一种用于定量骨骼肌脂肪浸润的新方法。
A novel method for the quantification of fatty infiltration in skeletal muscle.
作者信息
Biltz Nicole K, Meyer Gretchen A
机构信息
Program in Physical Therapy, Washington University in St. Louis, 4444 Forest Park Blvd, St. Louis, 63108, MO, USA.
Departments of Neurology, Biomedical Engineering and Orthopaedic Surgery, Washington University, St. Louis, MO, USA.
出版信息
Skelet Muscle. 2017 Jan 10;7(1):1. doi: 10.1186/s13395-016-0118-2.
BACKGROUND
Fatty infiltration of the skeletal muscle is a common but poorly understood feature of many myopathies. It is best described in human muscle, where non-invasive imaging techniques and representative histology have been optimized to view and quantify infiltrating fat. However, human studies are limited in their ability to identify cellular and molecular mechanisms regulating fatty infiltration, a likely prerequisite to developing targeted interventions. As mechanistic investigations move to small animals, studies may benefit from new or adapted imaging tools optimized for high resolution and whole muscle quantification.
RESULTS
Here, we describe a novel method to evaluate fatty infiltration, developed for use with mouse muscle. In this methodology, muscle cellular membranes and proteins are removed via decellularization, but fatty infiltrate lipid is spared, trapped in its native distribution in a transparent extracellular matrix construct. This lipid can then be stained with visible or fluorescent dyes and imaged. We present three methods to stain and evaluate lipid in decellularized muscles which can be used individually or combined: (1) qualitative visualization of the amount and 3D spatial distribution of fatty infiltration using visible lipid soluble dye Oil Red O (ORO), (2) quantitative analysis of individual lipid droplet metrics (e.g., volume) via confocal imaging of fluorescent lipid soluble dye boron-dipyrromethene (BODIPY), and (3) quantitative analysis of total lipid content by optical density reading of extracted stained lipid. This methodology was validated by comparing glycerol-induced fatty infiltration between two commonly used mouse strains: 129S1/SvlmJ (129S1) and C57BL/6J (BL/6J). All three methods were able to detect a significant increase in fatty infiltrate volume in the 129S1 muscle compared with that in BL/6J, and methods 1 and 2 additionally described a difference in the distribution of fatty infiltrate, indicating susceptibility to glycerol-induced fatty infiltration is strain-specific.
CONCLUSIONS
With more mechanistic studies of fatty infiltration moving to small animal models, having an alternative to expensive non-invasive imaging techniques and selective representative histology will be beneficial. In this work, we present a method that can quantify both individual adipocyte lipids and whole muscle total fatty infiltrate lipid.
背景
骨骼肌脂肪浸润是许多肌病常见但了解甚少的一个特征。在人体肌肉中对其描述最为详尽,在人体中,非侵入性成像技术和代表性组织学已得到优化,用于观察和量化浸润脂肪。然而,人体研究在识别调节脂肪浸润的细胞和分子机制方面能力有限,而这可能是开发靶向干预措施的一个必要前提。随着机制研究转向小动物,研究可能会受益于针对高分辨率和全肌肉量化而优化的新的或改良的成像工具。
结果
在此,我们描述了一种用于评估脂肪浸润的新方法,该方法是为小鼠肌肉开发的。在这种方法中,通过去细胞处理去除肌肉细胞膜和蛋白质,但保留脂肪浸润脂质,使其被困在透明细胞外基质构建体中的天然分布位置。然后可以用可见或荧光染料对这种脂质进行染色并成像。我们提出了三种对去细胞化肌肉中的脂质进行染色和评估的方法,这些方法可以单独使用或组合使用:(1)使用可见脂溶性染料油红O(ORO)对脂肪浸润的量和三维空间分布进行定性可视化,(2)通过对荧光脂溶性染料硼二吡咯亚甲基(BODIPY)进行共聚焦成像,对单个脂滴指标(如体积)进行定量分析,(3)通过对提取的染色脂质进行光密度读数,对总脂质含量进行定量分析。通过比较两种常用小鼠品系129S1/SvlmJ(129S1)和C57BL/6J(BL/6J)之间甘油诱导的脂肪浸润,验证了该方法。与BL/6J相比,所有三种方法都能够检测到129S1肌肉中脂肪浸润体积的显著增加,并且方法1和2还描述了脂肪浸润分布的差异,表明对甘油诱导的脂肪浸润的易感性具有品系特异性。
结论
随着越来越多关于脂肪浸润的机制研究转向小动物模型,拥有一种替代昂贵的非侵入性成像技术和选择性代表性组织学的方法将是有益的。在这项工作中,我们提出了一种可以量化单个脂肪细胞脂质和全肌肉总脂肪浸润脂质的方法。
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