZin2)进行了平行和系统的比较,以评估每种探针在测量囊泡锌库方面的性能。我们的结果表明,SpiroZin2 是一种特异性溶酶体囊泡锌探针,可通过适当的校准在单细胞水平上均匀测量静止锌水平。相比之下,FluoZin-3 AM 产生高度可变的荧光强度,并非特异性地定位于细胞质和多个囊泡区室。我们进一步将 SpiroZin2 应用于哺乳期小鼠乳腺上皮细胞,并在催乳激素处理 24 小时后检测到溶酶体游离锌的短暂增加,这表明溶酶体在哺乳期锌稳态调节中发挥作用。本研究表明,需要对小分子荧光探针进行严格的特征描述,以确定不同细胞群体中分析物的浓度和定位,并揭示 SpiroZin2 能够报告溶酶体锌的各种扰动。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f04e/6177427/d1fe4727e6fa/41598_2018_33102_Fig1_HTML.jpg

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