Examining the Feasibility of Quantifying Receptor Availability Using Cross-Modality Paired-Agent Imaging

This study compares receptor availability values recovered using an all-optical PAI approach and a cross-modality PAI approach from the same animals (n = 18). Each animal was co-administered a targeted optical contrast agent, an untargeted optical agent, and a GBCA. The kinetic behaviors of all three were imaged simultaneously for approximately 1 h using an MRI-coupled fluorescence tomography system [10]. The kinetics data is included as supplementary material (Table S1). This enabled RA to be determined using the two optical agents (single-modality PAI) and the targeted optical/GBCA (cross-modality PAI).

This study represents an extended analysis of an earlier study that evaluated single-modality PAI using the same animals [11]. As such, agent and animal preparation and fluorescence tomographic image reconstruction procedures are only briefly summarized here and referenced accordingly. Herein, we detail the recovery of cross-modality RA and the corresponding correlation analysis.

Two cell lines were used in this study: U251 glioma cells (moderate EGFR expressing) (provided from Dr. Israel at Dartmouth College, Lebanon, NH) and 9L rat sarcoma cells (negative for EGFR expression) (provided from Dr. Wheeler at Wake Forest University, Winston-Salem, NC), providing a range of receptor expression profiles [8, 12, 22]. Cells were maintained in DMEM culture media supplemented with 5% fetal bovine serum and 1% antibiotic at 5% CO₂, 37°C.

Animal studies were conducted in accordance with protocols approved by the Institutional Animal Care and Use Committee (IACUC) at Dartmouth College. Female nude mice were purchased from Charles River Laboratories (Wilmington, MD). Mice were orthotopically implanted with 1 × 10⁶ tumor cells, as previously described [23]. Animals were monitored for recovery post tumor implantation and continually monitored for neurological signs of tumor growth. Approximately 3–5 weeks post tumor implantation, mice were imaged with gadolinium-enhanced MRI (Gd-MRI) to confirm presence of orthotopic tumors.

The targeted imaging agent was ABY-029, a GLP formulation of anti-EGFR affibody (Affibody AB (Solna, Sweden)) conjugated to IRDye 800CW Maleimide (LI-COR Biosciences, Inc., Lincoln, Nebraska) as described [24]. The untargeted counterpart was Affibody imaging agent, negative control bound to LI-COR’s IRDye 680RD [12]. For MRI-PAFT studies, the targeted and untargeted optical imaging agents (concentration of 0.2 nmol per agent) were mixed with an MRI contrast agent, Gadovist (0.5 mmol/kg) (Bayer, Leverkusen, Germany), in an injection solution of 200 μl per dose and administered to the animals via tail vein injection.

The MRI-coupled fluorescence tomography (FMT) system has been described in previous publications [10, 11, 25‐28]. Briefly, the instrument consists of a clinical Philips Achieva 3.0 T scanner and a spectrometer-based FMT system that includes eight optical fibers extending into the bore of the MRI scanner and positioned around the head of the animal using a custom rodent optical/RF coil. Each fiber acts as a source or a detector, allowing an excitation source multiplexer to sequentially illuminate each fiber while the remaining seven fibers detect the transmitted light using high-sensitivity spectrometers. Optical filtering and spectral decomposition enable the separation of the two fluorescent agents prior to image reconstruction [27].

After positioning the animal in the RF/optical coil, MRI and fluorescence tomography images were acquired once just prior to administration of the 3-contrast-agent cocktail (two fluorescent and one GBCA). Immediately after administration, dynamic data was acquired of all three agents concurrently for about 60 min. Dynamic GBCA data were acquired by repeating a T1-weighted turbo spin echo sequence (TR = 121 ms, TE = 10 ms, FOV = 90 mm × 90 mm, number of slices = 4, dimension of reconstruction matrix = 256 × 256, slice thickness = 1 mm, and flip angle = 90°, 89 s per frame). An additional high-resolution T1-weighted turbo spin echo sequence (TR = 744 ms, TE = 10 ms, FOV = 90 mm × 90 mm, number of slice = 30, dimension of reconstruction matrix = 256 × 256, slice thickness= 0.75 mm, and flip angle = 90°) was acquired for 15 min into the sequence to provide a template for the optical reconstruction. Optical data consisted of full tomographic projections of each spectral channel (i.e., for each optical imaging agent) acquired at about one frame per 108 s. Volumetric images of fluorescence intensities were reconstructed at each frame and for each agent using a hard-priors technique guided by an anatomically segmented high-resolution MRI volume [26]. This data processing technique produced the following three data sequences for the 1-h acquisition: (1) dynamic MRI scans of GBCA, (2) dynamic fluorescent intensity of the targeted fluorescent agent, and (3) dynamic fluorescent intensity of the untargeted fluorescent agent, in the tumor, brain tissue, and “outside of brain” tissue. Because acquisition points were not strictly simultaneous, data points along the sequence were linearly interpolated to align with each other prior to analysis. The kinetic curves of each agent were normalized to their own area under the curve (AUC) for comparison and correlation analysis.

Paired-agent recovery of RA was accomplished using the snapshot technique [29], which is a simple approach that compares normalized targeted and untargeted signal intensities at a given time. The intensities for each agent at a given time, t, are normalized to the intensities from the first measurements: \( \frac{T(t)}{T(0)}=\overset{\sim }{T}(t) \)and \( \frac{UT(t)}{UT(0)}=\overset{\sim }{UT}(t) \), where T(t) and UT(t) represent targeted and untargeted agents intensities at time t and \( \overset{\sim }{T}(t) \) and \( \overset{\sim }{UT}(t) \)are normalized intensities for targeted and untargeted agents. T(0) and UT(0) are targeted and untargeted agent intensities at the first dynamic measurement after contrast administration. The snapshot RA, at time t, is calculated as follows:

The snapshot RA calculated using this equation is essentially identical to the “nondisplaceable binding potential” referred to in PET kinetic modeling, which is the product of the receptor concentration available to bind and the affinity of the imaging agent [30]. These values were computed for both the all-optical single-modality and optical/MRI cross-modality agent pairs. The snapshot approach provided estimates of RA recovered at each time point over the entire dynamic sequence.

To assess the correlation between single- and cross-modality PAI, a repeated measures correlation coefficient analysis was applied following the method reported by Bland and Altman for calculating correlation coefficient with repeated observations [31‐33]. Specifically, analysis of covariance (ANCOVA) was performed to account for inter-individual variability among observations by providing parallel linear regression for individual samples. ANCOVA analyses were performed using the MATLAB (Matlab_R2020a) tool: aoctool. From the ANCOVA, regression sum of the squares (SSR) and error sum of squares (SSE) were calculated as:

for an experiment including j = n subjects with each subject provided i = m_j measurements. SSR is the sum of squared differences between the predicted value, \( {\hat{y}}_{ij} \), and the mean of dependent variable for each participant, \( {\overline{y}}_j \). SSE is the sum of squared differences between the dependent variables, y_ij, and the regression-predicted values. The repeated measures correlation coefficient (r) was then calculated as a ratio of the regression sum of squares and the error sum of squares:

The value of r does not change based on which variable is specified as dependent variable, since switching the dependent and independent variable in a regression model only changes the values of the sum of squares relatively. In this study, the cross-modality PAI results were used as the dependent variables, while the conventional PAI results were used as the independent variables. The significance, p value, is determined by the F test associated with the ANCOVA.