Shireman P K, Hampton B, Burgess W H, Greisler H P
Division of Peripheral Vascular Surgery, Department of Surgery, Loyola University Medical Center, Maywood, Ill. 60153-3304, USA.
J Vasc Surg. 1999 May;29(5):852-61; discussion 862. doi: 10.1016/s0741-5214(99)70213-2.
Fibrin glue (FG) has been used as a delivery system for bioactive agents on grafts and angioplasty sites. Reports from two different institutions suggest that heparin concentrations of 500 U/mL in FG inhibit smooth muscle cell (SMC) proliferation, but do not effect endothelial cell (EC) proliferation. The purposes of this study were to (1) quantify the diffusive release of fibroblast growth factor-1 (FGF-1) and heparin from FG; (2) determine the effect of heparin and FGF-1 on SMC proliferation when the cells are immediately plated on the FG; and (3) by means of the diffusive release data, design a new in vitro model that may differentiate the effect of FG-incorporated FGF-1 and heparin, rather than the released, solubilized components of these two factors, on SMC and EC proliferation.
125I-FGF-1 or 3H-heparin release from FG into the overlying media was measured serially in a 96-hour period, either with or without cells. SMCs were immediately plated on FG containing various concentrations of FGF-1 and heparin. SMCs or ECs were plated on identical groups of FG containing FGF-1 and heparin 24 hours after the FG was made to exclude the effect on cell growth of the initial release of FGF-1 into the media.
In the first 24 hours, 70% +/- 1% of the FGF-1 and 59% +/- 2% of the heparin in the FG was released into the overlying media, with minimal release occurring thereafter. The cell type or absence of cells did not affect release, but there was five times more FGF-1 and four times more heparin in the media at 72 hours for the immediate plating versus the delayed plating because of a diffusive release primarily in the first 24 hours. A heparin concentration of 500 U/mL inhibited SMC proliferation, as compared with 5 U/mL heparin, only when immediate plating of SMCs was used. Comparing immediate versus delayed SMC plating, at equivalent FGF-1 and heparin doses, immediate plating induced greater proliferation than delayed plating; this was likely caused by the higher soluble FGF-1 concentration. Heparin doses as high as 500 U/mL had little effect on SMC proliferation. In contrast, ECs died with delayed plating on FG containing 500 U/mL heparin, and their growth was inhibited at 50 U/mL heparin, as compared with 5 U/mL heparin.
The differences in SMC proliferation when comparing immediate versus delayed plating are likely caused by diffusive release of heparin and FGF-1 into the media. Our ongoing work uses an optimized in vitro FG system that minimizes the effects of soluble factors. This is an important distinction, because the cytokines that are released in vivo will be removed by blood flow and, thus, may not exert an effect unless they are contained within the FG.
纤维蛋白胶(FG)已被用作生物活性剂在移植物和血管成形术部位的递送系统。来自两个不同机构的报告表明,FG中500 U/mL的肝素浓度可抑制平滑肌细胞(SMC)增殖,但不影响内皮细胞(EC)增殖。本研究的目的是:(1)量化FG中碱性成纤维细胞生长因子-1(FGF-1)和肝素的扩散释放;(2)确定当细胞立即接种在FG上时肝素和FGF-1对SMC增殖的影响;(3)根据扩散释放数据,设计一种新的体外模型,该模型可以区分FG中掺入的FGF-1和肝素,而不是这两种因子释放的、可溶解的成分,对SMC和EC增殖的影响。
在96小时内连续测量125I-FGF-1或3H-肝素从FG释放到上层培养基中的情况,有无细胞均可。将SMC立即接种在含有不同浓度FGF- 和肝素的FG上。在FG制备24小时后,将SMC或EC接种在含有FGF-1和肝素的相同FG组上,以排除FGF-1最初释放到培养基中对细胞生长的影响。
在最初的24小时内,FG中70%±1%的FGF-1和59%±2%的肝素释放到上层培养基中,此后释放量极小。细胞类型或有无细胞均不影响释放,但由于主要在最初24小时的扩散释放,立即接种组在72小时时培养基中的FGF-1是延迟接种组的5倍,肝素是4倍。与5 U/mL肝素相比,仅当立即接种SMC时,500 U/mL的肝素浓度可抑制SMC增殖。在相同的FGF-1和肝素剂量下,比较立即接种与延迟接种SMC,立即接种比延迟接种诱导的增殖更大;这可能是由于可溶性FGF-1浓度较高。高达500 U/mL的肝素剂量对SMC增殖影响很小。相比之下,在含有500 U/mL肝素的FG上延迟接种时EC死亡,与5 U/mL肝素相比,50 U/mL肝素可抑制其生长。
比较立即接种与延迟接种时SMC增殖的差异可能是由于肝素和FGF-1扩散释放到培养基中。我们正在进行的工作使用了一种优化的体外FG系统,该系统可将可溶性因子的影响降至最低。这是一个重要的区别,因为体内释放的细胞因子将被血流清除,因此,除非它们包含在FG中,否则可能不会发挥作用。
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