Abstract:
Methods for regulation of lipid and cholesterol uptake are described which are based on regulation of the expression or function of the SR-BI HDL receptor. The examples demonstrate that estrogen dramatically downregulates SR-BI under conditions of tremendous upregulation of the LDL-receptor. The examples also demonstrate the upregulation of SR-BI in rat adrenal membranes and other non-placental steroidogenic tissues from animals treated with estrogen, but not in other non-placental non-steroidogenic tissues, including lung, liver, and skin. Examples further demonstrate the uptake of fluorescently labeled HDL into the liver cells of animal, which does not occur when the animals are treated with estrogen. Examples also demonstrate the in vivo effects of SR-BI expression on HDL metabolism, in mice transiently overexpressing hepatic SR-BI following recombinant adenovirus infection. Overexpression of the SR-BI in the hepatic tissue caused a dramatic decrease in cholesterol blood levels. These results demonstrate that modulation of SR-BI levels, either directly or indirectly, can be used to modulate levels of cholesterol in the blood.

Description:
CROSS REFERENCE TO RELATED APPLICATIONS  
       [0001]    This application claims priority to U.S. Provisional Application Serial No. 60/417,083 filed on Oct. 8, 2002. 
     
    
       [0002] The U.S. government has certain rights to this invention by virtue of grants HL52212, HL 66105 and HL64737 from the National Institutes of Health-National Heart, Lung and Blood Institute. 
     
    
     
       FIELD OF THE INVENTION  
         [0003]    The present invention is generally in the area of compounds for modulation of cholesterol transport and lipid regulation mediated via the SR-BI scavenger receptor.  
         BACKGROUND OF THE INVENTION  
         [0004]    The intercellular transport of lipids through the circulatory system requires the packaging of these hydrophobic molecules into water-soluble carriers, called lipoproteins, and the regulated targeting of these lipoproteins to appropriate tissues by receptor-mediated pathways. The most well characterized lipoprotein receptor is the LDL receptor, which binds to apolipoproteins B-100 (apoB-100), and E (apoE), which are constituents of low density lipoprotein (LDL), the principal cholesteryl-ester transporter in human plasma, very low-density lipoprotein (VLDL), a triglyceride-rich carrier synthesized by the liver, intermediate-density lipoprotein (IDL), and catabolized chylomicrons (dietary triglyceride-rich carriers). Kreiger, et al., in WO96/00288 “Class BI and CI Scavenger Receptors” by Massachusetts Institute of Technology, U.S. Pat. Nos. 6,359,859 and 6,429,289 (“Krieger, et al.”) characterized and cloned hamster and murine homologs of SR-BI, an AcLDL and LDL binding scavenger receptor. It was reported by Kreiger, et al. that the SR-BI receptor is expressed principally in steroidogenic tissues and liver and appears to mediate HDL-transfer and uptake of cholesterol. Competitive binding studies show that SR-BI binds LDL, modified LDL, negatively charged phospholipid, and HDL. Direct binding studies show that SR-BI expressed in mammalian cells (for example, a variant of CHO cells) binds HDL, without cellular degradation of the HDL-apoprotein, and lipid is accumulated within cells expressing the receptor. These studies indicated that SR-BI might play a major role in transfer of cholesterol from peripheral tissues, via HDL, into the liver and steroidogenic tissues, and that increased or decreased expression in the liver or other tissues may be useful in regulating uptake of cholesterol by cells expressing SR-BI, thereby decreasing levels in foam cells and deposition at sites involved in atherogenesis.  
           [0005]    Subsequent studies confirmed that SR-BI not only binds to lipid, but also transfers cholesterol into and out of cells, as described in U.S. Pat. Nos. 5,962,322 and 5,925,333 to Krieger, et al. Moreover, SR-BI is preferentially expressed in steroidogenic tissues, and plays a role in lipid regulation, affecting not only cholesterol levels but also female fertility, as described by WO99/11288 by Massachusetts Institute of Technology.  
           [0006]    The role of SR-BI in cholesterol uptake and transfer can be manipulated via SR-BI, for example, as demonstrated using probucol treatment to restore female fertility, as described by Miettinen, et al. (2001)  J. Clin. Invest.  108(11): 1717-1722. This work clearly demonstrates that there is a need for additional drugs that that stimulate or inhibit SR-BI mediated lipid uptake and metabolism.  
           [0007]    It is an object of the present invention to provide drugs and methods and reagents for designing drugs, that can stimulate or inhibit the binding to and lipid movements mediated by SR-BI and redirect uptake and metabolism of lipids and cholesterol by cells.  
         SUMMARY OF THE INVENTION  
         [0008]    Compounds for regulation of cholesterol transport are described which are based on regulation of the expression or function of SR-BI. SR-BI mediates both selective uptake of lipids, mainly cholesterol esters, from HDL to cells and efflux of cholesterol from cells to lipoproteins. The mechanism underlying these lipid transfers is distinct from classic receptor mediated endocytosis, but remains poorly understood. To investigate SR-BI&#39;s mechanism of action and in vivo function, a high throughput screen was developed to identify small molecule inhibitors of SR-BI-mediated lipid transfer in intact cells. Two hundred compounds were identified that block lipid transport (BLTs), both selective uptake and efflux, in the low nanomolar to micromolar range. The effects of these compounds were highly specific to the SR-BI pathway, because they did not interfere with clathrin-based receptor-mediated endocytosis or with other forms of intracellular vesicular traffic. As demonstrated by the examples, five BLTs (BLT-1 [MIT 9952-53]; BLT-2 [MIT 9952-61]; BLT-3 [MIT 9952-19]; BLT-4 [MIT 9952-29]; and BLT-5 [MIT 9952-6]) enhanced, rather than inhibited, HDL binding by increasing SR-BI&#39;s binding affinity for HDL (decreased dissociation rates). Others inhibited HDL binding. These should be useful in the management of atherosclerosis, treatment of infertility, or conversely, as contraceptives and in the treatment of Tangier&#39;s disease. 
       
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS  
       [0009]    [0009]FIGS. 1A-1C are graphs of the concentration dependence of the inhibition by BLTs of SR-BI-mediated lipid transfer between HDL and cells. ldlA[mSR-BI] cells were incubated with the indicated concentrations of BLTs and their effects on (A) DiI uptake from DiI-HDL, (B) [ 3 H]CE uptake from [ 3 H]CE-HDL and (C) the efflux of [ 3 H]cholesterol from cells to HDL were determined. The 100% of control values were: A, 50.6 ng HDL protein equivalents/well (384-well plates) and B, 3908 ng HDL protein equivalents/mg cellular protein. In C, the data were normalized such that the maximum amount of [ 3 H]cholesterol transferred from cells to HDL in the absence of compounds (55.7% of total) was set to 100%. The 0% value corresponds to the efflux of [3H] cholesterol transferred from ldlA[mSR-BI] cells to HDL without BLTs and in the presence of saturating inhibitory amounts of the specific anti-SR-BI blocking monoclonal antibody KKB-1 (15% of total). The efflux of [ 3 H]cholesterol from ldlA-7 cells measured in the absence or presence of KKBI was 15% and 10% of total cellular [ 3 H]cholesterol, respectively.  
         [0010]    [0010]FIGS. 2A-2D are graphs of cell surface expression of SR-BI. ldlA[mSR-BI] and ldlA-7 cells were treated for 3 hrs with or without BLTs at their corresponding IC CE 95 concentrations (1 μM for BLT-1 (MIT 9952-53) and BLT-2 (MIT 9952-61), 50 μM for BLT-3 (MIT 9952-19), BLT-4 (MIT 9952-29) and BLT-5 (MIT 9952-6)) followed by determination of surface expression levels of SR-BI by flow cytometry. Panels A-C show histograms of the surface expression for ldlA[mSR-BI] cells without BLTs, ldlA[mSR-BI] cells with 1 μM BLT-1 (MIT 9952-53), and ldlA-7 cells without BLTs, respectively. Panel D summarizes the results in ldlA[mSR-BI] cells for all five BLTs, with the value determined without compounds set to 100%. n, number of independent determinations; SD, standard deviation.  
         [0011]    [0011]FIGS. 3A-3E shows the effects of BLTs on SR-BI-mediated cholesterol ether uptake from HDL, cellular cholesterol efflux to HDL and HDL binding. The effects of indicated concentrations of BLTs (panels A-E) on SR-BI-mediated uptake of [ 3 H]CE from [ 3 H]CE-HDL (solid lines, no symbols), efflux of [ 3 H]cholesterol from cells to HDL (dashed lines), or binding of  125 I-HDL to cells (solid lines, filled symbols) were determined using ldlA[mSR-BI] cells. To simplify comparisons, the lowest observed [ 3 H]CE uptake and [ 3 H]cholesterol efflux values (from FIG. 2) were compared as 0% and the values in the absence of BLTs as 100%. The 100% control value for the  125 I-HDL binding in the absence of BLTs was 403 ng HDL protein/mg cell protein.  
         [0012]    [0012]FIG. 4 is a graph of the effects of BLT-1 (MIT 9952-53) on the concentration dependence of  125 I-HDL binding to ldlA[mSR-BI] cells. The binding of  125 I-HDL to ldlA[mSR-BI] cells was determined in duplicate at the indicated concentrations of HDL in the presence (blue) or absence (black) of 1 μM BLT-1 (MIT 9952-53; IC CE 95). Each value was corrected for binding of  125 I-HDL in the presence of 40-fold excess of unlabeled HDL to ldlA [mSR-BI] cells in the presence of BLT-1 (MIT 9952-53). 
     
    
     DETAILED DESCRIPTION OF THE INVENTION  
       [0013]    I. Modulators of SR-BI Transport of Cholesterol.  
         [0014]    Libraries of compounds have been screened using an assay such as the assays described below for alteration in HDL binding. These compounds can be proteins, DNA sequences, polysaccharides, or synthetic organic compounds. Approximately 200 that have been identified as having activity are listed below in Table I.  
         [0015]    II. Screening of Compounds to Inhibit or Enhance SR-BI Activity.  
         [0016]    The SR-BI proteins and antibodies and their DNAs can be used in screening of drugs which modulate the activity and/or the expression of SR-BI. The cDNA encoding SR-BI has been cloned and is reported U.S. Pat. No. 6,359,859 and 6,429,289 and is listed in GenBank. The cDNA encoding SR-BI yields a predicted protein sequence of 509 amino acids. The drugs which enhance SR-BI activity should be useful in treating or preventing atherosclerosis, fat uptake by adipocytes, and some types of endocrine disorders. The drugs which inhibit SR-BI activity should be useful as contraceptives and in the treatment of Tangiers disease.  
         [0017]    The assays described below clearly provide routine methodology by which a compound can be tested for an inhibitory effect on binding of a specific compound, such as a radiolabeled modified HDL and LDL or polyion. The in vitro studies of compounds which appear to inhibit binding selectively to the receptors can then be confirmed by animal testing. Since the molecules are so highly evolutionarily conserved, it is possible to conduct studies in laboratory animals such as mice to predict the effects in humans.  
         [0018]    Studies based on inhibition of binding are predictive for indirect effects of alteration of receptor binding. For example, inhibition of cholesterol-HDL binding to the SR-BI receptor leads to decreased uptake by cells of cholesterol and therefore inhibits cholesterol transport by cells expressing the SR-BI receptor. Increasing cholesterol-HDL binding to cells increases removal of lipids from the blood stream and thereby decreases lipid deposition within the blood stream. Studies have been conducted using a stimulator to enhance macrophage uptake of cholesterol and thereby treat atherogenesis, using M-CSF (Schaub, et al., 1994  Arterioscler. Thromb.  14(1), 70-76; Inaba, et al., 1993  J. Clin. Invest.  92(2), 750-757).  
         [0019]    The following assays can be used to screen for compounds which are effective in methods for alter SR-BI expression, concentration, or transport of cholesterol.  
         [0020]    Assays for Alterations in SR-BI Binding or Expression  
         [0021]    Northern blot analysis of murine tissues shows that SR-BI is most abundantly expressed in adrenal, ovary, liver, testes, and fat and is present at lower levels in some other tissues. SR-BI mRNA expression is induced upon differentiation of 3T3-L1 cells into adipocytes. Both SR-BI and CD36 display high affinity binding for acetylated LDL with an apparent dissociation constant in the range of approximately 5 μg protein/ml. The ligand binding specificities of CD36 and SR-BI, determined by competition assays, are similar, but not identical: both bind modified proteins (acetylated LDL, maleylated BSA), but not the broad array of other polyanions (e.g. fucoidin, polyinosinic acid, polyguanosinic acid) which are ligands of the class A receptors. SR-BI displays high affinity and saturable binding of HDL which is not accompanied by cellular degradation of the HDL. HDL inhibits binding of AcLDL to CD36, suggesting that it binds HDL, similarly to SR-BI. Native LDL, which does not compete for the binding of acetylated LDL to either class A receptors or CD36, competes for binding to SR-BI.  
         [0022]    [0022] 125 I-AcLDL Binding, Uptake and Degradation Assays.  
         [0023]    Scavenger receptor activities at 37° C. are measured by ligand binding, uptake and degradation assays as described by Krieger,  Cell  33, 413-422, 1983; and Freeman et al., (1991)  Proc Natl Acad Sci USA.  1991 Jun. 1;88(11):4931-5). The values for binding and uptake are combined and are presented as binding plus uptake observed after a 5 hour incubation and are expressed as ng of  125 I-AcLDL protein per 5 hr per mg cell protein.  
         [0024]    Degradation activity is expressed as ng of  125 I-AcLDL protein degraded in 5 hours per mg of cell protein. The specific, high affinity values represent the differences between the results obtained in the presence (single determinations) and absence (duplicate determinations) of excess unlabeled competing ligand. Cell surface 4° C. binding is assayed using either method A or method B as indicated. In method A, cells are prechilled on ice for 15 min, re-fed with  125 I-AcLDL in ice-cold medium B supplemented with 10% (v/v) fetal bovine serum, with or without 75-200 μg/ml unlabeled M-BSA, and incubated 2 hr at 4° C. on a shaker. Cells are then washed rapidly three times with Tris wash buffer (50 mM Tris-HCl, 0.15 M NaCl, pH 7.4) containing 2 mg/ml BSA, followed by two 5 min washes, and two rapid washes with Tris wash buffer without BSA. The cells are solubilized in 1 ml of 0.1 N NaOH for 20 min at room temperature on a shaker, 30 μl are removed for protein determination, and the radioactivity in the remainder is determined using a LKB gamma counter. Method B differs from method A in that the cells are prechilled for 45 minutes, the medium contains 10 mM HEPES and 5% (v/v) human lipoprotein-deficient serum rather than fetal bovine serum, and the cell-associated radioactivity released by treatment with dextran sulfate is measured as described by Krieger, (1983)  Cell  33, 413-422; Freeman et al., (1991)  Proc Natl Acad Sci USA.  1991 Jun. 1;88(11):4931-5)).  
         [0025]    Northern Blot Analysis.  
         [0026]    0.5 micrograms of poly(A)+ RNA prepared from different murine tissues or from 3T3-L1 cells on zero, two, four, six or eight days after initiation of differentiation into adipocytes as described by Baldini et al., 1992  Proc. Natl. Acad. Sci. U.S.A.  89, 5049-5052, is fractionated on a formaldehyde/agarose gel (1.0%) and then blotted and fixed onto a Biotrans™ nylon membrane. The blots are hybridized with probes that are  32 P-labeled (2×10 6  dpm/ml, random-primed labeling system). The hybridization and washing conditions, at 42° C. and 50° C., respectively, are performed as described by Charron et al., 1989  Proc. Natl. Acad. Sci. U.S.A.  86, 2535-2539. The probe for SR-BI mRNA analysis was a 0.6 kb BamHI fragment from the cDNAs coding region. The coding region of murine cytosolic hsp70 gene (Hunt and Calderwood, 1990 Gene 87, 199-204) is used as a control probe for equal mRNA loading.  
         [0027]    SR-BI protein in tissues is detected by blotting with polyclonal antibodies to SR-BI.  
         [0028]    HDL Binding Studies  
         [0029]    HDL and VLDL binding to SR-BI and CD36 are conducted as described for LDL and modified LDL.  
         [0030]    Studies conducted to determine if the HDL which is bound to SR-BI is degraded or recycled and if lipid which is bound to the HDL is transferred into the cells are conducted using fluorescent lipid-labeled HDL,  3 H-cholesteryl ester labeled HDL and  125 I-HDL added to cultures of transfected or untransfected cells at a single concentration (10 μg protein/ml). HDL associated with the cells is measured over time. A steady state is reached in approximately thirty minutes to one hour. A fluorescent ligand, DiI, or  3 H-cholesterol ester is used as a marker for lipid (for example, cholesterol or cholesterol ester) uptake by the cell. Increasing concentration of DiI indicates that lipid is being transferred from the HDL to the receptor, then being internalized by the cell. The DiI-depleted HDL is then released and replaced by another HDL molecule.  
         [0031]    HDL Binding to SR-BI  
         [0032]    Competition binding studies demonstrate that HDL and VLDL (400 μg/ml) competitively inhibit binding of  125 I-AcLDL to SR-BI. Direct binding of  125 I-HDL to cells expressing SR-BI is also determined.  
         [0033]    Tissue distribution of SR-BI  
         [0034]    To explore the physiological functions of SR-BI, the tissue distribution of SR-BI was determined in murine tissues, both in control animals and estrogen treated animals, as described in the following examples. Each lane is loaded with 0.5 μg of poly(A)+ RNA prepared from various murine tissues: kidney, liver, adrenals, ovaries, brain, testis, fat, diaphragm, heart, lung, spleen, or other tissue. The blots are hybridized with a 750 base pair fragment of the coding region of SR-BI. SR-BI mRNA is most highly expressed in adrenals, ovary and liver is moderately or highly expressed in fat depended on the source and is expressed at lower levels in other tissues. Blots using polyclonal antibodies to a cytoplasmic region of SR-BI demonstrate that very high levels of protein are present in liver, adrenal tissues, and ovary in mice and rats, but only very low or undetectable levels are present in either white or brown fat, muscle or a variety of other tissues. Bands in the rat tissues were present at approximately 82 kD. In the mouse tissues, the 82 kD form observed in the liver and steroidogenic tissues is the same size observed in SR-BI-transfected cultured cells.  
         [0035]    Assays for testing compounds for useful activity can be based solely on interaction with the receptor protein, preferably expressed on the surface of transfected cells such as those described above, although proteins in solution or immobilized on inert substrates can also be utilized, where the indication is inhibition or increase in binding of lipoproteins.  
         [0036]    Alternatively, the assays can be based on interaction with the gene sequence encoding the receptor protein, preferably the regulatory sequences directing expression of the receptor protein. For example, antisense which binds to the regulatory sequences, and/or to the protein encoding sequences can be synthesized using standard oligonucleotide synthetic chemistry. The antisense can be stabilized for pharmaceutical use using standard methodology (encapsulation in a liposome or microsphere; introduction of modified nucleotides that are resistant to degradation or groups which increase resistance to endonucleases, such as phosphorothiodates and methylation), then screened initially for alteration of receptor activity in transfected or naturally occurring cells which express the receptor, then in vivo in laboratory animals. Typically, the antisense would inhibit expression. However, sequences which block those sequences which “turn off” synthesis can also be targeted.  
         [0037]    II. Methods of Regulation of SR-BI Cholesterol Transport.  
         [0038]    The HDL receptor SR-BI plays an important role in controlling the structure and metabolism of HDL (Acton, et al. (1996)  Science  271, 518-20; Krieger, M. (1999)  Annu Rev Biochem  68, 523-58). Studies in mice have shown that alterations in SR-BI expression can profoundly influence several physiologic systems, including those involved in biliary cholesterol secretion, female fertility, red blood cell development, atherosclerosis and the development of coronary heart disease (Trigatti, et al. (1999)  Pro. Nat. Acad. Sci. USA  96, 9322-7; Kozarsky, et al. (2000)  Arterio. Thromb. Vasc. Biol.  20, 721-7; Arai, et al. (1999)  J. Biol. Chem.  274, 2366-71; Holm, et al. (2002)  Blood  99, 1817-24; Miettinen, et al. (2001)  J. Clin. Invest.  108, 1717-22; Ueda, et al. (2000)  J. Biol. Chem.  275, 20368-73; Kozarsky, et al. (1997)  Nature  387, 414-7; Braun, et al. (2002)  Cir. Res.  90, 270-276; Mardones, et al. (2001)  J. Lipid Res.  42, 170-180)) SR-BI controls HDL metabolism by mediating the cellular selective uptake of cholesteryl esters and other lipids from plasma HDL. During selective uptake (Glass, et al. (1983)  Proc. Nat. Acad. Sci. USA  80, 5435-9; Glass, et al. (1985)  J. Biol. Chem.  260, 744-50; Stein, et al. (1983)  Biochimica et Biophysica Acta  752, 98-105), HDL binds to SR-BI and its lipids, primarily neutral lipids such as cholesteryl esters in the core of the particles, are transferred to the cells. The lipid-depleted particles are subsequently released back into the extracellular space. Although the mechanism of SR-BI-mediated selective lipid uptake and the subsequent intracellular transport of these lipids has only just begun to be explored (Krieger 1999; Krieger, M. (2001)  J Clin Invest  108, 793-7; Uittenbogaard, et al. (2002)  J. Biol. Chem.  277, 4925-4931), it is clearly fundamentally different from the pathway of receptor-mediated endocytosis via clathrin-coated pits and vesicles used by the low-density lipoprotein (LDL) receptor to deliver cholesterol esters from LDL to cells (Brown, M. S. &amp; Goldstein, J. L. (1986)  Science  232, 34-47). SR-BI can also mediate cholesterol efflux from cells to HDL (Temel, et al. (2002)  J Biol Chem  8, 8).  
         [0039]    It has now been demonstrated that SR-BI plays critical roles in HDL lipid metabolism and cholesterol transport. SR-BI appears to be responsible for cholesterol delivery to steroidogenic tissues and liver, and actually transfers cholesterol from HDL particles through the liver cells and into the bile canniculi, where it is passed out into the intestine. Data indicates that SR-BI is also expressed in the intestinal mucosa. It would be useful to increase expression of SR-BI in cells in which uptake of cholesterol can be increased, freeing HDL to serve as a means for removal of cholesterol from storage cells such as foam cells where it can play a role in atherogenesis.  
         [0040]    Compounds which alter receptor protein binding are preferably administered in a pharmaceutically acceptable vehicle. Suitable pharmaceutical vehicles are known to those skilled in the art. For parenteral administration, the compound will usually be dissolved or suspended in sterile water, phosphate buffered saline, or saline. For enteral administration, the compound will be incorporated into an inert carrier in tablet, liquid, or capsular form. Suitable carriers may be starches or sugars and include lubricants, flavorings, binders, and other materials of the same nature. The compounds can also be administered locally by topical application of a solution, cream, gel, or polymeric material (for example, a Pluronic™, BASF). The compounds may also be formulated for sustained or delayed release.  
         [0041]    Alternatively, the compound may be administered in liposomes or microspheres (or microparticles). Methods for preparing liposomes and microspheres for administration to a patient are known to those skilled in the art. U.S. Pat. No. 4,789,734 describe methods for encapsulating biological materials in liposomes. Essentially, the material is dissolved in an aqueous solution, the appropriate phospholipids and lipids added, along with surfactants if required, and the material dialyzed or sonicated, as necessary. A review of known methods is by G. Gregoriadis, Chapter 14. “Liposomes”,  Drug Carriers in Biology and Medicine  pp. 287-341 (Academic Press, 1979). Microspheres formed of polymers or proteins are well known to those skilled in the art, and can be tailored for passage through the gastrointestinal tract directly into the bloodstream. Alternatively, the compound can be incorporated and the microspheres, or composite of microspheres, implanted for slow release over a period of time, ranging from days to months. See, for example, U.S. Pat. Nos. 4,906,474, 4,925,673, and 3,625,214.  
         [0042]    The present invention will be further understood by reference to the following non-limiting examples.  
       EXAMPLE 1  
     Identification of Chemical Inhibitors of the Selective Transfer of Lipids mediated by the HDL Receptor SR-BI  
       [0043]    Abbreviations  
                                                       HDL   High Density Lipoprotein           mSR-BI   Murine Scavenger Receptor, class B, type I           LDL   Low Density Lipoprotein           BLT   Block Lipid Transfer           DiI   1′-dioctadecyl-3,3,3′,3′-               tetramethylindocarbocyanine perchlorate           CE   Cholesteryl ether           DMSO   Dimethylsulfoxide           PBS   Phosphate Buffered Saline           EGF   Epidermal Growth Factor           VSV-G   Vesicular Stomatitis Virus Glycoprotein           EGFP   enhanced Green Fluorescent Protein           IC   Inhibitory Concentration           EC   Effective Concentration           ACTH   Adrenocorticotropic Hormone           FC   Free cholesterol                      
 
         [0044]    A high-throughput screen of a chemical library to identify potent small molecule inhibitors of SR-BI-mediated lipid transport. Five chemicals that block lipid transport, BLT-1-BLT-5 (BLT-1 corresponds to MIT 9952-53; BLT-2 corresponds to MIT 9952-61; BLT-3 corresponds to MIT 9952-19; BLT-4 corresponds to MIT 9952-29; and BLT-5 corresponds to MIT 9952-6), were tested and their effects on SR-BI activity in cultured cells. All five inhibited SR-BI-mediated selective lipid uptake from HDL and efflux of cellular cholesterol to HDL. One of these, BLT-1, was particularly potent, inhibiting lipid transport in the low nanomolar concentration range. Unexpectedly, all five BLTs enhanced HDL binding to SR-BI by increasing the binding affinity.  
         [0045]    Methods  
         [0046]    Lipoproteins and Cells  
         [0047]    Human HDL was isolated and labeled with either  125 I ( 125 I-HDL), 1,1′-dioctadecyl-3,3,3′,3′-tetramethylindocarbocyanine perchlorate (DiI, Molecular Probes; DiI-HDL) or [ 3 H]cholesteryl oleyl ether ([ 3 H]CE, [ 3 H]CE-HDL) (Gu, et al. (1998)  J.    
         [0048]    Biol. Chem. 273, 26338-48; Gu, et al. (2000)  J. Biol. Chem.  275, 29993-30001; Acton, et al. (1994)  J. Biol. Chem.  269, 21003-9; Pitas, et al. (1981)  Arteriosclerosis  1, 177-85). LDL receptor deficient Chinese hamster ovary cells that express low levels of endogenous SR-BI, ldlA-7 (Kingsley, et al. (1984)  Proc. Nat. Acad. Sci. USA  81, 5454-8), ldlA-7 cells stably transfected to express high levels of murine SR-BI (ldlA[mSR-BI])(Acton, et al., 1996), Y1-BS1 murine adrenocortical cells that express high levels of SR-BI after induction with ACTH (Rigotti, et al. (1996)  J. Biol. Chem.  271, 33545-9), monkey kidney BS-C1 cells (Kapoor, et al. (2000)  Journal of Cell Biology  150, 975-88) and HeLa cells (Temel, et al. (2002)  J Biol Chem  8, 8) were maintained as previously described.  
         [0049]    High Throughput Screen  
         [0050]    On day 0, ldlA[mSR-BI] cells were plated at 15,000 cells/well in clear bottom, black wall 384-well black assay plates (Costar) in 50 μl of medium A (Ham&#39;s F12 supplemented with 2 mM L-glutamine, 50 units/ml penicillin/50 μg/ml streptomycin, and 0.25 mg/ml G418.) supplemented with 10% fetal bovine serum (medium B). On day 1, cells were washed once with medium C (medium A with 1% (w/v) bovine serum albumin (BSA) and 25 mM HEPES pH 7.4, but no G418) and refed with 40 μl of medium C.  
         [0051]    Compounds (16,320 from the DiverSet E, Chembridge Corp.) dissolved in 100% DMSO were individually robotically ‘pin’ transferred (40 nl) (http://iccb.med.harvard.edu) to the wells to give a nominal concentration of 10 μM (0.01% DMSO). After an 1 hr incubation at 37° C., DiI-HDL (final concentration of 10 μg protein/ml) in 20 μl of medium C was added. Two hours later, fluorescence was measured at room temperature (approximately 2 minutes/plate) using a Analyst plate reader (Rhodamine B dichroic filter, emission 525 nm and excitation 580 nm; LJL Biosystems), both prior to removing the incubation medium (to test for autofluorescence and quenching) and after the medium removal and four washes with 80 μl of PBS/1 mM MgCl 2 /0.1 mM CaCl 2  to determine cellular uptake of DiI. All compounds were sampled in duplicate on different plates, and each screen included ldlA-7 and ldlA[mSR-BI] cells in the presence and/or absence of a 40-fold excess of unlabeled HDL, but with no added compounds, as controls.  
         [0052]    Assays  
         [0053]    For the assays, all media and buffers contained 0.5% DMSO and 0.5% bovine serum albumin to maintain compound solubility. Cells were pre-incubated with BLTs for 1 hr (or 2.5 hrs for transferrin, EGF and cholera toxin uptake experiments) and all the experiments were performed at 37° C. Detailed characterization of the BLTs and their effects was performed with compounds whose identities and purities were confirmed by LC-MS.  
         [0054]    (i) Lipid Uptake from HDL, Cholesterol Efflux to HDL and HDL Binding Assays.  
         [0055]    Assays for the uptake of lipids from DiI-HDL and [ 3 ]CE-HDL, efflux of [ 3 H]cholesterol from labeled cells, and  125 I-HDL binding were performed as described by Acton et al.  Science  (1996) January 26;271(5248):518-20; Gu, et al.  J Biol. Chem.  (2000) September 29;275(39):29993-30001; and Ji, et al.,  J. Biol. Chem.  (1997) 272, 20982-5. In some experiments, values were normalized so that the 100% of control represents activity in the absence of compounds and 0% represents activity determined in the presence of a 40-fold excess of unlabeled HDL or, for Y1-BS1 cells, in the presence of a 1:500 dilution of the KKB-1 blocking antibody (Gu, et al., 2000, generous gift from Karen Kozarsky). The amounts of cell-associated [ 3 H]cholesteryl ether are expressed as the equivalent amount of [ 3 H]CE-HDL protein (ng) to permit direct comparison of the relative amounts of  125 I-HDL binding and [ 3 H]CE uptake.  
         [0056]    The rates of HDL dissociation from cells were determined by incubation of the cells with  125 I-HDL (10 μg protein/ml, 2 hrs, 37° C.) with and without BLTs. The medium was then either replaced with the same medium in which the  125 I-HDL was substituted by a 40-fold excess of unlabeled HDL or a 40-fold excess of unlabeled HDL was added to the labeled incubation medium. The amounts of cell-associated  125 I-HDL were then determined as a function of time. The two methods gave similar results.  
         [0057]    (ii) Fluorescence Microscopic Analysis of Intracellular Trafficking and Cytoskeletal Organization.  
         [0058]    Receptor mediated endocytosis of Alexa-594 labeled transferrin or FITC labeled epidermal growth factor (EGF, Molecular Probes) by HeLa cells (Spiro, et al. (1996)  Mol Biol Cell  7, 355-67) and uptake of Alexa-594-labeled holo-cholera toxin (kind gift of Dr Wayne Lencer, Childrens Hospital, HMS) by BSC-1 cells were detected by fluorescent microscopy. The intracellular transport of the temperature sensitive glycoprotein of vesicular stomatitis virus (VSVG ts045 ) fused at its carboxyl terminus to EGFP (VSVG ts045 -EGFP) from the endoplasmic reticulum to the plasma membrane, after a shift from 40° C. to 32° C. for 2 hrs, was determined by fluorescent microscopy. The effects of the compounds on the distribution of actin using rhodamine labeled phalloidin and tubulin using the FITC labeled DM1 α monoclonal antibody (Sigma Co.) in ldlA[mSR-BI] cells were determined as described by Rigotti, et al. (1996)  J. Biol. Chem.  271, 33545-9 by fluorescence microscopy using an air 63× objective (Nikon).  
         [0059]    (iii) Flow Cytometric Analysis of SR-BI Cell Surface Expression.  
         [0060]    Cells were incubated for 3 hrs (medium C) with or without BLTs at their IC CE 95 concentrations, harvested with PBS containing 2 mM EDTA and compounds, and the levels of SR-BI surface expression in unfixed cells were determined by flow cytometry with the KKB-1 antibody (Gu, et al. (1998)  J. Biol. Chem.  273, 26338-48).  
         [0061]    Results  
         [0062]    High-Throughput Screening for Inhibitors of SR-BI-Mediated Selective Lipid Uptake.  
         [0063]    Cellular uptake and accumulation of the fluorescent lipophilic dye DiI from DiI-labeled HDL (DiI-HDL) is a reliable surrogate of SR-BI-dependent selective uptake of the cholesteryl esters in HDL. To identify small molecule inhibitors of SR-BI-mediated selective lipid uptake, 16,320 compounds representing the DiverSet E of the Chembridge library collection were screened for their abilities to block the cellular uptake of DiI from DiI-HDL. The compounds were tested at a nominal concentration of 10 micromolar in a 384-well-plate assay using ldlA[mSR-BI] cells that express a high level of mSR-BI.  
         [0064]    [0064]FIG. 1 shows results from a representative assay plate along with controls (no compounds, addition of excess unlabeled HDL or use of untransfected ldlA-7 cells). The figure is an example of a fluorescent read-out obtained from a single 384-well plate during the first round of the high-throughput screen. SR-BI-expressing ldlA[mSR-BI] cells were plated into 384-well plates and the effect of approximately 10 micromolar compounds on the uptake of DiI from DiI-HDL (10 μg protein/ml) was determined using a high speed fluorescence plate reader. Columns 1-20 show results (fluorescence in arbitrary units) from 16 independent wells per column (different colored symbols) from a single plate, representing a total of 320 compounds. Controls without compounds are wells either containing ldlA[mSR-BI] cells in the absence or presence of a 40-fold excess of unlabeled HDL, or containing untransfected ldlA-7 cells (very low SR-BI expression). Wells containing an inhibitory compound named BLT-1 and wells with compounds that quenched DiI-HDL fluorescence (Q) are indicated.  
         [0065]    Compounds that quenched (‘Q’) or enhanced the intrinsic fluorescence of DiI-HDL were not examined further. Approximately 200 compounds that reproducibly blocked DiI uptake in a first round of screening were retested. These are shown in Table I.  
                     TABLE I                       Structures of SR-BI Inhibitors                                                                                  MIT 9952-1                                                         MIT 9952-2                                                         MIT 9952-3                                                         MIT 9952-4                                                         MIT 9952-5                                                         MIT 9952-6                                                         MIT 9952-7                                                         MIT 9952-8                                                         MIT 9952-9                                                         MIT 9952-10                                                         MIT 9952-11                                                         MIT 9952-12                                                         MIT 9952-13                                                         MIT 9952-14                                                         MIT 9952-15                                                         MIT 9952-16                                                         MIT 9952-17                                                         MIT 9952-18                                                         MIT 9952-19                                                         MIT 9952-20                                                         MIT 9952-21                                                         MIT 9952-22                                                         MIT 9952-23                                                         MIT 9952-24                                                         MIT 9952-25                                                         MIT 9952-26                                                         MIT 9952-27                                                         MIT 9952-28                                                         MIT 9952-29                                                         MIT 9952-30                                                         MIT 9952-31                                                         MIT 9952-32                                                         MIT 9952-33                                                         MIT 9952-34                                                         MIT 9952-35                                                         MIT 9952-36                                                         MIT 9952-37                                                         MIT 9952-38                                                         MIT 9952-39                                                         MIT 9952-40                                                         MIT 9952-41                                                         MIT 9952-42                                                         MIT 9952-43                                                         MIT 9952-44                                                         MIT 9952-45                                                         MIT 9952-46                                                         MIT 9952-47                                                         MIT 9952-48                                                         MIT 9952-49                                                         MIT 9952-50                                                         MIT 9952-51                                                         MIT 9952-52                                                         MIT 9952-53                                                         MIT 9952-54                                                         MIT 9952-55                                                         MIT 9952-56                                                         MIT 9952-57                                                         MIT 9952-58                                                         MIT 9952-59                                                         MIT 9952-60                                                         MIT 9952-61                                                         MIT 9952-62                                                         MIT 9952-63                                                         MIT 9952-64                                                         MIT 9952-65                                                         MIT 9952-66                                                         MIT 9952-67                                                         MIT 9952-68                                                         MIT 9952-69                                                         MIT 9952-70                                                         MIT 9952-71                                                         MIT 9952-72                                                         MIT 9952-73                                                         MIT 9952-74                                                         MIT 9952-75                                                         MIT 9952-76                                                         MIT 9952-77                                                         MIT 9952-78                                                         MIT 9952-79                                                         MIT 9952-80                                                         MIT 9952-81                                                         MIT 9952-82                                                         MIT 9952-83                                                         MIT 9952-84                                                         MIT 9952-85                                                         MIT 9952-86                                                         MIT 9952-87                                                         MIT 9952-88                                                         MIT 9952-89                                                         MIT 9952-90                                                         MIT 9952-91                                                         MIT 9952-92                                                         MIT 9952-93                                                         MIT 9952-94                                                         MIT 9952-95                                                         MIT 9952-96                                                         MIT 9952-97                                                         MIT 9952-98                                                         MIT 9952-99                                                         MIT 9952-100                                                         MIT 9952-101                                                         MIT 9952-102                                                         MIT 9952-103                                                         MIT 9952-104                                                         MIT 9952-105                                                         MIT 9952-106                                                         MIT 9952-107                                                         MIT 9952-108                                                         MIT 9952-109                                                         MIT 9952-110                                                         MIT 9952-111                                                         MIT 9952-112                                                         MIT 9952-113                                                         MIT 9952-114                                                         MIT 9952-115                                                         MIT 9952-116                                                         MIT 9952-117                                                         MIT 9952-118                                                         MIT 9952-119                                                         MIT 9952-120                                                         MIT 9952-121                                                         MIT 9952-122                                                         MIT 9952-123                                                         MIT 9952-124                                                         MIT 9952-125                                                         MIT 9952-126                                                         MIT 9952-127                                                         MIT 9952-128                                                         MIT 9952-129                                                         MIT 9952-130                                                         MIT 9952-131                                                         MIT 9952-132                                                         MIT 9952-133                                                         MIT 9952-134                                                         MIT 9952-135                                                         MIT 9952-136                                                         MIT 9952-137                                                         MIT 9952-138                                                         MIT 9952-139                                                         MIT 9952-140                                                         MIT 9952-141                                                         MIT 9952-142                                                         MIT 9952-143                                                         MIT 9952-144                                                         MIT 9952-145                                                         MIT 9952-146                                                         MIT 9952-147                                                         MIT 9952-148                                                         MIT 9952-149                                                         MIT 9952-150                                                         MIT 9952-151                                                         MIT 9952-152                                                         MIT 9952-153                                                         MIT 9952-154                                                         MIT 9952-155                                                         MIT 9952-156                                                         MIT 9952-157                                                         MIT 9952-158                                                         MIT 9952-159                                                         MIT 9952-160                                                         MIT 9952-161                                                         MIT 9952-162                                                         MIT 9952-163                                                         MIT 9952-164                                                         MIT 9952-165                                                         MIT 9952-166                                                         MIT 9952-167                                                         MIT 9952-168                                                         MIT 9952-169                                                         MIT 9952-170                                                         MIT 9952-171                                                         MIT 9952-172                                                         MIT 9952-173                                                         MIT 9952-174                                                         MIT 9952-175                                                         MIT 9952-176                                                         MIT 9952-177                                                         MIT 9952-178                                                         MIT 9952-179                                                         MIT 9952-180                                                         MIT 9952-181                                                         MIT 9952-182                                                         MIT 9952-183                                                         MIT 9952-184                                                         MIT 9952-185                                                         MIT 9952-186                                                         MIT 9952-187                                                         MIT 9952-188                                                         MIT 9952-189                                                         MIT 9952-190                                                         MIT 9952-191                                                         MIT 9952-192                                                         MIT 9952-193                                                         MIT 9952-194                                                         MIT 9952-195                                                         MIT 9952-196                                                         MIT 9952-197                                                         MIT 9952-198                                                         MIT 9952-199                                                         MIT 9952-200                                                         MIT 9952-201                                                         MIT 9952-202                                                         MIT 9952-203                                                         MIT 9952-204                                                         MIT 9952-205                                                         MIT 9952-206                                                         MIT 9952-207                                                         MIT 9952-208                                                         MIT 9952-209                                                         MIT 9952-210                                                         MIT 9952-211                                                         MIT 9952-212                                                         MIT 9952-213                                                         MIT 9952-214                                                         MIT 9952-215                                                         MIT 9952-216                                                         MIT 9952-217                                                         MIT 9952-218                                                         MIT 9952-219                                                         MIT 9952-220                                                         MIT 9952-221                                                         MIT 9952-222                                                         MIT 9952-223                                                         MIT 9952-224                                                         MIT 9952-225                                                         MIT 9952-226                                                         MIT 9952-227                                                         MIT 9952-228                                                         MIT 9952-229                                                         MIT 9952-230                                                         MIT 9952-231                                                         MIT 9952-232                                                         MIT 9952-233                                                         MIT 9952-234                                                         MIT 9952-235                                                         MIT 9952-236                                                         MIT 9952-237                                                         MIT 9952-238                                                         MIT 9952-239                                                         MIT 9952-240                                                         MIT 9952-241                                                         MIT 9952-242                                                         MIT 9952-243                                                         MIT 9952-244                                                         MIT 9952-245                                                         MIT 9952-246                                                         MIT 9952-247                                                         MIT 9952-248                                                         MIT 9952-249                                                         MIT 9952-250                                                         MIT 9952-251                                                         MIT 9952-252                                                         MIT 9952-253                                                         MIT 9952-254                                                         MIT 9952-255                                                         MIT 9952-256                                                         MIT 9952-257                                                         MIT 9952-258                                                         MIT 9952-259                                                         MIT 9952-260                                                         MIT 9952-261                                                         MIT 9952-262                                                         MIT 9952-263                                                         MIT 9952-264                                                         MIT 9952-265                                                         MIT 9952-266                                                         MIT 9952-267                                                         MIT 9952-268                                                         MIT 9952-269                                                         MIT 9952-270                                                         MIT 9952-271                                                         MIT 9952-272                                                         MIT 9952-273                                                         MIT 9952-274                                                         MIT 9952-275                                                         MIT 9952-276                                                         MIT 9952-277                                                         MIT 9952-278                                                         MIT 9952-279                                                         MIT 9952-280                                                         MIT 9952-281                                                         MIT 9952-282                                                         MIT 9952-283                                                         MIT 9952-284                                                         MIT 9952-285                                                         MIT 9952-286                                                         MIT 9952-287                                                         MIT 9952-288                                                                 MIT 9952-289                                                         MIT 9952-290                                                         MIT 9952-291                                                         MIT 9952-292                                                         MIT 9952-293                                                         MIT 9952-294                                                         MIT 9952-295                                                         MIT 9952-296                                                         MIT 9952-297                                                         MIT 9952-298                                                         MIT 9952-299                                                         MIT 9952-300                                                         MIT 9952-301                                                         MIT 9952-302                                                         MIT 9952-303                                                         MIT 9952-304                                                         MIT 9952-305                                                         MIT 9952-306                                                         MIT 9952-307                                                         MIT 9952-308                                                         MIT 9952-309                                                         MIT 9952-310                                                         MIT 9952-311                                                         MIT 9952-312                                                         MIT 9952-313                                                         MIT 9952-314                                                         MIT 9952-315                                                         MIT 9952-316                                                         MIT 9952-317                                                         MIT 9952-318                                                         MIT 9952-319                                                         MIT 9952-320                                                         MIT 9952-321                                                         MIT 9952-322                                                         MIT 9952-323                                                         MIT 9952-324                                                         MIT 9952-325                                                         MIT 9952-326                                                         MIT 9952-327                                                 MIT 9952-328                                                         MIT 9952-329                                                         MIT 9952-330                                                         MIT 9952-331                                                         MIT 9952-332                                                         MIT 9952-333                                                         MIT 9952-334                                                         MIT 9952-335                                                         MIT 9952-336                                                         MIT 9952-337                                                         MIT 9952-338                                                         MIT 9952-339                                                         MIT 9952-340                                                         MIT 9952-341                                                         MIT 9952-342                  
 
         [0066]    Five of the most effective compounds with IC DiI 50s in the micromolar or lower range (FIG. 2A) were designated BLT-1-BLT-5 and further characterized. Strikingly, the most potent of these, BLT-1 and BLT-2, inhibited in the nanomolar range and are structurally related (Table II). Inhibition of DiI uptake did not require de novo protein synthesis, because pretreatment of cells for 30 min with 100 micrograms/ml cycloheximide did not diminish their inhibitory effects. Finally, none of the BLTs substantially inhibited the low background level of uptake of DiI or [ 3 H]CE by untransfected ldlA-7 cells expressing minimal amounts of SR-BI.  
         [0067]    The IC CE 50s for inhibition of uptake of the more physiologic lipid [ 3 H]cholesteryl ether ([ 3 H]CE) from [ 3 H]CE-HDL by ldlA[mSR-BI] cells were similar to those for DiI uptake (FIG. 2B and Table II). The inhibition of [ 3  H]CE uptake was reversible (1 hr incubation with compounds followed by 3-6 hr washout period). Moreover, the compounds also blocked the uptake of [ 3 H]CE by YL-BS1 adrenocortical cells that express high levels of SR-BI (Rigotti, et al. (1996)  J. Biol. Chem.  271, 33545-9) (Table II), indicating that the inhibitory effects by the compounds are not cell-type specific. Experiments in which the cells or the labeled HDL were pre-incubated with the compounds indicated that the cells rather than the HDL were the target of the compounds.  
                                                                                             TABLE 2                           Results of Testing for SR-BI binding.                ENDOVIS   ENDOHDL   ENDOQUENCH                Test   Test   Test   Test   Test   Test       Chemical ID   1   2   1   2   1   2                    MIT 9952-1   0       0.62   0.55   1.04   1.14       MIT 9952-2   0       1.34   1.2   1.1   1.06       MIT 9952-3   0       1.32   1.17   1.06   1.2       MIT 9952-4   0       1.17   1.33   1.06   1       MIT 9952-5   0       1.19   1.75   1.02   1.03       MIT 9952-6   0       0.52   0.54   0.99   1.03       MIT 9952-7   0       0.5   0.51   1.02   1.1       MIT 9952-8       MIT 9952-9   0       MIT 9952-10       MIT 9952-11       MIT 9952-12   0       1.25   1.26   0.9   0.93       MIT 9952-13   0       0.55   0.67   0.94   0.94       MIT 9952-14   0       1.24   1.21   1.16   1.07       MIT 9952-15   0       0.55   0.61   0.87   0.81       MIT 9952-16   0       1.25   1.26   0.92   0.99       MIT 9952-17   0       1.32   1.17   1.06   1.12       MIT 9952-18   0       1.21   1.22   1.01   1.06       MIT 9952-19   0   5       MIT 9952-20   0   0       MIT 9952-21   0       1.26   1.58   0.94   0.94       MIT 9952-22   0       1.27   1.4   1.01   1       MIT 9952-23   1   1       MIT 9952-24   0   0       MIT 9952-25   0       1.21   1.69   0.98   0.98       MIT 9952-26   0       1.28   1.32   0.95   0.97       MIT 9952-27   0       1.36   1.17   0.9   0.88       MIT 9952-28   7       1.96   1.61   1.0   1.06       MIT 9952-29   0       0.62   0.6   0.94   0.99       MIT 9952-30   0       0.51   0.43   0.91   0.88       MIT 9952-31   0       1.33   1.17   1.01   1.07       MIT 9952-32   0       1.26   1.21   0.9   1.0       MIT 9952-33   0       1.37   1.5   1.04   1.0       MIT 9952-34   0       1.28   1.34   0.94   1.09       MIT 9952-35   0       0.56   0.56   0.99   0.93       MIT 9952-36   0       1.22   1.36   1.02   1.97       MIT 9952-37   0       1.23   1.36   1.03   1.13       MIT 9952-38   0       0.34   0.52   0.17   0.12       MIT 9952-39   0       1.22   1.39   1.08   1.05       MIT 9952-40   0       1.28   1.23   1.01   1.97       MIT 9952-41   0       1.32   1.25   1.06   0.92       MIT 9952-42   0       1.27   1.21   0.97   0.99       MIT 9952-43   0       1.44   1.32   1.09   1.08       MIT 9952-44   0       0.42   0.39   0.86   0.95       MIT 9952-45   0       0.44   0.46   1.35   1.27       MIT 9952-46   0       1.32   1.18   0.99   0.98       MIT 9952-47   0       1.18   1.37   1.14   0.98       MIT 9952-48   0       0.68   0.49   1.13   1.18       MIT 9952-49   0       1.47   1.35   0.95   0.91       MIT 9952-50   0       1.27   1.98   1.02   0.98       MIT 9952-51   0       0.33   0.46   1.02   0.93       MIT 9952-52   0       1.22   1.35   0.92   0.91       MIT 9952-53   0       0.53   0.46   1.0   1.03       MIT 9952-54   6       0.46   0.59   0.95   0.9       MIT 9952-55   0       0.52   0.46   0.98   1.05       MIT 9952-56   0       1.26   1.26   0.91   0.95       MIT 9952-57   0       1.13   1.25   1.05   1.96       MIT 9952-58   0       1.28   1.19   1.02   1.11       MIT 9952-59   0       0.35   0.44   0.86   0.93       MIT 9952-60   0       1.13   1.17   0.89   1.07       MIT 9952-61   0       0.7   0.57   1.09   1.01       MIT 9952-62   0       1.28   1.24   0.99   0.9       MIT 9952-63   0       0.69   0.63   0.95   0.85       MIT 9952-64   0       0.58   0.58   0.98   0.92       MIT 9952-65   0       1.29   1.24   1.07   1.02       MIT 9952-66   0       1.22   1.11   1.96   1.03       MIT 9952-67   0       0.55   0.54   1.24   0.94       MIT 9952-68   0       0.57   0.69   0.84   0.98       MIT 9952-69   0       1.18   1.32   1.07   1.1       MIT 9952-70 (1 st )   0       0.45   0.75   0.97   0.88       MIT 9952-71   0       0.62   0.55   1.04   1.14       MIT 9952-72   0   0   1.07   1.12   1.01   0.93       MIT 9952-73   0   0   0.61   0.59   1.02   1.04       MIT 9952-74   0   0   0.71   0.69   0.83   0.88       MIT 9952-75   0   0   0.64   0.71   1.05   1.95       MIT 9952-76   0       1.25   1.26   0.9   0.93       MIT 9952-77   0       0.55   0.67   0.94   0.94       MIT 9952-78   0       1.25   1.26   0.9   0.93       MIT 9952-79   1       0.61   0.63   1.0   0.97       MIT 9952-80   0       1.34   1.2   1.1   1.06       MIT 9952-81   0       1.32   1.17   1.06   1.2       MIT 9952-82   0       1.27   1.4   1.02   1.0       MIT 9952-83   0       1.25   1.26   0.92   0.99       MIT 9952-84   0   0   0.74   0.66   0.83   0.81       MIT 9952-85   0   0   0.56   0.68   1.03   1.12       MIT 9952-86   0       1.24   1.21   1.16   1.07       MIT 9952-87   0   0   0.67   0.67   0.9   0.99       MIT 9952-88   0   0   0.73   0.77   0.92   0.97       MIT 9952-89   0       0.55   0.61   0.87   0.81       MIT 9952-90   0   0   0.62   0.61   1.14   1.02       MIT 9952-91   0   0   0.52   0.54   0.99   1.03       MIT 9952-92   0   0   0.7   0.63   1.11   1       MIT 9952-93   0   0   0.66   0.71   0.95   0.91       MIT 9952-94   0       1.21   1.22   1.01   1.06       MIT 9952-95   2   2   0.79   0.73   0.96   1.03       MIT 9952-96   0       1.32   1.17   1.06   1.2       MIT 9952-97   5   5   0.74   0.69   0.94   0.9       MIT 9952-98   0   5       MIT 9952-99   0   0       MIT 9952-100   0       0.5   0.51   1.02   1.1       MIT 9952-101   0   0       MIT 9952-102   0   0   0.56   0.49   1.05   1.05       MIT 9952-103   1   1   0.56   0.61   0.96   1.09       MIT 9952-104   0   0       MIT 9952-105   0   0       MIT 9952-106   0   0   0.6   0.53   1.16   1.16       MIT 9952-107   1   1       MIT 9952-108   0   0       MIT 9952-109   0       1.19   1.75   1.02   1.03       MIT 9952-110   0       1.17   1.33   1.06   1.1       MIT 9952-111       MIT 9952-112   0   0       MIT 9952-113       MIT 9952-114   0   0       MIT 9952-115       (2 nd )       MIT 9952-116   0   0       MIT 9952-117   0       1.26   1.58   0.94   0.94       MIT 9952-118   0       0.51   0.63   0.91   1.11       MIT 9952-119   0   0   0.62   0.64   1.06   1.04       MIT 9952-120   0       1.21   1.69   0.98   0.98       MIT 9952-121   0   0   0.54   0.57   0.95   1.02       MIT 9952-122   0   0   0.55   0.82   0.82   0.82       MIT 9952-123   0   0   0.59   0.64   1.02   1.05       MIT 9952-124   0       1.33   1.17   1.01   1.17       MIT 9952-125   0   0   0.63   0.66   1.0   0.99       MIT 9952-126   0   0   0.55   0.53   0.93   0.98       MIT 9952-127   0   0   0.62   0.6   0.97   0.92       MIT 9952-128   0       1.23   1.36   1.03   1.13       MIT 9952-129   0   0   0.57   0.54   0.8   0.79       MIT 9952-130   0   0   0.62   0.65   0.96   1.05       MIT 9952-131   0   0   0.56   0.52   0.9   0.92       MIT 9952-132   0   0   0.65   0.46   1.15   1.17       MIT 9952-133   0   0   0.5   0.52   1.15   1.09       MIT 9952-134   0   0   0.58   0.59   0.9   0.9       MIT 9952-135   0   0   0.44   0.46   1.35   1.27       MIT 9952-136   0   0   0.63   0.59   1.12   1.1       MIT 9952-137   0   0   1.32   1.25   1.06   0.92       MIT 9952-138   0   0   0.54   0.63   1.11   1.04       MIT 9952-139   0       1.22   1.39   1.08   1.05       MIT 9952-140   0   0   0.52   0.58   1.44   1.37       MIT 9952-141   0   0   0.63   0.77   1.0   0.99       MIT 9952-142   0       1.28   1.32   0.95   0.97       MIT 9952-143   0   0   0.66   0.65   1.15   1.03       MIT 9952-144   0       0.56   0.56   0.99   0.93       MIT 9952-145   0       1.28   1.34   0.94   1.09       MIT 9952-146   0   0   0.62   0.71   0.95   1.02       MIT 9952-147   0   0   0.63   0.53   0.9   0.99       MIT 9952-148   0       1.44   1.32   1.09   1.08       MIT 9952-149   0   0   0.62   0.6   0.94   0.99       MIT 9952-150   0       0.34   0.52   0.17   0.16       MIT 9952-151(3 rd )   0       1.22   1.36   1.02   1.97       MIT 9952-152   0       0.51   0.43   0.91   0.88       MIT 9952-153   0   0   0.6   0.57   0.88   0.91       MIT 9952-154   0   0   0.47   0.45   0.07   0.08       MIT 9952-155   0   0   0.69   0.47   1.04   1.17       MIT 9952-156   0   0   0.57   0.62   1.09   1.03       MIT 9952-157   0   0   1.26   1.21   0.9   1.0       MIT 9952-158   0       0.42   0.39   0.86   0.95       MIT 9952-159   0       1.28   1.23   1.01   0.97       MIT 9952-160   0       0.48   0.55   0.96   1.0       MIT 9952-161   0   0   1.37   1.5   1.04   1.0       MIT 9952-162   0   0   0.55   0.4   1.01   0.95       MIT 9952-163   0   0   0.6   0.69   1.0   1.01       MIT 9952-164   0       0.6   0.61   0.88   0.89       MIT 9952-165   0       0.57   0.6   0.93   0.94       MIT 9952-166   0       0.56   0.67   0.95   0.99       MIT 9952-167   0       1.32   1.18   0.99   0.98       MIT 9952-168   4   4   0.5   0.56   0.93   1.12       MIT 9952-169   0   0   0.54   0.6   1.0   1.04       MIT 9952-170   0   0   0.54   0.54   0.12   0.1       MIT 9952-171   0   0   0.58   0.54   0.96   1.03       MIT 9952-172   0   0   0.55   0.56   0.92   0.84       MIT 9952-173   7       1.96   1.61   1.0   1.06       MIT 9952-174   0   0   0.6   0.62   0.85   0.84       MIT 9952-175   0   0   0.42   0.51   1.0   0.98       MIT 9952-176   0       1.36   1.17   0.9   0.88       MIT 9952-177   0   0   0.68   0.49   1.13   1.18       MIT 9952-178   0   0   0.4   0.38   0.95   0.86       MIT 9952-179   0   0   0.54   0.54   1.08   1.04       MIT 9952-180(4 th )   0   0   0.43   0.45   1.14   1.02       MIT 9952-181   0   0   0.6   0.54   1.07   0.95       MIT 9952-182   0   0   0.71   0.41   0.95   1.1       MIT 9952-183   0   0   0.59   0.65   0.94   1.0       MIT 9952-184   0   0   0.6   0.58   0.93   0.94       MIT 9952-185   0   0   0.53   0.46   1.0   1.03       MIT 9952-186   0   0   0.5   0.5   1.07   1.05       MIT 9952-187   0       0.33   0.46   1.02   0.93       MIT 9952-188   0   0   0.61   0.58   0.94   1.08       MIT 9952-189   0   0   0.56   0.58   1.09   1.0       MIT 9952-190   0       1.47   1.35   0.95   0.91       MIT 9952-191   0       1.27   1.98   1.02   0.98       MIT 9952-192   0   0   0.57   0.52   1.1   1.09       MIT 9952-193   0   0   0.66   0.69   0.92   1.0       MIT 9952-194   0   0   0.76   0.46   0.97   1.02       MIT 9952-195   0       1.22   1.35   0.92   0.91       MIT 9952-196   0   0   0.63   0.6   1.09   1.07       MIT 9952-197   0   0   0.58   0.71   0.95   0.96       MIT 9952-198   0   0   0.67   0.64   1.07   1.11       MIT 9952-199   0   0   0.52   0.46   0.98   1.05       MIT 9952-200   0   0   0.73   0.8   1.02   0.96       MIT 9952-201   0   0   0.69   0.67   1.26   1.25       MIT 9952-202   0   0   1.23   1.11   0.98   1.03       MIT 9952-203   0   0   0.73   0.7   0.97   1.0       MIT 9952-204   0   0   0.55   0.62   0.78   1.07       MIT 9952-205   0   0   1.08   1.0   0.93   1.03       MIT 9952-206   0   0   0.56   0.52   1.05   1.1       MIT 9952-207   0       1.28   1.19   1.02   1.11       MIT 9952-208   0   0   0.57   0.55   0.95   0.98       MIT 9952-209   6       0.46   0.59   0.95   0.9       (5 th )       MIT 9952-210   0   0   0.59   0.56   0.88   0.91       MIT 9952-211   0   0   0.59   0.56   1.02   1.07       MIT 9952-212   0   0   0.57   0.49   1.0   0.95       MIT 9952-213   0   0   0.66   0.57   0.92   0.96       MIT 9952-214   0   0   0.63   0.35   1.05   1.0       MIT 9952-215   0   0   0.57   0.53   1.03   1.04       MIT 9952-216   0   0   0.54   0.58   1.1   1.14       MIT 9952-217   0   0   0.57   0.53   1.0   0.98       MIT 9952-218   0   0   0.64   0.33   1.06   1.0       MIT 9952-219   0   0   0.55   0.55   0.95   0.98       MIT 9952-220   0   0   1.13   1.25   1.05   0.96       MIT 9952-221   0   0   0.62   0.59   1.01   0.91       MIT 9952-222   4   4   0.58   0.6   1.07   0.9       MIT 9952-223   0   0   0.64   0.57   1.06   1.05       MIT 9952-224   0   0   0.6   0.5   0.99   0.97       MIT 9952-225   0   0   0.56   0.59   1.05   1.03       MIT 9952-226   0   0   0.5   0.56   0.95   1.0       MIT 9952-227   0   0   0.58   0.53   0.96   1.0       MIT 9952-228   0   0   0.46   0.63   0.93   0.94       MIT 9952-229   0   0   0.58   0.58   1.22   1.31       MIT 9952-230   2   2   0.61   0.51   0.99   1.01       MIT 9952-231   0   0   0.46   0.54   0.99   0.96       MIT 9952-232   0   0   0.61   0.56   0.99   1.02       MIT 9952-233   0   0   0.59   0.33   1.0   0.94       MIT 9952-234   0   0   0.58   0.54   0.94   0.93       MIT 9952-235   0   0   0.62   0.33   0.91   1.06       MIT 9952-236   0   0   0.57   0.38   0.97   1.23       MIT 9952-237   0   0   0.53   0.39   0.91   0.83       MIT 9952-238   0   0   0.61   0.6   1.01   1.13       MIT 9952-239   0   0   0.48   0.4   0.9   0.96       (6 th )       MIT 9952-240   0   0   0.64   0.71   0.97   1.07       MIT 9952-241   1   1   0.48   0.52   0.92   0.93       MIT 9952-242   0       1.26   1.26   0.91   0.95       MIT 9952-243   0   0   0.42   0.6   1.05   1.09       MIT 9952-244   0   0   0.56   0.54   1.02   1.07       MIT 9952-245   0   0   0.54   0.64   1.03   1.02       MIT 9952-246   0   0   0.56   0.52   0.99   0.98       MIT 9952-247   0   0   0.63   0.64   1.05   1.03       MIT 9952-248   0   0   0.68   0.66   0.98   0.91       MIT 9952-249   0   0   0.7   0.57   1.09   1.01       MIT 9952-250   0   0   1.28   1.24   0.99   0.9       MIT 9952-251   0   0   0.52   0.57   1.06   1.06       MIT 9952-252   1   1   0.58   0.39   0.98   0.9       MIT 9952-253   0   0   0.59   0.65   1.03   1.06       MIT 9952-254           0.69   1.01   0.91   1.05       MIT 9952-255   0   0   0.61   0.6   1.01   0.94       MIT 9952-256   0   0   0.65   0.92   0.92   0.97       MIT 9952-257   0   0   0.66   0.61   1.0   1.0       MIT 9952-258   0   0   0.51   1.0   0.88   0.82       MIT 9952-259   0   0   0.59   0.55   0.96   0.94       MIT 9952-260   0   0   0.56   0.58   1.06   1.04       MIT 9952-261   0   0   0.62   0.66   1.05   1.05       MIT 9952-262   0   0   0.53   0.45   0.98   1.01       MIT 9952-263   0   0   0.66   0.65   1.04   0.98       MIT 9952-264   0   0   0.45   0.56   1.1   1.11       MIT 9952-265   0   0   0.26   0.89   0.8   0.87       MIT 9952-266   0   0   0.71   0.68   1.08   1.01       MIT 9952-267   0   0   0.57   1.11   0.96   1.07       MIT 9952-268   0   0   0.59   0.65   0.98   1.04       (7 th )       MIT 9952-269   0   0   0.74   0.66   0.99   1.05       MIT 9952-270   0   0   0.66   0.66   0.95   0.96       MIT 9952-271   0   0   0.59   0.54   0.94   0.89       MIT 9952-272   0   0   0.61   0.51   0.91   0.92       MIT 9952-273   0   0   0.51   0.48   0.79   0.73       MIT 9952-274   0   0   0.65   0.6   0.93   0.93       MIT 9952-275   0   0   0.43   0.44   0.92   0.97       MIT 9952-276   0   0   0.73   0.68   1.03   1.0       MIT 9952-277   0   0   0.66   0.65   1.0   1.0       MIT 9952-278   0   0   0.71   0.67   1.09   0.98       MIT 9952-279   0   0   0.64   0.63   1.12   1.11       MIT 9952-280   0   0   0.75   0.67   1.01   1.12       MIT 9952-281   0   0   0.59   0.34   1.0   0.96       MIT 9952-282   0   0   0.49   0.5   0.82   0.89       MIT 9952-283   0   0   0.53   0.48   0.97   1.0       MIT 9952-284   0   0   0.65   0.54   0.91   0.96       MIT 9952-285   0   0   0.57   0.53   0.9   1.07       MIT 9952-286   0   0   0.62   0.64   0.96   1.11       MIT 9952-287   0       1.18   1.32   1.07   1.1       MIT 9952-288   0   0   0.59   0.52   0.77   0.77       MIT 9952-289   0   0   0.6   0.64   1.0   0.98       MIT 9952-290   0   0   0.52   0.56   0.87   0.82       MIT 9952-291   0   0   0.55   0.51   0.94   0.97       MIT 9952-292   0   0   0.47   0.58   1.06   1.01       MIT 9952-293   0   0   0.69   0.67   0.85   0.95       MIT 9952-294   0   0   0.61   0.56   0.93   0.95       MIT 9952-295   0   0   0.64   0.58   1.01   0.95       MIT 9952-296   0   0   0.63   0.61   1.05   0.98       MIT 9952-297   0   0   0.56   0.46   1.07   1.09       MIT 9952-298   0   0   1.29   1.24   1.07   1.02       (8 th )       MIT 9952-299   0       0.73   0.57   1.05   0.99       MIT 9952-300   0       0.66   0.66   1.18   0.97       MIT 9952-301   0       0.71   0.7   1.01   0.98       MIT 9952-302   0   0   0.52   0.55   0.79   0.85       MIT 9952-303   0       0.58   0.58   0.98   0.92       MIT 9952-304   0       0.35   0.44   0.86   0.93       MIT 9952-305   0   0   0.67   0.6   1.07   1.01       MIT 9952-306   0       0.79   0.72   1.0   0.96       MIT 9952-307   0       0.69   0.63   0.95   0.85       MIT 9952-308   0       0.57   0.69   0.84   0.98       MIT 9952-309   0       0.7   0.68   1.14   1.08       MIT 9952-310   0       0.97   1.11   0.96   1.01       MIT 9952-311   0       0.63   0.65   0.98   0.99       MIT 9952-312   0       0.45   0.75   0.97   0.88       MIT 9952-313   0       0.79   0.77   0.94   0.98       MIT 9952-314   0       0.55   0.54   1.24   0.94       MIT 9952-315   0   0   0.51   0.53   0.86   0.73       MIT 9952-316   0       0.71   0.72   1.13   1.1       MIT 9952-317   0       0.69   0.73   1.0   0.96       MIT 9952-318   0       0.67   0.81   1.18   0.94       MIT 9952-319   0       1.13   1.17   0.89   1.07       MIT 9952-320   0       0.54   0.83   1.04   1.01       MIT 9952-321   0       1.22   1.11   1.96   1.03       MIT 9952-322   0       0.79   0.86   0.1   0.96       MIT 9952-323   0   0   0.46   0.63   0.93   0.94       MIT 9952-324   0   0   0.55   0.56   0.92   0.84       MIT 9952-325   0   0   0.56   0.49   1.05   1.05       MIT 9952-326   0   0   0.55   0.53   0.93   0.98       MIT 9952-327   0   0   0.4   0.45   1.18   1.13       MIT 9952-328   4   4   0.5   0.56   0.93   1.12       MIT 9952-329   0   0   0.57   0.53   1.0   0.98       MIT 9952-330   0   0   0.59   0.56   1.02   1.07       MIT 9952-331   0   0   0.63   0.35   1.05   1.0       MIT 9952-332   0   0   0.69   0.67   1.26   1.25       MIT 9952-333   0   0   0.56   0.59   1.05   1.03       MIT 9952-334   0   0   0.57   0.55   0.95   0.98       MIT 9952-335   0   0   0.57   0.49   1.0   0.95       MIT 9952-336   0   0   0.54   0.58   1.1   1.14       MIT 9952-337   0   0   0.6   0.57   0.92   0.96       MIT 9952-338   0   0   0.61   0.6   1.01   1.13       (9 th )       MIT 9952-339   0   0   0.58   0.54   0.94   0.93       MIT 9952-340   0   0   0.48   0.44   0.9   0.96       MIT 9952-341   2   2   0.61   0.51   0.99   1.01       MIT 9952-342   0   0   0.43   0.44   0.92   0.97                  
 
         [0068]    Inhibition of Selective Lipid Uptake by BLTs is Specific.  
         [0069]    The specificity of BLT inhibition was tested by testing their effects on several other cellular properties at their concentrations that inhibit [ 3 H]CE uptake by 95% (IC CE 95) (FIG. 3). None of the BLTs disrupted the integrity of the actin- and tubulin networks. They also did not inhibit the uptake or alter the intracellular distribution of the fluorescently labeled endocytic receptor ligands transferrin and epidermal growth factor. The BLTs also failed to inhibit the uptake of fluorescently labeled cholera toxin from the cell surface to perinuclear regions through a pathway believed to depend in part on cholesterol- and sphingolipid-rich lipid rafts (Lencer, et al. (1999)  Biochim. Biophys. Acta  1450, 177-190). Moreover, BLTs did not interfere with the secretory pathway, as assessed by analysis of the transport of the enhanced green fluorescent protein-labeled integral viral membrane glycoprotein VSV G (VSVG ts045 -EGFP). Thus, BLTs do not induce general defects in clathrin-dependent and clathrin-independent intracellular membrane trafficking or in the organization of the cytoskeleton and are, by these criteria, specific inhibitors of SR-BI-dependent lipid uptake.  
         [0070]    BLTs Inhibit SR-BI-Mediated Cholesterol Efflux from Cells to HDL.  
         [0071]    In addition to mediating selective lipid uptake from HDL, SR-BI can facilitate the efflux of unesterified cholesterol from cells to HDL particles (Jian, et al. (1998)  J Biol Chem  273, 5599-606. Ji, et al. (1997)  J. Biol. Chem.  272, 20982-5). To determine if the BLTs could inhibit this SR-BI-mediated lipid transport activity, cells were labeled with [ 3 H]cholesterol and its efflux to unlabeled HDL measured in the presence or absence of the BLTs. (FIG. 2C, table II). Cells were incubated for 3 hrs in the absence (top panels) or presence (bottom panels) of 50 micromolar BLT-1 (MIT 9952-53) and epifluorescence light microscopy was used to monitor the following cellular activities: clathrin-dependent endocytosis of fluorescently labeled transferrin (A,B; HeLa cells) and EGF (C,D; HeLa cells); clathrin-independent endocytosis of fluorescently labeled cholera toxin (E, F; BSC-1 cells), and transport of the temperature sensitive fluorescent membrane protein VSVG ts045 -EGFP from the ER to the cell surface (G,H; BSC-1 cells). In addition, the intracellular distributions of the actin cytoskeleton (visualized with rhodamine labeled phalloidin, I,J; ldlA-[mSRBI] cells) and the tubulin network (visualized with fluorescently labeled antibodies specific to y-tubulin, K,L; BSC-1 cells) were determined. BLT-1 (MIT 9952-53) and the other BLTs (not shown) had no effects on any of these cellular properties or activities.  
         [0072]    As shown in Table III, all BLTs inhibited SR-BI-mediated cholesterol efflux with relative potencies (IC FC 50s) similar to those for [ 3 H]CE uptake; although in the cases of BLT-3 (MIT 9952-19), BLT-4 (MIT 9952-29) and BLT-5 (MIT 9952-6), the IC FC 50s for efflux were higher than those for uptake, suggesting that the BLTs may have uncovered possible differences in the mechanisms of uptake and efflux. The BLTs had little effect on the SR-BI-independent efflux (not inhibited by the specific anti-SR-BI blocking antibody KKB-1) (Kapoor, et al. (2000)  Journal of Cell Biology  150, 975-88). In untransfected ldlA-7 cells expressing relatively low levels of endogenous SR-BI, total and SR-BI-dependent (e.g. KKB-1-inhibitable) cholesterol efflux were substantially lower (˜5-10-fold) than in ldlA[mSR-BI] cells. The BLTs were able to inhibit the low SR-BI-dependent cholesterol efflux in ldlA-7 cells, but had no inhibitory effect on the similarly low SR-BI-independent efflux.  
                                                                                                                 TABLE III                                                                                                                                                   BLT-1   BLT-2           n   meant ± SD   meant ± SD                        (A) EC50 (μM)                   DiI-HDL uptake   3   0.06 ± 0.04   0.35 ± 0.18       [ 3 H]CEt HDL uptake   6   0.11 ± 0.08   0.24 ± 0.1        (Y1-BS1 cells)   2   0.38 NA   0.41 NA       [ 3 H]cholesterol efflux   3   0.15 ± 0.09   0.47 ± 0.23         1n I-HDL binding   3   0.088 ± 0.05    0.25 ± 0.13       (B) Binding       Parameters       apparent K d  (μg ml −1 )   3    4.7 ± 0.05   6.0 ± 6.0       K off  (min −1 )   2   0.06 NA   0.062 NA       Bmax (%)       95.8 ± 10.1   93.0 ± 20.5       EC 50  (μM)                                                                                                                        BLT-3   BLT-4           meant ± SD   meant ± SD                            (A) EC50 (μM)                   DiI-HDL uptake   0.51 ± 0.15   2.0 ± 1.0           [ 3 H]CEt HDL uptake   2.3 ± 1.5     12  3.9 1  ± 0.76           (Y1-BS1 cells)   1.7 NA   4.4 NA           [ 3 H]cholesterol efflux   17.2 ± 4.0    54.9 ± 35.2             1n I-HDL binding   46.5 ± 49.3   24.9 ± 14.8           (B) Binding           Parameters           apparent K d  (μg ml −1 )   8.0 ± 4.0   8.9 ± 2.3           K off  (min −1 )   0.08 NA   0.082 NA           Bmax (%)   85.8 ± 15.8   79.9 ± 15.9            EC 50  (μM)                                                                                              BLT-5   No ELT           meant ± SD   meant ± SD                            (A) EC50 (μM)                   DiI-HDL uptake   7.1 ± 3.7   —           [ 3 H]CEt HDL uptake   13.8 1  ± 8.5  11      —           (Y1-BS1 cells)   8.0 NA   —           [ 3 H]cholesterol efflux   75.3 ± 40.1   —             1n I-HDL binding   18.0 ± 3.7    —           (B) Binding           Parameters           apparent K d  (μg ml −1 )   12.0 ± 1.6    16.6 ± 1.5            K off  (min −1 )   0.079 NA   0.11 NA           Bmax (%)   92.1 ± 36.8   100.0 ± 18.4            EC 50  (μM)                                              
 
         [0073]    BLTs Do Not Change the Surface Expression of SR-BI.  
         [0074]    To determine if BLTs inhibited SR-BI function by reducing its cell surface expression, we measured surface expression using the KKB-1 anti-mSR-BI antibody and flow cytometry. FIG. 4 shows that, after a 3 hr incubation at their IC CE 95s (corresponding tol AM for BLTs 1 (MIT 9952-53) and 2 (MIT 9952-61), 50 μM for BLTs 3-5 (MIT 9952-19, MIT 9952-29, and MIT 9952-6)), the BLTs did not alter the expression of mSR-BI on the surfaces of ldlA[mSR-BI] cells.  
         [0075]    BLTs Enhance Binding of HDL to SR-BI.  
         [0076]    It was initially expected that the BLTs would function by inhibiting HDL binding to SR-BI. However, when cells were incubated with a sub-saturating concentration of either [ 3 H]CE-HDL or  125 I-labeled HDL ( 125 I-HDL) (10 μg protein/ml) and increasing amounts of compound (FIG. 5), the decreases in [ 3 H]CE uptake (solid lines, no symbols, data from FIG. 2B) and [3H]cholesterol efflux (dashed lines, data from FIG. 2C) were accompanied by corresponding increases in  125 I-HDL binding (solid lines, square symbols). The concentration dependence of  125 I-HDL binding was determined in the presence or absence of BLTs at their IC CE 95 concentrations (FIG. 6 and Table II). The BLTs did not substantially alter the number of binding sites (B max ), but rather induced small, yet significant, increases in the affinity of SR-BI for HDL (lower apparent Kds). Furthermore, the BLTs reduced the rates of dissociation of  125 I-HDL from SR-BI (Table II), indicating that the tighter binding induced by the BLTs was due, at least in part, to a decrease in the dissociation rate.  
         [0077]    Discussion  
         [0078]    200 compounds, shown in Table I, altering SR-BI mediated lipid transport were identified using in vitro assays. Results of testing are shown in Table II. BLT-1 (MIT 9952-53) through BLT-5 (MIT 9952-6) were identified as small molecules that inhibit the transfer of lipids between HDL and cells mediated by the HDL receptor SR-BI. BLTs inhibited both cellular selective lipid uptake of HDL cholesteryl ether and efflux of cellular cholesterol to HDL. The inhibitory effects of the BLTs were specific (for example, they specifically alter SR-BI binding), as they required the expression of active SR-BI receptors and they did not interfere with several clathrin-dependent and independent endocytic pathways, the secretory pathway nor the actin- or tubulin cytoskeletal networks. Strikingly, inhibition of lipid transfer by BLTs was accompanied by enhanced HDL binding affinity (reduced dissociation rates).  
         [0079]    Modifications and variations of the methods and materials described herein will be obvious to those skilled in the art and are intended to be encompassed by the following claims. The teachings of the references cited herein are specifically incorporated herein.