组成型活性糖原合酶激酶-3β基因转移可维持细胞凋亡,抑制血管平滑肌细胞增殖,并减少大鼠球囊损伤后的新生内膜形成。
Constitutively active glycogen synthase kinase-3beta gene transfer sustains apoptosis, inhibits proliferation of vascular smooth muscle cells, and reduces neointima formation after balloon injury in rats.
作者信息
Park Kyung-Woo, Yang Han-Mo, Youn Seock-Won, Yang Hyun-Ju, Chae In-Ho, Oh Byung-Hee, Lee Myoung-Mook, Park Young-Bae, Choi Yun-Shik, Kim Hyo-Soo, Walsh Kenneth
机构信息
Cardiovascular Laboratory, Clinical Research Institute, Seoul National University Hospital, Korea.
出版信息
Arterioscler Thromb Vasc Biol. 2003 Aug 1;23(8):1364-9. doi: 10.1161/01.ATV.0000081633.53390.B4. Epub 2003 Jun 12.
OBJECTIVE
Glycogen synthase kinase (GSK)-3beta is a crucial factor in many cellular signaling pathways and may play an important role in smooth muscle proliferation and apoptosis after angioplasty.
METHODS AND RESULTS
To investigate the effect of GSK-3beta modulation on neointima formation, smooth muscle proliferation, and apoptosis after balloon injury in vivo, we delivered adenoviral vectors expressing the constitutively active form of GSK-3beta (GSK-S9A: 9th serine switched to alanine) or a control gene into rat carotid arterial segments after balloon injury with a 2F Fogarty catheter. Viral infusion mixtures (5x108 pfu) were incubated in the arterial lumen for 20 minutes, and the effects of gene delivery were evaluated 3 days and 2 weeks after gene delivery with morphometry and immunohistochemical staining for proliferating and apoptotic cells. There were no significant differences in intimal, medial, and lumen areas at 3 days after the procedure. However, 2 weeks after gene delivery, the active GSK-3beta gene transfer resulted in a significantly lower intima to media ratio (0.29+/-0.06 versus 0.86+/-0.09, P<0.01) and a greater lumen area (0.41+/-0.02 versus 0.31+/-0.01 mm2, P<0.01) compared with the control gene transfected group. This was attributable to a significant reduction in intimal area (0.05+/-0.01 versus 0.15+/-0.02 mm2, P<0.01), whereas the medial area was similar (0.17+/-0.01 versus 0.18+/-0.01 mm2, P=0.21). Proliferation index was significantly reduced both at 3 days and 2 weeks in the active GSK-3beta gene transferred group (2.97+/-0.29% versus 5.71+/-0.50%, P<0.01). In addition, apoptotic index, which was not significantly different between the 2 groups at 3 days, was significantly higher in the active GSK-3beta gene transferred group at 2 weeks (3.14+/-0.68% versus 22.7+/-1.63%, n=10, P<0.01, for control versus active GSK-3beta gene transfer).
CONCLUSIONS
In vivo delivery of the active GSK-3beta gene inhibits smooth muscle proliferation, sustains apoptosis, and reduces neointima formation after balloon injury in rats and may be a future therapeutic target to limit neointima hyperplasia after angioplasty.
目的
糖原合酶激酶(GSK)-3β是多种细胞信号通路中的关键因子,可能在血管成形术后平滑肌增殖和凋亡中发挥重要作用。
方法与结果
为研究GSK-3β调节对体内球囊损伤后新生内膜形成、平滑肌增殖和凋亡的影响,我们在大鼠颈动脉段用2F Fogarty导管进行球囊损伤后,将表达GSK-3β组成型活性形式(GSK-S9A:第9位丝氨酸替换为丙氨酸)的腺病毒载体或对照基因导入其中。将病毒输注混合物(5×10⁸ 噬斑形成单位)在动脉腔内孵育20分钟,并在基因导入后3天和2周通过形态计量学以及对增殖和凋亡细胞进行免疫组织化学染色来评估基因递送的效果。术后3天,内膜、中膜和管腔面积无显著差异。然而,基因导入2周后,与对照基因转染组相比,活性GSK-3β基因转移导致内膜与中膜比值显著降低(0.29±0.06对0.86±0.09,P<0.01),管腔面积更大(0.41±0.02对0.31±0.01 mm²,P<0.01)。这归因于内膜面积显著减小(0.05±0.01对0.15±0.02 mm²,P<0.01),而中膜面积相似(0.17±0.01对0.18±0.01 mm²,P = 0.21)。活性GSK-3β基因转移组在3天和2周时增殖指数均显著降低(2.97±0.29%对5.71±0.50%,P<0.01)。此外,凋亡指数在术后3天两组间无显著差异,但在活性GSK-3β基因转移组2周时显著更高(对照与活性GSK-3β基因转移相比,3.14±0.68%对22.7±1.63%,n = 10,P<0.01)。
结论
活性GSK-3β基因的体内递送可抑制大鼠球囊损伤后平滑肌增殖,维持凋亡并减少新生内膜形成,可能成为限制血管成形术后新生内膜增生的未来治疗靶点。
Zotero 插件