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2. Conformation of a tetradecapeptide epitope of myelin basic protein.

Author

Mendz GL, Barden JA, and Martenson RE

Subjects
Amino Acid Sequence, Animals, Carbon Isotopes, Magnetic Resonance Spectroscopy, Molecular Sequence Data, Myelin Basic Protein immunology, Protein Conformation, Rabbits, Epitopes chemistry, Myelin Basic Protein chemistry
Abstract

The peptide AcAla-Ser-Gln-Lys-Arg-Pro-Ser-Gln-Arg-His-Gly-Ser-Lys-Tyr, which comprises the first 14 residues of the acetylated N-terminus of myelin basic protein, is an epitopic site for two monoclonal antibodies to the human protein. The conformations of the tetradecapeptide in aqueous solutions were investigated employing high-resolution 1H- and 13C-NMR spectroscopy. Two-dimensional techniques were used to assign the spectra observed from both nuclei. Nuclear-Overhauser-effect data, amide proton temperature coefficients, 13C spin-lattice relaxation times, distance geometry calculations and dynamic simulated annealing provided evidence that the solution conformations of the tetradecapeptide included a nascent alpha-helix in the N-terminal segment, and a loop extending from Ser7 to Ser12 that bring His10 and Tyr14 into close proximity.

Published
1995
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3. Photoaffinity labeling of the dopamine reuptake carrier protein with 3-azido[3H]GBR-12935.

Author

Berger SP, Martenson RE, Laing P, Thurkauf A, Decosta B, Rice KC, and Paul SM

Subjects
Animals, Corpus Striatum metabolism, Corpus Striatum ultrastructure, Dopamine Plasma Membrane Transport Proteins, Glycoproteins metabolism, Kinetics, Light, Male, Membranes metabolism, Molecular Weight, Protein Binding, Rats, Rats, Inbred Strains, Tritium, Affinity Labels, Azides metabolism, Carrier Proteins metabolism, Membrane Glycoproteins, Membrane Transport Proteins, Nerve Tissue Proteins, Piperazines metabolism
Abstract

A high affinity tritiated azido-diphenylpiperazine derivative, 3-azido[3H]GBR-12935, was synthesized as a potential photoaffinity probe of the dopamine transporter. Initially, the reversible binding of 3-azido[3H]GBR-12935 to crude synaptosomal membranes from the rat striatum was characterized. Specific binding was sodium dependent and inhibited by a variety of drugs that are known to potently inhibit dopamine uptake. Other neurotransmitter uptake inhibitors, as well as cis-flupenthixol, a potent inhibitor of [3H]GBR-12935 binding to piperazine binding sites, failed to inhibit specific binding at concentrations of less than or equal to 10 microM. A good correlation was observed between the relative potencies of these drugs in inhibiting dopamine uptake into synaptosomes and in inhibiting specific 3-azido[3H]GBR-12935 binding to rat striatal membranes (r = 0.95, p less than 0.01). These data suggest that 3-azido[3H]GBR-12935, like other diphenylpiperazines such as [3H]GBR-12935 and [3H]GBR-12909, binds primarily to the dopamine transporter under defined assay conditions. After UV photolysis of crude synaptosomal membranes preincubated with 3-azido[3H]GBR-12935 (1-2 nM), a single radiolabeled polypeptide with an apparent molecular mass of 80 kDa was observed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and fluorography. Photoincorporation of 3-azido[3H]GBR-12935 into this polypeptide was inhibited selectively by compounds that inhibit the uptake of dopamine (but not other biogenic amines) and was completely dependent on the presence of Na+. No photolabeled proteins were observed when cerebellar membranes were substituted for striatal membranes. Essentially complete adsorption of the radiolabeled 80-kDa polypeptide to wheat germ agglutinin and elution with N-acetyl-D-glucosamine strongly suggest that the dopamine transporter polypeptide photolabeled by 3-azido[3H]GBR-12935 is glycosylated.

Published
1991

4. Interactions of myelin basic protein with mixed dodecylphosphocholine/palmitoyllysophosphatidic acid micelles.

Author

Mendz GL, Brown LR, and Martenson RE

Subjects
Animals, Chemical Phenomena, Chemistry, Physical, Circular Dichroism, Detergents, Humans, Magnetic Resonance Spectroscopy, Phosphorylcholine metabolism, Protein Conformation, Choline analogs & derivatives, Colloids, Lysophospholipids metabolism, Micelles, Myelin Basic Protein metabolism, Phosphorylcholine analogs & derivatives
Abstract

The interactions of myelin basic protein and peptides derived from it with detergent micelles of lysophosphatidylglycerol, lysophosphatidylserine, palmitoyllysophosphatidic acid, and sodium lauryl sulfate, and with mixed micelles of the neutral detergent dodecylphosphocholine and the negatively charged detergent palmitoyllysophosphatidic acid, were investigated by 1H NMR spectroscopy and circular dichroic spectropolarimetry. The results with single detergents suggested that there are discrete interaction sites in the protein molecule for neutral and anionic detergent micelles and that at least some of these sites are different for each type of detergent. The data on the binding of the protein and peptides to mixed detergent micelles suggested that intramolecular interactions in the intact protein and in one of the longer peptides limited the formation of helices and also that a balance between hydrophobic and ionic forces is achieved in the interactions of the peptides with the detergents. At high detergent/protein molar ratios, hydrophobic interactions appeared to be favored.

Published
1990
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5. Identification of multiple in vivo phosphorylation sites in rabbit myelin basic protein.

Author

Martenson RE, Law MJ, and Deibler GE

Subjects
Amino Acid Sequence, Animals, Brain Chemistry, Chromatography, Thin Layer, Electrophoresis, Polyacrylamide Gel, Peptide Fragments analysis, Phosphorylation, Rabbits, Trypsin metabolism, Myelin Basic Protein metabolism
Abstract

Myelin basic protein of rabbit brain (Mr = 18,200) was initially freed of the bulk of the nonphosphorylated species (mainly component 1) by Cm-cellulose chromatography at high pH. The remainder of the protein was subjected to peptic digestion at pH 6.00, which resulted in specific, essentially complete cleavage at several bonds (Phe-44--Phe-45, Phe-87--Phe-88, Leu-109--Ser-110, and Leu-151--Phe-152) and partial cleavage at the Tyr-14--Leu-15 bond. Gel filtration of the digest through Sephadex G-25 (fine) yielded three fractions, the first containing primarily peptides 1-44 and 45-87, the second peptides 15-44, 88-109, and 110-151, and the third peptides 1-14 and 152-168. Each fraction was chromatographed on Cm-cellulose at pH 8.2, and the resulting subfractions and partially purified peptides were analyzed for phosphoserine and phosphothreonine. Materials containing significant amounts of the phosphoamino acids were subsequently chromatographed on Cm-cellulose at pH 4.65, and the analyses for phosphoserine and phosphothreonine were repeated. The resulting purified peptic phosphopeptides were identified by amino acid analysis and tryptic peptide mapping. Comparison of the maps with those of the unphosphorylated counterparts located the tryptic phosphopeptides. These were recovered and their identities were established by amino acid analysis. In those cases where the phosphopeptide contained 2 Ser residues, the position of the phosphoserine was established by aminopeptidase M digestion. Five phosphorylation sites were found: Ser-7, Ser-56, Thr-96, Ser-113, and Ser-163. Only a small fraction of these sites was phosphorylated in the total basic protein, with values ranging from about 2 (ser-113) to 6% (Thr-96). With the possible exception of Ser-56, these sites are not the ones that have been reported to be phosphorylated in vitro by cyclic AMP-dependent protein kinase.

Published
1983

6. Interaction of myelin basic protein with micelles of dodecylphosphocholine.

Author

Mendz GL, Moore WJ, Brown LR, and Martenson RE

Subjects
Animals, Circular Dichroism, Histidine, Hydrogen-Ion Concentration, Magnetic Resonance Spectroscopy, Phosphorylcholine metabolism, Protein Conformation, Rabbits, Spin Labels, Tyrosine, Choline analogs & derivatives, Colloids, Micelles, Myelin Basic Protein metabolism, Phosphorylcholine analogs & derivatives
Abstract

Interactions of myelin basic protein (MBP) and peptides derived from it with micelles of dodecylphosphocholine (DPC) and perdeuterated DPC have been studied by proton nuclear magnetic resonance (NMR) at 400 MHz and by circular dichroism (CD). When MBP binds to DPC micelles, it acquires about 18% alpha-helicity. The CD spectra of various peptides derived by cleavage of MBP indicate that a major alpha-helical region occurs in residues 85-99 just before the sequence of three prolyl residues 100-102. From line broadenings by fatty acid spin-labels in the micelles and from changes in chemical shifts, the NMR data identify specific residues in MBP that participate in lipid binding. One such sequence is an alpha-helical region from residues 85 to 95, and others occur around methionine-21 and between residues 117 and 135. The different effects of C5, C12, and C16 spin-labels suggest that some segments of the protein may penetrate beyond the dipolar interfacial region of the micelles into the hydrophobic interior, but no part of the protein is protected by the micelles against rapid exchange of its amide groups with the aqueous environment. Even at a lipid to protein molar ratio of 200/1, most NMR resonances from side chains of amino acid residues are not appreciably broadened, suggesting that much of the polypeptide remains highly mobile.

Published
1984
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7. Evidence for multiple human T cell recognition sites on myelin basic protein.

Author

Richert JR, Robinson ED, Deibler GE, Martenson RE, Dragovic LJ, and Kies MW

Subjects
Amino Acid Sequence, Animals, Cattle, Chickens, Clone Cells analysis, Clone Cells immunology, Guinea Pigs, Humans, Molecular Sequence Data, Myelin Basic Protein genetics, Myelin Basic Protein isolation & purification, Protein Conformation, Rabbits, Sequence Homology, Nucleic Acid, Species Specificity, T-Lymphocytes immunology, Lymphocyte Activation, Myelin Basic Protein immunology, T-Lymphocytes analysis
Abstract

Myelin basic protein (BP)-specific T cell clones were used to study human T cell recognition sites on the BP molecule. Proliferation assays performed with a panel of xenogeneic BPs of known amino acid sequence and with large peptide fragments of human and guinea pig BPs demonstrated ten different patterns of reactivity. The data provide evidence for at least four different human T cell epitopes within the C-terminal half of the BP molecule, three within the N-terminal half, and three located within the central portion of the molecule. The results indicate that attempts to inhibit anti-BP responses in vivo in an antigen-specific manner will require the suppression of multiple T cell populations.

Published
1989
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8. Experimental allergic encephalomyelitis in the Lewis rat: farther delineation of active sites in guinea pig and bovine myelin basic proteins.

Author

Martenson RE, Nomura K, Levine S, and Sowinski R

Subjects
Amino Acid Sequence, Animals, Binding Sites, Cattle, Encephalomyelitis, Autoimmune, Experimental immunology, Guinea Pigs, Immunization, Passive, Rats, Species Specificity, Structure-Activity Relationship, Encephalomyelitis, Autoimmune, Experimental etiology, Myelin Basic Protein immunology, Myelin Basic Protein pharmacology
Abstract

Highly encephalitogenic peptide (37-88), derived from the guinea pig myelin basic protein by peptic digestion, was treated chemically to destroy its tyrosyl and histidyl residues and enzymatically to remove its C-terminal sequence Val-His-Phe. Neither of the modifications resulted in loss of activity in Lewis rats. The enccephalitogenic region within peptide (37-88) was located by examination of derivative peptides obtained by selective proteolytic cleavage. The results showed that peptide (61-88), like peptide (43-88), was fully active at the level of 0.02 nmole whereas peptides (72-88) and (72-84) were fully active at levels of 0.5 and 2.5 nmole, respectively. In contrast, peptides (43-71) and (75-88) were completely inactive. These results demonstrated that the undecapeptide Gln-Lys-Ser-Gln-Arg-Ser-Gln-Asp-Glu-Asn-Pro (residues 72-84), although not as encephalitogenic as peptides (43-88) or (61-88), does contain the elements essential for the induction of disease. At the levels tested (10.8 and 2.2 nmole) only peptides (43-88) and (61-88) were capable of inhibiting the induciton of disease by passively transferred lymph node cells; this inhibition, however, was less than that achieved by the intact guinea pig basic protein. Further studies on the encephalitogenicity of the bovine basic protein in Lewis rats demonstrated that the active site in the C-terminal half of this protein is present in its entirety within residues 89 to 115.

Published
1977

9. Cleavage of rabbit myelin basic protein by pepsin.

Author

Martenson RE, Lüthy V, and Deibler GE

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Cattle, Chemical Phenomena, Chemistry, Chromatography, Gel, Chromatography, Ion Exchange, Guinea Pigs, Hydrogen-Ion Concentration, Peptides analysis, Rabbits, Trypsin metabolism, Myelin Basic Protein, Pepsin A
Abstract

Rapid cleavage of bovine and guinea pig myelin basic proteins by pepsin at pH 6.0 is limited to the Phe-Phe bond in the middle of the molecule. In the rabbit protein, however, rapid cleavages occur elsewhere in addition to the Phe87-Phe88 bond in regions in which there are amino acid substitutions. Rapid cleavage occurs at the Leu151-Phe152 bond, at which Ile-151 has been replaced by Leu, the residue that actually contributes the scissile bond. Rapid cleavages occur at the Phe44-Phe45 and Leu109-Ser110 bonds, which in the bovine and guinea pig proteins are relatively resistant under the experimental conditions (pH 6.0). The increased susceptibility of these bonds in the rabbit protein appears to be related to the replacement of Gly-46 by Ser and the change in the sequence immediately NH2-terminal to Leu-109, from Leu-Ser to Thr-Val. These cleavages of the rabbit protein at the four very susceptible bonds have permitted us to isolate peptides (1-44), (45-87), (88-109), (110-151), and (152-168) in high yield. We have also isolated peptides (88-151), (1-14), and (15-44) in low yield; the latter two result from limited cleavage at the relatively resistant Tyr14-Leu15 bond. Peptide (88-109) has been chromatographically resolved into species differing in the degree of methylation of Arg-105; this resolution is thought to result from differences in hydrogen bonding ability of the guanidinium groups.

Published
1981
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10. Treatment of an encephalitogenic peptide from guinea pig myelin basic protein with alpha-protease and thermolysin. Isolation of fragments and determination of cleavage sites.

Author

Nomura K, Martenson RE, and Deibler GE

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Guinea Pigs, Kinetics, Peptide Fragments analysis, Rats, Rats, Inbred Lew, Myelin Basic Protein, Myelin Sheath analysis, Peptide Hydrolases, Thermolysin
Abstract

Two peptic fragments (residues 37-88 and 43-88) of guinea pig myelin basic protein which are capable of inducing experimental allergic encephalomyelitis in Lewis rats were cleaved to shorter fragments with alpha-protease (Crotalus atrox proteinase, EC 3.4.24.1) and thermolysin (EC 3.4.24.4). The fragments were isolated, purified, and identified by amino acid composition and NH2- and COOH-terminal residues. The time courses of the reactions, monitored by thin layer electrophoresis of the digests, showed that alpha-protease cleaves peptide (43-88) initially at the Pro(71)-Gln(72) bond, and that the product peptides are subsequently attacked at the Arg(63) -Thr(64), Ser(74)-Gln(75), Arg(78)-Ser(79), and Ser(76)-Gln(80) bonds. No significant cleavages occurred at the -Leu, -Val, and -Ala bonds. These results are in striking contrast to those obtained previously by others workers with other peptide substrates, where selective cleavage at hydrophobic residues occurred. Thermolysin was found to attack peptide (37-88) at the Phe(42)-Phe(43) bond very rapidly; the product peptides were subsequently attacked at the His(60)-Ala(61), Ser(38)-Ile(39)-Tyr(67)-Gly(68), and Pro(84)-Val(85) bonds. These cleavages are compatible with the known specificity of this enzyme. Several of the fragments prepared with these two enzymes, peptides (43-71), (61-88), (75-88), and (72-84) have been used in other studies to locate the encephalitogenic site in the parent peptic peptide.

Published
1977

11. Cleavage of rabbit myelin basic protein by plasmin: isolation and identification of the major products.

Author

Law MJ, Deibler GE, Martenson RE, and Krutzsch HC

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Chromatography, Gel, Chromatography, Ion Exchange, Electrophoresis, Polyacrylamide Gel, Peptide Fragments analysis, Peptide Fragments isolation & purification, Rabbits, Time Factors, Fibrinolysin metabolism, Myelin Basic Protein metabolism
Abstract

Rabbit myelin basic protein (BP) was subjected to partial cleavage with plasmin, and 15 cleavage products were isolated by a combination of gel filtration and ion-exchange chromatography. Their identification was achieved by amino acid analysis and tryptic peptide mapping, supplemented in some instances by carboxy-terminal analyses with carboxypeptidases A, B, and Y and amino-terminal analyses with dipeptidyl aminopeptidase I. The results showed that major plasmic cleavage sites included the Lys89-Asn90, Lys133-Ser134, and Lys153-Leu154 bonds. Cleavages also occurred at the Arg31-His32, Lys53-Arg54, and Arg25-His26 bonds, but these appeared to be less extensive. A large number of additional peptides were produced in relatively low yield. The smaller of these were isolated from heterogeneous fractions by high-voltage electrophoresis-TLC. Amino acid analysis of these peptides showed that minor cleavage sites included the Arg9-His10, Lys13-Tyr14, Lys103-Gly104, Lys137-Gly138, Lys140-Gly141, and Arg160-Ser161 bonds. In spite of a lower selectivity toward peptide bonds in BP as compared with pepsin, cathepsin D, and thrombin, plasmin has the advantage over the former proteinases in that it does not cleave at or near the Phe44-Phe45 bond. Instead it cleaves at the Arg31-His32 and Lys53-Arg54 bonds, thus preserving the entire hydrophobic sequence Ile-Leu-Asp-Ser-Ile-Gly-Arg-Phe-Phe as well as short sequences to either side.

Published
1985
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12. Myelin basic protein is an endogenous inhibitor of the high-affinity cannabinoid binding site in brain.

Author

Nye JS, Voglmaier S, Martenson RE, and Snyder SH

Subjects
Amino Acids analysis, Animals, Binding Sites drug effects, Brain drug effects, Brain Chemistry, Chromatography, Gel, Dronabinol metabolism, Electrophoresis, Polyacrylamide Gel, Male, Molecular Weight, Myelin Basic Protein isolation & purification, Rabbits, Rats, Rats, Inbred Strains, Swine, Brain metabolism, Cannabinoids metabolism, Dronabinol analogs & derivatives, Myelin Basic Protein pharmacology
Abstract

Radioligand binding studies with the water-soluble cannabinoid [3H]5'-trimethylammonium delta 8-tetrahydrocannabinol ([3H]TMA) have revealed a saturable high-affinity site in brain that is specific for cannabinoids. To determine whether endogenous compounds of brain might act upon the site physiologically, we sought inhibitors in extracts of brain. An endogenous inhibitor has been purified to homogeneity by acid extraction of rat brain followed by adsorption to a reverse-phase matrix and gel filtration chromatography. The purified inhibitor has a subunit molecular mass of 14,500 daltons by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE). Inhibition of [3H]TMA binding by the purified inhibitor occurs with a Ki of about 4 nM in a noncompetitive manner. The molecular weight, abundance, and extraction properties are the same as a species of myelin basic protein (MBP). The MBPs of rat, rabbit, pig, and cow also inhibit [3H]TMA binding noncompetitively with similar potencies. The purified inhibitor comigrates with rat MBP-small form on SDS-PAGE, has a similar amino acid composition, and is recognized by antibody directed against MBP. Studies of fragments of rabbit MBP suggest that the determinants of affinity for the [3H]TMA site are contained primarily within the C-terminal half of the rabbit MBP. Synthetic polycationic peptides such as polylysine and polyarginine mimic the effects of MBP, suggesting that the high-affinity cannabinoid binding site recognizes large polycations. The identification of the endogenous inhibitor of [3H]TMA binding as MBP suggests that MBP interacts physiologically with the high-affinity cannabinoid site.

Published
1988
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13. Low-ultraviolet circular dichroism spectroscopy of sequential peptides 1-63, 64-95, 96-128, and 129-168 derived from myelin basic protein of rabbit.

Author

Martenson RE, Park JY, and Stone AL

Subjects
Amino Acid Sequence, Animals, Circular Dichroism, Protein Conformation, Rabbits, Trifluoroethanol, Myelin Basic Protein isolation & purification, Peptide Fragments isolation & purification
Abstract

Four sequential peptides (sequences 1-63, 64-95, 96-128, and 129-168) derived from rabbit myelin basic protein by thrombic cleavage were examined by low-ultraviolet circular dichroism spectroscopy in 0.5 mM tris(hydroxymethyl)aminomethane hydrochloride (pH approximately 7.2) containing 0-92% trifluoroethanol (TFE). In the absence of the alcohol, all of the peptides contained a significant amount (17-29%) of beta-structure. In the presence of relatively low concentrations (up to 30%) of TFE, all of the peptides except 96-128 adopted considerable alpha-helix (16-33%). This involved a transition from the beta-structure in peptide 1-63 and transitions from the nonordered structure in peptides 1-63, 64-95, and 129-168. Furthermore, additional alpha-helix formed in peptide 1-63 between 30% and 92% TFE at the expense of nonordered structure, whereas the alpha-helix formation above 50% TFE in peptide 129-168 resulted largely from a beta-structure----alpha-helix transition. With the exception of the 129-168 peptide, approximately 65-100% of the maximum level of beta-structure persisted throughout the entire range of TFE concentration. In the case of peptide 129-168, however, most of the beta-structure was converted to alpha-helix and nonordered structure at 75% TFE. While the present results support our previous assignments of beta-structure- and alpha-helix-forming regions to specific amino acid sequences of the basic protein, they also demonstrate that the beta-structure----alpha-helix transitions evidenced at various concentrations of TFE were influenced to a considerable degree by the length of the peptide, presumably due to the presence or absence of interactions between noncontiguous portions of the myelin basic protein polypeptide chain.

Published
1985
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14. Characterization of a novel monoclonal anti-myelin basic protein antibody: use in immunoblotting and immunohistochemical studies.

Author

Bansal G, Martenson RE, Leveille P, and Campagnoni AT

Subjects
Animals, Brain Chemistry, Cattle, Electrophoresis, Polyacrylamide Gel, Epitopes immunology, Guinea Pigs, Haplorhini, Humans, Immunologic Techniques, Mice, Myelin Basic Protein immunology, Peptide Fragments analysis, Rabbits, Rats, Species Specificity, Swine, Antibodies, Monoclonal isolation & purification, Myelin Basic Protein analysis
Abstract

Monoclonal antibodies (MAbs) to the myelin basic protein (MBP) were produced in CAF1 (BALB/c x A/J) mice immunized with intact bovine MBP. A number of MAbs were obtained, one of which was characterized in detail with respect to its isotype, antigenic determinant on the MBP, the spectrum of antigens with which it reacted in mouse brain, and its immunohistochemical staining characteristics. This monoclonal, GB-1 (an IgG1), recognized an epitope within residues 30-51 of bovine MBP. It also reacted with a family of MBP-related proteins present in brain homogenates of mice from 7-35 days. Immunohistochemically, GB-1 stained myelinated fibers and oligodendrocytes in the rodent CNS. A second monoclonal (GB-2, and IgM) was partially characterized. It reacted with intact MBP when it was immobilized to plastic or nitrocellulose, but it was not found to be useful for immunoblots or immunohistochemistry.

Published
1987
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15. Comparative studies of guinea pig and bovine myelin basic proteins. Partial characterization of chemically derived fragments and their encephalitogenic activities in Lewis rats.

Author

Martenson RE, Deibler GE, Kramer AJ, and Levine S

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Cattle, Encephalomyelitis, Autoimmune, Experimental chemically induced, Guinea Pigs, Oxidation-Reduction, Peptide Fragments analysis, Rats, Rats, Inbred Lew, Species Specificity, Myelin Basic Protein isolation & purification, Myelin Basic Protein metabolism, Myelin Sheath analysis
Published
1975
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16. Amino acid sequence of porcine myelin basic protein.

Author

Kira J, Deibler GE, Krutzsch HC, and Martenson RE

Subjects
Amino Acid Sequence, Animals, Chromatography, Gel, Peptide Fragments analysis, Swine, Thermolysin metabolism, Trypsin metabolism, Brain Chemistry, Myelin Basic Protein analysis
Abstract

The myelin basic protein (BP) of pig brain was cleaved into its constituent tryptic peptides and the amino acid composition of each was determined. Those tryptic peptides that had not been sequenced previously were cleaved with dipeptidyl peptidases and the resulting dipeptides were trimethylsilated, separated by gas chromatography, and identified by mass spectrometry. Carboxypeptidases B and Y were used to establish the COOH-terminal sequences of some of the tryptic peptides; one tryptic peptide (sequence 76-92) was cleaved with thermolysin and the thermolytic peptides were analyzed. From the results of the present study together with those reported previously, it has been possible to determine the complete amino acid sequence of the protein. The protein consists of 172 residues and has a theoretical molecular weight of 18,604. Its amino acid sequence is identical with that reported for the homologous bovine protein with the following exceptions: Ser replaces (bovine) Ala2; His-Gly is inserted between Arg9 and Ser10; Ala replaces Ser45; His and Gly replace Gly76 and His77, respectively; Pro replaces Ser131 and Ser135; Ala is inserted between Gly142 and His143; and Gln replaces His143.

Published
1985
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17. Methylation of the lysine residues of monellin.

Author

Morris RW, Cagan RH, Martenson RE, and Deibler G

Subjects
Amino Acids analysis, Chemical Phenomena, Chemistry, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Methylation, Peptide Fragments, Taste, Lysine, Plant Proteins chemical synthesis, Sweetening Agents chemical synthesis
Published
1978
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18. Low-ultraviolet circular dichroism spectroscopy of oligopeptides 1-95 and 96-168 derived from myelin basic protein of rabbit.

Author

Stone AL, Park JY, and Martenson RE

Subjects
Amino Acid Sequence, Animals, Brain Chemistry, Circular Dichroism methods, Protein Conformation, Rabbits, Spectrophotometry, Ultraviolet methods, Structure-Activity Relationship, Myelin Basic Protein analysis, Peptide Fragments analysis
Abstract

Myelin basic protein (MBP) is a major protein constituent of the myelin sheath of the central nervous system, where it is believed to have functional alpha-helical segments. One element of the function of the protein might be "conformational adaptability" of specific regions of its amino acid sequence, since the purified protein appears to be largely devoid of ordered structure. To pursue this question, low-ultraviolet circular dichroism (CD) spectroscopy was conducted on the sequential thrombic peptides 1-95 and 96-168 of the protein in the presence of 0-92% trifluoroethanol (TFE), a solvent known to promote stable secondary structures in polypeptides. The series of CD spectra of the oligopeptides were subjected to a computerized best-fit analysis of four peptide conformations, the alpha-helix, beta-structure, beta-turn, and nonordered form. Agreement between experimental and best-fit composite spectra was achieved when standard CD curves of peptide conformations were derived from known theoretical spectra and experimental spectra of polypeptides. In dilute buffer alone, oligopeptides 1-95 and 96-168 evidence no alpha-helix but significant beta-structure (18% and 23%, respectively), as well as a predominant, extended nonordered conformation. However, the two parts of the protein differed in conformational adaptability. From 0% to 30% TFE, 96-168 exhibited concomitant transitions to 10% helix and 32% beta-structure from the nonordered form. In contrast, in 10-30% TFE, 1-95 underwent a transition to approximately 21% helix with partial loss of beta-structure as well as nonordered form; higher concentrations of TFE (40-75%) promoted additional transitions to both helix and beta-structure (totaling 33% and 25%, respectively).(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1985
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19. Human cytotoxic T-cell recognition of a synthetic peptide of myelin basic protein.

Author

Richert JR, Robinson ED, Deibler GE, Martenson RE, Dragovic LJ, and Kies MW

Subjects
Cytotoxicity Tests, Immunologic, Humans, In Vitro Techniques, Myelin Basic Protein chemical synthesis, Epitopes, Myelin Basic Protein immunology, T-Lymphocytes, Cytotoxic immunology
Abstract

Previous studies with a panel of myelin basic protein (MBP)-specific human T-cell clones suggested a clustering of epitopes in the middle and at the C terminus of the molecule. The current study demonstrates that 19 of 40 clones recognize a synthetic peptide corresponding to residues 152 to 170 of the human MBP molecule and that 9 clones recognize a synthetic peptide corresponding to residues 86 to 105. Myelin basic protein-specific cytotoxic activity was restricted to the clones that recognized peptide 152-170, and this peptide served as a preferential cytotoxic T-cell target when attached to an autologous B-cell line. The specificity of MBP-directed cytotoxic activity appears to be much more restricted than the specificity demonstrated for proliferative activity.

Published
1989
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20. Large peptides of bovine and guinea pig myelin basic proteins produced by limited peptic hydrolysis.

Author

Martenson RE, Kramer AJ, and Deibler GE

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Brain Chemistry, Cattle, Chromatography, Gel, Chromatography, Ion Exchange, Electrophoresis, Polyacrylamide Gel, Guinea Pigs, Hydrogen-Ion Concentration, Pepsin A, Peptide Fragments analysis, Species Specificity, Myelin Basic Protein
Abstract

Bovine and guinea pig myelin basic proteins were cleaved with pepsin at pH 3.0 or pH 6.0 (enzyme/substrate, 1:500, w/w), and the peptides were isolated and identified. At pH 3.0 cleavage of the bovine protein occurred principally at three sites: Phe-Phe (88-89), Phe-Phe (42-43), and Leu-Asp (36-37). Minor cleavages occurred at Leu-Ser (110-111), Phe-Ser (113-114), and Ile-Phe (152-153). A study of the time course of the hydrolysis showed that the reaction was biphasic; nearly all of the protein was cleaved at Phe-Phe (88-89) before significant cleavages at other sites occurred. At pH 6.0 cleavage of the bovine protein occurred almost exclusively at a single site, the Phe-Phe bond at position 88-89, resulting in bisection of the protein. Treatment of the guinea pig protein with pepsin under the same conditions resulted in the production of peptides which were identical with those of the bovine protein in chromatographic and electrophoretic properties and in N-terminal and C-terminal residues but which differed slightly in amino acid composition.

Published
1975
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21. The significance of circulating and cell-bound antibodies in experimental allergic encephalomyelitis.

Author

Gonatas NK, Gonatas JO, Stieber A, Lisak R, Suzuki K, and Martenson RE

Subjects
Animals, Antibodies, Anti-Idiotypic, Cell Membrane immunology, Chemical Precipitation, Chromatography, DEAE-Cellulose, Chromatography, Gel, Electrophoresis, Disc, Electrophoresis, Polyacrylamide Gel, Encephalomyelitis, Autoimmune, Experimental blood, Encephalomyelitis, Autoimmune, Experimental pathology, Female, Guinea Pigs immunology, Immunity, Cellular, Iodine Radioisotopes, Lymph Nodes immunology, Lymph Nodes pathology, Male, Microscopy, Electron, Myelin Sheath immunology, Peroxidases, Proteins isolation & purification, Rabbits immunology, Rats, Rats, Inbred BN, Rats, Inbred Lew, Antibodies, Encephalomyelitis, Autoimmune, Experimental immunology
Abstract

Conjugates of horseradish peroxidase with myelin basic protein (BP) of guinea pig or Lewis rat were used to identify antibody-containing cells in draining lymph nodes during experimental allergic encephalomyelitis (EAE). Peroxidase activity was revealed for light and electron microscopic preparations with the diaminobenzidine reaction of Graham and Karnovsky. Basic proteins (BP) were also iodinated with (125)I for determination of circulating antibody against BP by radio-immunoassay of (125)I BP using coprecipitation with antirat IgG or with antirat serum proteins. Encephalitogenicity was lost after conjugation of guinea pig BP or Lewis rat BP with peroxidase, whereas iodination did not affect the encephalitogenicity of guinea pig or Lewis rat BPs. EAE was induced in Lewis rats with guinea pig or Lewis rat spinal cord BPs in complete Freund's adjuvant. Draining lymph nodes were studied by light and electron microscopy during the course of the immune reaction, and cells with specific antibody against BP were identified with the use of BP-horseradish peroxidase conjugates. Lymph node sections from animals immunized with high antigen doses (500 mug) showed numerous plasma cells with intracellular antibody against BP in medullary cords 10 days after immunization and 4 days prior to histologic appearance of EAE. Numbers of positive cells correlated with levels of circulating antibody against BP. Immunization with a low antigen dose (5 mug) resulted in EAE, few or no antibody-containing cells, and significantly lower levels of circulating antibody. Brown Norwegian rats, a strain resistant to EAE, immunized with 500 mug of BP had positive cells in draining lymph nodes and high levels of circulating antibody against BP in the absence of histologic evidence of EAE. Lewis rats injected with Lewis rat small BP failed to develop EAE. Nevertheless, these animals showed levels of circulating antibody and antibody-containing cells similar to those of animals which developed EAE after injection of the mixture of Lewis rat large and small BP. It is concluded that although the BP-peroxidase labeling method reveals cells with specific anti-BP antibody, these cells are probably unrelated to EAE. The lack of correlation between EAE induced by low antigen doses and levels of circulating anti-BP antibody (determined with the use of highly encephalitogenic (125)I-BP) suggests that effector cells can be stimulated at low antigen doses, but higher antigen doses are required to induce the production of levels of circulating antibody detectable by the method of immune coprecipitation.

Published
1974

23. Sites in myelin basic protein that react with monoclonal antibodies.

Author

Hruby S, Alvord EC Jr, Martenson RE, Deibler GE, Hickey WF, and Gonatas NK

Subjects
Amino Acid Sequence, Animals, Cattle, Cerebellar Cortex immunology, Chickens, Guinea Pigs, Haplorhini, Histocytochemistry, Humans, Hybridomas immunology, Immunoenzyme Techniques, Immunoglobulin G immunology, Immunoglobulin M immunology, Mice, Rabbits, Rats, Species Specificity, Structure-Activity Relationship, Tryptophan, Antibodies, Monoclonal immunology, Epitopes immunology, Myelin Basic Protein immunology
Abstract

The epitopes (antigenic sites) for seven monoclonal antibodies (MAbs) evoked in rats or mice by guinea pig or monkey myelin basic protein (BP) have been located in four different sequences of the BPs extracted from various species. Six of the MAbs were evoked by guinea pig BP. (1) One epitope, possibly a pair, is included within residues 1-14 of all BPs tested and reacts with two rat IgG MAbs. (2) A definite pair of overlapping epitopes includes the central Phe91-Phe92 sequence. One epitope is contained entirely within sequence 90-99 and reacts with a rat IgG MAb. The substitution of Ser in chicken BP for Thr97 destroys this epitope. The other epitope appears to include residues on the amino side of Phe44 and even of His32 and suggests some tertiary structure in BP. This epitope reacts with a mouse IgM MAb that does not recognize the chicken substitution. (3) The third epitope lies within residues 114-121, specifically including Trp118, and reacts with a rat IgG MAb. A cross-reacting epitope probably includes residues 44-45 in certain species (guinea pig and bovine but not rabbit). (4) Another pair of epitopes is located within residues 131-140 but is severely species-restricted. This region in guinea pig BP evoked a species-specific mouse IgM MAb. The same region in monkey BP evoked the seventh MAb, a mouse IgG, which reacts with human, chimpanzee, monkey, bovine, and rat-18.5 kDa BPs and to a lesser extent rabbit BP but not with guinea pig, pig, or chicken BPs. Some tertiary structure in guinea pig BP is also suggested by the reactivities with the IgM MAb. All of the MAbs react with myelin in histologic preparations, but the optimum method of preparation of the tissue varies with each.

Published
1985
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25. NMR studies of myelin basic protein. IX. Complete assignments of the tyrosine residues by proton NMR of proteins from six species.

Author

Mendz GL, Moore WJ, and Martenson RE

Subjects
Animals, Cattle, Chickens, Gadolinium, Humans, Hydrogen-Ion Concentration, Magnetic Resonance Spectroscopy, Protein Conformation, Rabbits, Rats, Species Specificity, Swine, Myelin Basic Protein, Tyrosine
Abstract

All the proton resonances from the tyrosine residues are assigned in 400 MHz NMR spectra in aqueous solution of myelin basic proteins from human, cow, pig, rabbit, rat (small protein) and chicken. Assignments are based on species comparisons, spectra of enzymatic cleavage products of the basic protein, pH titrations, broadening effects of Gd(III), and nuclear Overhauser effects. The mobile extended polypeptide chain structure of the protein facilitates the detection of interactions between nearest neighbors. Evidence is found for reverse turns in the structure in regions of encephalitogenic determinants.

Published
1983
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26. Prediction of the secondary structure of myelin basic protein.

Author

Martenson RE

Subjects
Amino Acid Sequence, Circular Dichroism, Models, Chemical, Models, Molecular, Protein Conformation, Myelin Basic Protein
Abstract

An investigation into the probable secondary structure of the myelin basic protein was carried out by the application of three procedures currently in use to predict the secondary structures of proteins from knowledge of their amino acid sequences. In order to increase the accuracy of the predictions, the amino acid substitutions that occur in the basic protein from different species were incorporated into the predictive algorithms. It was possible to locate regions of probable alpha-helix, beta-structure, beta-turn, and unordered conformation (coil) in the protein. One of the predictive methods introduces a bias into the algorithm to maximize or minimize the amounts of alpha-helix and/or beta-structure present; this made it possible to assess how conditions such as pH and protein concentration or the presence of anionic amphiphilic molecules could influence the protein's secondary structure. The predictions made by the three methods were in reasonably good agreement with one another. They were consistent with experimental data, provided that the stabilizing or destabilizing effects of the environment were taken into account. According to the predictions, the extent of possible alpha-helix and beta-structure formation in the protein s severely restricted by the low frequency and extensive scattering of hydrophobic residues, along with a high frequency and extensive scattering of residues that favor the formation of beta-turns and coils. Neither prolyl residues nor cationic residues per se are responsible for the low content of alpha-helix predicted in the protein. The principal ordered conformation predicted is the beta-turn. Many of the predicted beta-turns overlap extensively, involving in some cases up to 10 residues. In some of these structures it is possible for the peptide backbone to oscillate in a sinusoidal manner, generating a flat, pleated sheetlike structure. Cationic residues located in these structures would appear to be ideally oriented for interaction with lipid phosphate groups located at the cytoplasmic surface of the myelin membrane. An analysis of possible and probable conformations that the triproline sequence could assume questions the popular notion that this sequence produces a hairpin turn in the basic protein.

Published
1981
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27. Sequence of guinea pig myelin basic protein.

Author

Deibler GE, Martenson RE, Krutzsch HC, and Kies MW

Subjects
Amino Acid Sequence, Animals, Cattle, Endopeptidases metabolism, Guinea Pigs, Trypsin metabolism, Myelin Basic Protein analysis, Serine Endopeptidases
Abstract

This paper proposes a tentative amino acid sequence of guinea pig myelin basic protein obtained by comparison of peptide fragments of the guinea pig and bovine proteins. Analyses of the tryptic peptides confirmed the known sequence differences in the NH2-terminal half of the molecule and showed that in the COOH-terminal half of the guinea pig protein Ser131 was missing, Ala136 - His137 was deleted, Leu140 was replaced by Phe, and an extra Ala was inserted somewhere within sequence 142-151 (tryptic peptide T23 ). Sequence determination of guinea pig tryptic peptides corresponding to residues 130-134 ( T20 ), 135-138 ( T21 ), and 142-151 ( T23 ) of the bovine protein confirmed the above sequence changes and placed the extra Ala between Gly142 and His143 . The sequence of the region corresponding to bovine residues 130-143 is thus Ala-Asp-Tyr-Lys-Ser-Lys-Gly-Phe-Lys-Gly-Ala-His. No species differences were observed in the amino acid compositions of the remaining tryptic peptides obtained from the COOH-terminal half of the molecule. Based upon these results, the guinea pig basic protein contains 167 amino acid residues and has a molecular weight of 18,256.

Published
1984
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28. Cleavage of rabbit myelin basic protein by thrombin.

Author

Law MJ, Martenson RE, and Deibler GE

Subjects
Amino Acid Sequence, Amino Acids analysis, Animals, Humans, Kinetics, Peptide Fragments analysis, Rabbits, Myelin Basic Protein metabolism, Thrombin metabolism
Abstract

Rabbit myelin basic protein (BP) contains several Arg-X bonds with differing susceptibilities to thrombic cleavage as measured by the yields of the various cleavage products obtained under three different conditions. Under conditions where the thrombin-to-substrate ratio was very low (1 NIH unit/mg BP), the concentration of substrate was relatively low (4 mg BP/ml), and the incubation time was short (2 h), the rabbit BP was cleaved essentially completely and specifically at a single site, the Arg(95)-Thr(96) bond. The BPs of other species (beef, pig, guinea pig, rat) were similarly cleaved, no doubt because all have the same amino acid sequence in this region of the protein. Under conditions in which the enzyme-to-substrate ratio and the substrate concentration were higher (2 NIH units/mg BP, 8 mg BP/ml) and the incubation time was long (24 h), additional, partial cleavages occurred, principally at the Arg(43)-Phe(44) and Arg(128)-Ala(129) bonds, but with some cleavage at the Arg(31)-His(32) and Arg(63)-Thr(64) bonds as well. Under conditions in which all three variables were elevated (5 NIH units/mg peptide, 20 mg peptide/ml, 24 h), more extensive cleavage occurred at the above sites. In peptide (96-168), which we examined in detail, nearly complete cleavage of the Arg(128)-Ala(129) bond occurred, with partial cleavage at the unmethylated Arg(105)-Gly(106), Arg(111)-Phe(112), Arg(150)-Leu(151), and Arg(160)-Ser(161) bonds. The susceptibilities to cleavage of the Arg-X bonds in the BP can be explained with varying degrees of success in terms of the known specificity of thrombin. Cleavage of two of the bonds, Arg(128)-Ala(129) and Arg(160)-Ser(161), suggests the occurrence of a chain reversal or beta-turn in the sequence preceding the scissile bonds. Most cleavages of the BP with thrombin do not occur in the more hydrophobic regions; in particular, the hydrophobic region in the center of the molecule that includes the Phe-Phe(87-88) sequence is left intact.

Published
1984
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29. Conformation of two antigenic regions in myelin basic protein.

Author

Martenson RE, Mendz GL, and Moore WJ

Subjects
Amino Acid Sequence, Animals, Cattle, Gadolinium, Humans, Hydrogen-Ion Concentration, Magnetic Resonance Spectroscopy, Peptide Fragments immunology, Protein Conformation, Rabbits, Species Specificity, Epitopes analysis, Myelin Basic Protein immunology
Abstract

Four different regions of myelin basic protein from various species have been reported to be the antigenic sites (epitopes) for seven monoclonal antibodies evoked in rats or mice by guinea pig or monkey basic protein. The structures of the epitopes located in the amino-terminal region and in the eight-residue sequence including S-133, were examined by proton n. m. r at 400 MHz in aqueous solutions of peptides obtained by enzymatic cleavage of the rabbit protein. The data suggest conformational similarities between the two regions.

Published
1985
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30. Evidence for specific polypeptide chain folding in myelin basic protein from reactions between fragments of the protein and monoclonal antibodies.

Author

Alvord EC Jr, Hruby S, Martenson RE, Deibler GE, and Law MJ

Subjects
Amino Acid Sequence, Animals, Antigens immunology, Binding, Competitive, Chemical Phenomena, Chemistry, Epitopes immunology, Guinea Pigs, Mice, Protein Conformation, Antibodies, Monoclonal immunology, Myelin Basic Protein immunology, Peptide Fragments immunology
Abstract

The specificities of two monoclonal IgM antibodies (18.25 and 21.14.2) evoked in mice with guinea pig myelin basic protein were examined and interpreted in terms of a specific folding of the protein's polypeptide chain. Studies with guinea pig and rabbit myelin basic protein fragments showed that a region encompassing the central Phe-Phe (87-88) sequence is obligatory, but not sufficient, for reactivity with antibody 18.25. Appreciable reactivity was observed for rabbit peptides 22-95 and 45-151, and lower, but significant, reactivity was shown by peptide 32-95. Only very weak reactivity was seen with peptide 44-95. No reactivity was observed with peptide 1-95 after its lysine residues were acetylated, acetamidinated, or guanidinated. These results have been interpreted in terms of a polypeptide chain folding that creates an epitope within sequence Val-Val-His-Phe-Phe-Lys-Asn-Ile-Val (84-92). The specific conformation of this epitope, which includes probably the Lys-89 and possibly the Asn-90 and Val-92 side chains, could be formed by the association of sequence 84-92 with either sequence Ile-Leu-Asp-Ser-Ile-Gly-Arg-Phe-Phe (37-45) or with sequence Val-Leu-Ser-Arg-Phe (108-112) to form beta-sheet structures essentially identical with those that appear to be present in the intact BP [Martenson R.E.J. Neurochem. 46, 1612-1622 (1986)]. The second monoclonal antibody, no. 21.14.2, reacts only with guinea pig myelin basic protein and fragments containing the species-restricted sequence Arg-Ala-Asp-Tyr-Lys-Ser-Lys (129-135).(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1986
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31. A general model of the P2 protein of peripheral nervous system myelin based on secondary structure predictions, tertiary folding principles, and experimental observations.

Author

Martenson RE

Subjects
Amino Acid Sequence, Animals, Cattle, Humans, Models, Molecular, Myelin P2 Protein, Protein Conformation, Rabbits, Species Specificity, Myelin Basic Protein isolation & purification, Myelin Sheath analysis, Peripheral Nerves analysis
Abstract

The amino acid sequence of the P2 protein of peripheral myelin was analyzed with regard to regions of probable alpha-helix, beta-structure, beta-turn, and unordered conformation by means of several algorithms commonly used to predict secondary structure in proteins. Because of the high beta-sheet content and virtual absence of alpha-helix shown by the circular dichroic spectra of the protein, a bias was introduced into the algorithms to favor the beta-structure over the alpha-helical conformation. In order to define those beta-sheet residues that could lie on the external hydrophilic surface of the protein and those that could lie in its hydrophobic interior, the predicted beta-strands were examined for charged and uncharged amino acids located at alternating positions in the sequence. The sequential beta-strands in the predicted secondary structure were then ordered into beta-sheets and aligned according to generally accepted tertiary folding principles and certain chemical properties peculiar to the P2 protein. The general model of the P2 protein that emerged was a "Greek key" beta-barrel, consisting of eight antiparallel beta-strands with a two-stranded ribbon of antiparallel beta-structure emerging from one end. The model has an uncharged, hydrophobic core and a highly hydrophilic surface. The two Cys residues, which form a disulfide, occur in a loop connecting two adjacent antiparallel strands. Two hydrophilic loops, each containing a cluster of acidic residues and a single Phe, protrude from one end of the molecule. The general model is consistent with many of the properties of the actual protein, including the relatively weak nature of its association with myelin lipids and the positions of amino acid substitutions. Alternative beta-strand orderings yield three specific models having different interstrand connections across the barrel ends.

Published
1983
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33. Isolation and identification of large overlapping fragments of rabbit myelin basic protein produced by limited peptic hydrolysis.

Author

Martenson RE, Law MJ, Deibler GE, and Lüthy V

Subjects
Amino Acid Sequence, Animals, Carboxypeptidases, Pepsin A, Peptide Fragments analysis, Rabbits, Trypsin, Myelin Basic Protein
Abstract

Treatment of rabbit myelin basic protein component 1 with pepsin (enzyme:substrate, 1:500 w/w) in 0.5 M-ammonium formate (pH 6.00) for 15-20 min at room temperature resulted in limited cleavage of the protein. The resulting fragments were isolated by ion-exchange chromatography and gel filtration and identified by amino acid and COOH-terminal analyses and by tryptic peptide mapping. All of the possible products resulting from incomplete cleavages at the highly susceptible Phe44-Phe45, Phe87-Phe88, Leu109-Ser110, and Leu151-Phe152 bonds were isolated: peptides (1-151), (1-109), (1-87), (45-168), (45-151), (45-109), (88-168), (88-151), and (110-168). Of these, peptides (1-151), (1-87), and (88-151) were recovered in the greatest yield (0.14-0.19 mol per mol of starting protein). Relatively low yields (0.04 mol/mol starting protein) were obtained for peptides (1-109) and (110-168), indicating that the Leu109-Ser110 bond is somewhat more resistant to peptic cleavage than are the Phe-Phe and Leu-Phe bonds. Smaller fragments of the basic protein were also recovered: peptides (1-44), (1-28), (45-87), (88-109), (110-151), and (152-168). Many of the individual peptides could be readily identified in electrophoretograms of the total peptic digest. The relative electrophoretic mobilities of the above-mentioned peptides, together with the previously isolated peptides (1-14) and (15-44), were determined in 15% (w/w) polyacrylamide slab gels containing 1 M-acetic acid and 8 M-urea.

Published
1981
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34. Monoclonal antibodies reactive with myelin basic protein.

Author

Hruby S, Alvord EC Jr, Groome NP, Dawkes A, and Martenson RE

Subjects
Amino Acid Sequence, Animals, Antibody Specificity, Cattle, Chickens, Enzyme-Linked Immunosorbent Assay, Guinea Pigs, Humans, Rabbits, Species Specificity, Antibodies, Monoclonal immunology, Epitopes analysis, Myelin Basic Protein immunology
Abstract

New monoclonal antibodies (MAbs) to myelin basic protein (BP) reveal epitopes to be in sequences 22-34, 75-82, 83-96, 118-131 and 125-131. Comparison of these results with those previously reported suggest that almost every sequence of about 10 amino acid residues may be sufficiently antigenic to make a single MAb but that certain regions are immunodominant, strong enough to make practically the same MAb repeatedly. One of these new MAbs (clone 3) has especially interesting reactivity, sharply limited to residues 75-82 in bovine and porcine BP: Lys-Ala-Gln-His-Gly-Arg-Pro. Whales presumably have the same sequence, since their BPs are fully reactive with clone 3 MAb, but all other species of BP, with known sequences of BP, have at least two changes in this sequence. Deletion of Lys75 (as in a tryptic peptide of porcine BP) reduces reactivity with the MAb about 10-fold, whereas substitution of Ala76 by Ser (as in all other species of BP) and either deletion of Gln77 (as in human, monkey and rabbit BP) or His78 (as in the guinea pig and rat BP) or substitution of Pro82 by Thr (as in human, monkey, rat and mouse BP) eliminates reactivity. We speculate that woodchuck and prairie dog BPs in this region closely resemble chicken BP, which has about 2% of the original reactivity. However, squirrel BP is unique, probably having only one of the changes in this region of BP, since it possesses 10-20 times the reactivity of chicken BP but still only 20-50% of the original reactivity with clone 3 MAb, a degree of reactivity not seen with any other species of BP.

Published
1987
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36. Reaction of peptide 89-169 of bovine myelin basic protein with 2-(2-nitrophenylsulfenyl)-3-methyl-3'-bromoindolenine.

Author

Martenson RE, Deibler GE, and Kramer AJ

Subjects
Amino Acids analysis, Animals, Bromine, Cattle, Chemical Phenomena, Chemistry, Electrophoresis, Polyacrylamide Gel, Skatole analogs & derivatives, Spectrophotometry, Ultraviolet, Tryptophan analogs & derivatives, Myelin Basic Protein analysis, Peptides analysis, Sulfenic Acids
Abstract

The C-terminal half of the bovine myelin basic protein, peptide 89-169, was treated with BNPS-skatole [2-(2-nitrophenylsulfenyl)-3-methyl-3'-bromoindolenine], and the products were isolated by repeated gel filtration through Sephadex G-50. They consisted of uncleaved peptide 89-169 in which approximately 30% of the tyrosine had been monobrominated and the tryptophan converted to oxindolealanine, peptide 116-169 modified by partial bromination (30%) of the tyrosine, and two chromatographic forms of peptide 89-115. The major form contained the lactone of dioxindolealanine at the C terminus; the minor form contained the uncyclized oxidation product. Each form of peptide 89-115 was resolved into several components by electrophoresis in polyacrylamide gels (10%, w/w) containing 1 M acetic acid and 8 M urea. The presence of three of these components could be explained by partial deamidation of Asn-91 and Gln-102. Studies on the oxidation of tryptophan-containing model peptides by BNPS-skatole indicated that the reaction can also include partial bromination of the dioxindole and its lactone and partial cleavage at the amino peptide bond of the tryptophan.

Published
1977
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37. The use of gel filtration to follow conformational changes in proteins. Conformational flexibility of bovine myelin basic protein.

Author

Martenson RE

Subjects
Animals, Cattle, Chromatography, Gel, Guanidines, Hydrogen-Ion Concentration, Osmolar Concentration, Protein Conformation, Myelin Basic Protein
Abstract

The hydrodynamic behavior of bovine myelin basic protein was studied by gel filtration through Sephadex G-100 under conditions which included variations in pH from 2 to 12, variations in ionic strength from 0.01 to 1.5 M at pH 2 and from 0.1 to 2 M at pH 7, and variations in guanidinium chloride concentration from 0 to 6 M. A number of well characterized compact globular proteins were subjected to the same conditions for comparison. Compact globular proteins showed major conformational transitions due to acid, alkali, and guanidinium chloride denaturation and, possibly, minor transitions as well. Myelin basic protein behaved like a flexible linear polyelectrolyte, expanding continuously between pH 11 and pH 2 to 3 at ionic strength 0.1 M and contracting continuously with increase in ionic strength at pH 2 and at pH 7 to the point of salting-out. Relatively low concentrations of guanidinium chloride (approximately 0.5 M) were sufficient to cause the basic protein to expand. With increasing concentration of the denaturant the molecule continued to expand, but in a noncooperative manner. These results demonstrated the lack of significant intramolecular stabilization in the protein.

Published
1978

38. Myelin basic protein speciation.

Author

Martenson RE

Subjects
Amino Acid Sequence, Animals, Encephalomyelitis, Autoimmune, Experimental immunology, Humans, Myelin Basic Protein immunology, Myelin Basic Protein genetics, Species Specificity
Published
1984

39. Possible hydrophobic region in myelin basic protein consisting of an orthogonally packed beta-sheet.

Author

Martenson RE

Subjects
Amino Acid Sequence, Chemical Phenomena, Chemistry, Physical, Macromolecular Substances, Models, Molecular, Myelin Sheath ultrastructure, Protein Conformation, Myelin Basic Protein
Abstract

Theoretical analysis was carried out to determine how the approximately 20% of beta-structure observed in the 18.5 kilodalton (kDa) myelin basic protein (MBP) could be organized into a relatively stable beta-sheet. The beta-sheet is presumed to consist of the five most hydrophobic segments of polypeptide chain, which have beta-structure potential. These correspond approximately to sequences 15-21, 37-45, 84-92, 106-112, and 148-154 (rabbit MBP sequence numbering) and constitute beta-strands a, b, c, d, and e, respectively. A number of constraints are imposed upon the sheet; e.g., it should have the same topology in all MBP forms (21.5, 18.5, 17, and 14 kDa); strand e should lie at the sheet edge; strands b, c, and d should be ordered sequentially; the sheet formed by strands a, b, c, and d should be antiparallel; a maximum of the nonpolar surface area should be removed from the aqueous milieu; and charged side chains should be solvent-accessible. On the basis of these constraints it is possible to propose six orthogonally packed beta-sheets having different topologies. If strand e is restricted to an antiparallel alignment, the number of different sheets is reduced to four. Each of these sheets can form a relatively compact hydrophobic globular region. Two of the strands (a and e) can undergo transitions to alpha-helix without disrupting the structure of the remaining sheet bcd or producing major topologic rearrangements of the polypeptide chain.

Published
1986
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40. Electroimmunoblotting of myelin basic protein peptides: a novel approach to the rapid characterisation of antigenic specificities of monoclonal and polyclonal anti-MBP antibodies.

Author

Sheng HZ, Martenson RE, Grgacic EV, Dowse CA, Carnegie RL, and Bernard CC

Subjects
Antibodies immunology, Antibodies, Monoclonal immunology, Antibody Specificity, Enzyme-Linked Immunosorbent Assay, Humans, Myelin Basic Protein analysis, Peptide Fragments analysis, Epitopes analysis, Immunoelectrophoresis, Myelin Basic Protein immunology, Peptide Fragments immunology
Abstract

A rapid and sensitive method for the identification of antigenic determinants recognised by monoclonal and polyclonal antibodies directed against myelin basic protein (MBP) is described. By electroimmunoblotting a series of overlapping peptides covering the entire MBP molecule with monoclonal anti-MBP antibodies, the binding pattern of immunoreactive peptides can be rapidly determined and the reactive antigenic determinant identified. This procedure, which can be performed with both native and synthetic peptides, can also with appropriate modification, be applied to the analysis of naturally occurring or experimentally induced polyclonal anti-MBP autoantibodies.

Published
1988
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41. Conformation of a heptadecapeptide comprising the segment encephalitogenic in rhesus monkey.

Author

Price WS, Mendz GL, and Martenson RE

Subjects
Amino Acid Sequence, Animals, Encephalomyelitis, Autoimmune, Experimental immunology, Epitopes immunology, Hydrogen-Ion Concentration, Macaca mulatta, Magnetic Resonance Spectroscopy, Molecular Sequence Data, Phosphorylation, Protein Conformation, Rabbits, Myelin Basic Protein immunology, Peptide Fragments immunology
Abstract

The 17-residue peptide FKLGGRDSRSGSPMARR derived from myelin basic protein, containing an epitope encephalitogenic in rhesus monkey, has been studied in aqueous solution by high-resolution one- and two-dimensional carbon and proton nuclear magnetic resonance spectroscopy. The resonances of the spectra from both nuclei were assigned with the aid of two-dimensional correlated spectroscopy, pH and solvent titrations, and one-dimensional spin-decoupling techniques and by comparison of the spectra of the heptadecapeptide with those of a phosphorylated form of the peptide, the pentadecapeptide FKLGGRDSRSGSPMA, and the nonapeptide FKLGGRDSR. Amide proton temperature coefficients, coupling constants, 13C- spin-lattice relaxation times, and nuclear Overhauser effect data suggest the existence of three structured regions comprising residues 3-6, 7-12, and 12-14 in the solution conformations of the encephalitogenic heptadecapeptide.

Published
1988
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42. NMR studies of myelin basic protein. XIII. Assignment of histidine residues in rabbit, bovine and porcine proteins.

Author

Mendz GL, Moore WJ, and Martenson RE

Subjects
Animals, Cattle, Hydrogen-Ion Concentration, Magnetic Resonance Spectroscopy, Peptide Fragments, Protein Denaturation, Rabbits, Solutions, Swine, Urea, Histidine, Myelin Basic Protein
Abstract

Myelin basic protein from three species (rabbit, cow and pig) and peptides from enzymatic digests or cleavage of the proteins have been examined in aqueous solutions by proton nuclear magnetic resonance (NMR) at 400 MHz. The epsilon 1-CH and delta 2-CH resonances of all the histidine residues in the three proteins have been assigned and the pK values have been measured. The heterogeneity of chemical shifts among these resonances can be variously ascribed to persistent localized secondary structures and to effects arising from charged side-chains, particularly those of aspartic acid residues, and from side-chains of aromatic moieties.

Published
1986
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43. The location of regions in guinea pig and bovine myelin basic proteins which induce experimental allergic encephalomyelitis in Lewis rats.

Author

Martenson RE, Levine S, and Sowindki R

Subjects
Amino Acid Sequence, Animals, Cattle, Female, Guinea Pigs, Immunity, Maternally-Acquired, Immunization, Passive, Lymphocytes immunology, Peptides immunology, Rats, Species Specificity, Encephalomyelitis, Autoimmune, Experimental immunology, Epitopes, Myelin Basic Protein immunology
Abstract

Myelin basic proteins and peptides derived from them by limited cleavage with pepsin were tested for their ability to induce experimental allergic encephalomyelitis (EAE) in Lewis rats. The encephalitogenicity of the weakly active bovine protein was found to be associated with both halves of the molecule, peptides (1-88) and (89-169). Of the four smaller derivates of peptide (1-88), peptides (1-36), (43-88), (1-42), and (37-88), only the last two were active. This demonstrated that the overlap region consisting of residues 37-42 (sequence Asp-Ser-Leu-Gly-Arg-Phe) constitutes an encephalitogenic determinant. Of the two smaller derivatives of peptide (89-169), peptides (111-169) and (89-152), only the last was active. This indicated that the second encephalitogenic determinant begins between residues 88 and 111 and ends before residue 153. This region contains the sequence Leu-Ser-Leu-Ser-Arg-Phe (residues 108-113), which is strikingly similar to that of the first encephalitogenic determinant. Studies involving the extremely encephalitogenic guinea pig protein demonstrated that virtually all of the activity was recovered in the peptides corresponding to bovine peptides (37-88) and (43-88). These peptides, but not those comprising the remainder of the protein, were active in inhibiting the passive transfer of EAE with lymph node cells from donors immunized with guinea pig spinal cord.

Published
1975

44. Electroimmunoblotting of small peptides separated on urea-dodecyl sulphate (SUDS) gels. Application to myelin basic protein.

Author

Sheng HZ, Martenson RE, Carnegie PR, and Bernard CC

Subjects
Animals, Cattle, Collodion, Molecular Weight, Nylons, Rabbits, Urea, Electrophoresis methods, Immunosorbent Techniques, Myelin Basic Protein analysis, Peptides analysis
Abstract

A method for the electroimmunoblotting and immunodetection of peptides of less than 50 amino acid residues is described. Excellent resolution of a mixture of myelin basic protein (MBP) peptides was achieved by electrophoresis in a polyacrylamide stacking, urea-dodecyl sulphate minislab gel. Following electrophoresis, the peptides were transferred to various matrices and probed with monoclonal and polyclonal antibodies. Variables such as transfer time, membrane type, fixation and the amount of peptide loaded on the gel have been optimized as a consequence native and synthetic peptides can now be visualized in gels and immunodetected on immobilizing matrices. This procedure is particularly suited to the analysis and identification of small MBP fragments arising in various neuropathological conditions as well as for the rapid characterization of antigenic determinants recognized by monoclonal and polyclonal anti-MBP antibodies.

Published
1988
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45. The presence of cysteine in frog myelin basic protein.

Author

Martenson RE, Deibler GE, and Kramer AJ

Subjects
Amino Acids analysis, Animals, Anura, Chromatography, Gel, Chromatography, Ion Exchange, Electrophoresis, Polyacrylamide Gel, Hydrogen-Ion Concentration, Macromolecular Substances, Rana pipiens, Cysteine analysis, Myelin Basic Protein isolation & purification
Published
1975
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46. Experimental allergic encephalomyelitis in rabbits. A major encephalitogenic determinant within residues 1-44 of myelin basic protein.

Author

Kira J, Bacon ML, Martenson RE, Deibler GE, Kies MW, and Alvord EC Jr

Subjects
Amino Acid Sequence, Animals, Methionine metabolism, Methylation, Myelin Basic Protein analysis, Peptide Fragments analysis, Rabbits, Encephalomyelitis, Autoimmune, Experimental immunology, Epitopes, Myelin Basic Protein immunology, Peptide Fragments immunology
Abstract

Experimental allergic encephalomyelitis could be induced in rabbits by injection in Freund's complete adjuvant of either peptide 1-44 or peptide 45-87 of rabbit myelin basic protein. In order to localize the encephalitogenic determinant present in peptide 1-44, several smaller derivative peptides were prepared and examined. Peptic peptide 15-44 and thrombic peptide 1-31 were as active as peptide 1-44, whereas peptic peptides 1-14 and 18-38 and BrCN peptide 22-44 were virtually inactive. Weak activity was shown by BrCN peptide 1-21. These results provide evidence that a major encephalitogenic determinant present in peptide 1-44 lies within sequence 15-31. The encephalitogenic activity of peptide 15-44 was essentially destroyed by oxidation of methionine-21 to methionine sulfoxide; methylation of Met-21, on the other hand, appeared to be relatively ineffective in eliminating the encephalitogenicity of peptide 1-44.

Published
1986
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47. A reinvestigation of the amino acid sequences of bovine, rabbit, monkey, and human myelin basic proteins.

Author

Deibler GE, Krutzsch HC, and Martenson RE

Subjects
Amino Acid Sequence, Animals, Cattle, Chickens, Guinea Pigs, Humans, Mice, Pan troglodytes, Peptide Fragments analysis, Rabbits, Rats, Species Specificity, Swine, Trypsin, Myelin Basic Protein genetics
Abstract

In order to determine whether bovine, rabbit, and monkey myelin basic proteins (BPs) have the sequence Gly-His or His-Gly at positions corresponding to bovine sequence 76-77, we isolated the tryptic peptides encompassing the sequence in question in these proteins and cleaved them into dipeptides with dipeptidyl aminopeptidase I (EC 3.4.14.1). Analysis by gas chromatography/mass spectrometry of the dipeptides released showed that in no case did His follow Gly or Gly precede His. The identification of peptides Ala-Gln and His-Gly (bovine BP) and Ser-His and Gly-Arg (rabbit and monkey BPs) established the His-Gly sequence. A similar sequence analysis of tryptic peptide (80-91) of human BP confirmed the sequence Thr-Gln-Asp-Glu-Asn-Pro (80-85).

Published
1985

48. Epitopes in myelin basic protein reactive with monoclonal antibodies.

Author

Hruby S, Alvord EC Jr, Martenson RE, Deibler GE, Hickey WF, and Gonatas NK

Subjects
Animals, Cross Reactions, Guinea Pigs, Haplorhini, Mice, Peptide Fragments immunology, Rats, Antibodies, Monoclonal analysis, Epitopes immunology, Myelin Basic Protein immunology
Abstract

The epitopes (antigenic determinants) evoked by guinea pig or monkey myelin basic protein (BP) for 7 monoclonal antibodies (MAb) have been localized to 4 different sequences of the BPs extracted from various species. The first pair of epitopes is included within residues 1-14 and reacts with 2 rat IgG MAbs having slightly different specificities. The second pair of epitopes overlap within the sequence 86-100, requiring the Phe(91)-Phe(92) residues. One includes only residues 90-100 and reacts with a rat IgG MAb, the other is longer and reacts with a mouse IgM MAb. The third epitope lies within residues 114-124 (specifically including the single Trp) and reacts with a rat IgG MAb. A cross-reacting epitope in the amino half of the molecule is present in certain species (human, bovine and guinea pig). The fourth pair of epitopes includes residues 131-140 and is severely species-restricted. A mouse IgM MAb reacts practically only with guinea pig BP. Another IgG MAb reacts with human, chimpanzee, monkey, bovine and rat-18.5 kDa BPs, to a much lesser extent with rabbit and rat-14 kDa BPs and not with guinea pig, pig or chicken BPs. A cross-reacting epitope in the amino half of the molecule may be present in the more reactive species.

Published
1984

49. In vivo incorporation of [32P]orthophosphate into myelin basic protein of developing rabbit brain: its location in components 3 and 5 and in a new protein tentatively identified as basic protein component 7.

Author

Agrawal HC, Martenson RE, and Agrawal D

Subjects
Animals, Brain metabolism, Electrophoresis, Polyacrylamide Gel, Molecular Weight, Rabbits, Brain growth & development, Myelin Basic Protein biosynthesis, Polyphosphates metabolism
Abstract

Myelin was isolated from the brains of 16-day-old rabbits that had received intracerebral injections of [32P]orthophosphate 24 h earlier. The basic protein was extracted and examined by polyacrylamide gel electrophoresis both at low and at high pH. At low pH a single band corresponding to the basic protein contained all of the covalently bound protein radioactivity. At high pH, three bands of radioactivity corresponding to basic protein components 3, 5, and 7 were observed. Estimation of the specific radioactivities of the components in conjunction with their high pH electrophoretic mobilities indicated that components 3, 5, and 7 contained one, two, and three phosphate groups per molecule of protein, respectively.

Published
1982
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