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Reflective imaging improves spatiotemporal resolution and collection efficiency in light sheet microscopy

机译:反射成像提高了光片显微镜的时空分辨率和采集效率

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摘要

Light-sheet fluorescence microscopy (LSFM) enables high-speed, high-resolution, and gentle imaging of live specimens over extended periods. Here we describe a technique that improves the spatiotemporal resolution and collection efficiency of LSFM without modifying the underlying microscope. By imaging samples on reflective coverslips, we enable simultaneous collection of four complementary views in 250 ms, doubling speed and improving information content relative to symmetric dual-view LSFM. We also report a modified deconvolution algorithm that removes associated epifluorescence contamination and fuses all views for resolution recovery. Furthermore, we enhance spatial resolution (to <300 nm in all three dimensions) by applying our method to single-view LSFM, permitting simultaneous acquisition of two high-resolution views otherwise difficult to obtain due to steric constraints at high numerical aperture. We demonstrate the broad applicability of our method in a variety of samples, studying mitochondrial, membrane, Golgi, and microtubule dynamics in cells and calcium activity in nematode embryos.
机译:光片荧光显微镜(LSFM)可以对活体标本进行长时间的高速,高分辨率和柔和成像。在这里,我们描述了一种无需修改底层显微镜即可提高LSFM的时空分辨率和采集效率的技术。通过在反射性盖玻片上对样本成像,我们可以在250µms内同时收集四个互补视图,相对于对称双视图LSFM,速度提高了一倍,并提高了信息含量。我们还报告了一种改进的去卷积算法,该算法消除了相关的落射荧光污染并融合了所有视图以恢复分辨率。此外,通过将我们的方法应用于单视图LSFM,我们提高了空间分辨率(在所有三个维度上均<300 nm),允许同时获取两个高分辨率视图,否则由于高数值孔径的空间限制而难以获得。我们展示了我们的方法在各种样品中的广泛适用性,研究了线粒体,膜,高尔基体和细胞中微管动力学以及线虫胚胎中的钙活性。

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