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High speed functional imaging with source localized multifocal two-photon microscopy

机译:源局部多焦点双光子显微镜的高速功能成像

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摘要

Multifocal two-photon microscopy (MTPM) increases imaging speed over single-focus scanning by parallelizing fluorescence excitation. The imaged fluorescence’s susceptibility to crosstalk, however, severely degrades contrast in scattering tissue. Here we present a source-localized MTPM scheme optimized for high speed functional fluorescence imaging in scattering mammalian brain tissue. A rastered line array of beamlets excites fluorescence imaged with a complementary metal-oxide-semiconductor (CMOS) camera. We mitigate scattering-induced crosstalk by temporally oversampling the rastered image, generating grouped images with structured illumination, and applying Richardson-Lucy deconvolution to reassign scattered photons. Single images are then retrieved with a maximum intensity projection through the deconvolved image groups. This method increased image contrast at depths up to 112 μm in scattering brain tissue and reduced functional crosstalk between pixels during neuronal calcium imaging. Source-localization did not affect signal-to-noise ratio (SNR) in densely labeled tissue under our experimental conditions. SNR decreased at low frame rates in sparsely labeled tissue, with no effect at frame rates above 50 Hz. Our non-descanned source-localized MTPM system enables high SNR, 100 Hz capture of fluorescence transients in scattering brain, increasing the scope of MTPM to faster and smaller functional signals.
机译:多焦点双光子显微镜(MTPM)通过并行化荧光激发提高了单焦点扫描的成像速度。成像的荧光容易受到串扰的影响,但会严重降低散射组织中的对比度。在这里,我们提出了一种针对散布哺乳动物脑组织中的高速功能荧光成像而优化的源本地化MTPM方案。小束的光栅线阵列激发用互补金属氧化物半导体(CMOS)相机成像的荧光。我们通过在时间上对光栅图像进行过采样,生成具有结构化照明的分组图像并应用Richardson-Lucy反卷积来重新分配散射光子,来缓解散射引起的串扰。然后通过反卷积图像组以最大强度投影检索单个图像。这种方法在分散的脑组织中增加了深度达112μm时的图像对比度,并减少了神经元钙成像过程中像素之间的功能串扰。在我们的实验条件下,源定位不会影响密集标记组织中的信噪比(SNR)。在稀疏标记的组织中,低帧速率下SNR降低,而高于50 Hz的帧速率下则没有影响。我们未扫描的源本地化MTPM系统可实现高SNR,100 Hz捕获散射脑中荧光瞬变的捕获,从而将MTPM的范围扩大到更快和更小的功能信号。

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