Abstract
Objective
To develop a three-dimensional (3D) high-resolution free-breathing magnetization transfer ratio (MTR) sequence for contrast-free assessment of myocardial infarct and coronary vein anatomy.
Materials and methods
Two datasets with and without off-resonance magnetization transfer preparation were sequentially acquired to compute MTR. 2D image navigators enabled beat-to-beat translational and bin-to-bin non-rigid motion correction. Two different imaging sequences were explored. MTR scar localization was compared against 3D late gadolinium enhancement (LGE) in a porcine model of myocardial infarction. MTR variability across the left ventricle and vessel sharpness in the coronary veins were evaluated in healthy human subjects.
Results
A decrease in MTR was observed in areas with LGE in all pigs (non-infarct: 25.1 ± 1.7% vs infarct: 16.8 ± 1.9%). The average infarct volume overlap on MTR and LGE was 62.5 ± 19.2%. In humans, mean MTR in myocardium was between 37 and 40%. Spatial variability was between 15 and 20% of the mean value. 3D whole heart MT-prepared datasets enabled coronary vein visualization with up to 8% improved vessel sharpness for non-rigid compared to translational motion correction.
Discussion
MTR and LGE showed agreement in infarct detection and localization in a swine model. Free-breathing 3D MTR maps are feasible in humans but high spatial variability was observed. Further clinical studies are warranted.
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Introduction
MRI plays an important role for non-invasive assessment of myocardial fibrosis in patients with ischemic and non-ischemic cardiomyopathies. Myocardial scar assessment has been shown to have important prognostic value [1,2,3]. Furthermore, in patients requiring cardiac resynchronization therapy, detection of focal fibrosis and coronary sinus/vein anatomy may help to guide the intervention [4]. In these applications, the accurate discrimination of fibrotic or scarred tissue from surrounding healthy myocardium is crucial.
Late gadolinium enhancement (LGE) MRI is the gold standard for the assessment of myocardial fibrosis [5]. LGE shows enhanced signal intensity by targeting the enlarged extracellular space in fibrotic tissue using gadolinium-based contrast agents [6]. LGE is a qualitative approach where the time point of imaging after the injection of a contrast agent determines the pattern of enhancement. While core infarct regions will enhance strongly and at a late stage during the contrast washout (> 25 min), the signal from the rim of an infarcted region (area at risk) might enhance very early on (2–3 min), only to return to normal at the late stage [7]. Furthermore, the use of gadolinium-based contrast agents may generate accumulation in the neural system [8] and/or adverse contrast reaction. Therefore, the development of a semi-quantitative and gadolinium-free approach for the assessment of myocardial fibrosis may be of great interest.
Magnetization transfer (MT) is an endogenous MR contrast mechanism, which does not require the injection of a contrast agent. MT has shown to be sensitive to structural changes associated with myocardial fibrosis, such as the increase in collagen content [9,10,11]. MT was first demonstrated by Wolff and Balaban in kidney and skeletal muscle [12], showing a signal decrease from free water protons, after selectively saturating a pool of protons with restricted motion with an off-resonance preparation. The signal decrease is explained by an exchange of magnetization between the water protons (free pool) and those with restricted motion (bound pool). The characteristics of the exchange are determined by the tissue composition, in particular, the size and distribution of its macromolecular or bound pool component.
A common application of MT contrast has been to suppress signal coming from protein-rich tissue, such as white matter or muscle [13, 14]. This effect can generate good contrast between myocardium and blood irrespective of blood oxygenation and therefore improve cardiac vein visualization [15]. While T2 preparation is known to be useful in coronary angiography [16], the large reduction in T2 of deoxygenated blood causes difficulty in coronary vein imaging. MT preparation is largely independent of the magnetic susceptibility effect that causes T2 reduction in venous blood and has been shown to generate a contrast enhancement that is superior to T2-based approaches in the cardiac veins [17].
Another application of MT in cardiac MRI is the semi-quantitative magnetization transfer ratio (MTR). In MTR, two images are acquired, with and without MT preparation, and the percentage difference or ratio between them is calculated. A breath-held 2D cine steady state technique showed reduced MTR values associated with LGE enhancement in acute myocardial infarction (MI) patients [18]. However, breath-holding can be difficult in sick patients, where the length of breath-hold may limit the spatial resolution and different breath-hold positions may lead to misregistration artefacts between slices. Germain et al. has recently proposed a diaphragmatic navigated free-breathing 3D on-resonance MT approach [19], where they show some agreement between LGE enhancement and reduced MT effects in patients with acute or recent MI. However, partial volume effects and likely residual motion seem to have caused significant intra- and intersubject variability. We hypothesize that a significant increase in slice resolution and two-dimensional navigation may have a good impact in reproducibility and accuracy.
To address the above challenges, we developed and evaluated a novel free-breathing motion corrected 3D whole-heart MTR sequence for the simultaneous assessment of localized fibrosis and coronary vein anatomy without the administration of a contrast agent.
Methods
Sequence acquisition and reconstruction
A prototype motion-corrected free-breathing 3D magnetization transfer contrast imaging sequence was implemented on a 1.5 T MR scanner (MAGNETOM Aera, Siemens Healthcare, Erlangen, Germany). The sequence comprised two sequentially acquired 3D datasets, one with MT preparation and one without any preparation (hereon dataset REF).
A pulse diagram of the sequence is shown in Fig. 1a. Each acquisition was performed with a Cartesian trajectory with spiral profile order [20] and preceded by a 2D image navigator (iNAV) [21] to enable beat-to-beat translational motion correction in foot-to-head and left-to-right directions. The iNAVs were generated by spatially encoding the first 14 (start-up) pulses of the imaging sequence. The high-resolution 3D datasets were acquired in segmented fashion over multiple heartbeats, and data sampling started with the 15th RF pulse to the end of the echo train in every heartbeat. The spiral-profile Cartesian trajectory was chosen because it produces incoherent and noise-like undersampling artefacts which are beneficial for undersampled reconstruction. In addition, it provides some motion robustness associated with spiral sampling while maintaining a Cartesian computationally efficient reconstruction.
Spoiled gradient echo (SPGR) and balanced steady-state free-precession (bSSFP) imaging modules were investigated with the described MT preparation module. Data sampling was made to coincide with the diastolic resting period to minimize the impact of cardiac motion. The subject-specific trigger delay time and data acquisition window were determined using a free-breathing 2D cine, acquired in transversal orientation prior to the proposed sequence.
The MT preparation (represented in Fig. 1b) consisted of a train of 20 Sinc-shaped off-resonance RF pulses with individual length of 20.48 ms, separated by 1.5 ms pause periods. The preparation train was played out immediately before the imaging module in every heartbeat (or segment) of the MT-prepared image. The off-resonance frequency and flip angle of the pulses were optimized as described in the following sections.
Off-line reconstruction and post-processing was done in Matlab (The MathWorks, Inc., Natick, MA, USA). Two types of motion correction approaches were evaluated: (I) beat-to-beat 2D translational motion correction and (II) combined beat-to-beat 2D translational plus bin-to-bin non-rigid motion correction [22]. A scheme of the data flow is shown in Fig. 2a.
Beat-to-beat translational motion correction was performed by compensating the displacement in image space with a linear phase shift in k-space, using a property of Fourier transformations [23]:
where \({K}_{\mathrm{a}\mathrm{c}\mathrm{q}}\) and \({K}_{\mathrm{c}\mathrm{o}\mathrm{r}}\) represent the acquired and corrected data, respectively, \(\overrightarrow{k}\) is the k-space trajectory vector \({(k}_{x},{k}_{y})\) and \(\overrightarrow{d}\) is the respiratory motion displacement \({(d}_{x},{d}_{y})\) in the left-to-right and foot-to-head directions, respectively, obtained from the iNAVs by normalized cross-correlation.
In the non-rigid motion correction framework, respiratory motion in the foot–head direction was derived from the iNAVs to assign the data into respiratory phases or bins (3–5 bins, maximum bin size 3.5 mm). Then, beat-to-beat 2D translation motion correction in the left-to-right and foot-to-head directions [according to Eq. (1)] was applied with respect to the centre of each bin, followed by iterative SENSE reconstruction to obtain an intra-bin motion-corrected 3D image for image of each respiratory phase so that 3D motion fields between respective respiratory phases (i.e. bins) could be obtained via non-rigid registration [24] of the 3D images. The parameters involved in the estimation of 3D motion fields include the weight of the penalty (i.e. in our case the bending energy) for an objective function based on normalized mutual information (using values as proposed by Modat et al. [24]) and the spacing or size of the deformation grid (in each of the three dimensions). Spacing was adjusted according to image resolution with an iterative experimental approach.
The motion fields, coil sensitivity maps, sampling trajectory and measured k-space data were incorporated in a motion-corrected generalized matrix description (GMD) [22, 25], whereby a motion-corrected 3D dataset was then obtained by solving the inverse problem using a conjugate gradient algorithm.
Motion correction was applied to the MT-prepared and REF datasets independently. In each, an end-expiration position iNAV was chosen as ‘reference’ for the cross-correlation procedure. After motion-corrected reconstruction, the MT-prepared and REF datasets were co-registered to correct any small misalignments [24]. MTR maps were calculated voxel-wise as:
where \({I}_{\mathrm{M}\mathrm{T}}\) and \({I}_{\mathrm{R}\mathrm{E}\mathrm{F}}\) are the signal intensity of the MT and REF datasets, respectively.
Numerical simulations
Bloch simulations with a two-pool model of exchange were used to determine optimal MT preparation parameters. The evolution of the transverse and longitudinal magnetization of the free pool (\({M}_{x,y}^{A}\), \({M}_{z}^{A}\), respectively) and bound pool (\({M}_{x,y}^{B}\), \({M}_{z}^{B}\), respectively) under off-resonance irradiation with frequency ∆F and amplitude \({\omega }_{1}\) can be described by a modified set of Bloch equations [26]:
where \(\mathfrak{I}\) and \(\mathcal{R}\) are the imaginary and real parts of \({\omega }_{1}\), respectively. The modification includes precession terms associated with the irradiation frequency (\(\Delta F\)), which are added in Eqs. (3) and (4), while terms dependent on the exchange rate (\(R\)) are added in Eqs. (5) and (6). \({R}_{A}\) and \({R}_{B}\) are the longitudinal relaxation rates of the free (A) and bound (B) pools, respectively.
Under off-resonance irradiation, the bound pool experiences direct saturation of its longitudinal magnetization. This is due to its extremely short \({ T}_{2}\), which causes negligible feedback with the transversal components. The saturation rate of the bound pool (\({R}_{\mathrm{R}\mathrm{F}\mathrm{B}}\)) is calculated as proportional to the RF power (\({\omega }_{1}^{2}\)) and the bound pool’s line absorption shape using an experimental super-Lorentzian approximation for semisolid systems [27]. In this model, the bound pool \({T}_{2}\) was fixed at \({T}_{2}^{B}=14\) μs for all simulations. The equilibrium magnetizations of the bound pool and free pool (\({M}_{0}^{B}{,M}_{0}^{A}\)) represent their size and therefore the ratio \(PSR=\frac{{M}_{0}^{B}}{{M}_{0}^{A}+{M}_{0}^{B}}\) is the relative size of the bound pool [28, 29].
For a series of short and shaped off-resonance pulses, both \({\omega }_{1}\) and \({R}_{\mathrm{R}\mathrm{F}\mathrm{B}}\) are time dependent and no closed-form solution for the resulting magnetization can be found. Portnoy and Stanisz proposed a numerical approach [30] in which the RF pulse is split into small time intervals \(\mathrm{d}t\approx 50\) µs, whereby its amplitude may be considered constant. The evolution of the net magnetization vector \({\overrightarrow{M}}_{A,B}\left(t\right)\) over a time \(\mathrm{d}t\) is then solved as a linear problem and each transient solution propagates as the initial state for the next interval, until the end of the pulse is reached.
The MTR sequence was simulated using the described model to optimize its sensitivity to the pool size ratio (PSR) in myocardium-like tissue.
Simulated MT preparation parameters included bandwidth = 270 Hz, Sinc shape, length = 20.48 ms, delay between pulses = 1.5 ms, and pulse repetitions n = 20. Tissue parameters in myocardial simulations were performed using an exchange rate R of 50 Hz, \({T}_{1}^{A}\)/\({T}_{2}^{A}\) times of 1100/55 ms, and PSR of 15%, unless stated otherwise.
Simulations in myocardial-like tissue were performed over a range of ΔF (200–8000 Hz), MT pulse flip angles (360–900°), B0 inhomogeneity (from − 250 to 250 Hz), free pool relaxation times (\({T}_{1}^{A}\)=1000–1500 ms, \( {T}_{2}^{A}\)= 30–80 ms), and exchange-related parameters (R = 20–70 Hz, PSR = 0–30%). A simulated constant heart rate of 65 beats per minute (bpm) was used. The signal was measured from the 15th echo (the sampling of the k-space centre) during the fifth heartbeat, to ensure pseudo steady-state conditions. Two different imaging modules were simulated: (I) SPGR with sequence parameters including TR/TE = 3.8/1.6 ms and FA = 15°, (II) bSSFP with sequence parameters including TR/TE = 3.2/1.4 ms and FA = 70°. A single-pool (no exchange) model was assumed during the pulses of the imaging module.
Phantom study
Agar samples with different concentrations (1%, 2%, 2.5% and 5% agar in water) were prepared and used to validate the signal model and evaluate the performance of the proposed sequence in the presence of different MT exchange parameters and in the absence of motion. The proposed sequence was acquired using SPGR (TR/TE = 3.8/1.6 ms, FA = 15°, BW = 401 Hz/px, field of view (FoV) = 300 × 300 × 112 mm3, resolution = 1.4 × 1.4 × 4 mm3, number of profiles/excitations = 30) and bSSFP (TR/TE = 3.2/1.4 ms, FA = 70°, BW = 925 Hz/px). The MT pulse parameters were the same as described for the simulations. Data were acquired over a wide range of MT pulse flip angles (360–900˚) and off-resonance frequencies (400–8000 Hz).
Animal study
Animal experiments were conducted in Landrace pigs (n = 3) at the Institut de Chirurgie Guidée par l’image (IHU), Strasbourg, France. The pigs were scanned in vivo 6 weeks after undergoing left anterior descending artery occlusion for 3 h, using the procedure described by Tschabrunn et al. [31]. Each animal was scanned with the proposed sequence using the following imaging parameters: coronal orientation, FoV = 300 × 300 × 108 mm3, resolution = 1.7 × 1.7 × 6 mm3, SPGR (TR/TE = 3.8/1.76 ms, FA = 15°, BW = 535 Hz/px). MT preparation pulses had bandwidth, shape, length, and delay between pulses as described in the phantom study. MT off-resonance frequency was ∆F = 1500 Hz, pulse repetitions n = 10 and flip angle = 720°.
A 3D bSSFP LGE dataset was obtained following 10–20 min after injection of the contrast agent (Gadovist, Bayer, Germany). Imaging parameters included coronal orientation (matching the MTR scan), FoV = 200 × 260 × 105mm3, resolution = 1.2 × 1.2 × 1.2mm3, and bSSFP (TR/TE = 3.2/1.58 ms, FA = 90°, BW = 930 Hz/px).
Respiratory motion was very limited due to ventilation and did not affect the heart position, therefore no motion correction/compensation procedures were applied.
Scar, remote and total myocardium area were manually segmented in LGE images by a single observer (Lopez) with experience in cardiac LGE (approximately 3 years). Automated segmentation was not attempted. MTR scar volume was determined by thresholding in each separate animal as follows: (1) after manually selecting a remote (myocardium) area in the MTR map, mean and standard deviations (σ) were calculated; (2) a mask (m1) of the entire myocardium was manually drawn using the MT-weighted dataset (intrinsically co-registered to the MTR map); (3) finally, MTR voxels under the threshold mean-2σ and within m1 were automatically selected as scar volume. The overlap was defined as the number of coincidences between LGE and MTR scar voxels, divided by the total number of LGE scar voxels:
The false positive percentage was calculated using the number of coincidences between MTR scar voxels and LGE remote voxels:
Healthy subjects study
Ten healthy human subjects (29 ± 3 years, two males) were recruited for a proof-of-concept evaluation of the proposed sequence with translational and non-rigid motion corrections. Each subject was imaged twice, using bSSFP (TR/TE = 3.2/1.4 ms, FA = 70°, BW = 925 Hz/px) and SPGR (TR/TE = 3.8/1.6 ms, FA = 15°, BW = 500 Hz) imaging modules. To avoid artefacts observed at the liver interface, the MT preparation was of equivalent power deposition but higher off resonance frequency than that of the animal study (see Supplementary data, Fig. 1). The modified MT preparation parameters were: MT flip angle = 800˚, ΔF = 3000 Hz and pulse repetitions n = 20. Other imaging parameters included: 3D coronal orientation, FoV = 300 × 300 × 112 mm3, acquired resolution = 1.4 × 1.4 × 4 mm, reconstructed resolution = 1.4 mm3, 100% respiratory gating efficiency, and nominal scan time of 9:02 min at 60 bpm.
A data flow scheme for the image analysis pipeline is shown in Fig. 2b. All datasets were reformatted in short axis orientation, using tri-linear interpolation. A 2D Gaussian filter was applied (kernel size 5 pixel, σ = 3 pixel) on every slice of the MTR maps to reduce the noise and improve visualization.
Manual segmentation was performed for the three left ventricular slices (basal, mid and apical) using the American Heart Association (AHA) 16-segment model of myocardial segmentation [32].
The SPGR and bSSFP variants of the sequence were compared using the following metrics: (I) average global MTR and average MTR per segment; (II) spatial variation of MTR in each segment, calculated as the ratio between the standard deviation and the mean MTR (expressed as a percentage); (III) contrast ratio (CR) between blood MTR and myocardial MTR.
MTR mean values and spatial variability were also calculated in regions of interest (ROIs) in the liver and pectoral muscle to compare with myocardial values and to assess the impact of different types of motion in the spatial variability of MTR.
Based on the bSSFP results in simulations and phantom experiments, the quality of coronary vein visualization was evaluated in the SPGR datasets only, using vessel sharpness (VS) and contrast-to-noise ratio (CNR) measurements. Translational vs non-rigid motion correction approaches were compared using a reformatted 2D representation of the 3D course of the cardiac veins [33]. VS was calculated for the posterior branch of the cardiac vein (PCV) and the great cardiac vein (GCV) from the reformatted images. VS was defined as the average intensity gradient along the edges normalized to the signal intensity of the centre of the vessel. Contrast-to-noise-ratio (CNR) between blood and myocardium was obtained from the reformatted images using:
where \({S}_{\mathrm{B}\mathrm{l}\mathrm{o}\mathrm{o}\mathrm{d}}\) and \({S}_{\mathrm{M}\mathrm{y}\mathrm{o}}\) are the mean signal intensity in blood and myocardium ROI, respectively, and \({\sigma }_{\mathrm{L}\mathrm{u}\mathrm{n}\mathrm{g}\mathrm{s}}\) is the standard deviation in a small region of the lungs with no vessels.
Results
Numerical simulations and phantom study
Bloch-simulated MTR sensitivity to B0 inhomogeneity in myocardium-like tissue with both imaging modules (bSSFP vs SPGR) is shown in Fig. 3a and b, respectively. SPGR yielded an almost flat MTR response with less than 3% variation across the studied B0 range. The bSSFP module led to generally higher MTR values, but had a strong sensitivity to B0 inhomogeneity with approximately 20% variation towards the 1/2TR bands at ± 150 Hz.
MTR sensitivity curves with respect to the relaxation rates and exchange-related parameters are shown in Fig. 4, both for SPGR and bSSFP imaging modules. MTR sensitivity to \({T}_{1}^{A}\) and \({T}_{2}^{A}\) using SPGR was lower than bSSFP (\({T}_{2}^{A}\): < 2.3% vs < 4.3%; \({T}_{1}^{A}\): < 0.7% vs < 2.5%, respectively) within the simulated range of myocardial relaxation rates (Fig. 4a). MTR values were found to increase as a function of PSR and R (Fig. 4b). PSR proved to be the major contributor to MTR, showing a near-linear dependency within the range associated with human muscle (PSR = 5–15%). MTR dependency of the exchange rate was slowly increasing (less than 7%) within a range of R = 20–70 Hz. The imaging module (bSSFP vs. SPGR) was found to have little impact on the shape of MTR as a function of R and PSR, as observed in Fig. 4b.
The effects of ∆F and MT flip angle on MTR values using SPGR on a 2.5% agar sample are shown in Fig. 5a and b, respectively. MTR values showed a strong non-linear frequency dependency for low ∆F (< 1 kHz) and a less strong dependency at higher ∆F. The MTR dependency on the flip angle was near linear for flip angles < 800° with a stronger flip angle dependency for lower off-resonance frequencies. The phantom measurements and simulated data were in good agreement over a wide range of ∆F (> 0.4 Hz and < 8 kHz) and MT flip angles (> 360° and < 800°). MTR maps obtained with bSSFP and SPGR using three different flip angles and fixed ∆F = 400 Hz are shown in Fig. 5c. The MTR maps acquired with bSSFP showed multiple artefacts, likely associated with B0 inhomogeneity. The SPGR-based MTR maps were homogenous throughout but noisier than bSSFP.
Animal study
MTR decrease was found in regions associated with scar and was in good agreement with the presence of LGE in all three animals. MTR maps allowed accurate localization and visualization of the scar (see Fig. 6). Mean MTR values in remote myocardium were 25.1 ± 1.7%, while mean MTR values in scar were 16.8 ± 1.9%. Voxel-to-voxel comparison with LGE showed a mean overlap of 62.5 ± 19.2% and a mean false positive percentage of 9.6 ± 6.0% over all animals (n = 3).
Healthy subjects
The bSSFP module yielded higher CNR than SPGR (13.9 ± 1.2, vs. 8.1 ± 0.7, p < 0.05) in the MT-prepared datasets. CR measurements in the MTR maps (between blood and myocardium) showed no statistically significant difference between the two imaging modules [bSSFP: 2.50 ± 0.16 vs. SPGR: 2.48 ± 0.32, p = not statistically significant (NS)].
Representative MTR maps and myocardial segment mean values across all subjects using SPGR and bSSFP are shown in Fig. 7. The MTR maps acquired with bSSFP demonstrated increased MTR values towards the lateral and inferior regions. This may be due to B0 inhomogeneity at the lung–myocardium interface. A typical artefact in this region is shown in Fig. 7 (middle column). Whole heart myocardium MTR averaged over all subjects and obtained after translational motion correction was 39.2 ± 1.9% using bSSFP and 37.0 ± 2.1% using SPGR. Spatial variation of MTR was 19.3 ± 2.9% vs. 15.7 ± 2.1% (p = 0.01) for bSSFP vs. SPGR, respectively. SPGR led to reduced MTR variability between segments compared to bSSFP (8.0 ± 2.3% vs 10.3 ± 1.9%, p = 0.07), as seen in Fig. 7 (right column). Mean MTR values and spatial variation did not show statistically significant difference between translational and non-rigid motion correction, as shown in Table 1.
MTR values in pectoral muscle showed significantly reduced spatial variability compared to myocardium: MTR = 43.8 ± 1.7 (spatial variability: 9.5 ± 3.4%, p < 0.01) and MTR = 41.0 ± 2.4 (spatial variability: 5.8 ± 3.6%, p < 0.01), for bSSFP and SPGR, respectively. Liver MTR measurements showed similar spatial variability compared to myocardium, with MTR = 32.3 ± 2.9 (spatial variability: 18.4 ± 4.3%, p = 0.4) and MTR = 29.6 ± 3.5 (spatial variability: 15.5 ± 0.8%, p = 0.7), for bSSFP and SPGR, respectively. One reason for this similarity may be that the liver and the heart experience similar extent of respiratory motion.
The use of translational motion correction allowed good depiction of the PCV and GCV. The non-rigid motion correction improved visualization of the entire cardiac anatomy with respect to the translational motion correction. This was observed in an increase in vessel sharpness in the GCV (40.8 ± 2.0% vs 32 ± 2.5%, p < 0.05) and the PCV (34.1 ± 3.2% vs 30.0 ± 1.7%, p < 0.05). Three examples from representative subjects are shown in Fig. 8.
Discussion
A motion-corrected free-breathing 3D whole heart MTR mapping sequence was developed and successfully validated in phantoms, healthy subjects and pigs. MTR maps allowed the localization of myocardial fibrosis without the injection of a contrast agent in a pig model of myocardial infarction. Significantly lower MTR values were found in areas that corresponded with hyperintense signal on LGE. In human healthy subjects, MT-prepared images reconstructed with non-rigid motion correction enabled the visualization of the cardiac veins with vessel sharpness between 30 and 40% along the main cardiac veins.
MTR values found in an agar-based phantom and healthy subjects were overall consistent with Bloch simulations using a two-pool exchange model, which suggested increased MT effects associated with increased pool size ratio. Though a small discrepancy was observed in Fig. 5b, at low off-resonance frequency (Δ = 400 Hz) and high flip angles, this was likely due to residual on-resonance saturation of the free pool not being included in the model, which seems to “inflate” the measured MTR increasingly as the flip angle increases.
In accordance with the simulations, MTR myocardial values obtained with an SPGR imaging module had less spatial variability compared to those obtained with bSSFP. This result was in agreement with a study of coronary vein imaging [17] that found that SSFP sequences were more prone to artefacts than SPGR, especially in regions surrounding deoxygenated blood (e.g. coronary veins), likely because of the spread of the resonant frequency. A similar effect was discussed in a study of coronary artery imaging [34], which highlights the challenges in finding a good shimming solution for the heart due to, at least in part, cardiac and respiratory motion, blood flow, chemical shift, and susceptibility variations at air–tissue interfaces.
In healthy subjects, the spatial variability of myocardial MTR was higher than in static tissues such as pectoral muscle. This suggests that respiratory motion might have an impact on spatial variability of MTR and that residual respiratory motion may have been present in the MTR maps. While non-rigid respiratory motion correction was shown to improve vessel sharpness in the MT-prepared dataset, the standard deviation of myocardial MTR was not significantly improved compared to translational motion correction only. The use of more advanced navigation techniques such as 3D iNAVs [35, 36] may help to tackle unaccounted respiratory motion. Error or bias associated with non-rigid motion within a respiratory phase may be reduced upon optimization of the size and number of bins which, in this study, were based on values previously obtained by our research group [20] for the visualization of coronary vessels. The differences between bSSFP and SPGR also suggest that field inhomogeneity may play a role in increased spatial variability. The individual contributions of residual motion and field inhomogeneity to MTR spatial variability may be assessed with an MT-prepared breath-held single-shot sequence in future studies.
Six-week-old scar in pigs was easily visualized and was characterized by a decrease in MTR. These results are in good agreement with previous studies which reported decreased MTR values in porcine heart 4 weeks after MI [37] and acute MI in humans [18, 38]. In the latter setting, it was hypothesized that the presence of oedema leads to an increase in the absolute size of the free pool and thus a relative decrease in the MT effect and MTR. In a post-mortem study that compared MTR with histology [39], Crooijmans et al. found a relationship between increased MTR and fibrotic tissue, as well as a relationship between decreased MTR and inflammatory response, due to granulocyte infiltration or oedema. In another study in pigs performed 6 weeks after coronary occlusion, Dhanjal et al. showed massive cellularity (stromal cells such as fibroblasts and myofibroblasts), vascularity and heterogeneity in the scarred zones [40], which might help to explain the significant decrease in MTR associated with scar in our experiments. A histopathology experiment in conjunction with MTR imaging could help to support this hypothesis in future studies.
Another contrast-free approach to probe the spins with restricted motion is the T1-ρ technique, which explores spin–lattice relaxation within the rotating frame. Multiple studies have found increased T1-ρ in knee cartilage in patients with osteoarthritis due to the loss of proteoglycans and collagen (type II) integrity [41, 42], i.e. a decrease in the size of the macromolecular pool. However, 8 weeks post-MI, pigs also showed increased T1-ρ values associated with collagenous (mostly type I and III) scar [43, 44] where the size of the extracellular matrix (and macromolecular pool) was expected to have increased. In a study with acute MI patients, Muthupillai et al. suggested that changes in T1-ρ in the infarct zone were also associated with the loss in macromolecular content due to myocyte death [45].
At least two competing processes that may increase or decrease the size of the bound pool are at play in cardiac remodelling after MI, namely, the growth of the extracellular matrix and the death of protein-rich cardiomyocytes, respectively. The presence of connective tissue or oedema within the fibrotic scar may also increase the size of the free pool. Our results in 6-week-old (post MI) scar showed that MTR was significantly decreased, suggesting that the proposed MT preparation might be more sensitive to myocyte death rather than the known increase in collagen content associated with chronic infarct [46].
This interpretation would greatly benefit from data at various stages of the cardiac remodelling process to assess the specificity and utility of the technique in clinical practice. In an experimental mouse model, Vandsburger et al. reported increasing MT effects after induced MI from day 7 to 21 with a cine CEST technique [47]. To the best of our knowledge, there are no longitudinal studies in large animals that show the evolution of MTR or MT effects along the time course of the cardiac remodelling process beyond 6–8 weeks after MI.
Limitations
The conflation of bound pool size, free pool size, exchange rate and all the relaxation rates into a single parameter, i.e. the MTR, may hinder the applicability of the technique within clinical settings, where oftentimes the aetiology of the scar may be unknown or multi-pronged. In these cases, a quantitative approach using a multi-parameter MT model could be more appropriate.
The number of off-line post-processing steps and setup parameters may slow down widespread clinical adoption; however, more automated or end-product frameworks that apply many of these same techniques are currently being developed by the present research group and others.
The small number of pigs used in this study was a limitation; however, the results showed consistency across all three cases. Other limitations included the relatively long scan time and anisotropic resolution in the human subjects. The anisotropic resolution affected image quality, specifically when reformatting to orientations other than coronal. The resolution was compromised to maintain a short scan time (< 10 min) that was clinically appealing. Future work might benefit from isotropic resolution paired with an accelerated acquisition framework.
Conclusion
We have developed a non-contrast high-resolution 3D sequence that allows calculation of magnetization transfer ratio (MTR) maps for the assessment of myocardial scar and visualization of cardiac veins across the whole heart. Good agreement was found between MTR and LGE in a small cohort of pigs with 6-week-old scar. Further studies are warranted to fully characterize the potential of MT for imaging of myocardial fibrosis.
References
Bruder O, Wagner A, Jensen CJ, Schneider S, Ong P, Kispert EM, Nassenstein K, Schlosser T, Sabin GV, Sechtem U, Mahrholdt H (2010) Myocardial scar visualized by cardiovascular magnetic resonance imaging predicts major adverse events in patients with hypertrophic cardiomyopathy. J Am Coll Cardiol 56(11):875–887
Kelle S, Roes SD, Klein C, Kokocinski T, de Roos A, Fleck E, Bax JJ, Nagel E (2009) Prognostic value of myocardial infarct size and contractile reserve using magnetic resonance imaging. J Am Coll Cardiol 54(19):1770–1777
Klem I, Weinsaft JW, Bahnson TD, Hegland D, Kim HW, Hayes B, Parker MA, Judd RM, Kim RJ (2012) Assessment of myocardial scarring improves risk stratification in patients evaluated for cardiac defibrillator implantation. J Am Coll Cardiol 60(5):408–420
Shetty AK, Duckett SG, Ginks MR, Ma Y, Sohal M, Bostock J, Kapetanakis S, Singh JP, Rhode K, Wright M, O'Neill MD, Gill JS, Carr-White G, Razavi R, Rinaldi CA (2013) Cardiac magnetic resonance-derived anatomy, scar, and dyssynchrony fused with fluoroscopy to guide LV lead placement in cardiac resynchronization therapy: a comparison with acute haemodynamic measures and echocardiographic reverse remodelling. Eur Heart J Cardiovasc Imaging 14(7):692–699
Flett AS, Hasleton J, Cook C, Hausenloy D, Quarta G, Ariti C, Muthurangu V, Moon JC (2011) Evaluation of techniques for the quantification of myocardial scar of differing etiology using cardiac magnetic resonance. JACC Cardiovasc Imaging 4(2):150–156
Mewton N, Liu CY, Croisille P, Bluemke D, Lima JA (2011) Assessment of myocardial fibrosis with cardiovascular magnetic resonance. J Am Coll Cardiol 57(8):891–903
Kim RJ, Chen EL, Lima JA, Judd RM (1996) Myocardial Gd-DTPA kinetics determine MRI contrast enhancement and reflect the extent and severity of myocardial injury after acute reperfused infarction. Circulation 94(12):3318–3326
Kanda T, Fukusato T, Matsuda M, Toyoda K, Oba H, Kotoku J, Haruyama T, Kitajima K, Furui S (2015) Gadolinium-based contrast agent accumulates in the brain even in subjects without severe renal dysfunction: evaluation of autopsy brain specimens with inductively coupled plasma mass spectroscopy. Radiology 276(1):228–232
Laurent D, Wasvary J, Yin J, Rudin M, Pellas TC, O'Byrne E (2001) Quantitative and qualitative assessment of articular cartilage in the goat knee with magnetization transfer imaging. Magn Reson Imaging 19(10):1279–1286
Phinikaridou A, Andia ME, Saha P, Modarai B, Smith A, Botnar RM (2013) In vivo magnetization transfer and diffusion-weighted magnetic resonance imaging detects thrombus composition in a mouse model of deep vein thrombosis. Circ Cardiovasc Imaging 6(3):433–440
Wang C, Witschey W, Goldberg A, Elliott M, Borthakur A, Reddy R (2010) Magnetization transfer ratio mapping of intervertebral disc degeneration. Magn Reson Med 64(5):1520–1528
Wolff SD, Balaban RS (1989) Magnetization transfer contrast (MTC) and tissue water proton relaxation in vivo. Magn Reson Med 10(1):135–144
Wolff SD, Eng J, Balaban RS (1991) Magnetization transfer contrast: method for improving contrast in gradient-recalled-echo images. Radiology 179(1):133–137
McDaniel JD, Ulmer JL, Prost RW, Franczak MB, Jaradeh S, Hamilton CA, Mark LP (1999) Magnetization transfer imaging of skeletal muscle in autosomal recessive limb girdle muscular dystrophy. J Comput Assist Tomogr 23(4):609–614
Stoeck CT, Han Y, Peters DC, Hu P, Yeon SB, Kissinger KV, Goddu B, Goepfert L, Manning WJ, Kozerke S, Nezafat R (2009) Whole heart magnetization-prepared steady-state free precession coronary vein MRI. J Magn Reson Imaging 29(6):1293–1299
Botnar RM, Stuber M, Danias PG, Kissinger KV, Manning WJ (1999) Improved coronary artery definition with T2-weighted, free-breathing, three-dimensional coronary MRA. Circulation 99(24):3139–3148
Nezafat R, Han Y, Peters DC, Herzka DA, Wylie JV, Goddu B, Kissinger KK, Yeon SB, Zimetbaum PJ, Manning WJ (2007) Coronary magnetic resonance vein imaging: imaging contrast, sequence, and timing. Magn Reson Med 58(6):1196–1206
Weber OM, Speier P, Scheffler K, Bieri O (2009) Assessment of magnetization transfer effects in myocardial tissue using balanced steady-state free precession (bSSFP) cine MRI. Magn Reson Med 62(3):699–705
Germain P, El Ghannudi S, Labani A, Jeung MY, Gangi A, Ohlmann P, Roy C (2018) A dual flip angle 3D bSSFP magnetization transfer-like method to differentiate between recent and old myocardial infarction. J Magn Reson Imaging 47(3):798–808
Prieto C, Doneva M, Usman M, Henningsson M, Greil G, Schaeffter T, Botnar RM (2015) Highly efficient respiratory motion compensated free-breathing coronary MRA using golden-step Cartesian acquisition. J Magn Reson Imaging 41(3):738–746
Henningsson M, Koken P, Stehning C, Razavi R, Prieto C, Botnar RM (2012) Whole-heart coronary MR angiography with 2D self-navigated image reconstruction. Magn Reson Med 67(2):437–445
Cruz G, Atkinson D, Henningsson M, Botnar RM, Prieto C (2017) Highly efficient nonrigid motion-corrected 3D whole-heart coronary vessel wall imaging. Magn Reson Med 77(5):1894–1908
Bracewell R, Chang K, Jha A, Wang Y (1993) Affine theorem for two-dimensional Fourier transform. Electron Lett IEE 29:304–304
Modat M, Ridgway GR, Taylor ZA, Lehmann M, Barnes J, Hawkes DJ, Fox NC, Ourselin S (2010) Fast free-form deformation using graphics processing units. Comput Methods Programs Biomed 98(3):278–284
Batchelor PG, Atkinson D, Irarrazaval P, Hill DL, Hajnal J, Larkman D (2005) Matrix description of general motion correction applied to multishot images. Magn Reson Med 54(5):1273–1280
Sled JG, Pike GB (2001) Quantitative imaging of magnetization transfer exchange and relaxation properties in vivo using MRI. Magn Reson Med 46(5):923–931
Morrison C, Stanisz G, Henkelman RM (1995) Modeling magnetization transfer for biological-like systems using a semi-solid pool with a super-Lorentzian lineshape and dipolar reservoir. J Magn Reson B 108(2):103–113
Ropele S, Seifert T, Enzinger C, Fazekas F (2003) Method for quantitative imaging of the macromolecular 1H fraction in tissues. Magn Reson Med 49(5):864–871
Stikov N, Perry LM, Mezer A, Rykhlevskaia E, Wandell BA, Pauly JM, Dougherty RF (2011) Bound pool fractions complement diffusion measures to describe white matter micro and macrostructure. Neuroimage 54(2):1112–1121
Portnoy S, Stanisz GJ (2007) Modeling pulsed magnetization transfer. Magn Reson Med 58(1):144–155
Tschabrunn CM, Roujol S, Nezafat R, Faulkner-Jones B, Buxton AE, Josephson ME, Anter E (2016) A swine model of infarct-related reentrant ventricular tachycardia: electroanatomic, magnetic resonance, and histopathological characterization. Heart Rhythm 13(1):262–273
Cerqueira MD, Weissman NJ, Dilsizian V, Jacobs AK, Kaul S, Laskey WK, Pennell DJ, Rumberger JA, Ryan T, Verani MS, American Heart Association Writing Group on Myocardial S, Registration for Cardiac I (2002) Standardized myocardial segmentation and nomenclature for tomographic imaging of the heart. A statement for healthcare professionals from the Cardiac Imaging Committee of the Council on Clinical Cardiology of the American Heart Association. Circulation 105(4):539–542
Etienne A, Botnar RM, Van Muiswinkel AM, Boesiger P, Manning WJ, Stuber M (2002) "Soap-Bubble" visualization and quantitative analysis of 3D coronary magnetic resonance angiograms. Magn Reson Med 48(4):658–666
Deshpande VS, Shea SM, Li D (2003) Artifact reduction in true-FISP imaging of the coronary arteries by adjusting imaging frequency. Magn Reson Med 49(5):803–809
Luo J, Addy NO, Ingle RR, Baron CA, Cheng JY, Hu BS, Nishimura DG (2017) Nonrigid motion correction with 3D image-based navigators for coronary MR angiography. Magn Reson Med 77(5):1884–1893
Powell J, Prieto C, Henningsson M, Koken P, Botnar R (2014) CMRA with 100% navigator efficiency with 3D self navigation and interleaved scanning. J Cardiovasc Magn Reson 16(1):O8
van Oorschot J (2016) Detection of myocardial infarcts without contrast agent injection: comparison of spin-lock with magnetization transfer MR imaging. In: ISMRM 24th Annual Meeting and Exhibition, Singapore, 22 April 2016
Stromp TA, Leung SW, Andres KN, Jing L, Fornwalt BK, Charnigo RJ, Sorrell VL, Vandsburger MH (2015) Gadolinium free cardiovascular magnetic resonance with 2-point Cine balanced steady state free precession. J Cardiovasc Magn Reson 17:90
Crooijmans HJ, Ruder TD, Zech WD, Somaini S, Scheffler K, Thali MJ, Bieri O (2014) Cardiovascular magnetization transfer ratio imaging compared with histology: a postmortem study. J Magn Reson Imaging 40(4):915–919
Dhanjal TS, Lellouche N, von Ruhland CJ, Abehsira G, Edwards DH, Dubois-Rande JL, Moschonas K, Teiger E, Williams AJ, George CH (2017) Massive accumulation of myofibroblasts in the critical isthmus is associated with ventricular tachycardia inducibility in post-infarct swine heart. JACC Clin Electrophysiol 3(7):703–714
Li X, Benjamin Ma C, Link TM, Castillo DD, Blumenkrantz G, Lozano J, Carballido-Gamio J, Ries M, Majumdar S (2007) In vivo T(1rho) and T(2) mapping of articular cartilage in osteoarthritis of the knee using 3 T MRI. Osteoarthr Cartil 15(7):789–797
Witschey WR, Borthakur A, Fenty M, Kneeland BJ, Lonner JH, McArdle EL, Sochor M, Reddy R (2010) T1rho MRI quantification of arthroscopically confirmed cartilage degeneration. Magn Reson Med 63(5):1376–1382
van Oorschot JW, El Aidi H, JansenofLorkeers SJ, Gho JM, Froeling M, Visser F, Chamuleau SA, Doevendans PA, Luijten PR, Leiner T, Zwanenburg JJ (2014) Endogenous assessment of chronic myocardial infarction with T(1rho)-mapping in patients. J Cardiovasc Magn Reson 16:104
Witschey WR, Pilla JJ, Ferrari G, Koomalsingh K, Haris M, Hinmon R, Zsido G, Gorman JH 3rd, Gorman RC, Reddy R (2010) Rotating frame spin lattice relaxation in a swine model of chronic, left ventricular myocardial infarction. Magn Reson Med 64(5):1453–1460
Muthupillai R, Flamm SD, Wilson JM, Pettigrew RI, Dixon WT (2004) Acute myocardial infarction: tissue characterization with T1rho-weighted MR imaging—initial experience. Radiology 232(2):606–610
Hervas A, Ruiz-Sauri A, de Dios E, Forteza MJ, Minana G, Nunez J, Gomez C, Bonanad C, Perez-Sole N, Gavara J, Chorro FJ, Bodi V (2016) Inhomogeneity of collagen organization within the fibrotic scar after myocardial infarction: results in a swine model and in human samples. J Anat 228(1):47–58
Vandsburger M, Vandoorne K, Oren R, Leftin A, Mpofu S, Delli Castelli D, Aime S, Neeman M (2015) Cardio-chemical exchange saturation transfer magnetic resonance imaging reveals molecular signatures of endogenous fibrosis and exogenous contrast media. Circ Cardiovasc Imaging 8(1):e002180
Acknowledgements
This work was funded by EPSRC grants EP/P001009/1 and EP/P007619/1. Animal experiments were funded by a Wellcome Trust Health Innovation Challenge Fund grant (HICF-R10-698) and supported by the Wellcome/EPSRC Centre for Medical Engineering at King’s College London [WT 203148/Z/16/Z] and by the Department of Health through a National Institute of Health Research comprehensive Biomedical Research Centre award to Guy’s and St Thomas’ NHS Foundation Trust in partnership with King’s College London and King’s College Hospital NHS Foundation Trust. Karina Lopez is funded by the King’s College London & Imperial College London EPSRC Centre for Doctoral Training in Medical Imaging (EP/L015226/1), in conjunction with Siemens Healthcare Limited. Dr Mukherjee is a recipient of a Fellowship from the National Institute of Health Research comprehensive Biomedical Research Centre at Guy’s and St Thomas’ NHS Foundation Trust and King’s College London. Dr Whitaker is a recipient of a Fellowship award from the Medical Research Council (MRC CRTF N001877/1).
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KL: design, acquisition of all data related to phantom and human experiments, analysis and interpretation of all data and drafting of manuscript. RN: design, acquisition of data and critical revision. RKM: acquisition of data related to the animal study and critical revision. JW: acquisition of data related to the animal study and critical revision. AP: acquisition of data related to the phantom experiments and critical revision. RR: critical revision. CP: conception and design of data acquisition and motion correction, acquisition of data and critical revision. SR: design and critical revision. RB: conception, design, data acquisition, interpretation of data and critical revision. To clarify, here, acquisition of data involves the collection of data itself as well as the development of techniques and/or samples specially tailored for the collection of data in this study.
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R. Neji is an employee of Siemens Heathcare Limited. All other authors declare that they have no conflict of interest.
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All procedures performed in studies involving human participants were in accordance with the ethical standards of our institutional review board (IRB) and with the 1964 Helsinki Declaration and its later amendments or comparable ethical standard. Informed consent was obtained from all individual participants included in the study. All applicable international, national, and institutional guidelines for the care and use of animals were followed. Animal studies complied with the French law and were performed at the Institut de Chirurgie Guidée par l’image (IHU), Strasbourg, France. The experimental protocol was approved by the local institutional animal care and ethics committee and was compliant with the Guiding Principles for the Use and Care of Animals published by the National Institutes of Health (NIH Publication no. 85-23, Revised 1996).
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López, K., Neji, R., Mukherjee, R.K. et al. Contrast-free high-resolution 3D magnetization transfer imaging for simultaneous myocardial scar and cardiac vein visualization. Magn Reson Mater Phy 33, 627–640 (2020). https://doi.org/10.1007/s10334-020-00833-9
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DOI: https://doi.org/10.1007/s10334-020-00833-9