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Depleting extracellular vesicles from fetal bovine serum alters proliferation and differentiation of skeletal muscle cells in vitro

机译:从胎牛血清中耗尽细胞外囊泡可在体外改变骨骼肌细胞的增殖和分化

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摘要

Background: Fetal bovine serum (FBS) contains a wide range of growth factors, hormones, vitamins, amino acids, fatty acids and trace elements required for cell growth. It was shown that animal sera contain also extracellular vesicles (EVs) with important biological properties; thus we wondered whether EVs present in FBS would influence muscle cell phenotype. EVs were removed from sera by ultracentrifugation (18 h). C2C12, L6 and human primary myoblasts, were grown either in classical media (CM) or in EVs-depleted media. Differentiation was induced by replacing the culture medium either with CM or EV-depleted media. qRT-PCR of relevant genes and miRNA involved in proliferation, differentiation, energy metabolism and EVs formation and secretion were performed. Results: Growth of myoblasts in EV-free media during proliferation produces the most unfavorable situation for proper myotube formation, when considering C212 and human myoblasts. Removing EVs from serum committed myoblasts to differentiate precociously (induction of myogenin and decreased expression of myomiR involved in myogenesis). C2C12 and human myoblasts, grown constantly in EV-depleted media during proliferation and differentiation, formed less myotubes than in CM. They had a reduced level of myogenin and a strong increase in myostatin expression, a negative regulator of muscle cell differentiation that affects myotube size. This situation was not reversed when confluent myoblasts were switched to CM for differentiation. Like C2C12 and human cells, L6 formed less myotubes in EVs-depleted media. However, as they do not express myostatin, L6 myotubes were larger and expressed higher level of CKTM2 compared to myotubes grown in CM suggesting that they had reached a higher level of differentiation. Conclusions: Researchers studying the role of muscle EVs in culture conditions should consider that depleting EVs from serum alters the phenotype of muscle cells. Interestingly, the cross-talk between myoblasts and myotubes during myogenesis (Forterre 2014, PLoS One. 2014 Jan 2;9(1):e84153) can be recapitulate by using FBS-EVs as well. This implies that EVs can transfer specific signals to cells from unrelated species and that part of serum EV composition is evolutionarily conserved (e.g.; myomiR are detected in FBS-EVs). EVs in body fluids could have an unsuspected function during embryogenesis and in regulation of cellular processes such as hypertrophy and hyperplasia.
机译:背景:胎牛血清(FBS)包含多种生长因子,激素,维生素,氨基酸,脂肪酸和细胞生长所需的微量元素。研究表明,动物血清中还含有具有重要生物学特性的细胞外囊泡(EVs)。因此,我们想知道FBS中存在的EV是否会影响肌肉细胞表型。通过超速离心(18小时)从血清中去除电动汽车。 C2C12,L6和人类原代成肌细胞在经典培养基(CM)或电动车贫乏培养基中生长。通过用CM或EV耗尽培养基替代培养基来诱导分化。进行了涉及增殖,分化,能量代谢以及电动汽车形成和分泌的相关基因和miRNA的qRT-PCR。结果:当考虑C212和人类成肌细胞时,在无EV培养基中成肌细胞在增殖过程中的生长会产生最不利于正确形成肌管的情况。从血清中去除EV可使成肌细胞早熟分化(诱导肌生成素和参与肌发生的myomiR表达降低)。 C2C12和人类成肌细胞在EV耗尽的培养基中不断增殖和分化期间不断生长,形成的肌管比CM少。他们的肌生成素水平降低,而肌生长抑制素表达却大大增加,这是影响肌管大小的肌肉细胞分化的负调节剂。当融合成肌细胞改用CM分化时,这种情况并没有得到扭转。像C2C12和人类细胞一样,L6在贫乏电动汽车的培养基中形成较少的肌管。然而,由于它们不表达肌生长抑制素,因此与在CM中生长的肌管相比,L6肌管更大并且表达的CKTM2水平更高,这表明它们已经达到了更高的分化水平。结论:研究肌肉电动车在培养条件下的作用的研究人员应考虑从血清中耗竭电动车会改变肌肉细胞的表型。有趣的是,成肌细胞和肌管在成肌过程中的串扰(Forterre 2014,PLoS One。2014 Jan 2; 9(1):e84153)也可以通过使用FBS-EV来概括。这意味着EV可以将特定信号从无关物种转移到细胞,并且血清EV成分的一部分在进化上是保守的(例如,在FBS-EV中检测到myomiR)。体液中的电动势在胚胎发生过程中以及在调节细胞肥大和增生等过程中可能具有意想不到的功能。

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