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成年猪全层视网膜的培养移植

Transplantation of cultured adult porcine full-thickness retina.

作者信息

Engelsberg Karl, Ghosh Fredrik

机构信息

Department of Ophthalmology, Lund University Hospital, Lund, Sweden.

出版信息

Cell Transplant. 2007;16(1):31-9. doi: 10.3727/000000007783464506.

Abstract

In this study we wanted to examine how an adult neuroretina from an animal with an eye similar to the human one survives in vitro. We also wanted to investigate how the culture process affects the adult retina when used in a transplantation paradigm. Full-thickness neuroretinal sheets from adult porcine eyes were dissected into pieces measuring 3 mm in diameter. These were kept in culture for 1-3 days. After this time, the explants were fixed or transplanted subretinally to adult pigs, which were killed after 72-74 days. Transplanted eyes, as well as tissue kept in culture only, were processed for hematoxylin and eosin staining and immunohistochemistry. Explants kept 1 day in vitro (DIV) displayed the normal morphology. In these specimens, single pyknotic cells were evident in the outer nuclear layer (ONL) and ganglion cell layer, but were more frequent in the inner nuclear layer (INL). After longer times in vitro, severe degenerative changes appeared. Transplanted explants kept 1 DIV prior to transplantation exhibited normal retinal lamination in two out of four specimens. Transducin and recoverin labeling revealed photoreceptors with inner segments in these grafts. Rod bipolar cells displayed a normal morphology. Vertically arranged Müller cells were also seen in the laminated grafts. Two of the three transplants kept 2 DIV displayed minimal lamination. Eyes with transplants kept 3 DIV prior to transplantation displayed degenerated grafts in all eyes. This study shows that adult porcine neuroretinal explants kept in culture for 1 day display a normal morphology in their major part. Additionally, 1-day explants can survive transplantation with retained morphology even after several months. This indicates the possibility of storing adult donor tissue between harvest and transplantation. The culture system may also be used in the future as a tool for manipulating retinal donor tissue prior to transplantation.

摘要

在本研究中,我们想探究来自眼睛与人类相似的动物的成年神经视网膜在体外的存活情况。我们还想研究在移植范例中使用时,培养过程如何影响成年视网膜。将成年猪眼的全层神经视网膜片切成直径为3毫米的小块。将这些小块置于培养中1至3天。在此之后,将外植体固定或视网膜下移植到成年猪体内,这些猪在72至74天后被处死。对移植的眼睛以及仅在培养中保存的组织进行苏木精和伊红染色及免疫组织化学处理。在体外保存1天(体外培养天数,DIV)的外植体呈现正常形态。在这些标本中,单个固缩细胞在外核层(ONL)和神经节细胞层中明显可见,但在内核层(INL)中更为常见。在体外培养更长时间后,出现了严重的退行性变化。移植前保存1 DIV的移植外植体在四个标本中有两个呈现正常的视网膜分层。转导蛋白和恢复蛋白标记显示这些移植物中有带有内节的光感受器。视杆双极细胞呈现正常形态。在分层的移植物中也可见垂直排列的米勒细胞。三个保存2 DIV的移植物中有两个呈现最小程度的分层。移植前保存3 DIV的移植眼睛在所有眼中均显示移植物退化。本研究表明,在培养中保存1天的成年猪神经视网膜外植体在其主要部分呈现正常形态。此外,1天的外植体即使在几个月后也能在移植后保持形态存活。这表明在收获和移植之间储存成年供体组织的可能性。该培养系统未来也可能用作在移植前处理视网膜供体组织的工具。

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