Accelerated 3D metabolite T1 mapping of the brain using variable‐flip‐angle SPICE

Author:

Zhao Yibo12ORCID,Li Yudu13ORCID,Guo Rong14ORCID,Jin Wen12,Sutton Brad135ORCID,Ma Chao6ORCID,El Fakhri Georges6,Li Yao78ORCID,Luo Jie7ORCID,Liang Zhi‐Pei12

Affiliation:

1. Beckman Institute for Advanced Science and Technology University of Illinois at Urbana‐Champaign Urbana Illinois USA

2. Department of Electrical and Computer Engineering University of Illinois at Urbana‐Champaign Urbana Illinois USA

3. National Center for Supercomputing Applications University of Illinois at Urbana‐Champaign Urbana Illinois USA

4. Siemens Medical Solutions USA, Inc. Urbana Illinois USA

5. Department of Bioengineering University of Illinois at Urbana‐Champaign Urbana Illinois USA

6. Department of Radiology and Biomedical Imaging Yale University School of Medicine New Haven Connecticut USA

7. School of Biomedical Engineering Shanghai Jiao Tong University Shanghai China

8. Institute of Medical Robotics Shanghai Jiao Tong University Shanghai China

Abstract

AbstractPurposeTo develop a practical method to enable 3D T1 mapping of brain metabolites.Theory and MethodsDue to the high dimensionality of the imaging problem underlying metabolite T1 mapping, measurement of metabolite T1 values has been currently limited to a single voxel or slice. This work achieved 3D metabolite T1 mapping by leveraging a recent ultrafast MRSI technique called SPICE (spectroscopic imaging by exploiting spatiospectral correlation). The Ernst‐angle FID MRSI data acquisition used in SPICE was extended to variable flip angles, with variable‐density sparse sampling for efficient encoding of metabolite T1 information. In data processing, a novel generalized series model was used to remove water and subcutaneous lipid signals; a low‐rank tensor model with prelearned subspaces was used to reconstruct the variable‐flip‐angle metabolite signals jointly from the noisy data.ResultsThe proposed method was evaluated using both phantom and healthy subject data. Phantom experimental results demonstrated that high‐quality 3D metabolite T1 maps could be obtained and used for correction of T1 saturation effects. In vivo experimental results showed metabolite T1 maps with a large spatial coverage of 240 × 240 × 72 mm3 and good reproducibility coefficients (< 11%) in a 14.5‐min scan. The metabolite T1 times obtained ranged from 0.99 to 1.44 s in gray matter and from 1.00 to 1.35 s in white matter.ConclusionWe successfully demonstrated the feasibility of 3D metabolite T1 mapping within a clinically acceptable scan time. The proposed method may prove useful for both T1 mapping of brain metabolites and correcting the T1‐weighting effects in quantitative metabolic imaging.

Funder

National Institutes of Health

Publisher

Wiley

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