Jabbarzadeh Ehsan, Abrams Cameron F
Department of Chemical Engineering, Drexel University, 3141 Chestnut St., Philadelphia, PA 19104, USA.
Tissue Eng. 2007 Aug;13(8):2073-86. doi: 10.1089/ten.2006.0057.
Control over angiogenesis (formation of new capillaries from preexisting vessels) is often a crucial requirement for implantable porous biomaterials serving as scaffolds for tissue regeneration. Angiogenesis is influenced by the transport of chemoattractants such as vascular endothelial growth factor (VEGF) through the implant. To investigate this influence, we developed a computational model of capillary formation based on endothelial cell migration by modeling the random motion of sprout tips biased along spatially and temporally evolving concentration gradients of VEGF. The model focuses on the effect of diffusive VEGF transport inside a 2D domain on the directed migration of sprouts to test several chemical and physical strategies to stimulate and control angiogenesis. We considered a 2D porous membrane that is located between the primary vessel and a line source of VEGF. We assess the vascular network formed in 2 cases of a high and zero VEGF degradation rates applying 3 strategies of VEGF production: (1) only a line source; (2) a line source plus controlled release from a small number of VEGF sources that are randomly dispersed on the pore boundaries; and (3) a line source plus controlled release of VEGF from the pore boundaries themselves. Results show that in the limiting cases where VEGF degradation rate is relatively high, strategies 2 and 3 lead to a substantial increase in the number of vessels. This increase depends on the relative rates at which the line source and embedded sources or solid boundaries produce VEGF. Using strategy 2 results in a newly formed capillary network that is highly localized around the embedded sources. However, using strategy 3 leads to a more uniformly distributed vessel network and a higher degree of vessel ingrowth inside the porous membrane. In addition, the duration at which we engineer the embedded sources or pore boundaries to release VEGF determines the morphology of the capillary network. Although a higher release duration leads to a dense network of newly formed vessels near the primary vessel, it hinders further vessel penetration inside the porous membrane. Therefore, in applying both strategies 2 and 3, there is an optimum release duration that leads to a deeper penetration of vessels inside the membrane. It is hoped that insights from this study will aid in the design of materials with optimal structural and chemical properties to facilitate controlled angiogenesis.
对于用作组织再生支架的可植入多孔生物材料而言,控制血管生成(从已有血管形成新的毛细血管)通常是一项关键要求。血管生成受趋化因子(如血管内皮生长因子,VEGF)通过植入物的运输影响。为了研究这种影响,我们通过对芽尖的随机运动进行建模,基于内皮细胞迁移建立了一个毛细血管形成的计算模型,该随机运动沿VEGF的时空演化浓度梯度产生偏向。该模型聚焦于二维域内VEGF扩散运输对芽的定向迁移的影响,以测试多种刺激和控制血管生成的化学及物理策略。我们考虑了位于主血管和VEGF线源之间的二维多孔膜。我们应用三种VEGF产生策略评估在VEGF降解率高和为零的两种情况下形成的血管网络:(1)仅一个线源;(2)一个线源加上从随机分散在孔边界上的少量VEGF源进行控释;(3)一个线源加上从孔边界本身进行VEGF控释。结果表明,在VEGF降解率相对较高的极限情况下,策略2和3会使血管数量大幅增加。这种增加取决于线源与嵌入式源或固体边界产生VEGF的相对速率。使用策略2会形成一个高度局限于嵌入式源周围的新毛细血管网络。然而,使用策略3会导致血管网络分布更均匀,且多孔膜内的血管向内生长程度更高。此外,我们设计嵌入式源或孔边界释放VEGF的持续时间决定了毛细血管网络的形态。虽然较长的释放持续时间会在主血管附近形成密集的新血管网络,但它会阻碍血管在多孔膜内的进一步穿透。因此,在应用策略2和3时,存在一个最佳释放持续时间,可使血管更深地穿透到膜内。希望本研究的见解将有助于设计具有最佳结构和化学性质的材料,以促进可控的血管生成。
