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自由活动动物的闭环双光子功能成像。

Closed-loop two-photon functional imaging in a freely moving animal.

作者信息

McNulty Paul, Wu Rui, Yamaguchi Akihiro, Heckscher Ellie S, Haas Andrew, Nwankpa Amajindi, Skanata Mirna Mihovilovic, Gershow And Marc

机构信息

Department of Physics, New York University, New York, NY, USA.

Department of Molecular Genetics and Cell Biology, University of Chicago, Chicago, IL, USA.

出版信息

Nat Commun. 2025 Jul 1;16(1):5950. doi: 10.1038/s41467-025-60648-x.

Abstract

Direct measurement of neural activity in freely moving animals is essential for understanding how the brain controls and represents behaviors. Genetically encoded calcium indicators report neural activity as changes in fluorescence intensity, but brain motion confounds quantitative measurement of fluorescence. Translation, rotation, and deformation of the brain and the movements of intervening scattering or autofluorescent tissue all alter the amount of fluorescent light captured by a microscope. Compared to single-photon approaches, two-photon microscopy is less sensitive to scattering and off-target fluorescence, but more sensitive to motion, and two photon imaging has always required anchoring the microscope to the brain. We developed a closed-loop resonant axial-scanning high-speed two-photon (CRASH2p) microscope for real-time 3D motion correction in unrestrained animals, without implantation of reference markers. We complemented CRASH2p with a 'Pong' scanning strategy and a multi-stage registration pipeline. We performed volumetric ratiometrically corrected functional imaging in the CNS of freely moving Drosophila larvae and discovered previously unknown neural correlates of behavior.

摘要

直接测量自由活动动物的神经活动对于理解大脑如何控制和表现行为至关重要。基因编码钙指示剂将神经活动报告为荧光强度的变化,但大脑运动干扰了荧光的定量测量。大脑的平移、旋转和变形以及中间散射或自发荧光组织的运动都会改变显微镜捕获的荧光量。与单光子方法相比,双光子显微镜对散射和非目标荧光不太敏感,但对运动更敏感,并且双光子成像一直需要将显微镜固定在大脑上。我们开发了一种闭环共振轴向扫描高速双光子(CRASH2p)显微镜,用于在无束缚动物中进行实时3D运动校正,无需植入参考标记。我们用“乒乓”扫描策略和多阶段配准管道对CRASH2p进行了补充。我们在自由活动的果蝇幼虫的中枢神经系统中进行了体积比率校正功能成像,并发现了以前未知的行为神经关联。

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