Cationic Contrast Agent Diffusion Differs Between Cartilage and Meniscus.

Contrast enhanced computed tomography (CECT) is a non-destructive imaging technique used for the assessment of composition and structure of articular cartilage and meniscus. Due to structural and compositional differences between these tissues, diffusion and distribution of contrast agents may differ in cartilage and meniscus. The aim of this study is to determine the diffusion kinematics of a novel iodine based cationic contrast agent (CA(2+)) in cartilage and meniscus. Cylindrical cartilage and meniscus samples (d = 6 mm, h ≈ 2 mm) were harvested from healthy bovine knee joints (n = 10), immersed in isotonic cationic contrast agent (20 mgI/mL), and imaged using a micro-CT scanner at 26 time points up to 48 h. Subsequently, normalized X-ray attenuation and contrast agent diffusion flux, as well as water, collagen and proteoglycan (PG) contents in the tissues were determined. The contrast agent distributions within cartilage and meniscus were different. In addition, the normalized attenuation and diffusion flux were higher (p < 0.05) in cartilage. Based on these results, diffusion kinematics vary between cartilage and meniscus. These tissue specific variations can affect the interpretation of CECT images and should be considered when cartilage and meniscus are assessed simultaneously.

Introduction

Articular cartilage and meniscus are crucial tissue structures for the healthy functioning of the knee joint. Articular cartilage is an avascular specialized connective tissue with inhomogeneous structure that covers the ends of articulating bones. It enables low-friction joint movement, and together with meniscus, distributes loads in the knee joint.7,10 The crescent shaped menisci are mostly avascular fibrocartilaginous tissues located between the medial and lateral condyles of femur and tibial plateaus. In addition to load distribution, menisci stabilize the joint, absorb shocks, and improve joint lubrication.10,12,13 Structural constituents of these tissues are similar, but their contents and tissue structures differ significantly. The extracellular matrix of cartilage and meniscus consists of water (68–85% vs. 60–75%), proteoglycans (PGs) (5–10% vs. <1–2%), and collagens (10–20%, mainly type II vs. 15–25%, mainly type I), respectively.10,27 Due to the avascular nature of these tissues, the transport of nutrients occurs primarily via diffusion and convection from the synovial fluid, thus hindering the regeneration of cartilage and meniscus.10,11,16,26,28

Contrast enhanced computed tomography (CECT) is a non-destructive imaging technique to examine the biochemical composition, structure, and integrity of articular cartilage. From a clinical perspective, assessment of both cartilage and meniscus is key for successful diagnosis and treatment of degenerative diseases, e.g. osteoarthritis (OA). In order to address this imaging need, CECT has widely been investigated for the detection of cartilage degeneration and lesions,18,20,34,38 as well as, recently, to the imaging of bovine and human meniscus.14,24

CECT requires the use a contrast agent and commonly employs anionic contrast agents such as ioxaglate (q = −1) or gadopentate (q = −2),25 which distribute mainly by diffusion into the tissue and equilibrate inversely to the spatial distribution of the negatively charged PGs.4,35 In addition to PG content and distribution, contrast agent diffusion and distribution are influenced by the water content, collagen content, and structural integrity of the tissue matrix.9,19,21,36 Recently, novel cationic contrast agents were introduced for CECT imaging of cartilage2,17,37 and meniscus.24 As the cationic contrast agent molecules are attracted by the negative fixed charge density (FCD) of the tissues, CECT using cationic contrast agents offers a sensitive technique for direct monitoring of changes in cartilage and meniscus PG contents. Indeed, previous studies describe strong positive correlations between contrast agent distribution of a cationic contrast agent bearing four positive charges (CA4+) and PG content in these tissues.3,23,24

CECT has the potential to become a quantitative laboratory or clinical tool for assessment of knee joint composition and condition, given that articular cartilage and meniscus can be assessed simultaneously. Thus, it is important to determine the diffusion kinematics of the cationic contrast agent in cartilage and meniscus. Since the composition and structure of cartilage and meniscus are different, we hypothesize that the diffusion characteristics of the cationic contrast agent will vary between these tissues. Moreover, the previous studies mentioned above used CA4+ with a molecular weight of 1355 g/mol, and we rationalized that a smaller (686 g/mol, CA2+) but still cationic contrast agent may have a greater utility for CECT, as it should exhibit shorter times to equilibrium. Thus, the aim of this ex vivo study was to compare the diffusion of a smaller molecular weight cationic contrast agent bearing two positive charges, CA2+, into articular cartilage and meniscus. Herein, we report the: (1) CECT of bovine cartilage and meniscus plugs using a micro-CT scanner; (2) determination of the time to equilibrium and diffusion flux for CA2+ in both cartilage and meniscus tissues; (3) distribution of the cationic contrast agent within these tissues; and (4) dependence of these values on compositional (PG, water, hydroxyproline, and uronic acid) characteristics.

Materials and Methods

Sample Preparation

Similarly to our previous study,15 skeletally mature bovine knees (n = 10, one knee joint per animal) were obtained from a local slaughterhouse (HK Ruokatalo Oy, Outokumpu, Finland) within 24 h of slaughtering. Osteochondral plugs (d = 25.4 mm) were drilled from the upper lateral quadrant of the patellae (Fig. 1a). The plug was cut into quadrants and from one quadrant a sample plug (d = 6.0 mm) was punched out. Additionally, approximately 2.0 mm thick plug (d = 6.0 mm) from the central region of the medial meniscus was detached (Fig. 1b). One osteochondral and one meniscal plug were harvested from each joint. Surrounding tissue of the cartilage and meniscus plugs was collected for compositional analysis (Figs. 1a and 1b). Only healthy tissues, i.e., no visible signs of surface fibrillation or other early degenerative changes, were harvested.

Figure 1

(a) An osteochondral plug (d = 25.4 mm) was drilled from the upper lateral quadrant of a healthy bovine patella and trimmed to have ~ 2 mm bone under the cartilage. Subsequently, the disk was cut into four similar sections and a smaller osteochondral plug (d = 6 mm) was punched from a section with the flattest cartilage surface. The tissue surrounding the 6 mm plug was harvested for compositional analyzes. (b) A cylindrical plug (d = 6 mm) from the central region of medial bovine meniscus was harvested and trimmed to be 2 mm in height. In addition, the surrounding tissue (rectangular area ~ 2 mm around the plug, h ≈ 2 mm) was harvested for compositional analyzes.

CECT Imaging

The edges of the osteochondral and meniscus plugs were carefully sealed with a thin film of cyanoacrylate and glued on the bottom of plastic tubes. The tubes were filled with phosphate buffered saline (PBS) to completely immerse the plugs and a non-contrast image was acquired at room temperature. Subsequently, the PBS was carefully removed and replaced with a novel iodine based cationic contrast agent (CA2+) (q = +2, M = 686 g/mol)17 diluted with PBS including penicillin–streptomycin (100 units mL−1 penicillin, 100 μg mL−1 streptomycin; EuroClone, Siziano, Italy), antimycotic agent (Gibco Fungizone Antimycotic, 250 μg mL−1 amphotericin B, 205 μg mL−1 sodium deoxycholate; Life Technologies, Carlsbad, CA, USA) and proteolytic inhibitors [5 mM ethylenediaminetetraacetic acid disodium salt (EDTA; VWR International, Fontenay, France) and 5 mM benzamidine hydrochloride hydrate (Sigma-Aldrich Inc., St. Louis, MO, USA)] to 20 mgI/mL concentration. Both plugs were imaged for 48 h in isotonic contrast agent bath (330 mOsm/kg, 2 mL) at the following time points: 10, 20, 30, 40, 50, 60, 70, 80 90 and 100 min, and 2, 2.5, 3, 3.5, 4, 4.5, 5, 6, 7, 16, 20, 24, 28, 44, 46 and 48 h. CECT imaging was performed using a micro-CT-scanner (SkyScan 1172, SkyScan, Kontich, Belgium) with an isotropic voxel size of 25 µm × 25 µm × 25 µm, 100 kV tube voltage, and acquisition time of 10 min. Since the edges of the plugs were sealed, contrast agent penetration was allowed only through the articulating surface. After 48 h of contrast agent immersion the CA2+ was washed out by immersing the plugs in PBS for 48 h at 9°C. Subsequently, the plugs were fixed in 10% formalin, dehydrated in ascending series of ethanol, decalcified (cartilage + bone) and embedded in paraffin to enable cutting the sections for histological analysis.

Micro-CT data-analysis was conducted using custom made MATLAB scripts (R2012a, MathWorks, Inc., Natick, MA, USA). The image stacks for each time point were co-registered. 51 subsequent coronal slices were averaged to enhance the signal-to-noise-ratio. A similar procedure was done for the non-contrast image, which was subtracted from the CECT images. A 1275 µm wide region (51 pixels) of interest (ROI), height matched with full thickness of the tissue, was selected in the center of the sample. The pixel rows in the ROI were horizontally averaged and the X-ray attenuation was normalized with that in the surrounding contrast agent bath to obtain a depth-wise normalized attenuation (i.e. contrast agent partition) profile (Fig. 2).

Figure 2

(a) A micro-CT image (average of 51 consecutive 25 µm thick slices) of one representative cartilage sample after 10 min of contrast agent diffusion and before background (non-contrast image) subtraction. The analyzed region of interest (ROI) is delineated with a solid line and the ROI for normalization delineated with a dashed line. The width of the analyzed ROI was 1275 µm (51 pixels) and the height was matched with the full thickness of the cartilage. An identical approach was used when CECT images of the menisci were analyzed. Scale bar = 2 mm. (b) A magnified image of the analyzed cartilage area after background subtraction. Scale bar = 500 µm. (c) A depth-wise contrast agent distribution profile. The horizontal axis represents the relative distance from the surface (0) to the cartilage-bone interface (1). To create the distribution profiles the pixel rows in subfigure (b) were horizontally averaged and normalized with the average X-ray attenuation value within the normalization ROI shown in the subfigure (a).

Time dependent normalized attenuation was determined by fitting an exponential function to the bulk X-ray attenuation values, C (%), determined at different time points t (s):where a, b, and c are the fitting coefficients.24 The time required to reach equilibrium was determined as the time at which the change in the normalized attenuation was less than 0.05% per hour.15 The diffusion flux, J (mol/m2/s), through the tissue surface was calculated as follows:where h (m) is the sample thickness, t (s) is time and is the bulk contrast agent concentration (mol/m3) within the sample derived from Eq. (1).

Histology and Compositional Analyzes

The paraffin embedded samples were halved and cut into 3 and 5 µm thick sections for analysis of PG and collagen distributions, respectively. Subsequently, the paraffin was dissolved and the 3 µm sections were stained with Safranin-O. The spatial distribution of the stain in the section was measured using quantitative digital densitometry (DD) revealing the PG distribution.31 Three sections per sample (1275 µm in width, full thickness) were analyzed and the depth-wise profiles were averaged. The measurements were done utilizing a light microscope (Nikon Microphot-FXA, Nikon Co., Tokyo, Japan), equipped with a monochromatic light source and a 12-bit CCD camera (ORCA-ER, Hamamatsu Photonics K.K., Hamamatsu, Japan). The system was calibrated with neutral density filters (Schott, Mainz, Germany) covering optical density (OD) range from 0 to 2.6.

The collagen distribution in 5 µm sections, adjacent to the ones used in DD, was determined using Fourier transform infrared (FTIR) microspectroscopy (Hyperion 3000, Bruker Corporation, Billerica, MA, USA). After deparaffinization, the sections were moved on Zinc-Selenide (ZnSe) IR-windows. A 1 mm wide, full sample thickness ROI was determined from three sections per sample. Data was collected within wavenumber range of 2000-720 cm−1 using a pixel size of 20 × 20 µm2 and spectral resolution of 8 cm−1. The background was measured on a clean ZnSe-window using the same parameters as above. Collagen content in each pixel was determined as the amide I (1720–1595 cm−1) peak area.32 The depth-wise profiles of collagen content were calculated for each section and the three profiles were averaged.

Water, hydroxyproline and uronic acid contents (the latter two corresponding to collagen and PG contents, respectively) were determined from the tissues surrounding the sample plugs using compositional analyzes. Water content was determined via lyophilization. Hydroxyproline and uronic acid contents were determined from the plugs digested with 1 mg/mL concentration of papain in 150 mM sodium acetate including 50 mM Cys-HCl and 5 mM EDTA at pH of 6.5 in 60°C for 3 h to digest the PGs. Enzyme inactivation was managed by boiling the sections for 10 min. Subsequently, the hydroxyproline content was determined from the freeze dried and papain digested sections with spectrophotometric assay.6 The uronic acid content was quantified from the ethanol-precipitated samples dissolved in water.5 The contents were determined three times for each sample, normalized by the sample wet weights and averaged.

Statistical Analyzes

Wilcoxon signed rank test was used to determine the significance of the differences between the parameter values of cartilage and meniscus. The Wilcoxon signed rank test was chosen due to the relatively low number of paired samples. Spearman’s rho was determined to analyze the significance of relationships between the normalized attenuation and reference parameters (i.e. water, uronic acid and hydroxyproline contents and bulk OD values). Multiple linear regression analysis was conducted between the compositional parameters (i.e., water, hydroxyproline and uronic acid contents) and the normalized attenuation of pooled samples. The statistical tests were conducted using SPSS (v. 21.0.0.0, SPSS Inc., IBM Company, Armonk, NY, USA).

Results

After 48 h of diffusion, the normalized attenuation reached 289.4 ± 44.2% in cartilage and 159.7 ± 11.2% in the meniscus (Table 1; Fig. 3a). At all time points after 50 min, the normalized attenuation was significantly higher (p < 0.05) in cartilage than in meniscus (Figs. 3a and 4; Table 1). The diffusion flux was significantly higher (p < 0.05) in cartilage at all time points (Fig. 3b). However, no significant differences (p = 1.0) were found in the time to reach equilibrium for CA2+ in cartilage and meniscus (35.8 ± 6.5 and 37.3 ± 9.6 h, respectively). The contrast agent distribution within the cartilage and meniscus sample plugs was different (Figs. 4, 5a and 5b). Moreover, the majority of CA2+ accumulated in the deep zone of cartilage, while in the meniscus, the CA2+ accumulated closer to the articulating surface (Figs. 3, 5a and 5b).

Table 1

Normalized attenuation at 1 and 48 h time points, water, hydroxyproline and uronic acid contents and optical densities of bovine cartilage (n = 10) and meniscus (n = 10).

	Normalized attenuation (%), 1 h	Normalized attenuation (%), 48 h	Water (%)	Hydroxyproline (µg/mg, w.w.)	Uronic acid (µg/mg, w.w.)	Optical density	Thickness (mm)
Cartilage	57.5 ± 16.6*	289.4 ± 44.2*	80.4 ± 2.4*	15.4 ± 2.3*	9.0 ± 3.4*	1.66 ± 0.09*	2.01 ± 0.33
	(22.8, 80.1)	(225.0, 340.3)	(76.6, 83.1)	(11.0, 19.0)	(4.4, 14.8)	(1.47, 1.75)	(1.55, 2.58)
Meniscus	39.5 ± 12.0*	159.7 ± 11.2*	72.1 ± 1.8*	33.7 ± 3.4*	3.3 ± 0.5*	0.88 ± 0.24*	1.83 ± 0.30
	(21.4, 60.2)	(141.0, 178.2)	(69.3, 75.1)	(26.7, 39.8)	(2.4, 3.9)	(0.52, 1.16)	(1.45, 2.25)

Mean values (±SD) of the parameters are presented in the top row and the range in parentheses (min, max) in the bottom row

* Significant difference (p < 0.05) between cartilage and meniscus samples, Wilcoxon signed rank test

Figure 3

(a) Mean (n = 10) normalized attenuation in bovine cartilage (+SD) and meniscus (-SD) at 26 different time points (10, 20, 30, 40, 50, 60, 70, 80 90 and 100 min, and 2, 2.5, 3, 3.5, 4, 4.5, 5, 6, 7, 16, 20, 24, 28, 44, 46 and 48 h after immersion). The normalized attenuation was significantly higher (p < 0.05) in cartilage than in meniscus at all time points after 50 min. (b) Mean (n = 10) diffusion fluxes for cartilage and meniscus as a function of immersion time. The diffusion flux was significantly higher (p < 0.05) in cartilage than in meniscus at all time points.

Figure 4

Mean (n = 10) depth-wise contrast agent distribution within cartilage (left) and meniscus (right) through the experiment. Values at vertical axis represent the relative thickness of the samples, 0 corresponds to the articular surface and 1 to the bottom of the tissue.

Figure 5

Mean (n = 10) depth-wise optical density profile (dashed line) corresponding to PG distribution and contrast agent distribution (solid line) in cartilage (a) and meniscus (b) after 48 h of immersion in cationic contrast agent. Mean (n = 10) depth-wise amide I peak area corresponding to the collagen distribution in cartilage (c) and meniscus (d). The horizontal axis represents the relative distance from the articular surface (0) to the bottom (1) of the tissue.

Water and uronic acid contents and bulk OD values were significantly higher (p = 0.005 for all) and hydroxyproline content was significantly lower (p = 0.005) in cartilage than in meniscus (Table 1). The depth-wise PG distribution was similar, while the depth-wise collagen content distribution was different between the tissues (Fig. 5). There was no significant (p > 0.05) relationship between the normalized attenuation and water, uronic acid, and hydroxyproline contents as well as bulk OD values within cartilage or meniscus sample pools. However, when samples from both tissues were pooled (n = 20), the composition significantly predicted the normalized attenuation at diffusion equilibrium (48 h): F(3, 16) = 27.934, p < 0.001, R 2 = 0.84. However, only uronic acid was significant (p < 0.05) predictor of the normalized attenuation.

Discussion

The aim of this study was to investigate the diffusion kinematics of cationic contrast agent (CA2+) in healthy bovine articular cartilage and meniscus. Accordingly, we determined the normalized attenuation at 26 different time points over 48 h of contrast agent diffusion. Subsequently, the diffusion flux was determined. Normalized attenuation was found to be significantly higher in cartilage than in meniscus after 50 min of diffusion. Furthermore, the diffusion flux was systematically higher in cartilage throughout the whole experiment. However, no statistically significant difference was observed between the tissues in the time required to reach the diffusion equilibrium.

The normalized attenuation at equilibrium was >100% in both tissues compared with the initial bath attenuation. This is due to accumulation of cationic contrast agent molecules in the tissue, due to the electrostatic attraction between PGs and contrast agent molecules. With anionic contrast agents, instead, the normalized attenuation (i.e. contrast agent partition) at diffusion equilibrium is <100%,14,15,18,22,30 as the anionic contrast agents are repelled by the negative FCD of the tissues. The normalized attenuation was significantly higher in cartilage than in meniscus, which reflects the higher PG and water contents in cartilage. These results are consistent with previous studies using the CA4+ cationic contrast agent which reported a strong positive relationship between the normalized attenuation and PG content in cartilage and meniscus.3,23,24 In addition, solute diffusivity has been shown to correlate positively with water content in cartilage.9

At diffusion equilibrium, most of the contrast agent accumulated in the deep cartilage (50–94% of the thickness1,8,16,39), i.e., in zone with the highest PG concentration. In the meniscus, the highest contrast agent accumulation was in the lamellar layer (150–200 µm thick layer ~10 µm beneath the surface33). Interestingly, the distribution of cationic contrast agent within the meniscus was similar to that reported previously for an anionic contrast agent.15 Possibly, this finding could be related to higher water content in the surface and lamellar layers of the meniscus, making these regions more accessible for the CA2+ molecules. The high water content in these layers is also suggested by lower PG and collagen concentrations compared with those in the central layer of the meniscus. Furthermore, the steric hindrance may be greater in the meniscus than in cartilage as the hydroxyproline content of the meniscus was over 200% of that in cartilage. This could hinder accumulation of CA2+ in the central layer of the meniscus.

The diffusion flux was significantly higher in cartilage than in meniscus, due to the differences in the PG and collagen concentrations and distributions in the tissues. The higher PG concentration of cartilage, as compared with that of the meniscus, creates higher electrostatic attraction to the cationic contrast agent molecules. The diffusion towards the deep cartilage maintains the higher diffusion flux of cartilage also at later time points. Furthermore, due to the higher collagen content, the contrast agent molecules may be more affected by the steric hindrance of the matrix in the meniscus than in cartilage. The amount of contrast agent diffused into cartilage was also substantially greater. The majority of CA2+ accumulated close to the articulating surface (i.e., in the lamellar layer) in the meniscus samples. In cartilage samples, CA2+ accumulated in the deep zone, which prolonged the diffusion process. For these reasons, the time required to reach diffusion equilibrium was not different between the tissues, although the diffusion flux was higher in cartilage.

In this study, cylindrical osteochondral and meniscal plugs excised from healthy bovine knee joints were used to study the diffusion kinematics of a cationic contrast agent. Due to the relatively small homogenous sample population (n = 10 for cartilage and meniscus), the variation of tissue properties was limited, and no statistical significances were observed between the normalized attenuation and reference parameters in cartilage or meniscus sample pools. However, the homogeneity in sample population allowed a reliable comparison of the diffusion kinematics between cartilage and meniscus tissues.

The main constituents (water, PGs and collagens) are the same in cartilage and meniscus, but their distributions within the tissue differ. However, in case of intact tissues, the amount of contrast agent content at diffusion equilibrium, indicated by the bulk value of normalized attenuation, should be related to the amount of these constituents rather than to their distributions. Thus, the pooling of cartilage and meniscus samples was justified to assess the relationship between contrast agent intake and compositional constituents of the tissues.

As the samples were imaged while immersed in contrast agent bath, diffusion still occurred during the scan. Hence, the normalized attenuation at each time point represents the average value over the scan time rather than precise value at the time point. However, we believe that this had no significant effect on the presented results or conclusions, as the diffusion occurs over many hours.

CECT, using cationic contrast agents, is a promising imaging technique for laboratory purposes, e.g. comprehensive CT-based 3D histopathological evaluation29 of the knee joint. However, if an intact knee joint is imaged, the differences in contrast agent diffusion in cartilage and meniscus must be acknowledged when interpreting the results. In addition, the concentration of the contrast agent bath must be maintained at a high level, for example, by intermittent injection of contrast agent. This is because the contrast agent starts to dilute and efflux from the joint capsule. The effluxion takes place in both intact ex vivo and in vivo situations, but is more rapid in vivo due to perfusion. In addition, due to longer diffusion distance, the time required to reach diffusion equilibrium is likely to be longer when full thickness menisci are imaged. The time to reach diffusion equilibrium is too long for clinical applications, even with a cationic contrast agent of small molecular size (M = 686 g/mol).

In summary, the distribution of the cationic contrast agent, CA2+, within tissue is different between cartilage and meniscus. The intake of contrast agent is significantly higher in cartilage than in meniscus at all time points after 50 min of immersion. In addition, the diffusion flux is significantly higher in cartilage at all time points up to 48 h. Nevertheless, the diffusion equilibrium is reached at the same time in both tissues. When both cartilage and meniscus samples are included in the analysis, the compositional parameters predicted the normalized attenuation at 48 h. However, the differences in diffusion kinematics between cartilage and meniscus must be acknowledged in the interpretation of CECT images of knee joint.