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首页> 外文期刊>Scientific reports. >Nanometric axial resolution of fibronectin assembly units achieved with an efficient reconstruction approach for multi-angle-TIRF microscopy
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Nanometric axial resolution of fibronectin assembly units achieved with an efficient reconstruction approach for multi-angle-TIRF microscopy

机译:纤连蛋白组装单元的纳米轴向分辨率通过多角度TIRF显微镜的有效重建方法实现

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摘要

High resolution imaging of molecules at the cell-substrate interface is required for understanding key biological processes. Here we propose a complete pipeline for multi-angle total internal reflection fluorescence microscopy (MA-TIRF) going from instrument design and calibration procedures to numerical reconstruction. Our custom setup is endowed with a homogeneous field illumination and precise excitation beam angle. Given a set of MA-TIRF acquisitions, we deploy an efficient joint deconvolution/reconstruction algorithm based on a variational formulation of the inverse problem. This algorithm offers the possibility of using various regularizations and can run on graphics processing unit (GPU) for rapid reconstruction. Moreover, it can be easily used with other MA-TIRF devices and we provide it as an open-source software. This ensemble has enabled us to visualize and measure with unprecedented nanometric resolution, the depth of molecular components of the fibronectin assembly machinery at the basal surface of endothelial cells.
机译:为了了解关键的生物学过程,需要在细胞-基质界面上对分子进行高分辨率成像。在这里,我们为从仪器设计和校准程序到数值重建的多角度全内反射荧光显微镜(MA-TIRF)提出了一条完整的流程。我们的自定义设置具有均匀的场照明和精确的激发光束角度。给定一组MA-TIRF采集,我们基于反问题的变式展开部署有效的联合反卷积/重构算法。该算法提供了使用各种正则化的可能性,并且可以在图形处理单元(GPU)上运行以进行快速重建。而且,它可以很容易地与其他MA-TIRF设备一起使用,并且我们将其作为开源软件提供。这种集合使我们能够以空前的纳米分辨率可视化和测量内皮细胞基底表面纤连蛋白组装机械分子组分的深度。

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