Published April 16, 2024 | Version v1
Dataset Open

Data for: Plastic vasomotion entrainment in eLife

  • 1. Tohoku University

Description

The presence of global synchronization of vasomotion induced by oscillating visual stimuli was identified in the mouse brain. Endogenous autofluorescence was used and the vessel "shadow" was quantified to evaluate the magnitude of the frequency-locked vasomotion. This method allows vasomotion to be easily quantified in non-transgenic wild-type mice using either the wide-field macro-zoom microscopy or the deep-brain fiber photometry methods. Vertical stripes horizontally oscillating at a low temporal frequency (0.25 Hz) were presented to the awake mouse and oscillatory vasomotion locked to the temporal frequency of the visual stimulation was induced not only in the primary visual cortex but across a wide surface area of the cortex and the cerebellum. The visually induced vasomotion adapted to a wide range of stimulation parameters. Repeated trials of the visual stimulus presentations resulted in the entrainment of the amplitude of the vasomotion. Horizontally oscillating visual stimulus is known to induce horizontal optokinetic response (HOKR). The amplitude of the eye movement is known to increase with repeated training sessions and the flocculus region of the cerebellum is known to be essential for this learning to occur. Here, we show a strong correlation between the average HOKR performance gain and the vasomotion entrainment magnitude in the cerebellar flocculus. Therefore, the plasticity of vasomotion and neuronal circuits appeared to occur in parallel. Efficient energy delivery by the entrained vasomotion may contribute to meeting the energy demand for increased coordinated neuronal activity and the subsequent neuronal circuit reorganization.

Notes

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 22KJ0262

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 22K15218

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 20H05896

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 23H04659

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 18H05110

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 20H056046

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 19H03338

Funding provided by: Japan Society for the Promotion of Science
Crossref Funder Registry ID: https://ror.org/00hhkn466
Award Number: 22H02713

Funding provided by: Research Foundation for Opto-Science and Technology
Crossref Funder Registry ID: https://ror.org/01fvvv243
Award Number:

Funding provided by: Takeda Science Foundation
Crossref Funder Registry ID: https://ror.org/02y123g31
Award Number:

Funding provided by: NOVARTIS Foundation for the Promotion of Science*
Crossref Funder Registry ID:
Award Number:

Funding provided by: Uehara Memorial Foundation
Crossref Funder Registry ID: https://ror.org/00gc20a07
Award Number:

Methods

Imaging data were collected using macro-zoom fluorescence stereo microscope.

Data were processed using mainly ImageJ and AxoGraph softwares.

Files

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