Association between native T1 mapping of the kidney and renal fibrosis in patients with IgA nephropathy

This was a prospective, single-centre, observational pilot study conducted in the UK. The NHS Health Research Authority provided ethical approval and all participants gave written informed consent. All adult patients with biopsy proven IgAN with independent renal function and seen in within the last 12 months in outpatient clinics were given patient information sheets about the project, those who replied were contacted by research team on a first come first serve basis. Patients with renal transplantation or on renal replacement therapy were excluded. Twenty patients with biopsy-proven IgAN were recruited from general nephrology clinics at the Leicester General Hospital. In addition, 10 healthy subjects with no known kidney disease were recruited through local advertising within the hospital. Ten patients with IgAN underwent repeat MRI scan within 14 days of initial scan, to assess test-retest reproducibility of the technique. Patients were not fasted, and no instructions given regarding fluid intake prior to the scan.

All participants underwent the following investigations during a single visit: blood pressure, height and weight measurement, blood sampling for renal function, urine collection for protein creatinine ratio and an MRI scan as described below. Estimated glomerular filtration rate (e-GFR) was calculated using the Chronic Kidney Disease Epidemiology Collaboration (CKD-EPI) formula. Previous renal biopsy report was reviewed and a recognised IgAN morphological biopsy classification was applied Oxford-MEST classification [20, 21].

MRI of both kidneys was performed on a 3-Tesla scanner (Magnetom Skyra, Siemens AG, Healthcare Sector, Erlangen, Germany), using an 18-channel phased-array body coil, and an identical protocol in patients and controls. Following localisers, T1 imaging was undertaken using a prototype, breath-held, end-expiratory, ECG-gated single-shot Modified Look-Locker Inversion Recovery (MOLLI) sequence [22] with the 3(3)3(3)5 sampling pattern, and the following typical parameters: slice thickness 5 mm, field of view 300 × 400 mm, flip angle 32°, minimum TI 120 ms, inversion-time increment 80 ms. MOLLI images of both kidneys were acquired in coronal plane, with the slice planned through the centre of the renal pelvis, after applying a tight shim. If artefacts were present, imaging was repeated after increasing the field of view or swapping the phase encoding direction. This was followed by acquisition of three axial slices covering the superior, mid and inferior poles of each kidney, ensuring the presence of cortex and medulla. The MOLLI sequence produces a series of 11 images with different inversion times, with data collected over 17 heart-beats. The Siemens software (Syngo MR D13) then employs inline reconstruction software to produce a T1 parametric map, with pixel-by-pixel computation of the T1 values [22].

For measurement of bipolar kidney length a T1 volume-interpolated breath hold examination (VIBE) sequence was used. Slices were positioned in the true axial plane to include both kidneys in a single breath-hold, with the following typical parameters: slice thickness 2.5 mm, no inter-slice gap, field of view 300 × 400 mm, flip angle 9°.

Renal native T1 parametric maps were used to calculate native T1, which was performed using CMR42 software (Circle Cardiovascular Imaging, Calgary, Alberta, Canada). On the coronal images, three regions of interest were manually drawn in the renal cortex, covering the superior, middle and inferior poles (Fig. 1). Regions of interest were also drawn in the axial slices to quantify the average cortical T1 time in the superior, middle and inferior poles of each kidney (Fig. 1). Using the T1 VIBE sequence a 3D reconstructed image of each kidney was acquired in the true bipolar long-axis. The true maximal bipolar kidney length could then be defined.

Nineteen patients had analysable coronal T1 maps for both kidneys. Eighteen patients had analysable axial T1 maps for both kidneys. Mean cortical native T1 time for both coronal and axial images for patients with IgAN were significantly longer than for control subjects (1542 ± 107 ms versus 1443 ± 80 ms, p = 0.017 and 1540 ms ± 110 ms versus 1446 ± 88 ms for controls, p = 0.038 respectively) (Fig. 2). There were no differences in mean cortical T1 time between coronal and axial images for patients with IgAN (1541 ± 113 ms versus 1540 ± 110 ms, p = 0.906), or for control subjects (1438 ± 83 ms versus 1446 ± 88 ms, p = 0.531).

The mean time between the two MRI scans for patients undertaking the test-retest reproducibility study was 5.3 ± 5.8 days. One patient had multiple cysts on one kidney and was excluded from the analysis. Bland-Altman analysis of repeated sagittal and coronal native T1 maps did not reveal any evidence of systematic bias with all data plots falling within 95% confidence intervals (Fig. 3). There were strong correlations between test-retest renal native T1 times for sagittal and coronal images (r = 0.96 and r = 0.93 respectively) with excellent test-retest reproducibility (CoV of 2.9 and 3.68% respectively).

There were significant correlations between cortical native T1 time and eGFR, as well as proteinuria (r = − 0.444, p = 0.016 and r = 0.533, p = 0.003 respectively) (Fig. 3). Patients with IgAN who had an eGFR decline of > 2 ml/min/year over the preceding 24 months tended to have increased cortical coronal native T1 time compared to those with an eGFR decline of < 2 ml/min/year (1615 ± 135 ms versus 1516 ± 87 ms, p = 0.068). There were no significant correlations between age, haemoglobin or blood pressure and native T1 time. (Scatter plots to be added).

In IgAN patients, the mean cortical native T1 time was marginally reduced in patients with a histological ‘T’-score of 0, compared to patients with a histological ‘T’-score of > 0, though not to statistical significance (1496 ± 105 ms versus 1575 ± 106 ms, p = 0.131). There was no significant difference between native T1 time for patients with IgAN who had an ‘S’ score of 0 on histology, compared to those with an ‘S’-score of > 0 on histology (1507 ± 53 ms versus 1565 ± 136 ms, p = 0.402).

The sample size of this pilot study is relatively small, although even with small numbers we have been able to demonstrate the potential utility of this technique. One of the major advantages of MRI scanning are its multi-parametric capabilities [17]. Previous studies that have looked at native T1 mapping in patients with renal disease have done so as part of a more comprehensive MRI protocol that has included measures such as arterial spin labelling, diffusion-weighted imaging, T2* imaging and renal artery and vein blood flow [17, 23]. We deliberately focussed on native T1 mapping in this study due to local expertise in the acquisition and the analysis of native T1 mapping [15, 22], but this does not mean future studies should not explore the roles of other MRI-derived measures. We deliberately focussed on patients with a single, defined renal disease, proven histologically to minimise confounding factors that may influence native T1 times. Fibrosis is the common end-point of many parenchymal renal diseases. Whilst the findings of this study are not automatically generalizable to all renal diseases, the potential for native T1 to characterise renal cortical fibrosis in related progressive nephropathies is clear and should and tested in other, defined, disease populations across the spectrum of CKD, preferably with histology. Another limitation of this study is the time between renal biopsy and the time of scan, but this study was not powered or designed to assess this, and findings are only exploratory in nature. Future studies should seek to conduct renal biopsy and MRI scan at the same time points.