Highly spatial–temporal electrochemical profiling of molecules trafficking at a single mitochondrion in one living cell

IF 9.1 1区 综合性期刊 Q1 MULTIDISCIPLINARY SCIENCES Proceedings of the National Academy of Sciences of the United States of America Pub Date : 2025-03-20 DOI:10.1073/pnas.2424591122
Kang Liu, Lina Wu, Yuanyuan Ma, Desheng Chen, Rujia Liu, Xiaobo Zhang, Dechen Jiang, Rongrong Pan
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Abstract

Simultaneous profiling of multiple molecules trafficking at a single organelle and the surrounding cytosol within a living cell is crucial for elucidating their functions, necessitating advanced techniques that provide high spatial–temporal resolution and molecule specificity. In this study, we present an electrochemical nanodevice based on a θ-nanopipette designed to coanalyze calcium ions (Ca 2+ ) and reactive oxygen species (ROS) at a single mitochondrion and its surrounding cytosol, thereby enhancing our understanding of their trafficking within the signaling pathways of cellular autophagy. Two independent nanosensors integrated within the channels of the θ-nanopipette spatially isolate a single target mitochondrion from the cytosol and simultaneously measure the release of Ca 2+ and ROS with high spatial–temporal resolution. Dynamic tracking reveals the direct trafficking of lysosomal Ca 2+ to the mitochondrion rather than to the cytosol, which triggers ROS-induced ROS release within the mitochondria. Furthermore, highly temporal and concurrent observations revealed a second burst of Ca 2+ in both the mitochondrion and the cytosol, which is not consistent with the change in ROS. These dynamic data elucidate the potential role of a beneficial feedback loop between the Ca 2+ signaling pathway and the subsequent generation of mitochondrial ROS in ML-SA-induced autophagy. More importantly, this innovative platform facilitates detailed profiling of the molecular interactions between trafficking molecules within the mitochondria and the adjacent cytosolic environment, which is hardly realized using the current superresolution optical microscopy.
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一个活细胞中单个线粒体分子运输的高度时空电化学分析
同时分析活细胞内单个细胞器和周围细胞质中的多个分子运输对于阐明其功能至关重要,这需要提供高时空分辨率和分子特异性的先进技术。在这项研究中,我们提出了一种基于θ-纳米吸管的电化学纳米装置,旨在共同分析单个线粒体及其周围细胞质中的钙离子(ca2 +)和活性氧(ROS),从而增强我们对它们在细胞自噬信号通路中的运输的理解。两个独立的纳米传感器集成在θ-纳米吸管的通道内,从细胞质中分离出单个目标线粒体,同时以高时空分辨率测量ca2 +和ROS的释放。动态跟踪显示溶酶体ca2 +直接运输到线粒体而不是细胞质,这触发了ROS诱导的线粒体内ROS释放。此外,高时间和并发的观察显示,线粒体和细胞质中ca2 +的第二次爆发,这与ROS的变化不一致。这些动态数据阐明了ca2 +信号通路和随后产生的线粒体ROS之间有益反馈回路在ml - sa诱导的自噬中的潜在作用。更重要的是,这个创新的平台有助于详细分析线粒体内运输分子与邻近细胞质环境之间的分子相互作用,这是目前超分辨率光学显微镜很难实现的。
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来源期刊
CiteScore
19.00
自引率
0.90%
发文量
3575
审稿时长
2.5 months
期刊介绍: The Proceedings of the National Academy of Sciences (PNAS), a peer-reviewed journal of the National Academy of Sciences (NAS), serves as an authoritative source for high-impact, original research across the biological, physical, and social sciences. With a global scope, the journal welcomes submissions from researchers worldwide, making it an inclusive platform for advancing scientific knowledge.
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