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Axial resolution improvement of two-photon microscopy by multi-frame reconstruction and adaptive optics

机译:多框架重建和自适应光学通过轴向分辨率改进双光子显微镜

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摘要

Two-photon microscopy (TPM) has been widely used in biological imaging owing to its intrinsic optical sectioning and deep penetration abilities. However, the conventional TPM suffers from poor axial resolution, which makes it difficult to recognize some three-dimensional fine features. We present multi-frame reconstruction two-photon microscopy (MR-TPM) using a liquid lens as a fast axial scanning engine. A sensorless adaptive optics (AO) approach is adopted to correct the aberrations caused by both the liquid lens and the optical system. By overcoming the effect of optical aberrations, inadequate sampling, and poor focusing capability of a conventional TPM, the axial resolution can be improved by a factor of 3 with a high signal-to-noise ratio. The proposed technology is compatible with the conventional TPM and requires no optical post-processing. We demonstrate the proposed method by imaging fluorescent beads, in vitro imaging of the neural circuit of mouse brain slice, and in vivo time-lapse imaging of the morphological changes of microglial cells in septic mice model. The results suggest that the axon of the neural circuit and the process of microglia along the axial direction, which cannot be resolved using conventional TPM, become distinguishable using the proposed AO MR-TPM.
机译:由于其内在光学切片和深渗透能力,两光高显微镜(TPM)已广泛用于生物成像。然而,传统的TPM具有较差的轴向分辨率,这使得难以识别一些三维细小特征。我们使用液体透镜作为快速轴向扫描发动机呈现多帧重建两光子显微镜(MR-TPM)。采用无传感器自适应光学(AO)方法来校正由液体透镜和光学系统引起的像差。通过克服光学像差,采样不足和传统TPM的聚焦能力差的效果,可以通过高信噪比来提高轴向分辨率。所提出的技术与传统的TPM兼容,不需要光学后处理。通过成像荧光珠,小鼠脑切片的神经回路的体外成像,以及体内延迟成像的荧光珠,体内延迟成像进行了仿制方法。结果表明,使用常规TPM不能解决的神经电路的轴突和沿着轴向的微胶质过程,使用所提出的AO MR-TPM可区分。

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