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(Circulation. 2002;106:1397.)
© 2002 American Heart Association, Inc.

Basic Science Reports

Detection of Experimental Autoimmune Myocarditis in Rats by ¹¹¹In Monoclonal Antibody Specific for Tenascin-C

Mikio Sato, MD; Tetsuya Toyozaki, MD; Kenichi Odaka, MD; Tomoya Uehara, MS; Yasushi Arano, PhD; Hiroshi Hasegawa, MD; Katsuya Yoshida, MD; Kyoko Imanaka-Yoshida, MD; Toshimichi Yoshida, MD; Michiaki Hiroe, MD; Hiroyuki Tadokoro, MD; Toshiaki Irie, PhD; Shuji Tanada, MD; Issei Komuro, MD

From the Department of Cardiovascular Science and Medicine (M.S., K.O., K.Y., I.K., H.H.), the Department of Basic Pathology (T.T), Graduate School of Medicine, and the Department of Molecular Imaging and Radiotherapy (T.U., Y.A.), Graduate School of Pharmaceutical Sciences, Chiba University, Chiba, Japan; the Department of Pathology (K.I.-Y., T.Y.), Mie University School of Medicine, Tsu, Japan; the Cardiology Division (M.H.), International Medical Center of Japan, Tokyo; and the Division of Medical Imaging (H.T., T.I., S.T.), National Institute of Radiological Sciences, Chiba, Japan.

Correspondence to Katsuya Yoshida, MD, Department of Cardiovascular Science and Medicine, Chiba University Graduate School of Medicine, 1-8-1 Inohana, Chuo-ku, Chiba-shi, Chiba 260-8670, Japan. E-mail yoshi@ med.m.chiba-u.ac.jp

	Abstract

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Background— Although the identification of inflammatory infiltrates in endomyocardial biopsy specimens is necessary for the definite diagnosis of myocarditis, the biopsy test is invasive and is not sensitive. Therefore, a new diagnostic technique for the early and noninvasive evaluation of myocarditis has been awaited. Expression of tenascin-C (TNC), one of the oligometric extracellular glycoproteins, is induced in various pathological states, including inflammation, suggesting that TNC can be a molecular marker of myocarditis.

Methods and Results— An ¹¹¹In anti-TNC monoclonal antibody Fab' fragment was injected intravenously into rats with experimental autoimmune myocarditis (EAM), and the biodistribution of this radiotracer was measured. Rapid clearance of radioactivity from the blood was observed in both EAM and control rats (<1% at 6 hours after injection). Myocardial uptake of the tracer was much higher in EAM rats than in control rats (7.54-, 4.39-, and 3.51-fold at 6, 24, and 48 hours after injection, respectively). By autoradiography, high radioactivities were clearly observed in the regions indicative of inflammation in EAM rats. Single-photon emission CT imaging demonstrated the focal myocardial uptake of ¹¹¹In anti-TNC Fab' in vivo.

Conclusions— Radiolabeled anti-TNC Fab' may be useful for the noninvasive diagnosis of myocarditis.

Key Words: myocarditis • antibodies • nuclear medicine

	Introduction

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Viral infection is mostly responsible for myocarditis in humans.^1–3 The principal mechanism of heart involvement in viral myocarditis is believed to be a cell-mediated immunological reaction to cell surface changes or a new antigen related to the virus.⁴ More intriguing is the possibility that viral myocarditis may culminate in dilated cardiomyopathy, presumably as a consequence of virus-mediated immunological cardiac damage.^{5– 7} In spite of the development of various diagnostic modalities, early and definite diagnosis of myocarditis still depends on the detection of inflammatory infiltrates in endomyocardial biopsy specimens according to the Dallas criteria.⁸ However, this technique is invasive and prone to sampling error.⁹ Therefore, a new diagnostic technique for the early, precise, and noninvasive diagnosis of myocarditis has been awaited.

Tenascin-C (TNC), one of the algometric extracellular matrix glycoproteins, is expressed during embryogenesis but not in normal adult tissues.^10,11 However, in various pathological states, such as wound healing, cancer invasion, or inflammation, TNC is transiently reexpressed.¹² We recently demonstrated that TNC is specifically expressed in myocardium during the active stage of myocarditis in a mouse model. Immunoreactivity of TNC appeared at the initial stage of myocytolysis, remained during the active stage while cell infiltration and necrosis continued, and disappeared with the formation of scar tissue in the healed stage.¹³ This highly spatiotemporal specificity of TNC expression suggests that molecular imaging of TNC would be useful for the noninvasive diagnosis of myocarditis.

In the present study, we examined whether injected anti-TNC monoclonal antibody can target myocarditis. This antibody was used as a Fab' fragment because of the rapid pharmacokinetics and lower immunogenicity.^14,15 Experimental autoimmune myocarditis (EAM) was induced by the immunization of rats with purified myosin with complete Freund’s adjuvant.^16,17 We injected ¹¹¹In anti-TNC Fab' intravenously into EAM rats and control rats and measured its biodistribution. The localization of the radioactivity in the myocardium was also analyzed by ex vivo imaging (autoradiography) and in vivo imaging (single-photon emission CT [SPECT]).

	Methods

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Induction of EAM
Forty female 7-week-old Lewis rats purchased from Charles River Japan Inc (Atsugi, Kanagawa, Japan) were used under the protocol approved by the Special Committee on Animal Welfare of the Inohana Campus of Chiba University. EAM was induced in rats as previously described.¹⁷ In brief, rats were immunized twice at a 7-day interval with 10 mg/mL porcine cardiac myosin (Sigma Chemical Co) with Freund’s complete adjuvant (Sigma Chemical Co) or with Freund’s complete adjuvant alone (control rats). All experiments were performed at 17 days after the first immunization.

Antibody and Western Blotting
A mouse monoclonal antibody against TNC, clone 4F10TT, was raised by immunization of a TNC-null mouse¹⁸ with purified human TNC¹⁹ as described previously.¹³ Isolated splenic cells from a TNC-null mouse immunized with TNC were fused with SP2/0 myeloma cells. Immunoglobulin was purified from the culture supernatant of hybridoma cell clone 4F10TT cultured in serum-free media. The Fab' fragments of the antibody were prepared by reducing the disulfide bonds of the F(ab')₂ fragments with mercaptoethanol after pepsin digestion of the intact antibody.

As a nonspecific control antibody, an isotype-matched monoclonal antibody against the V protein of parainfluenza virus type II (clone 53-1, isotype IgG1; kindly provided by the Department of Microbiology, Mie University School of Medicine) was also digested to the Fab' fragment as described above.

Immunoblotting was performed as previously described.²⁰ In brief, hearts were removed from rats on day 21, and the myocardium was homogenized in 4 mL buffer A (20 mmol/L Tris-HCl, 0.15 mol/L NaCl, 1 mmol/L EDTA, 1 mmol/L phenylmethylsulfonyl fluoride, and 1 mmol/L dithiothreitol, pH 7.4). Samples of protein (20 µg/lane) were subjected to SDS-PAGE with 2% to 15% gradation polyacrylamide gel and electrophoretically transferred onto Immobilon membranes (Millipore). The transferred proteins were immunostained with 4F10TT (1 µg/mL) by using the indirect immunoperoxidase method.

Immunohistochemical Staining
Immunostaining of tissue sections was performed as described previously.²¹ In brief, the sections were first incubated with primary antibodies 4F10TT (1 µg/mL) and then with peroxidase-conjugated anti-mouse IgG (1:500, MBL, Nagoya, Japan). After the sections were washed, diaminobenzidine/H₂O₂ solution was used to demonstrate antibody binding. The slides were lightly counterstained with hematoxylin for microscopic examination.

Radiolabeling With ¹¹¹In
The thiol groups of the purified Fab' fragments of the 2 antibodies were conjugated with the maleimide groups of 1-4-[(5-maleimidopentylamino)benzyl]-EDTA (EMCS-Bz-EDTA) to place radiometal chelates distal from the antigen binding site of the antibodies, as described previously.^22,23 To a 1-mL solution of Fab' (1 mg/mL) in 0.1 mol/L phosphate buffer (pH 6.0) was added 60 µL EMCS-Bz-EDTA (5.3 mg/mL) in the same buffer. After a 3-hour incubation, 20 µL iodoacetamide (10 mg/mL) was added to mask unreacted thiol groups. The number of EMCS-Bz-EDTA molecules conjugated per molecule of the respective antibody fragment was determined.²³ Each conjugate was then purified from unreacted low molecular weight compounds by Sephadex G-50 column chromatography (1.8 cmx40 cm), equilibrated, and eluted with MES-buffered saline (pH 6.0).

The purified conjugates were labeled with ¹¹¹In, as previously reported.^{23 111}In antibody fragments were purified by a centrifuged column procedure using Sephadex G-50 equilibrated with 0.1 mol/L PBS (pH 6.0). Radiochemical purities of the ¹¹¹In antibody fragments were determined by cellulose acetate electrophoresis and size-exclusion high-performance liquid chromatography.

Biodistribution Study
Ten EAM rats and 10 control rats were injected with 100 µg (111 KBq) of ¹¹¹In anti-TNC Fab' in 300 µL saline solution intravenously through the tail vein. Groups of 3 or 4 animals were euthanized at 6, 24, and 48 hours after the tracer injection. Hearts, other organs (lung, liver, kidney, spleen, cerebrum, foot pad, and hindlimb muscle), and blood were weighed and then counted for radioactivity with the blood samples. Pleural effusion was also sampled in EAM rats. The percentage of the injected dose of the radioactivity per gram tissue weight was calculated. To evaluate the dose-dependent changes in EAM-targeting properties of the radiotracer, groups of 3 rats each were administered different amounts of ¹¹¹In anti-TNC Fab' (10, 50, or 100 µg per rat) and euthanized at 6 hours after injection, and the uptake of the radiotracer in the heart and other organs was estimated.

The specific uptake of anti-TNC antibody in EAM rats was also estimated by comparing, at 6 hours after injection, the radioactivity distribution of the same amounts (3 µCi, 50 µg) of ¹¹¹In anti-TNC Fab' (n=3) or ¹¹¹In nonspecific Fab' (n= 5).

Histopathologic and Quantitative Autoradiographic Study
Two groups of EAM rats were administered similar amounts (740 KBq, 50 µg) of either ¹¹¹In anti-TNC Fab' or ¹¹¹In nonspecific Fab'. A similar amount of ¹¹¹In anti-TNC Fab' was also injected into control rats. At 6 hours after injection, the hearts were excised and embedded in Tissue-Tek OCT compound (Miles). Sections of 5-µm thickness were mounted on a slide and stained with hematoxylin and eosin (H-E) for pathological analysis. Sections of 20-µm thickness were exposed to autoradiography. The imaging plate was exposed for 24 hours and studied by image analyzer (BAS-1800 system, Fuji Film Co Ltd). Autoradiographic intensities of each myocardial tissue were presented as (PSL-BG)/A, where PSL is photostimulated luminescence, BG is PSL of the background, and A is area (mm²).

In Vivo Imaging
¹¹¹In anti-TNC Fab' in vivo imaging was performed in an EAM rat by use of SPECT. The SPECT system consisted of a 3-headed -camera (Toshiba GCA 9300A) equipped with 1.0-mm pinhole collimators. ¹¹¹In anti-TNC Fab' (2.2 MBq) was injected intravenously, and after 5.5 hours, 37 MBq of ^99mTc sestamibi (MIBI) (DRL, Tokyo, Japan) was injected. Thirty minutes later, a rat was anesthetized by an intraperitoneal injection of pentobarbital (30 µg/g), and 60-minute data acquisition was performed at 120 seconds per view with stepwise rotation for each 4° over 120° and with multiple peak acquisition (15% windows for the ^99mTc and both ¹¹¹In peaks). The matrix was 128x128 for data acquisition and for the image display with 0.6-mm pixel size.

	Results

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Expression of TNC in EAM Hearts
Western blot analysis of the myocardium showed that in the EAM rat, 2 strong bands were observed at 270 and 230 kDa (Figure 1; arrowheads, lane 2), whereas no band was observed in the normal rat myocardium (lane 1). In human glioma TNC, 3 bands were detected at 300, 240, and 210 kDa (arrows, lane 3).

View larger version (11K): [in this window] [in a new window]   Figure 1. Western blot analysis of myocardial tissue. Extracted proteins from hearts of a normal rat (lane 1) and a rat on day 21 of myosin-induced autoimmune myocarditis (lane 2) as well as purified TNC from human glioma cells (lane 3) were electrophoresed and stained immunochemically with mouse monoclonal anti-TNC clone 4F10TT.

At 21 to 28 days after the first injection of the antigen, severe inflammatory cell infiltration and myocyte necrosis were recognized throughout the myocardium (Figure 2b). Strong immunostaining for TNC was observed in the interstitium. On the other hand, no immunostaining was detected in the normal myocardium (Figure 2a).

View larger version (135K): [in this window] [in a new window]   Figure 2. Immunostaining for TNC of sections from normal rat myocardial tissue (a) and from rat myocardial tissue at day 21 after first injection of myosin (b). Bar=50 µm (a).

In Vivo Biodistribution of ¹¹¹In Anti-TNC Fab'
The numbers of EMCS-Bz-EDTA groups attached per antibody molecule were 1.4 and 1.6 for anti-TNC antibody and control antibody, respectively. Fewer than 0.05 free thiol groups were found per molecule of each antibody fragment after the addition of iodoacetamide. After purification by centrifuged column procedure, ¹¹¹In anti-TNC Fab' and ¹¹¹In nonspecific Fab' were obtained with radiochemical purities of 96.9% and 97.6% for anti-TNC antibody and the nonspecific antibody, respectively.

The tissue uptake of ¹¹¹In anti-TNC Fab' is summarized in Table 1 as a percentage of the injected dose per gram tissue. Rapid clearance of radioactivity from the circulation was observed with ¹¹¹In anti-TNC Fab' in both EAM and control rats (<1% at 6 hours after injection). The kidney uptake was the highest at all time points, with the spleen and liver being next and then the myocardium. However, myocardial uptake was significantly lower in control rats compared with EAM rats. Radioactivity was much higher in EAM rat hearts than in control rat hearts; the increases were 7.54-, 4.39-, and 3.51-fold at 6, 24, and 48 hours, respectively. Heart-to-blood ratios of radioactivity were much higher in EAM rats than in control rats and increased gradually after injection (Table 1). Comparative myocardial uptakes with adjoining organs, such as the lung and liver, are also shown in Table 1. The radiotracer reached its highest heart-to-liver and heart-to-lung ratios of radioactivity at 6 hours after injection.

View this table: [in this window] [in a new window]   Table 1. Biodistribution of 111In-Labeled Anti-TNC Fab' in EAM and Control Rats

The dose-dependent changes in biodistribution of ¹¹¹In anti-TNC Fab' in EAM rats showed that the tracer uptake was higher with 10 µg radiolabeled antibodies in the liver and spleen than with 50 or 100 µg radiolabeled antibodies. In the heart, the tracer uptake was lower with 100 µg antibodies than with 10 or 50 µg antibodies. Thus, the antibody dose of 50 µg per rat was used in further experiments.

The comparison of radioactivity distribution between anti-TNC antibody and nonspecific antibody in EAM rats is summarized in Table 2. In the heart, much higher radioactivity was observed with an injection of ¹¹¹In anti-TNC Fab' compared with an injection of ¹¹¹In nonspecific Fab' (2.60±0.32 for ¹¹¹In anti-TNC Fab' versus 0.32±0.06 for ¹¹¹In nonspecific Fab'). Radioactivity of ¹¹¹In anti-TNC Fab', compared with ¹¹¹In-nonspecific Fab', was lower in the kidney and higher in the blood, liver, and spleen.

View this table: [in this window] [in a new window]   Table 2. Comparison of Biodistribution Between 111In Anti-TNC Fab' and Nonspecific Fab' in EAM Rats at 6 h After Injection

Histopathologic and Quantitative Autoradiographic Study
By autoradiography, high radioactivities were observed in the region indicative of inflammation in EAM rats administered ¹¹¹In anti-TNC Fab' (Figure 3, row 1). No accumulation of radioactivity was observed in EAM rats with ¹¹¹In nonspecific Fab' (row 2) or in normal rats with ¹¹¹In anti-TNC Fab' (row 3).

View larger version (111K): [in this window] [in a new window]   Figure 3. H-E stain (a), schema of H-E stain (b), and autoradiography (c) of adjacent sections from hearts of 3 rats (1 and 2, EAM rats; 3, normal rat) administered radiolabeled Fab' (1, anti-TNC Fab'; 2 and 3, nonspecific Fab'). Dark-gray lesions in schema show areas of inflammatory cell infiltration and myocardial cell damage.

The ratios of autoradiographic intensities of each myocardial tissue in each rat group are summarized in Table 3. Because the original autoradiographic images were very small, regions of interest were placed on the autoradiograms of the whole myocardium in this analysis. High accumulation of ¹¹¹In anti-TNC Fab' in EAM rat hearts was clearly shown.

View this table: [in this window] [in a new window]   Table 3. Autoradiographic Intensity Averages

In Vivo Imaging
Finally, we examined whether ¹¹¹In anti-TNC Fab' imaging could be used to detect in vivo myocardial injury. SPECT imaging (Figure 4a) and autoradiography (Figure 4d) clearly showed the focal uptake of ¹¹¹In anti-TNC Fab' (Figure 4a). ^99mTc-MIBI myocardial perfusion imaging (Figure 4b) demonstrated the image complementary to ¹¹¹In anti-TNC Fab' (Figure 4c).

View larger version (60K): [in this window] [in a new window]   Figure 4. Transverse dual-isotope tomographic images of 111In anti-TNC Fab' and 99mTc-MIBI in EAM rat. a, Arrow shows focal uptake of 111In anti-TNC Fab'. b, 99mTc-MIBI myocardial perfusion image is shown. c, Superimposed image demonstrated that focal uptake of 111In anti-TNC Fab' was detected on interventricular septum (S). d, Autoradiography. A indicates anterior; L, lateral; and P, posterior.

	Discussion

Top Abstract Introduction Methods Results Discussion References

 
Our results demonstrate that the myocardial uptake of ¹¹¹In anti-TNC Fab' was significantly higher in EAM rats than in control rats. By autoradiography, high radioactivities were clearly observed in the regions indicative of inflammation in EAM rats. SPECT imaging demonstrated the suitability of this tracer for in vivo imaging.

We have recently reported that TNC was expressed at the initial stage of myocarditis in an autoimmune mouse model before necrosis or inflammatory cell infiltration was histologically apparent.¹³ This result reveals the potential of early diagnosis of myocarditis by anti-TNC imaging. Moreover, the expression level of TNC might reflect the degree of inflammatory reactions.¹³

TNC expression is also induced in the injured cardiomyocytes in various heart diseases during the active stage.^24,25 We recently demonstrated that TNC is expressed transiently in the border zone of myocardial infarction in a rat model.²¹ These data show the potential usefulness of this imaging for other forms of myocardial injury. TNC is also recognized in human coronary atherosclerotic plaque²⁶ or restenotic neointima after angioplasty, ²⁷ suggesting that molecular imaging of TNC might become a useful tool for vascular injury.

¹¹¹In antimyosin Fab' imaging can visualize active myocyte damage^28,29 and, thus, has been used to diagnose myocarditis.^{30 99m}Tc annexin-V imaging has recently been reported for the noninvasive identification of apoptotic cell death in patients with cardiac allograft rejection pathologically similar to autoimmune myocarditis.³¹ Further studies are necessary to determine whether anti-TNC imaging is superior to anti-myosin and annexin-V imaging.

In the present study, the anti-TNC antibody fragment was labeled with ¹¹¹In by using EMCS-Bz-EDTA, so that the radioactivity provides inherent in vivo behaviors of the antibody fragment.^22,32 Western blot analysis confirmed that the anti-TNC monoclonal antibody, 4F10TT, bound to 2 isoforms of rat TNC (Figure 1). Specific accumulation of 4F10TT in the inflammatory myocardium was confirmed by significantly lower accumulation of the nonspecific antibody in the hearts of EAM rats (Table 2). The regions of high accumulation of ¹¹¹In anti-TNC Fab' in ex vivo imaging (autoradiography) coincided well with the regions of inflammatory cell infiltration (Figure 3), indicating that anti-TNC Fab' is highly specific to the inflammatory region of myocarditis. This was strongly supported by SPECT imaging, in which focal uptake of ¹¹¹In anti-TNC Fab' was clearly demonstrated at sites complementary to ^99mTc-MIBI uptake (Figure 4). This finding also suggests that anti-TNC antibody fragments would be useful for clinical imaging, although further manipulation of the radioactivity levels in the blood, kidney, and liver is necessary.^{33– 35}

Although inflammation and the expression of TNC in EAM rats peak at 21 days after the first immunization,¹⁷ all experiments were performed at 17 days because the hemodynamic abnormalities are too severe at 21 days to evaluate the kinetics of the tracer. In EAM rats, there is a characteristic initial focal inflammatory response in the myocardium, followed by massive myocardial damage at 21 days. In addition, the extent of TNC expression at 17 days is somewhat variable, as shown in Figure 3, a and b, and in Figure 4.

In conclusion, we investigated the inherent biodistribution of anti-TNC antibody Fab' fragments in the EAM rat model. The present study indicated a high ability of the antibody fragment to localize sites of inflammation in the heart by ex vivo and in vivo imaging. Although further studies are required, radiolabeled anti-TNC fragments may be an attractive radiopharmaceutical for the noninvasive diagnosis of myocarditis.

Received March 22, 2002; accepted June 12, 2002.

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