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Spatial organization of fibroblast nuclear chromocenters: component tree analysis

机译:成纤维细胞核色中心的空间组织:成分树分析

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摘要

The nuclei of mouse connective tissue fibroblasts contain chromocenters which are well-defined zones of heterochromatin that can be used as positional landmarks to examine nuclear remodeling in response to a mechanical perturbation. This study used component tree analysis, an image segmentation algorithm that detects high intensity voxels that are topologically connected, to quantify the spatial organization of chromocenters in fibroblasts within whole mouse connective tissue fixed and stained with 4',6-diamidino-2-phenylindole (DAPI). The component tree analysis method was applied to confocal microscopy images of whole mouse areolar connective tissue incubated for 30 min ex vivo with or without static stretch. In stretched tissue, the mean distance between chromocenters within fibroblast nuclei was significantly greater (vs. non-stretched, P < 0.001), corresponding to an average of a 500-nm increase in chromocenter separation (∼10% strain). There was no significant difference in chromocenter number or average size between stretch and no stretch. Average chromocenter distance was positively correlated with nuclear cross-sectional area (r = 0.78, P < 0.0001), and nuclear volume (r = 0.42, P < 0.0001), and negatively correlated with nuclear aspect ratio (r = −0.65, P < 0.0001) and nuclear concavity index (r = −0.44, P < 0.0001). These results demonstrate that component trees can be successfully applied to the morphometric analysis of nuclear chromocenters in fibroblasts within whole connective tissue. Static stretching of mouse areolar connective tissue for 30 min resulted in substantially increased separation of nuclear chromocenters in connective tissue fibroblasts. This interior remodeling of the nucleus induced by tissue stretch may impact transcriptionally active euchromatin within the inter-chromocenter space.
机译:小鼠结缔组织成纤维细胞的核中含有色中心,它们是异染色质的明确定义区域,可用作位置标记,以检查响应机械扰动的核重塑。这项研究使用成分树分析(一种图像分割算法,可检测拓扑连接的高强度体素)来量化固定并染色了4',6-diamidino-2-phenylindole( DAPI)。将成分树分析方法应用于在有或没有静态拉伸的情况下,离体孵育30分钟的整个小鼠乳晕结缔组织的共聚焦显微镜图像。在拉伸的组织中,成纤维细胞核内色心之间的平均距离明显更大(与未拉伸相比,P <0.001),对应于色心分离平均增加500 nm(约10%应变)。在拉伸和不拉伸之间,色心数目或平均大小没有显着差异。平均色心距离与核截面积(r = 0.78,P <0.0001)和核体积(r = 0.42,P <0.0001)正相关,与核长宽比(r = -0.65,P < 0.0001)和核凹度指数(r = -0.44,P <0.0001)。这些结果表明,成分树可以成功地应用于整个结缔组织内成纤维细胞核色心的形态分析。小鼠乳晕结缔组织的静态拉伸30分钟导致结缔组织成纤维细胞中核色中心的分离大大增加。由组织拉伸引起的细胞核的内部重塑可能影响色中心间空间内的转录活性常染色质。

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