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优化一种体外生物测定法以实时监测肌管的生长和形成。

Optimization of an in vitro bioassay to monitor growth and formation of myotubes in real time.

作者信息

Murphy Sylvia M, Kiely Maeve, Jakeman Philip M, Kiely Patrick A, Carson Brian P

机构信息

Food for Health Ireland, University of Limerick, Limerick, Ireland Department of Life Sciences, Materials and Surface Sciences Institute and Stokes Institute, University of Limerick, Limerick, Ireland 4i Centre for Interventions in Infection, Inflammation and Immunity, Graduate Entry Medical School, University of Limerick, Limerick, Ireland Physical Education and Sport Sciences, University of Limerick, Limerick, Ireland.

Food for Health Ireland, University of Limerick, Limerick, Ireland Physical Education and Sport Sciences, University of Limerick, Limerick, Ireland.

出版信息

Biosci Rep. 2016 May 6;36(3). doi: 10.1042/BSR20160036. Print 2016 Jun.

Abstract

The importance of growth and maintenance of skeletal muscle is vital for long term health and quality of life. Appropriate nutrition with specific bioactivities relevant to the functionalities of tissues such as skeletal muscle, can assist in maintaining and promoting adaptive responses to biological and environmental stresses which prevent muscle atrophy and promote hypertrophy. The aim of this investigation was to develop a novel in vitro cell-based electric impedance assay to study myoblast to myotube formation on the real time cell analysis (RTCA) platform (xCELLigence™, ACEA) and to validate the system by testing myotube responses to hypertrophic stimuli. C2C12 myoblasts were proliferated until 70% confluent in Dulbecco's Modified Eagles Medium (DMEM) (10% FBS) and subsequently differentiated to myotubes over 8 days in DMEM [2% horse serum (HS)]. Changes in cell behaviour and adhesion properties were monitored by measuring impedance via interdigitated microelectrodes in the base of E-16 cell culture dishes. To establish the suitability of this assay to monitor nutrient regulation of muscle hypertrophy, leucine, a known potent regulator of MPS was then supplemented to the fully formed myotubes in physiologically relevant conditions-0.20 mM, 0.40 mM, 0.6 mM, 0.8 mM and above 1.0 mM, 1.5 mM, 2.0 mM and impedance subsequently monitored. Parallel experiments highlighting alterations in myotube thickness, muscle protein synthesis (MPS) (mammalian target of rapamycin; mTOR) and differentiation (myogenin) were conducted to support RTCA bioassay findings. This in vitro bioassay can be used to monitor skeletal muscle behaviour and identify nutrient compounds with bioactivities promoting skeletal muscle hypertrophy, reducing muscle atrophy and thus inform the development of novel nutrient formulations for the maintenance of skeletal muscle.

摘要

骨骼肌的生长和维持对长期健康和生活质量至关重要。适当的营养以及与骨骼肌等组织功能相关的特定生物活性物质,有助于维持和促进对生物和环境应激的适应性反应,从而预防肌肉萎缩并促进肌肉肥大。本研究的目的是开发一种基于体外细胞的新型电阻抗测定法,以在实时细胞分析(RTCA)平台(xCELLigence™,ACEA)上研究成肌细胞向肌管的形成,并通过测试肌管对肥大刺激的反应来验证该系统。将C2C12成肌细胞在杜氏改良 Eagle 培养基(DMEM)(10%胎牛血清)中增殖至70%汇合,随后在DMEM[2%马血清(HS)]中分化8天形成肌管。通过测量E-16细胞培养皿底部叉指式微电极的阻抗来监测细胞行为和黏附特性的变化。为了确定该测定法监测肌肉肥大营养调节的适用性,然后在生理相关条件下(0.20 mM、0.40 mM、0.6 mM、0.8 mM以及高于1.0 mM、1.5 mM、2.0 mM)向完全形成的肌管中添加亮氨酸(一种已知的强大的肌肉蛋白质合成调节因子),随后监测阻抗。进行了平行实验,突出显示肌管厚度、肌肉蛋白质合成(MPS)(雷帕霉素哺乳动物靶标;mTOR)和分化(肌细胞生成素)的变化,以支持RTCA生物测定结果。这种体外生物测定法可用于监测骨骼肌行为,并鉴定具有促进骨骼肌肥大、减少肌肉萎缩生物活性的营养化合物,从而为开发用于维持骨骼肌的新型营养配方提供依据。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cc4a/4859084/2c6a2b2e387c/bsr036e330fig1.jpg

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