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通过对内源性 AMPA 受体的大规模成像来可视化体内的突触可塑性。

Visualizing synaptic plasticity in vivo by large-scale imaging of endogenous AMPA receptors.

机构信息

Department of Neuroscience, Johns Hopkins University School of Medicine, Baltimore, United States.

Kavli Neuroscience Discovery Institute, Baltimore, United States.

出版信息

Elife. 2021 Oct 18;10:e66809. doi: 10.7554/eLife.66809.

Abstract

Elucidating how synaptic molecules such as AMPA receptors mediate neuronal communication and tracking their dynamic expression during behavior is crucial to understand cognition and disease, but current technological barriers preclude large-scale exploration of molecular dynamics in vivo. We have developed a suite of innovative methodologies that break through these barriers: a new knockin mouse line with fluorescently tagged endogenous AMPA receptors, two-photon imaging of hundreds of thousands of labeled synapses in behaving mice, and computer vision-based automatic synapse detection. Using these tools, we can longitudinally track how the strength of populations of synapses changes during behavior. We used this approach to generate an unprecedentedly detailed spatiotemporal map of synapses undergoing changes in strength following sensory experience. More generally, these tools can be used as an optical probe capable of measuring functional synapse strength across entire brain areas during any behavioral paradigm, describing complex system-wide changes with molecular precision.

摘要

阐明突触分子(如 AMPA 受体)如何介导神经元通讯,并在行为过程中追踪其动态表达,对于理解认知和疾病至关重要,但当前的技术障碍阻碍了对体内分子动力学的大规模探索。我们开发了一系列创新方法,突破了这些障碍:一种带有荧光标记内源性 AMPA 受体的新型基因敲入小鼠品系、在行为小鼠中对数十万个标记突触进行双光子成像,以及基于计算机视觉的自动突触检测。使用这些工具,我们可以纵向跟踪在行为过程中突触群体强度的变化。我们使用这种方法生成了一个前所未有的详细时空图谱,显示了在感觉经验后强度发生变化的突触。更普遍地说,这些工具可用作光学探针,能够在任何行为范式下测量整个大脑区域的功能性突触强度,以分子精度描述复杂的全系统变化。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2902/8616579/0bcf79e3f066/elife-66809-fig1.jpg

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