Ocular tissue imaging using ultrahigh-resolution, full-field optical coherence tomography.

PURPOSE

Ultrahigh-resolution, full-field optical coherence tomography (OCT), which uses a white light source, allows bidimensional, noninvasive tomographic imaging without scanning. The goal of the present study was to apply full-field OCT to ocular tissue imaging in an attempt to explore the capabilities of the technique.

METHODS

This full-field OCT system uses a Linnik-type interferometer with a tungsten-halogen source. The spatial resolution is 0.9 x 0.7 microm (transverse x axial). Unstained tissue samples (cornea, lens, retina, choroid, and sclera) and whole, unfixed eyes of rat, mouse, and pig were examined under immersion. A charge-coupled device (CCD) camera recorded a pair of interferometric images that were combined to display en face (i.e., in the x-y plane) tomographic images in real time. The acquisition time per tomographic image, which includes summation of 10 raw images, was on the order of 1 s. Postprocessing allows volumetric navigation through the image stack as well as three-dimensional (3D) imaging.

RESULTS

Cellular-level resolution was achieved in isolated tissue samples. En face (x-y) images revealed corneal epithelial and stromal cells, lens fibers, nerve fibers, major vessels, and retinal pigment epithelial cells. In x-z reconstructions, cellular layers within the cornea and retina and arterioles and venules were clearly defined. Transscleral retinal imaging was achieved in albino animals.

CONCLUSIONS

Ultrahigh-resolution, full-field OCT allows cellular-level imaging of unstained ocular tissues with high penetration depth. Although the current system is unsuitable for clinical use, this simple technique has potential for in vivo ocular examination, for which a new system is currently under development.