Measuring Deformation in the Mouse Optic Nerve Head and Peripapillary Sclera.
Nguyen Cathy, Midgett Dan, Kimball Elizabeth C, Steinhart Matthew R, Nguyen Thao D, Pease Mary E, Oglesby Ericka N, Jefferys Joan L, Quigley Harry A
AI Summary
This study measured mouse optic nerve head and peripapillary sclera deformation under pressure. It found regional differences in how these tissues respond to acute and chronic IOP changes, providing insights into glaucoma's mechanical effects.
Abstract
Purpose
To develop an ex vivo explant system using multiphoton microscopy and digital volume correlation to measure the full-field deformation response to intraocular pressure (IOP) change in the peripapillary sclera (PPS) and in the optic nerve head (ONH) astrocytic structure.
Methods
Green fluorescent protein (GFP)-glutamate transporter-GLT1 (GLT1/GFP) mouse eyes were explanted and imaged with a laser-scanning microscope under controlled inflation. Images were analyzed for regional strains and changes in astrocytic lamina and PPS shape. Astrocyte volume fraction in seven control GLT1/GFP mice was measured. The level of fluorescence of GFP fluorescent astrocytes was compared with glial fibrillary acidic protein (GFAP) labeled astrocytes using immunohistochemistry.
Results
The ONH astrocytic structure remained stable during 3 hours in explants. Control strain-globally, in the central one-half or two-thirds of the astrocytic lamina-was significantly greater in the nasal-temporal direction than in the inferior-superior or anterior-posterior directions (each P≤ 0.03, mixed models). The PPS opening (perimeter) in normal eye explants also became wider nasal-temporally than superior-inferiorly during inflation from 10 to 30 mm Hg (P = 0.0005). After 1 to 3 days of chronic IOP elevation, PPS area was larger than in control eyes (P = 0.035), perimeter elongation was 37% less than controls, and global nasal-temporal strain was significantly less than controls (P = 0.007). Astrocyte orientation was altered by chronic IOP elevation, with processes redirected toward the longitudinal axis of the optic nerve.
Conclusions
The explant inflation test measures the strain response of the mouse ONH to applied IOP. Initial studies indicate regional differences in response to both acute and chronic IOP elevation within the ONH region.
MeSH Terms
Shields Classification
Key Concepts6
Control strain in the central one-half or two-thirds of the astrocytic lamina in GFP-glutamate transporter-GLT1 (GLT1/GFP) mouse eyes was significantly greater in the nasal-temporal direction than in the inferior-superior or anterior-posterior directions (each P≤ 0.03, mixed models).
The peripapillary sclera (PPS) opening (perimeter) in normal GFP-glutamate transporter-GLT1 (GLT1/GFP) mouse eye explants became wider nasal-temporally than superior-inferiorly during inflation from 10 to 30 mm Hg (P = 0.0005).
After 1 to 3 days of chronic intraocular pressure (IOP) elevation, the peripapillary sclera (PPS) area in GFP-glutamate transporter-GLT1 (GLT1/GFP) mouse eyes was larger than in control eyes (P = 0.035), perimeter elongation was 37% less than controls, and global nasal-temporal strain was significantly less than controls (P = 0.007).
Astrocyte orientation in GFP-glutamate transporter-GLT1 (GLT1/GFP) mouse eyes was altered by chronic intraocular pressure (IOP) elevation, with processes redirected toward the longitudinal axis of the optic nerve.
The optic nerve head (ONH) astrocytic structure remained stable during 3 hours in ex vivo explants from GFP-glutamate transporter-GLT1 (GLT1/GFP) mice.
The explant inflation test measures the strain response of the mouse optic nerve head (ONH) to applied intraocular pressure (IOP) using a system with multiphoton microscopy and digital volume correlation.
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