Department of Ophthalmology, University Hospital, Lund, Sweden.
Dev Neurosci. 2011;33(2):110-7. doi: 10.1159/000328170. Epub 2011 Jul 21.
Phenotypic characterization of human retinogenesis may be facilitated by use of the tissue culture system paradigm. Traditionally, most culture protocols involve isolation of retinal tissue and/or cells, imposing various degrees of trauma, which in many cases leads to abnormal development. In this paper, we present a novel culture technique using whole embryonic eyes to investigate whether the retina in situ can develop normally in vitro. All procedures were carried out in accordance with the Declaration of Helsinki. Human embryos were obtained from elective abortions with the informed consent of the women seeking abortion. A total of 19 eyes were enucleated. The ages of the embryonic retinas were 6-7.5 weeks. Eyecups from 2 eyes were fixed immediately, to be used as controls. The remaining 17 eyes were placed on culture plates and divided into 3 groups kept for 7 (n = 4), 14 (n = 7) and 28 (n = 6) days in vitro (DIV). After fixation, the specimens were processed for hematoxylin and eosin staining, immunohistochemistry and terminal deoxynucleotidyl transferase-mediated dUTP nick end labeling (TUNEL). Antibodies against recoverin (rods and cones), protein kinase C (PKC; rod bipolar cells) and vimentin (Müller cells) were used. TUNEL was used to detect apoptotic cells. In hematoxylin- and eosin-stained sections, the control retinas displayed a neuroblast cell layer (NBL) and an inner marginal zone. Specimens kept 7-14 DIV had a similar appearance, while 28-day specimens consisted of an NBL with almost no marginal zone. Thirteen of the 17 cultured retinas displayed completely normal lamination without rosettes or double folds. Pyknotic cells were found at the inner margin of the retinas, and the proportion of these cells increased with time in vitro. TUNEL staining revealed a few scattered cells in 7-DIV specimens, and the amount of stained cells in the inner part of the retinas progressively increased in 14- and 28-DIV specimens. Vimentin labeling showed cells arranged in a vertical pattern in all retinas. Labeling with recoverin revealed photoreceptors in 4 of the retinas kept for 14 DIV, and in all retinas kept for 28 DIV. After 28 DIV, 2 of the eyes labeled with PKC contained rod bipolar cells with minimal axons. Here we showed that human embryonic retinas can be kept in culture in situ within the eye for at least 4 weeks. Abnormal lamination is not as frequent as in isolated full-thickness retinas, indicating that physical and biochemical contact with surrounding tissues is vital for proper development. Several types of the retina-specific neuronal and glial cells were seen to differentiate according to the in vivo schedule. The results are important for future studies of retinal development, and the technique can also be used for testing the effects of various drugs on the immature retina.
使用组织培养系统范式可以促进人视网膜发生的表型特征分析。传统上,大多数培养方案涉及视网膜组织和/或细胞的分离,这会造成不同程度的创伤,而在许多情况下,这会导致发育异常。在本文中,我们提出了一种使用整个胚胎眼睛的新培养技术,以研究视网膜是否可以在体外正常发育。所有程序均符合《赫尔辛基宣言》的规定。胚胎来自人工流产,流产妇女知情同意。总共取出 19 只眼睛。胚胎视网膜的年龄为 6-7.5 周。2 只眼睛的眼杯立即固定,用作对照。其余 17 只眼睛置于培养板上,分为 3 组,分别在体外培养 7(n=4)、14(n=7)和 28(n=6)天。固定后,对标本进行苏木精和伊红染色、免疫组织化学和末端脱氧核苷酸转移酶介导的 dUTP 缺口末端标记(TUNEL)检测。使用针对 recoverin(视杆和视锥)、蛋白激酶 C(PKC;视杆双极细胞)和波形蛋白(Müller 细胞)的抗体。TUNEL 用于检测凋亡细胞。在苏木精和伊红染色切片中,对照视网膜显示神经母细胞层(NBL)和内边缘区。培养 7-14 天的标本具有相似的外观,而培养 28 天的标本则由 NBL 组成,几乎没有边缘区。在 17 个培养的视网膜中有 13 个显示出完全正常的分层,没有玫瑰花结或双折。在视网膜的内边缘发现了固缩细胞,并且这些细胞的比例随着体外时间的延长而增加。在 7 天培养的标本中发现了几个散在的 TUNEL 染色细胞,而在 14 天和 28 天培养的标本中,视网膜内部的染色细胞数量逐渐增加。波形蛋白标记显示所有视网膜中的细胞呈垂直排列。在培养 14 天的 4 个视网膜中,用 recoverin 标记发现了光感受器,在培养 28 天的所有视网膜中都发现了光感受器。培养 28 天后,2 只标记有 PKC 的眼睛含有具有最小轴突的视杆双极细胞。在这里,我们表明人类胚胎视网膜可以在眼睛内原位保持培养至少 4 周。分层异常并不像全厚视网膜那样频繁,这表明与周围组织的物理和生化接触对于正常发育至关重要。根据体内时间表,观察到几种类型的视网膜特有的神经元和神经胶质细胞分化。该结果对于视网膜发育的未来研究非常重要,并且该技术还可用于测试各种药物对未成熟视网膜的影响。
