Posted By: NITRC ADMIN - Dec 2, 2015
Tool/Resource: Journals
 

Quantitative β mapping for calibrated fMRI.

Neuroimage. 2015 Nov 24;

Authors: Shu CY, Sanganahalli BG, Coman D, Herman P, Rothman DL, Hyder F

Abstract
The metabolic and hemodynamic dependencies of the blood oxygenation level-dependent (BOLD) signal form the basis for calibrated fMRI, where the focus is on oxidative energy demanded by neural activity. An important part of calibrated fMRI is the power-law relationship between the BOLD signal and deoxyhemoglobin concentration, which in turn is related to the ratio between oxidative demand (CMRO2) and blood flow (CBF). The power-law dependence between BOLD signal and deoxyhemoglobin concentration is signified by a scaling exponent β. Until recently [R1.1] most studies assumed a β value of 1.5, which is based on numerical simulations of the extravascular BOLD component. Since basal value of CMRO2 and CBF can vary from subject-to-subject and/or region-to-region, a method to independently measure β in vivo should improve the accuracy of calibrated fMRI results. We describe a new method for β mapping through characterizing R2' - the most sensitive relaxation component of BOLD signal (i.e., the reversible magnetic susceptibility component that is predominantly of extravascular origin at high magnetic field) - as a function of intravascular magnetic susceptibility induced by an FDA-approved superparamagnetic contrast agent. In α-chloralose anesthetized rat brain, at 9.4T, we measured β values of ~0.8 uniformly across large neocortical swathes, with lower magnitude and more heterogeneity in subcortical areas. Comparison of β maps in rats anesthetized with medetomidine and α-chloralose revealed that β is independent of neural activity levels at these resting states. We anticipate this method for β mapping can help facilitate calibrated fMRI for clinical studies.

PMID: 26619788 [PubMed - as supplied by publisher]



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