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A New Method for Comprehensive Bird’s-Eye Analysis of the Internal Limiting Membrane

Toshio Hisatomi, MD, PhD; Hiroshi Enaida, MD, PhD; Taiji Sakamoto, MD, PhD; Takaaki Kanemaru, MD; Tadahisa Kagimoto, MD; Ichiro Yamanaka, MD, PhD; Akifumi Ueno, MD; Takao Nakamura, MD, PhD; Yasuaki Hata, MD, PhD; Tatsuro Ishibashi, MD, PhD

Arch Ophthalmol. 2006;124:1005-1011.

Objective  To elucidate the pathogenesis of macular hole formation, focusing in particular on the possible role of cellular migration on the cortical vitreous and internal limiting membrane (ILM) around the macular hole.

Methods  To gain a comprehensive overview of the ILM excised in macular hole surgery (n = 36), the ILMs were carefully unfolded and spread out onto glass slides as continuous flat sheets that each contained a macular hole. The specimens were observed by light microscopy and transmission electron microscopy (n = 9), and the cellular distribution was analyzed by scanning electron microscopy in a quantitative manner (n = 27). Immunohistochemistry for glial fibrillary acidic protein and cytokeratin 18 was carried out for cellular characterization. Cellular proliferation was assessed by immunohistochemistry for proliferating cell nuclear antigen and Ki-67.

Results  Cellular migration was not apparent around the macular hole in the early stage of development of the macular hole (stage 2, 0 µm). As the macular hole passed through the later stages of development, cellular migration developed around the macular hole (stage 3, 84 µm) and the area of cellular migration gradually enlarged (stage 4, 420 µm). The immunophenotypic analysis showed that these cells were mainly glial fibrillary acidic protein–positive glial cells and cytokeratin 18–positive retinal pigment epithelial cells. The proliferating cell nuclear antigen and Ki-67 immunohistochemistry showed that some of these cells were proliferating on the ILM.

Conclusions  Cellular migration on the ILM is not necessary for the initial formation of a macular break. Cellular migration developed after the macular break occurred, and the migration and proliferation increased gradually from the macular hole.

Clinical Relevance  This study provides a new method for understanding the ultrastructural analysis of the pathogenesis of the macular hole.

Author Affiliations: Department of Ophthalmology (Drs Hisatomi, Enaida, Kagimoto, Yamanaka, Ueno, Nakamura, Hata, and Ishibashi) and Morphology Core (Dr Kanemaru), Graduate School of Medical Sciences, Kyushu University, Fukuoka, and Department of Ophthalmology, Kagoshima University School of Medicine, Kagoshima (Dr Sakamoto), Japan.

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