Literature DB >> 31747332

Separation of hemodynamic signals from GCaMP fluorescence measured with wide-field imaging.

M T Valley1, M G Moore2, J Zhuang1, N Mesa1, D Castelli1, D Sullivan1, M Reimers2, J Waters1.   

Abstract

Wide-field calcium imaging is often used to measure brain dynamics in behaving mice. With a large field of view and a high sampling rate, wide-field imaging can monitor activity from several distant cortical areas simultaneously, revealing cortical interactions. Interpretation of wide-field images is complicated, however, by the absorption of light by hemoglobin, which can substantially affect the measured fluorescence. One approach to separating hemodynamics and calcium signals is to use multiwavelength backscatter recordings to measure light absorption by hemoglobin. Following this approach, we develop a spatially detailed regression-based method to estimate hemodynamics. This Spatial Model is based on a linear form of the Beer-Lambert relationship but is fit at every pixel in the image and does not rely on the estimation of physical parameters. In awake mice of three transgenic lines, the Spatial Model offers improved separation of hemodynamics and changes in GCaMP fluorescence. The improvement is pronounced near blood vessels and, in contrast with the Beer-Lambert equations, can remove vascular artifacts along the sagittal midline and in general permits more accurate fluorescence-based determination of neuronal activity across the cortex.NEW & NOTEWORTHY This paper addresses a well-known and strong source of contamination in wide-field calcium-imaging data: hemodynamics. To guide researchers toward the best method to separate calcium signals from hemodynamics, we compare the performance of several methods in three commonly used mouse lines and present a novel regression model that outperforms the other techniques we consider.

Entities:  

Keywords:  animal behavior; calcium imaging; hemodynamics; optical methods; systems neuroscience

Mesh:

Substances:

Year:  2019        PMID: 31747332     DOI: 10.1152/jn.00304.2019

Source DB:  PubMed          Journal:  J Neurophysiol        ISSN: 0022-3077            Impact factor:   2.714


  12 in total

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Journal:  Neurophotonics       Date:  2022-07-06       Impact factor: 4.212

5.  Chronic, cortex-wide imaging of specific cell populations during behavior.

Authors:  Joao Couto; Simon Musall; Xiaonan R Sun; Anup Khanal; Steven Gluf; Shreya Saxena; Ian Kinsella; Taiga Abe; John P Cunningham; Liam Paninski; Anne K Churchland
Journal:  Nat Protoc       Date:  2021-06-02       Impact factor: 17.021

6.  Miniaturized head-mounted microscope for whole-cortex mesoscale imaging in freely behaving mice.

Authors:  Mathew L Rynes; Daniel A Surinach; Samantha Linn; Michael Laroque; Vijay Rajendran; Judith Dominguez; Orestes Hadjistamoulou; Zahra S Navabi; Leila Ghanbari; Gregory W Johnson; Mojtaba Nazari; Majid H Mohajerani; Suhasa B Kodandaramaiah
Journal:  Nat Methods       Date:  2021-04-05       Impact factor: 28.547

7.  Wide-field calcium imaging of cortex-wide activity in awake, head-fixed mice.

Authors:  Chi Ren; Takaki Komiyama
Journal:  STAR Protoc       Date:  2021-11-20

8.  Correcting for the hemoglobin absorption artifact in fiber photometry data.

Authors:  Run Zhang; Christina K Kim
Journal:  Cell Rep Methods       Date:  2022-07-18

9.  Dopamine D1 receptor signalling in dyskinetic Parkinsonian rats revealed by fiber photometry using FRET-based biosensors.

Authors:  Jace Jones-Tabah; Hanan Mohammad; Shadi Hadj-Youssef; Lucy E H Kim; Ryan D Martin; Faïza Benaliouad; Jason C Tanny; Paul B S Clarke; Terence E Hébert
Journal:  Sci Rep       Date:  2020-09-02       Impact factor: 4.379

10.  Sources of widefield fluorescence from the brain.

Authors:  Jack Waters
Journal:  Elife       Date:  2020-11-06       Impact factor: 8.140

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