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首页> 外文期刊>Journal of Ophthalmology >ROCK Inhibitor-Induced Promotion of Retinal Pigment Epithelial Cell Motility during Wound Healing
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ROCK Inhibitor-Induced Promotion of Retinal Pigment Epithelial Cell Motility during Wound Healing

机译:岩石抑制剂诱导伤​​口愈合过程中视网膜色素上皮细胞运动的促进

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Purpose. No standard therapy for RPE tear, a complication of neovascular age-related macular degeneration, exists even though RPE tears cause severe vision loss, and promotion of cell proliferation and/or migration could be a candidate RPE tear therapy. The aim of this study is to evaluate the effect of Rho-associated coiled-coil containing kinase (ROCK) inhibitor Y27632 on retinal pigment epithelial (RPE) cell motility during wound healing. Methods. Human RPE cells were cultured in media with and without 10?μM Y27632. A luminescent cell viability assay and vinculin immunocytochemistry were used to test the Y27632 effect on RPE cell adhesion. The mean size of vinculin puncta was quantified from immunofluorescence images. RPE cell motility during wound healing was evaluated using time-lapse imaging and measuring cell migration distances and cell coverage rate in wound fields. Results. The number of adhered RPE and mean size of vinculin puncta were, respectively, 20519 cells and 3.65?μm2 under nontreatment and 23569?cells and 0.66?μm2 under Y27632 treatment. Cell migration distance and cell coverage percentage for untreated and Y27632-treated cells were 98.9 and 59.4% and 203.4 and 92.5%, respectively. Conclusions. Inhibition of ROCK signaling by using 10?μM Y27632 promoted RPE cell motility during wound healing by reducing RPE cell adhesion strength.
机译:目的。对于RPE撕裂没有标准治疗,即使RPE撕裂导致严重的视力丧失,也存在与新血管年龄相关的黄斑变性的并发症存在,并且促进细胞增殖和/或迁移可能是候选RPE撕裂治疗。本研究的目的是评估含有激酶(岩)抑制剂Y27632在伤口愈合期间视网膜色素上皮(RPE)细胞运动中的激酶(岩)抑制剂Y27632的效果。方法。用10?μmy27632在培养基中培养人RPE细胞。发光细胞活力测定和vinculin免疫细胞化学用于测试Y27632对RPE细胞粘附的影响。从免疫荧光图像量化vinculin puncta的平均尺寸。使用延时成像和测量伤口区域中的细胞迁移距离和细胞覆盖率评估伤口愈合过程中的RPE细胞运动。结果。在y27632处理下,分别在20519个细胞和3.65℃下的粘附的RPE和平均尺寸的vinculin puncta和3.65°2μm。未处理和Y27632处理细胞的细胞迁移距离和细胞覆盖率分别为98.9和59.4%和203.4和92.5%。结论。通过降低RPE细胞粘附强度,通过使用10·μmy27632促进摇滚肠动机促进RPE细胞运动的抑制。

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