PO-112利用组织工程骨骼肌组织表达肌因子的探索

Exercise Biochemistry Review Pub Date : 2018-10-04 DOI:10.14428/EBR.V1I4.9773

Tomohiro Nakamura, T. Shibahara, A. Takamori, A. Nunomiya, M. Miyata, T. Akimoto, R. Nagatomi, T. Fujisato

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摘要

目的最近有证据表明骨骼肌是一种分泌器官。许多肌因子是骨骼肌分泌的生物活性物质，已在平面肌培养细胞中发现。与平面肌肉培养细胞相比，组织工程肌肉作为一种模拟天然骨骼肌的培养系统是一种很好的模型。然而，组织工程肌肉的组成表达基因和分泌化合物尚未得到充分的分析。本研究的目的是1)阐明组成分泌化合物的动力学，2)探索组织工程肌肉中的组成表达基因。方法将C2C12细胞包埋于胶原凝胶溶液中，置于弹性酶处理的脱细胞猪血管肌腱之间。构建体在生长培养基中培养2天，在分化培养基中培养6天。为了与平面培养细胞进行比较，在与构建物相同的条件下，平面培养C2C12细胞。获得培养基，用MALDI-TOF质谱分析。此外，基于微阵列分析探索组织工程骨骼肌中的组成型上调基因，并通过RT-PCR证实。结果MALDI-TOF质谱分析结果显示，与平面肌肉培养细胞相比，组织工程肌肉的检测峰数量丰富，特别是在低分子量范围内。此外，检测到的峰在这些培养基中有很大的不同，在组织工程肌肉中鉴定出了特定的峰。基于微阵列分析，通过RT-PCR鉴定并证实了组织工程骨骼肌中胆囊收缩素的转录上调。结论与平面培养细胞相比，组织工程肌肉组织分泌了许多化合物，特别是在低分子量范围内。此外，在组织工程骨骼肌中，胆囊收缩素的转录上调。除了平面肌肉培养细胞外，利用组织工程肌肉也有可能获得新的肌肉因子。

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PO-112 The exploration of constitutively expressed myokines utilizing tissue-engineered skeletal muscle

Objective Recent evidence has identified skeletal muscle as a secretory organ. Many myokines, which are bioactive substances secreted from skeletal muscle, have been identified in plane muscle culture cells. Compared to the plane muscle culture cells, the tissue-engineered muscle is an excellent model as culture system mimicked native skeletal muscle. However, constitutively expressed genes and secreted compounds from tissue-engineered muscle have not been analyzed sufficiently. The purposes of this study were 1) to clarify kinetics of constitutively secreted compounds, and 2) to explore constitutively expressed genes in the tissue-engineered muscle. Methods C2C12 cells embedded within collagen gel solution were placed between two tendons made up of elastase-treated acelluar porcine blood vessel. The constructs were cultured in growth media for 2 days and cultured in differentiation media for 6 days. To compare with plane culture cells, C2C12 cells were cultured in plane under the same condition as the construct. The culture media were obtained, and analyzed by MALDI-TOF Mass Spectrometry. Furthermore, constitutively up-regulated genes in tissue-engineered skeletal muscle were explored based on microarray analysis and confirmed by RT-PCR. Results MALDI-TOF Mass Spectrometry revealed that the number of detected peaks in tissue-engineered muscle was abundant compared to that of plane muscle culture cells, especially at range of low molecular weight. Furthermore, the detected peaks were substantially different among these culture media and specific peaks were identified in tissue-engineered muscle. Based on microarray analysis, the transcription of cholecystokinin identified, and confirmed the up-regulation in tissue-engineered skeletal muscle by RT-PCR. Conclusions These results suggested that the tissue-engineered muscle constitutively secreted many compounds compared to plane culture cells, especially at range of low molecular weight. Furthermore, the transcription of cholecystokinin was up-regulated in tissue-engineered skeletal muscle. Besides of the plane muscle culture cells, it is possible to expect to obtain novel myokines utilizing tissue-engineered muscle.

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Exercise Biochemistry Review

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