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本文引用的文献

1
A Versatile Synthetic Extracellular Matrix Mimic via Thiol-Norbornene Photopolymerization.通过巯基-降冰片烯光聚合制备多功能仿生细胞外基质
Adv Mater. 2009 Dec 28;21(48):5005-5010. doi: 10.1002/adma.200901808. Epub 2009 Oct 7.
2
Enhanced proteolytic degradation of molecularly engineered PEG hydrogels in response to MMP-1 and MMP-2.响应 MMP-1 和 MMP-2,分子工程化 PEG 水凝胶的增强蛋白水解降解。
Biomaterials. 2010 Oct;31(30):7836-45. doi: 10.1016/j.biomaterials.2010.06.061. Epub 2010 Jul 27.
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Thiol-ene click chemistry.硫醇-烯点击化学。
Angew Chem Int Ed Engl. 2010 Feb 22;49(9):1540-73. doi: 10.1002/anie.200903924.
4
Regulation of valvular interstitial cell calcification by adhesive peptide sequences.黏附肽序列对瓣膜间质细胞钙化的调节。
J Biomed Mater Res A. 2010 Jun 15;93(4):1620-30. doi: 10.1002/jbm.a.32660.
5
In situ elasticity modulation with dynamic substrates to direct cell phenotype.利用动态基质进行原位弹性调节以指导细胞表型。
Biomaterials. 2010 Jan;31(1):1-8. doi: 10.1016/j.biomaterials.2009.09.025. Epub 2009 Sep 27.
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Characterization of valvular interstitial cell function in three dimensional matrix metalloproteinase degradable PEG hydrogels.三维基质金属蛋白酶可降解聚乙二醇水凝胶中瓣膜间质细胞功能的表征
Biomaterials. 2009 Dec;30(34):6593-603. doi: 10.1016/j.biomaterials.2009.08.031. Epub 2009 Sep 10.
7
Statins block calcific nodule formation of valvular interstitial cells by inhibiting alpha-smooth muscle actin expression.他汀类药物通过抑制α-平滑肌肌动蛋白表达来阻止瓣膜间质细胞的钙化结节形成。
Arterioscler Thromb Vasc Biol. 2009 Nov;29(11):1950-7. doi: 10.1161/ATVBAHA.109.195271. Epub 2009 Aug 13.
8
The effect of collagen I mimetic peptides on mesenchymal stem cell adhesion and differentiation, and on bone formation at hydroxyapatite surfaces.I型胶原模拟肽对间充质干细胞黏附与分化以及对羟基磷灰石表面骨形成的影响。
Biomaterials. 2009 Apr;30(10):1898-909. doi: 10.1016/j.biomaterials.2008.12.053. Epub 2009 Jan 20.
9
Substrate properties influence calcification in valvular interstitial cell culture.基质特性影响瓣膜间质细胞培养中的钙化。
J Heart Valve Dis. 2008 Nov;17(6):689-99.
10
Regulation of valvular interstitial cell calcification by components of the extracellular matrix.细胞外基质成分对瓣膜间质细胞钙化的调节作用。
J Biomed Mater Res A. 2009 Sep 15;90(4):1043-53. doi: 10.1002/jbm.a.32187.

小分子多肽功能化的巯基-烯水凝胶作为培养底物,用于理解瓣膜间质细胞的激活和新组织沉积。

Small peptide functionalized thiol-ene hydrogels as culture substrates for understanding valvular interstitial cell activation and de novo tissue deposition.

机构信息

Department of Chemical and Biological Engineering, University of Colorado, Boulder, CO 80303, USA.

出版信息

Acta Biomater. 2012 Sep;8(9):3201-9. doi: 10.1016/j.actbio.2012.05.009. Epub 2012 May 17.

DOI:10.1016/j.actbio.2012.05.009
PMID:22609448
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3470806/
Abstract

A thiol-ene polymerization platform was used to synthesize peptide functionalized poly(ethylene glycol) hydrogels, which were initially characterized and compared to theoretical predictions of Young's modulus via a theoretical crosslinking density equation presented herein. After thorough characterization, this material system's utility for answering specific biological hypotheses was demonstrated with the culture and observation of aortic valvular interstitial cells (VICs). Specifically, these materials were used to better understand the role of substrate elasticity and biochemical functionality on VIC α-smooth muscle (αSMA) expression and secretory properties (i.e. de novo extracellular matrix (ECM)). The Young's moduli of the hydrogels varied from 28kPa (activating, 90% myofibroblasts) to 4kPa (non-activating, 15% myofibroblast), and the biochemical functionality was tailored by incorporating three small adhesive peptide sequences, RGDS, VGVAPG and P15. To promote VIC adhesion, a basal [RGDS] of 0.8mM was used in all formulations, while the [VGVAPG] or [P15] were varied to be lower than, equal to or higher than 0.8mM. The substrates with 1.2mM VGVAPG and all gels with P15 led to significantly higher αSMA expression for both stiff and soft substrates, as compared to 0.8mM RGDS alone. Importantly, all gel conditions αSMA expression were significantly lower than tissue culture poly(styrene) (TCPS; ∼4- to 10-fold difference). The ECM produced decreased significantly as the total integrin-binding peptide concentration increased, but was significantly higher than that produced on TCPS. This easily tailored material system provides a useful culture platform to improve the fundamental understanding of VIC biology through isolating specific biological cues and observing VIC function.

摘要

采用硫醇-烯聚合平台合成了肽功能化聚乙二醇水凝胶,通过本文提出的理论交联密度方程对其进行了初步表征,并与杨氏模量的理论预测值进行了比较。在彻底表征后,通过培养和观察主动脉瓣膜间质细胞(VICs),展示了该材料系统在回答具体生物学假设方面的实用性。具体来说,这些材料被用于更好地理解基质弹性和生物化学功能对 VICα-平滑肌(αSMA)表达和分泌特性(即新的细胞外基质(ECM))的影响。水凝胶的杨氏模量从 28kPa(激活,90%肌成纤维细胞)到 4kPa(非激活,15%肌成纤维细胞)不等,通过掺入三个小的粘附肽序列 RGDS、VGVAPG 和 P15 来调整生物化学功能。为了促进 VIC 黏附,所有配方均使用基础浓度为 0.8mM 的 [RGDS],而 [VGVAPG] 或 [P15] 的浓度则低于、等于或高于 0.8mM。与单独使用 0.8mM RGDS 相比,含有 1.2mM VGVAPG 的基质和所有含有 P15 的凝胶都导致硬基质和软基质的 αSMA 表达显著增加。重要的是,与组织培养聚苯乙烯(TCPS;4 到 10 倍差异)相比,所有凝胶条件下的 αSMA 表达均显著降低。随着整联蛋白结合肽总浓度的增加,细胞外基质的产生显著减少,但仍明显高于 TCPS 上的细胞外基质的产生。这种易于调整的材料系统提供了一个有用的培养平台,可以通过分离特定的生物学线索并观察 VIC 的功能,从而提高对 VIC 生物学的基本理解。