The responses of cells in the visual cortex to stimulation of the two
eyes changes dramatically following a period of monocular visual
deprivation (MD) during a critical period in early life. This phenomenon,
referred to as ocular dominance (OD) plasticity, is a widespread model for
understanding cortical plasticity. In this study, we designed stimulus
patterns and quantification methods to analyze OD in the mouse visual
cortex using optical imaging of intrinsic signals. Using periodically
drifting bars restricted to the binocular portion of the visual field, we
obtained cortical maps for both contralateral (C) and ipsilateral
(I) eyes and computed OD maps as (C −
I)/(C + I). We defined the OD index
(ODI) for individual animals as the mean of the OD map. The ODI
obtained from an imaging session of less than 30 min gives reliable
measures of OD for both normal and monocularly deprived mice under
Nembutal anesthesia. Surprisingly, urethane anesthesia, which yields
excellent topographic maps, did not produce consistent OD findings. Normal
Nembutal-anesthetized mice have positive ODI (0.22 ±
0.01), confirming a contralateral bias in the binocular zone. For mice
monocularly deprived during the critical period, the ODI of the
cortex contralateral to the deprived eye shifted negatively towards the
nondeprived, ipsilateral eye (ODI after 2-day MD: 0.12 ±
0.02, 4-day: 0.03 ± 0.03, and 6- to 7-day MD: −0.01 ±
0.04). The ODI shift induced by 4-day MD appeared to be near
maximal, consistent with previous findings using single-unit recordings.
We have thus established optical imaging of intrinsic signals as a fast
and reliable screening method to study OD plasticity in the mouse.
