Your search keyword '"Dixon JE"' showing total 478 results

451. Assignment of disulfide bonds in proteins by fast atom bombardment mass spectrometry.

Author

Yazdanparast R, Andrews PC, Smith DL, and Dixon JE

Subjects

Amino Acid Sequence, Animals, Cattle, Chickens, Chromatography, High Pressure Liquid, Cyanogen Bromide pharmacology, Egg White, Muramidase, Protein Conformation, Protein Processing, Post-Translational, Ribonuclease, Pancreatic, Spectrophotometry, Atomic, Trypsin metabolism, Disulfides analysis, Proteins analysis

Abstract

A rapid and sensitive method for assignment of disulfide bonds using fast atom bombardment mass spectrometry is described for hen egg white lysozyme and bovine ribonuclease A. The protein is initially digested to a mixture of peptides using chemical and enzymatic methods under conditions which minimize disulfide bond reduction and exchange. The digested sample is analyzed directly by fast atom bombardment mass spectrometry before and after chemical reduction of cystine residues. An important feature of the method is that it is not necessary to completely resolve the peptides in the digest chromatographically prior to analysis. The disulfide-containing peptides are also characterized directly by prolonged exposure of the sample to the high energy xenon atom beam which results in the reduction of cystine residues. Intra- as well as interchain disulfide bond assignments are made on the basis of the mass difference between the molecular ions (MH+) of the oxidized and reduced peptides. Confirmation of the mass assignments may be obtained from the mass spectra of the digests after one cycle of manual Edman degradation. Although the quantity of protein required to unambiguously assign all of the disulfide linkages will depend on the ease with which the appropriate peptide fragments can be formed, results from these studies indicate that approximately 1 nmol of protein is usually sufficient.

Published

1987

452. A nonamidated peptide homologous to porcine peptide YY and neuropeptide YY.

Author

Andrews PC, Hawke D, Shively JE, and Dixon JE

Subjects

Amino Acid Sequence, Amino Acids analysis, Animals, Chromatography, High Pressure Liquid, Fishes, Neuropeptide Y, Peptide YY, Protein Conformation, Nerve Tissue Proteins analysis, Peptides analysis

Abstract

A 37-residue peptide has been purified from the endocrine pancreas of the anglerfish. The first 36 residues were sequenced by gas phase Edman degradation. The sequence at the carboxyl-terminus was determined by sequencing the carboxyl-terminal tryptic dipeptide. The sequence of the peptide, which is consistent with the amino acid composition, was determined to be: Y X P X P X K X P X E X T X P X G X S X N X A X S X P X E X D X W X A X S X Y X Q X A X A X V X R X H X Y X V X N X L X I X T X R X Q X R X Y X G. Fast atom bombardment/mass spectrometry of the peptide identified a molecular ion with an average mass of 4221.3, in good agreement with the theoretical mass based upon the determined amino acid sequence. The peptide has an equal degree of sequence identity to both porcine neuropeptide YY (64%) and gastrointestinal peptide YY (64%), but less sequence identity to porcine pancreatic polypeptide (47%). Unlike the related mammalian peptides, the major form of the anglerfish peptide terminates in tyrosyl-glycine rather than tyrosineamide.

Published

1985

453. The Nalpha-acetylation of corticotropin and fragments of corticotropin by a rat pituitary Nalpha-acetyltransferase.

Author

Woodford TA and Dixon JE

Subjects

Acetylation, Amino Acid Sequence, Amino Acids analysis, Animals, Dipeptides metabolism, Kinetics, Peptide Fragments, Rats, Serine metabolism, Substrate Specificity, Tissue Distribution, Acetyltransferases metabolism, Adrenocorticotropic Hormone metabolism, Pituitary Gland metabolism

Published

1979

454. A method for increasing the sensitivity of chloramphenicol acetyltransferase assays in extracts of transfected cultured cells.

Author

Crabb DW and Dixon JE

Subjects

Acetyl Coenzyme A metabolism, Acetyltransferases genetics, Animals, Cell Extracts metabolism, Cell Line, Chloramphenicol O-Acetyltransferase, Hot Temperature, Humans, Hydrolysis, Acetyltransferases metabolism, Transfection

Abstract

Transfection of several cell lines (HeLa, COS, PC-12, CA-77, and H4IIE C3) with pRSV-CAT by a variety of methods yielded rather low chloramphenicol acetyltransferase (CAT) activity in cell extracts. Extracts of these cells were found to interfere with the assay of added CAT. The extracts were capable of deacetylating acetylchloramphenicol and of accelerating the rate of hydrolysis of the acetyl-CoA present in the assay. Heating the cell extract to 60 degrees C for 10 min completely prevented the interference and slowed the hydrolysis of acetyl-CoA. Substantially higher CAT activities were observed when the extract was heat treated in the presence of EDTA prior to enzyme assay for most cell lines tested. This simple reliable method makes possible the accurate assessment of CAT activities in different cell lines. These observations are particularly pertinent to investigators studying tissue-specific gene expression.

Published

1987

455. Cyclosporine A: a tool for analyzing the function of class I MHC antigen-reactive T cells in vivo.

Author

Hodgkin PD, Dixon JE, Andrus L, and Lafferty KJ

Subjects

Animals, Cytotoxicity, Immunologic drug effects, Graft vs Host Reaction drug effects, Interleukin-2 immunology, Mice, T-Lymphocytes classification, T-Lymphocytes drug effects, Cyclosporins pharmacology, Histocompatibility Antigens Class II immunology, Major Histocompatibility Complex, T-Lymphocytes immunology

Published

1984

456. Identification of the promoter sequences involved in the cell specific expression of the rat somatostatin gene.

Author

Andrisani OM, Hayes TE, Roos B, and Dixon JE

Subjects

Acetyltransferases genetics, Base Sequence, Cell Line, Chloramphenicol O-Acetyltransferase, DNA Restriction Enzymes, Escherichia coli genetics, Genes, Bacterial, HeLa Cells metabolism, Humans, Plasmids, Genes, Promoter Regions, Genetic, Somatostatin genetics

Abstract

DNA sequences containing the 5' flanking region of the rat somatostatin gene were linked to the coding sequence of the bacterial chloramphenicol acetyl transferase gene. This recombinant plasmid is active in expressing CAT activity in the neuronally derived, somatostatin producing CA-77 cell line. Deletion analyses of the somatostatin promoter show that the sequences proximal to position -60, relative to the cap site are required for expression of this promoter. A 4 base pair deletion of residues -46 through -43 within the somatostatin promoter results in a down mutation in vivo suggesting the existence of an element critical for the expression of the promoter in CA-77 cells. In addition, the somatostatin recombinant and its 5' deletion constructs preferentially express CAT activity in CA-77 cells, whereas only basal level of expression is observed in HeLa, BSC40, and RIN-5F cell lines, pointing to the cell specific nature of this promoter.

Published

1987

457. Cotranslational and posttranslational proteolytic processing of preprosomatostatin-I in intact islet tissue.

Author

Noe BD, Andrews PC, Dixon JE, and Spiess J

Subjects

Amino Acid Sequence, Animals, Protein Processing, Post-Translational, Protein Sorting Signals metabolism, Fishes metabolism, Islets of Langerhans metabolism, Protein Precursors metabolism, Somatostatin biosynthesis, Somatostatin metabolism

Abstract

Preprosomatostatin-I (PPSS-I) is processed in anglerfish islets to release a 14-residue somatostatin (SS-14). However, very little is known regarding other processing events that affect PPSS-I. This is the first study to identify and quantify the levels of nonsomatostatin products generated as a result of processing of this somatostatin precursor in living islet tissue. The products of PPSS-I processing in anglerfish islet tissue were identified in radiolabeling studies using a number of criteria. These criteria included immunoreactivity, specific radiolabeling by selected amino acids, radiolabel sequencing, and chromatographic comparison to isolated, structurally characterized fragments of anglerfish PPSS-I using reverse-phase high performance liquid chromatography. Intact prosomatostatin-I (aPSS-I) was isolated from tissue incubated with [3H]tryptophan and [14C]leucine. Significant 14C radioactivity was observed in the products of 11 of the first 44 sequencer cycles in positions consistent with the generation of a 96-residue prosomatostatin. These results indicate that signal cleavage occurs after the cysteine located 25 residues from the initiator Met of PPSS-I, resulting in a signal peptide 25 amino acids in length. Nonsomatostatin-containing fragments of the precursor were also found in tissue incubated with a mixture of 3H-amino acids. Only a small quantity of the dodecapeptide representing residues 69-80 in the prohormone was found (10 nmol/g tissue). Two other fragments of aPSS-I, also observed to be present in low abundance, were found to correspond to residues 1-27 (16 nmol/g tissue) and to residues 1-67 (7 nmol/g tissue) of aPSS-I. No evidence for the presence of the fragment corresponding to residues 29-67 was found. However, large quantities of SS-14 were observed (287 nmol/g tissue), indicating that the major site of aPSS-I cleavage is at the basic dipeptide immediately preceding SS-14. Recovery of much lower levels of the nonsomatostatin fragments of aPSS-I suggests that prohormone processing at the secondary sites identified in this study occurs at a low rate relative to release of SS-14 from aPSS-I.

Published

1986

458. Isolation and structure of a peptide hormone predicted from a mRNA sequence. A second somatostatin from the catfish pancreas.

Author

Andrews PC and Dixon JE

Subjects

Amino Acid Sequence, Animals, Chromatography, High Pressure Liquid, Cloning, Molecular, Fishes, Peptide Fragments analysis, Somatostatin isolation & purification, Trypsin, Pancreas metabolism, RNA, Messenger genetics, Somatostatin genetics

Abstract

This laboratory recently observed a cDNA reverse transcript to a specific mRNA from the channel catfish (Ictalurus punctata) pancreas which predicted the presence of a somatostatin gene product different from the previously reported catfish somatostatin (Oyama, H., Bradshaw, R. A., Bates, O. J., and Permutt, A. (1980) J. Biol. Chem. 255, 2251-2254). The gene product was purified using reverse phase high performance liquid chromatography. The peptide was shown to be structurally identical with somatostatin-14 from other species by tryptic mapping, amino acid composition, and sequence. The level of somatostatin-14 in the catfish endocrine pancreas was determined to be 104 micrograms of immunoreactive somatostatin/g of tissue. These observations suggest that the catfish pancreas has at least two structurally distinct somatostatins.

Published

1981

459. Rapid identification of clones using the same degenerate oligonucleotide mixture for both screening and sequencing.

Author

Nichols R and Dixon JE

Subjects

Animals, Base Composition, Base Sequence, DNA analysis, Nucleic Acid Hybridization, Peptides analysis, Plasmids, Cloning, Molecular, Oligonucleotides analysis

Abstract

A simple and rapid strategy for distinguishing between positively hybridizing colonies and false positive-hybridization signals is described. The isolation of a specific DNA sequence depends on the ability to distinguish between a clone that contains the correct sequence and a false hybridization-positive or background signal. This procedure utilizes the same oligonucleotide mixture both as a screening probe and as a sequencing primer. The mixture of oligonucleotides is used as a primer to obtain sequence information directly from double-stranded DNA. Conditions for sequencing with oligonucleotides having up to 64-fold degeneracy are described. Since the sequence information obtained is directly adjacent to the site of oligonucleotide:DNA hybridization, it is necessary to know only a minimal length of DNA or peptide sequence to both design oligonucleotide probes and confirm the authenticity of the hybridization positives. The advantages of the degenerate oligonucleotide sequencing method include the rapid, reliable identification of authentic versus false hybridization positives made directly without subcloning into single-stranded M13 phage, without sequencing large regions of DNA, or without synthesizing sequence-specific primers.

Published

1988

460. Immunological identity between bovine preparations of thiol:protein-disulphide oxidoreductase, glutathione-insulin transhydrogenase and protein-disulphide isomerase.

Author

Bjelland S, Wallevik K, Krøll J, Dixon JE, Morin JE, Freedman RB, Lambert N, Varandani PT, and Nafz MA

Subjects

Animals, Cattle, Immunodiffusion, Liver enzymology, Pancreas enzymology, Protein Disulfide-Isomerases, Epitopes analysis, Isomerases immunology, Oxidoreductases immunology, Protein Disulfide Reductase (Glutathione) immunology

Abstract

Five preparations of bovine thiol:protein-disulphide oxidoreductase/glutathione-insulin transhydrogenase (EC 1.8.4.2) and one preparation of bovine liver protein-disulphide isomerase (EC 5.3.4.1) from four different laboratories showed immunological identity in double immunodiffusion and rocket-line immunoelectrophoresis. Consequently, thiol:protein-disulphide oxidoreductase/glutathione-insulin transhydrogenase and protein-disulphide isomerase, formerly classified as two separate enzymes, should be considered as alternative activities of the same enzyme.

Published

1983

461. Genes encoding pancreatic polypeptide and neuropeptide Y are on human chromosomes 17 and 7.

Author

Takeuchi T, Gumucio DL, Yamada T, Meisler MH, Minth CD, Dixon JE, Eddy RE, and Shows TB

Subjects

Amino Acid Sequence, Base Sequence, Chromosome Mapping, Genes, Humans, Neuropeptide Y, Nucleic Acid Hybridization, Protein Precursors genetics, Chromosomes, Human, 16-18, Chromosomes, Human, 6-12 and X, Nerve Tissue Proteins genetics, Pancreatic Polypeptide genetics

Abstract

Pancreatic polypeptide and neuropeptide Y share 50% amino acid homology (18 out of 36 residues), suggesting that they may have common ancestral origins. cDNA clones complementary to human mRNAs encoding pancreatic polypeptide and neuropeptide Y were used to detect specific human genomic DNA sequences in human-mouse somatic cell hybrid lines. The pancreatic polypeptide gene (PPY) segregated with human chromosome 17, while the neuropeptide Y gene (NPY) segregated with human chromosome 7. Examination of cell hybrids with chromosomal rearrangements assigned PPY to the p11.1-qter region and NPY to the pter-q22 region of their respective chromosomes.

Published

1986

462. Postnatal development of cholecystokinin-like immunoreactivity and its mRNA level in rat brain regions.

Author

Takeda K, Koshimoto H, Uchiumi F, Haun RS, Dixon JE, and Kato T

Subjects

Aging metabolism, Animals, Brain metabolism, Cerebellum metabolism, Corpus Striatum metabolism, DNA Probes, Frontal Lobe metabolism, Hippocampus metabolism, Nucleic Acid Hybridization, RNA, Messenger genetics, Rats, Rats, Inbred Strains, Superior Colliculi metabolism, Brain growth & development, Cholecystokinin metabolism, RNA, Messenger metabolism

Abstract

Developmental changes of preprocholecystokinin mRNA (CCK mRNA) and cholecystokinin-like immunoreactivity (CCK-LI) were examined in rat brain regions (frontal cortex, colliculi, hippocampus, striatum, and cerebellum) using RNA dot blot assays with cholecystokinin (CCK) cDNA and radioimmunoassay, respectively. The CCK-LI levels in all regions examined were very low at birth. Excluding the cerebellum, the levels in these regions increased postnatally and reached adult values at 28 days of age. In contrast to CCK-LI, CCK mRNA levels changed dramatically during development. A considerable amount of CCK mRNA was detected in the frontal cortex and hippocampus at birth. The changes in the level of CCK mRNA in the frontal cortex and colliculi paralleled those of CCK-LI, including a rapid increase from 7 to 14 days of age. The synthesis of CCK mRNA preceded the appearance of CCK-LI. CCK mRNA levels in the hippocampus and striatum exhibited a transient increase, with a peak at 14 days of age. In the adult brain, the CCK mRNA levels were high in the frontal cortex, moderate in the hippocampus and colliculi, and low in the striatum. The cerebellum contained only a negligible amount of CCK mRNA during development. The relatively high level of CCK-LI compared with the low level of CCK mRNA in the striatum supports the idea that most of the striatal CCK-LI is supplied from extrastriatal regions.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1989

463. Catabolism of neuropeptides by a brain proline endopeptidase.

Author

Taylor WL and Dixon JE

Subjects

Amino Acid Sequence, Animals, Prolyl Oligopeptidases, Rats, Substrate Specificity, Brain metabolism, Endopeptidases metabolism, Nerve Tissue Proteins, Peptides, Serine Endopeptidases

Published

1980

464. Purification and characterization of a thyrotropin-releasing hormone deamidase from rat brain.

Author

Rupnow JH, Taylor WL, and Dixon JE

Subjects

Amidohydrolases metabolism, Animals, Kinetics, Rats, Subcellular Fractions enzymology, Thyrotropin-Releasing Hormone, Amidohydrolases isolation & purification, Brain enzymology

Abstract

This report describes the purification of a rat brain thyrotropin-releasing hormone (TRH) deamidating enzyme to apparent homogeneity. Criteria for purity include sodium dodecyl sulfate and disc gel electrophoresis, as well as isoelectric focusing (pI = 4.5). Enzyme purification was facilitated by development of a rapid and sensitive continuous assay using the substrate L-pyroglutamyl-Nim-benzylhistidyl-L-prolyl-beta-naphthylamide, which, upon hydrolysis of the naphthylamide, results in the appearance of the fluorescent product, beta-naphthylamine (beta NA). With this substrate the homogeneous enzyme had a specific activity of 14.5 mumol of beta NA min-1 mg-1. The only peptide product formed was shown to be L-pyroglutamyl-Nim-benzylhistidyl-L-proline. Hydrolysis of [L-prolyl-2,3-3H]TRH was shown to yield L-pyro-glutamyl-L-histidyl-L-proline as the only radiolabeled product. Characterization of the brain deamidase by gel filtration chromatography and sodium dodecyl sulfate gel electrophoresis indicated that the enzyme consists of a single polypeptide chain having molecular weights of 70,000 and 73,500, respectively. Rat brain TRH deamidase has an apparent Km of 34 micron, and a pH optimum between 7 and 8 using L-pyroglutamyl-Nim-benzylhistidyl-L-prolyl-beta-naphthylamide as a substrate. With this substrate, TRH was shown to be a competitive inhibitor with an apparent Ki of 120 +/- 20 micron.

Published

1979

465. Characterization of primary translation products from ovine and rat salivary gland mRNAs.

Author

Nichols R, Carlson DM, and Dixon JE

Subjects

Animals, Cell-Free System, Molecular Weight, Parotid Gland analysis, Peptide Biosynthesis, Rats, Serine metabolism, Sheep, Sublingual Gland analysis, Submandibular Gland analysis, Gastric Mucins, Mucins biosynthesis, Protein Biosynthesis, RNA, Messenger metabolism, Salivary Glands analysis

Abstract

Ovine and rat salivary gland mRNAs have been prepared and their translation products characterized. A 60 kD translation product from ovine submaxillary and sublingual gland mRNAs is identical in mass to the ovine apomucin. Two additional ovine translation products, 25 and 40 kD, are specific to mucin-producing salivary glands. Four rat mRNA translation products are encoded by mucin-producing salivary glands (38, 44, 67, 69 kD). These polypeptides were not detected in the parotid gland mRNAs, a serous gland. Each of these products has a high level of [3H]serine incorporation, a characteristic of mucins. The nature of these products suggests that they are mucins or mucin-like and that their molecular weights should approximate that of the corresponding apomucins.

Published

1987

466. Responses of pregnant ewes and young lambs to cold exposure.

Author

Olson DP, Parker CF, Leamaster BR, and Dixon JE

Abstract

The effects of cold stress were studied in pregnant ewes during the last three weeks of gestation and in their progeny during the first three days of life. In general, ewes were unaffected by treatment whereas changes were observed in the cold-stressed lambs. Cold-induced changes in lambs included physical weakness, depression, and poor nursing response. Serum concentrations of glucose and insulin were lowered whereas concentrations of blood urea nitrogen, alkaline phosphatase, aspartate aminotransferase, lactate dehydrogenase, triglycerides, and cortisol tended to be higher in cold exposed lambs. The mortality rate was higher (40%) in cold-stressed lambs than in lambs kept at warmer temperatures (10%). At necropsy, cold-exposed lambs had reduced amounts of adipose tissue in perirenal areas, and extensive subcutaneous hemorrhages and edema in the distal portions of the thoracic and pelvic limbs.

Published

1987

467. Isolation, characterization, and DNA sequence of the rat somatostatin gene.

Author

Tavianini MA, Hayes TE, Magazin MD, Minth CD, and Dixon JE

Subjects

Animals, Base Sequence, DNA Restriction Enzymes metabolism, Nucleic Acid Hybridization, Rats, Rats, Inbred Strains, Repetitive Sequences, Nucleic Acid, Transcription, Genetic, DNA isolation & purification, Somatostatin genetics

Abstract

The gene encoding rat somatostatin has been isolated from a lambda phage gene library. Phage harboring the gene were identified by plaque hybridization using a nick-translated fragment derived from the cDNA for rat somatostatin. The transcriptional unit includes exons of 238 and 367 base pairs (bp) separated by one intron of 621 bp. The intron is located between the codons for Gln (-57) and Glu (-56) of prosomatostatin. Analysis of the nucleotide sequence 5' to the start of transcription reveals a number of sequences which may be involved in the expression of somatostatin. A variant of the "TATA" box, TTTAAA, lies 26 bp upstream from the start of transcription, and a sequence homologous to the "CAAT" box (GGCTAAT) is 92 bp upstream from the transcription start. A long alternating purine-pyrimidine stretch, (GT)25, which is similar to Z DNA-forming sequences in other genes, lies 628 bp 5' to the transcription start and is flanked by small repeats. Hybridization analysis shows that this region is highly repeated in the genome and that homologous sequences are located approximately 2 kilobase pairs downstream from the poly(A) addition site. Southern hybridization of the lambda clone with probes derived from brain or liver poly(A+) RNA demonstrates that another transcribed sequence lies about 7 kilobase pairs downstream from the poly(A) addition site of the rat somatostatin gene. Analysis of rat DNA suggests that there may be restriction-site polymorphisms in or near the gene or that additional somatostatin-hybridizing sequences may exist in the genome.

Published

1984

468. The nature of the multiple forms of bovine thiol:protein disulfide oxidoreductase.

Author

Pace M and Dixon JE

Subjects

Animals, Cattle, Centrifugation, Electrophoresis, Polyacrylamide Gel, Freezing, Hot Temperature, Liver enzymology, Macromolecular Substances, Time Factors, Oxidoreductases, Protein Disulfide Reductase (Glutathione)

Abstract

Preparations of thiol"protein disulfide oxidoreductase from bovine liver were shown to be homogeneous by polyacrylamide gel electrophoresis, sedimentation equilibrium centrifugation and NH2-terminal analysis (Carmichael et al., 1977). When the enzyme was subjected to prolonged storage at -20 degrees, freeze-thawing, or heating at 60 degrees, at least one new protein species was observed using polyacrylamide gel electrophoresis. The new protein results from dimerization of the enzyme. The dmier consisted of two monomers held together by an intermolecular disulfide bond. The formation of this dimer can be reversed and partially prevented by thiols.

Published

1979

469. In vitro transcription directed from the somatostatin promoter is dependent upon a purified 43-kDa DNA-binding protein.

Author

Andrisani OM, Zhu ZN, Pot DA, and Dixon JE

Subjects

Animals, Base Sequence, DNA-Binding Proteins isolation & purification, Genes, HeLa Cells metabolism, Humans, Molecular Sequence Data, Molecular Weight, Rats, Templates, Genetic, DNA-Binding Proteins metabolism, Promoter Regions, Genetic, Somatostatin genetics, Transcription, Genetic

Abstract

In vitro transcription analyses were used to establish the biological function of a 43-kDa affinity-purified DNA-binding protein. The 43-kDa affinity-purified protein protects the region from position -59 to position -35 of the somatostatin promoter from DNase I digestion. This region of the somatostatin promoter harbors the TGACGTCA motif, also found and required for function in a number of other cAMP-responsive and adenovirus E1A-inducible promoters. Efficient and authentic transcription in vitro directed from the somatostatin promoter requires the TGACGTCA promoter element. In vitro transcription assays performed in the presence of somatostatin (positions -60 to -29), enkephalin (positions -105 to -71), and adenovirus type 5 E3 gene (positions -72 to -42) competitor fragments, harboring similar TGACGTCA motifs, selectively inhibit transcription directed from the somatostatin promoter, suggesting that the TGACGTCA element is the site of interaction of a somatostatin gene transactivator. Furthermore, extracts depleted of the TGACGTCA-binding activities by affinity chromatography utilizing a biotinylated oligonucleotide-avidin resin, are incapable of directing transcription from the somatostatin but not from the adenovirus major late promoter. Addition of the purified 43-kDa protein to the affinity-depleted extract restores transcription from the somatostatin promoter. These results are consistent with the 43-kDa protein being a trans-activator of the somatostatin gene.

Published

1989

470. Identification of cellular prosomatostatin and nonsomatostatin peptides derived from its amino terminus.

Author

Aron DC, Andrews PC, Dixon JE, and Roos BA

Subjects

Amino Acid Sequence, Animals, Cell Line, Chromatography, High Pressure Liquid, Molecular Weight, Radioimmunoassay, Rats, Peptide Fragments analysis, Protein Precursors analysis, Somatostatin analysis, Thyroid Neoplasms analysis

Abstract

Rat prosomatostatin was isolated from a somatostatin-producing cell line and was partially microsequenced. This indicated the amino terminal structure of cellular prosomatostatin and implied a 92-amino acid sequence for the somatostatin precursor. Based on the structure for cellular prosomatostatin, a peptide was synthesized and used to develop a radioimmunoassay directed toward the amino terminal portion of prosomatostatin. This assay has revealed two peptides containing the amino-terminal portion of prosomatostatin in a somatostatin-secreting CA-77 rat medullary thyroid carcinoma cell line. These two peptides - MW 4000 and 8000 daltons - lack somatostatin immunoreactivity. Thus, processing of prosomatostatin occurs both at the amino and carboxyl regions. These results open the way for elucidation of the structure, function and metabolism of non-somatostatin peptides derived from the amino terminus of prosomatostatin.

Published

1984

471. Characterization, kinetics and comparative properties of thiol:protein disulfide oxidoreductase.

Author

Morin JE, Carmichael DF, and Dixon JE

Subjects

Cations, Divalent pharmacology, Deoxycholic Acid pharmacology, Glutathione metabolism, Hot Temperature, Hydrogen-Ion Concentration, Insulin metabolism, Iodoacetamide pharmacology, Molecular Weight, Protein Disulfide Reductase (Glutathione) isolation & purification, Ribonucleases metabolism, Substrate Specificity, Sulfhydryl Compounds metabolism, Oxidoreductases metabolism, Protein Disulfide Reductase (Glutathione) metabolism

Published

1978

472. Primary structural comparison of the preprohormones cholecystokinin and gastrin.

Author

Deschenes RJ, Narayana SV, Argos P, and Dixon JE

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cholecystokinin genetics, DNA analysis, Gastrins genetics, Protein Precursors genetics, Rats, Swine, Cholecystokinin analysis, Gastrins analysis, Protein Precursors analysis

Abstract

The nucleotide and amino acid sequences of rat preprocholecystokinin and porcine preprogastrin have been aligned and their secondary structures predicted. Both precursors are predicted to be largely in turn and helical configurations. The sequence homology and position of an intron which splits the preprohormones suggest their evolution from a common ancestral protein.

Published

1985

473. Immobilized enzymes: the catalytic properties of lactate dehydrogenase convalently attached to glass beads.

Author

Dixon JE, Stolzenbach FE, Berenson JA, and Kaplan NO

Subjects

Amines, Animals, Chickens, Drug Stability, Glutaral, Hydrogen-Ion Concentration, Kinetics, L-Lactate Dehydrogenase antagonists & inhibitors, Lithium pharmacology, Macromolecular Substances, Nitrites, Protein Binding, Protein Denaturation, Pyruvates, Spectrophotometry, Ultraviolet, Time Factors, Glass, L-Lactate Dehydrogenase metabolism

Published

1973

474. Full mouth extraction utilizing transitional or splint dentures.

Author

Dixon JE

Subjects

Humans, Postoperative Care, Denture, Complete, Immediate, Mouth, Edentulous, Tooth Extraction

Published

1968

475. Biologically active catecholamines covalentyly bound to glass beads.

Author

Venter JC, Dixon JE, Maroko PR, and Kaplan NO

Subjects

Animals, Cell Line, Chick Embryo, Clone Cells drug effects, Clone Cells metabolism, Culture Techniques, Cyclic AMP metabolism, Dogs, Epinephrine pharmacology, Glioma metabolism, Heart Rate drug effects, Isoproterenol pharmacology, Norepinephrine pharmacology, Propranolol pharmacology, Tritium, Catecholamines pharmacology, Glass

Abstract

Catecholamines bound covalently to glass beads have been found to have biological activity in several systems. Experimental evidence has been found that immobilized epinephrine and isoproterenol accelerate the heart rate in dogs, chick embryo, and chick heart cells grown in culture, whereas immobilized propranolol results in a decrease in heart rate. Isoproterenol bound to glass beads has also been shown to markedly increase the level of adenosine 3':5'-cyclic monophosphoric acid in glial cells. The effects of the immobilized catecholamines are of longer duration than when the compounds are administered in solution. The present data indicate that the compounds are exerting their action when bound to the beads.

Published

1972

476. Comparison of the rate constants for general base catalyzed prototropy and racemization of the aldimine species formed from 3-hydroxypyridine-4-carboxaldehyde and alanine.

Author

Dixon JE and Bruice TC

Subjects

Acetates, Binding Sites, Catalysis, Formaldehyde, Hydrogen-Ion Concentration, Kinetics, Mathematics, Optical Rotation, Alanine, Imines, Pyridines

Published

1973

477. An apparatus for the determination of kinetic parameters associated with immobilized enzymes.

Author

Widmer F, Dixon JE, and Kaplan NO

Subjects

Animals, Chickens, Glass, Methods, Myocardium enzymology, Solubility, Spectrophotometry, Ultraviolet, Temperature, Time Factors, Kinetics, L-Lactate Dehydrogenase metabolism, Trypsin metabolism

Published

1973

478. Immobilized catecholamine and cocaine effects on contractility of cardiac muscle.

Author

Venter JC, Ross J Jr, Dixon JE, Mayer SE, and Kaplan NO

Subjects

Animals, Cats, Drug Synergism, Epinephrine pharmacology, Glass, Heart physiology, In Vitro Techniques, Isoproterenol pharmacology, Microscopy, Electron, Scanning, Norepinephrine pharmacology, Papillary Muscles drug effects, Reserpine pharmacology, Stimulation, Chemical, Tritium, Catecholamines pharmacology, Cocaine pharmacology, Heart drug effects

Abstract

Isoproterenol, norepinephrine, and epinephrine covalently bound to glass beads exert a positive inotropic effect on isometrically contracting papillary muscles from cats. Immobilized isoproterenol maintains increases in force and velocity of contraction for more than 5 hr. 1 muM Cocaine potentiates the action of immobilized norepinephrine, isoproterenol, and epinephrine, but not of isoproterenol in solution. The data presented indicate that the effects of immobilized catecholamines are not due to their coming off the glass. The effects observed with cocaine and immobilized catecholamines are not altered by prior treatment of the muscle with reserpine. These results suggest that the major site of catecholamine action is on receptors located on the extended surface of myocardial cells and a post-junctional site for cocaine potentiation.

Published

1973