Your search keyword '"Wirtz KW"' showing total 229 results

151. Effect of nonspecific phospholipid transfer protein on cholesterol esterification in microsomes from Morris hepatomas.

Author

van Heusden GP, van der Krift TP, Hostetler KY, and Wirtz KW

Subjects

Acyl Coenzyme A metabolism, Animals, Carbon Radioisotopes, Male, Rats, Rats, Inbred BUF, Acyltransferases metabolism, Carrier Proteins metabolism, Cholesterol metabolism, Cholesterol Esters biosynthesis, Liver Neoplasms, Experimental metabolism, Membrane Proteins, Microsomes metabolism, Phospholipid Transfer Proteins, Phospholipids metabolism, Sterol O-Acyltransferase metabolism

Abstract

The content of cholesterol and cholesterol ester as well as the levels of acyl coenzyme A:cholesterol acyltransferase activity were determined in the microsomes from Morris hepatomas 7777, 5123D, and 7787. The free cholesterol content, expressed per mg microsomal protein, was significantly increased only in the microsomes from Morris hepatoma 7777 [47.8 +/- 0.4 micrograms (S.D.); p less than 0.001] and hepatoma 7787 (37.6 +/- 6.2 micrograms; p less than 0.01) as compared to normal liver (28.8 +/- 2.4 micrograms). The cholesterol ester content in the microsomes of the three different tumors did not significantly differ from that of normal liver (2.1 +/- 1.2 micrograms cholesterol per mg microsomal protein). The microsomal acyl coenzyme A:cholesterol acyltransferase activity was decreased in Morris hepatoma 7777 (8.6 +/- 2.3 pmol/min/mg protein; p less than 0.01) and in hepatoma 5123D (7.5 +/- 1.7 pmol/min/mg protein; p less than 0.02), and was normal in the hepatoma 7787 (16.5 +/- 7.8 pmol/min/mg protein) as compared to rat liver (16.0 +/- 2.9 pmol/min/mg protein). In a previous study (B. J. H. M. Poorthuis and K. W. A. Wirtz, Biochim. Biophys. Acta, 710: 99-105, 1982), this acyltransferase activity was shown to be stimulated by preincubation of rat liver microsomes with cholesterol-containing vesicles and the nonspecific phospholipid transfer protein. In this paper, a similar 4-fold stimulation of activity was observed for the microsomes of the various hepatomas investigated. The possible role of the nonspecific phospholipid transfer protein in intracellular cholesterol esterification is discussed.

Published

1983

152. Identification of the lipid-binding site of phosphatidylcholine-transfer protein with phosphatidylcholine analogs containing photoactivable carbene precursors.

Author

Westerman J, Wirtz KW, Berkhout T, van Deenen LL, Radhakrishnan R, and Khorana HG

Subjects

Amino Acid Sequence, Animals, Binding Sites, Cattle, Hydrocarbons, Liver metabolism, Peptide Fragments isolation & purification, Phospholipid Transfer Proteins, Photochemistry, Spectrometry, Fluorescence, Androgen-Binding Protein, Carrier Proteins metabolism, Lipid Metabolism, Methane analogs & derivatives, Phosphatidylcholines metabolism

Abstract

The lipid binding site of the phosphatidylcholine transfer protein from bovine liver has been investigated by use of phosphatidylcholine analogs which carry a diazirinophenoxy group linked to the omega-carbon of either the sn-2-[1-14C]hexanoyl (PC I) or sn-2-[1-14C]undecanoyl chain (PC II). Photolysis of the PC I(PC II)-transfer protein complex resulted in a covalent coupling of 30-40% of the label to the protein as shown by sodium dodecyl sulfate/polyacrylamide gel electrophoresis. Upon mild alkaline treatment of the photolysed complex the protein containing covalently coupled 14C-label was separated from the noncoupled 14C-label by gel permeation chromatography. The 14C-labeled protein was degraded with protease from Staphylococcus aureus, trypsin and cyanogen bromide and specific 14C-labeled peptides were sequenced by automated Edman degradation. Major sites of coupling shown by release of radioactivity were identified as Tyr54 and the peptide segment Val171-Phe-Met-Tyr-Tyr-Phe-Asp177. Both PC I and PC II coupled extensively to Tyr54 (90% and 50% of total labeling, respectively). The remainder of the radioactivity was released from the peptide Val171-Asp177 with a distinct difference in in the pattern of release depending on whether PC I or PC II were used. Thus, coupling occurred preferentially to Tyr175 and Asp177 with PC I while Val171 and Met173 were labeled preferentially with PC II. This shift in coupling is compatible with an increase of 0.6 nm for the sn-2-fatty-acyl chains of PC I and II, assuming that the peptide Val171-Asp177 has adopted the strongly predicted beta-strand configuration. These data have been interpreted in terms of the localization of phosphatidylcholine in the phosphatidylcholine transfer protein.

Published

1983

153. The non-specific lipid transfer protein (sterol carrier protein 2) from rat and bovine liver.

Author

van Amerongen A, Teerlink T, van Heusden GP, and Wirtz KW

Subjects

Amino Acids analysis, Animals, Carrier Proteins isolation & purification, Cattle, Cell Line, Cholesterol metabolism, Female, Kinetics, Liver Neoplasms, Experimental metabolism, Male, Rats, Species Specificity, Tissue Distribution, Carrier Proteins metabolism, Liver metabolism, Plant Proteins, Sterols metabolism

Abstract

The non-specific lipid transfer protein (nsL-TP) purified from rat and bovine liver accelerates the transfer of all common diacylglycerophospholipids, cholesterol as well as glycosphingolipids and gangliosides between membranes. These proteins have molecular weights in the order of 14 500 and are highly basic (isoelectric points between 8.5 and 9.5). The primary structure of nsL-TP from bovine liver has been elucidated yielding a single polypeptide chain of 121 aminoacid residues. The protein contains one cysteine residue, essential for transfer activity, a single tryptophan residue and lacks histidine, arginine and tyrosine residues. Rat liver nsL-TP was found to be identical to sterol carrier protein 2, stimulating the microsomal conversion of intermediates between lanosterol and cholesterol. Evidence was presented that nsL-TP binds cholesterol, suggesting that it acts as a carrier. On the other hand, failure to bind phospholipids disagrees with this proposed mode of action. A sensitive enzyme immunoassay was developed to determine levels of nsL-TP in rat tissues. By use of this assay, nsL-TP was found to be most prominently present in liver and intestinal mucosa (0.78 and 0.46 microgram nsL-TP per mg protein in 105 000 X g supernatant, respectively). Subfractionation studies showed that approx. 70% of nsL-TP was present in the membrane-free cytosol. However, application of an immunosorbent-purified antibody and protein A-linked gold particles to rat liver slices demonstrated a concentration of label over the peroxisomes. By way of immunoblotting it was shown that nsL-TP was absent from peroxisomes and that the immunoreactive material was a protein of mol. wt. 58 000. nsL-TP is capable of mediating net transfer of cholesterol to membranes, deficient in this lipid. Under such conditions of net transfer, nsL-TP stimulated the microsomal esterification of cholesterol and its conversion to pregnenolone by adrenal mitochondria. Levels of nsL-TP in Reuber H35 hepatoma cells was six per cent of that found in rat hepatocytes. This very low level of nsL-TP had no effect on de novo cholesterol biosynthesis and intracellular cholesterol esterification. These results raise doubts as to whether nsL-TP has a function in in situ cholesterol metabolism.

Published

1985

154. Identification of the lipid binding site of the phosphatidylcholine exchange protein with a photosensitive nitrene and carbene precursor of phosphatidylcholine.

Author

Wirtz KW, Moonen P, van Deenen LL, Radhakrishnan R, and Khorana HG

Subjects

Amino Acid Sequence, Animals, Binding Sites, Cattle, Chemical Phenomena, Chemistry, Liver metabolism, Phosphatidylcholines chemical synthesis, Phospholipid Transfer Proteins, Photochemistry, Photolysis, Protein Conformation, Androgen-Binding Protein, Carrier Proteins metabolism, Lipid Metabolism, Phosphatidylcholines metabolism

Published

1980

155. Nonspecific lipid transfer protein (sterol carrier protein 2) is bound to rat liver mitochondria: its role in spontaneous intermembrane phospholipid transfer.

Author

Megli FM, De Lisi A, van Amerongen A, Wirtz KW, and Quagliariello E

Subjects

Animals, Hydrogen-Ion Concentration, In Vitro Techniques, Mersalyl pharmacology, Potassium Chloride pharmacology, Rats, Sulfhydryl Compounds physiology, Carrier Proteins physiology, Mitochondria, Liver metabolism, Phospholipids metabolism, Plant Proteins

Abstract

In the present study we have investigated the transfer of phospholipids between vesicles and rat liver mitochondria. Transfer was measured by electron paramagnetic resonance spectroscopy using vesicles that contained spin-labeled phospholipids. A spontaneous transfer was observed which could be strongly inhibited by treating the mitochondria with the thiol reagent mersalyl. Transfer was also greatly reduced after a saline wash of the mitochondria; the transfer activity was then recovered in the wash. This activity was inhibited by tryptic digestion and mersalyl. By gel chromatography, enzyme immunoassay and immunoblotting it was demonstrated that the activity in the wash was due to the nonspecific lipid transfer protein (sterol carrier protein 2). We could estimate that up to 85% of the spontaneous phospholipid transfer between vesicles and rat liver mitochondria was mediated by this transfer protein.

Published

1986

156. Evidence for the existence of different pools of microsomal phosphatidylinositol by the use of phosphatidylinositol-exchange protein.

Author

Brophy PJ, Burbach P, Nelemans SA, Westerman J, Wirtz KW, and van Deenen LL

Subjects

Animals, Chymotrypsin pharmacology, In Vitro Techniques, Inositol metabolism, Liposomes metabolism, Phosphatidylinositols biosynthesis, Rats, Trypsin pharmacology, Carrier Proteins metabolism, Intracellular Membranes metabolism, Microsomes, Liver metabolism, Phosphatidylinositols metabolism

Abstract

1. The phosphatidylinositol-exchange protein from bovine brain was used to determine to what extent phosphatidylinositol in rat liver microsomal membranes is available for transfer. 2. The microsomal membranes used in the transfer reaction contained either phosphatidyl[2-(3)H]inositol or (32)P-labelled phospholipid. The (32)P-labelled microsomal membranes were isolated from rat liver after an intraperitoneal injection of [(32)P]P(i). The (3)H-labelled microsomal membranes and rough- and smooth-endoplasmic-reticulum membranes were prepared in vitro by the incorporation of myo-[2-(3)H]inositol into phosphatidylinositol by either exchange in the presence of Mn(2+) or biosynthesis de novo in the presence of CTP and Mg(2+). 3. Tryptic or chymotryptic treatment of the microsomes impaired the biosynthesis de novo of phosphatidylinositol. It was therefore concluded that the biosynthesis of phosphatidylinositol and/or its immediate precursor CDP-diacylglycerol takes place on the cytoplasmic surface of the microsomal membrane. 4. Under the conditions of incubation 42% of the microsomal phosphatidyl[2-(3)H]inositol was transferred with an estimated half-life of 5min; 38% was transferred with an estimated half-life of about 1h; the remaining 20% was not transferable. Identical results were obtained irrespective of the method of myo-[2-(3)H]inositol incorporation. 5. Both measurement of phosphatidylinositol phosphorus in the microsomes after transfer and the transfer of microsomal [(32)P]phosphatidylinositol indicate that phosphatidyl[2-(3)H]-inositol formed by exchange or biosynthesis de novo was homogeneously distributed throughout the microsomal phosphatidylinositol. 6. We present evidence that the slowly transferable pool of phosphatidylinositol does not represent the luminal side of the microsomal membrane; hence we suggest that this phosphatidylinositol is bound to membrane proteins.

Published

1978

157. A comparative fluorescence polarization study of cis-parinaroyl-phosphatidylcholine and diphenylhexatriene in membranes containing different amounts of cholesterol.

Author

Christiansson A, Kuypers FA, Roelofsen B, Wirtz KW, and Op den Kamp JA

Subjects

Carrier Proteins analysis, Erythrocyte Membrane analysis, Fluorescence Polarization, Humans, Lipids analysis, Liposomes, Membranes, Artificial, Microsomes metabolism, Phosphatidylcholines blood, Phosphatidylethanolamine Binding Protein, Phospholipid Transfer Proteins, Prostatein, Pulmonary Surfactants blood, Secretoglobins, Temperature, Uteroglobin, Androgen-Binding Protein, Cholesterol analysis, Diphenylhexatriene analysis, Lysophosphatidylcholines, Phosphatidylcholines analysis, Polyenes analysis

Abstract

The steady state fluorescence anisotropy (rs) of 1-acyl-2-cis parinaroyl phosphatidylcholine (PnPC) was compared with that of diphenylhexatriene (DPH) in a variety of model- and biological membrane systems. The fluorescence anisotropy of both probes responded similarly to temperature changes and variations in the acyl chain composition in phosphatidylcholine (PC) liposomes. The presence of proteins and cholesterol increased rs for both DPH and PnPC in the biological membranes as compared to the isolated polar membrane lipids. Comparison of DPH and PnPC in dipalmitoyl-PC-liposomes with and without 50 mol% cholesterol, showed at temperatures above the phase transition of pure dipalmitoyl-PC the presence of cholesterol increased the rs-value for DPH strongly, whereas the rs-value for PnPC was much less affected. In the cholesterol-rich erythrocyte membrane as well as in microsomes from Morris hepatoma 7787, which have an increased cholesterol content as compared to normal rat liver microsomes, the rs of DPH was higher than that of PnPC. No large differences between the rs-values of both probes were evident in the normal cholesterol-poor rat liver microsomes. These effects are discussed in terms of structural differences between the probes and variation of cholesterol content. Alterations in the fatty acid composition of PC present in human erythrocyte membranes were introduced with the aid of a PC-specific transfer protein. Fluorescence anisotropy values of both probes hardly changed upon enrichment of the red cell membrane with either dipalmitoyl PC or 1-palmitoyl-2-arachidonyl PC.

Published

1984

158. The protein-mediated net transfer of phosphatidylinositol in model systems.

Author

Demel RA, Kalsbeek R, Wirtz KW, and Van Deenen LM

Subjects

Animals, Biological Transport, Cattle, Membranes, Artificial, Models, Biological, Phosphatidylcholines, Protein Binding, Brain metabolism, Nerve Tissue Proteins isolation & purification, Phosphatidylinositols metabolism

Abstract

The phospholipid monolayer technique has been used to study the transfer activity of the phospholipid exchange protein from beef brain. In measuring the transfer between a monolayer consisting of equimolar amounts of phosphatidylcholine and phosphatidylinositol and liposomes consisting of 98 mol% phosphatidylcholine and 2 mol% phosphatidylinositol, the beef brain protein demonstrates an 8-fold higher transfer activity for phosphatidylinositol than for phosphatidylcholine. Under similar conditions the phosphatidylcholine exchange protein from beef liver showed a great preference for phosphatidylcholine. Phosphatidylcholine liposomes devoid of phosphatidylinositol still functioned as receptors of phosphatidylinositol when the beef brain exchange protein was present. This indicates that this protein can catalyse a net transfer of phosphatidylinopsitol. Binding of both phosphatidylinositol and phosphatidylcholine to the beef brain protein was shown.

Published

1977

159. Static and time-resolved fluorescence studies of fluorescent phosphatidylcholine bound to the phosphatidylcholine transfer protein of bovine liver.

Author

Berkhout TA, Visser AJ, and Wirtz KW

Subjects

Binding Sites, Kinetics, Phospholipid Transfer Proteins, Spectrometry, Fluorescence, Structure-Activity Relationship, Tryptophan, Androgen-Binding Protein, Carrier Proteins metabolism, Phosphatidylcholines metabolism

Abstract

Phosphatidylcholine analogues containing a cis- parinaroyl chain at the sn-1, sn-2, or both sn-1 and sn-2 positions (1-PnA-PC, 2-PnA-PC, and diPnA -PC, respectively) have been used to investigate the lipid binding site of the phosphatidylcholine transfer protein (PC-TP) from bovine liver by fluorometric techniques. Binding of these fluorescent lipids to the protein was registered by measuring the enhancement of parinaroyl fluorescence and the quenching of the tryptophanyl fluorescence. The fluorescence intensity of 1-PnA-, 2-PnA- and diPnA -PC bound to PC-TP was proportional to the chromophore content. The energy-transfer efficiency between the tryptophan residues and the bound chromophores was approximately 40% for 1-PnA- and 2-PnA-PC and 60% for diPnA -PC. Quenching of the tryptophanyl fluorescence was, in part, accounted for by a decrease of the fluorescence lifetimes. The orientation of the 1 and 2 fatty acyl chains of the PnA-PC analogues on the transfer protein was analyzed by time-resolved fluorescence anisotropy measurements. The fluorescence anisotropy decayed according to a single exponential function yielding a rotational correlation time of 26 ns for 1-PnA-PC, 11 ns for 2-PnA-PC, and 15 ns for diPnA -PC. These correlation times indicate that both fatty acyl chains are immobilized at different positions on the protein. From the difference in correlation time we propose that the shape of the phosphatidylcholine transfer protein is ellipsoidal (axial ratio congruent to 2.5) with the 1 fatty acyl chain oriented parallel to the long symmetry axis and having an angle of 60-90 degrees with the 2 fatty acyl chain.

Published

1984

160. Phosphatidylcholine transfer protein from bovine liver.

Author

Westerman J, Kamp HH, and Wirtz KW

Subjects

Animals, Carbon Radioisotopes, Cattle, Kinetics, Phospholipid Transfer Proteins, Radioisotope Dilution Technique, Substrate Specificity, Androgen-Binding Protein, Carrier Proteins isolation & purification, Carrier Proteins metabolism, Microsomes, Liver metabolism, Phosphatidylcholines metabolism

Published

1983

161. The lipid binding site of the phosphatidylcholine transfer protein from bovine liver.

Author

van Loon D, Berkhout TA, Demel RA, and Wirtz KW

Subjects

Animals, Cattle, Fatty Acids analysis, Fluorescence Polarization, Kinetics, Models, Biological, Peptide Fragments analysis, Phospholipid Transfer Proteins, Protein Binding, Structure-Activity Relationship, Androgen-Binding Protein, Carrier Proteins metabolism, Liver metabolism, Phosphatidylcholines metabolism

Abstract

The phosphatidylcholine transfer protein (PC-TP) from bovine liver has a binding site for phosphatidylcholine (PC). Structural and molecular characteristics of this site were investigated by binding PC-analogues carrying photolabile, fluorescent and short-chain fatty acids. Analysis of the photolabeled PC/PC-TP adduct showed that the hydrophobic peptide segment Val171-Phe-Met-Tyr-Tyr-Phe-Asp177 is part of the lipid binding site for the 2-acyl chain. This site was further studied by binding PC carrying cis-parinaric acid at the sn-2-position. Time resolved fluorescence anisotropy measurements indicated that the 2-acyl chain was immobilized following the rotation of PC-TP. Similar experiments with PC carrying cis-parinaric acid at the sn-1-position demonstrated that the 1-acyl chain was immobilized as well but at a site distinctly different from that of the 2-acyl chain. Binding sites for the 1- and 2-acyl chain were then explored by use of PC-isomers carrying decanoic, lauric and myristic acid at the sn-1- (or sn-2-)-position and oleic acid at the sn-2- (or sn-1-)-position. Incubation with vesicles prepared of these PC-species indicated that binding to PC-TP diminished with decreasing acyl chain length but more so for species with short-chain fatty acids on the sn-2-position than on the sn-1-position. Transfer experiments confirmed that PC-TP discriminates between PC-isomers of apparently equal hydrophobicity favouring the transfer of these species carrying oleic acid at the sn-2-position.

Published

1985

162. The synthesis and esterification of cholesterol by hepatocytes and H35 hepatoma cells are independent of the level of nonspecific lipid transfer protein.

Author

van Heusden GP, Souren J, Geelen MJ, and Wirtz KW

Subjects

Animals, Biological Transport, Active, Cell Line, Cholesterol biosynthesis, Cholesterol Esters biosynthesis, In Vitro Techniques, Male, Rats, Rats, Inbred Strains, Sterol O-Acyltransferase metabolism, Carrier Proteins metabolism, Cholesterol metabolism, Liver metabolism, Liver Neoplasms, Experimental metabolism

Abstract

The level of the nonspecific lipid transfer protein (i.e., sterol carrier protein 2) is 16-fold lower in the Reuber H35 hepatoma cells as compared to the hepatocytes in culture (49 and 810 ng of protein per mg of 105000 X g supernatant protein, respectively). In order to establish whether there is a relationship between the level of nonspecific transfer protein and intracellular cholesterol metabolism, we have determined the biosynthesis and esterification of cholesterol in these hepatoma cells and hepatocytes. Both types of cells incorporated [3H]mevalonate into cholesterol and cholesterol ester. Incubation of both cell types with [3H]cholesterol in the medium resulted in a time-dependent uptake and subsequent conversion into cholesterol ester. In both instances, the amount of 3H label incorporated into cholesterol per mg of cellular protein was about 2-fold higher for the hepatoma cells. The kinetics of esterification of endogenously synthesized cholesterol were similar for both hepatoma cells and hepatocytes. Esterification of cholesterol derived from the medium proceeded 2-times faster in the hepatoma cells than in the hepatocytes. From the kinetics of cholesterol esterification we conclude that cells do not discriminate between cholesterol synthesized de novo and cholesterol derived from the medium. In addition, the proposition that the nonspecific lipid transfer protein is involved in cholesterol synthesis and esterification is not substantiated by this study.

Published

1985

163. Transfer of phosphatidylcholine between liposomes.

Author

Hellings JA, Kamp HH, Wirtz KW, and Van Deenen LL

Subjects

Binding Sites, Biological Transport, Carbon Radioisotopes, Chromatography, DEAE-Cellulose, Phosphatidic Acids metabolism, Phosphatidylcholines metabolism, Protein Binding, Surface Properties, Liposomes metabolism

Published

1974

164. Binding of phospholipids to the phosphatidylinositol transfer protein from bovine brain as studied by steady-state and time-resolved fluorescence spectroscopy.

Author

Van Paridon PA, Visser AJ, and Wirtz KW

Subjects

Animals, Binding Sites, Cattle, Fluorescent Dyes, Isoelectric Focusing, Lysophosphatidylcholines metabolism, Phosphatidylcholines metabolism, Phosphatidylinositols metabolism, Phospholipid Transfer Proteins, Spectrometry, Fluorescence, Brain Chemistry, Carrier Proteins metabolism, Lysophospholipids, Membrane Proteins, Phospholipids metabolism

Abstract

The phosphatidylinositol transfer protein isolated from brain, liver, heart and platelets was found to be present in two subforms which could be distinguished on the basis of the isoelectric points. In this study we have demonstrated that the two subforms isolated from bovine brain are due to the presence of either phosphatidylinositol or phosphatidylcholine in the lipid binding site of the protein. The transfer protein accommodates one phosphatidylinositol molecule in the binding site. The binding site for the sn-2 fatty acyl chain was investigated by incorporating in the transfer protein either phosphatidylinositol or phosphatidylcholine carrying a parinaroyl-chain attached at the sn-2 position. Time-resolved fluorescence spectroscopy revealed that the sn-2 fatty acyl chains for both phospholipids in the lipid-protein complex were completely immobilized (i.e., rotational correlation times of 17.4 ns for phosphatidylcholine and 16.3 ns for phosphatidylinositol). The similarity in correlation times suggests that the sn-2 fatty acyl chains of both phospholipids are accommodated in the same hydrophobic binding site of the protein.

Published

1987

165. Cholesterol transfer from mitochondrial membranes and cells to human and rat serum lipoprotein fractions.

Author

van Heusden GP, van Schijndel JW, and Wirtz KW

Subjects

Animals, Apolipoproteins blood, Cattle, Cholesterol blood, Humans, In Vitro Techniques, Intracellular Membranes metabolism, Lipoproteins, HDL blood, Rats, Tumor Cells, Cultured metabolism, Cholesterol metabolism, Lipoproteins blood, Mitochondria, Heart metabolism

Abstract

We have investigated the transfer of [14C]cholesterol from labeled bovine heart mitochondria and Friend erythroleukemic cells to high density lipoprotein (HDL), low density lipoprotein (LDL), and very low density lipoprotein (VLDL) fractions from human and rat plasma. The lipoprotein fractions were obtained by molecular sieve chromatography of plasma on agarose A-5m columns. For either membrane system, the highest rate of [14C]cholesterol transfer was observed with the human and the rat HDL fraction. Since the mitochondria lack the receptors for HDL, one may conclude that the observed preferential transfer is not governed by a receptor-controlled interaction of HDL with the membrane. Under conditions where the pool of free cholesterol in the lipoprotein fractions was the same, HDL was a much more efficient acceptor of [14C]cholesterol from mitochondria than LDL or VLDL. Similarly, transfer of [14C]cholesterol proceeded at a higher rate to HDL than to sonicated egg phosphatidylcholine (PC) vesicles, even under conditions where there was a tenfold excess of the vesicle-PC pool over the HDL phospholipid pool. This preferred transfer of [14C]cholesterol to HDL cannot be explained by a random diffusion of monomer cholesterol molecules. Rather, it shows that HDL has a specific effect on this process in the sense that it most likely enhances the efflux of cholesterol from the membrane. Treatment of HDL with trypsin reduced the rate of [14C]cholesterol transfer by 40-50%, indicating that protein component(s) are involved. One of these components appears to be apoA-I, as this protein was shown to enhance the transfer of [14C]cholesterol from mitochondria to lipid vesicles.

Published

1989

166. Free fatty acids and esters can be immobilized by receptor rich membranes from Torpedo marmorata but not phospholipid acyl chains.

Author

Rousselet A, Devaux PF, and Wirtz KW

Subjects

Animals, Cell Membrane metabolism, Electric Organ metabolism, Electron Spin Resonance Spectroscopy, Fishes, Kinetics, Phospholipids, Spin Labels, Structure-Activity Relationship, Receptors, Cholinergic metabolism, Stearic Acids

Published

1979

167. Interaction of C-reactive protein with artificial phosphatidylcholine bilayers.

Author

Volanakis JE and Wirtz KW

Subjects

Binding Sites, Detergents, Liposomes, Lysophosphatidylcholines, Membranes, Artificial, Phosphorylcholine, Structure-Activity Relationship, C-Reactive Protein, Phosphatidylcholines

Abstract

C-Reactive protein (CRP), the most characteristic of the 'acute phase proteins' (ref. 1) is thought to participate in the mediation and/or modulation of acute inflammatory processes, but its exact function is unknown. CRP has a Ca2+-dependent binding specificity for phosphorylcholine, the polar head group of two widely distributed lipids, lecithin (phosphatidylcholine, PC) and sphingomyelin (SM). A number of observations suggest that at least some of the biological activities of CRP depend on its interaction with phospholipids of cell membranes. In addition, interaction of CRP with PC- and SM-containing lipid dispersions and with PC-containing liposomes can activate the complement system. We report here that binding of CRP to model membranes of PC requires the incorporation into the bilayer of lysophosphatidylcholine (LPC). Thus, a disturbance of the molecular organisation of the bilayer appears to be necessary for binding of CRP. These findings provide a possible biochemical explanation for binding of CRP to damaged but not intact cell membranes and might be relevant to its biological function.

Published

1979

168. Immunological comparison of phosphatidylinostiol and phosphatidylcholine exchange proteins in bovine brain, liver and heart.

Author

Helmkamp GM Jr, Nelemans SA, and Wirtz KW

Subjects

Amino Acids analysis, Animals, Binding Sites, Cattle, Immunodiffusion, Muscle Proteins immunology, Muscle Proteins metabolism, Nerve Tissue Proteins immunology, Nerve Tissue Proteins metabolism, Organ Specificity, Phosphatidylinositols, Protein Binding, Proteins immunology, Brain metabolism, Liver metabolism, Myocardium metabolism, Phosphatidylcholines metabolism, Proteins metabolism

Abstract

The two phosphatidylinositol exchange proteins isolated from bovine cerebral cortex, I (isoelectric point pH 5.2) and II (isoelectric point pH 5.5), had essentially identical amino acid compositions. Rabbit antisera preparations specific to each of these brain proteins were equally effective in inhibiting the phosphatidylinositol transfer activity of both protein I and II. Judged by double diffusion on agar gels, immunoprecipitation was not observed between either of the brain phosphatidylinositol exchange proteins and anti-liver phosphatidylcholine exchange protein antibody or between liver phosphatidylcholine exchange protein and anti-brain phosphatidylinositol exchange protein antibody. Phosphatidylinositol and phosphatidylcholine transfer activity was measured in microsome-liposome assay systems. For membrane-free tissue preparations phosphatidylinositol activity increased in the order: brain greater than heart greater than liver, while phosphatidylinositol exchange proteins transferred phosphatidylinositol and phosphatidylcholine in the ratio 1.4: liver phosphatidylcholine exchange protein transferred exclusively phosphatidylcholine. Phosphatidylinositol transfer activity in brain, heart and liver was more than 80% inhibited by anti-brain phosphatidylinositol exchange protein antibody. The proportion of phosphatidylcholine transfer activity sensitive to anti-liver phosphatidylcholine exchange protein antibody was 15% for brain, 75% for liver and 20% for heart, while the proportion sensitive to anti-brain phosphatidylinositol exchange protein antibody was 65% for brain, 10% for liver and 60% for heart. Together these two classes of phospholipid exchange proteins accounted for approx. 80% of the phosphoatidylcholine transfer activity in selected bovine tissues. A protein which was chemically, immunologically, and catalytically similar to liver phosphatidylcholine exchange protein was identified in brain and contributed about 20% of the phosphatidylcholine transfer activity in that tissue.

Published

1976

169. The phosphatidylcholine transfer protein from bovine liver discriminates between phosphatidylcholine isomers. A monolayer study.

Author

van Loon D, Demel RA, and Wirtz KW

Subjects

Animals, Binding Sites, Carbon Radioisotopes, Cattle, Liver metabolism, Phospholipid Transfer Proteins, Pressure, Structure-Activity Relationship, Tritium, Androgen-Binding Protein, Carrier Proteins metabolism, Phosphatidylcholines metabolism

Abstract

The activity of the phosphatidylcholine transfer protein from bovine liver toward phosphatidylcholine isomers carrying a long and a short fatty acyl chain on either the sn-1- or sn-2-position was determined by way of the monolayer-vesicle assay. In this assay equimolar mixtures of the isomers were spread at the air/water interface and their transfer measured to the vesicles in the subphase initiated by addition of the transfer protein. The following isomers were tested: 1-decanoyl-2-[3H]oleoyl-sn-glycero-3-phosphocholine (C10:0/[3H]C18:1-PC) and 1-oleoyl-2-decanoyl-sn-glycero-3-phospho[14C]choline (C18:1/C10:0-[14C]PC); 1-lauroyl-2-[3H]oleoyl-sn-glycero-3-phosphocholine (C12:0/[3H]C18:1-PC) and 1-oleoyl-2-[14C]lauroyl-sn-glycero-3-phosphocholine (C18:1/[14C]C12:0-PC); 1-myristoyl-2-[3H]oleoyl-sn-glycero-3-phosphocholine (C14:0/[3H]C18:1-PC) and 1-oleoyl,2-myristoyl-sn-glycero-3-phospho[14C]choline (C18:1/C14:0-[14C]PC). It was found that the protein transferred C10:0/[3H]C18:1-PC twice as fast as C18:1/C10:0-[14C]PC. Similar differences in rate were observed for C12:0/[3H]C18:1-Pc and C18:1/[14C]C12:0-PC but not for the isomers carrying myristic acid. We propose that the transfer protein can discriminate between PC isomers due to the presence of distinct binding sites for the sn-1- and sn-2-acyl chain (Berkhout et al. (1984) Biochemistry, 23, 1505-1513).

Published

1986

170. The primary structure of the nonspecific lipid transfer protein (sterol carrier protein 2) from bovine liver.

Author

Westerman J and Wirtz KW

Subjects

Amino Acid Sequence, Amino Acids analysis, Animals, Cattle, Carrier Proteins analysis, Liver analysis, Plant Proteins

Abstract

The primary structure of the nonspecific lipid transfer protein (sterol carrier protein 2) from bovine liver has been determined. The protein consists of a single polypeptide chain of 121 amino acid residues with serine as the amino-terminal and alanine as the carboxy-terminal residue. The protein contains one single cysteine and tryptophan residue and lacks tyrosine, histidine and arginine.

Published

1985

171. Increased cholesterol esterification in rat liver microsomes in purified non-specific phospholipid transfer protein.

Author

Poorthuis BJ and Wirtz KW

Subjects

Acyl Coenzyme A metabolism, Animals, Carbon Radioisotopes, Carrier Proteins isolation & purification, Cholesterol metabolism, Kinetics, Male, Rats, Rats, Inbred Strains, Tritium, Carrier Proteins metabolism, Cholesterol Esters biosynthesis, Membrane Proteins, Microsomes, Liver metabolism, Phospholipid Transfer Proteins

Abstract

The effect of the non-specific phospholipid transfer protein purified from rat liver on the activity of acyl-CoA:cholesterol acyltransferase (EC 2.3.1.26) in rat liver microsomes was studied. The activity of cholesterol acyltransferase was measured from the rate of incorporation of [1-14C] oleoyl-CoA into cholesteryl oleate. Activity was stimulated by preincubation by the microsomes with the non-specific phospholipid transfer protein alone, but most effectively when vesicles consisting of phosphatidylcholine/cholesterol (molar ratio 1:1) also were present in the preincubation mixture. Preincubation with vesicles consisting of only phosphatidylcholine or phosphatidylcholine/phosphatidylethanolamine (molar ratio 1:1) had no effect. The stimulating effect is dependent on transfer protein and vesicle concentration and on the length of preincubation. Treatment of the transfer protein with N-ethylmaleimide abolished its effect on cholesterol ester formation. Preincubation of the microsomes with transfer protein and phosphatidylcholine/cholesterol vesicles containing radioactively labeled cholesterol shows that exogenous cholesterol is converted readily to cholesterol ester. The data are explained by the ability of non-specific phospholipid transfer protein to effect net transfer of cholesterol to those microsomes that contain cholesterol acyltransferase. Enlargement of the cholesterol substrate pool would then give rise to stimulation of the cholesterol acyltransferase activity. This study suggests a role for the transfer protein in modulating cholesterol metabolism by its ability to transport cholesterol between membranes.

Published

1982

172. Tissue distribution and subcellular localization of phosphatidylcholine transfer protein in rats as determined by radioimmunoassay.

Author

Teerlink T, Van der Krift TP, Post M, and Wirtz KW

Subjects

Aging, Animals, Intracellular Membranes metabolism, Liver cytology, Liver metabolism, Lung metabolism, Male, Organ Specificity, Phospholipid Transfer Proteins, Prostatein, Radioimmunoassay methods, Rats, Rats, Inbred Strains, Secretoglobins, Subcellular Fractions metabolism, Tissue Distribution, Uteroglobin, Androgen-Binding Protein, Carrier Proteins metabolism

Abstract

A radioimmunoassay for the phosphatidylcholine-transfer protein from rat liver was used to measure levels of PC-transfer protein in rat tissues. The assay as described before (Teerlink, T., Poorthuis, B.J.H.M., Van der Krift, T.P. and Wirtz, K.W.A., Biochim. Biophys. Acta 665 (1981) 74-80) was modified in order to measure PC-transfer protein in tissue homogenates and subcellular membrane fractions. To this end both a detergent (Triton X-100) and a proteolytic enzyme inhibitor (aprotinin) were added to the assay medium. The radioimmunoassay measured levels of PC-transfer protein in the range of 5-50 ng and was specific for PC-transfer protein from rat tissues. Subcellular distribution studies showed that in 10% (w/v) homogenates of liver approximately 60% of the PC-transfer protein was present in the 105000 X g supernatant fraction, the remainder being evenly distributed over the particulate fractions. PC-transfer protein associated with the particulate fractions was almost completely removed by a single washing step, suggesting a dynamic equilibrium between membrane-bound and soluble PC-transfer protein. Both 105000 X g supernatants and homogenates of various rat tissues were assayed. The highest levels of PC-transfer protein were measured in liver and intestinal mucosa. Lower values were found in kidney, spleen and lung, whereas heart and brain contained hardly any PC-transfer protein. PC-transfer protein levels in regenerating rat liver did not differ significantly from levels in normal liver. In fetal lung a change in PC-transfer protein content during development was observed, with a clear maximum 2 days before term, suggesting an involvement of PC-transfer protein in the secretion of lung surfactant.

Published

1982

173. Affinity chromatography of the phosphatidylcholine exchange protein from bovine liver.

Author

Barsukov LI, Dam CW, Bergelson LD, Muzja GI, and Wirtz KW

Subjects

Animals, Carrier Proteins metabolism, Cattle, Chromatography, Affinity methods, Liver metabolism, Carrier Proteins isolation & purification, Liver analysis, Phosphatidylcholines metabolism

Abstract

Affinity chromatography has been used to purify the phosphatidylcholine exchange protein from bovine liver. The affinity resin consisted of 1-acyl-2-(9-carboxy)nonyl-glycero-3-phosphocholine linked to AH-Sepharose 4 B via the carboxyl group. Application of a crude exchange protein fraction to the affinity column resulted in a complete adsorption of the phosphatidylcholine exchange protein. The exchange protein eluted with a buffer containing 0.15% sodium deoxycholate. The most active fraction was 130-fold purified and accounted for 62% of the activity.

Published

1978

174. Phosphatidylcholine exchange protein from beef liver.

Author

Kamp HH and Wirtz KW

Subjects

Amino Acids analysis, Animals, Carbon Radioisotopes, Cattle, Chromatography, Gel, Chromatography, Ion Exchange, Egg Yolk, Female, Hydrogen-Ion Concentration, Immunoelectrophoresis, Isotope Labeling, Kinetics, Liposomes metabolism, Male, Methods, Microsomes, Liver metabolism, Molecular Weight, Proteins isolation & purification, Rats, Tritium, Liver metabolism, Membranes metabolism, Phosphatidylcholines metabolism, Proteins metabolism, Receptors, Drug

Published

1974

175. Corticotropin-(1--24)-tetracosapeptide affects protein phosphorylation and polyphosphoinositide metabolism in rat brain.

Author

Jolles J, Zwiers H, Dekker A, Wirtz KW, and Gispen WH

Subjects

Animals, Brain drug effects, Calcium pharmacology, Dose-Response Relationship, Drug, In Vitro Techniques, Kinetics, Magnesium pharmacology, Male, Phospholipids metabolism, Phosphorylation, Rats, Adrenocorticotropic Hormone analogs & derivatives, Brain metabolism, Cosyntropin pharmacology, Nerve Tissue Proteins metabolism, Phosphatidylinositols metabolism

Abstract

1. Effects of corticotropin-(1--24)-tetracosapeptide on the endogenous phosphorylation of proteins and lipids were studied in a membrane/cytosol fraction prepared from a lysed crude mitochondrial/synaptosomal fraction. 2. The labelling of proteins and lipids was monitored by incubation of the subcellular fraction for 10s with [gamma-32P]ATP. 3. The phosphorylation of proteins was dose-dependently inhibited by the peptide (40% of control incubations at 100 microM-corticotropin). 4. Of the membrane phospholipids only phosphatidylinositol phosphate, phosphatidylinositol bisphosphate and phosphatidic acid became labelled. Corticotropin dose-dependently increased the formation of phosphatidylinositol bisphosphate and inhibited the production of phosphatidic acid (470% and 50% respectively of control incubations, at 100 microM of the peptide) and had no effect on phosphatidylinositol phosphate. 5. Phosphatase activity was observed to act on phosphatidylinositol bisphosphate, phosphatidylinositol phosphate and phosphoprotein but not on phosphatidic acid. 6. Corticotropin interacted with the kinases rather than with the phosphatases. 7. The formation of phosphatidylinositol bisphosphate and phosphatidic acid was maximal at 1--10mM-Mg2+ in the absence of Ca2+, and the production of phosphatidylinositol phosphate was maximal at 30mM-Mg2+. 8. The basal value of lipid phosphorylation decreased with increasing Ca2+ concentration. 9. Ca2+ abolished the effect of corticotropin on phosphatidylinositol bisphosphate formation (470%, 190% and 100% of control incubations at respectively 0, 0.1 and 1 mM-Ca2+). 10. The data provide evidence that the effects of corticotropin on protein phosphorylation and on polyphosphoinositide metabolism in brain membranes are related.

Published

1981

176. Phospholipid exchange between membranes. Purification of bovine brain proteins that preferentially catalyze the transfer of phosphatidylinositol.

Author

Helmkamp GM Jr, Harvey MS, Wirtz KW, and Van Deenen LL

Subjects

Animals, Binding Sites, Carbon Radioisotopes, Chromatography, DEAE-Cellulose, Chromatography, Gel, Chromatography, Thin Layer, Egg Yolk, Electrophoresis, Disc, Female, Hydrogen-Ion Concentration, Isoelectric Focusing, Isotope Labeling, Kinetics, Liposomes metabolism, Male, Mercaptoethanol pharmacology, Microsomes, Liver drug effects, Molecular Weight, Nerve Tissue Proteins isolation & purification, Phosphatidylcholines metabolism, Protein Binding, Rats, Temperature, Time Factors, Tritium, Trypsin, Cerebral Cortex metabolism, Membranes metabolism, Microsomes, Liver metabolism, Nerve Tissue Proteins metabolism, Phosphatidylinositols metabolism, Receptors, Drug

Published

1974

177. Phosphatidylinositol exchange protein. Effects of membrane structure on activity and evidence for a ping-pong mechanism.

Author

Helmkamp GM Jr, Wirtz KW, and van Deenen LL

Subjects

Animals, Biological Assay, Biological Transport, Active, Cattle, Cerebral Cortex metabolism, Energy Transfer, Hydrogen-Ion Concentration, Kinetics, Liposomes, Mathematics, Microsomes, Liver metabolism, Nerve Tissue Proteins isolation & purification, Rats, Temperature, Thermodynamics, Nerve Tissue Proteins metabolism, Phosphatidylinositols metabolism

Published

1976

178. The membrane-embedded segment of cytochrome b5 as studied by cross-linking with photoactivatable phospholipids. II. The nontransferable form.

Author

Takagaki Y, Radhakrishnan R, Wirtz KW, and Khorana HG

Subjects

Amino Acid Sequence, Animals, Cyanogen Bromide, Cytochromes b5, Iodobenzoates pharmacology, Kinetics, Lipid Bilayers analysis, Peptide Fragments analysis, Phosphatidylcholines metabolism, Photochemistry, Photolysis, Rabbits, Cytochrome b Group metabolism, Phospholipids metabolism

Abstract

Rabbit liver cytochrome b5 was reconstituted into vesicles containing dipalmitoyl-sn-glycero-3-phosphocholine and the radioactively labeled photoactivatable 1-palmitoyl-2-omega-(m-diazirinophenoxy)undecanoyl-sn-glycero-3-phosphocholine (PC-I) by the cholate-gel filtration method. The cytochrome inserted predominantly in the nontransferable form (Preparation I). In addition, reconstituted vesicles containing asymmetrically distributed radioactively labeled PC-I were prepared by the use of the phosphatidylcholine transfer protein. This preparation (Preparation II) contained [14C]PC-I in the outer leaflet and [3H]PC-I predominantly in the inner leaflet. Following photolysis of the labeled vesicle preparations, the purified cross-linked products were analyzed for the distribution of the sites of cross-links. In Preparation I, a broad distribution (Asn-105 to Met-130) was found, similar to that observed with the transferable form. On the other hand, the peptide fragments obtained from the asymmetrically labeled preparation II showed 14C/3H ratios which decreased in going from Asn-105 to Met-130. We conclude that the membrane-embedded segment in the nontransferable form of cytochrome b5 spans the bilayer.

Published

1983

179. Prediction of secondary structural elements in the phosphatidylcholine-transfer protein from bovine liver.

Author

Akeroyd R, Lenstra JA, Westerman J, Vriend G, Wirtz KW, and van Deenen LL

Subjects

Amino Acid Sequence, Animals, Cattle, Models, Molecular, Phospholipid Transfer Proteins, Protein Conformation, Androgen-Binding Protein, Carrier Proteins isolation & purification, Liver metabolism

Abstract

Secondary structural elements of the phosphatidylcholine-transfer protein from bovine liver have been predicted from its primary structure with the aid of two computerized methods. The predicted alpha-helix and beta-strand content have been compared with the values derived from circular dichroism spectra. The hydrophobicity profile (Rose plot) of the protein indicated that the supposed lipid-binding site occurs in the most hydrophobic region. The predicted secondary structural elements have been folded in a tentative model of the protein molecule according to its hydrophobicity profile.

Published

1982

180. Kinetic model of the protein-mediated phosphatidylcholine exchange between single bilayer liposomes.

Author

van den Besselaar AM, Helmkamp GM Jr, and Wirtz KW

Subjects

Animals, Binding Sites, Cattle, Chromatography, Gel, Kinetics, Liver, Mathematics, Membranes, Artificial, Models, Biological, Protein Binding, Time Factors, Liposomes, Phosphatidylcholines, Proteins

Abstract

The phosphatidylcholine exchange protein from beef liver catalyzes the exchange of phosphatidylcholine between single bilayer liposomes (Hellings et al. (1974), Eur. J. Biochem. 47, 601). A model has been proposed which describes the kinetics of this exchange. Steady-state equations have been derived from the model and have been used for the derivation of the theoretical rate equation. Computer analysis shows a good fit with the experimental results. It follows from the analysis that the apparent dissociation constant of the exchange protein-liposome complex decreases with an increasing phosphatidic acid content of the liposomes. This suggests that in this model system it is the phospholipid composition of the membranes involved that regulates the amount of exchange protein available to function as a carrier of phosphatidylcholine.

Published

1975

181. Identification of an essential lysine residue in the phosphatidylcholine-transfer protein from bovine liver by modification with phenylisothiocyanate.

Author

van Loon D, Westerman J, Akeroyd R, and Wirtz KW

Subjects

Animals, Cattle, Cyanogen Bromide pharmacology, Electrophoresis, Polyacrylamide Gel, Isothiocyanates, Phospholipid Transfer Proteins, Androgen-Binding Protein, Carrier Proteins analysis, Liver analysis, Lysine analysis, Thiocyanates pharmacology

Abstract

Modification by phenylisothiocyanate inhibits the phosphatidylcholine-transfer protein from bovine liver. Inhibition by this apolar reagent was greatly enhanced in the presence of vesicles, indicating that an effective modification of an essential lysine residue(s) from the interface may occur. Labeling with [14C]phenylisothiocyanate demonstrated that Lys55 was the major site of modification. We propose that Lys55 is part of the peptide segment that interacts with the membrane.

Published

1986

182. Complete exchange of phospholipids between microsomes and plasma lipoproteins mediated by liver phospholipid-exchange proteins.

Author

Jackson RL, Westerman J, and Wirtz KW

Subjects

Animals, Cell-Free System, Humans, Lipoproteins blood, Liposomes, Phosphatidylcholines metabolism, Phosphatidylinositols metabolism, Rats, Carrier Proteins metabolism, Microsomes, Liver metabolism, Phospholipids metabolism

Published

1978

183. Protein-mediated transfer of phosphatidylcholine between membranes and liposomes.

Author

Wirtz KW, Kamp HH, and Van Deenen LL

Subjects

Animals, Biological Transport, Active, Cations, Divalent, Cations, Monovalent, Cattle, Cholesterol Esters metabolism, Liver metabolism, Mitochondria, Liver metabolism, Myocardium metabolism, Oleic Acids metabolism, Phosphatidylinositols metabolism, Rats, Receptors, Drug, Liposomes metabolism, Membranes metabolism, Phosphatidylcholines metabolism, Proteins metabolism

Published

1975

184. Action of phospholipases on the phosphatidylcholine exchange protein from beef liver.

Author

Kamp HH, Sprengers ED, Westerman J, Wirtz KW, and Van Deenen LL

Subjects

Animals, Biological Transport, Active, Butanols pharmacology, Cattle, Deoxycholic Acid pharmacology, Dioxanes pharmacology, Kinetics, Liver drug effects, Protein Binding, Liver metabolism, Phosphatidylcholines metabolism, Phospholipases pharmacology, Proteins metabolism, Receptors, Drug drug effects

Abstract

The phospholipases A2, C and D have been used to investigate the localization of phosphatidylcholine in the phosphatidylcholine exchange protein from beef liver. The rate of enzymatic hydrolysis of the protein-bound phosphatidylcholine was found to be very low. Addition of deoxycholate, isobutanol or dioxane to the native protein, under conditions where delipidation did not occur, greatly enhanced the hydrolytic action of the phospholipases. From these results it is concluded that phosphatidylcholine may be buried in the protein molecule.

Published

1975

185. Polyphosphoinositides undergo charge neutralization in the physiological pH range: a 31P-NMR study.

Author

van Paridon PA, de Kruijff B, Ouwerkerk R, and Wirtz KW

Subjects

Animals, Calcium, Chickens, Egg Yolk, Magnetic Resonance Spectroscopy, Micelles, Phosphatidylinositol 4,5-Diphosphate, Phosphatidylinositol Phosphates, Hydrogen-Ion Concentration, Phosphatidylinositols

Abstract

The charge state of phosphatidylinositol 4-phosphate and phosphatidylinositol 4,5-bisphosphate was determined as a function of pH by way of 31P-NMR spectroscopy. The pK values for the first protonation of the phosphomonoester residues in phosphatidylinositol 4-phosphate and phosphatidylinositol 4,5-bisphosphate were found to be 6.2 and 6.6, respectively, for the 4-phosphate moiety, and 7.7 for the 5-phosphate moiety.

Published

1986

186. Kinetic analysis of the interaction of the phosphatidylcholine exchange protein with unilamellar vesicels and multilamellar liposomes.

Author

Wirtz KW, Vriend G, and Westerman J

Subjects

Hydrogen-Ion Concentration, Kinetics, Phosphatidic Acids, Carrier Proteins metabolism, Liposomes metabolism, Membranes, Artificial, Phosphatidylcholines metabolism

Abstract

The mode of action of the phosphatidylcholine exchange protein from bovine liver has been studied by using unilamellar vesicles and multilamellar liposomes both of which membranes contain phosphatidylcholine and phosphatidic acid. The protein-mediated exchange of phosphatidylcholine between vesicles and liposomes fit the kinetic model presented in a previous study [V.D. Besselaar et al. (1975) Biochemistry, 1j, 1852]. Kinetic analysis of the rates of exchange indicate that the apparent dissociation constant of the exchange protein-vesicle complex decreases with an increasing phosphatidic acid content of the vesicles. Both vesicles and liposomes of 10 mol% phosphatidic acid show the same dissociation constant; on the other hand, both the formation and the disruption of the protein-membrane complex was 50--100-times higher for the vesicles than for the liposomes. This implies that the exchange protein can discriminate between vesicles and liposomes. Equilibrium gel chromatography of a column of Bio Gel A-5m confirmed that the exchange protein binds more strongly to vesicles of an increased phosphatidic acid content. The protein-mediated exchange of phosphatidylcholine in the vesicle-liposome system demonstrates a pH optimum at 4.0 to 5.5. The kinetic analysis at pH 5.0 as compared to pH 7.4 indicates that the enhanced exchange at pH 5.0 can solely be accounted for by altered interaction of the exchange protein with the liposomes.

Published

1979

187. The complete primary structure of the phosphatidylcholine-transfer protein from bovine liver. Isolation and characterization of the cyanogen bromide peptides.

Author

Akeroyd R, Moonen P, Westerman J, Puyk WC, and Wirtz KW

Subjects

Amino Acid Sequence, Animals, Cattle, Cyanogen Bromide, Peptide Fragments analysis, Peptide Hydrolases, Phospholipid Transfer Proteins, Trypsin, Androgen-Binding Protein, Carrier Proteins, Liver analysis, Phosphatidylcholines

Published

1981

188. Influence of membrane phosphatidylinositol content on the activity of bovine brain phospholipid transfer protein.

Author

Harvey MS, Helmkamp GM Jr, Wirtz KW, and Van Deenen LL

Subjects

Animals, Binding Sites, Biological Transport, Brain cytology, Brain drug effects, Cell Membrane drug effects, Cell Membrane metabolism, Kinetics, Liposomes metabolism, Microsomes, Liver metabolism, Phosphatidylcholines metabolism, Phosphatidylinositols metabolism, Protein Binding, Rats, Tritium, Ultrasonics, Brain metabolism, Nerve Tissue Proteins metabolism, Phosphatidylinositols pharmacology, Phospholipids metabolism

Published

1974

189. Transfer of cholesterol and oxysterol derivatives by the nonspecific lipid transfer protein (sterol carrier protein 2): a study on its mode of action.

Author

van Amerongen A, Demel RA, Westerman J, and Wirtz KW

Subjects

Animals, Biological Transport, Cattle, In Vitro Techniques, Membranes, Artificial, Mitochondria, Heart metabolism, Phosphatidylcholines metabolism, Protein Binding, Carrier Proteins physiology, Cholesterol metabolism, Plant Proteins, Sterols metabolism

Abstract

The nonspecific lipid transfer protein (nsLTP) facilitates the transfer of both phospholipids and cholesterol between membrane interfaces. In this study, we have investigated the transport of 14C-labelled cholesterol, 7-ketocholesterol, 7 alpha-hydroxycholesterol and 25-hydroxycholesterol from a mixed lipid monolayer at the air/water interface to acceptor vesicles in the subphase. In the absence of nsLTP the transport of cholesterol was virtually nil, whereas the spontaneous transport of the oxysterol derivatives increased in the order 7-ketosterol less than 7 alpha-hydroxycholesterol less than 25-hydroxycholesterol. In the presence of nsLTP, the transport of both cholesterol and the oxysterol derivatives was greatly enhanced; the highest rate of transport was observed for 25-hydroxycholesterol. In the absence of vesicles, binding of cholesterol and of 25-hydroxycholesterol from the monolayer to nsLTP was negligible. Similarly, nsLTP did not bind cholesterol from radiolabeled bovine heart mitochondria under conditions where it stimulated the transfer of cholesterol to vesicles. In agreement with this failure to bind, nsLTP was unable to carry cholesterol between two separate monolayers. From the monolayer experiments it became apparent that nsLTP is highly surface-active. Measurement of the transport of cholesterol and of oxysterol derivatives by the monolayer-vesicles assay and of a series of pyrene-labeled phosphatidylcholine species by the fluorescent transfer assay showed a high correlation between the spontaneous and the nsLTP-mediated lipid transport. This supports the notion that nsLTP lowers the energy barrier for the lipid monomer-membrane interface equilibration process. In view of the above observations, we propose that nsLTP may facilitate the transfer of lipids by being part of a transient collisional complex between donor and acceptor membrane.

Published

1989

190. Determination of nonspecific lipid transfer protein in rat tissues and Morris hepatomas by enzyme immunoassay.

Author

Teerlink T, Van der Krift TP, van Heusden GP, and Wirtz KW

Subjects

Animals, Immunoenzyme Techniques, Liver analysis, Methods, Phosphatidylethanolamines metabolism, Rabbits, Rats, Rats, Inbred BUF, Subcellular Fractions analysis, Tissue Distribution, Carrier Proteins analysis, Liver Neoplasms, Experimental analysis

Abstract

Rat tissues contain a nonspecific transfer protein which in vitro mediates the transfer of diacylphospholipids as well as cholesterol between membranes. This protein appears identical to sterol carrier protein. A specific enzyme immunoassay for this protein was developed using antibodies raised in rabbits, against a homogeneous protein from rat liver. This assay was based on the very high affinity of the nonspecific lipid transfer protein for polyvinyl surfaces. A reproducible adsorption was achieved by presenting the protein to the surface in the presence of a large excess of bovine serum albumin. The adsorbed protein was detected with specific immunoglobulin (IgG) isolated by antigen-linked affinity chromatography and a goat anti-rabbit IgG-enzyme conjugate. Adsorption was proportional to the amount of protein present, giving rise to a linear standard curve. The enzyme immunoassay measured transfer protein levels in the range 0.2-2 ng. The highest concentrations of transfer protein were found in liver and intestinal mucosa. Levels in other tissues including brain, lung, kidney, spleen, heart, adrenals, ovary and testis were 5-10-fold lower than in liver. In the fast-growing Morris hepatoma 7777 the concentration of nonspecific lipid transfer protein was approximately one-tenth of that measured in the host liver, whereas a reduction of 65% was observed in the slow-growing Morris hepatomas 7787 and 9633. Subcellular distribution studies showed that approx. 70% of the transfer protein was present in the soluble supernatant fraction.

Published

1984

191. Phosphatidylcholine transfer protein from rat liver: purification and radioimmunoassay.

Author

Teerlink T, Poorthuis BJ, and Wirtz KW

Subjects

Animals, Carrier Proteins metabolism, Molecular Weight, Phospholipid Transfer Proteins, Prostatein, Radioimmunoassay methods, Rats, Secretoglobins, Uteroglobin, Androgen-Binding Protein, Carrier Proteins isolation & purification, Liver metabolism, Phosphatidylcholines metabolism

Published

1983

192. Interaction of the phosphatidylcholine exchange protein with phospholipids. A fluorescence and circular dichroism study.

Author

Wirtz KW and Moonen P

Subjects

Animals, Cattle, Circular Dichroism, Dioxanes, Kinetics, Liver metabolism, Lysophosphatidylcholines, Protein Conformation, Protein Denaturation, Spectrometry, Fluorescence, Spectrophotometry, Ultraviolet, Carrier Proteins metabolism, Phosphatidylcholines metabolism, Phospholipids metabolism

Abstract

The phosphatidylcholine exchange protein from bovine liver has a fluorescence emission maximum at 327 nm. Fluorescence was enhanced in the presence of vesicles containing phosphatidylcholine and various amounts of either phosphatidic acid or phosphatidylglycerol. From the increase in fluorescence it was derived that the apparent dissociation constant of the exchange protein-vesicle complex decreased with an increased vesicle content of acidic phospholipids. Fluorescence indicated that the exchange protein interacted with lysophosphatidylcholine micelles at pH 3.5, 5.9 and 8.5. The increase in fluorescence was most prominent at the acidic pH. Circular dichroism indicated that the alpha-helix content of the native protein was low between pH 3.6 and 8.0. Interaction with lysophosphatidylcholine micelles had a negligible effect on the secondary structure of the protein, except at pH 3.6 where distinct minima at 208 nm and 220 nm in the circular dichroic spectrum became apparent.

Published

1977

193. The synthesis of sphingomyelin in the Morris hepatomas 7777 and 5123D is restricted to the plasma membrane.

Author

van den Hill A, van Heusden GP, and Wirtz KW

Subjects

Animals, Carrier Proteins metabolism, Male, Microsomes, Liver metabolism, Mitochondria, Liver metabolism, Phospholipid Transfer Proteins, Prostatein, Rats, Rats, Inbred BUF, Secretoglobins, Uteroglobin, Androgen-Binding Protein, Cell Membrane metabolism, Liver Neoplasms, Experimental metabolism, Sphingomyelins biosynthesis

Abstract

The site of sphingomyelin synthesis in the rapidly growing Morris hepatomas 7777 and 5123D was determined by incubating plasma membrane, mitochondrial and microsomal membrane fractions with vesicles of phosphatidyl[methyl-14C]choline in the presence of phosphatidylcholine transfer protein. In agreement with a previous study on rat liver (Voelker, D.R. and Kennedy, E.P., 1982, Biochemistry 21, 2753-2759) we have demonstrated that sphingomyelin synthesis in these hepatomas is restricted to the plasma membrane. The greatly elevated sphingomyelin content of mitochondria and microsomes (Hostetler, K.Y., Zenner, B.D. and Morris, H.P., 1979, Cancer Res. 39, 2978-2983) suggests that rapidly growing hepatomas, in contrast to liver, have an effective mechanism of intracellular sphingomyelin transfer.

Published

1985

194. On the relationship between the dual specificity of the bovine brain phosphatidylinositol transfer protein and membrane phosphatidylinositol levels.

Author

Van Paridon PA, Gadella TW Jr, Somerharju PJ, and Wirtz KW

Subjects

Animals, Cattle, Fluorescent Dyes, Kinetics, Liposomes metabolism, Phosphatidylcholines metabolism, Phospholipid Transfer Proteins, Pyrenes, Spectrometry, Fluorescence, Brain Chemistry, Carrier Proteins metabolism, Membrane Lipids metabolism, Membrane Proteins, Phosphatidylinositols metabolism

Abstract

The phosphatidylinositol transfer protein from bovine brain has a remarkable specificity pattern with a distinct preference for phosphatidylinositol (PI) and a low affinity for phosphatidylcholine (PC). In this study we have determined the affinity of PI-transfer protein for PI relative to that for PC by measuring the binding of the fluorescent pyrene-labeled analogs of these phospholipids. From competition binding experiments it was estimated that the transfer protein has a 16-fold higher affinity for PI than for PC. This relative affinity together with the relative abundance of PI and PC, determines what proportion of the protein contains PI (e.g. 65% of the PI-transfer protein in the case of bovine brain). From measuring lipid transfer between donor vesicles consisting of equimolar amounts of PC and PI, and an excess of acceptor vesicles consisting of various ratios of PC and PI, we have observed that the relative rates of the PI-transfer protein-mediated transfer of PI and PC varies between 5 and 20. Kinetic analysis has indicated that PI-transfer protein carrying a PI molecule has different kinetic properties than the PI-transfer protein carrying a PC molecule. It will be discussed that because of the dual specificity, PI-transfer protein is ideally suited for maintaining PI levels in intracellular membranes.

Published

1987

195. Phospholipid transfer activities in Morris hepatomas and the specific contribution of the phosphatidylcholine exchange protein.

Author

Poorthuis BJ, van der Krift TP, Teerlink T, Akeroyd R, Hostetler KY, and Wirtz KW

Subjects

Amino Acids analysis, Animals, Carrier Proteins isolation & purification, Cattle, Immunodiffusion, Mitochondria metabolism, Mitochondria, Liver metabolism, Molecular Weight, Phosphatidylcholines isolation & purification, Phospholipid Transfer Proteins, Prostatein, Rats, Secretoglobins, Species Specificity, Uteroglobin, Androgen-Binding Protein, Carrier Proteins metabolism, Liver metabolism, Liver Neoplasms, Experimental metabolism, Phosphatidylcholines metabolism, Phospholipids metabolism

Abstract

Phospholipid transfer activities for phosphatidylcholine, phosphatidylinositol and phosphatidylethanolamine were measured in three hepatomas of increasing growth rate and degree of dedifferentiation, the hepatomas of 9633 and 7777, and compared to the activities found in normal and host liver. A 2-3-fold increase was found in the phosphatidylcholine and phosphatidylinositol transfer activities in the fast-growing 7777 hepatoma, while these activities were moderately or not increased in the 7787 and 9633 hepatomas. Phosphatidylethanolamine transfer was found to be extremely low in all three hepatomas. The possible significance of these findings with respect to the altered phospholipid content and composition of the hepatoma membranes is discussed. The contribution of the phosphatidylcholine specific exchange protein to the total phosphatidylcholine transfer activity was determined in normal and host liver and in the hepatomas 7777 and 9633 with the aid o f a phosphatidylcholine exchange protein specific antiserum. To this end a new procedure for the purification of the phosphatidylcholine exchange protein from rat liver was developed which leads to a final purification factor of 5300 and a high overall yield of 17%. In addition, this protein was chemically and immunologically characterized and its properties were compared to those of the bovine phosphatidylcholine exchange protein purified in our laboratory previously.

Published

1980

196. Determination of the acyl chain specificity of the bovine liver phosphatidylcholine transfer protein. Application of pyrene-labeled phosphatidylcholine species.

Author

Somerharju PJ, van Loon D, and Wirtz KW

Subjects

Animals, Binding Sites, Cattle, Kinetics, Lipid Bilayers, Phospholipid Transfer Proteins, Pyrenes metabolism, Spectrometry, Fluorescence, Structure-Activity Relationship, Substrate Specificity, Androgen-Binding Protein, Carrier Proteins metabolism, Liver metabolism, Phosphatidylcholines metabolism

Abstract

The phosphatidylcholine transfer protein from bovine liver has specific binding sites for the sn-1 and sn-2 acyl chains of the phosphatidylcholine molecule [Berkhout, T.A., Visser, A.J. W.G., & Wirtz, K.W.A. (1984) Biochemistry 23, 1505-1513]. In the present study, we have investigated the properties of these binding sites by determining both binding and transfer of several sets of pyrenylphosphatidylcholine species. These sets consisted of positional isomers in which the length of the pyrene-labeled acyl chain (i.e., 5-13 methylene units) or of the unlabeled saturated acyl chain (i.e., 9-19 methylene units) was varied in either the sn-1 or the sn-2 position. Binding studies showed that there was a considerable discrimination between positional isomers with the higher affinity observed for those lipids that carry the pyrenyl chain in the sn-2 position. In addition, the affinity is markedly dependent on the length of the acyl chains; pyrenyl acyl chains of 9 and 11 methylene units and the palmitoyl chain provided the most efficient binding. The affinity of the transfer protein for the strongest bound pyrene lipid was approximately 2.5 times higher than for an average egg phosphatidylcholine molecule. In general, the transfer studies were in agreement with the binding data. However, with some short-chain derivatives, transfer rates were faster than expected on the basis of the binding data. This emphasizes the importance of kinetic factors (i.e., activation energy) in the transfer process. The rates of spontaneous transfer decreased monotonically with increasing chain length and were very similar for all positional isomer pairs studied.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1987

197. Transfer of phospholipids between subcellular fractions of the lung.

Author

Engle MJ, van Golde LM, and Wirtz KW

Subjects

Animals, Animals, Newborn, Biological Transport, Active, Cytosol metabolism, Female, Lung embryology, Mice, Microsomes metabolism, Mitochondria metabolism, Pregnancy, Rats, Subcellular Fractions, Carrier Proteins metabolism, Lung metabolism, Phospholipids metabolism

Published

1978

198. Identification of membrane proteins of human blood platelets with a hydrophobic photolabel.

Author

Berkhout TA, Schiphorst ME, Wirtz KW, and Sixma JJ

Subjects

Azides metabolism, Electrophoresis, Polyacrylamide Gel, Humans, Phospholipids blood, Photochemistry, Blood Platelets analysis, Membrane Proteins blood

Abstract

A photoactivable glycolipid probe, 12-(4-azido-2-nitrophenoxy)stearoyl[1-14C]glucosamine, was used to label proteins and lipids of platelet membranes. The proteins were analyzed by two-dimensional high-resolution gelelectrophoresis. The labeling patterns showed that three membrane proteins were labeled which were not previously identified by ectolabeling (Sixma, J.J. and Schiphorst, M.E. (1980) Biochim. Biophys. Acta 603, 70-83). Analysis of the lipid fraction showed that phosphatidylcholine, phosphatidylethanolamine and phosphatidylserine were labeled by the probe. The distinct labeling of phosphatidylserine strongly suggests that the probe redistributes between the two halves of the bilayer.

Published

1984

199. Purification of nonspecific lipid transfer protein (sterol carrier protein 2) from human liver and its deficiency in livers from patients with cerebro-hepato-renal (Zellweger) syndrome.

Author

van Amerongen A, Helms JB, van der Krift TP, Schutgens RB, and Wirtz KW

Subjects

Amino Acids analysis, Brain Diseases complications, Carrier Proteins deficiency, Hepatorenal Syndrome complications, Humans, Immunoassay, Immunologic Techniques, Liver metabolism, Brain Diseases metabolism, Carrier Proteins isolation & purification, Hepatorenal Syndrome metabolism, Kidney Diseases metabolism, Liver analysis

Abstract

The nonspecific lipid transfer protein (i.e., sterol carrier protein 2) from human liver was purified to homogeneity using ammonium sulfate precipitation, CM-cellulose chromatography, molecular sieve chromatography and fast protein liquid chromatography. Its amino acid composition was determined and found to be very similar to that of the nonspecific lipid transfer protein from bovine and rat liver with, as main feature, the absence of arginine, histidine and tyrosine. By way of a specific enzyme immunoassay using affinity-purified antibodies, the levels of nonspecific lipid transfer protein were determined in human livers. Levels varied from approximately 150 ng nonspecific lipid transfer protein per mg 105,000 X g supernatant protein for juvenile and adult humans to 40 ng per mg supernatant protein for a young infant. Levels of nonspecific lipid transfer protein in livers of infants with cerebro-hepato-renal (Zellweger) syndrome were extremely low (i.e., 2 ng per mg supernatant protein). Immunoblotting revealed the presence of crossreactive proteins of molecular masses of 40,000 and 58,000. The 40 kDa and 58 kDa proteins occurred in control livers, whereas only the 40 kDa protein was present in Zellweger livers. As in rat the 58 kDa protein could be demonstrated in a peroxisomal preparation isolated from an adult liver. A possible link between the occurrence of nonspecific lipid transfer protein and the presence of peroxisomes is discussed.

Published

1987

200. Transbilayer distribution and mobility of phosphatidylcholine in intact erythrocyte membranes. A study with phosphatidylcholine exchange protein.

Author

van Meer G, Poorthuis BJ, Wirtz KW, Op den Kamp JA, and van Deenen LL

Subjects

Animals, Cattle, Humans, Intracellular Membranes metabolism, Kinetics, Microsomes, Liver metabolism, Organ Specificity, Phosphatidylcholines metabolism, Rats, Erythrocyte Membrane metabolism, Erythrocytes metabolism, Lipid Bilayers, Phosphatidylcholines blood

Abstract

1. The exchange of phosphatidylcholine between intact human or rat erythrocytes and rat liver microsomes was greatly stimulated by phosphatidylcholine-specific exchange proteins from rat liver and beef liver. It was found, however, that compared to the exchange reaction between phospholipid vesicles and rat liver microsomes, much higher concentrations of exchange protein were required in the case of intact red blood cells and microsomes. 2. In human erythrocytes, 75% of the phosphatidylcholine was available for exchange within 2 h at 37 degrees C. No additional exchange was observed during the next 2 h, indicating slow, if any, transbilayer movement of the residual phosphatidylcholine. 3. In rat erythrocytes 50--60% of the phosphatidylcholine was readily available for the exchange proteins. The residual phosphatidylcholine was exchanged at a much lower rate with a half time for equilibration of 7 h. 4. These results confirm in an independent way the asymmetric distribution of phosphatidylcholine over the membrane of human and rat erythrocytes as well as the occurrence of a slow transbilayer movement of this lipid in rat erythrocytes.

Published

1980