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使用无标记非线性显微镜重建早期斑马鱼胚胎的细胞谱系。

Cell lineage reconstruction of early zebrafish embryos using label-free nonlinear microscopy.

机构信息

Laboratory for Optics and Biosciences, Ecole Polytechnique, CNRS, INSERM, Palaiseau, France.

出版信息

Science. 2010 Aug 20;329(5994):967-71. doi: 10.1126/science.1189428.

Abstract

Quantifying cell behaviors in animal early embryogenesis remains a challenging issue requiring in toto imaging and automated image analysis. We designed a framework for imaging and reconstructing unstained whole zebrafish embryos for their first 10 cell division cycles and report measurements along the cell lineage with micrometer spatial resolution and minute temporal accuracy. Point-scanning multiphoton excitation optimized to preferentially probe the innermost regions of the embryo provided intrinsic signals highlighting all mitotic spindles and cell boundaries. Automated image analysis revealed the phenomenology of cell proliferation. Blastomeres continuously drift out of synchrony. After the 32-cell stage, the cell cycle lengthens according to cell radial position, leading to apparent division waves. Progressive amplification of this process is the rule, contrasting with classical descriptions of abrupt changes in the system dynamics.

摘要

量化动物早期胚胎发生过程中的细胞行为仍然是一个具有挑战性的问题,需要进行整体成像和自动化图像分析。我们设计了一种用于对未染色的整条斑马鱼胚胎进行成像和重建的框架,以进行其前 10 次细胞分裂周期,并报告沿细胞谱系进行的具有亚微米空间分辨率和分钟级时间精度的测量。针对胚胎最内部区域进行优化的点扫描多光子激发提供了固有信号,突出显示所有有丝分裂纺锤体和细胞边界。自动化图像分析揭示了细胞增殖的现象学。卵裂球不断失去同步。在 32 细胞阶段之后,细胞周期根据细胞的径向位置延长,导致明显的分裂波。这种过程的逐渐放大是规则,与系统动力学中突然变化的经典描述形成对比。

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