Corneal Angiogenesis Assay in Mice

The corneal micropocket assay was performed as described^{37 (link),38 (link)}. Seven-week-old Akt1^WT and Akt1^∆SMC mice were anesthetized with chloral hydrate (450 mg/kg, i.p.). After 10 min, alcaine was dropped into the eye. A corneal micropocket was created with a modified von Graef knife and MVR knife in both eyes. A micropellet of sucralfate (Sigma-Aldrich) coated with hydron polymer (Sigma–Aldrich) containing 200 ng of VEGF was implanted into each corneal pocket. The pellet was positioned approximately 1 mm from the corneal lymbus. Seven days later, the mice were anesthetized with 1–2% inhaled isoflurane, and the eyes were captured using a digital camera. For staining, eyes were fixed with 4% paraformaldehyde for 12 h at 4 °C. The primary antibody was incubated in blocking buffer (3% BSA in PBS-Tween-20) overnight at 4 °C. The secondary antibody was diluted in blocking buffer and incubated for 2 h at room temperature. Corneas were flat-mounted using an anti-fading reagent, and images were obtained using a confocal microscope (K1-Fluo, Nanoscope Systems, Daejeon, Korea). Sprouting was quantified by measuring the VEGF-induced vessel sprouting length using ImageJ (National Institutes of Health).

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Ha J.M., Jin S.Y., Lee H.S., Kum H.J., Vafaeinik F., Ha H.K., Song S.H., Kim C.D, & Bae S.S. (2022). Akt1-dependent expression of angiopoietin 1 and 2 in vascular smooth muscle cells leads to vascular stabilization. Experimental & Molecular Medicine, 54(8), 1133-1145.

Publication 2022

sucralfate hydron polymer

Akt1 Alcaine Antibody Assay Buffer Camera Chloral hydrate Confocal microscope Corneas Eyes Fluo Isoflurane Mice Paraformaldehyde Polymer Sucralfate Tween 20 Vegf Vessel

Corresponding Organization :

Other organizations : Pusan National University

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Variable analysis

independent variables

Genotype: Akt1^WT and Akt1^∆SMC mice

dependent variables

VEGF-induced vessel sprouting length

control variables

Age of mice: 7 weeks old
Anesthesia: Chloral hydrate (450 mg/kg, i.p.)
Corneal micropocket creation: Modified von Graef knife and MVR knife
Micropellet implantation: Sucralfate coated with hydron polymer containing 200 ng of VEGF
Micropellet positioning: Approximately 1 mm from the corneal lymbus
Observation time: 7 days
Anesthesia for imaging: 1-2% inhaled isoflurane
Tissue fixation: 4% paraformaldehyde for 12 h at 4 °C
Immunostaining: Primary antibody incubation in blocking buffer overnight at 4 °C, Secondary antibody incubation for 2 h at room temperature
Imaging: Confocal microscopy

controls

Positive control: Not mentioned
Negative control: Not mentioned

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