Table 1.
Overview of the spatiotemporal resolution, specificity, observed patterns, and considerations for all of the discussed imaging modalities.
| Electrode arrays | Optical imaging of fluorescence and intrinsic signals | fMRI | EEG | |
|---|---|---|---|---|
| Number of neurons | One to hundreds | Tens to hundreds | n/a | Millions, cortical surface |
| n/a | ||||
| Spatial resolution | 200 to | 50 to | 400 to | 10 to 20 mm |
| Time resolution | Millisecond | Millisecond (depends on kinetics of sensor) | Second | Millisecond to hundreds of milliseconds |
| Second | ||||
| Cell-type specificity | Limited | High (depends on the promoter) | Very low signal from hemodynamic response to neural activity. | Low signal predominantly from EPSPs and IPSPs in cortical pyramidal apical dendrites |
| n/a | ||||
| Patterns found | (1) Slow oscillation generated around layer 5 (in vitro ferret occipital cortex, in vivo rats and cats) 6,7,8,9,10 | (1) Global plane waves traveling anterior to posterior (mice)13,14 | (1) Propagating activity, such as QPPs (rats and humans)16,17,18–22 | (1) Transient spatial configurations, such as EEG and microstates (humans)31,26,27,28,29,30 |
| (2) Brief spontaneous depolarizations, localized to an area of a barrel column (rats and mice)11 | (2) Standing waves that have no net movement (mice)15 | (2) Transient spatial configurations, such as CAPs (rats and humans)23,16,24,25 | ||
| (3) Propagating waves that traveled horizontally across dorsal cortex (rats and mice)11,12 | (3) Local source, sink, and saddle points (mice)15 | |||
| Pitfalls | (1) Large artifacts | (1) Problems of light delivery | (1) Low temporal resolution | (1) Low spatial resolution |
| (2) Tissue damage | (2) Dependent on efficiency of viral transfection | (2) No cell type specificity | (2) Signal primarily from postsynaptic potentials of apical dendrites | |
| (3) Potential toxicity of opsins | (3) Low SNR | (3) Superficial signal, no localization at greater cortical depths | ||
| (4) Unspecific effects |