论文标题

OCT4在人类胚胎干细胞中的表达:时空动力学和命运转变

OCT4 expression in human embryonic stem cells: spatio-temporal dynamics and fate transitions

论文作者

Wadkin, Laura E, Orozco-Fuentes, Sirio, Neganova, Irina, Lako, Majlinda, Barrio, R A, Baggaley, A W, Parker, Nicholas G, Shukurov, Anvar

论文摘要

人类胚胎干细胞(HESC)多能性和分化轨迹的体外调节需要改善其有前途的临床应用。控制多能性的分子相互作用的时间和空间定量对于成功的数学和计算模型的发展也是必要的。在这里,我们使用OCT4-MCHERRY荧光强度的延时实验数据来量化在存在和不存在BMP4的情况下,在不断增长的hESC菌落中,多能转录因子OCT4的时间和空间动力学量化。我们使用Hurst指数和自相关分析表征OCT4的内部自我调节,量化细胞内波动,并考虑单个细胞和后代对的Oct4进化的扩散性。我们发现,子细胞中的Oct4丰度在细微的范围内波动,显示出抗稳定的自我调节。我们获得了不同细胞态之间管理hESC跃迁的固定概率分布,并确定了菌落中pro污染细胞(后来引起多能或分化细胞)簇的时间。通过量化邻近细胞之间的OCT4表达之间的相似性,我们表明hESC在实验的前两天和BMP4处理前的前两天表达了与其本地邻居内部细胞相似的OCT4。我们的框架使我们能够量化增殖的hESC菌落的相关特性,并且该过程广泛适用于其他转录因子和细胞种群。

The improved in-vitro regulation of human embryonic stem cell (hESC) pluripotency and differentiation trajectories is required for their promising clinical applications. The temporal and spatial quantification of the molecular interactions controlling pluripotency is also necessary for the development of successful mathematical and computational models. Here we use time-lapse experimental data of OCT4-mCherry fluorescence intensity to quantify the temporal and spatial dynamics of the pluripotency transcription factor OCT4 in a growing hESC colony in the presence and absence of BMP4. We characterise the internal self-regulation of OCT4 using the Hurst exponent and autocorrelation analysis, quantify the intra-cellular fluctuations and consider the diffusive nature of OCT4 evolution for individual cells and pairs of their descendants. We find that OCT4 abundance in the daughter cells fluctuates sub-diffusively, showing anti-persistent self-regulation. We obtain the stationary probability distributions governing hESC transitions amongst the different cell states and establish the times at which pro-fate cells (which later give rise to pluripotent or differentiated cells) cluster in the colony. By quantifying the similarities between the OCT4 expression amongst neighbouring cells, we show that hESCs express similar OCT4 to cells within their local neighbourhood within the first two days of the experiment and before BMP4 treatment. Our framework allows us to quantify the relevant properties of proliferating hESC colonies and the procedure is widely applicable to other transcription factors and cell populations.

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