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Mechanical load induced by glass microspheres releases angiogenic factors from neonatal rat ventricular myocytes cultures and causes arrhythmias

机译:玻璃微球诱导的机械负荷从新生大鼠心室肌细胞培养物中释放血管生成因子并导致心律不齐

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摘要

In the present study, we tested the hypothesis that similar to other mechanical loads, notably cyclic stretch (simulating pre-load), glass microspheres simulating afterload will stimulate the secretion of angiogenic factors. Hence, we employed glass microspheres (average diameter 15.7 μm, average mass 5.2 ng) as a new method for imposing mechanical load on neonatal rat ventricular myocytes (NRVM) in culture. The collagen-coated microspheres were spread over the cultures at an estimated density of 3000 microspheres/mm2, they adhered strongly to the myocytes, and acted as small weights carried by the cells during their contraction. NRVM were exposed to either glass microspheres or to cyclic stretch, and several key angiogenic factors were measured by RT-PCR. The major findings were: (1) In contrast to other mechanical loads, such as cyclic stretch, microspheres (at 24 hrs) did not cause hypertrophy. (2) Further, in contrast to cyclic stretch, glass microspheres did not affect Cx43 expression, or the conduction velocity measured by means of the Micro-Electrode-Array system. (3) At 24 hrs, glass microspheres caused arrhythmias, probably resulting from early afterdepolarizations. (4) Glass microspheres caused the release of angiogenic factors as indicated by an increase in mRNA levels of vascular endothelial growth factor (80%), angiopoietin-2 (60%), transforming growth factor-β (40%) and basic fibroblast growth factor (15%); these effects were comparable to those of cyclic stretch. (5) As compared with control cultures, conditioned media from cultures exposed to microspheres increased endothelial cell migration by 15% (P<0.05) and endothelial cell tube formation by 120% (P<0.05), both common assays for angiogenesis. In conclusion, based on these findings we propose that loading cardiomyocytes with glass microspheres may serve as a new in vitro model for investigating the role of mechanical forces in angiogenesis and arrhythmias.
机译:在本研究中,我们测试了以下假设:类似于其他机械负荷,特别是循环拉伸(模拟预负荷),模拟后负荷的玻璃微球会刺激血管生成因子的分泌。因此,我们采用玻璃微球(平均直径15.7μm,平均质量5.2 ng)作为对培养的新生大鼠心室肌细胞(NRVM)施加机械负荷的新方法。胶原蛋白包被的微球以估计的3000微球/ mm 2 的密度分布在培养物中,它们牢固地粘附在心肌细胞上,并在收缩过程中担负着很小的重量。 NRVM暴露于玻璃微球或循环拉伸,并通过RT-PCR测量了几个关键的血管生成因子。主要发现是:(1)与其他机械负荷(例如循环拉伸)相反,微球(在24小时时)不会引起肥大。 (2)此外,与周期性拉伸相反,玻璃微球不影响Cx43的表达或通过微电极阵列系统测得的传导速度。 (3)在24小时时,玻璃微球会引起心律不齐,可能是由于早期去极化后引起的。 (4)玻璃微球引起血管生成因子的释放,血管内皮生长因子(80%),血管生成素2(60%),转化生长因子-β(40%)和碱性成纤维细胞生长的mRNA水平升高表明因素(15%);这些效果与周期性拉伸的效果相当。 (5)与对照培养物相比,暴露于微球的培养物的条件培养基使内皮细胞迁移增加了15%(P <0.05),并使内皮细胞管形成增加了120%(P <0.05),这都是血管生成的常用方法。总之,基于这些发现,我们建议用玻璃微球装载心肌细胞可以作为研究机械力在血管生成和心律不齐中作用的新的体外模型。

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