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Age and topographic variation of insulin-like growth factor-binding protein 2 in the human rpe.

机译:人rpe中胰岛素样生长因子结合蛋白2的年龄和地形变化。

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PURPOSE: Previous studies have shown that insulin-like growth factor-binding protein (IGFBP)-2 is markedly upregulated in senescent RPE cells in vitro, and might therefore be a marker of senescent cells in vivo. This study was conducted to determine whether IGFBP-2 expression in human RPE cells from the macula and periphery varies with age in vivo. METHODS: Paraformaldehyde (4%)-fixed and optimal cutting temperature (OCT) compound-embedded human eyes from 17 patients were cryosectioned and subjected to high-sensitivity digoxigenin (DIG)-labeled cRNA in situ hybridization to determine the expression of IGFBP-2. Complementary immunohistochemistry experiments using a polyclonal anti-IGFBP-2 antibody were performed to confirm IGFBP-2 protein expression. Specimens were examined by light microscopy, and images were captured with a digital camera. The total numbers of RPE cells and IGFBP-2 mRNA expression-positive RPE cells were counted for each section, and the ratio of labeled RPE cells to total RPE cells counted was calculated for both macular and peripheral regions of each donor. RESULTS: IGFBP-2 mRNA expression was detected in the ganglion cell layer, inner and outer nuclear layers, and inner segments of photoreceptor cells in all 17 eyes. In 16 of 17 eyes, IGFBP-2 mRNA expression was detected in the RPE. In 11, the ratio of labeled cells to total RPE cells counted per section in the macula was 1.2 times greater than the ratio in the periphery (P = 0.008). The ratio of labeled RPE cells in the macula decreased with age (P = 0.0064). Immunohistochemistry studies for IGFBP-2 confirmed the expression pattern found by in situ hybridization. CONCLUSIONS: There is a topographical and age-related change in IGFBP-2 expression in RPE cells from human donor eyes. This distribution is likely not to represent senescent RPE cells in vivo.
机译:目的:先前的研究表明,胰岛素样生长因子结合蛋白(IGFBP)-2在体外衰老的RPE细胞中明显上调,因此可能是体内衰老细胞的标志物。进行该研究以确定体内黄斑和外周的人RPE细胞中IGFBP-2表达是否随年龄而变化。方法:对17例患者中固定有低聚甲醛(4%)和最佳切割温度(OCT)复合物的人眼进行冷冻切片,并进行高敏感性地高辛配基(DIG)标记的cRNA原位杂交,以确定IGFBP-2的表达。使用多克隆抗IGFBP-2抗体进行了补充免疫组织化学实验,以确认IGFBP-2蛋白表达。通过光学显微镜检查样品,并用数码相机捕获图像。计算每个切片的RPE细胞和IGFBP-2 mRNA表达阳性RPE细胞的总数,并计算每个供体的黄斑和周边区域标记的RPE细胞与计数的总RPE细胞之比。结果:在全部17只眼的神经节细胞层,内外核层以及感光细胞的内部节段均检测到IGFBP-2 mRNA的表达。在17只眼中的16只眼中,在RPE中检测到了IGFBP-2 mRNA表达。在11中,在黄斑中每部分计数的标记细胞与RPE细胞总数之比是周围比率的1.2倍(P = 0.008)。黄斑中标记的RPE细胞的比例随着年龄的增长而降低(P = 0.0064)。对IGFBP-2的免疫组织化学研究证实了通过原位杂交发现的表达模式。结论:人类供体眼睛的RPE细胞中IGFBP-2表达存在地形变化和与年龄有关的变化。这种分布可能不代表体内衰老的RPE细胞。

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