The study of computation occurring in single neurons and small networks of interconnected neurons is often limited by (1) the number of sites that can be simultaneously probed with electrophysiology tools such as patch pipettes and (2) the recording speed of fluorescence imaging tools such as confocal or multiphoton microscopy. Even in the line scan mode of galvanometer-based scanners, where one scan dimension is sacrificed to gain overall speed, the effective frame rate is limited to less than 1 kHz with no flexibility in site selection. To overcome these limitations and allow the study of many sites throughout the dendritic arbor, we have developed an addressable confocal laser-scanning microscope that permits recording from user-selected sites-of-interest at high frame rates, in addition to conventional full frame imaging.; Our system utilizes acousto-optic deflectors (AODs) in the illumination pathway to allow for rapid user-defined positioning of a focused laser spot. However, since AODs rely on diffraction to steer a laser beam, they cannot effectively descan the fluorescence emission spectrum as done in mirror-based systems which utilize reflection; this prevents the use of a stationary pinhole as a spatial filter. Instead, we implement an addressable spatial filter using a digital micromirror device (DMD) in conjunction with the AODs to achieve confocality. A registration algorithm synchronizes the AODs and DMD such that point illumination and point detection are always colocalized in conjugate image planes.; The current version of the confocal system has a spatial resolution of ∼1 mum. Furthermore, by letting the user tailor which sites are visited, we have shown that recordings can be made at an aggregate frame rate of ∼40 kHz. We have successfully demonstrated that the system is capable of optical sectioning and thus exhibits the main advantage of a confocal microscope for light-scattering biological tissue. This property was used to create three-dimensional reconstructions of fluorescently labeled test specimens. Additionally, we have used the system to record intracellular calcium transients using the fluorescent calcium indicator Oregon Green BAPTA-1. The transients were a result of back-propagating action potentials elicited via 1 nA current injections in cultured hippocampal neurons from wild-type mice.
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机译:对单个神经元和相互连接的神经元的小型网络中发生的计算的研究通常受到以下因素的限制:(1)可以用电生理工具(例如贴片移液器)同时探测的位点数量,以及(2)荧光成像工具(例如,共聚焦或多光子显微镜。即使在基于振镜的扫描仪的线扫描模式下,为了获得整体速度而牺牲了一个扫描尺寸,有效帧频仍被限制为小于1 kHz,并且在站点选择上没有灵活性。为了克服这些限制并允许研究整个树突状乔木中的许多部位,我们开发了一种可寻址的共聚焦激光扫描显微镜,除了常规的全帧成像外,它还可以高帧频从用户选择的感兴趣部位进行记录。;我们的系统在照明路径中利用了声光偏转器(AOD),以实现用户定义的聚焦激光光斑的快速定位。但是,由于AOD依靠衍射来控制激光束,因此它们无法像利用反射的基于镜面的系统那样有效地对荧光发射光谱进行去扫描。这阻止了使用固定的针孔作为空间过滤器。取而代之的是,我们使用数字微镜设备(DMD)结合AOD来实现可寻址的空间滤波器,以实现共谋性。配准算法使AOD和DMD同步,以使点照度和点检测始终位于共轭图像平面中。当前版本的共聚焦系统的空间分辨率约为1微米。此外,通过让用户定制访问哪些站点,我们已经表明可以以约40 kHz的总帧速率进行录制。我们已经成功地证明了该系统能够进行光学切片,因此展现了共聚焦显微镜对生物组织进行光散射的主要优势。此属性用于创建荧光标记测试样本的三维重建。此外,我们已经使用该系统使用荧光钙指示剂Oregon Green BAPTA-1来记录细胞内钙瞬变。瞬态是通过从野生型小鼠培养的海马神经元中以1 nA电流注入引起的反向传播动作电位的结果。
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