皇家外科学院大鼠激光光凝后碱性成纤维细胞生长因子和胶质纤维酸性蛋白的免疫细胞化学定位。

Y Chu, M F Humphrey, V V Alder, I J Constable
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引用次数: 0

摘要

目的:氩气激光光凝减缓皇家外科学院(RCS)大鼠的光受体变性,与玻璃体内注射碱性成纤维细胞生长因子(bFGF)一样。我们假设视网膜bFGF的上调是RCS大鼠激光损伤的结果。因此,我们检测了激光后bFGF的定位,并将其与损伤后增加的梅勒细胞胶质纤维酸性蛋白(GFAP)表达联系起来。方法:将34只RCS大鼠于出生后第23天麻醉(氯胺酮40 mg/kg),用功率为120 mW的50微米光斑照射视网膜0.2 s,形成40个不重叠的氩绿病灶网格。在病变后0、6、12、24、48 h和7、14、21 d,麻醉大鼠,去核并冷冻切片,切片采用标准的亲和素-生物素化过氧化物酶复合物法使用bFGF或GFAP抗体进行处理。5只年龄匹配、无激光损伤的RCS大鼠作为对照。结果:碱性成纤维细胞生长因子免疫反应性(IR)通常位于神经节细胞层、内核层、视网膜色素上皮细胞和外核层细胞外基质/细胞膜中。在激光视网膜中,凝固的外节段在前24小时内bFGF-IR升高。视网膜血管/网膜细胞/星形胶质细胞在病变后立即在每个病变内和附近中度标记,48小时后变得更加强烈,并持续至少21天。第14天病变侧ONL中bFGF-IR升高。Muller细胞gap - ir在病变后6小时首次检测到,并在病变部位外扩散相当远的距离。在第7天和第14天,病变部位的 ller细胞已经发芽,而侧翼的细胞仍然是gmap - ir。结论:激光病变后,仅在病变中心24小时内bFGF水平升高。然而,在14天时,在ONL中观察到bFGF水平升高,并且延伸到病变侧翼的距离与光感受器存活增加的距离相似。这些结果为激光损伤诱导bFGF的假设提供了支持,这可能是光感受器幸免的机制。m ller细胞激活与生长因子刺激一致,但在ONL中比bFGF的变化更为广泛。然而,血管标记同样广泛存在,因此反应可能与激光病变后 ller细胞GFAP反应和血管bFGF定位有关。
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Immunocytochemical localization of basic fibroblast growth factor and glial fibrillary acidic protein after laser photocoagulation in the Royal College of Surgeons rat.

Purpose: Argon laser photocoagulation slows photoreceptor degeneration in the Royal College of Surgeons (RCS) rat, as does intravitreal injection of basic fibroblast growth factor (bFGF). We hypothesize that up-regulation of retinal bFGF is a consequence of laser lesioning in RCS rats. Therefore, we examined the localization of bFGF after laser and correlated this with Mailer cell glial fibrillary acidic protein (GFAP) expression, which is known to increase after injury.

Methods: A total of 34 RCS rats at postnatal day 23 were anaesthetized (ketamine 40 mg/kg) and their retinas were irradiated with a grid pattern of 40 non-overlapping argon green lesions with a power of 120 mW for 0.2 s using a 50 microm spot size. At 0, 6, 12, 24 and 48 h and 7, 14 and 21 days post-lesion, rats were anaesthetized and their eyes were enucleated and cryostat sectioned and the sections were processed using either an antibody to bFGF or GFAP using the standard avidin-biotinylated peroxidase complex method. Five age-matched RCS rats without laser lesions served as controls.

Results: Basic fibroblast growth factor immunoreactivity (IR) was normally located within cells in the ganglion cell layer inner nuclear layer and in retinal pigment epithelium cells and in the extracellular matrix/cell membranes of the outer nuclear layer (ONL). In lasered retinas, there was elevated bFGF-IR in the coagulated outer segments for the first 24 h. Retinal blood vessels/Müller cells/astrocytes were moderately labelled in and near each lesion immediately after lesion and became more intense after 48 h and persisted for at least 21 days. There was an elevation of bFGF-IR in the ONL on the lesion flanks at 14 days. Muller cell GFAP-IR was first detected at 6 h post-lesion and spread for a considerable distance beyond the lesion site. At 7 and 14 days, Müller cells at the lesion site had sprouted, while those on the flanks were still GFAP-IR.

Conclusions: Following laser lesion there was an increase in bFGF at the lesion core only for the first 24 h. However, elevated levels of bFGF were observed in the ONL at 14 days, which extended into the lesion flanks for a similar distance to that over which increased photoreceptor survival is found. These results provide support for the hypothesis that laser lesions induce bFGF and this may be the mechanism whereby photoreceptors are spared. Müller cell activation is consistent with growth factor stimulation, but was more widespread than the bFGF changes in ONL. However, blood vessel labelling was similarly widespread and so the responses may be linked between Müller cell GFAP reaction and blood vessel bFGF localization after laser lesions.

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