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An analytical model for elucidating tendon tissue structure and biomechanical function from in vivo cellular confocal microscopy images.

机译:从体内细胞共聚焦显微镜图像阐明肌腱组织结构和生物力学功能的分析模型。

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Fibered confocal laser scanning microscopes have given us the ability to image fluorescently labeled biological structures in vivo and at exceptionally high spatial resolutions. By coupling this powerful imaging modality with classic optical elastography methods, we have developed novel techniques that allow us to assess functional mechanical integrity of soft biological tissues by measuring the movements of cells in response to externally applied mechanical loads. Using these methods we can identify minute structural defects, monitor the progression of certain skeletal tissue disease states, and track subsequent healing following therapeutic intervention in the living animal. Development of these methods using a murine Achilles tendon model has revealed that the hierarchical and composite anatomical structure of the tendon presents various technical challenges that can confound a mechanical analysis of local material properties. Specifically, interfascicle gliding can yield complex cellular motions that must be interpreted within the context of an appropriate anatomical model. In this study, we explore the various classes of cellular images that may result from fibered confocal microscopy of the murine Achilles tendon, and introduce a simple two-fascicle model to interpret the images in terms of mechanical strains within the fascicles, as well as the relative gliding between fascicles.
机译:光纤共聚焦激光扫描显微镜使我们能够在体内以异常高的空间分辨率对荧光标记的生物结构进行成像。通过将这种强大的成像方式与经典的光学弹性成像方法相结合,我们开发了新颖的技术,使我们能够通过测量响应于外部施加的机械负荷的细胞运动来评估软生物组织的功能机械完整性。使用这些方法,我们可以识别出微小的结构缺陷,监视某些骨骼组织疾病状态的进展,并跟踪对动物进行治疗干预后的后续愈合。这些使用小鼠跟腱模型的方法的开发表明,肌腱的分层和复合解剖结构提出了各种技术挑战,这些挑战可能会混淆对局部材料特性的机械分析。具体而言,束间滑动可产生复杂的细胞运动,必须在适当的解剖模型的背景下对其进行解释。在这项研究中,我们探索了小鼠跟腱的纤维共聚焦显微镜可能产生的各种细胞图像,并介绍了一个简单的两束模型来解释图像中束和束中的机械应变。分束之间的相对滑动。

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