首页> 美国卫生研究院文献>Bosnian Journal of Basic Medical Sciences >The effects of platelet gel on cultured human retinal pigment epithelial (hRPE) cells
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The effects of platelet gel on cultured human retinal pigment epithelial (hRPE) cells

机译:血小板凝胶对培养的人视网膜色素上皮细胞(hRPE)的影响

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摘要

The positive role of platelet gel (PG) in tissue regeneration is well known, however, other characteristics of PG still remain to be determined. We investigated cellular and molecular changes in cultured human retinal pigment epithelial (hRPE) cells when treated with different concentrations of PG named PG1, PG2, and PG3. hRPE cells were isolated from donor eyes of two newborn children, within 24 hours after their death. The cells were treated with three concentrations of PG for 7 days: 3 × 104/ml (PG1), 6 × 104/ml (PG2), and 9 × 104/ml (PG3). Fetal bovine serum was used as a control. Immunocytochemistry was performed with anti-RPE65 (H-85), anti-Cytokeratin 8/18 (NCL-5D3), and anti-PAX6 antibody. We used MTT assay to determine cell viability. Gene expressions of PAX6, MMP2, RPE65, ACTA2, MKI67, MMP9, and KDR were analyzed using real-time PCR. A significant increase in viability was observed for PG3-treated cells compared to control (P = 0.044) and compared to PG1 group (P = 0.027), on day 7. Cellular elongation together with dendritiform extensions were observed in PG-treated cells on days 1 and 3, while epithelioid morphology was observed on day 7. All cells were immunoreactive for RPE65, cytokeratin 8/18, and PAX6. No significant change was observed in the expression of MKI67 and PAX6, but the expressions of MMP2, MMP9, ACTA2, and KDR were significantly higher in PG2-treated cells compared to controls (P < 0.05). Our results indicate that increased concentration of PG and extended exposure time have positive effects on viability of hRPE cells. PG may be useful for hRPE cell encapsulation in retinal cell replacement therapy.
机译:血小板凝胶(PG)在组织再生中的积极作用是众所周知的,但是,PG的其他特征仍有待确定。我们研究了用不同浓度的PG(分别称为PG1,PG2和PG3)处理后培养的人类视网膜色素上皮细胞(hRPE)中的细胞和分子变化。 hRPE细胞在两个婴儿死亡后的24小时内从他们的供体眼中分离出来。用三种浓度的PG处理细胞7天:3×10 4 / ml(PG1),6×10 4 / ml(PG2)和9× 10 4 / ml(PG3)。胎牛血清用作对照。用抗RPE65(H-85),抗细胞角蛋白8/18(NCL-5D3)和抗PAX6抗体进行免疫细胞化学。我们使用MTT测定法来确定细胞活力。使用实时PCR分析PAX6,MMP2,RPE65,ACTA2,MKI67,MMP9和KDR的基因表达。在第7天,与对照组相比(P = 0.044)和与PG1组(P = 0.027)相比,经PG3处理的细胞观察到活力显着提高。如图1和3所示,而在第7天观察到上皮样形态。所有细胞对RPE65,细胞角蛋白8/18和PAX6具有免疫反应性。与对照组相比,PG2处理的细胞中MKI67和PAX6的表达未见明显变化,但MMP2,MMP9,ACTA2和KDR的表达明显更高(P <0.05)。我们的结果表明增加的PG浓度和延长的暴露时间对hRPE细胞的活力有积极的影响。 PG对于视网膜细胞替代疗法中的hRPE细胞封装可能有用。

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