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使用基因编码的比率荧光传感器对细胞外三磷酸腺苷进行成像。

Imaging extracellular ATP with a genetically-encoded, ratiometric fluorescent sensor.

作者信息

Conley Jason M, Radhakrishnan Saranya, Valentino Stephen A, Tantama Mathew

机构信息

Department of Chemistry, Purdue University, West Lafayette, Indiana, United States of America.

Purdue Institute for Integrative Neuroscience, Purdue University, West Lafayette, Indiana, United States of America.

出版信息

PLoS One. 2017 Nov 9;12(11):e0187481. doi: 10.1371/journal.pone.0187481. eCollection 2017.

Abstract

Extracellular adenosine triphosphate (ATP) is a key purinergic signal that mediates cell-to-cell communication both within and between organ systems. We address the need for a robust and minimally invasive approach to measuring extracellular ATP by re-engineering the ATeam ATP sensor to be expressed on the cell surface. Using this approach, we image real-time changes in extracellular ATP levels with a sensor that is fully genetically-encoded and does not require an exogenous substrate. In addition, the sensor is ratiometric to allow for reliable quantitation of extracellular ATP fluxes. Using live-cell microscopy, we characterize sensor performance when expressed on cultured Neuro2A cells, and we measure both stimulated release of ATP and its clearance by ectonucleotidases. Thus, this proof-of-principle demonstrates a first-generation sensor to report extracellular ATP dynamics that may be useful for studying purinergic signaling in living specimens.

摘要

细胞外三磷酸腺苷(ATP)是一种关键的嘌呤能信号,介导器官系统内和系统间的细胞间通讯。我们通过对ATeam ATP传感器进行重新设计,使其在细胞表面表达,以满足对一种强大且微创的测量细胞外ATP方法的需求。使用这种方法,我们利用一种完全由基因编码且无需外源底物的传感器,对细胞外ATP水平的实时变化进行成像。此外,该传感器是比率型的,能够可靠地定量细胞外ATP通量。通过活细胞显微镜技术,我们对在培养的Neuro2A细胞上表达时的传感器性能进行了表征,并测量了ATP的刺激释放及其被外核苷酸酶清除的情况。因此,这一原理验证展示了一种用于报告细胞外ATP动态的第一代传感器,可能对研究活体标本中的嘌呤能信号传导有用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d7ab/5679667/a0de750e8907/pone.0187481.g001.jpg

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