ABSTRACT
When variably fatty acylated N-terminal amino acid sequences were appended to a green fluorescent reporter protein (GFP), chimeric GFPs were localized to different membranes in a fatty acylation-dependent manner. To explore the mechanism of localization, the properties of acceptor membranes and their interaction with acylated chimeric GFPs were analyzed in COS-7 cells. Myristoylated GFPs containing a palmitoylated or polybasic region colocalized with cholesterol and ganglioside GM(1), but not with caveolin, at the plasma membrane and endosomes. A dipalmitoylated GFP chimera colocalized with cholesterol and GM(1) at the plasma membrane and with caveolin in the Golgi region. Acylated GFP chimeras did not cofractionate with low-density caveolin-rich lipid rafts prepared with Triton X-100 or detergent-free methods. All GFP chimeras, but not full-length p62(c-yes) and caveolin, were readily solubilized from membranes with various detergents. These data suggest that, although N-terminal acylation can bring GFP to cholesterol and sphingolipid-enriched membranes, protein-protein interactions are required to localize a given protein to detergent-resistant membranes or caveolin-rich membranes. In addition to restricting acceptor membrane localization, N-terminal fatty acylation could represent an efficient means to enrich the concentration of signaling proteins in the vicinity of detergent-resistant membranes and facilitate protein-protein interactions mediating transfer to a detergent-resistant lipid raft core.
Subject(s)
Acylation , Caveolae/metabolism , Cholesterol/metabolism , Membrane Microdomains/metabolism , Proteins/metabolism , Sphingolipids/metabolism , src-Family Kinases , Animals , Biomarkers , COS Cells , Caveolin 1 , Caveolins/metabolism , Cell Fractionation , Cell Membrane/metabolism , Chlorocebus aethiops , Detergents , Filipin/metabolism , G(M1) Ganglioside/metabolism , Green Fluorescent Proteins , Luminescent Proteins/genetics , Luminescent Proteins/metabolism , Membrane Proteins/metabolism , Octoxynol , Organelles , Proto-Oncogene Proteins/metabolism , Proto-Oncogene Proteins c-yes , Solubility , Transferrin/metabolism , Vesicular Transport Proteins , XanthenesABSTRACT
Tumor necrosis factor-alpha (TNF-alpha) is a proinflammatory cytokine that activates several signaling cascades. We determined the extent to which ceramide is a second messenger for TNF-alpha-induced signaling leading to cytoskeletal rearrangement in Rat2 fibroblasts. TNF-alpha, sphingomyelinase, or C(2)-ceramide induced tyrosine phosphorylation of focal adhesion kinase (FAK) and paxillin, and stress fiber formation. Ly 294002, a phosphatidylinositol 3-kinase (PI 3-K) inhibitor, or expression of dominant/negative Ras (N17) completely blocked C(2)-ceramide- and sphingomyelinase-induced tyrosine phosphorylation of FAK and paxillin and severely decreased stress fiber formation. The TNF-alpha effects were only partially inhibited. Dimethylsphingosine, a sphingosine kinase (SK) inhibitor, blocked stress fiber formation by TNF-alpha and C(2)-ceramide. TNF-alpha, sphingomyelinase, and C(2)-ceramide translocated Cdc42, Rac, and RhoA to membranes, and stimulated p21-activated protein kinase downstream of Ras-GTP, PI 3-K, and SK. Transfection with inactive RhoA inhibited the TNF-alpha- and C(2)-ceramide-induced stress fiber formation. Our results demonstrate that stimulation by TNF-alpha, which increases sphingomyelinase activity and ceramide formation, activates sphingosine kinase, Rho family GTPases, focal adhesion kinase, and paxillin. This novel pathway of ceramide signaling can account for approximately 70% of TNF-alpha-induced stress fiber formation and cytoskeletal reorganization.
Subject(s)
Phosphotransferases (Alcohol Group Acceptor)/physiology , Sphingosine/analogs & derivatives , Sphingosine/biosynthesis , Stress Fibers/physiology , Tumor Necrosis Factor-alpha/metabolism , Animals , Cell Line , Cytoskeletal Proteins/metabolism , Cytoskeleton/metabolism , Cytoskeleton/physiology , Focal Adhesion Kinase 1 , Focal Adhesion Protein-Tyrosine Kinases , Humans , Paxillin , Phosphoproteins/metabolism , Phosphorylation , Phosphotransferases (Alcohol Group Acceptor)/metabolism , Protein-Tyrosine Kinases/metabolism , Rats , Sphingomyelin Phosphodiesterase/metabolism , Stress Fibers/metabolism , Tumor Necrosis Factor-alpha/pharmacology , Tyrosine/metabolism , cdc42 GTP-Binding Protein/metabolism , cdc42 GTP-Binding Protein/physiology , rac GTP-Binding Proteins/metabolism , rac GTP-Binding Proteins/physiology , ras Proteins/metabolism , ras Proteins/physiology , rhoA GTP-Binding Protein/metabolism , rhoA GTP-Binding Protein/physiologyABSTRACT
In addition to its role in reversible membrane localization of signal-transducing proteins, protein fatty acylation could play a role in the regulation of mitochondrial metabolism. Previous studies have shown that several acylated proteins exist in mitochondria isolated from COS-7 cells and rat liver. Here, a prominent fatty-acylated 165-kDa protein from rat liver mitochondria was identified as carbamoyl-phosphate synthetase 1 (CPS 1). Covalently attached palmitate was linked to CPS 1 via a thioester bond resulting in an inhibition of CPS 1 activity at physiological concentrations of palmitoyl-CoA. This inhibition corresponds to irreversible inactivation of CPS 1 and occurred in a time- and concentration-dependent manner. Fatty acylation of CPS 1 was prevented by preincubation with N-ethylmaleimide and 5'-p-fluorosulfonylbenzoyladenosine, an ATP analog that reacts with CPS 1 active site cysteine residues. Our results suggest that fatty acylation of CPS 1 is specific for long-chain fatty acyl-CoA and very likely occurs on at least one of the essential cysteine residues inhibiting the catalytic activity of CPS 1. Inhibition of CPS 1 by long-chain fatty acyl-CoAs could reduce amino acid degradation and urea secretion, thereby contributing to nitrogen sparing during starvation.
Subject(s)
Carbamoyl-Phosphate Synthase (Ammonia)/metabolism , Fatty Acids/metabolism , Mitochondria/enzymology , Acylation , Animals , Binding Sites , Carbamoyl-Phosphate Synthase (Ammonia)/antagonists & inhibitors , Carbamoyl-Phosphate Synthase (Ammonia)/isolation & purification , Chromatography, Thin Layer , Ethylmaleimide/pharmacology , Hydroxylamine/pharmacology , Kinetics , Liver/drug effects , Liver/enzymology , Liver/metabolism , Male , Palmitoyl Coenzyme A/metabolism , Rats , Rats, Sprague-Dawley , Submitochondrial Particles/enzymology , Submitochondrial Particles/metabolism , Substrate SpecificityABSTRACT
In the liver, malonyl-CoA is central to many cellular processes, including both fatty acid biosynthesis and oxidation. Malonyl-CoA decarboxylase (MCD) is involved in the control of cellular malonyl-CoA levels, and functions to decarboxylate malonyl-CoA to acetyl-CoA. MCD may play an essential role in regulating energy utilization in the liver by regulating malonyl-CoA levels in response to various nutritional or pathological states. The purpose of the present study was to investigate the role of liver MCD in the regulation of fatty acid oxidation in situations where lipid metabolism is altered. A single MCD enzyme of molecular mass 50.7 kDa was purified from rat liver using a sequential column chromatography procedure and the cDNA was subsequently cloned and sequenced. The liver MCD cDNA was identical to rat pancreatic beta-cell MCD cDNA, and contained two potential translational start sites, producing proteins of 50.7 kDa and 54.7 kDa. Western blot analysis using polyclonal antibodies generated against rat liver MCD showed that the 50.7 kDa isoform of MCD is most abundant in heart and liver, and of relatively low abundance in skeletal muscle (despite elevated MCD transcript levels in skeletal muscle). Tissue distribution experiments demonstrated that the pancreas is the only rat tissue so far identified that contains both the 50.7 kDa and 54. 7 kDa isoforms of MCD. In addition, transfection of the full-length rat liver MCD cDNA into COS cells produced two isoforms of MCD. This indicated either that both initiating methionines are functionally active, generating two proteins, or that the 54.7 kDa isoform is the only MCD protein translated and removal of the putative mitochondrial targeting pre-sequence generates a protein of approx. 50.7 kDa in size. To address this, we transiently transfected a mutated MCD expression plasmid (second ATG to GCG) into COS-7 cells and performed Western blot analysis using our anti-MCD antibody. Western blot analysis revealed that two isoforms of MCD were still present, demonstrating that the second ATG may not be responsible for translation of the 50.7 kDa isoform of MCD. These data also suggest that the smaller isoform of MCD may originate from intracellular processing. To ascertain the functional role of the 50. 7 kDa isoform of rat liver MCD, we measured liver MCD activity and expression in rats subjected to conditions which are known to alter fatty acid metabolism. The activity of MCD was significantly elevated under conditions in which hepatic fatty acid oxidation is known to increase, such as streptozotocin-induced diabetes or following a 48 h fast. A 2-fold increase in expression was observed in the streptozotocin-diabetic rats compared with control rats. In addition, MCD activity was shown to be enhanced by alkaline phosphatase treatment, suggesting phosphorylation-related control of the enzyme. Taken together, our data demonstrate that rat liver expresses a 50.7 kDa form of MCD which does not originate from the second methionine of the cDNA sequence. This MCD is regulated by at least two mechanisms (only one of which is phosphorylation), and its activity and expression are increased under conditions where fatty acid oxidation increases.
Subject(s)
Carboxy-Lyases/chemistry , Carboxy-Lyases/physiology , Fatty Acids/metabolism , Liver/enzymology , Oxygen/metabolism , Alkaline Phosphatase/pharmacology , Amino Acid Sequence , Animals , Base Sequence , Blood Glucose/metabolism , Blotting, Western , COS Cells , Chromatography, Agarose , Cloning, Molecular , DNA, Complementary/metabolism , Diabetes Mellitus, Experimental/metabolism , Fatty Acids/blood , Food Deprivation , Insulin/blood , Liver/metabolism , Male , Methionine/chemistry , Molecular Sequence Data , Myocardium/metabolism , Phosphorylation , Protein Biosynthesis , Protein Isoforms , Rats , Rats, Sprague-Dawley , Sequence Analysis, DNA , Streptozocin , Tissue Distribution , TransfectionABSTRACT
The serum-derived phospholipid growth factor, lysophosphatidate (LPA), activates cells through the EDG family of G protein-coupled receptors. The present study investigated mechanisms by which dephosphorylation of exogenous LPA by lipid phosphate phosphatase-1 (LPP-1) controls cell signaling. Overexpressing LPP-1 decreased the net specific cell association of LPA with Rat2 fibroblasts by approximately 50% at 37 degrees C when less than 10% of LPA was dephosphorylated. This attenuated cell activation as indicated by diminished responses, including cAMP, Ca(2+), activation of phospholipase D and ERK, DNA synthesis, and cell division. Conversely, decreasing LPP-1 expression increased net LPA association, ERK stimulation, and DNA synthesis. Whereas changing LPP-1 expression did not alter the apparent K(d) and B(max) for LPA binding at 4 degrees C, increasing Ca(2+) from 0 to 50 micrometer increased the K(d) from 40 to 900 nm. Decreasing extracellular Ca(2+) from 1.8 mm to 10 micrometer increased LPA binding by 20-fold, shifting the threshold for ERK activation to the nanomolar range. Hence the Ca(2+) dependence of the apparent K(d) values explains the long-standing discrepancy of why micromolar LPA is often needed to activate cells at physiological Ca(2+) levels. In addition, the work demonstrates that LPP-1 can regulate specific LPA association with cells without significantly depleting bulk LPA concentrations in the extracellular medium. This identifies a novel mechanism for controlling EDG-2 receptor activation.
Subject(s)
Calcium Signaling/physiology , Calcium/pharmacology , Lysophospholipids/pharmacology , Nuclear Proteins/metabolism , Phosphatidate Phosphatase/metabolism , Receptors, Cell Surface , Receptors, G-Protein-Coupled , Signal Transduction/physiology , Transcription Factors/metabolism , Animals , Calcium/metabolism , Cell Line , Cyclic AMP/metabolism , Fibroblasts , Green Fluorescent Proteins , Kinetics , Luminescent Proteins/analysis , Lysophospholipids/pharmacokinetics , Models, Biological , Oligodeoxyribonucleotides, Antisense/pharmacology , Phosphatidate Phosphatase/genetics , Phosphorylation , Rats , Receptors, Lysophosphatidic Acid , Recombinant Fusion Proteins/metabolism , Signal Transduction/drug effects , Transfection , Zinc FingersABSTRACT
Mammalian lipid phosphate phosphatases (LPPs, or Type 2 phosphatidate phosphohydrolases) constitute a family of enzymes that belongs to a phosphatase superfamily. The LPPs dephosphorylate a variety of bioactive lipid phosphates including phosphatidate, lysophosphatidate, sphingosine 1-phosphate, and ceramide 1-phosphate. Mouse LPP-1 was stably expressed in rat2 fibroblasts to determine its structural and functional properties. Transduced cells showed increased dephosphorylation of exogenous lysophosphatidate. This result is compatible with mutational studies that show the active site of LPP-1 to be located on the external surface of the plasma membrane. Elevated LPP-1 activity attenuated the ability of lysophosphatidate to stimulate mitogen-activated protein kinase (ERK1 and 2) activities and DNA synthesis. It is concluded that one function of LPP-1 is to dephosphorylate exogenous lysophosphatidate, thereby attenuating cell signaling through endothelial cell differentiation gene (EDG) receptors.
Subject(s)
Lysophospholipids/metabolism , Phosphatidate Phosphatase/metabolism , Signal Transduction , Amino Acid Sequence , Animals , Binding Sites , Cell Line , DNA Replication , Enzyme Activation , Mice , Mitogen-Activated Protein Kinases/metabolism , Molecular Sequence Data , Phosphatidate Phosphatase/chemistry , Phosphorylation , RatsABSTRACT
Apolipoprotein B (apoB) is an essential component of chylomicrons, very low density lipoproteins, and low density lipoproteins. ApoB is a palmitoylated protein. To investigate the role of palmitoylation in lipoprotein function, a palmitoylation site was mapped to Cys-1085 and removed by mutagenesis. Secreted lipoprotein particles formed by nonpalmitoylated apoB were smaller and denser and failed to assemble a proper hydrophobic core. Indeed, the relative concentrations of nonpolar lipids were three to four times lower in lipoprotein particles containing mutant apoB compared with those containing wild-type apoB, whereas levels of polar lipids isolated from wild-type or mutant apoB lipoprotein particles appeared identical. Palmitoylation localized apoB to large vesicular structures corresponding to a subcompartment of the endoplasmic reticulum, where addition of neutral lipids was postulated to occur. In contrast, nonpalmitoylated apoB was concentrated in a dense perinuclear area corresponding to the Golgi compartment. The involvement of palmitoylation as a structural requirement for proper assembly of the hydrophobic core of the lipoprotein particle and its intracellular sorting represent novel roles for this posttranslational modification.
Subject(s)
Apolipoproteins B/chemistry , Apolipoproteins B/metabolism , Cholesterol Esters/metabolism , Palmitic Acid/metabolism , Protein Processing, Post-Translational , Triglycerides/metabolism , Animals , Apolipoproteins B/genetics , Biological Transport , Chromatography, Thin Layer , Cysteine/genetics , Cysteine/metabolism , Endoplasmic Reticulum/metabolism , Fluorescent Antibody Technique, Indirect , Golgi Apparatus/metabolism , Humans , Hydroxylamine/metabolism , Lipids/analysis , Lipoproteins, LDL/chemistry , Lipoproteins, LDL/metabolism , Mutagenesis, Site-Directed , Rats , Sequence Deletion/genetics , Structure-Activity Relationship , Transfection , Tumor Cells, CulturedABSTRACT
Lipid phosphate phosphatase-1 (LPP-1) dephosphorylates exogenous lysophosphatidate and thereby regulates the activation of lysophosphatidate receptors and cell division. Mutation of seven amino acids in three conserved domains of mouse LPP-1 abolished its activity. A glycosylation site was demonstrated between conserved Domains 1 and 2. LPP-1 is expressed in the plasma membrane, and the present results demonstrate the active site to be located on the outer surface.
Subject(s)
Lysophospholipids/metabolism , Phosphatidate Phosphatase/metabolism , Amino Acid Sequence , Animals , Catalytic Domain , Cell Membrane/enzymology , Cells, Cultured , Conserved Sequence , Fibroblasts/cytology , Glycosylation , Membrane Proteins , Mice , Models, Molecular , Molecular Sequence Data , Mutagenesis, Site-Directed , Phosphatidate Phosphatase/genetics , Precipitin Tests , Protein Processing, Post-Translational , RatsABSTRACT
Several membrane-associating signals, including covalently linked fatty acids, are found in various combinations at the N termini of signaling proteins. The function of these combinations was investigated by appending fatty acylated N-terminal sequences to green fluorescent protein (GFP). Myristoylated plus mono/dipalmitoylated GFP chimeras and a GFP chimera containing a myristoylated plus a polybasic domain were localized similarly to the plasma membrane and endosomal vesicles, but not to the nucleus. Myristoylated, nonpalmitoylated mutant chimeric GFPs were localized to intracellular membranes, including endosomes and the endoplasmic reticulum, and were absent from the plasma membrane, the Golgi, and the nucleus. Dually palmitoylated GFP was localized to the plasma membrane and the Golgi region, but it was not detected in endosomes. Nonacylated GFP chimeras, as well as GFP, showed cytosolic and nuclear distribution. Our results demonstrate that myristoylation is sufficient to exclude GFP from the nucleus and associate with intracellular membranes, but plasma membrane localization requires a second signal, namely palmitoylation or a polybasic domain. The similarity in localization conferred by the various myristoylated and palmitoylated/polybasic sequences suggests that biophysical properties of acylated sequences and biological membranes are key determinants in proper membrane selection. However, dual palmitoylation in the absence of myristoylation conferred significant differences in localization, suggesting that multiple palmitoylation sites and/or enzymes may exist.
Subject(s)
Cell Membrane/chemistry , Fatty Acids/chemistry , Intracellular Membranes/chemistry , Acylation , Animals , COS Cells , Calcium-Binding Proteins/metabolism , Calreticulin , Endoplasmic Reticulum/metabolism , Fluorescent Antibody Technique , GTP-Binding Proteins/metabolism , Golgi Apparatus/metabolism , Green Fluorescent Proteins , Luminescent Proteins/metabolism , Microscopy, Fluorescence , Mutation , Myristic Acid/chemistry , Palmitic Acids/chemistry , Phosphorylation , Protein-Tyrosine Kinases/metabolism , Recombinant Fusion Proteins/metabolism , Ribonucleoproteins/metabolismABSTRACT
Lipid phosphate phosphohydrolase (LPP)-1 cDNA was cloned from a rat liver cDNA library. It codes for a 32-kDa protein that shares 87 and 82% amino acid sequence identities with putative products of murine and human LPP-1 cDNAs, respectively. Membrane fractions of rat2 fibroblasts that stably expressed mouse or rat LPP-1 exhibited 3.1-3. 6-fold higher specific activities for phosphatidate dephosphorylation compared with vector controls. Increases in the dephosphorylation of lysophosphatidate, ceramide 1-phosphate, sphingosine 1-phosphate and diacylglycerol pyrophosphate were similar to those for phosphatidate. Rat2 fibroblasts expressing mouse LPP-1 cDNA showed 1.6-2.3-fold increases in the hydrolysis of exogenous lysophosphatidate, phosphatidate and ceramide 1-phosphate compared with vector control cells. Recombinant LPP-1 was located partially in plasma membranes with its C-terminus on the cytosolic surface. Lysophosphatidate dephosphorylation was inhibited by extracellular Ca2+ and this inhibition was diminished by extracellular Mg2+. Changing intracellular Ca2+ concentrations did not alter exogenous lysophosphatidate dephosphorylation significantly. Permeabilized fibroblasts showed relatively little latency for the dephosphorylation of exogenous lysophosphatidate. LPP-1 expression decreased the activation of mitogen-activated protein kinase and DNA synthesis by exogenous lysophosphatidate. The product of LPP-1 cDNA is concluded to act partly to degrade exogenous lysophosphatidate and thereby regulate its effects on cell signalling.
