Your search keyword '"Marcel YL"' showing total 12 results

1. Seminal plasma choline phospholipid-binding proteins stimulate cellular cholesterol and phospholipid efflux.

Author

Moreau R, Frank PG, Perreault C, Marcel YL, and Manjunath P

Subjects

Apolipoproteins A pharmacology, Cells, Cultured, Fibroblasts, Humans, Lipoprotein(a) pharmacology, Lipoproteins, HDL pharmacology, Seminal Plasma Proteins, Cholesterol metabolism, Phospholipids metabolism, Prostatic Secretory Proteins, Proteins pharmacology, Semen chemistry

Abstract

Bovine seminal plasma (BSP) contains a family of phospholipid-binding proteins (BSP-A1/-A2, BSP-A3 and BSP-30-kDa, collectively called BSP proteins) that potentiate sperm capacitation induced by high-density lipoproteins. We showed recently that BSP proteins stimulate cholesterol efflux from epididymal spermatozoa and play a role in capacitation. Here, we investigated whether or not BSP proteins could stimulate cholesterol and phospholipid efflux from fibroblasts. Cells were radiolabeled ([3H]cholesterol or [3H]choline) and the appearance of radioactivity in the medium was determined in the presence of BSP proteins. Alcohol precipitates of bovine seminal plasma (designated crude BSP, cBSP), purified BSP-A1/-A2, BSP-A3 and BSP-30-kDa proteins stimulated cellular cholesterol and choline phospholipid efflux from fibroblasts. Efflux mechanistic differences were observed between BSP proteins and other cholesterol acceptors. Preincubation of BSP-A1/-A2 proteins with choline prevented cholesterol efflux, an effect not observed with apolipoprotein A-I. Also, the rate of BSP-induced efflux was rapid during the first 20 min, but leveled off thereafter in contrast to a relatively slow, but constant, rate of cholesterol efflux mediated by apolipoprotein A-I, apolipoprotein A-I-containing reconstituted lipoproteins (LpA-I) and high-density lipoproteins. These results indicate that fibroblasts are a good cell model to study the mechanism of lipid efflux mediated by BSP proteins.

Published

1999

2. Characterization of human apolipoprotein A-I expressed in Escherichia coli.

Author

Bergeron J, Frank PG, Emmanuel F, Latta M, Zhao Y, Sparks DL, Rassart E, Denèfle P, and Marcel YL

Subjects

Amino Acid Sequence, Apolipoprotein A-I genetics, Apolipoprotein A-I metabolism, Base Sequence, Cholesterol metabolism, DNA, Complementary genetics, Dimyristoylphosphatidylcholine metabolism, Epitope Mapping, Escherichia coli genetics, Humans, In Vitro Techniques, Kinetics, Lipoprotein(a) analogs & derivatives, Lipoprotein(a) isolation & purification, Lipoprotein(a) metabolism, Molecular Structure, Mutagenesis, Site-Directed, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sterol O-Acyltransferase metabolism, Apolipoprotein A-I isolation & purification

Abstract

Human apolipoprotein A-I (apoA-I), with an additional N-terminal extension (Met-Arg-Gly-Ser-(His)6-Met) (His-apoA-I), has been produced in Escherichia coli with a final yield after purification of 10 mg protein/1 of culture medium. We have characterized the conformation and structural properties of His-apoA-I in lipid-free form, and in reconstituted lipoproteins containing two apoA-I per particle (Lp2A-I) by both immunochemical and physicochemical techniques. The lipid-free forms of the two proteins present very similar secondary structure and stability, and have also very similar kinetics of association with dimyristoyl phosphatidylcholine. His-apoA-I and native apoA-I can be complexed with 1-palmitoyl-2-oleoyl phosphatidylcholine (POPC) to form similar, stable, either discoidal or spherical (sonicated) Lp2A-I particles. Lipid-bound native apoA-I and His-apoA-I showed very similar alpha-helical content (69% and 66%, respectively in discoidal Lp2A-I and 54% and 51%, respectively in spherical Lp2A-I). The conformation of His-apoA-I in lipid-free form and in discoidal or spherical Lp2A-I has also been shown to be similar to native apoA-I by immunochemical measurements using 13 monoclonal antibodies recognizing distinct apoA-I epitopes. In the free protein and in reconstituted Lp2A-I, the N-terminal has no effect on the affinity of any of the monoclonal antibodies and minimal effect on immunoreactivity values. Small differences in the exposure of some apoA-I epitopes are evident on discoidal particles, while no difference is apparent in the expression of any epitope of apoA-I on spherical Lp2A-I. The presence of the N-terminal extension also has no effect on the reaction of LCAT with the discoidal Lp2A-I or on the ability of complexes to promote cholesterol efflux from fibroblasts in culture. In conclusion, we show that His-apoA-I expressed in E. coli exhibits similar physicochemical properties to native apoA-I and is also identical to the native protein in its ability to interact with phospholipids and to promote cholesterol esterification and cellular cholesterol efflux.

Published

1997

3. Structure of the human apolipoprotein D gene promoter region.

Author

Lambert J, Provost PR, Marcel YL, and Rassart E

Subjects

Apolipoproteins D, Base Sequence, Exons, Genes, Regulator, Humans, Molecular Sequence Data, Oligodeoxyribonucleotides, Regulatory Sequences, Nucleic Acid, TATA Box, Transcription, Genetic, Apolipoproteins genetics, Promoter Regions, Genetic

Abstract

A human genomic clone of 18.2 kbp encompassing the apolipoprotein D (apoD) exon-1 and 2 and 10 kbp of upstream sequence was isolated and characterized. DNA sequencing and primer extension analysis revealed a transcriptional initiation site located 27 bp downstream of a consensus TATA box sequence. The exon 1 was 66 bp long. Computer analysis of DNA sequence from positions -557 to +129 revealed some putative transcriptional regulatory elements including a stretch of (pyrimidine/purine)26 located from nucleotide -263 to nucleotide -212, which could potentially form Z-DNA. Steroid hormone regulatory elements were identified which may be related to the modulation of apoD gene expression by androgens and estrogens in vitro.

Published

1993

4. Studies on the polymorphism of human apolipoprotein A-I.

Author

Nestruck AC, Suzue G, and Marcel YL

Subjects

Amino Acids analysis, Apolipoproteins isolation & purification, Apolipoproteins metabolism, Electrophoresis, Polyacrylamide Gel, Enzyme Activation, Epitopes, Humans, Hydrogen-Ion Concentration, Isoelectric Focusing, Male, Molecular Weight, Phosphatidylcholine-Sterol O-Acyltransferase metabolism, Polymorphism, Genetic, Solubility, Apolipoproteins blood, Lipoproteins, HDL blood

Abstract

Upon preparative isoelectric focussing of human apo-HDL, four major forms of apolipoprotein A-I have been isolated. As identified by the following nomenclature and pI, they comprise: apolipoprotein A-I1, pI 5.62; apolipoprotein A-I2, pI 5.53; apolipoprotein A-I3, pI 5.45; apolipoprotein A-I4 pI 5.36. These forms of apolipoprotein A-I were shown to have identical migration on polyacrylamide gel electrophoresis, molecular weights of 26 000 on sodium dodecyl sulfate gel electrophoresis and a common antigenicity with antisera against apolipoprotein A-I or A-I1. Each form had very similar amino acid compositions with the exception of form apolipoprotein A-I4 which contained one isoleucine residue per mol. All forms but apolipoprotein A-I4 were activators of lecithin:cholesterol acyltransferase, the latter was inhibitory to the reaction. From these results, it was concluded that apolipoprotein A-I1, A-I2 and A-I3 are equivalent forms of apolipoprotein A-I whereas apolipoprotein A-I4 is different or heterogeneous. Upon refocussing, the polymorphs were shown to be stable at their pI and not affected by changes in concentration and by the presence of urea or ampholytes. Exposure of a form of apolipoprotein A-I to alkaline pH partially regenerated the original heterogeneity; however, apolipoprotein A-I4 regenerated from apolipoprotein A-I1 did not contain isoleucine, which further demonstrates form apolipoprotein A-I4 heterogeneity.

Published

1980

5. Cholesteryl ester and apolipoprotein E transfer between human high density lipoproteins and chylomicrons.

Author

Marcel YL, Vezina C, and Milne RW

Subjects

Apolipoproteins E, Carbon Radioisotopes, Cold Temperature, Humans, Iodine Radioisotopes, Kinetics, Apolipoproteins blood, Cholesterol Esters blood, Chylomicrons blood, Lipoproteins, HDL blood

Abstract

The transfer of cholesteryl esters and apolipoprotein E has been studied between plasma HDL and chylomicrons isolated either from ascitic fluid or from the plasma of a patient with type V hyperlipoproteinemia. Whereas apolipoprotein E transfer was rapid and occurred at low temperature, cholesteryl ester transfer was suppressed at 4 degrees C. Apolipoprotein E transfer did not depend upon the presence of cholesteryl ester transfer protein and was in fact inhibited by the partially purified preparation of this protein. Apolipoprotein E transfer was not increased by reduction with dithiothreitol. The transfer of cholesteryl esters increased sharply at a chylomicron to HDL ratio of cholesteryl ester above 1/10, a value which may be of physiological significance at the peak of postprandial lipemia. At this ratio, the transfer of apolipoprotein E was minimal and increased only at ratios above 2/1. From these results, it is concluded that there is no connection between apolipoprotein E and cholesteryl ester transfer from HDL to chylomicrons. It is, therefore, proposed that whereas chylomicron apolipoprotein E is acquired rapidly and mostly in the lymphatic system, the concentration of chylomicron cholesteryl esters increases significantly and independently in the circulation.

Published

1983

6. Tangier disease apolipoprotein A-I compared with normal plasma A-I using monoclonal antibodies.

Author

Weech PK, Frohlich J, Marcel YL, N'Guyen TD, and Milne RW

Subjects

Antibodies, Monoclonal, Apolipoprotein A-I, Apolipoproteins A immunology, Apolipoproteins A isolation & purification, Epitopes analysis, Humans, Reference Values, Apolipoproteins A blood, Hypolipoproteinemias blood, Lipoproteins, HDL blood, Tangier Disease blood

Abstract

The molecular defect in Tangier disease is unknown. We have compared the electrophoretic and immunoreactive properties of Tangier disease and normal apolipoprotein A-I using four monoclonal antibodies. We verified that the molecular weight, pI and CNBr-cleaved fragments of Tangier disease and normal apolipoprotein A-I were not different, excluding the possibility that dimers, aggregates or fragments of apolipoprotein A-I could be responsible for its rapid catabolism in this disease.

Published

1985

7. Apolipoprotein A-I from normal human plasma: definition of three distinct antigenic determinants.

Author

Weech PK, Milne RW, Milthorp P, and Marcel YL

Subjects

Animals, Antibodies, Monoclonal, Apolipoprotein A-I, Apolipoproteins A immunology, Binding, Competitive, Female, Humans, Immunoglobulin G, Kinetics, Mice, Mice, Inbred BALB C, Apolipoproteins A blood, Epitopes analysis, Lipoproteins, HDL blood

Abstract

We have prepared, selected and cloned four mouse hybridomas that secreted monoclonal antibodies against human plasma apolipoprotein A-I. These antibodies are all of the IgG-I subclass, and were named anti-A-I 6B8, 5G6, 3D4 and 5A6. We characterized the specificity of the antibodies, finding that all four of them reacted similarly, and with only the major proteins having the molecular weight and isoelectric focusing characteristics of apolipoprotein A-I. The antibodies reacted with all known charge-polymorphs of apolipoprotein A-I and pro apolipoprotein A-I. Thus, the polymorphs of apolipoprotein A-I are alike in that they all contain the antigenic sites of these four antibodies. In a solid-phase, antibody competition radioimmunoassay we found inhibition or enhancement of antibody binding to apolipoprotein A-I, according to the pair of antibodies tested. Antibodies 6B8, 5G6 and 3D4 were different from one another and reacted with different antigenic determinants, but 5A6 was similar to 3D4 and reacted at the same site. We compared the reactions of the four antibodies with CNBr-cleaved fragments of apolipoprotein A-I separated by polyacrylamide gel electrophoresis. We found three different patterns of reaction with the apolipoprotein A-I fragments; 6B8, 5G6 and 3D4 were different, but 5A6 resembled 3D4. Thus, the four antibodies reacted with at least three different antigenic sites in apolipoprotein A-I, which were present in different CNBr fragments of apolipoprotein A-I, but not on fragment 4 which forms the carboxy-terminal segment.

Published

1985

8. The effect of portacaval shunt on plasma lipids and lipoproteins in swine.

Author

Nestruck AC, Lussier-Cacan S, Bergseth M, Bidallier M, Davignon J, and Marcel YL

Subjects

Animals, Cholesterol Esters blood, Female, Lipoproteins, HDL blood, Lipoproteins, LDL blood, Lipoproteins, VLDL blood, Swine, Time Factors, Cholesterol blood, Lipoproteins blood, Phospholipids blood, Portacaval Shunt, Surgical, Triglycerides blood

Abstract

Plasma lipids and lipoprotein composition and distribution were studied in fasted miniature swine prior to and at 5 and 19 weeks following portacaval shunt surgery or a sham operation. Plasma triacylglycerol and cholesterol levels were significantly reduced in the portacaval shunt swine at 5 weeks. These reductions were accompanied by significant decreases in the plasma very low density lipoprotein (d less than 1.006), low density lipoprotein (d = 1.02-1.07) and high density lipoprotein (d = 1.09-1.21) levels. The very low density lipoprotein were shown depleted in lipids and the low density lipoprotein was a cholesterol-depleted, triacylglycerol-enriched particle. No changes in the composition of the high density lipoprotein were observed. These reductions and changes in composition were maintained until killing at 19 weeks post-surgery.

Published

1977

9. Comparison of very-low-density lipoproteins isolated from rat liver perfusate, rat serum and human plasma as acceptors for cholesteryl ester transfer.

Author

Noël SP, Dupras R, Vézina C, and Marcel YL

Subjects

Animals, Cholesterol Ester Transfer Proteins, Humans, Kinetics, Lipoproteins, HDL blood, Lipoproteins, VLDL blood, Rats, Species Specificity, Carrier Proteins metabolism, Cholesterol Esters metabolism, Glycoproteins, Lipoproteins, VLDL metabolism, Liver metabolism

Abstract

Using two methods, we have compared the ability of three types of very-low-density lipoprotein (VLDL), namely, rat hepatic perfusate VLDL, rat serum VLDL and human plasma VLDL, to accept cholesteryl esters from human plasma high-density lipoprotein (HDL). Both net mass and isotopic transfers of cholesteryl ester were evaluated. The VLDL concentration in the incubation media was adjusted on the basis of equivalent amounts of either cholesteryl ester, apolipoprotein B or triacylglycerol. In each case, the net mass transfer of cholesteryl ester was found to be greatest to rat hepatic VLDL, lower to rat serum VLDL and lowest to human plasma VLDL. Similar results were obtained with the isotopic transfer method when the VLDL concentration was adjusted on the basis of cholesteryl ester or apolipoprotein B. However, when VLDL were matched on the basis of triacylglycerol concentration, the isotopic transfer rate into human plasma VLDL was twice as high as into rat hepatic VLDL which presumably reflects the decreased number of hepatic VLDL particles by this criterion. In conclusion under fasted conditions (chylomicron excluded), nascent VLDL have been shown to be the best cholesteryl ester acceptor compared to their plasma counterpart.

Published

1984

10. Preparative isoelectric focussing of apolipoproteins C and E from human very low density lipoproteins.

Author

Marcel YL, Bergseth M, and Nestruck AC

Subjects

Amino Acids analysis, Apolipoproteins analysis, Electrophoresis, Polyacrylamide Gel, Humans, Isoelectric Focusing, Lipoproteins, VLDL analysis, Apolipoproteins blood, Lipoproteins, VLDL blood

Abstract

The application of isoelectric focussing on a gel-stabilized layer for the separation of the Tris-urea-soluble apolipoproteins of very low density lipoproteins has been described. This method in one step, allows the separation of most apolipoproteins, which were then analyzed and characterized. Apolipoproteins CII and CI were isolated as single protein bands with apparent pI of 5.0 and 6.5, respectively. Apolipoprotein CII was biologically active and could activate lipoprotein lipase. Apolipoprotein CIII was separated into several protein bands with pI ranging from 4.7 to 5.1 as a function of their number of sialic acid residues. Apolipoprotein E was isolated and characterized into five polymorphic bands with pI of 5.7, 5.8, 5.9, 6.0, and 6.2, respectively.

Published

1979

11. A method for the determination of the initial rate of reaction of lecithin: cholesterol acyltransferase in human plasma.

Author

Marcel YL and Vezina C

Subjects

Adult, Cholesterol, Chromatography, Gas, Female, Humans, Kinetics, Lipoproteins, HDL pharmacology, Male, Methods, Phosphatidylcholines, Sex Factors, Acyltransferases blood

Published

1973

12. The preferred metabolic pathway from linoleic acid to arachidonic acid in vitro.

Author

Marcel YL, Christiansen K, and Holman RT

Subjects

Animals, Carbon Isotopes, Chromatography, Gas, Depression, Chemical, Dietary Fats metabolism, Fatty Acids pharmacology, Fatty Acids, Essential metabolism, Male, Rats, Stimulation, Chemical, Arachidonic Acids metabolism, Linoleic Acids metabolism, Liver metabolism, Microsomes metabolism

Published

1968