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Characterization of the Stability and Bio-functionality of Tethered Proteins on Bioengineered Scaffolds

机译:对生物工程支架上系环蛋白的稳定性和生物函数的表征

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Various engineering applications have been utilized to deliver molecules and compounds in both innate and biological settings. In the context of biological applications, the timely delivery of molecules can be critical for cellular and organ function. As such, previous studies have demonstrated the superiority of long-term protein delivery, by way of protein tethering onto bioengineered scaffolds, compared with conventional delivery of soluble protein in vitro and in vivo. Despite such benefits little knowledge exists regarding the stability, release kinetics, longevity, activation of intracellular pathway, and functionality of these proteins over time. By way of example, here we examined the stability, degradation and functionality of a protein, glial-derived neurotrophic factor (GDNF), which is known to influence neuronal survival, differentiation, and neurite morphogenesis. Enzyme-linked immunosorbent assays (ELISA) revealed that GDNF, covalently tethered onto polycaprolactone (PCL) electrospun nanofibrous scaffolds, remained present on the scaffold surface for 120 days, with no evidence of protein leaching or degradation. The tethered GDNF protein remained functional and capable of activating downstream signaling cascades, as revealed by its capacity to phosphorylate intracellular Erk in a neural cell line. Furthermore, immobilization of GDNF protein promoted cell survival and differentiation in culture at both 3 and 7 days, further validating prolonged functionality of the protein, well beyond the minutes to hours timeframe observed for soluble proteins under the same culture conditions. This study provides important evidence of the stability and functionality kinetics of tethered molecules.
机译:已经利用各种工程应用在先天和生物环境中递送分子和化合物。在生物应用的背景下,及时递送分子对于细胞和器官功能至关重要。因此,与在体外和体内的可溶性蛋白质的常规递送相比,以前的研究表明,通过蛋白质束缚在生物工程支架上,证明了长期蛋白质递送的优越性。尽管存在这种益处,但存在关于稳定性,释放动力学,寿命,细胞内途径的激活以及这些蛋白质随时间的效果的知识很少。举例来说,在这里,我们研究了蛋白质胶质源神经营养因子(GDNF)的稳定性,降解和功能,这是已知影响神经元存活,分化和神经突形态发生的。酶联免疫吸附试验(ELISA)显示,与聚己内酯(PCL)电纺纳面纤维支架上的GDNF共价束缚,保持在支架表面上120天,没有蛋白质浸出或降解的证据。束缚的GDNF蛋白仍然是官能的并且能够激活下游信号传导级联,如其在神经细胞系中磷酸化细胞内ERK的能力所揭示的。此外,在3和7天内,将GDNF蛋白的固定促进细胞存活和培养物中的分化,进一步验证蛋白质的延长官能度,远远超过在相同的培养条件下对可溶性蛋白观察到的时间框架。本研究提供了束缚分子稳定性和功能动力学的重要证据。

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