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TWISP:一种用于探究信号传播的转基因蠕虫

TWISP: A Transgenic Worm for Interrogating Signal Propagation in .

作者信息

Sharma Anuj Kumar, Randi Francesco, Kumar Sandeep, Dvali Sophie, Leifer Andrew M

机构信息

Department of Physics, Princeton University, Princeton, NJ, 08544.

Princeton Neuroscience Institute, Princeton University, Princeton, NJ, 08544.

出版信息

bioRxiv. 2023 Aug 5:2023.08.03.551820. doi: 10.1101/2023.08.03.551820.

Abstract

Genetically encoded optical indicators and actuators of neural activity allow for all-optical investigations of signaling in the nervous system. But commonly used indicators, actuators and expression strategies are poorly suited for systematic measurements of signal propagation at brain scale and cellular resolution. Large scale measurements of the brain require indicators and actuators with compatible excitation spectra to avoid optical crosstalk. They must be highly expressed in every neuron but at the same time avoid lethality and permit the animal to reach adulthood. And finally, their expression must be compatible with additional fluorescent labels to locate and identify neurons, such as those in the NeuroPAL cell identification system. We present TWISP, a Transgenic Worm for Interrogating Signal Propagation, that address these needs and enables optical measurements of evoked calcium activity at brain scale and cellular resolution in the nervous system of the nematode . We express in every neuron a non-conventional optical actuator, the gustatory receptor homolog GUR-3+PRDX-2 under the control of a drug-inducible system QF+hGR, and calcium indicator GCAMP6s, in a background with additional fluorophores of the NeuroPAL cell ID system. We show that this combination, but not others tested, avoids optical-crosstalk, creates strong expression in the adult, and generates stable transgenic lines for systematic measurements of signal propagation in the worm brain.

摘要

神经活动的基因编码光学指示器和促动器可用于对神经系统信号进行全光学研究。但常用的指示器、促动器和表达策略并不适合在脑尺度和细胞分辨率下对信号传播进行系统测量。对大脑进行大规模测量需要具有兼容激发光谱的指示器和促动器,以避免光学串扰。它们必须在每个神经元中高度表达,但同时要避免致死性并使动物能够成年。最后,它们的表达必须与用于定位和识别神经元的其他荧光标记兼容,例如NeuroPAL细胞识别系统中的那些标记。我们展示了TWISP,一种用于询问信号传播的转基因线虫,它满足了这些需求,并能够对线虫神经系统在脑尺度和细胞分辨率下诱发的钙活性进行光学测量。我们在每个神经元中,在药物诱导系统QF+hGR的控制下表达一种非常规光学促动器,即味觉受体同源物GUR-3+PRDX-2,以及钙指示剂GCAMP6s,背景是NeuroPAL细胞识别系统的其他荧光团。我们表明,这种组合而非其他测试组合,避免了光学串扰,在成虫中产生了强表达,并生成了稳定的转基因系,用于对线虫大脑中的信号传播进行系统测量。

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