Inhibitory Effect of TAS-301, a New Synthesized Constrictive Remodeling Regulator, on Renarrowing after Balloon Overstretch Injury of Porcine Coronary Artery

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Sasaki, E.
	Articles by Matsuura, N.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Sasaki, E.
	Articles by Matsuura, N.

Vol. 295, Issue 3, 1043-1050, December 2000

Inhibitory Effect of TAS-301, a New Synthesized Constrictive Remodeling Regulator, on Renarrowing after Balloon Overstretch Injury of Porcine Coronary Artery

Eiji Sasaki, Yasutaka Tanahashi, Yasundo Yamasaki, Nobuyuki Oda, Yoshihisa Nozawa, Hiroshi Terakawa, Kazuhisa Miyoshi, Yoshiyuki Muranaka, Hidekazu Miyake and Naosuke Matsuura

Cardiovascular Science Research Laboratory (E.S., Y.T., Y.Y., N.O., H.T., K.M., Y.M., H.M.) and Pharmacological Research Laboratory (Y.N., N.M.), Hanno Research Center, Taiho Pharmaceutical Co., Ltd., Hanno-City, Saitama, Japan

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

The purpose of this study was to determine the efficacy and the possible mechanism of action of a recently synthesized drug,TAS-301 [3-bis(4-methoxyphenyl)methylene-2-indolinone], on stenosisafter balloon overstretch injury of porcine arteries. We measuredthe diameter of vessels by angiography and conducted histologicalanalysis. The oral administration of TAS-301 kept dilated theangiographic luminal diameter of injured segment 4 weeks afteroverstretch injury and reduced calculated stenosis ratio in adose-dependent manner, significantly reducing it at doses of 30and 100 mg/kg. Histopathological analysis showed that TAS-301significantly reduced the adventitial area at doses of 30 and100 mg/kg with moderate reduction of the neointimal area, resultingin the larger residual lumen. In an in vitro assay, TAS-301 dosedependently inhibited the proliferation of adventitial fibroblastsstimulated by basic fibroblast growth factor or transforming growthfactor- $beta$ ₁. In addition, the drug reduced adventitial fibroblast-mediatedthree-dimensional collagen gel contraction. These findings indicatethat TAS-301, the first compound developed for targeting the constrictiveremodeling, showed a high inhibitory potency on coronary arterystenosis of micropigs after injury, mainly due to inhibition ofadventitial fibroblast proliferation and of the contractile abilityof myofibroblasts. Our results suggest the strong possibilitythat TAS-301 may be efficacious for prevention of restenosis afterangioplasty and the need to examine the therapeutic usefulnessof this drug in clinicaltrials.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Percutaneous transluminal coronary angioplasty (PTCA) has become increasingly important in the management of coronary arterydisease. However, restenosis in 30 to 40% of PTCA patients limitsits usefulness (Kuntz and Baim, 1993). Although the pathogenesisof this process is multifactorial, the formation of a neointimais common after balloon injury. Histological studies have shownthat intimal thickening in the restenotic lesion contains smoothmuscle cells in an abundant extracellular matrix. Although anincreasing amount of experimental evidence suggests that the proliferationof smooth muscle cells after balloon injury is the most likelymechanism for the development of postangioplasty restenosis, thereis controversy regarding the degree of the proliferative responsein biopsies from clinical postangioplasty restenotic lesions (Schwartzet al., 1992; Isner et al., 1994). Furthermore, in spite of encouragingresults in animal models, no systemic pharmacological agent hasbeen shown conclusively to produce a clinically worthwhile reductionin restenosis after PTCA (Franklin and Faxon, 1993; Moliternoand Topol, 1996).

Most of the therapies for preventing restenosis tested so far have been directed against neointimal hyperplasia. However,clinical observations have questioned prior assumptions that neointimaformation solely correlates with luminal narrowing (Luo et al.,1996; Mintz et al., 1996). This implies that neointimal hyperplasiais not the sole mechanism of restenosis after conventional balloonangioplasty in humans. Recent experimental and clinical studieshave suggested that late vessel constriction and vasospasm maybe the major factor (Ardissino et al., 1991; Kakuta et al., 1994;Mattsson and Clowes, 1995; Andersen et al., 1996).

Pigs have been used as models for postangioplasty restenosis with some success. Injury to porcine coronary arteries by PTCAusing an overexpanded balloon catheter stimulates the formationof vascular lesions morphologically similar to those seen in humanpostangioplasty restenosis (Muller et al., 1992). An advantageof this model is the ability of the investigator to study coronaryarteries rather than peripheral vessels. The findings in thismodel have shown that coronary injury results in a significantvasoconstriction, induced by autacoid from activated platelets,and in a significant remodeling of the adventitia, accompaniedby the proliferation and differentiation of adventitial fibroblastsinto myofibroblasts, which acquire $alpha$ -smooth muscle actin, duringthe formation of neointima (Kadokami et al., 1996; Scott et al.,1996; Shi et al., 1996a,b).

On the basis of the fact that there are striking similarities between the process of wound healing and the adventitial responseof the arterial wall to injury and because stimulation of adventitiato proliferate and constrict after angioplasty is thought to beone of the typical wound-healing processes (Darby et al., 1990;Clark, 1993; Yokozeki et al., 1997), we developed TAS-301, a newsynthesized constrictive remodeling regulator, and tested it onthree-dimensional (3D) collagen gel contraction, which is a frequentlyused and previously established in vitro model for wound repairprocess (Bell et al., 1979; Grinnell et al., 1994). TAS-301 showeda potent inhibitory effect on type-I collagen gel contractioncaused by fibroblasts precultured with TGF- $beta$ ₁, which cells acquireda strong gel-contracting ability under low-serum culture conditions(E. Sasaki, Y. Yamasaki, Y. Tanahashi, Y. Muranaka, H. Terakawa,K. Miyoshi, N. Oda, H. Miyake, and N. Matsuura, submitted). Wehave previously indicated that this compound potently inhibitsthe intimal thickening after balloon injury to rat common carotidartery due to inhibition of both migration of medial smooth musclecells and proliferation of medial and intimal smooth muscle cells(Muranaka et al., 1998).

In the present study, we undertook an examination of the possible effect of TAS-301 on stenosis after balloon overstretchinjury of porcine coronary arteries by measuring the diameterof vessels by angiography and conducting histological analysis,based on the results of the above-mentioned in vitro experimentson the proliferation of and 3D collagen gel contraction by adventitialfibroblasticcells.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Twenty-eight male Yucatan micropigs (18.4-29.2 kg; Charles River Laboratories, Wilmington, MA) were used in this study. Theanimals were housed in constant-temperature facilities and givenstandard lab chow and water ad libitum. All experiments were carriedout according to protocols approved by the Institutional AnimalCare and UseCommittee.

Animal Preparation. Animal experiments were performed as previously reported with minor modification (Hata et al., 1995). Each animal was randomlyassigned to one of the following five groups: control group (n= 5); TAS-301 10-mg/kg-treated group (n = 5); TAS-301 30-mg/kg-treatedgroup (n = 5); TAS-301 100-mg/kg-treated group (n = 5); or normalgroup (n = 5). In all groups except for the normal group, balloondilation was performed in the left anterior descending coronaryartery as describedbelow.

The animals were anesthetized with ketamine hydrochloride (20 mg/kg i.m.) followed by sodium pentobarbital (15 mg/kg i.v.).After incision of the right neck skin had been made, we carefullydissected the right common carotid artery. A balance human PTCAballoon catheter (BAL3, 3.5 mm inflated diameter, 2 cm; Navius,Rancho Cordova, CA) was advanced from the right common carotidartery into the left anterior descending coronary artery underfluoroscopy. The balloon was then inflated at 8 atm for 30 s,and this procedure was repeated two times at a 1-min intervalin eachanimal.

Experimental Protocol. Coronary arteriography was performed 3 min after intracoronary administration of nitroglycerin (20 µg/ml), which was givenbefore balloon dilation, immediately after the balloon dilation,and 4 weeks after the balloon dilation procedure to document changesin lumen size. Nitroglycerin treatment was performed to assessorganic stenosis in maximally dilated state. Furthermore, coronaryarteriography was also performed 3 min after intracoronary administrationof serotonin (10 µg/ml), 4 weeks after the balloon dilation procedure,to document changes in lumen size. TAS-301 (10, 30, and 100 mg/kg)was administered daily as a dietary admixture, from 1 day beforethe balloon dilation until 4 weeks afterit.

Data Analysis. The photocopies in end-diastolic frame were made for measurements of coronary artery diameter by use of commercially availablesoftware (CAM-1000; Nishimoto, Tokyo, Japan). The size of thecatheter was used to calibrate the actual vessel diameter in millimeters.The percentages of increase in and narrowing of the coronary diameterafter dilation procedure were calculated as follows: luminal dilation(%) = diameter immediately after balloon dilation (mm)/diameterbefore balloon dilation (mm) × 100, and luminal stenosis (%) =(1 $-$ diameter 4 weeks after balloon dilation (mm)/diameter immediatelyafter balloon dilation (mm)) ×100.

Vasoconstriction (vasoreactivity) after serotonin treatment was expressed as a percentage of the diameter at 4 weeks afterballoon dilation, which was assessed using the following equation:vasoreactivity (%) = diameter after serotonin treatment (mm)/diameterbefore serotonin treatment (mm) ×100.

Histopathological Approach. After the final arteriography, the arteries were perfused with 10% buffered formalin for 10 min at 100 mm Hg pressure. Fouror five cross-sectional segments in the lesion area were embeddedin paraffin. Sections were then cut (5 µm) and stained with H&Eor with Van Gieson elastin stain. From photographs of all sections,the areas for adventitia, media, intima, and lumen were measured;and the ratio for intimal area to medial area, that for adventitialarea to medial area, and that for luminal area to intimal plusluminal areas were calculated and compared betweengroups.

Cell Culture. Adventitial fibroblast cells from normal and injured coronary artery were isolated by an enzyme dispersion method using collagenase,as previously reported (Chamley-Campbell et al., 1981). The cellswere maintained in Dulbecco's modified Eagle's medium (DMEM),supplemented with 10% fetal bovine serum (FBS), 100 U/ml penicillin,100 U/ml streptomycin, and grown in a moist atmosphere of 95%air and 5% CO₂ at 37°C. For immunocytochemistry using antibodyagainst $alpha$ -smooth muscle actin (Boehringer Mannheim Biochemicals,Tokyo, Japan), these cells isolated from normal artery were faintlypositive, whereas they were markedly positive after having beenprecultured with TGF- $beta$ ₁ for 7 days (data not shown). It has beendemonstrated that TGF- $beta$ ₁ can induce $alpha$ -smooth muscle actin expressionin fibroblasts and cause these cells to change phenotypicallyinto myofibroblasts (Arora and McCulloch, 1994). Therefore, weidentified these cells as fibroblasts. Cells were passaged bytrypsinization (0.1% trypsin/0.02% EDTA in PBS; Kojin-Bio, Saitama,Japan) and were used at a subconfluent stage in passage 5 to9.

In Vitro Proliferation Assay. Cell proliferation was determined by incorporation of 5-bromo-2'-deoxyuridine (BrdU) by quiescent cells, as described previously(Magaud et al., 1988). Adventitial fibroblast cells were seededat 3 × 10³ cells/well in 96-well plates in DMEM containing 10% FBS. Threedays after the seeding, their growth was minimally arrested for5 days in DMEM containing 1% FBS. Then, the DMEM was removed andserum-free DMEM containing 0.1% BSA with or without TAS-301 wasadded to the quiescent cells 2 h before treatment with the desiredgrowth factor, i.e., TGF- $beta$ ₁ (1 pg/ml) or bFGF (10 ng/ml). Sixteenhours after stimulation, BrdU (10 µM) was added to the cultures,and 2 h later the cells were fixed. An enzyme-linked immunosorbentassay system was used according to the manufacturer's recommendations(RPN250; Amersham, Amersham, England) to detect and to quantifythe incorporated BrdU. The drugs were present during the entiretime of theexperiments.

Preparation of 3D Collagen Gel Culture. Collagen gels (3D) were prepared essentially as described previously (Zhang et al., 1996; Yokozeki et al., 1997). Adventitialfibroblasts-populated collagen gels were prepared by rapidly mixingtogether a suspension of fibroblast cells in DMEM with porcineskin type I collagen stock solution (3 mg/ml) and pouring themixture into a 24-well plate (Iwaki Co., Tokyo, Japan) that hadbeen precoated with 2% BSA dissolved in PBS. The plates were immediatelyincubated at 37°C in 95% air + 5% CO₂ to promote collagen fibrillogenesis.Under these conditions, the pH of the media remained neutral exceptfor a few seconds immediately upon addition of the collagen stocksolution. The cell-containing solution usually gelled within 1h after pouring. In the experiments described below, the finalFBS concentration was 0.1%; and the final cell concentration,1.5 × 10⁵/ml. The final collagen concentration was always 0.75 mg/ml. Aftergelation was complete, the gels were loosened or detached fromthe well surface by vigorous shaking. To determine the efficacyof TAS-301 on collagen gel contraction, this agent was incubatedwith the fibroblast cell suspension for 2 h before the cells weremixed with collagen stock solution. Collagen gel contraction wasdetermined by using NIH Image software to measure the area ofthe detached gel on the plates at 24 h after gel formation. Forthese in vitro assays, drugs were dissolved in dimethyl sulfoxideand diluted inmedium.

Materials. TAS-301 was synthesized by Taiho Pharmaceutical Co., Ltd. (Saitama, Japan). The following reagents with their source in parentheses,were used: serotonin (Sigma Chemical Co., St. Louis, MO), bFGFand TGF- $beta$ ₁ (Life Technologies, Grand Island, NY), and type I collagenstock solution (porcine skin; Wako Pure Chemical, Osaka,Japan).

Statistical Analysis. All data are expressed as means ± S.E.M. Multiple comparisons with vehicle were tested by Dunnett's multiple comparison test.Statistically significant differences between two groups werecalculated by (two-tailed) Aspin-Welch's t test. A P value <.05was considered to indicate statisticalsignificance.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Group Characteristics. There were no significant differences in animal weight among the control and three experimental groups at the time of theballoon injury. Three of 28 micropigs died during the initialprocedure. These deaths were attributed to ventricular arrhythmia.Heart rate and arterial pressure under anesthesia did not differamong the four groups (data notshown).

Angiographic Analysis. Angiographic analysis was performed with a computer-based system to determine the degree of vessel stretch, which was measuredas the ratio of artery diameter during and after balloon inflationto diameter before balloon inflation (Table 1). The mean LADcoronary artery diameter was not significantly different amongthe groups. Similarly, the luminal dilation after balloon injurydid not differ among groups: there was a greater than 40% averageincrease in vessel diameter after the injury (control group, 45.0± 1.5%; TAS-301 at 10 mg/kg, 41.0 ± 2.2%; at 30 mg/kg, 42.3 ±4.3%; and at 100 mg/kg, 43.5 ± 5.2%). This large stretch was associatedwith greater injury, as shown later.

View this table:
[in this window]
[in a new window]

TABLE 1
Effect of TAS-301 on LAD diameter of coronary artery in PTCA balloon-injured micropig
All data are shown as mean ± S.E.M.

Consistent with previous findings in this model, significant changes were noted in the angiographic luminal diameter of theinjured segment 4 weeks after overstretch injury in the controlgroup. The calculated luminal stenosis ratio was 40.3 ± 2.3% forthe control group, and the treatment with TAS-301 decreased thisstenosis ratio in a dose-dependent manner, significantly reducingit at doses of 30 and 100 mg/kg (21.5 ± 2.5 and 15.2 ± 4.1%, respectively;Fig. 1). Typical angiograms of LAD coronary arteries before and4 weeks after overstretch in micropigs of the control group andTAS-301 (100 mg/kg)-treated group are shown in Fig. 2.

View larger version (39K):
[in this window]
[in a new window]

Fig. 1. Effects of TAS-301 on stenosis ratio (%) 4 weeks after the balloon injury. Data show stenosis % (details under Experimental Procedures, mean ± S.E.M., n = 5). **P < .01 versus control (Dunnett's multiple test). Note the significant reduction of stenosis % by treatment with TAS-301.

View larger version (94K):
[in this window]
[in a new window]

Fig. 2. Coronary angiogram of left coronary artery after overstretch of the vessel in a micropig. A, immediately after the balloon injury. B, 4 weeks after the injury in control micropig. C, 4 weeks after the injury in a TAS-301 (100 mg/kg)-treated micropig. Note the remarkable reduction in the diameter of LAD coronary artery in the control 4 weeks after the injury and preservation of coronary artery diameter by the treatment with TAS-301.

Coronary Vasoreactivity. Table 2 shows the magnitude of vasoconstriction 4 weeks after angioplasty. Four weeks after the balloon injury, the vasoreactivityof the coronary artery was evaluated arteriographically afterintracoronary administration of serotonin. At a dose of 10 µg/kg,serotonin caused significant hyper-reactive vasoconstriction atthe angioplasty sites in control micropigs, whereas it did notinduce remarkable vasoconstriction at control sites in normalmicropigs, as previously described (Kadokami et al., 1996). Thetreatment with TAS-301 increased the diameter of coronary arteryin a dose-dependent manner before administration of serotonin.Administration of the monoamine induced vasoconstriction at theangioplasty sites in TAS-301-treated micropigs. This serotonin-inducedcoronary vasoreactivity (constriction ratio of diameter) in eachgroup of TAS-301-treated micropigs was similar to that seen inthe control micropigs. This means that TAS-301 did not have anyantagonistic effect against serotonin and did not change the vasoreactivityof the coronary artery.

View this table:
[in this window]
[in a new window]

TABLE 2
Effect of TAS-301 on LAD diameter of coronary artery treated with serotonin in PTCA balloon-injured micropig
All data are shown as mean ± S.E.M. Vasoreactivity is presented as the percentage ratio of LAD diameter before and after serotonin administration.

Histological Analysis. Histopathological analysis was performed on all injured segments (four to five sections per vessel). As previously reported(Shi et al., 1996a), there was rupture of the internal elasticlamina, with neointima growth replacing the disrupted media 4weeks after injury in all animals. The degree of injury achievedin TAS-301 treatment and control groups was probably rather uniformbecause all vessels included in the analysis demonstrated ruptureof the internal elastic lamina and eccentric lesions. Furthermore,adventitial thickness increased compared with that of normal vessels.As depicted in Fig. 3, the most striking changes in adventitialdimensions were found in the regions adjacent to the site of medialinjury. In contrast, the thickness of the adventitia oppositethe medial injury or in other uninjured sections from the samevessels remained largely unaffected. Several independent morphometricmeasurements of the vessels were performed to assess the responseto injury.

View larger version (64K):
[in this window]
[in a new window]

Fig. 3. Cross-section of micropig coronary artery 4 weeks after balloon injury. A, control. B, TAS-301, 100-mg/kg treatment. A, large neointimal lesion that fills the gap in the disrupted media is present. The adventitia exhibits thickening in the vicinity of the medial injury compared with the thickness on the opposite site of the same section in control. B, note the reduction in adventitial thickness by TAS-301 treatment. A, adventitia; I, intima; M, media; L, lumen. Scale bar, 200 µm.

To determine whether TAS-301 altered the response to injury, first we determined the extent of neointimal formation in eachgroup (Fig. 4). The average intimal area and the ratio of intimalarea to medial area (I/M) should reflect the proliferative responseat the site of vessel injury and thus serve as the best indicatorsof the ability of TAS-301 to reduce neointimal mass after injury.Animals receiving TAS-301 showed a reduced I/M, i.e., 238.7 ±12.5% for the control group, 205.2 ± 40.6% for TAS-301 at 10 mg/kg,160.8 ± 24.8% for TAS-301 at 30 mg/kg, and 150.9 ± 12.1% for TAS-301at 100 mg/kg; and the absolute intimal area was 1.59 ± 0.15 mm² for the control group, 1.23 ± 0.21 mm² for the drug at 10 mg/kg, 1.21 ± 0.18 mm² for the drug at 30 mg/kg, and 1.14 ± 0.08 mm² for the drug at 100 mg/kg. The effect on both measurements wasthus dose dependent. However, these changes in intimal formationwere not significant, but a clear tendency was observed in thehigh-dose TAS-301 group. Second, the extent of adventitial changewas determined in each group (Fig. 4). The average adventitialarea and the ratio of adventitial area to medial area (A/M) alsoreflect the proliferative response at the site of vessel injuryand thus serve as the best indicators of the ability of TAS-301to reduce adventitial mass after injury. Animals receiving TAS-301showed a decreased adventitial thickness or A/M (282.6 ± 19.8%for the control group, 240.5 ± 20.4% for TAS-301 at 10 mg/kg,186.0 ± 21.0% for TAS-301 at 30 mg/kg, and 184.5 ± 13.6% for thedrug at 100 mg/kg); and a decreased absolute adventitial area(1.88 ± 0.09 mm² for the control group, 1.52 ± 0.05 mm² for TAS-301 at 10 mg/kg, 1.44 ± 0.17 mm² for TAS-301 at 30 mg/kg, and 1.41 ± 0.07 mm² for the drug at 100 mg/kg). These dose-dependent changes in theadventitia caused by TAS-301 treatment were significant at dosesof 30 and 100 mg/kg. The residual lumen (the ratio of luminalarea to intimal plus luminal area) was determined to demonstratethe change in vessel geometry after injury and repair and maymore closely parallel the clinical entity of restenosis. As illustratedin Fig. 4, the residual lumen was dose dependently larger in theTAS-301 treatment groups, and the effect of TAS-301 at doses of30 and 100 mg/kg were significant (45.5 ± 1.9% for the controlgroup, 63.0 ± 3.7% for TAS-301 at 30 mg/kg, and 66.0 ± 1.4% forTAS-301 at 100 mg/kg).

View larger version (27K):
[in this window]
[in a new window]

Fig. 4. Effects of TAS-301 on histological parameter 4 weeks after balloon injury to micropig coronary artery. A, ratio of intimal area to medial area (%). B, ratio of adventitial area to medial area (%). C, residual lumen (%). Data are expressed as means ± S.E.M. of five micropigs. *P < .05, **P < .01 versus control (Dunnett's multiple test). Note the significant reduction in the ratio of adventitial area to medial area and increase in residual lumen (%) by treatment with TAS-301.

Adventitial Fibroblast Proliferation (In Vitro Assay). The hypercellularity of the adventitial layer and proliferation of fibroblasts are believed to be associated with the developmentof the thickened adventitia in the coronary artery injury modelin micropigs, and TAS-301 caused a significant reduction in adventitialthickness 4 weeks after overstretch injury in this study. As bFGFand TGF- $beta$ ₁ are well known mitogens for fibroblasts, the effectof TAS-301 on the proliferation of micropig adventitial fibroblastsstimulated by these cytokines in vitro was examined (Fig. 5).

View larger version (31K):
[in this window]
[in a new window]

Fig. 5. Effects of TAS-301 on bFGF- (A) and TGF- $beta$ ₁- (B) induced BrdU incorporation into adventitial fibroblast cells. Data show BrdU incorporation (O.D.) induced by bFGF or TGF- $beta$ ₁ treatment (mean ± S.E.M., n = 8 except for basal condition, n = 4). *P < .05, **P < .01 versus control (Dunnett's multiple test). ^##P < .01 versus control (Aspin-Welch's t test). Note the potent inhibitory effect of TAS-301 on BrdU incorporation into the cells.

Pronounced BrdU incorporation by the cells, an index of DNA synthesis, was induced by the treatment with bFGF (0.03-100 ng/ml)or TGF- $beta$ ₁ (0.003-10 pg/ml), and submaximum incorporation was observedwith bFGF at a dose of 10 ng/ml or TGF- $beta$ ₁ at a dose of 1 pg/ml(data not shown). TAS-301 reduced bFGF (10 ng/ml)-induced BrdUincorporation (O.D. change: 0.072) in a dose-dependent manner(1 to 10 µM) and significantly inhibited it at doses of 3 and10 µM, by 64.3% (P < .05) and 95.3% (P < .01), respectively. Furthermore,TAS-301 also reduced TGF- $beta$ ₁ (1 pg/ml)-induced BrdU incorporation(O.D. change: 0.160) in a dose-dependent manner (1 to 10 µM) andsignificantly inhibited it at a dose of 10 µM, by 77.0% (P < .05).

Gel Contraction by Adventitial Fibroblast (In Vitro Assay). Because the alteration of the adventitial fibroblast phenotype to the myofibroblastic one is believed to be associated withthe development of a thickened adventitia and because the constrictiveability of myofibroblasts contributes to the narrowing of thevessel lumen after coronary artery injury, we decided to examinethe 3D collagen gel contraction model using adventitial fibroblastsfrom the angioplasty sites 4 weeks after injury in micropigs (INJ-fibroblasts)as an extrapolation model for the in vivo constrictive remodelingresulting in restenosis after angioplasty. In this model, we foundthat the degree of gel contraction was dependent on both serumconcentration and cell density; and we determined the optimalconditions to be an FBS concentration of 0.1% and a cell concentrationof 1.5 × 10⁵ cells/ml (data notshown).

INJ-fibroblasts showed a higher constrictive ability than the adventitial fibroblasts from normal coronary artery when incubatedin 0.1% FBS-containing medium. TAS-301 reduced the strong contractileability of INJ-fibroblasts significantly and concentration dependently(Fig. 6). Its inhibitory effect was 20.7, 44.8, and 77.6% at 0.3,1, and 3 µM, respectively.

View larger version (30K):
[in this window]
[in a new window]

Fig. 6. Effect of TAS-301 on collagen gel contraction by INJ-fibroblasts. Collagen gels were prepared by mixing 1.5 × 10⁵ cells/ml of INJ-fibroblasts (after preincubation of the cells with various doses of TAS-301 for 2 h) and 0.75 mg/ml type I collagen and then incubated in the presence of 0.1% FBS for 24 h. Data are expressed as means ± S.E.M. of six collagen gels. Note the potent reduction in the contractile ability of INJ-fibroblasts by the treatment with TAS-301. *P < .05, **P < .01 versus control (Dunnett's multiple test). ^##P < .01 versus control (Aspin-Welch's t test).

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

Recent advances in interventional cardiology have led to more aggressive strategies to relieve coronary obstruction. Thus,a deep medial injury that may potentially affect the adventitiaappears to be common in clinical practice. The possibility ofmyofibroblast formation and the deposition of extracellular matrixin the adventitia after coronary artery injury in humans may leadto vascular tissue retraction (den Heijer et al., 1994; Shi etal., 1996a). In fact, recent findings obtained by the intravascularultrasound technique appear to corroborate this possibility (DiMario et al., 1994). The failure of many pharmacological approachesto reduce restenosis in clinical settings has stimulated considerableinterest in site-specific therapy after coronary angioplasty.Furthermore, the successful application of a vascular stent tothe atherosclerotic plaque, resulting in less frequency of restenosis,has shown the importance of preserving the vessel in the dilatedstate; but its use is still limited, by few sites conductive toapplication, induction of coagulation, and restenosis due to intimalhyperplasia (Marso et al., 1999). The involvement of the adventitiain the vascular repair process may require the development ofstrategies allowing for the administration of potentially activecompounds to this site (Edelman et al., 1993; Hadeishi et al.,1994).

On the basis of this background, we synthesized TAS-301 as a first trial drug to target constrictive remodeling and developedit for the prevention of restenosis after angioplasty. The majorfinding of this study is that TAS-301 reduced the vascular responseto balloon injury without changing vasoreactivity, as demonstratedmainly by a larger lumen diameter and decreased A/M ratio as judgedby angiographical and histopathological analysis 4 weeks afterinjury.

Several recent studies on the vessel response to injury as it pertains to clinical restenosis have suggested that two measurementsof this response should be independently evaluated: the growthof neointima, as a marker of the biological response to injury,and the follow-up luminal diameter, as a marker to the clinicalsignificance of the result. Because there was no significant reductionin intimal area or I/M ratio in this study, we cannot relate theincrease in lumen diameter observed to a change in smooth musclecell proliferation and intimal mass. Recent analysis of the relationbetween intimal mass and lumen diameter has failed to show a significantcorrelation between these variables. Scott et al. (1996) indicatedthat cell proliferation at the earliest time point after angioplastyof porcine coronary arteries was greater in the adventitia thanin the media and that the adventitia may be an important regionwith respect to the first wave of growth after angioplasty ofcoronary arteries. Furthermore, they hypothesized that the cellsthat proliferate in the adventitia may also contribute to vascularlesion formation by synthesizing growth and/or differentiationfactors. Their study suggests that the adventitia may play a rolein vascular lesion formation by contributing to the cellular massof the neointima and the synthesis of growth factors and alsothe adventitia may contribute to vascular remodeling and constrictionof the external elastic lamina through an accumulation of myofibroblastsin the adventitia surrounding the injurysite.

In view of the striking similarities between the process of wound healing and the response of the adventitial fibroblaststo injury, we tested TAS-301 on the basis of this wound-healingrestenosis hypothesis by using adventitial fibroblast-populatedcollagen gel matrix that forms a three-dimensional lattice usingadventitial fibroblasts. TAS-301 inhibited the gel contractionby fibroblasts taken from the overstretched coronary artery 4weeks after injury, to the same extent as neutralizing antibodyagainst TGF- $beta$ _1,2,3 (E. Sasaki, Y. Yamasaki, Y. Tanahashi, Y. Muranaka,H. Terakawa, K. Miyoshi, N. Oda, H. Miyake, and N. Matsuura, submitted).The change of phenotype from fibroblast to myofibroblast may havecontributed to the constrictive remodeling resulting in renarrowingof the coronary artery after angioplasty, and TAS-301 might haveprevented thischange.

Furthermore, TAS-301 showed potent inhibition of mitogen (bFGF and TGF- $beta$ ₁, well known mitogen for fibroblast)-induced proliferationof adventitial fibroblasts. Previously, we reported that TAS-301potently inhibited the migration of rat vascular smooth musclecells induced by PDGF-BB, insulin-like growth factor-1, and heparin-bindingepidermal growth factor-like growth factor and also inhibitedthe proliferation induced by bFGF in vitro (Muranaka et al., 1998).When rat vascular smooth muscle cells were stimulated with PDGF-BB,TAS-301 inhibited the transient and sustained increase in freeintracellular Ca²⁺ concentration, as monitored by Fura-2 fluorescence (Sasaki etal., 2000). This finding indicates that TAS-301 inhibits intracellularCa²⁺ mobilization via intracellular Ca²⁺ release and extracellular Ca²⁺ influx induced by PDGF-BB. Considering that TGF- $beta$ and bFGF induceextracellular Ca²⁺ influx in fibroblasts (Muldoon et al., 1988; Munaron et al.,1995), we guess that TAS-301 inhibits the proliferation of adventitialfibroblasts by regulating TGF- $beta$ and bFGF-induced intracellularCa²⁺mobilization.

Preliminarily, we determined that the plasma level of TAS-301 given to micropigs at the dose of 100 mg/kg was maintained atover 3 µM during the experimental period, because TAS-301 wasadministered daily as a dietary mixture. Because the concentrationof TAS-301 we used in the in vitro experiment is almost consistentwith its plasma concentration in the micropigs, these in vitroeffects also might have resulted in the reduction in the adventitialthickness and increment of residual lumen diameter of the coronaryartery 4 weeks after the angioplastic injury. TGF- $beta$ ₁ is involvedin tissue repair by modulating the growth of mesenchymal cells,augmenting the synthesis of several extracellular matrix proteins,and facilitating both migration and proliferation of fibroblasts(Miyazaki et al., 1998). Myofibroblasts represent highly specializedmesenchymal cells that play a central role in tissue repair. Ithas also been suggested that TGF- $beta$ ₁ provides the signal for fibroblaststo acquire a differentiated phenotype that imparts synthetic andmechanical properties (Desmouliere et al., 1993; Arora and McCulloch,1994; Shi et al., 1996c). Previously, we found that the strong3D gel-contracting ability of fibroblasts from injured coronaryartery could be blocked by antibody against TGF- $beta$ _1,2,3. Furtherinvestigation on the contribution of TGF- $beta$ ₁ in this model is neededto understand the precise mechanism of TAS-301 action in vascularremodeling.

In summary, our new synthesized TAS-301, a first compound developed for targeting constrictive remodeling, inhibited coronaryartery stenosis of micropigs after injury as judged angiographically.This effect of TAS-301 appears to be due to a reduction in adventitialfibroblast proliferation and lessened contractile ability of myofibroblasts.This highly potent activity of TAS-301 suggests the potentialuse of this drug for the prevention of restenosis after angioplastyvia regulation of arterial remodeling by adventitial fibroblastsand the need to examine the therapeutic usefulness of this drugin clinicaltrials.

	Footnotes

Accepted for publication August 10, 2000.

Received for publication February 1, 2000.

Send reprint requests to: Yasundo Yamasaki, Cardiovascular Science Research Laboratory, Hanno Research Center, Taiho Pharmaceutical Co., Ltd. 1-27 Misugidai, Hanno-City, Saitama 357-8527, Japan. E-mail: yamasaki{at}taiho.co.jp

	Abbreviations

PTCA, percutaneous transluminal coronary angioplasty; 3D, three-dimensional; DMEM, Dulbecco's modified Eagle's medium; FBS, fetal bovine serum; BrdU, 5-bromo-2'-deoxyuridine; bFGF, basic fibroblast growth factor; LAD, left anterior descending; I/M, intimal area to medial area; A/M, adventitial area to medial area; INJ, injury; PDGF-BB, platelet-derived growth factor-BB.

	References

Top Abstract Introduction Experimental Procedures Results Discussion References

Andersen HR, Mæng M, Thorwest M and Erling F (1996) Remodeling rather than neointimal formation explains luminal narrowing after deep vessel wall injury: Insights from a porcine coronary (re)stenosis model. Circulation 93: 1716-1724[Abstract/Free Full Text].
Ardissino D, Barberis P, De Servi S, Merlini PA, Bramucci E, Falcone C and Specchia G (1991) Abnormal coronary vasoconstriction as a predictor of stenosis after successful coronary angioplasty in patients with unstable angina pectoris. N Engl J Med 325: 1053-1057[Abstract].
Arora PD and McCulloch CA (1994) Dependence of collagen remodeling on $alpha$ -smooth muscle actin expression by fibroblasts. J Cell Physiol 159: 161-175[Medline].
Bell E, Ivarsson B and Merrill C (1979) Production of a tissue-like structure by contraction of collagen lattices by human fibroblasts of different proliferative potential in vitro. Proc Natl Acad Sci USA 76: 1274-1278[Abstract/Free Full Text].
Chamley-Campbell JH, Campbell GR and Ross R (1981) Phenotype-dependent response of cultured aortic smooth muscle to serum mitogens. J Cell Biol 89: 379-383[Abstract/Free Full Text].
Clark RA (1993) Regulation of fibroplasia in cutaneous wound repair. Am J Med Sci 306: 42-48[Medline].
Darby I, Skalli O and Gabbiani G (1990) $alpha$ -Smooth muscle actin is transiently expressed by myofibroblasts during experimental wound healing. Lab Invest 63: 21-29[Medline].
Desmouliere A, Geinoz A, Gabbiani F and Gabbiani G (1993) Transforming growth factor- $beta$ 1 induces $alpha$ -smooth muscle actin expression in granulation tissue myofibroblasts and in quiescent and growing cultured fibroblasts. J Cell Biol 122: 103-111[Abstract/Free Full Text].
Edelman ER, Nugent MA and Karnovsky MJ (1993) Perivascular and intravenous administration of basic fibroblast growth factor: Vascular and solid organ deposition. Proc Natl Acad Sci USA 90: 1513-1517[Abstract/Free Full Text].
Franklin SM and Faxon DP (1993) Pharmacological prevention of restenosis after coronary angioplasty: Review of the randomized clinical trials. Coron Artery Dis 4: 232-242[Medline].
Grinnell F (1994) Fibroblasts, myofibroblasts, and wound contraction. J Cell Biol 124: 401-404[Free Full Text].
Hadeishi H, Mayberg MR and Seto M (1994) Local application of calcium antagonists inhibits intimal hyperplasia after arterial injury. Neurosurgery 34: 114-121[Medline].
Hata H, Ohara Y, Kuga T, Fukai T, Kasuya H, Tomoike H and Takeshita A (1995) Vasoreactivity and restenosis after coronary angioplasty in the atherosclerotic pig model. Coron Artery Dis 6: 503-511[Medline].
den Heijer P, Foley DP, Escaned J, Hillege HL, van Dijk RB, Serruys PW and Lie KI (1994) Angioscopic versus angiographic detection of intimal dissection and intracoronary thrombus. J Am Coll Cardiol 24: 649-654[Abstract].
Isner JM, Kearney M and Bauters C (1994) Use of human tissue specimens obtained in vivo by directional atherectomy to study restenosis and related human vascular disorder. Trends Cardiovasc Med 4: 213-221.
Kadokami T, Shimokawa H, Fukumoto Y, Ito A, Takayanagi T, Egashira K and Takeshita A (1996) Coronary artery spasm does not depend on the intracellular calcium store but is substantially mediated by the protein kinase C-mediated pathway in a swine model with interleukin-1 in vivo. Circulation 94: 190-196[Abstract/Free Full Text].
Kakuta T, Currier JW, Haudenschild CC, Ryan TJ and Faxon DP (1994) Differences in compensatory vessel enlargement, not intimal formation, account for restenosis after angioplasty in the hypercholesterolemic rabbit model. Circulation 89: 2809-2815[Abstract/Free Full Text].
Kuntz RE and Baim DS (1993) Defining coronary restenosis: Newer clinical and angiographic paradigms. Circulation 88: 1310-1323[Free Full Text].
Luo H, Nishioka T, Eigler NL, Forrester JS, Fishbein MC, Berglund H and Siegel RJ (1996) Coronary artery restenosis after balloon angioplasty in humans is associated with circumferential coronary constriction. Arterioscler Thromb Vasc Biol 16: 1393-1398[Abstract/Free Full Text].
Magaud JP, Sargent I and Mason DY (1988) Detection of human white cell proliferative responses by immunoenzymatic measurement of bromodeoxyuridine uptake. J Immunol Methods 106: 95-100[Medline].
Di Mario C, Ruygrok PN and Serruys PW (1994) Vascular remodeling in coronary artery disease. J Cardiovas Pharmacol 24 (Suppl 3): S5-S15.
Marso SP, Ellis SG and Raymond R (1999) Intracoronary stenting: An overview for the clinician. Clev Clin J Med 66: 434-442[Medline].
Mattsson E and Clowes AW (1995) Current concepts in restenosis following balloon angioplasty. Trends Cardiovasc Med 5: 200-204.
Mintz GS, Popma JJ, Pichard AD, Kent KM, Satler LF, Wong SC, Hong MK, Kovach JA and Leon MB (1996) Arterial remodeling after coronary angioplasty: A serial intravascular ultrasound study. Circulation 94: 35-43[Abstract/Free Full Text].
Miyazaki M, Ohashi R, Tsuji T, Mihara K, Gohda E and Namba M (1998) Transforming growth factor-beta1 stimulates or inhibits cell growth via down- or up-regulation of p21/Waf1. Biochem Biophys Res Commun 246: 873-880[Medline].
Moliterno DJ and Topol EJ (1996) Clinical evaluation of restenosis, in Atherosclerosis and Coronary Artery Disease (Fuster V, Ross R andTopol EJ eds) pp 1505-1526, Lippincott-Raven, New York.
Muldoon LL, Rodland KD and Magun BE (1988) Transforming growth factor $beta$ and epidermal growth factor alter calcium influx and phosphatidylinositol turnover in rat-1 fibroblasts. J Biol Chem 263: 18834-18841[Abstract/Free Full Text].
Muller DWM, Ellis SG and Topol EJ (1992) Experimental models of coronary artery restenosis. J Am Coll Cardiol 19: 418-432[Abstract].
Munaron L, Distasi C, Carabelli V, Baccino FM, Bonelli G and Lovisolo D (1995) Sustained calcium influx activated by basic fibroblast growth factor in Balb-c 3T3 fibroblasts. J Physiol (Lond) 484: 557-566[Medline].
Muranaka Y, Yamasaki Y, Nozawa Y, Terakawa H, Tanahashi Y, Oda N, Satoh A, Asao T, Miyake H and Matsuura N (1998) TAS-301, an inhibitor of smooth muscle cell migration and proliferation, inhibits intimal thickening after balloon injury to rat carotid arteries. J Pharmacol Exp Ther 285: 1280-1286[Abstract/Free Full Text].
Sasaki E, Miyoshi K, Nozawa Y, Kanda A, Nakano K, Yamasaki Y, Miyake H and Matsuura N (2000) TAS-301, a new synthetic inhibitor of neointimal thickening after balloon injury, inhibits calcium-dependent signal transduction and cytoskeletal reorganization. Pharmacology, in press.
Schwartz RS, Holmes DR, Jr and Topol EJ (1992) The restenosis paradigm revisited: An alternative proposal for cellular mechanisms. J Am Coll Cardiol 20: 1284-1293[Abstract].
Scott NA, Cipolla GD, Ross CE, Dunn B, Martin FH, Simonet L and Wilcox JN (1996) Identification of a potential role for the adventitia in vascular lesion formation after balloon overstretch injury of porcine coronary arteries. Circulation 93: 2178-2187[Abstract/Free Full Text].
Shi Y, Pieniek M, Fard A, O'Brien J, Mannion JD and Zalewski A (1996a) Adventitial remodeling after coronary arterial injury. Circulation 93: 340-348[Abstract/Free Full Text].
Shi Y, O'Brien JE, Fard A, Mannion JD, Wang D and Zalewski A (1996b) Adventitial myofibroblasts contribute to neointimal formation in injured porcine coronary arteries. Circulation 94: 1655-1664[Abstract/Free Full Text].
Shi Y, O'Brien JE, Fard A and Zalewski A (1996c) Transforming growth factor- $beta$ 1 expression and myofibroblast formation during arterial repair. Arterioscler Thromb Vasc Biol 16: 1298-1305[Abstract/Free Full Text].
Yokozeki M, Moriyama K, Shimokawa H and Kuroda T (1997) Transforming growth factor- $beta$ ₁ modulates myofibroblastic phenotype of rat palatal fibroblasts in vitro. Exp Cell Res 231: 328-336[Medline].
Zhang HY, Gharaee-Kermani M, Zhang K, Karmiol S and Phan SH (1996) Lung fibroblast $alpha$ -smooth muscle actin expression and contractile phenotype in bleomycin-induced pulmonary fibrosis. Am J Pathol 148: 527-537[Abstract].

This article has been cited by other articles:

R. J. Pettersen, Z. A. Muna, K. K.J. Kuiper, E. Svendsen, F. Muller, P. Aukrust, R. K. Berge, and J. Erik Nordrehaug
Sustained retention of tetradecylthioacetic acid after local delivery reduces angioplasty-induced coronary stenosis in the minipig
Cardiovasc Res, November 1, 2001; 52(2): 306 - 313.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Submit a response

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Google Scholar

Google Scholar

Articles by Sasaki, E.

Articles by Matsuura, N.

Search for Related Content

PubMed

PubMed Citation

Articles by Sasaki, E.

Articles by Matsuura, N.