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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

The pericytes in retinal vasculature were examined by immunofluorescent staining with platelet-derived growth factor receptor β after retro-orbital injection of fluorescent tomato lectin. The labeled retina was further treated with the tissue-clearing method and whole mounted for visualizing the three-dimensional views of pericytes surrounding retinal vasculature under a confocal microscope.

Abstract

Retinal pericytes are essential for vascular development and stability of the retina, playing a key role in maintaining the integrity of the retinal vasculature. To provide a detailed view of the morphological characteristics of pericytes, this study described a new approach combining the retro-orbital injection of a fluorescent agent, immunofluorescent-staining, and tissue-clearing treatment. Firstly, the fluorescent tomato lectin was injected into the retro-orbital sinus of the live mouse to label the retinal vasculature. After 5 min, the mouse was sacrificed, and its intact retina was carefully removed from the retinal cup and immunofluorescently stained with platelet-derived growth factor receptor β to reveal the pericytes. Additionally, the stained retina was treated with tissue-clearing reagent and whole mounted on the microscope slide. Through these approaches, the retinal vasculature and pericytes were clearly observed in the transparent retina. Under a confocal microscope, we obtained more opportunities to take high-resolution images for further reconstructing and analyzing the morphological characteristics of pericytes along the retinal vascular tree in a three-dimensional view. Methodologically, this protocol offers an effective approach for visualizing pericytes within the retinal vasculature, providing valuable insights into their role under both physiological and pathological conditions.

Introduction

Retinal pericytes are embedded within the basement membrane along the abluminal side of vascular endothelial cells, displaying a mesh-like pattern of short-range processes wrapped around the retinal blood vessels1. This intimate contact between pericytes and the retinal vasculature contributes to maintaining retina environmental homeostasis2. Although numerous studies have provided morphological evidence of pericytes in retinal vasculature, most of our understanding of the morphological characteristics of retinal pericytes comes from conventional histological techniques3.

In line with these studies, we designed this study to effectively showcase more morphological details of pericytes in the retinal microvasculature by combining traditional histological techniques with modern cutting-edge scientific methods. The approach here integrates three key techniques: retro-orbital injection of fluorescent tomato lectin in live mice, immunofluorescent staining with platelet-derived growth factor receptor β (PDGFR-β), and the solvent-based tissue clearing strategy. Retro-orbital injection of fluorescent tomato lectin has been proven effective and reliable for observing mouse retinal vasculature in both in vivo and in vitro settings4,5. PDGFR-β serves as a commonly used biomarker for the immunofluorescent staining of pericytes6. To capture high-resolution images of pericytes within the thicker and whole-mount retinas, the tissue-clearing strategy enhances histological transparency2,7,8.

While each of these techniques has been applied individually in retinal studies, their combined compatibility for investigating pericytes in mouse retinal vasculature remains uncertain. Since the average thickness of the mouse retina is approximately 180-220 µm9, antibody labeling and confocal imaging at this thick tissue without clearing treatment often result in high background signals, complicating the observation of the spatial relationship between pericytes and blood vessels10. Through the approaches described here, we aim to provide a straightforward method for visualizing pericytes within the retinal vasculature in a three-dimensional (3D) view under a confocal microscope. This enhanced cellular information from pericytes in the retinal vasculature could improve our understanding of retinal environmental homeostasis and underscore potential strategies for vascular protection, thereby enhancing functional outcomes in retinal vascular disorders.

Protocol

For this study, three young adult male C57BL/6 mice (8-10 weeks old, weighing 20-25 g) were used. They were housed in a 12 h light/dark cycle with controlled temperature and humidity and allowed free access to food and water. This study was approved by the Ethics Committee of the Institute of Acupuncture and Moxibustion, China Academy of Chinese Medical Sciences (approval No. 2023-03-14-04) and conducted in accordance with the National Institutes of Health Guide for the Care and Use of Laboratory Animals (National Academy Press, Washington, D.C., 1996).

1. In vivo retro-orbital injection of fluorescent tomato lectin

  1. Inject 50 mg/kg pentobarbital intraperitoneally to anesthetize the mouse. Assess the depth of anesthesia by evaluating the absence of a response to a toe pinch stimulus.
  2. Place the mouse in the right lateral recumbency with its head facing to the left.
  3. Press two fingers gently on the peri-orbital area to expose the mouse's left eye to allow the easiest administration of the injection into the left retro-orbital sinus of the animal11.
  4. Use a 1 mL syringe equipped with a 27G needle to gently pierce about 2-3 mm into the mouse's orbital venous sinus with the bevel on the needle facing forward at a 45° angle.
  5. Inject 0.1 mL (1 mg/mL) of fluorescent tomato lectin into the mouse's orbital venous sinus.

2. Perfusion and enucleation of eyes

  1. At 5 min after retro-orbital injection, inject tribromoethanol solution (250 mg/kg) intraperitoneally to deeply anesthetize the mouse. Subsequently, euthanize the animal via exsanguination and cardiac perfusion. Once breathing stops, open the thoracic cavity with surgical scissors12.
  2. Once breathing stops, open the thoracic cavity with surgical scissors. Sterilize surgical instruments in advance and operate in a fume hood. Use a 24G needle and insert it 2 mm into the left cardiac ventricle through the left ventricular apex. Perform perfusion at a rate of 3 mL/min with 20 mL of 0.9% physiological saline followed by 20 mL of 4% formaldehyde in 0.1 M phosphate buffer (PB, pH 7.4).
  3. Place the sacrificed mouse on its side and remove the skin covering the eyes with scissors. Enucleate the eyes with scissors and forceps.
  4. Cut the optic nerve and surrounding tissues, then lift out the eye and transfer to a 12-well plate for post-fixing in 4% formaldehyde in 0.1 M PB for 2 h.
  5. Cryoprotect the tissue in 25% sucrose in 0.1 M PB (pH 7.4) at 4 °C until it sinks to the bottom of the solution.
    NOTE: Since ocular tissue dehydrates well in a sucrose solution, the retina can be more easily and completely detached, facilitating subsequent comprehensive studies.

3. Dissection of retinas

  1. Transfer the eyes into a Petri dish containing 0.1 M PB (pH 7.4) using a plastic Pasteur pipette.
  2. Pierce the edge of the cornea with sharp scissors, cut around the cornea and iris, and discard.
  3. Use forceps to remove the lens and vitreous humor. Then, pull the cup-shaped retina away from the center of the eye with fine forceps. Rinse the retina with 0.1 M PB (pH 7.4) in a clean Petri dish.

4. Immunofluorescent-staining and tissue-clearing of retinas

  1. Carefully remove the cup-shaped retina and incubate it in a 2% Triton X-100 solution in 0.1 M PB (pH 7.4) overnight at 4 °C.
  2. Transfer the retina into the blocking solution (0.1 M PB + 1% Triton-X 100 + 0.2% sodium azide + 10% normal donkey serum) and rotate at 72 rpm on the shaker overnight at 4 °C.
  3. Transfer the retina into the solution containing the primary antibodies of goat anti-PDGFR-β (10 µg/mL) in dilution buffer (0.1 M PB + 0.2% Triton-X 100 + 0.2% sodium azide + 1% normal donkey serum) in a microcentrifuge tube and rotate on the shaker for 2 days at 4 °C.
  4. Wash the retina 2x with washing buffer (0.1 M PB + 0.2% Triton-X 100) at room temperature, then keep them in washing buffer overnight at 4 °C on the shaker.
  5. The next day, transfer the retina into the mixed solution containing the 1 mg/mL secondary antibody of donkey anti-goat 488 and 0.2 ng/mL fluorescent nuclear 4',6-diamidino-2-phenylindole (DAPI) in a microcentrifuge tube and rotate at 72 rpm on the shaker for 5 h at 4 °C.
  6. Wash the retina in a 6-well plate with washing buffer for 1 h, 2x, at room temperature. Keep the retina in washing buffer on the shaker overnight at 4 °C. Perform imaging and analysis as per step 5 to obtain the before tissue clearing views.
  7. Transfer the retina to the tissue-clearing reagent and gently rotate it at 60 rpm on the shaker for 1 h at 37 °C.
  8. After tissue clearing treatment, rinse the cup-shaped retina with 0.1 M PB (pH 7.4) in a clean Petri dish.
  9. Make 4 radial incisions reaching approximately 2/3 of the radius of the retina using spring scissors to create a petal shape.
  10. Flatten and mount the retina on a microscope slide, and then remove any excess PB with a small piece of absorbent paper. Keep the inside of the retina facing up on the slide.
  11. Circle the mounted retina with a spacer and fill the gap with fresh tissue-clearing reagent and a coverslip.

5. Imaging and analyses

  1. Obtain the outside views of the retina before (after completing step 4.6) and after tissue-clearing treatment.
  2. Scan the montage views of labeled retina with the panoramic tissue slice scanner. Use a 2x objectives lens with NA of 0.08.
  3. Take the higher magnification images by confocal imaging system equipped with the following objectives lenses: 10x lens with NA of 0.40 and 40x lens with NA of 0.95. Set the confocal pinhole at 152 µm (10x objective lens) and 105 µm (40x objective lens). Set the spatial resolution of image capture at 1024 x 1024 pixels (10x objective lens) and 640 x 640 pixels (40x objective lens).
  4. Capture 50 images (Z-stack) in 2 µm frames from the labeled retina. Integrate all images in a single in-focus under the projection/topography mode. For the setup, click Set Start Focal Plane > Set End focal plane > Set step size > Choose Depth Pattern > Image Capture > Z series.
  5. Capture images using the following excitation and emission wavelengths for different fluorescence signals: Green fluorescence signals at 499 nm and 519 nm; red fluorescence signals at 591 nm and 618 nm; and blue fluorescence signals at 401 nm and 421 nm.
  6. Reconstruct the images in the three-dimensional pattern by importing Z-stack confocal images into an analysis software by selecting Add New Surfaces > Choose Volume settings > Choose Source Channel > Adjust display > Adjust Surface Angle > Snapshot.

Results

From the outside views of the whole-mount retina, the tissue transparency of the whole-mount retina was increased using the tissue-clearing treatment compared to that of the retina without tissue-clearing (Figure 1).

For the histological examination on the whole-mount retina, the retinal vasculature was labeled in red with fluorescent tomato lectin through the retro-orbital injection, and retinal pericytes are shown in green with PDGFR-β (

Discussion

In this study, we detailed the technical process for demonstrating the morphology of pericytes in retinal vasculature using retro-orbital injection of fluorescent tomato lectin, immunofluorescent examination with PDGFR-β, and solvent-based tissue clearing. The results show that these techniques are highly compatible for highlighting pericytes in the whole-mount retina. The combination of these methodologies offers an effective approach for visualizing the morphological characteristics of pericytes in retinal vascula...

Disclosures

No conflicts of interest.

Acknowledgements

This study was supported by the Beijing Natural Science Foundation (No. 7244480), the CACMS Innovation Fund (No. CI2021A03407), the National Natural Science Foundation of China (No. 82004492), and the Fundamental Research Funds for the Central public welfare research institutes (Nos. ZZ-YQ2023008, ZZ14-YQ-032, ZZ-JQ2023008, ZZ-YC2023007).

Materials

NameCompanyCatalog NumberComments
4',6-diamidino-2-phenylindole (DAPI)Thermo Fisher ScientificD3571Protect from light
Alexa Fluor 488 donkey anti-goat IgG (H+L)Thermo Fisher ScientificA-11055Protect from light
C57BL/6 mouseBeijing Vital River Laboratory Animal Technology Co., Ltd.SCXK (Jing) 2021-0006
Confocal imaging systemOlympusFV1200
Goat anti-PDGFR-βResearch and DevelopmentAF104225 µg 
Imaris softwareOxford Instrumentsv.9.0.1
Lycopersicon esculentum(Tomato) lectin, DyLight594Thermo Fisher ScientificL324711 mg
Microcentrifuge tubeAxygenMCT-150-C1.5 mL
Normal donkey serumJackson ImmunoResearch017-000-12110 mL
Panoramic tissue slice scannerOlympusVS120-S6-W
Photoshop and  IllustrationAdobeCS6
RapiClear 1.52 SolutionSunJin LabRC15200110 mL
Six-well plateCostar3335
Spring scissors Fine Science Tools15003-08
Superfrost Plus microscope slideThermo Fisher Scientific4951PLUS-00125 mm x 75 mm x 1 mm

References

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3D VisualizationRetinal Vascular PericytesImmunostainingFluorescent AgentTissue clearing TreatmentRetro orbital InjectionPlatelet derived Growth Factor ReceptorConfocal MicroscopeMorphological CharacteristicsRetinal VasculatureHigh resolution ImagingPhysiological ConditionsPathological Conditions

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