Sequential activation of two discrete brain areas appears as waves in simulated EEG phase latency maps.

(A) Schematic illustration of simulated EEG. Two brain areas (green and red ellipses) are defined on the cortex by a set of dipoles that are activated uniformly with a time delay (ΔT) between areas. A finite element forward model in Brainstorm (Tadel et al., 2011) is used to simulate the resulting potentials measured with EEG electrodes (purple dots). (B) Latency to peak measured across electrodes following the sequential activation of two sets of dipoles (green and red circles in the background) with a distance of 11cm (Δx/σx=16.9) and time delay of 20ms (ΔT/σT=0.2). A continuous delay patterns propagating from posterior (P) to anterior (A) is observed. (C) Phase-latency distance correlations (PLDC) for different distances and different delays between two activated areas. PLDC remains close to 1 (indicating apparent wave propagation) for a wide range of values.

Sequential activation of discrete spiking populations underlies LFP waves in turtle cortex.

(A) Schematic of the experimental setup. The brain with eye attached is extracted and the visual cortex is flattened on a MEA and its activity is measured in response to visual stimulation of the retina. (B) A cortical response following visual stimulation at t=0. Traces show the following data: raw electrode (grey), low-pass filtered (<2Hz, blue with dotted line marking the first oscillation cycle), high-pass filtered (>200Hz, black), ALSA (red) and the instantaneous phase of the low-pass filtered trace (green). (C) Power spectral density (averaged over 1000 randomly selected trials from one experiment). (D) Dynamics of low-pass filtered (<2Hz) and averaged (n=4000) cortical responses to visual stimulation. The amplitude in each time window (200-750ms post stimulus in 50ms intervals) is color coded and presented on the physical space of the electrode. Filled color-coded circles mark the electrodes recorded in (E). M=Medial, A=Anterior, L=Lateral, P=Posterior. (E) Averaged (n=4000) low-pass filtered (<2Hz) traces for channels along the delay gradient. The maximum is marked by a circle and its location on the array is color coded in (D). (F) Phase Latency-distance correlation (PLDC) distribution for all trials with strong waves (n=2415, blue) from this experiment and for the same trials with shuffled latencies (red). (G) Spiking responses (black dots) in a single visual stimulation trial. Empty circles mark the π/2 phase crossing. Red circles denote the ALSA onset for each electrode. Electrodes were reordered according to the LFP phase crossings. (H) The distribution of LFP phase crossing times and first spike times for the response in (G) with corresponding DIP values (0.85 and 0.0002, respectively). (I-J) Latency maps on the electrode array’s physical space extracted from the Hilbert phase (I) and ALSA (J). Black line denotes the wave center path extracted from the Hilbert phase (see Methods). (K) DIP-test p-value distribution of the 1st spikes (blue), Hilbert phase crossings (red) and differences between both per trial (gray) for strong waves with enough spikes (n=902). Distribution medians (solid black line) are connected by a dashed black line (blue line connects the distributions’ means). (L) Same as (K) but for ALSA. (M,N) Medians of the DIP-test p-values (black lines in K,L, respectively) from 6 recordings in 4 animals. Dashed black line marks the median over all experiments. All results except (N,M) are from the same recording.

A simple analytic model of sequentially activated Gaussians exhibits travelling peaks with a diversity of patterns.

(A) The spatiotemporal potential of two sequentially activated one dimensional spatial Gaussians (centers; x1=-0.5 and x2=0.5; standard deviation σx=1), each with a temporal Gaussian activation profile (peaking at t1=-1 and t2=1; standard deviation σt=1), as in Equation 1. Notice wave-like propagation. (B) Spatial profile of Equation 1 at time (dotted line in (A)) for 3 conditions. Notice that for Δx≤2σx the spatial profile is concave. (C) The spatial derivative of V(x,t) in (A). Black line marks Gaussian peak dynamics (zero crossing points of the spatial derivate). (D) Peak dynamics for different values of distances between Gaussian centers (Δx). Notice that the average velocity increases with Δx. (E,F) Same as in (A,C) but for a model of a periodically fluctuating Gaussian (Equation 3) (x1=-0.5, x2=0.5, σx=1, f=1, ⍰1=-3π/8, ⍰2=3π/8).(G,H) The peak dynamics (as in (D)) for the model in (E,F) as a function of the phase difference between Gaussians, Δ⍰(G), and f, the frequency of the oscillation (H). f=1 in (G) and ⍰1=-π/4, ⍰2=π/4 in (H). Notice that wave velocity increases with frequency and can changes sign as a function of Δ⍰. (I) PDLC values calculated for different Δx and σx. Black line marks the Δx=2σx border. (J) Plane, radial and spiral-like propagation patterns and the resulting phase latency maps (right) for different spatial arrangements of two sequentially activated Gaussians (left).

Sequential activation of two discrete small brain areas appears as waves in simulated EEG phase latency maps.

(A) Latency to peak as measured across electrodes following the sequential activation of two sets of localized dipoles (green and red, as in Figure 1B) simulating the activation of small cortical areas. A wave like delay pattern is observed. (B) Phase latency distance correlations (PLDC) for different distances and different delays between two activated areas (as in Figure 1C). PLDC remains close to 1 (indicating wave propagation) for a wide range of values. (C) Activation dynamics before and after filtering into a narrow band frequency range (10-12Hz). (D) PLDC for two sequentially activated large areas (as in Figure 1C) after narrow band filtering (C). Filtering increases PLDC values making rendering them more wave-like.

Identification of waves during single oscillation cycles.

(A) The lowpass filtered (0-2Hz) voltage responses across all electrodes to a single visual stimulation. Red circle marks the same oscillation phase across electrodes. Traces of different electrodes are displaced along the y axis. (B) Single cycles are identified (colored center dots with different colors marking different cycles) from the filtered traces in (A). Within each cycle, the oscillation phase is marked by empty circles with color coded amplitude. Channels in (A,B) are reordered according to the phase time of the first oscillation cycle. Cycle durations are marked by black lines at the bottom.

Phase latency maps of single trials.

The phase latency is plotted on the physical space of the electrodes for the first oscillation cycle in 48 single trials. Color code is normalized between maximum and minimum for every trial. The strongest events with most electrode participating in the first oscillation cycle were used. Electrodes that did not participate in a specific oscillation event (see oscillation cycle detection method) were not plotted.

Spikes are locked to the 0-2Hz oscillation.

(A) The distribution for the first spikes to the visual stimulation relative to the 0-2Hz oscillation. (B,C) same as (A) but for ALSA onset times (B) and for all spikes during all cycles in the recording (C). Notice that both the spikes and ALSA exhibit a similar locking with the ALSA distribution being narrower. Shown above is the mode of the distribution calculated over 36 bins with width of π/18.

DIP statistics captures segregation of propagating activity into modules.

(A) Phase latency map for the LFP in the trial shown in Figure 2G. The wave center path is shown in black. (B) Single trial’s phase crossing events (red triangle) plotted together with the wave center path (black) as points in 3d space (2 spatial coordinates representing the electrode layout and one temporal coordinate). (C) The distribution of phase delays in time and the corresponding DIP test value for this distribution. (D,E) Same as (A-C) but for ALSA onset times. While the LFP phase crossings (A-C) are spread around the wave center path in space and time, the ALSA onset times are organized as clustered groups. Correspondingly, the DIP value for the LFP is considerably higher than for ALSA. Panels (A,C,D,F) are identical to panels (H,I,J), but shown here for comparison.

Identification of waves for single oscillation cycles in the β band.

(A) The bandpass filtered (12-35Hz) voltage responses across all electrodes to a single visual stimulation. Red circle marks the same oscillation phase across electrodes. Traces of different electrodes are displaced along the y axis. (B) Single cycles are identified (colored center dots with different colors marking different cycles) from the filtered traces in (A). (B) Single cycles are identified (color dots with different colors marking different cycles; cycle durations are marked by black lines) from the filtered traces in (A). Within each cycle, the oscillation phase is marked by empty circles with color coded amplitude. Channels in (A,B) are reordered according to the phase time of the first oscillation cycle. Cycle durations are marked by black lines at the bottom (Events with less than 100 of 120 active channels were excluded from analysis). (C) Examples of phase latency maps extracted from single waves in the 12-35Hz band.