Bovine apolipoprotein (apo)A-I displays more enhanced antioxidant and anti-atherosclerotic activity in lipid-free and lipid-bound states than human and porcine apoA-I

  • Authors:
    • Seong-Min Kim
    • Ga-Young Park
    • Inho Choi
    • Kyung-Hyun Cho
  • View Affiliations

  • Published online on: August 22, 2013     https://doi.org/10.3892/ijmm.2013.1473
  • Pages: 843-850
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Abstract

Apolipoprotein A-I (apoA-I) is a major component of high-density lipoprotein (HDL), which displays anti-atherosclerotic activity in plasma. In the current study, we compared the functional and structural characteristics of human, bovine and porcine apoA-I as regards their antioxidant ability and protein stability. In the lipid-free state, the immunoreactivity of bovine and porcine apoA-I differed from that of human apoA-I and bovine and porcine apoA-I exhibited greater resistance to denaturation induced by urea treatment. Bovine apoA-I showed the weakest binding ability of dimyristoyl phosphatidylcholine; however, bovine apoA-I formed slightly larger reconstituted HDL (rHDL) particles with palmitoyl oleoyl phosphatidylcholine, with a higher number of apoA-I-containing particles. Bovine and porcine apoA-I comprised of pentameric structures, whereas human apoA-I in the rHDL state consisted of trimeric structures. Although apoA-I from all three species showed a similar content of α-helicity in the lipid-free state (approximately 53%), bovine apoA-I showed a lower α-helicity content (approximately 66%) compared with human apoA-I (approximately 74%) in the rHDL state. Bovine apoA-I was more resistant to denaturation and glycation upon treatment with urea and fructose, respectively. Furthermore, bovine apoA-I showed a greater inhibition of cupric ion-mediated low-density lipoprotein (LDL) oxidation and uptake of acetylated LDL by macrophages compared with human or porcine apoA-I in the lipid-free and lipid-bound states. In conclusion, bovine apoA-I has unique functional properties in the lipid-free and lipid-bound states, and displays significantly enhanced anti-atherosclerotic activity.

Introduction

Human apolipoprotein A-I (apoA-I), the major component of high-density lipoprotein (HDL), is a protein of 243 amino acids with repeated 22-residue homologous segments separated by prolines (1). HDL plays a critical role in reverse cholesterol transport (RCT), which is involved in the removal of excess cholesterol from peripheral cells and its delivery to the liver and steroidogenic cells for catabolism (2). In vertebrates, normal HDL exerts potent antioxidant and anti-inflammatory effects (3) and has anti-infective properties in plasma (4). It is well established that there are strong correlations between apoA-I structure and function, and the beneficial effects of HDL are highly dependent on its apoA-I content and conformation. Lipid-free apoA-I, as well as apoA-I in reconstituted HDL (rHDL) particles, may stimulate insulin secretion from pancreatic β-cells (5). These data raise the possibility that lipid-free apoA-I may play a unique role in the mammalian health system.

As a tool for gene delivery, we previously reported that the efficiency of viral delivery and adenovirus stability can be significantly enhanced by applying proteoliposomes (PLs) containing apoA-I to human cells and zebrafish models (6). Recently, a PL containing apoA-I and its mutant (V156K) was shown to enhance the rapid tumor regression activity of human origin oncolytic adenovirus in tumor-bearing zebrafish and nude mice (7). These studies raise the possibility that apoA-I may be applied to the generation of vehicles for the delivery of pharmaceuticals, genes and vaccines.

Over the past three decades, the characterization of apoA-I and its mutants from a variety of sources in both the lipid-free and lipid-bound states has been extensively attempted with purified apoA-I from human plasma, animal plasma, and/or various recombinant apoA-I produced in an E. coli-based expression system (1,8). As a result, many functional-structural domains have been elucidated, as described in the study by Bashtovyy et al (9). Phylogenetic comparisons of apoA-I sequences have been described in the study by Brouillette et al (10), as they observed that the deletion of a single residue in exon 4 of the pig and cow did not drastically alter the straight alignment of the hydrophobic face, whereas the rat and mouse displayed several amino acid deletions in exon 4 that altered the straight hydrophobic face.

However, there has been no direct comparison of the functional and structural properties of human apoA-I with those of major vertebrates in domestic animals, such as pigs or cattle. In the present study, we compared the functional characteristics of human, bovine and porcine apoA-I in plasma in the lipid-free and lipid-bound states, as regards their antioxidant and anti-atherosclerotic activities.

Materials and methods

Materials

Dimyristoyl phosphatidylcholine (DMPC, #850345) and palmitoyl oleoyl phosphatidylcholine (POPC, #850457) were obtained from Avanti Polar Lipids, Inc. (Alabaster, AL, USA). Bis(sulfosuccinimidyl) suberate (BS3, #S5799) and sodium cholate (#C1254) were purchased from Sigma (St. Louis, MO, USA). α-linolenic acid (all-cis-9,12,15-octadecatrienoic acid, 18:3, #L2376) was purchased from Sigma. Bovine and porcine plasma was obtained from the Bovine Genome Resources Bank of Korea at Yeungnam University (Gyeongsan, Korea) and a local slaughter house (Gyeongsan, Korea), respectively, with the addition of EDTA (final concentration, 1 mM) as an anti-coagulant.

Purification of HDL and apoA-I

HDL and apoA-I were purified from human, bovine and porcine plasma using ultracentrifugation and column chromatography, according to a previously described method (11). The NH2-terminal amino-acid sequence of apoA-I was determined using an Applied Biosystems Procise 491 HT protein sequencer (Applied Biosystems, Foster City, CA, USA) located in the Seoul Branch of the Korea Basic Research Institute (Seoul, Korea).

DMPC clearance assay

The interactions of apoA-I from each species with DMPC (3.5 mg/ml) were monitored by the method described in the study by Pownall et al (12) with slight modifications. The mass ratio of DMPC to protein was 2:1 (w/w) in a total reaction volume of 0.76 ml.

Purification and oxidation of low-density lipoprotein (LDL)

LDL (density, >1.019 to <1.063) was purified from healthy human plasma (Blood Bank of Yeungnam University Medical Center, Daegu, Korea) by ultracentrifugation (100,000 × g) for 22 h at 4°C. Oxidized LDL (oxLDL) was produced by incubating the LDL fraction with copper sulphate (CuSO4) (final concentration, 10 μM) for 4 h at 37°C. The oxLDL was then filtered (0.2 μm filter) and analyzed by thiobarbituric acid reactive substances (TBARS) assay to determine the extent of oxidation, as previously described (13).

Synthesis of reconstituted HDL

Discoidal rHDL was prepared using the sodium cholate dialysis method (14,15) with an initial molar ratio of POPC:cholesterol:apoA-I:sodium cholate of 95:5:1:150. The size and hydrodynamic diameter of rHDL particles were determined by 8–25% native polyacrylamide gradient gel electrophoresis (PAGGE; Pharmacia PhastSystem) by comparison with standard globular proteins (GE Healthcare, Uppsala, Sweden).

BS3-cross-linking

The number of apoA-I molecules per rHDL particle, as well as the self-association properties of lipid-free proteins, were determined by cross-linking with BS3 as previously described (16), followed by the analysis of reaction products by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) on pre-cast 8–25% gradient gels (GE Healthcare).

Circular dichroism (CD)

The average α-helix contents of proteins in the lipid-free and lipid-bound states were measured by CD spectroscopy using a J-715 Spectropolarimeter (Jasco, Tokyo, Japan). Spectra were obtained from 250–190 nm at 25°C in a 0.1-cm path-length quartz cuvette at a bandwidth of 1.0 nm, a speed of 50 nm/min, and a 4-sec response time. The protein samples were diluted to 0.07 mg/ml so that lipid-free proteins could avoid apolipoprotein self-association, whereas lipid-bound proteins were diluted to 0.1 mg/ml. Four scans were accumulated and averaged. The α-helix content was calculated from the molar ellipticity at 222 nm as previously described (17).

Characterization of tryptophan (Trp) fluorescence and isothermal denaturation

The wavelength of maximum fluorescence (WMF) of Trp residues in apoA-I protein was determined from uncorrected spectra obtained using an LS55 spectrofluorometer (Perkin-Elmer, Norwalk, CT, USA) in conjunction with the WinLab software package 4.00 (Perkin-Elmer) and a 1-cm path-length Suprasil quartz cuvette (Fisher Scientific, Pittsburgh, PA, USA). Briefly, the samples were excited at 295 nm to avoid tyrosine fluorescence, and the emission spectra were then scanned from 305–400 nm at room temperature. The effects of the addition of urea on the secondary structure of apoA-I in the lipid-bound state were monitored by observing the WMF as described in our previous study (15).

Glycation of apoA-I in lipid-free and lipid-bound state

In order to compare protein glycation, apoA-I from each species in the lipid-free or lipid-bound state was incubated with D-fructose (final concentration, 250 mM) as described our previous study (18). apoA-I was incubated for upto 72 h under air gas containing 5% CO2 at 37°C. The extent of advanced glycation reactions was determined from reading the fluorometric intensity at 370 nm (excitation) and 440 nm (emission), as described previously (18).

Western blot analysis

To compare the cross-reactivity of each apoA-I protein with antibodies specific to the human variant, equal amounts (2.5 μg of protein) of apoA-I were loaded and electrophoresed on 15% SDS-PAGE gels and detected by anti-human full-length apoA-I goat antibody (ab7613; Abcam, Cambridge, UK) and donkey anti-goat immunoglobulin G-horseradish peroxidase (HRP) (SC2020; Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA) as the secondary antibody (diluted 1:2,000). The apoA-I protein concentration in the rHDL and lipid-free states was determined using the Lowry assay as modified by Markwell et al (19) with bovine serum albumin as the standard.

Inhibition of LDL oxidation

In order to determine the extent of oxidation, purified human LDL was incubated with 10 μM CuSO4 for up to 3 h in the presence of apoA-I in the lipid-free or rHDL state (final 2 μM of protein). During incubation, the quantity of conjugated dienes formed was monitored by following the absorbance at 234 nm (A234) at 37°C (20) using a Beckman DU 800 spectrophotometer (Beckman Coulter, Inc., Fullerton, CA, USA) equipped with a MultiTemp III Thermocirculator (Amersham Biosciences, Uppsala, Sweden).

To verify the spectroscopic data, oxidized samples were subjected to electrophoresis on 0.5% agarose gels in order to compare their electromobilities as previously described (21); migration of each lipoprotein is known to depend on its intact charge and size. The gels were then dried and the bands were stained with 0.125% Coomassie Brilliant Blue.

Acetylation of LDL

The acetylation of LDL (acLDL) was performed using saturated sodium acetate and acetic anhydride according to a previously described method (22). Following acetylation and subsequent dialysis, the acLDL protein content was determined and filtered through a 0.22 μm filter (Millex; Millipore, Bedford, MA, USA). To visualize the phagocytosis of acLDL, a fluorescent cholesterol derivative [22-(N-7-nitrobenz-2-oxa-1,3-diazol-4-yl)amino-23,24-bisnor-5-cholen-3-ol (NBD-cholesterol), Molecular Probes N-1148; 70 μg of NBD-cholesterol/mg of apoA-I] was added to the acLDL particles.

LDL phagocytosis assay

THP-1 cells, a human monocytic cell line, were obtained from the American Type Culture Collection (ATCC; #TIB-202™; Manassas, VA, USA) and maintained in RPMI-1640 medium (HyClone, Logan, UT, USA) supplemented with 10% fetal bovine serum (FBS) until needed for experimentation. Cells that had undergone no more than 20 passages were incubated in medium containing phorbol 12-myristate 13-acetate (PMA; final concentration, 150 nM) in 24-well plates for 24 h at 37°C in a humidified incubator (5% CO2, 95% air) to induce differentiation into macrophages. The differentiated and adherent macrophages were then rinsed with warm PBS and incubated with 400 μl of fresh RPMI-1640 medium containing 1% FBS, 50 μl of (acLDL; 1 mg of protein/ml in PBS), and 50 μl of PBS or each protein (final 2 μM) for 48 h at 37°C in a humidified incubator. Following incubation, the cells were washed with PBS three times and then fixed in 4% paraformaldehyde for 10 min. The fixed cells were then stained with oil Red O staining solution (0.67%) and then washed with distilled water. THP-1 macrophage-derived foam cells were then observed and photographed using a Nikon Eclipse TE2000 microscope (Nikon, Tokyo, Japan) at ×600 magnification.

Statistical analysis

All data are expressed as the means ± SD of at least three independent experiments with duplicate samples. Comparisons between the results were made using the Student’s t-test with SPSS software (version 12.0; SPSS, Inc., Chicago, IL, USA). A P-value <0.05 was considered to indicate a statistically significant difference.

Results

Identification of apoA-I and sequence comparisons

Although apoA-I from all species (>95% purity) exhibited 28–29 kDa molecular weight in the lipid-free state from SDS-PAGE (Fig. 1A), bovine apoA-I showed the highest position with the slowest mobility in the native gel electrophoresis (Fig. 1B).

N-terminal amino acid sequencing confirmed the identities of bovine (lane B) and porcine (lane P) apoA-I. In each protein, 16 amino acids were identical to the GenBank sequences for bovine (ID AAI02942.1) and porcine (ID CAA49234.1) apoA-I. Bovine and porcine apoA-I differed from the human protein in their 2nd amino acid (Asp), which corresponds to Glu; the 4th Pro in the human sequence was deleted from the bovine and porcine proteins. Furthermore, Pro7 in human apoA-I was replaced by Ser in bovine apoA-I; the 14th residue, leucine, in human apoA-I was replaced by Phe in the bovine and porcine variants (data not shown).

Immunodetection of bovine and porcine apoA-I

The human specific antibody for apoA-I could not detect bovine or porcine protein (2.5 μg/lane), suggesting that the antigenic epitope was dissimilar between the species (Fig. 1C). The comparison of the amino acid sequences revealed the deletion of the 4th amino acid in the human protein, Pro, in the bovine and porcine apoA-I sequences; the loss of this residue may have disrupted the epitope. Pro4 and Ala187 in the human protein sequence were deleted in bovine apoA-I; Pro4, Glu120 and Asn184 were deleted in porcine apoA-I.

Characterization of rHDL

Electrophoretic analysis of POPC-rHDL-associated apoA-I demonstrated that the major particle size ranged from 98–105 Å (Fig. 2A). The bovine apoA-I-containing particles were the largest, at approximately 105 Å in diameter. BS3-cross-linking revealed that bovine and porcine apoA-I rHDL contained up to five apoA-I units per particle, whereas human apoA-I rHDL contained three apoA-I units/particle (Fig. 2B).

DMPC clearance

In order to compare the phospholipid and polyunsaturated fatty acid binding capacity of the apoA-I, we monitored the clearance speed of the lipid emulsion. Bovine and porcine apoA-I displayed a much weaker phospholipid-binding ability compared with human apoA-I; values for the repair half-time (T1/2) values were calculated at around 81 and 66 min, respectively, from the regression curve (Fig. 2C). The phospholipid-binding ability of human apoA-I was much more pronounced as the approximate T1/2 value was around 17 min.

Spectroscopic analyses of secondary structure

In the lipid-free state, human and bovine apoA-I showed a WMF of 347 and 348 nm, respectively, whereas porcine apoA-I showed a WMF of 345 nm. Bovine and porcine proteins contained Trp residues at the 7th, 49th, 71st and 107th positions. In the rHDL state, the WMF apoA-I from all species demonstrated a blue shift of 3–4 nm (Table I). Secondary structure determination revealed α-helicity in human apoA-I of 53 and 74% in the lipid-free and rHDL states, respectively, which was a 21% increase. However, bovine apoA-I showed 53 and 66% α-helicity in the lipid-free and rHDL states, respectively, indicating the lowest increase in α-helicity (approximately 13%). Porcine apoA-I exhibited 55 and 70% α-helicity in the lipid-free and rHDL states, respectively, which was a 15% increase in α-helicity.

Table I

Compositional and spectroscopic analyses of apoA-I from bovine, porcine and human plasma in the lipid-bound state (rHDL)a.

Table I

Compositional and spectroscopic analyses of apoA-I from bovine, porcine and human plasma in the lipid-bound state (rHDL)a.

BovinePorcineHuman
WMFb (nm) at urea 0 M341±3 (348±1)c341±2 (346±2)344±2 (348±2)
WMF (nm) at urea 7 M354±2 (355±1)357±2 (359±2)355±1 (357±2)
α-helicityd (%)66±3 (53±4)70±4 (55±3)74±2 (53±3)
Sizee (Å)10510198, 80
No. of apoA-If/rHDL2–52–52, 3
pIg (calculated)5.325.115.24

a rHDL was synthesized with palmitoyl oleoyl phosphatidylcholine (POPC):cholesterol:apoA-I:sodium cholate at a molecular ratio of 95:5:1:150, respectively.

b Determined from fluorospectroscopy (excitation, 295 nm; emission, 305–400 nm).

c Numbers in parentheses indicate proteins in the lipid-free state.

d Determined from circular dichroic spectroscopy.

e Determined from 8–25% native-gradient gel electrophoresis with densitometric scanning analysis.

f Determined from BS3-cross-linking and 8–25% SDS-PAGGE.

g Isoelectric point (pI) was calculated using protean module of DNASTAR software (version 5.07).

Denaturation under urea treatment

In the lipid-free state, porcine and bovine apoA-I were resistant to denaturation at a urea concentration <2 M (Fig. 3A). Exposure to 7 M urea stimulated the highest WMF of porcine apoA-I, whereas bovine and human apoA-I showed their highest WMF upon treatment with 5 M urea. These results suggest that porcine and bovine apoA-I show variable sensitivity upon complete Trp exposure in the aqueous phase due to protein denaturation. In the rHDL state, porcine and bovine apoA-I were resistant to denaturation at a urea concentration <5 M. Human apoA-I was the most susceptible to urea-induced denaturation (Fig. 3B).

Inhibition of LDL oxidation

In the lipid-free state, bovine apoA-I was the most resistant to cupric ion-mediated LDL oxidation during 40 min of incubation (Fig. 4A) (final concentration of each apoA-I, 2 μM); bovine apoA-I demonstrated an increase in A234 of 54%, whereas porcine and human apoA-I were inhibited to a lesser degree (increase in A234 of 84–89%). Agarose electrophoresis revealed that LDL treated with bovine apoA-I (final 2 μM) migrated the slowest. This result suggests that LDL treated with bovine apoA-I was more resistant to the oxidation, as more oxLDL migrates faster due to an increase in the negative charge and smaller particle size (Fig. 4B).

Inhibition of acLDL uptake by macrophages

We monitored the uptake of acLDL into THP-1 cells in the presence of each apoA-I (Fig. 5) relative to the PBS-treated control (Fig. 5A) based on the detection of a fluorescent cholesterol derivative. In the lipid-free state, bovine apoA-I demonstrated the greatest inhibition of acLDL phagocytosis. Specifically, in the presence of lipid-free bovine apoA-I, the fluorescence decreased by 56% compared with the acLDL control (Fig. 5).

Glycation sensitivity of apoA-I

By fructosylation, apoA-I is usually prone to an increase in the WMF by the glycation process via the modification of its tertiary structure, resulting in the exposure of Trp in the aqueous phase. In the lipid-free state, porcine and human apoA-I showed an increase in WMF of approximately 2 nm during 72 h of incubation (Fig. 6A). However, bovine apoA-I did not show any change in WMF in the lipid-free state (approximately 347 nm). Although apoA-I has four Trp in the protein sequence, the sensitivity to fructosylation differed between the species. In the rHDL state, bovine apoA-I and human apoA-I showed the lowest increase in WMF (approximately 1 nm) during 72 h of incubation (from 335 to 336 nm), while porcine apoA-I showed the highest increase (approximately 3 nm; from 337 to 340 nm) (Fig. 6B). These results suggest that bovine apoA-I is the most resistant to glycation; however, the mechanisms invovled remain to be elucidated.

Discussion

In the current study, we found several properties unique to bovine apoA-I compared with other mammalian apoA-I (human and porcine). Bovine apoA-I exhibited the weakest binding ability with DMPC (Fig. 2C) and the weakest sensitivity to denaturation by urea (Fig. 3). Bovine apoA-I was the most resistant to glycation with inhibition against LDL oxidation (Fig. 4) and foam cell formation via the phagocytosis of macrophages (Fig. 5).

apoA-I is a major component of HDL particles, which have strong antioxidant, anti-inflammatory and anti-infective properties (23). The overexpression of apoA-I in mice elicits resistance to diet-induced atherosclerosis (24). These studies raise the possibility of protein adaptation for the development of anti-atherosclerotic and anti-diabetic therapeutics. Serum HDL cholesterol and apoA-I levels are inversely associated with diabetic retinopathy, and serum apoA-I and apo-B are both strong biomarkers of this pathology. The infusion of rHDL with wild-type apoA-I or several mutant variants of apoA-I has been reported as an emerging therapy for acute regression (25,26). These results suggest that apoA-I has potent therapeutic activities for the treatment of chronic metabolic diseases, such as diabetes and atherosclerosis.

The apoA-I amino acid sequence is conserved in higher vertebrates, such as pigs and cattle. Bovine apoA-I (GenBank ID AAI02942.1) and porcine apoA-I (GenBank ID CAA49234.1) consist of 241 and 240 amino acids, respectively, in their mature sequences. Furthermore, they exhibit 78% (bovine) or 80% (porcine) sequence identity to the human protein (AAH05380.1). Due to these amino acid differences, it is possible that the location of antigenic amino acids varies according to species. Collet et al (27) reported that several monoclonal antibodies (mAbs) against human apoA-I are unable to detect porcine or bovine protein, suggesting that apoA-I immunoreactivity may differ among species. They also tested 20 different mAbs against apoA-I proteins from humans, pigs and cattle. Between humans and pigs, only five mAbs displayed 50–100% immunoreactivity. On the other hand, between cattle and humans, only one mAb displayed 50–100% immunoreactivity with two coincidental epitope regions around amino acids 23–29 and amino acids 60–82.

Secondary structure determination revealed α-helicity in human apoA-I of 53 and 74% in the lipid-free and rHDL states, respectively, which was a 21% increase. However, bovine apoA-I showed 53 and 66% α-helicity in the lipid-free and rHDL states, respectively, indicating a 13% increase in α-helicity. Porcine apoA-I exhibited 55 and 70% α-helicity in the lipid-free and rHDL states, respectively, which was a 15% increase in α-helicity. These results indicate that the α-helicity of individual apoA-I from bovine or porcine plasma is lower than that isolated from human plasma. The inclusion of more bovine or porcine apoA-I molecules into rHDL (Fig. 2B) suggests that additional α-helicity is non-essential. Another interpretation of this finding is that more bovine or porcine apoA-I molecules are required for rHDL formation due to their lower α-helicity.

As regards the structural and functional analysis of apoA-I, Jonas and Krajnovich (28) reported that bovine apoA-I displays a blue shift of approximately 10 nm in its WMF between the lipid-free and lipid-bound (DMPC-rHDL) states. Additionally, they observed that the α-helicity of bovine apoA-I was 58 or 72% in the lipid-free and lipid-bound states, respectively. This is consistent with our current results, although we used POPC as a phospholipid in this study. The weakened DMPC clearance activity of bovine and porcine apoA-I positively correlated with the reduced α-helicity and the increased molecular number of apoA-I in the POPC-rHDL state, as greater α-helicity is necessary to generate larger rHDL particles.

The atheroprotective functions of HDL are characterized by the potent inhibition of LDL oxidation, as well as the expression of endothelial cell adhesion molecules and monocyte chemoattractant protein-1. HDL promotes the efflux of cholesterol from foam cells. In the present study, bovine apoA-I showed the most potent inhibitory activity toward LDL oxidation and macrophage uptake, suggesting that it may be used in nanoparticles for the delivery of therapeutic drugs. The strong inhibition of LDL oxidation by bovine apoA-I (Fig. 4) positively correlated with the decrease in macrophage acLDL phagocytosis (Fig. 5).

Another major function of apoA-I is its antioxidant activity toward LDL. It is well known that the oxidation of LDL participates in the initiation of atherosclerosis and coronary artery disease. Further, the uptake of oxLDL into macrophages, which results in foam cell formation, is an early step in the generation of atherosclerotic plaque. Based on the characterization of rHDL (Table I), bovine apoA-I possesses the greatest capacity to form rHDL among the species, although its minor band size varied. Human apoA-I rHDL contained smaller particles of approximately 80 and 98 Å, whereas rHDL containing either bovine or porcine apoA-I exhibited particles of 105 Å (Fig. 2A). Therefore, bovine and porcine apoA-I possibly facilitate the formation of larger rHDL particles with the same molar ratio as greater numbers of apoA-I molecules are required to increase rHDL. Furthermore, bovine apoA-I cross-linking resulted in pentameric structures without any monomeric band, indicating that the majority of bovine apoA-I monomer participated in the cross-linking. These results indicate the enhanced susceptibility of bovine apoA-I to cross-linking. Bovine apoA-I has reportedly been associated with immune function in cattle as reported in the study by Oikawa et al (29). The serum concentration of apoA-I was decreased in cows infected with Salmonella typhimurium. In addition, bovine apoA-I-rHDL had the largest particle size (approximately 105 Å) (Table I). In our previous study, higher HDL levels were associated with a stronger antioxidant ability compared with lower HDL levels (30). Taken together, these data suggest that the stronger antioxidant ability of bovine apoA-I may be due to the increased particle size. In future studies, structural and functional correlations should be investigated in greater detail.

In conclusion, bovine and porcine apoA-I exhibit unique properties in the lipid-free and lipid-bound (rHDL) states compared with human apoA-I. Specifically, they demonstrated enhanced antioxidant abilities and were resistant to denaturation by urea, suggesting that they may be effective delivery vehicles for therapeutic drugs or vaccines. Future studies are required for the development of encapsulated viral particles in HDL-like structures and to examine their bio-availability in such endeavors.

Acknowledgements

This study was supported by the Yeungnam University Research grants in 2010. The authors are grateful for the BK21 plus program of the National Research Foundation for the support of graduate students.

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October 2013
Volume 32 Issue 4

Print ISSN: 1107-3756
Online ISSN:1791-244X

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Spandidos Publications style
Kim S, Park G, Choi I and Cho K: Bovine apolipoprotein (apo)A-I displays more enhanced antioxidant and anti-atherosclerotic activity in lipid-free and lipid-bound states than human and porcine apoA-I. Int J Mol Med 32: 843-850, 2013
APA
Kim, S., Park, G., Choi, I., & Cho, K. (2013). Bovine apolipoprotein (apo)A-I displays more enhanced antioxidant and anti-atherosclerotic activity in lipid-free and lipid-bound states than human and porcine apoA-I. International Journal of Molecular Medicine, 32, 843-850. https://doi.org/10.3892/ijmm.2013.1473
MLA
Kim, S., Park, G., Choi, I., Cho, K."Bovine apolipoprotein (apo)A-I displays more enhanced antioxidant and anti-atherosclerotic activity in lipid-free and lipid-bound states than human and porcine apoA-I". International Journal of Molecular Medicine 32.4 (2013): 843-850.
Chicago
Kim, S., Park, G., Choi, I., Cho, K."Bovine apolipoprotein (apo)A-I displays more enhanced antioxidant and anti-atherosclerotic activity in lipid-free and lipid-bound states than human and porcine apoA-I". International Journal of Molecular Medicine 32, no. 4 (2013): 843-850. https://doi.org/10.3892/ijmm.2013.1473