Cloning and Characterization of HB2, a Candidate High Density Lipoprotein Receptor
SEQUENCE HOMOLOGY WITH MEMBERS OF THE IMMUNOGLOBULIN SUPERFAMILY OF MEMBRANE PROTEINS*

(Received for publication, April 16, 1997)

Akiyo Matsumoto Dagger , Alana Mitchell §, Hideaki Kurata Dagger , Louise Pyle §, Kazuo Kondo Dagger , Hiroshige Itakura Dagger and Noel Fidge §

From the § Baker Medical Research Institute, Melbourne, Victoria 3181, Australia and the Dagger  National Institute of Health and Nutrition, Tokyo 162, Japan

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES


ABSTRACT

The protection against coronary artery disease attributed to high density lipoprotein (HDL) may be associated with several functions, including its central role in reverse cholesterol transport, possible antioxidant and antithrombotic properties and others not yet identified which may depend on specific interactions between HDL and cell receptors. Several HDL-binding proteins have been identified including two candidate liver HDL receptors, HB1 and HB2 recently purified in this laboratory. We now report the cloning, sequencing, and some properties of HB2, the most abundant of the pair. It shows significant homology with the adhesion molecules ALCAM and BEN of the immunoglobulin superfamily and the cDNA, when transfected into HepG2 or COS cells, caused specific HDL3 binding to increase by 80-100%. Further, ligand blotting of glycoproteins isolated from phorbol 12-myristate 13-acetate-treated THP-1 cells or from transfected HepG2 and Chinese hamster ovary cells also provided evidence of increased binding of HDL3 to HB2. Differentiation of THP-1 cells into macrophages resulted in a striking increase in HB2 mRNA which was attenuated if cells were cholesterol-loaded by incubation with acetylated low density lipoprotein. If the interaction between HDL and HB2 reduces the adhesion-induced inflammatory cellular events that characterize arterial wall injury, thereby achieving the protection associated with higher plasma levels of HDL, these findings may provide a clue to one mitigating effect of HDL in heart disease.


INTRODUCTION

The incidence of premature artery disease is lowered in the presence of high levels of circulating high density lipoprotein (HDL)1 suggesting that HDL may protect individuals against atherosclerosis (1). Part of this protection may be attributed to the participation of HDL in the reverse cholesterol transport pathway, a mechanism which reduces the accumulation of cholesterol in the arterial wall and the narrowing which subsequently occurs (2).

More recent evidence would indicate that HDL influences many other biological events in a manner consistent with a protective function, suggesting that the antiatherogenic role of HDL is likely to be complex. HDL may have antioxidant and antithrombotic properties (3-5), it may act as a signal transductant and as a secretagogue (6), and it may possibly influence the production of some cell adhesion molecules such as VCAM and ICAM (7).

Despite these observations, the mechanism(s) responsible for the HDL-induced physiological effects remain enigmatic. The fact that HDL binds to a variety of cells with varying degrees of specificity has invited speculation about the existence of an HDL receptor. Our laboratory (8) and others (9, 10) have purified liver cellular HDL-binding proteins, thereby strengthening the evidence for the existence of HDL receptor(s) that may have important functions as determinants of HDL metabolism. To date, only SR-B1, a member of the scavenger receptor class of membrane proteins that binds LDL, modified LDL and HDL, has been shown to elicit a physiological response, viz. the transfer of cholesteryl ester into cells, particularly in steroidogenic tissues (11).

We have identified two liver plasma membrane proteins named HB1 and HB2 (HDL-binding proteins 1 and 2) which are candidate HDL receptors (8, 12). Although present in low abundance, HB2 was purified in sufficient quantities to provide amino acid sequence data. This paper describes the subsequent cloning of HB2, its complete amino acid sequence, and evidence for increased binding of HDL to HB2 in cells overexpressing HB2.


MATERIALS AND METHODS

Cell Lines and Tissue Culture

HepG2, COS, CHO, and THP-1 cells were obtained from the American Type Culture Collection (Rockville, MD) and maintained under standard tissue culture conditions using Dulbecco's modified Eagle's medium for HepG2 and COS, alpha -minimal essential medium for CHO cells, and RPMI 1640 medium for THP-1 cells, plus 10% fetal bovine serum. THP-1 cells were differentiated into adherent macrophages by treatment with 200 nM phorbol 12-myristate 13-acetate (PMA) for 72 h.

Isolation and Labeling of HDL

Human HDL3 (d 1.12-1.21 g/ml) was obtained from plasma as described previously and contained apoAI and apoAII but no apoE (8). HDL3 was radioiodinated using IODOBEADS (Pierce) to specific activities ranging from 150-210 cpm/ng of protein. HDL3 was also labeled with [3H]cholesteryl oleoyl ether (13). Briefly, HDL3 was incubated with donor particles containing egg yolk phosphatidylcholine, [3H]cholesteryl oleoyl ether, and lipoprotein-deficient serum (d > 1.21 g/ml) as a source of cholesteryl ester (CE) transfer protein for 6 h at 37 °C, and the HDL was then separated from donor particles by ultracentrifugation at 1.06 g/ml. HDL3 was labeled with [14C]CE by incubating a d > 1.12 g/ml (dialyzed) fraction of human plasma (lecithin:cholesterol acyltransferase source) with [14C]cholesterol (Amersham). The CE-labeled HDL was isolated by ultracentrifugation at d 1.21 g/ml and dialyzed.

Protein Sequencing

HB2, a glycoprotein of Mr 100,000 was purified from rat liver plasma membrane as described previously (12). Attempts at NH2-terminal sequencing were unsuccessful. Internal sequences were obtained following cleavage with an endoproteinase (Lys C) using an enzyme substrate ratio of 1:10 (w/w). Peptides were separated by high performance liquid chromatography using an RP300 column (30-min gradient of acetonitrile from 0-60%) in 0.1% trifluoroacetic acid as mobile phase. This approach produced low yields and limited sequence information. Better yields were obtained following digestion of HB2 with cyanogen bromide (CNBr) for 16 h at room temperature. The CNBr fragments were separated by SDS-PAGE (12% acrylamide) and transferred to Problott membranes (Applied Biosystems), and the peptides were detected by staining with Coomassie Blue. Bands on Problott membranes were excised, cut into pieces, and applied directly to the cartridge of an Applied Biosystems Model 470A sequencer equipped with an on-line Model 120A PTH analyzer. Sequences, ranging from 11 to 20 amino acid residues, were obtained from several peptides.

cDNA Cloning and Sequence Analysis

Total RNA was prepared from both liver and lung of male Sprague-Dawley rats by homogenizing with guanidium isothiocyanate and centrifugation through a cushion of CsCl (14). Total RNA was used for cDNA synthesis using Moloney murine leukemia virus reverse transcriptase and random hexamers and oligo(dT)16 as primers. PCR was performed with oligonucleotides 9511 (forward) and 9519 (reverse) (based on the amino acid sequence of internal peptides of HB2) as follows: primer 9511, 5'-CA(A/G)TAFGAFGA(T/C)GT(F/G)CC(F/G)GA(A/G)TA; 9519, 5'-T(A/G)AAFTCFTC(F/G)GG(F/G)GGNGG(A/G)TT (F = T/C, N = any). As indicated, 5'-fluoro-dUMP (F) was incorporated into the oligonucleotides during synthesis (Bresatec, Australia) to limit degeneracy (15). Conditions for PCR were 95 °C, 2 min for one cycle, then 30 cycles of 95 °C, 1 min, an annealing step commencing at 53 °C for 30 s, then increasing to 72 °C at a ramp rate of 0.1 °C/s; 72 °C, 2 min ending with 5-min elongation at 72 °C. The amplified product was subcloned into vector, pCRTMII, using a TA cloning kit (Invitrogen). Double-stranded sequencing of the fragment was performed using M13 forward and reverse primers and Sequenase Version 2 (U. S. Biochemical Corp.).

Synthesis of Rat Lung cDNA Library

Poly(A)+ RNA from rat lung was isolated from total RNA by Oligotex [d(T)]30 (Roche). Synthesis of cDNA from 5 µg of poly(A)+ RNA was catalyzed by Moloney murine leukemia virus reverse transcriptase with a Timesaver cDNA synthesis kit (Pharmacia) which includes EcoRI/NotI adapters. The cDNA was ligated into the EcoRI site of Lambda ZAP II vector (Stratagene) and packaged into phage particles with Gigapack III Gold packaging extract (Stratagene). The recombinant phage was used to infect Escherichia coli strain XL1-Blue MRF.

Approximately 2.5 × 105 plaque-forming units were screened for HB2 clones after lifting onto Colony/Plaque ScreenTM membrane (DuPont). The PCR product from primers 9511/9519 was labeled with [alpha -32P]dCTP by random priming. Hybridization was performed at 42 °C in 5 × SSPE, 5 × Denhardt's solution, 1% SDS, 50% formamide, and 100 µg/ml denatured salmon sperm DNA. Filters were washed three times with 2 × SSC and 0.1% SDS solution at 50 °C for 15 min, then washed with 0.1 × SSC and 0.1% SDS solution at 50 °C for 30 min. Thirty-three positive plaques remained after tertiary screening from which 15 clones were selected, excised in vivo, and used for further sequencing analysis.

Expression in COS, HepG2, and CHO Cells

The HB2 cDNA (1- 2,771 nucleotides) was introduced into the EcoRI site of the expression vector, pcDNA I/Amp (Invitrogen) for transient expression. Transfection was performed by the DEAE-dextran method for COS and CHO cells and by calcium phosphate precipitation for HepG2 cells (16). The same procedure was followed, except for the omission of the plasmid, to produce mock-transfected cells. After 24 h, the cells were removed from the flasks and dispensed into 12-well plates at appropriate seeding densities in preparation for binding experiments which were performed at 48 h after transfection. In some experiments, cells were washed and harvested, and membranes were recovered for ligand blotting analysis (see below).

Binding Experiments

COS or HepG2 cells in monolayers were maintained in DMEM containing 10% fetal bovine serum. Prior to binding experiments, cells were washed with serum-free DMEM, and the growth medium was replaced with DMEM containing 0.2% (w/v) bovine serum albumin and 25 mM HEPES, pH 7.4. Transfected and mock-transfected cells were incubated with 125I-labeled HDL3 (as described under "Results") with or without unlabeled HDL3. Specific binding was determined as described previously (17).

Western and Northern Blots

Cell membranes were prepared as described previously (8). Immunoblotting was performed after transfer of membrane proteins (following SDS-PAGE) to nitrocellulose which was incubated with antiserum against HB2 and then horseradish peroxidase-conjugated second antibody (8).

For Northern blot analysis of rat tissues, total RNA was isolated from tissues including liver, intestine, lung, spleen, kidney, brain, ovary, and thymus, fractionated by formaldehyde-agarose gel electrophoresis, and transferred to nylon membranes. These were probed with 32P-labeled probes (see "Results"), and hybridizing bands were identified by autoradiography or bioimaging. Membranes were stripped and rehybridized with a cDNA probe for rat glyceraldehyde phosphate dehydrogenase. For detection of HB2 mRNA in human tissues, human multiple RNA blots (CLONTECH) were similarly probed as described above, except that the actin probe provided with the blots was used as an internal standard.

Ligand Blots

Cells were lysed in the presence of 20 mM CHAPS, and solubilized proteins were recovered by centrifugation at 18,000 × g for 10 min. Glycoproteins were isolated with wheat germ lectin agarose (Pharmacia) and then applied to SDS-PAGE gels. Ligand blotting was performed as described previously (12).

Computer Analysis

Data base searches with the nucleotide sequence of rat HB2 cDNA were performed with GenBank and EMBL data bases by the FASTA program from the Genetics Computer Group sequence analysis software. Alignments and consensus sequence derivation of peptide sequences were analyzed by GENETYX (version 9.0) from Software Development Co., Ltd. (Tokyo, Japan). Further analyses of the HB2 gene product for common motifs and potential secondary structure were performed using GENETYX.


RESULTS

HB2 antiserum was used to probe membranes from various rat organs as described under "Materials and Methods." As shown previously (18), the strongest expression of HB2 was present in liver, lung, and intestine. Total RNA from lung and liver were therefore subjected to reverse transcription-PCR as described under "Materials and Methods," with primers 9511 and 9519.

Under the annealing/elongation conditions described for PCR, a single product of 600 base pairs was amplified from lung, but not from liver. Sequencing of this fragment confirmed the presence of both primers as well as an additional internal peptide of HB2, in the correct reading frame. To obtain a full-length clone, a lung cDNA library was prepared and probed with the 600-base pair fragment. Of 2.5 × 105 plaque-forming units probed, 33 positive clones remained after three rounds of screening. Fifteen of these were further analyzed. As shown in Fig. 1, the cDNA of HB2 encoded a protein of 65 kDa constituted from 583 amino acids, considerably smaller than the apparent size of 100 kDa of the glycosylated form of HB2 identified by ligand blotting as previously reported by our laboratory (12). Over the entire coding region, rat HB2 showed highest homology with human ALCAM (93%) (19) and the avian protein BEN (70%) (20), which are adhesion proteins of the immunoglobulin superfamily. Alignment with ALCAM and BEN is also shown in Fig. 1. There was no significant homology with any other lipoprotein receptor including candidate HDL receptors previously reported (11, 21).



Fig. 1. Amino acid sequence deduced from nucleotide sequence of HB2 and alignment with homologous members of the immunoglobulin superfamily, ALCAM and BEN. Amino acid sequences obtained from peptide sequencing analysis of rat HB2 protein are underlined.
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Binding to HDL3

To demonstrate that this transmembrane protein functions as an HDL-binding protein, COS, CHO, or HepG2 cells were transfected or mock-transfected as described under "Materials and Methods." As shown in Fig. 2, A and B, specific binding of 125I-labeled HDL3 was increased (at saturation) approximately 2-fold in transfected HepG2 cells and by 1.8-fold in transfected COS cells compared with mock-transfected cells. This increased binding however was not associated with transfer of cholesteryl esters from HDL to cells because no differences were observed in cholesteryl ester uptake between mock and transfected COS or HepG2 cells (data not shown).


Fig. 2. Activation of HDL binding in cells transfected with HB2. A and B, specific binding (total minus nonspecific) of 125I-labeled HDL3 to transfected (bullet ) or mock-transfected (black-square) HepG2 (A) or COS (B) cells. Cells were transfected, and after a 48-h incubation in DMEM containing 10% fetal calf serum, the cells were washed three times with serum-free DMEM, and duplicate wells were incubated with the indicated concentration of 125I-HDL3 for 3 h at 37 °C in DMEM. Parallel wells were incubated with 20 × excess unlabeled HDL3 to determine nonspecific binding. C and D, ligand blotting of glycoproteins isolated from HepG2 (C) or CHO (D) cells. Cultures of mock- transfected or transfected cells were harvested and homogenized in the presence of 20 mM CHAPS. The solubilized glycoprotein was applied to lanes, in duplicate, of SDS-PAGE gels and transblotted, and the nitrocellulose strips were incubated with HDL3 as described previously. Lanes 1 and 2, mock-transfected cells; 3 and 4, transfected cells; 5, positive control of partially purified HB2.
[View Larger Version of this Image (17K GIF file)]

Glycoproteins isolated from mock- or transiently transfected CHO or HepG2 cells were compared for their HDL binding capacity by ligand blots. As shown in Fig. 2C, untransfected HepG2 cells showed binding of HDL3 to both HB2 and HB1, but the signal for HB2 was much stronger in transfected cells. Similarly the faint signal for HB2 observed in mock-transfected CHO cells was markedly increased when membrane proteins from transfected CHO cells were incubated with HDL3 (Fig. 2D).

Expression of HB2 mRNA in Rat and Human Tissues

Fig. 3A shows Northern blot analyses of HB2 mRNA expression in various rat tissues. Strongest expression was found in the lung, then brain, liver, and kidney. In comparison, to the rat, human mRNA to HB2 (probed with rat HB2 cDNA) was strongest in the brain, prostate, pancreas, small intestine, and liver of human (Fig. 3B), but lower in the lung.


Fig. 3. A, tissue distribution of rat HB2 mRNA. Northern blot analysis of RNA isolated from the tissues indicated were probed with 32P-labeled rat HB2 cDNA. 1, liver; 2, lung; 3, spleen; 4, kidney; 5, heart; 6, muscle; 7, brain. B, tissue distribution of human homologue of HB2 mRNA. RNA blots of the tissues indicated were probed with 32P-labeled HB2 rat cDNA. 1, thymus; 2, spleen; 3, prostate; 4, testis; 5, ovary; 6, small intestine; 7, colon; 8, peripheral blood; 9, heart; 10, brain; 11, placenta; 12, lung; 13, liver; 14, skeletal muscle; 15, kidney; 16, pancreas.
[View Larger Version of this Image (101K GIF file)]

To determine whether blood monocytes or macrophages express HB2, RNA from THP-1 cells or from cells differentiated by treatment with PMA was subjected to Northern blot analysis. As shown in Fig. 4A, HB2 mRNA, hardly detectable in untreated THP-1 cells, was strongly induced when the cells were transformed into macrophages by PMA treatment. After incubating THP-1 cells with 50 or 100 µg/ml acetylated LDL, a dose-dependent reduction in HB2 mRNA expression was observed. No changes were observed in expression of glyceraldehyde phosphate dehydrogenase mRNA with any of the treatments (Fig. 4B). Ligand blots of membrane proteins revealed weak HDL3 binding for THP1 cells, but after differentiation with PMA, strong binding was detected for HB2 (Fig. 4C) as well as an increase in binding to HB1. Binding was also stronger to another protein (approximately 66 kDa) which may represent degraded HB2 or another isoform of HB2.


Fig. 4. Expression of HB2 in monocytes and macrophages. Northern blots: RNA was prepared from THP-1 cells before and after treatment with 200 nM PMA for 72 h. Cells were then incubated in RPMI 1640 with 10% lipoprotein-deficient fetal calf serum for 8 h when acetylated LDL at 0, 50, or 100 µg/ml was added, and the cells incubated for an additional 24 h. RNA blots were probed with 32P-labeled HB2 (A) and glyceraldehyde-3-phosphate dehydrogenase (B) cDNA. Lanes 1 and 2, -PMA; 3 and 4, +PMA, -AcLDL. 5 and 6, +PMA, +50 µg/ml AcLDL; 7 and 8, +PMA, +100 µg/ml AcLDL. C, ligand blot of THP-1 cells or differentiated THP-1 cells. Cells treated or untreated with PMA as described above were harvested, washed, and extracted, and ligand blotting was performed as described in Fig. 2. The lower molecular mass band (approximately 66 kDa), which binds HDL, may represent a degraded or partly processed form of HB2 since it cross-reacts with anti HB2 on immunoblots (results not shown). Lanes 1 and 2, -PMA; 3 and 4, +PMA; 5, positive control as for Fig. 2, C and D.
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DISCUSSION

Cloning and sequencing of HB2, one of a pair of HDL-binding proteins previously identified and purified in this laboratory (12), have revealed its identity with a subclass of the immunoglobulin superfamily of proteins with adhesion type properties. To confirm that HB2 performed a role as an HDL-binding protein, HepG2, CHO, and COS cells were transiently transfected with HB2 cDNA. Compared with control (mock-transfected) cells, HepG2 and COS cells (transfected) demonstrated an 80-100% increase in HDL binding, establishing that HB2, together with other candidate HDL receptors (11, 21), may play an important role in HDL metabolism in the body. The level of HDL binding activity resulting from transfection with HB2 cDNA was intermediate between that of an HDL-binding protein found in endothelial cells when expressed in COS cells (21) and that of SR-B1 (11), another candidate HDL receptor. It is not surprising that untransfected cells will demonstrate variable levels of specific HDL binding in view of the presence on most cells of "specific" but low affinity HDL binding sites recently identified in this laboratory (22). This phenomenon is a characteristic of the interaction between HDL and cells and the most likely explanation for the relatively high level of specific binding observed in the mock-transfected cells in this study.

Additional evidence that HB2 is involved in the cellular recognition of HDL came from ligand blotting studies which confirmed that this membrane protein, when overexpressed in HepG2, CHO, and THP-1 cells, bound HDL3. Untransfected cells, apparently expressing low levels of HB2 compared with HB1 (Fig. 2C) showed a marked increase in HB2 that was active in binding HDL3, when transfected with HB2 cDNA. Similarly, ligand blotting revealed a significant increase in HDL binding to HB2 present in transiently transfected CHO cells, compared with controls. The up-regulation of HB2 mRNA that followed transformation of THP-1 cells into "macrophages" following PMA treatment was also associated with an increase in expression of HB2 which was active in binding HDL3 as seen in Fig. 4C.

These experiments have not yet provided definitive information about the clinical relevance of HB2, but they do support a functional role for HB2 that involves interaction with HDL. Expression of HB2 mRNA, barely detectable in blood monocytes, is up-regulated when THP-1 cells undergo differentiation to macrophages on treatment with PMA, and further, a reduction in expression of HB2 mRNA follows cholesterol loading with acetylated LDL. This suggests some association, either direct or indirect, between HB2 and cholesterol metabolism. If, as expected, sterol synthesis was decreased in the cholesterol-loaded cells, it would be consistent with a finding reported by this laboratory previously (23) that the administration of simvastatin to rats down-regulated HB2 (and HB1) expression by 50%. More studies are planned to investigate these relationships between HDL binding, HB2 levels, and cell cholesterol metabolism. Our present studies however have demonstrated that expression of HB2 is not associated with selective uptake of HDL cholesteryl ester by cells, a function which has been demonstrated for another candidate HDL receptor, SR-B1 (11).

Another function attributed to the family of membrane proteins that includes HB2, BEN, and ALCAM is adhesion. When expression of HB2 is up-regulated in cells (such as blood monocytes as described above) it is conceivable that the increased adhesion that follows may produce vascular remodelling and the initiation of atherogenesis. While many proteins which elicit injurious effects on the vessel wall are known to be produced by stimulated macrophages, increased levels of HDL or of apoAI-rich particles, may compete with binding sites on the HB2 adhesion molecules to significantly reduce the migration of macrophages into the arterial wall thereby achieving some protection against damage to the vessel. This model is entirely consistent with the protective role of HDL against premature atherosclerosis. The scavenger receptor cysteine-rich domain of CD6 is also recognized by this family of adhesion molecules (24), and interruption of this interaction by HDL may contribute to a decreased cell-cell association that is injurious to the vessel wall. Together with the observation that HDL apparently down-regulates the expression of soluble adhesion molecules (7), the combined inhibitory effect of HDL on cell adhesion may provide a formidable protective action against vascular disease. Clearly, these and other systems need to be explored, because the protective role of HDL is apparently not only limited to metabolic processes connected with lipid metabolism, such as reverse cholesterol transport, but may include mitogenic effects, secretagogue activity, and possible cellular signaling pathways (6). In fact, the tissue distribution of HB2 mRNA is consistent with any of the functions suggested above. In the human, organs that play important roles in lipoprotein transport such as the liver and intestine and steroidogenic tissue express HB2, but others such as the lung, brain, placenta, and pancreas, which may participate in the alternative protective functions listed above, also contain varying proportions of HB2 mRNA.

The structural features of HB2 are also consistent with a "receptor" role for this membrane protein. As shown in the working model (Fig. 5) based on available structural information on this group of membrane proteins of the IgG superfamily, HB2 is characterized by a 32-amino acid cytoplasmic domain, a 24-amino acid hydrophobic transmembrane domain, and approximately 500 residues of an extracellular domain terminating in the NH2 residue. Data base searches of consensus sequences for N-glycosylation sites revealed eight potential sites, all extracellular, at residues 95, 167, 265, 306, 361, 457, 480, and 499. It is likely that most sites are glycosylated since the protein is mainly expressed in the higher Mr form, although in HepG2 cells the presence of a faster migrating HB2 isoform was found by Western blotting.2 The function of glycosylation in HDL binding is unclear, although previous ligand blot studies (12) indicate that glycosylation is not essential for HDL binding. The carbohydrate however may contribute to other essential functions such as intracellular transport and influence the capacity of HB2 (in some tissues) to reach sites for HDL binding. Some provisional protein kinase C phosphorylation sites (residues 8, 73, 74, 209, and 421) were found, but since all are extracellular, their potential function as determinants of signaling via protein kinase C is weakened. cAMP- and cGMP-dependent protein kinase phosphorylation sites were also found. Possibly, sites which are inactive when HB2 is membrane-bound are activated if the protein is internalized. Further experiments are planned to investigate the interrelationships between structure and function, as related to HDL binding, and cellular localization of HB2.


Fig. 5. Schematic model of HB2. The protein traverses the membrane once, via 24 hydrophobic amino acid residues, and 32 residues of the COOH terminus are situated intracellularly. Approximately 500 extracellular amino acids, including the NH2 terminus, may provide a domain recognized by HDL or by apoAI. At least eight potential N-glycosylation sites are identified as shown starting from the NH2 terminus at positions 95, 167, 265, 306, 361, 457, 480, and 499.
[View Larger Version of this Image (15K GIF file)]


FOOTNOTES

*   This work was supported in part by grants from the National Heart Foundation (Australia) and the Human Health Sciences Foundation and by a grant for research on aging and health from the Ministry of Health and Welfare, Japan.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
   To whom correspondence should be addressed. Tel.: 61-3-9522-4333; Fax: 61-3-9521-1362.
1   The abbreviations used are: HDL, high density lipoprotein; LDL, low density lipoprotein; HB, high density lipoprotein-binding protein; apo, apolipoprotein; PAGE, polyacrylamide gel electrophoresis; PMA, phorbol 12-myristate 13-acetate; CHO, Chinese hamster ovary; DMEM, Dulbecco's modified Eagle's medium; CE, cholesteryl ester; PCR, polymerase chain reaction; CHAPS, 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonic acid.
2   A. Matsumoto, A. Mitchell, H. Kurata, L. Pyle, K. Kondo, H. Itakura, and N. Fidge, unpublished data.

ACKNOWLEDGEMENTS

We are grateful to Anne Au and Ann Seward for expert technical assistance.


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