Simplifying [¹⁸F]GE-179 PET: are both arterial blood sampling and 90-min acquisitions essential?

An 83-region grey-matter-only ROI map was produced for each participant using multi-atlas propagation with enhanced registration (MAPER) [8]. MAPER is an automated anatomical segmentation method that involves co-registering the participant’s T1-weighted magnetic resonance image (MRI) to that of 30 healthy controls that have already been manually labelled (the atlases). This yields individual anatomical segmentations that are fused via vote-rule decision [9] to produce the ROI map (see Additional file 1: Figure S2).

PET data pre-processing and the generation of parent plasma input functions were performed as previously described [2, 6]. Emission data had been reconstructed using Fourier rebinning (FORE [10]) and 2D-filtered backprojection (FBP; ramp filter kernel 2.0 mm full width at half maximum).

The fraction of plasma radioactivity attributable to the parent [¹⁸F]GE-179 had been fitted to a sigmoid function normalised to unity at 0 min using CLICKFIT in-house software version 1.7 (Hinz R, Cunningham VJ, Imaging Research Solutions Limited, London, UK) running in MATLAB 2014a (The MathWorks, Natick, MA, USA.).

The original, continuous parent plasma input functions (ppIFs) were derived as follows [11]: (1) cross-calibration of continuous and discrete whole blood radioactivity concentrations, (2) multiplication of the cross-calibrated continuous (0–15 min) whole blood radioactivity concentrations by the plasma-over-whole-blood ratio, (3) spline interpolation of the continuous (0–15 min) plasma radioactivity concentrations curve over the additional discrete measurements, and (4) multiplication of the continuous (0–90 min) plasma radioactivity curve by the parent fraction.

Voxelwise “classic” SA [12] was performed using Piwave 8.0 [13], using time constants of 5 s (fast boundary = 0.2 s⁻¹) and 5100 s (slow boundary = 0.000196 s⁻¹). We confirmed the suitability of “classic” voxelwise SA by demonstrating that the resultant original ppIF-derived V_Ts were strongly correlated with original ppIF-derived V_Ts derived from compartmental modelling (Additional file 1).

SUV images (see [11]) were calculated for all 10-min epochs from 20–30 to 80–90 min from decay-corrected summation images, using MICKPM (version 5.4 software, running in MATLAB (The MathWorks Inc., Cambridge, UK)). “MICKPM” (Modelling, Input functions and Compartmental Kinetics—Parametric Maps) is a quantitative PET analysis software that is available on request from Rainer Hinz (Wolfson Molecular Imaging Centre, University of Manchester; rainer.hinz@manchester.ac.uk). Epochs of 30–60 and 60–90 min were also tested, but yielded very similar results (data not shown).

The generation of PBIFs can be split into “magnitude normalisation” and “scaling” stages, described below.

After controlling for weight and injected dose, we identified a near-significant (p = 0.08) negative (r = − 0.66) correlation between age and area under the parent fraction curve. We therefore incorporated this additional variable into the method used to generate the “magnitude normalised” input functions: (1) normalisation of participants’ ppIFs according to weight, then injected dose, then age (multiplying each participant’s ppIF according to the ratio [median value/participant value]); (2) alignment of each ppIF peak to peak at 80 s; and (3) calculation of the median (i.e. standardised) ppIF from the 19 ppIFs.

In order to generate individualised PBIFs, the median ppIF was scaled as follows: (1) linear regression of the area under the 19 other participants’ ppIF curves (AUCs) with the parent radioactivity concentration in plasma at 90 min post-injection (assumed equivalent to venous plasma [14]) and then (2) scaling of the median ppIF according to the ratio of the AUC predicted (according to the linear regression) by the parent radioactivity concentration in the participant’s arterial plasma at 90 min to the AUC of the median ppIF.

Our PBIF method depended on a single parent plasma sample. Other approaches to scaling, i.e. according to injected dose and/or body mass (kg) alone or in combination, were found to yield weaker correlations with original ppIF-derived V_Ts (data not shown).

The PBIFs were used to perform voxelwise SA, as above.

Voxelwise SA was performed using the original ppIFs and dynamic emission data over t = 0–60, t = 0–70 min, and t = 0–80 min, using slow component boundaries of 0.000290, 0.000256, and 0.000222 s⁻¹, respectively.

We calculated the mean (original ppIF derived or PBIF derived, as applicable) V_T/SUV within seven cortical and subcortical bilateral ROIs using Analyze 7.0 (AnalyzeDirect Inc., Kansas, USA): cerebelli, hippocampi, occipital lobes, occipito-temporal (fusiform) gyri, parahippocampal gyri, putamina, superior frontal gyri (SFG), and thalami. Correlations were interrogated using Spearman’s rank coefficient. Pooled correlations were quantified using 140 data points (20 participants × seven ROIs) per variable. Original ppIF-derived and PBIF-derived V_Ts, and separately original ppIF-derived V_Ts that were calculated using 90- or 60-min datasets, were compared using Bland–Altman plots. Binding estimates were compared between subgroups [6] (epilepsy not on antidepressants, epilepsy on antidepressants, controls) by multivariate analysis of variance, with age as a covariate; a significant effect (p = 0.007 overall; individual ROIs p < 0.001) of subgroup on original ppIF-derived 90-min V_Ts was already reported [6].

SUVs were correlated with 90-min original ppIF-derived V_Ts derived from SA (seven ROIs pooled: increasing with time and reaching a maximum of ρ = 0.78 for 80–90 min; all p < 0.001; Fig. 1; Additional file 1).

The ranges of ρ were 0.34 (SFG) to 0.60 (cerebelli) for the interval 10–20 min, and 0.65 (hippocampi) to 0.79 (cerebelli and occipital lobes; all p ≤ 0.001) for the interval 80–90 min.

There was very little difference (< 1.3 percentage points) in the ROI between-subject coefficients of variation (BS-CVs) between the 80–90 min SUVs and the original ppIF-derived V_Ts (Additional file 1: Table S1). Larger differences were seen using earlier intervals.

The influence of subgroup on original ppIF-derived V_T [6] was not replicated for SUV data (p ≥ 0.05 for each interval).

PBIF-derived V_Ts were correlated with V_Ts calculated using the participants’ original ppIFs (seven ROIs pooled ρ = 0.90, p < 0.001). A small bias toward overestimation of PBIF-derived V_T was observed (linear regression y = 1.02x − 0.20; see Fig. 2) with a large variability (mean overestimate 0.7% ± 13.4%).

The range of ρ was 0.81 (hippocampi and occipital lobes) to 0.92 (cerebelli; all p < 0.001; see Additional file 1: Table S2). The absolute percent difference between PBIF-derived V_Ts and those calculated using the participants’ original ppIFs varied somewhat unpredictably across ROIs (Fig. 2), but was worse for elderly, healthy control participants.

An increase in BS-CV was observed that ranged from 2.5 percentage points (SFG) to 4.1 percentage points (occipital lobes; see Additional file 1: Table S2), i.e. mean ± standard deviation BS-CV was 26 ± 2% compared to 23 ± 2% for original ppIF-derived V_Ts.

The influence of subgroup on original ppIF-derived V_T [6] was not replicated for PBIF-derived V_Ts (p = 0.11).

ROI original ppIF-derived V_Ts calculated using 60-, 70-, and 80-min datasets were positively correlated with original ppIF-derived V_Ts derived from the full 90-min dataset (seven ROIs pooled ρ = 0.98, ρ = 0.99, and ρ = 1.00 respectively; all p < 0.001; Table 1, Fig. 3).

Correlation coefficients ranged from 0.97 (SFG and thalami, 60 min) to 1.00 (multiple ROIs and scan durations; all p < 0.001). The original ppIF-derived V_T was increasingly underestimated (relative to original ppIF-derived V_Ts calculated using 90-min datasets) with scan shortening, particularly for medial temporal lobe ROIs (Table 1, Fig. 4).

There was very little difference (< 0.9 percentage points) in ROI BS-CVs between the shortened original ppIF-derived V_Ts and the original ppIF-derived 90-min V_Ts.

The influence of subgroup on original ppIF-derived V_T [6] was replicated using all shortened datasets: 60 min (p = 0.001), 70 min (p = 0.003), and 80 min (p = 0.005).