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Cryosectioning and Immunostaining of Mouse Retina
* These authors contributed equally
In This Article
Summary
A protocol for preparing mouse retinal cryosections and performing immunostaining on photoreceptors is described. This article enables researchers to consistently produce mouse retinal frozen sections with well-preserved morphology and high-quality immunostaining results.
Abstract
Tissue sectioning and immunohistochemistry are essential techniques in histological and pathological studies of retinal diseases using animal models. These methods enable detailed examinations of tissue morphologies and the localization of specific proteins within the tissue, which provide valuable insights into disease processes and mechanisms. Mice are the most widely used model for this purpose. However, because mouse eyeballs are small and mouse retinas are extremely delicate tissues, obtaining high-quality retinal sections and immunostaining images from mouse eyeballs is typically challenging. This study describes an improved protocol for cryosectioning mouse retinas and performing immunohistochemistry. An essential point of this protocol involves coating the eyeball with a layer of super glue, which prevents deformation of the eyeballs during the processes of cornea removal, lens extraction, and embedding. This step ensures the integrity of retinal morphologies is well preserved. This protocol highlights critical technical considerations and optimization strategies for consistently producing high-quality retinal sections and achieving excellent immunostaining results.
Introduction
Cryosectioning and immunohistochemistry (IHC) are indispensable techniques in biomedical research, particularly for studying complex biological structures such as the retina1. These advanced methodologies are integral to understanding the intricate cellular composition and molecular organization of the retina. They provide researchers with the ability to investigate retinal functionality and pathology at a detailed level, offering insights that are critical for advancing knowledge in this field.
Cryosectioning plays a vital role in maintaining the morphological integrity of retinal tissue. It ensures that the delicat....
Protocol
The procedure adhered to the guidelines established by the Association for Research in Vision and Ophthalmology for the Use of Animals in Research. Approval was obtained from the Institutional Animal Care and Use Committee (IACUC) of Sichuan Provincial People's Hospital. Male C57Bl/6J mice, aged two to three months and weighing 25-30 g, were used for this protocol. A comprehensive list of the reagents and equipment utilized in this study is provided in the Table of Materials.
1. Reagent preparation
- 1x PBS buffer
- Weigh 8 g of NaCl, 1.42 g of Na2HPO4, 0.42 g o....
Representative Results
Following the protocol outlined above, eyes from 1-month-old wild-type C57Bl/6J mice were fixed in 4% PFA. The fixed samples were then embedded in OCT and cryosectioned. The sections were immunostained with an anti-PDE6B antibody and counterstained with DAPI to label the nuclei. PDE6B is a phototransduction protein specifically expressed in rod photoreceptor cells4. Compared to traditional protocols, this protocol significantly improves both the morphology of mouse retinas and the quality of immun.......
Discussion
A number of factors influence the quality of tissue sections, including the composition of the fixation solution, fixation and cryoprotection time, and embedding methods5. When enucleating the eyeball from the mouse, it is essential to remove the extraocular muscles and other connective tissue attached to the eyeball. If not properly removed, these tissues can cause deformation of the eyeball during extraction from the eye socket, potentially leading to retinal detachment. During the fixation proc.......
Disclosures
The authors have no conflicts to disclose.
Acknowledgements
This research project was supported by the National Natural Science Foundation of China (82371059 (H.Z.), 82102470 (J.W.)), Sichuan Science and Technology Program (2023JDZH0002 (H.Z.)).
....Materials
| Name | Company | Catalog Number | Comments |
| -80 °C freezer | Haier | DW-86L626 | |
| Adhesion microscope slides | CITOTEST | 80312-3161 | |
| Alexa488-Goat anti-Rabbit | Proteintech | SA00006-2 | |
| C57BL/6J mouse | The Jackson Laboratory | 664 | |
| Cryosection microtome | Leica | N/A | |
| Cryostat | LEICA | N/A | |
| DAPI | Cell Signaling Technology | 4083S | |
| Dissecting microscope | ZEISS | 3943030830 | |
| Donkey serum | Solarbio | S9100 | |
| Embedding molds | Thermo Fisher Scientific | 1841 | |
| Fine dissection scissors | RWD | S13001-10 | |
| Fine forceps | RWD | F11020-11 | |
| Fluoromount aqueous mounting medium | Sigma-Aldrich | F4680 | |
| Incubator | Shanghai Yuejin | N/A | |
| KCl | Sigma-Aldrich | 1049330500 | |
| KH2PO4 | Sigma-Aldrich | 1048771000 | |
| Kimwipes | Thermo Fisher Scientific | FIS-06666 | |
| Laser confocal microscope | ZEISS | N/A | |
| Microscope cover Glass | CITOTEST | 80340-3610 | |
| Na2HPO4 | Sigma-Aldrich | 1065860500 | |
| NaCl | Sigma-Aldrich | S9888 | |
| NaOH | Sigma-Aldrich | 1091371003 | |
| O.C.T compound | Sakura | 4583 | |
| Pap pen | Sigma-Aldrich | Z672548 | |
| PFA | Sigma-Aldrich | 441244 | |
| Rabbit anti-PDE6B | Proteintech | 22063-1-AP | |
| Shaker | SCILOGEX | 8042210200 | |
| Spring scissors | RWD | S11036-08 | |
| Sucrose | BioFroxx | 1245GR500 | |
| Super glue | Deli | 7147S | |
| Tennis string (1.24 mm) | Gosen | TS761 | |
| Tribromoethanol | Macklin | T831042 | |
| Triton X-100 | Solarbio | IT9100 |
References
- Tokuyasu, K. T. Immunochemistry on ultrathin frozen sections. Histochem J. 12 (4), 381-403 (1980).
- Ramos-Vara, J. A., Miller, M. A., et al. When tissue antigens and ant....
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