1 H-MRS processing parameters affect metabolite quantification: The urgent need for uniform and transparent standardization

Alex A Bhogal; Remmelt R Schür; Lotte C Houtepen; Bart van de Bank; Vincent O Boer; Anouk Marsman; Peter B Barker; Tom W J Scheenen; Jannie P Wijnen; Christiaan H Vinkers; Dennis W J Klomp

doi:https://doi.org/10.1002/nbm.3804

1 H-MRS processing parameters affect metabolite quantification: The urgent need for uniform and transparent standardization

Alex A Bhogal, Remmelt R Schür, Lotte C Houtepen, Bart van de Bank, Vincent O Boer, Anouk Marsman, Peter B Barker, Tom W J Scheenen, Jannie P Wijnen, Christiaan H Vinkers, Dennis W J Klomp

Research output: Contribution to journal › Article › Academic › peer-review

25 Citations (Scopus)

Abstract

Proton magnetic resonance spectroscopy (1 H-MRS) can be used to quantify in vivo metabolite levels, such as lactate, γ-aminobutyric acid (GABA) and glutamate (Glu). However, there are considerable analysis choices which can alter the accuracy or precision of 1 H-MRS metabolite quantification. It is currently unknown to what extent variations in the analysis pipeline used to quantify 1 H-MRS data affect outcomes. The purpose of this study was to evaluate whether the quantification of identical 1 H-MRS scans across independent and experienced research groups would yield comparable results. We investigated the influence of model parameters and spectral quantification software on fitted metabolite concentration values. Sixty spectra in 30 individuals (repeated measures) were acquired using a 7-T MRI scanner. Data were processed by four independent research groups with the freedom to choose their own individualized and optimal parameter settings using LCModel software. Data were processed a second time in one group using an independent software package (NMRWizard) for an additional comparison with a different post-processing platform. Correlations across research groups of the ratio between the highest and, arguably, the most relevant resonances for neurotransmission [N-acetyl aspartate (NAA), N-acetyl aspartyl glutamate (NAAG) and Glu] over the total creatine [creatine (Cr) + phosphocreatine (PCr)] concentration, using Pearson's product-moment correlation coefficient (r), were calculated. Mean inter-group correlations using LCModel software were 0.87, 0.88 and 0.77 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. The mean correlations when comparing NMRWizard results with LCModel fitting results at University Medical Center Utrecht (UMCU) were 0.87, 0.89 and 0.71 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. Metabolite quantification using identical 1 H-MRS data was influenced by processing parameters, basis sets and software choice. Locally preferred processing choices affected metabolite quantification, even when using identical software. Our results reinforce the notion that standard practices should be established to regularize outcomes of 1 H-MRS studies, and that basis sets used for processing should be made available to the scientific community.

Original language	English
Journal	NMR in biomedicine
Volume	30
Issue number	11
DOIs	https://doi.org/10.1002/nbm.3804
Publication status	Published - Nov 2017
Externally published	Yes

Keywords

Aspartic Acid/analogs & derivatives
Creatine/analysis
Glutamic Acid/analysis
Humans
Magnetic Resonance Spectroscopy/methods
Phosphocreatine/analysis

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https://doi.org/10.1002/nbm.3804

Cite this

@article{e0eaaa4e4a78495ab0e2afb7fdc9be9a,

title = "1 H-MRS processing parameters affect metabolite quantification: The urgent need for uniform and transparent standardization",

abstract = "Proton magnetic resonance spectroscopy (1 H-MRS) can be used to quantify in vivo metabolite levels, such as lactate, γ-aminobutyric acid (GABA) and glutamate (Glu). However, there are considerable analysis choices which can alter the accuracy or precision of 1 H-MRS metabolite quantification. It is currently unknown to what extent variations in the analysis pipeline used to quantify 1 H-MRS data affect outcomes. The purpose of this study was to evaluate whether the quantification of identical 1 H-MRS scans across independent and experienced research groups would yield comparable results. We investigated the influence of model parameters and spectral quantification software on fitted metabolite concentration values. Sixty spectra in 30 individuals (repeated measures) were acquired using a 7-T MRI scanner. Data were processed by four independent research groups with the freedom to choose their own individualized and optimal parameter settings using LCModel software. Data were processed a second time in one group using an independent software package (NMRWizard) for an additional comparison with a different post-processing platform. Correlations across research groups of the ratio between the highest and, arguably, the most relevant resonances for neurotransmission [N-acetyl aspartate (NAA), N-acetyl aspartyl glutamate (NAAG) and Glu] over the total creatine [creatine (Cr) + phosphocreatine (PCr)] concentration, using Pearson's product-moment correlation coefficient (r), were calculated. Mean inter-group correlations using LCModel software were 0.87, 0.88 and 0.77 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. The mean correlations when comparing NMRWizard results with LCModel fitting results at University Medical Center Utrecht (UMCU) were 0.87, 0.89 and 0.71 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. Metabolite quantification using identical 1 H-MRS data was influenced by processing parameters, basis sets and software choice. Locally preferred processing choices affected metabolite quantification, even when using identical software. Our results reinforce the notion that standard practices should be established to regularize outcomes of 1 H-MRS studies, and that basis sets used for processing should be made available to the scientific community.",

keywords = "Aspartic Acid/analogs & derivatives, Creatine/analysis, Glutamic Acid/analysis, Humans, Magnetic Resonance Spectroscopy/methods, Phosphocreatine/analysis",

author = "Bhogal, {Alex A} and Sch{\"u}r, {Remmelt R} and Houtepen, {Lotte C} and {van de Bank}, Bart and Boer, {Vincent O} and Anouk Marsman and Barker, {Peter B} and Scheenen, {Tom W J} and Wijnen, {Jannie P} and Vinkers, {Christiaan H} and Klomp, {Dennis W J}",

year = "2017",

month = nov,

doi = "https://doi.org/10.1002/nbm.3804",

language = "English",

volume = "30",

journal = "NMR in biomedicine",

issn = "0952-3480",

publisher = "John Wiley and Sons Ltd",

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TY - JOUR

T1 - 1 H-MRS processing parameters affect metabolite quantification

T2 - The urgent need for uniform and transparent standardization

AU - Bhogal, Alex A

AU - Schür, Remmelt R

AU - Houtepen, Lotte C

AU - van de Bank, Bart

AU - Boer, Vincent O

AU - Marsman, Anouk

AU - Barker, Peter B

AU - Scheenen, Tom W J

AU - Wijnen, Jannie P

AU - Vinkers, Christiaan H

AU - Klomp, Dennis W J

PY - 2017/11

Y1 - 2017/11

N2 - Proton magnetic resonance spectroscopy (1 H-MRS) can be used to quantify in vivo metabolite levels, such as lactate, γ-aminobutyric acid (GABA) and glutamate (Glu). However, there are considerable analysis choices which can alter the accuracy or precision of 1 H-MRS metabolite quantification. It is currently unknown to what extent variations in the analysis pipeline used to quantify 1 H-MRS data affect outcomes. The purpose of this study was to evaluate whether the quantification of identical 1 H-MRS scans across independent and experienced research groups would yield comparable results. We investigated the influence of model parameters and spectral quantification software on fitted metabolite concentration values. Sixty spectra in 30 individuals (repeated measures) were acquired using a 7-T MRI scanner. Data were processed by four independent research groups with the freedom to choose their own individualized and optimal parameter settings using LCModel software. Data were processed a second time in one group using an independent software package (NMRWizard) for an additional comparison with a different post-processing platform. Correlations across research groups of the ratio between the highest and, arguably, the most relevant resonances for neurotransmission [N-acetyl aspartate (NAA), N-acetyl aspartyl glutamate (NAAG) and Glu] over the total creatine [creatine (Cr) + phosphocreatine (PCr)] concentration, using Pearson's product-moment correlation coefficient (r), were calculated. Mean inter-group correlations using LCModel software were 0.87, 0.88 and 0.77 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. The mean correlations when comparing NMRWizard results with LCModel fitting results at University Medical Center Utrecht (UMCU) were 0.87, 0.89 and 0.71 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. Metabolite quantification using identical 1 H-MRS data was influenced by processing parameters, basis sets and software choice. Locally preferred processing choices affected metabolite quantification, even when using identical software. Our results reinforce the notion that standard practices should be established to regularize outcomes of 1 H-MRS studies, and that basis sets used for processing should be made available to the scientific community.

AB - Proton magnetic resonance spectroscopy (1 H-MRS) can be used to quantify in vivo metabolite levels, such as lactate, γ-aminobutyric acid (GABA) and glutamate (Glu). However, there are considerable analysis choices which can alter the accuracy or precision of 1 H-MRS metabolite quantification. It is currently unknown to what extent variations in the analysis pipeline used to quantify 1 H-MRS data affect outcomes. The purpose of this study was to evaluate whether the quantification of identical 1 H-MRS scans across independent and experienced research groups would yield comparable results. We investigated the influence of model parameters and spectral quantification software on fitted metabolite concentration values. Sixty spectra in 30 individuals (repeated measures) were acquired using a 7-T MRI scanner. Data were processed by four independent research groups with the freedom to choose their own individualized and optimal parameter settings using LCModel software. Data were processed a second time in one group using an independent software package (NMRWizard) for an additional comparison with a different post-processing platform. Correlations across research groups of the ratio between the highest and, arguably, the most relevant resonances for neurotransmission [N-acetyl aspartate (NAA), N-acetyl aspartyl glutamate (NAAG) and Glu] over the total creatine [creatine (Cr) + phosphocreatine (PCr)] concentration, using Pearson's product-moment correlation coefficient (r), were calculated. Mean inter-group correlations using LCModel software were 0.87, 0.88 and 0.77 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. The mean correlations when comparing NMRWizard results with LCModel fitting results at University Medical Center Utrecht (UMCU) were 0.87, 0.89 and 0.71 for NAA/Cr + PCr, NAA + NAAG/Cr + PCr and Glu/Cr + PCr, respectively. Metabolite quantification using identical 1 H-MRS data was influenced by processing parameters, basis sets and software choice. Locally preferred processing choices affected metabolite quantification, even when using identical software. Our results reinforce the notion that standard practices should be established to regularize outcomes of 1 H-MRS studies, and that basis sets used for processing should be made available to the scientific community.

KW - Aspartic Acid/analogs & derivatives

KW - Creatine/analysis

KW - Glutamic Acid/analysis

KW - Humans

KW - Magnetic Resonance Spectroscopy/methods

KW - Phosphocreatine/analysis

U2 - https://doi.org/10.1002/nbm.3804

DO - https://doi.org/10.1002/nbm.3804

M3 - Article

C2 - 28915314

SN - 0952-3480

VL - 30

JO - NMR in biomedicine

JF - NMR in biomedicine

IS - 11

ER -