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通过改进的荧光溶致变色芘探针对细胞和胚胎进行极性测绘。

Polarity Mapping of Cells and Embryos by Improved Fluorescent Solvatochromic Pyrene Probe.

机构信息

Laboratoire de Bioimagerie et Pathologies, UMR 7021 CNRS, Université de Strasbourg, 74 route du Rhin, 67401, Illkirch, France.

Research and Education Faculty, Multidisciplinary Science Cluster, Interdisciplinary Science Unit, Kochi University, 2-5-1, Akebono-cho, Kochi-shi, Kochi, 780-8520, Japan.

出版信息

Anal Chem. 2020 May 5;92(9):6512-6520. doi: 10.1021/acs.analchem.0c00023. Epub 2020 Mar 19.

Abstract

Solvatochromic dyes enable sensing and imaging of biomolecular organization in living systems by monitoring local polarity (lipophilicity), but most such dyes suffer from limited brightness, photostability, lack of a convenient spectral range, and limited sensitivity to polarity. Moreover, the presence of an electron acceptor group, typically a carbonyl, in its push-pull structure raises concerns about its potential chemical reactivity within the biological environment. In order to achieve robust bioimaging, we synthesized a push-pull pyrene probe bearing a ketone acceptor group (PK) and compared it with a recently developed aldehyde analogue (PA). We found that in live cells the aldehyde analogue PA transforms slowly (in ∼100 min) into blue-emissive species, assigned to in situ formation of an imine analogue, whereas the PK probe is stable in the presence of primary amines and inside cells. Like the parent PA, the new probe shows strong solvatochromism and an emission color response to lipid order in membranes (ordered vs disordered liquid phases), while its blue-shifted absorption is more optimal for excitation with 400 nm light sources. In live cells, the PK probe enables high-contrast polarity mapping of organelles using two-color ratiometric detection, suggesting that polarity increases in the following order: lipid droplets < plasma membranes < endoplasmic reticulum. In the zebrafish embryo, polarity imaging with the PK probe reveals a new dimension in visualizing the organization of tissues-lipophilicity distribution, where biomembranes, lipid droplets, cells, yolk, extracellular space, and newly formed organs are revealed by specific emission wavelengths of the probe. The newly developed probe and the proposed approach of polarity mapping open new opportunities for bioimaging at the cellular and animal level.

摘要

变色染料通过监测局部极性(亲脂性)来实现活系统中生物分子组织的传感和成像,但大多数此类染料的亮度、光稳定性有限,缺乏方便的光谱范围,对极性的灵敏度也有限。此外,在其推拉结构中存在电子受体基团(通常为羰基)引起了人们对其在生物环境中潜在化学活性的关注。为了实现稳健的生物成像,我们合成了一种带有酮受体基团(PK)的推拉芘探针,并将其与最近开发的醛类似物(PA)进行了比较。我们发现,在活细胞中,醛类似物 PA 缓慢转化(约 100 分钟)为蓝色发射物质,归因于原位形成亚胺类似物,而 PK 探针在存在伯胺和细胞内时是稳定的。与母体 PA 一样,新探针显示出强烈的溶剂化变色和对膜中脂质有序性(有序相与无序液相)的发射颜色响应,而其蓝移吸收更适合用 400nm 光源激发。在活细胞中,PK 探针可使用双色比率检测对细胞器进行高对比度极性映射,表明极性按以下顺序增加:脂滴<质膜<内质网。在斑马鱼胚胎中,使用 PK 探针进行极性成像揭示了可视化组织亲脂性分布的新维度,其中生物膜、脂滴、细胞、卵黄、细胞外空间和新形成的器官可以通过探针的特定发射波长揭示。新开发的探针和提出的极性映射方法为细胞和动物水平的生物成像开辟了新的机会。

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