Stimulation of Cholesterol Release from Rabbit Foam Cells by the Action of a New Inhibitor for Acyl CoA:Cholesterol Acyltransferase (ACAT), HL-004

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Vol. 287, Issue 1, 115-121, October 1998

Stimulation of Cholesterol Release from Rabbit Foam Cells by the Action of a New Inhibitor for Acyl CoA:Cholesterol Acyltransferase (ACAT), HL-004

Itsuko Ishii, Noriko Yokoyama, Mamoru Yanagimachi, Naoya Ashikawa, Masayuki Hata, Shigeru Murakami¹, Yumiko Asami¹, Nobuhiro Morisaki², Yasushi Saito², Shigeru Ohmori³ and Mitsukazu Kitada³

Faculty of Pharmaceutical Sciences, Chiba University, 1-33, Yayoi-cho, Inage-ku, Chiba 263-8522, Japan

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

A new inhibitor of acyl CoA:cholesterol acyltransferase (ACAT), HL-004 [N-(2, 6-diisopropylphenyl)tetradecylthioacetamide],suppressed the synthesis of cholesterol [¹⁴C]oleate at 10⁹ ~ 10⁷ M in a concentration-dependent manner in both THP-1 cell-derivedmacrophages and foam cells prepared from aortic intima of rabbitsfed a high cholesterol diet. Incorporation of [³H]cholesterol oleate- $beta$ very low density lipoproteins was not inhibitedby HL-004 at 10⁹ ~ 10⁷ M. Release of radioactivity from the cells loaded with [³H]cholesterol oleate- $beta$ very low density lipoproteins was increasedby the inhibition of ACAT activity with HL-004. HL-004 did notaffect on acid and neutral cholesterol esterases. As a result,cholesterol ester content in foam cells decreased. These datasuggested that HL-004 decreases cholesterol ester in foam cellsby increasing the release of cholesterol and therefore might suppressatherosclerotic lesions.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The development of atherosclerotic diseases is associated with the accumulation of cholesterol ester in arteries. Large numbersof foam cells derived from macrophages and smooth muscle cellsand containing a large amount of cholesterol ester are found inatherosclerotic lesions (Rosenfeld et al., 1987; Lewis et al.,1985; Stary et al., 1990). These foam cells have a high activityof ACAT, which catalyzes the esterification of free cholesterol(Suckling et al., 1985). The increase of lipid deposition in foamcells is due to this excessive cholesterol esterification by theACAT action (Goldstein et al., 1980). Thus, it might be expectedthat atherosclerosis is reduced by the inhibition of ACAT activity.

It is known that intracellular cholesterol metabolism is regulated by some enzymes such as acid cholesterol esterase and neutralcholesterol esterase besides ACAT (Brown et al., 1979, 1980; Khooet al., 1981, 1984; Goldberg et al., 1990). It is reported thatan imbalance between cholesterol esterase and ACAT activitiesmight induce either foam cell formation (Ishii et al., 1992, 1994,1995b) or cell toxicity (Warner et al., 1995). For example, whenACAT activity was induced and neutral cholesterol esterase activitywas low, cells accumulated excess cholesterol ester and were convertedinto foam cells (Ishii et al., 1992, 1994, 1995a). There are severalreports on the effects of ACAT inhibitors on intracellular cholesterolcontent and metabolism. An ACAT inhibitor, Sandoz 58-035, reducedintracellular cholesterol ester content in J774 cells, mouse peritonealmacrophages, Fu5AH hepatoma cells (Bernard et al., 1990) and monkeyarterial smooth muscle cells under conditions of hyperlipidemia(Ross et al., 1984). Other ACAT inhibitors, CL 277,082 and CI-976,also inhibited ACAT activity and cholesterol absorption (Krauseet al., 1993; Largis et al., 1989). On the other hand, when freecholesterol accumulated by the inhibition of ACAT activity withSandoz 58-035 and Pfizer 113,818, cell toxicity was induced (Warneret al., 1995). For the safe use of ACAT inhibitors, this problemmust be solved. We hypothesized that an ideal condition for reducingcholesterol in foam cells by the use of ACAT inhibitors is toincrease the release of intracellular free cholesterol producedby acid and neutral cholesterol esterase. Some kinds of ACAT inhibitorsmight indirectly stimulate this process. In this study, we investigatedthis possibility using a new ACAT inhibitor, HL-004 [N-(2, 6-diisopropylphenyl)tetradecylthioacetamide],compared with CI-976 (2,2-dimethyl-N1-(2,4,6-trimethylphenyl)-dodecanamide).

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Materials. HL-004 was synthesized by Taisho Pharmaceutical (Ohmiya, Japan). HL-004 was synthesized as reported (Japanese patent No. JP-316129,1995), and the purity was >99% by HPLC. CI-976 was obtained fromWarner-Lambert (Ann Arbor, MI). HL-004 and CI-976 were first dissolvedin DMSO, and the final concentration was 10⁴ M. [³H]Cholesterol oleate (3.0 GBq/mmol) and [¹⁴C]oleic acid (1.5 GBq/mmol) were purchased from New England NuclearCorporation (Boston, MA). [8-³H]Adenine (666 GBq/mmol) was purchased from Amersham Corp. (Buckinghamshire,UK). TPA was obtained from Sigma (St. Louis, MO). THP-1 cells(human monocyte leukemia cell line) were obtained from Japan CellCulture System (Tokyo, Japan). DMEM and RPMI 1640 were obtainedfrom Nissui Pharmaceutical (Tokyo, Japan).

Preparation of cells. THP-1 cells (5 × 10⁶ cells/ml) were treated with 1 × 10⁸ M TPA overnight in RPMI 1640 containing 10% FBS (10% FBS/RPMI), andthe adherent cells were used as macrophages (Hayashi et al., 1991).

Rabbit atherosclerotic lesion cells were obtained as reported previously (Jaakkola et al., 1988

; Pitas et al., 1990

). Rabbitswere fed a high cholesterol diet containing 1% cholesterol ina normal chow diet for 16 weeks. The aorta was removed and theadventitia was carefully separated. Then, the media and intimawere cut into pieces (1 × 1 mm) and digested with collagenase(Sigma, Type III, 500 units/ml) and elastase (Sigma, Type III,100 units/ml) for 30 min at 37°C. The tissue digest was centrifugedat 1000 × g for 5 min and the pellet was suspended with DMEM.This process was repeated 3 times. The resultant cell suspensionwas seeded onto plates and incubated in DMEM containing 10% FBS(10% FBS/DMEM). After 4 hr, unattached cells were washed off withDMEM. We called these adherent cells atherosclerotic lesion cells.Esterase staining demonstrated that 75% ~ 82% of the attachedcells were able to hydrolyze $alpha$ -naphthylacetate (data not shown),indicating that these cells were mainly macrophages and the remainingcells were smooth muscle cells.

Measurment of ACAT inhibitor-induced cell toxicity. ACAT inhibitor-induced cell toxicity was measured by the modified (Warner et al., 1995; Reid et al., 1992) method of Shirhattiand Krishna (Shirhatti et al., 1985). Briefly, after 18-hr incubationof cells with DMEM containing 0.2% BSA, 37 kBq of [³H]adenine was added to each well and cells were incubated for2 hr. Then, wells were washed 3 times with 1 ml of DMEM containing0.2% BSA (0.2% BSA/DMEM) and incubated for an additional 10 minwith 0.2% BSA/DMEM. Media were removed, and fresh 0.2% BSA/DMEMwas added with ACAT inhibitor. At indicated times, 200 µl of themedia was removed from triplicate cultures and their radioactivitieswere counted. [³H]Adenine release from macrophages was expressed as a percentageof release compared with control treatment (0.2% BSA): (cpm inmedium of treatment $-$ cpm in medium of control)/([³H]adenine content at time zero) × 100, or as a percent releaseof total cell [³H]adenine content at time zero.

Preparation of lipoproteins. HDL (d = 1.063 ~ 1.21 g/ml) and LPDS (d > 1.25 g/ml) were isolated from human plasma by sequential ultracentrifugation andwere dialyzed against 20 mM Tris-HCl (pH 7.4), 2 mM EDTA, 0.15M NaCl and 0.02% NaN₃ for 24 hr (Havel et al., 1955).

Preparation of reconstituted [³H]cholesterol oleate into $beta$ VLDL. $beta$ VLDL (density < 1.006) was isolated from cholesterol-fed rabbit serum by ultracentrifugation for 16 hr (Brown et al., 1975).Incorporation of [³H]cholesterol oleate into $beta$ VLDL was done essentially by the methodof Brown et al (1975). Then, 37 MBq of [³H]cholesterol oleate was added with 1 ml of DMSO. The mixturewas sonicated for 30 sec. Then 2 ml of plasma density buffer (0.154M NaCl, 1 mM EDTA, 10 mM Tris-HCl, pH 7.4, 0.01% NaN₃) was added,and the mixture was resonicated for 30 sec. It was then addeddropwise to 6 ml of $beta$ VLDL (10 mg total cholesterol/ml) in 3 min.The solution was incubated for 8 hr at 37°C and then was dialyzedagainst 3 liters of plasma density buffer for 10 hr. After dialysis,the solution was centrifuged for 16 hr at 105,000 × g. The toplayer was used as [³H]cholesterol oleate-incorporated $beta$ VLDL. The specific activitywas about 3.4 × 10⁷ dpm/mg total cholesterol and 5.4 × 10⁷ dpm/mg cholesterol ester.

[³H]Cholesterol oleate- $beta$ VLDL incorporation into cells. TPA-treated THP-1 cells (1 × 10⁶ cells) and atherosclerotic lesion cells (5 × 10⁵ cells) were plated in 12-well plates and incubated for certaintime periods in 0.75 ml of DMEM containing 5% LPDS (5% LPDS/DMEM)and 200 µg cholesterol of [³H]cholesterol oleate- $beta$ VLDL (1.6 × 10⁶ dpm). Then, after 8-hr incubation, the cells were washed 3 timeswith 10% FBS/DMEM, and their radioactivity was measured with ascintillation counter. Furthermore, to determine the free [³H]cholesterol released from the cells during incubation, organicsolvent (chloroform:methanol = 2:1) was added to the medium, andlipids were extracted from the chloroform layer. The lipids wereapplied to thin layer chromatography (Gillies et al., 1986). Theradioactivity in the free cholesterol fraction was then counted.The total uptake amounts were the sums of intracellular radioactivityand free [³H]cholesterol radioactivity in the medium.

Release of radioactivity from [³H]cholesterol oleate- $beta$ VLDL-loaded cells. TPA-treated THP-1 cells (2 × 10⁶ cells) and atherosclerotic lesion cells (2 × 10⁶ cells) were plated in 12-well plates and incubated for 24 hrin 1 ml of 5% LPDS/DMEM containing 200 µg of [³H]cholesterol oleate- $beta$ VLDL. Then the cells were washed 3 timeswith 5% LPDS/DMEM. These [³H]cholesterol oleate- $beta$ VLDL-loaded cells were incubated furtherin 2 ml of 5% LPDS/DMEM containing HDL (0.3 mg protein/ml). Atthe times indicated in figure 3, 0.4 ml of the medium was removed,and its radioactivity was measured.

Synthesis of cholesterol [¹⁴C]oleate from [¹⁴C]oleate in intact cells. Cells (2 × 10⁵ cells/well) were treated with $beta$ VLDL (100 µg cholesterol/ml) and albumin-[¹⁴C]oleic acid complex (0.1 µCi/ml) (Goldstein et al., 1974). Afterincubation for 8 hr, the cells were washed with medium three timesand with PBS twice. The intracellular lipids were extracted bychloroform/methanol (2:1) and separated by thin-layer chromatography(Macherery-Nagel Duren, Merk) using a solvent, hexane/diethylether/acetic acid (146:50:4). Nonlabeled free cholesterol andcholesterol ester were spotted as marker in the plate, and thespot was detected by iodide. The radioactivity of the cholesterolester fraction was estimated as the ACAT activity in intact cells.

Measurement of acid and neutral cholesterol esterase activity. Macrophages (2 × 10⁷ cells) were washed 3 times with PBS and suspended in 1 ml of 10 mM Tris-HCl (pH 7.4) containing 0.25 Msucrose. Then the cells were sonicated twice for 15 sec and usedas the enzyme solution. The reaction mixture (Ishii et al., 1992;Ishii et al., 1994, 1995) contained 0.5 mM cholesterol oleate,0.37 MBq of cholesterol [¹⁴C]oleate, 0.5 mM phosphatidic acid and 100 mM Tris-HCl (pH 7.4)for neutral cholesterol esterase, or 0.5 mM phosphatidylcholineand sodium acetate buffer (pH 4.0) for acid cholesterol esterase,certain concentration of ACAT inhibitors, and the enzyme solution,in a total volume of 200 µl. The incubation was carried out at37°C for 1 hr. The [¹⁴C]oleate released was extracted by a modification of the methodof Belfrage et al (1969). Briefly, the reaction was stopped with3.25 ml of chloroform/methanol/heptane (1.42:1.25:1.00), and then1 ml of 0.1 N NaOH was added. The radioactivity in the water phasewas measured.

Determination of cholesterol ester content. The cholesterol ester content was measured as the difference between the total and free cholesterol contents (Ishii et al.,1995). The lipids of the washed cells in each well were extractedwith 1 ml of hexane/isopropanol (2:1). The organic solvent wasevaporated and the pellet was dissolved in 100 µl of methanol,and the total and free cholesterol contents in the methanol solutionwere assayed enzymatically with Determiner TC 555 and DeterminerFC 555 kits (Kyowa Medics, Tokyo, Japan).

Determination protein concentration. Protein concentration was determined with a kit using Bradford's method (BioRad, Protein Assay, Richmond, CA).

Statistics treatment. The significance of differences in a treatment series was determined by a one-way analysis of variance. Individual treatmentswere compared with the control by Dunnett's test.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Effect of HL-004 on synthesis of cholesterol [¹⁴C]oleate in TPA-treated THP-1 cells. To determine the effect of the ACAT inhibitor, HL-004 on cholesterol esterification in macrophages compared with the effectof CI-976, we examined the inhibition of cholesterol [¹⁴C]oleate synthesis in TPA-treated THP-1 cells. Figure 1A showsthat HL-004 decreased the synthesis of cholesterol [¹⁴C]oleate in a concentration-dependent manner and the effect ofHL-004 was stronger than that of CI-976, the inhibition being~90% at 10⁷ M and ~100% at 10⁶ M. Then, 50% inhibition (IC₅₀) of HL-004 and CI-976 were 1.1× 10⁹ M and 1.2 × 10⁷ M, respectively.

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Fig. 1. Effect of concentration of HL-004 and CI-976 on cholesterol [¹⁴C]oleate synthesis in TPA-treated THP-1 cells and release of [³H]adenine. A, Cholesterol [¹⁴C]oleate synthesis; TPA-treated THP-1 cells (5 × 10⁶ cells/well) were preincubated with HL-004 at indicated concentrations for 24 hr. The medium was changed and the cells were treated with $beta$ VLDL (100 µg cholesterol/ml), [¹⁴C]oleate (37 MBq/well) and HL-004 for 8 hr. Incorporation of [¹⁴C]oleate into cellular cholesterol [¹⁴C]oleate was measured as described in Materials and Methods. 100% Value was 28.3 nmol/mg cell protein. B, Release of [³H]adenine. Release of [³H]adenine from TPA-treated THP-1 cells (5 × 10⁶ cells/well) treated with HL-004 was measured as described in Materials and Methods. $bullet$ , HL-004-treated cells; $open circle$ , CI-976-treated cells. Triplicate determination was measured at each experiment. Values are mean ± S.D. for three experiments. *P < .05, **P < .01. (Asterisks beside circles, compared with nontreated groups.)

In preliminary studies, we observed that the release of radiolabeled adenine correlated with the release of lactate dehydrogenase,a well accepted marker of cell toxicity in cholesterol-loadedmacrophages. Figure 1B shows [³H]adenine release from TPA-treated THP-1 cells incubated in thepresence of HL-004 and CI-976. The release of [³H]adenine from CI-976-treated cells increased in a concentration-dependentmanner, and the amount of the released radioactivities from HL-004-treatedcells was nearly equal in all groups. There was a statisticallysignificant difference between HL-004- and CI-976-treated cells.These data suggested that HL-004 did not induce cell toxicitywhen it inhibited ACAT activity compared with CI-976.

Figure 2 shows the time course of the effect of the ACAT inhibitors. HL-004 (10⁷ M) inhibited 80% ~ 90% of the synthesis of cholesterol [¹⁴C]oleate during the first 24-hr incubation, but the activity thenreturned to 70% of control at 48 hr. CI-976 (10⁷ M) inhibited ~60% during 12-hr incubation but ~20% after 24-hrincubation. These data suggested that the duration of HL-004 effectwas longer that that of CI-976. In the following experiments,the HL-004 effect was determined within 24 hr.

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Fig. 2. Time-dependent effect of HL-004 and CI-976 on cholesterol [¹⁴C]oleate synthesis in TPA-treated THP-1 cells. TPA-treated THP-1 cells (5 × 10⁶ cells/well) were incubated with $beta$ VLDL (100 µg cholesterol/ml) and [¹⁴C]oleate (37 MBq/well) in the presence of 10⁷ M ACAT inhibitors for indicated times. Incorporation of [¹⁴C]oleate into cellular cholesterol [¹⁴C]oleate was measured as described in Materials and Methods.

, control; $bullet$ , HL-004-treated cells; $open circle$ , CI-976-treated cells. Triplicate determination was measured at each experiment. Values are mean ± S.D. for three experiments. *P < .05, **P < .01.

Effect of HL-004 on cholesterol metabolism in TPA-treated THP-1 cells. Cholesterol metabolism of macrophages is as follows; macrophages take up lipoproteins such as $beta$ VLDL and denatured LDL. First,cholesterol ester in lipoproteins is hydrolyzed by acid cholesterolesterase in lysosomes (Brown et al., 1979; Brown, et al., 1980).Then the product, free cholesterol, is reesterified by ACAT andstored as cholesterol ester in intracellular lipid droplets. Afterthat, the reesterified cholesterol is hydrolyzed by neutral cholesterolesterase (Khoo et al., 1981, 1984; Goldberg et al., 1990), andfinally, free cholesterol is released from the cells. Thus, theeffects of HL-004 on the incorporation of $beta$ VLDL, release of cholesterol,acid cholesterol esterase activity and neutral cholesterol esteraseactivity were measured compared with CI-976.

HL-004 and CI-976 did not change the incorporation of [³H]cholesterol oleate- $beta$ VLDL (fig. 3A). The released radioactivity fromcells treated with both ACAT inhibitors increased in a dose-dependentmanner. However, the release from HL-004 was about twice thatfrom CI-976 at the concentration of 10⁷ M (fig. 3B). Chemical form of radioactivity in media with HDL(fig. 3B) was free cholesterol (~80%) and cholesterol ester (~20%).Cellular free cholesterol mass was measured but there is no significantdifference at each concentration of each ACAT inhibitor. However,the ratio of free [³H]cholesterol to total [³H]cholesterol in THP-1 cells treated with HL-004 and CI-976 was44% and 32%, respectively. Figure 4 shows that HL-004 did notchange the acid and neutral cholesterol esterase activities atthe concentration of 10⁹ ~ 10⁷ M. CI-976 decreased both enzyme activities at 10⁷ M. Then, we suggested that HL-004 is more efficient for cholesteroltransport.

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Fig. 3. Effect of concentration of HL-004 and CI-976 on incorporation of [³H]cholesterol oleate- $beta$ VLDL and release of radioactivity from TPA-treated THP-1 cells loaded with [³H]cholesterol oleate- $beta$ VLDL. A, Incorporation of [³H]cholesterol oleate- $beta$ VLDL into TPA-treated THP-1 cells. TPA-treated THP-1 cells (1 × 10⁶ cells/well) were incubated with ACAT inhibitors at indicated concentrations for 12 hr. The medium was changed and the cells were treated with [³H]cholesterol oleate- $beta$ VLDL, and again with ACAT inhibitors for 8 hr. Incorporation of [³H]cholesterol oleate- $beta$ VLDL into the cells was measured as described in Materials and Methods. B, Release of radioactivity from TPA-treated THP-1 cells loaded with [³H]cholesterol oleate- $beta$ VLDL. TPA-treated THP-1 cells (1 × 10⁶ cells/well) were incubated with [³H]cholesterol oleate- $beta$ VLDL for 24 hr. After that, cells were incubated with 5% LPDS/DMEM containing HDL (0.3 mg protein/ml) and ACAT inhibitors for 12 hr. Total incorporated and released radioactivity were measured as described in Materials and Methods. $bullet$ , HL-004-treated cells; $open circle$ , CI-976-treated cells. Triplicate determination was measured at each experiment. Values are mean ± S.D. for three experiments. *P < .05, **P < .01.

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Fig. 4. Effect of concentration of HL-004 and CI-976 on acid and neutral cholesterol esterase activities. Acid and neutral cholesterol esterase activities were measured as described in Materials and Methods. A, Acid cholesterol esterase. B, Neutral cholesterol esterase. $bullet$ , HL-004-treated cells; $open circle$ , CI-976-treated cells. Triplicate determination was measured at each experiment. Values are mean ± S.D. for three experiments. *P < .05, **P < .01. (Asterisks beside circles, compared with nontreated groups.)

Effect of HL-004 on cholesterol metabolism of foam cells. Next, we examined the effects of HL-004 on the cholesterol metabolism of foam cells. Figure 5A shows the effect of HL-004and CI-976 on the synthesis of cholesterol [¹⁴C]oleate in foam cells. Synthesis of cholesterol [¹⁴C]oleate of control cells was in the range of 3.7 ~ 5.7 nmol/mgprotein. HL-004 decreased the synthesis in a concentration-dependentmanner, the inhibition being 83% at 10⁷ M. Although CI-976 decreased the synthesis in a concentration-dependentmanner, the inhibition was much lower than that of HL-004, being21% at 10⁷ M. Figure 5B shows the effect of HL-004 and CI-976 on the releaseof [³H]adenine. The release of HL-004-treated groups was almost thesame as CI-976-treated groups and was not different from thatof nontreated group. These data on HL-004 were quite similar tothose in THP-1 cell-derived macrophages (fig. 1).

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Fig. 5. Effect of concentration of HL-004 and CI-976 on cholesterol [¹⁴C]oleate synthesis in atherosclerotic lesion cells and release of [³H]adenine. A, Atherosclerotic lesion cells (5 × 10⁵ cells/well) were preincubated with HL-004 or CI-976 at indicated concentrations for 24 hr. The medium was changed and the cells were treated with $beta$ VLDL (100 µg cholesterol/ml) and [¹⁴C]oleate (37 MBq/well), and again with HL-004 or CI-976 for 8 hr. Incorporation of [¹⁴C]oleate into cellular cholesterol [¹⁴C]oleate was measured as described in Materials and Methods. 100% Value was 118.2 nmol/mg cell protein. B, Release of [³H]adenine; Release of [³H]adenine from TPA-treated THP-1 cells (5 × 10⁶ cells/well) treated with HL-004 or CI-976 was measured as described in Materials and Methods. $bullet$ , HL-004-treated cells; $open circle$ , CI-976-treated cells. Values are mean ± S.D. for three experiments. Triplicate determination was measured at each experiment. Data are expressed as mean ± SD values obtained from 3 animals. **P < .01. (Asterisks beside circles, compared with nontreated groups.)

Then, to clarify the effect of HL-004 on the incorporation of $beta$ VLDL, we measured the incorporation of [³H]cholesterol oleate- $beta$ VLDL into foam cells (fig. 6). It did notchange until 10⁸ M of HL-004 and decreased only by 10% at 10⁷ M. These results indicated that HL-004 at concentrations of 10⁹ ~ 10⁷ M had little effect on the incorporation of $beta$ VLDL.

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Fig. 6. Effect of HL-004 on incorporation of [³H]cholesterol oleate- $beta$ VLDL into atherosclerotic lesion cells. Atherosclerotic lesion cells (5 × 10⁵ cells/well) were incubated with HL-004 at indicated concentrations for 12 hr. The medium was changed and the cells were treated with [³H]cholesterol oleate- $beta$ VLDL, and again with HL-004. Incorporation of [³H]cholesterol oleate- $beta$ VLDL into the cells was measured as described in Materials and Methods. Triplicate determination was measured at each experiment. Data are expressed as mean ± S.D. values obtained from 3 animals. *P < .05.

Free cholesterol by acid and neutral cholesterol esterases could be released from cells through the cell membrane. If ACATactivity is inhibited beforehand and then [³H]cholesterol oleate- $beta$ VLDL is added to the cells, it can be assumedthat incorporated [³H]cholesterol oleate is hydrolyzed by acid cholesterol esterasein lysosome and that [³H]cholesterol may be released from the cells. Furthermore, if[³H]cholesterol oleate- $beta$ VLDL is first added to the cells, [³H]cholesterol ester accumulates in lipid droplets, and if theACAT inhibitor is then added, [³H]cholesterol oleate in lipid droplets may be hydrolyzed by theneutral cholesterol esterase and [³H]cholesterol may be released. Figure 7 shows the former typeof experiment. Radioactivity increased in a time-dependent mannerin all of the groups. Released radioactivity from HL-004 (10⁹ ~ 10⁷ M)-treated cells was significantly higher than that from control,the concentration of 10⁷ M being the most effective as far as mean ratio of release wasconcerned.

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Fig. 7. Effect of HL-004 pretreatment on release of radioactivity from atherosclerotic lesion cells loaded with [³H]cholesterol oleate- $beta$ VLDL. Percentage of released radioactivity to total incorporated radioactivity. Atherosclerotic lesion cells (2 × 10⁶ cells/well) were preincubated with 5% LPDS/DMEM containing HL-004 at indicated concentrations for 12 hr. After that, cells were incubated with 5% LPDS/DMEM containing [³H]cholesterol oleate- $beta$ VLDL (100 µg total cholesterol/ml) and HL-004 for 24 hr. The cells were washed with 5% LPDS/DMEM and then incubated with 5% LPDS/DMEM containing HDL (0.3 mg protein/ml) and HL-004. $triangle$ , control; $black-triangle$ , 10⁹ M; $bullet$ , 10⁸ M; $open circle$ , 10⁷ M. Total incorporated and released radioactivity were measured as described in Materials and Methods. Triplicate determination was measured at each experiment. Data are expressed as mean ± S.D. values obtained from 3 animals. *P < .05.

The latter experiment is shown in figure 8. Released radioactivity increased in a time-dependent manner in all groups. Releasedradioactivity from the HL-004-treated groups was significantlyhigher than that from the control cells. Released radioactivityfrom foam cells treated with 10⁸ M HL-004 was most effective. In addition, HL-004 did not influencethe total incorporation of [³H]cholesterol oleate- $beta$ VLDL into cells in either of the experiments(fig. 6), suggesting that the difference in the release of cholesterolis not due to the different incorporation of $beta$ VLDL.

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Fig. 8. Effect of HL-004 treatment on release of radioactivity from [³H]cholesterol oleate- $beta$ VLDL-loaded atherosclerotic lesion cells. Percentage of released radioactivity to total incorporated radioactivity. Atherosclerotic lesion cells (2 × 10⁶ cells/well) were incubated with 5% LPDS/DMEM containing [³H]cholesterol oleate- $beta$ VLDL (100 µg total cholesterol/ml) for 24 hr. The cells were washed with 5% LPDS/DMEM and then incubated with 5% LPDS/DMEM containing HDL (0.3 mg protein/ml) and HL-004 at indicated concentrations. $triangle$ , control; $black-triangle$ , 10⁹ M; $bullet$ , 10⁸ M; $open circle$ , 10⁷ M. Total incorporated and released radioactivity were measured as described in Materials and Methods. Triplicate determination was measured at each experiment. Data are expressed as mean ± S.D. values obtained from 3 animals. *P < .05, **P < .01.

These data suggested that the release of free cholesterol from foam cells could be accelerated by the inhibition of ACAT activityby HL-004 and that there might be two pathways for the releaseof free cholesterol from the cells: one is dependent on acid cholesterolesterase and the other on neutral cholesterol esterase.

Finally, we measured the cholesterol ester content in foam cells after incubation with $beta$ VLDL, and it was observed to increasesignificantly. However, by preincubation with HL-004 followedby incubation with $beta$ VLDL, the content in cells decreased concentration-dependentlyand that in treated with 10⁷ M HL-004 was almost the same as that in control cells (fig. 9).

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Fig. 9. Effect of HL-004 on cholesterol ester content in atherosclerotic lesion cells. Atherosclerotic lesion cells (5 × 10⁵ cells/well) were preincubated with HL-004 for 12 hr. The cells were then incubated with $beta$ VLDL (1 mg cholesterol/ml) for 12 hr. Cholesterol ester content was measured as described in Materials and Methods. Triplicate determination was measured at each experiment. Data are expressed as mean ± S.D. values obtained from 3 animals. **P < .01.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The concentration-dependent effect of HL-004 on rabbit foam cells was almost the same as that on THP-1 derived macrophages(figs. 1 and 3). It was also similar to that on rat macrophages(Murakami et al., 1995b) and smooth muscle cells (Murakami etal., 1995a). These data indicate that the inhibitory effect onACAT by HL-004 is universal regardless of cell type and origin.From our results, the difference of HL-004 and other ACAT inhibitor(CI-976 in this report) is as follows: (1) the effective concentrationof HL-004 was low (10⁹ ~ 10⁷ M), (2) the cell toxicity of HL-004 was low and (3) the effectof HL-004 on incorporation of $beta$ VLDL, acid cholesterol esteraseand neutral cholesterol esterase was very little, whereas CI-976affected these metabolisms. These data suggested that HL-004 wasa unique ACAT inhibitor compared with other ACAT inhibitors.

HL-004 was effective on macrophages and foam cells at a very low concentration (10⁹ ~ 10⁷ M), apparently without any cell toxicity (figs. 1B and 5B). Orallyadministered ACAT inhibitors generally inhibit ACAT activity ofvarious organs such as the liver and intestine, but the side effectof adrenocortical cytotoxicity has been reported (Dominick etal., 1993). Then, the question arises why HL-004 is free fromtoxicity. HL-004 is a noncompetitive inhibitor against oleoyl-CoAand its specificity for ACAT is very high because it does notinfluence the synthesis of phospholipids and triglycerides. Ifthis ACAT inhibitor acts on only ACAT and free cholesterol istransported out of cells, cell toxicity would not occur. To findthe differences between both HL-004 and CI-976, the stable structureswere obtained by a semiempirical molecular orbital method withP3 approximation (Stewart, 1989a, 1989b) in figure 10. For HL-004,the structure of molecule at grand minimized potential energywas a linear conformation. Phenyl ring and peptide bond mightbe conjugated but area of delocalization might be smaller comparedwith that of CI-976. When "S" in HL-004 was changed to "C" andthe minimum energy was calculated, the energy of a turned conformationwas 1.9 kcal/mol low compared with the energy of a linear conformation.Thus, a presence of "S" may be important for a linear conformation.For CI-976, the structure was folded between peptide bond andalkyl chain. Conjugation of phenyl ring, methoxy group and peptidebond would raise up delocalization of electrons, and then themolecule might be stable. To clear this reason, we calculatedthe potential energy of grand minimum between a linear conformationand a turned conformation of CI-976. The energy of the turnedconformation was 2.1 kcal/mol low. Therefore, the turned conformationwas stable compared with a linear conformation. These resultssuggested that the unique structure of HL-004 indicates that thisinhibitor specifically acts on ACAT as a noncompetitive inhibitorand does not affect other proteins related to the free cholesteroltransport system.

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Fig. 10. The stable structures of ACAT inhibitors obtained by PM3 method. Computation program used was MOPAC Ver. 6 (Stewart, 1989c

). Numerals are the change densities calculated by Mulliken's population analysis. $open circle$ , H; shaded circle, C; large dots, O; small dots, O; stipes, S.

Cholesterol efflux was very low compared with that in figures 7 and 8 without HDL (data not shown). This suggested that HL-004enhanced the HDL-mediated cholesterol efflux from atheroscleroticlesion cells. It is reported that ACAT inhibitors enhanced HDL-mediatedcholesterol efflux from macrophages (Furuchi et al., 1993; Schmitzet al., 1988, 1985). In the experiments of figures 7 and 8, asufficient level of HDL (0.3 mg protein/ml) was added to the medium.In a similar experiment using 10% FBS/DMEM, the total releaseof cholesterol was low (the released cholesterol was up to ~30%of the total incorporated cholesterol) and there was no statisticaldifference between control and HL-004-treated foam cells (datanot shown). Both cholesterol-releasing pathways from lysosomeand cytosol required HDL (figs. 7 and 8). It was recently reportedthat free cholesterol produced by the addition of ACAT inhibitorinduced cell toxicity (Warner et al., 1995). This points out theneed for sufficient acceptors for the released cholesterol, suchas HDL, to avoid such toxicity by ACAT inhibitors.

Clinically, it is speculated that plaque rupture caused by foam cells containing a lot of cholesterol ester is a trigger ofacute coronary syndrome (Davies et al., 1985; Hackett et al.,1988). Our studies showed that HL-004 was effective at low concentrations(10⁹ ~ 10⁷) and might decrease foam cell formation without toxicity. Consideringthese findings, it seems reasonable to expect that acute coronarysyndrome (acute coronary thrombosis, and so on) can be reducedby the use of HL-004 together with a sufficient presence of HDL.

	Acknowledgments

The computations were carried out by the DRIA System at the Faculty of Pharmaceutical Sciences, Chiba University.

	Footnotes

Accepted for publication May 8, 1998.

Received for publication October 2, 1997.

¹ Present address: Research Center, Taisho Pharmaceutical Co. Ltd., Ohmiya 330-0031, Japan.

² Present address: Second Department of Internal Medicine, Chiba University, Chiba 260-0856, Japan.

³ Present address: Division of Pharmacy, Chiba University Hospital, Faculty of Medicine, Chiba University, Chiba 260-8677, Japan.

Send reprint requests to: Dr. Itsuko Ishii, Faculty of Pharmaceutical Sciences, Chiba University, Inage-ku 1-33, Yayoi-cho, Chiba, 263-0022, Japan.

	Abbreviations

ACAT, acyl CoA:cholesterol acyltransferase; $beta$ VLDL, $beta$ very low density lipoproteins; FBS, fetal bovine serum; HDL, high density lipoprotein; HL-004, N-(2, 6-diisopropylphenyl) tetradecylthioacetamide; LPDS, lipoprotein-deficient serum; TPA, 12-tetra-decanoyl-phorbol-13-acetate.

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