87 results
Search Results
2. Forthcoming Papers.
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BIOCHEMISTRY , *DEOXYRIBOSE , *ESCHERICHIA coli , *GENES , *TERATOCARCINOMA - Abstract
Presents several forthcoming papers published on the December 1, 1983 issue of the "European Journal of Biochemistry." "Purification and Properties of a Thiol Protease From Rat-Liver Nuclei"; Changes in Proteoglycan Compositiion of F9 Teratocarcinoma Cells Upon Differentiation"; "Supercoiling and the Mechanism of Restriction Endonucleases"; Identification of the Gene for DNA Helicase II of Escherichia Coli."
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- 1983
3. Forthcoming Papers.
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BIOCHEMISTRY , *ENDONUCLEASES , *YEAST , *MITOCHONDRIA , *ESCHERICHIA coli , *CYTOCHROME c , *AZOTOBACTER , *PYRUVATE carboxylase , *CIRCULAR dichroism - Abstract
Presents several articles to be published in the "European Journal of Biochemistry." "An Endonuclease From Yeast Mitochondrial Fractions," by R. Morosoli and C. V. Lusena; "Antigenic Relationships Between Pore Proteins of Escherichia coli K12," by N. Overbeeke, G. van Scharrenburg and B. Lugtenberg; "Respiratory Properties of Cytochrome-c-Deficient Mutants of Azotobacter vinelandii," by P.S. Hoffman, T. V. Morgan and D. V. DerVartanian; "Hydroxyl-Ion-Induced Subunit Dissociation of Yeast Cytoplasmic Pyruvate Decarboxylase. A Circular Dichroism Study," by R. F. W. Hopmann; Others.
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- 1980
4. Forthcoming papers.
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MEDICAL research , *NUCLEOTIDE sequence , *ESCHERICHIA coli , *CONNECTIVE tissues , *NUCLEIC acid analysis - Abstract
The article presents a list of forthcoming article in the "European Journal of Biochemistry." Some of the article are: Nucleotide sequence of the promoter and amino-terminal encoding region of the escherichia coli pepN gene, Solubilization of the bovine cardiac sarcolemmal binding sites for calcium channel blockers, Hyperchromic effect of collagen induced by human collagenase, etc.
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- 1986
5. Forthcoming papers.
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BIOCHEMISTRY , *ESCHERICHIA coli , *FERRITIN , *PROTEIN kinases , *REDSHIFT - Abstract
This article presents information on forthcoming papers on biochemistry, to be published in the periodical "European Journal of Biochemistry." The papers include "Expression in Escherichia Coli of a Secreted Invertebrate Ferritin," by Matthias von Dart, Pauline M. Harrison and Werner Bottke, "Regulation of Protein Kinase A Subunits During Germination of Mucor Rouxii Sporangiospores," by Silvia Rossi and Silvia Moreno and "Optical Spectrum of Myeloperoxidase — Origin of the Red Shift," by René Plans, Younkyoo Kim, Gerald T. Babcock and Ron Wever.
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- 1994
6. Forthcoming papers.
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ESCHERICHIA coli , *NEUTROPHILS , *GRANULOCYTES , *NEISSERIA meningitidis , *PUBLISHING - Abstract
The article presents information on several forthcoming papers to be published in the "European Journal of Biochemistry." Some of the papers, which are included are as: "The Respiratory Burst of Bovine Neutrophils--Role of ab Type Cytochrome and Coenzyme Specificity,"; "Structure of the Capsular Antigen of Neisseria Meningitidis Serogroup K,"; "NMR Studies of the trp Repressor From Escherichia Coli--Characterization and Assignments of Residue Types,"; "Preliminary Identification of the Secondary Structure of the trp Repressor From Escherichia Coli,"; "Identification of the Secondary Structure of the trp Repressor of Escherichia Coli et al."
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- 1985
7. Forthcoming Papers.
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BIOLOGICAL research , *BIOTECHNOLOGY , *ESCHERICHIA coli , *ANTIBIOTICS , *ENZYMES - Abstract
This article presents information about some forthcoming research papers related to the "European Journal of Biotechnology." Some of those papers are: "Mutation-Induced Instability of Antibiotic-Resistant Mammalian Ribosomes," by P.J. Wejksnora and J.R. Warner; "Phosphoribosylpyrophosphate Synthetase of Escherichia coli. Identification of a Mutant Enzyme," by B. Hove-Jensen, P. Nygaard; "The Fl-Gene Product of Bacteriophage Lambda. Purification and Properties," by S. Benchimol and A. Becker.
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- 1982
8. Forthcoming Papers.
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PROTEINS , *BIOMOLECULES , *MEMBRANE proteins , *BIOLOGICAL membranes , *ESCHERICHIA coli , *MEDICAL sciences - Abstract
The article presents information on various research papers which will be published in the forthcoming issue of the "European Journal of Biochemistry". Some of the papers discusses are "Enzymatic Synthesis of Neolactotetraosylceramide by the N-Acctyllactosamine Synthase of Human Serum". "Rate of Transplantation and Kinetics of Processing of Newly Synthesized Molecules of Two Major Outer-Membrane Proteins, the OmpA and OmpF Proteins of Escherichia Coli," by the researchers I. Crowlesmith and K. Gamon.
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- 1982
9. Forthcoming Papers.
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BIOCHEMISTRY , *PERIODICALS , *ESCHERICHIA coli , *NUCLEOTIDE sequence , *HEMOGLOBINS , *MEDICAL sciences - Abstract
Presents several forthcoming papers to be published in the "European Journal of Biochemistry." "Molecular Properties of Two Mutant Species of the Elongation Factor Tu" by P. H. van der Meide, F. J. Duisterwinkel, J. M. de Graaf, B. Kraal, L. Bosch, J. Douglass and T. Blumenthal; "The Mechanism of Uncoupling by Picrate in Escherichia coli K-12 Membrane System," by M. Michels and E. P. Bakker; "Nucleotide Sequence for a Novel Dunk Alpha-Globin Gene," by G. V. Paddock and J. Gaubatz; "Studies on the Actomyosin ATPase and the Role of the Alkali Light Chains," by B. Pope, P. D. Wagner and A. G. Weeds.
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- 1981
10. Forthcoming Papers.
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PUBLISHING , *BIOCHEMISTRY , *BIOLOGICAL membranes , *BACTERIOPHAGES , *ESCHERICHIA coli - Abstract
The paper presents various articles, which are to be published in the future issues of the European Journal of Biochemistry. Some of the articles to be published are — "Mechanisms for Albumin-Mediated Membrane Damage," by D. Dramas, E. Harvey, Al Lawrence and A. Thomas, "Transfer RNA Precursors Are Accumulated in Escherichia Coli in the Absence of RNase E," by B.K. Ray and D. Apirion, "A New Procedure for the Simultaneous Large-Scale Purification of Bacteriophage-T4-Induced Polynucleotide Kinase, DNA Ligase, RNA Ligase and DNA Polymerase," by G.M. Dolganov, A. V. Chestukhin and M.F. Shemyakin.
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- 1980
11. Forthcoming papers.
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ESCHERICHIA coli , *ESCHERICHIA , *LIPIDS - Abstract
The article presents information on the forthcoming papers to be published in the "European Journal of Biochemistry." Some of them are: "Structural studies of the O-antigenic polysaccharide of Fusobacterium necrophorum by M.M. Garcia and M.B. Perry," "The Structure of the gene encoding chicken ribosomal protein L37 a by M. Machida," "Role of acidic lipids in the translocation and channel activity of colicins A and N in Escherichia coli cells by W. Dowhan" and "Purification and sequence determination of guanylate kinase from pig brain by G.E. Schulz."
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- 1993
12. Forthcoming papers.
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BIOCHEMISTRY , *PERIODICALS , *BIOLOGICAL literature , *CHEMICAL literature , *ESCHERICHIA coli , *GENE expression , *CANDIDA - Abstract
Lists papers to be published in the "European Journal of Biochemistry" after January 1987. "Expression of bovine pancreatic ribonuclease A in Escherichia coli," by K.P. Nambiar, et al; "Phenobarbital-mediated modulation of gene expression in rat liver — Analysis of cDNA clones; "Complete amino-acid sequence of the natural ATPase inhibitor from the mitochondria of the yeast Candida utilis.
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- 1987
13. Forthcoming Papers.
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ESCHERICHIA coli , *GLYCOPROTEINS , *GLYCOGEN , *TRYPANOSOMA , *ELECTROPHORESIS - Abstract
The article presents information on various forthcoming papers to be published in the March 15, 1984 issue of the "European Journal of Biochemistry." Some of them are "Studies on the Structure and Expression of Escherichia Coli pyrC, pyrD and pyrF Using the Cloned Genes," "Rat-Liver Lysosomal Sialidase. Solubilization, Substrate Specificity and Comparison With the Cytosolic Sialidase," "Diamine-Induced Dissociation of the First Component of Human Complement," "Evidence for the Glycoprotein Nature of Retina Glycogen," and "Mapping of Surface Glycoproteins of Trypanosoma Cruzi by Two-Dimensional Electrophoresis. A Correlation With the Cell Invasion Capacity."
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- 1984
14. Forthcoming Papers.
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BIOCHEMISTRY , *ESCHERICHIA coli , *FIBRONECTINS , *CHROMATIN , *BARLEY - Abstract
Presents a list of articles to be published in the "European Journal of Biochemistry." "Cooperative Effects in the Peptidyltransferase Center of Escherichia Coli Ribosomes," by S. B. Bourd, M. K. Kukhanova, B. P. Gottikh; "Distribution of Secondary Structure Along the Fibronectin Molecule," by S. Yu. Venyaminov, M. L. Metsis, M. A. Chernousov and V. E. Koteliansky; "Chromatin Structure in Barley Nuclei," by G. Mithieux and B. Roux.
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- 1983
15. 2-Amino-2,6-Dideoxy-L-Mannose (L-Rhamnosamine) Isolated from the Lipopolysaccharide of <em>Escherichia coli</em> 03:K2ab(L):H2.
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Jann, B. and Jann, K.
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ENDOTOXINS , *ESCHERICHIA coli , *AMINO sugars , *ACETALDEHYDE , *CHROMATOGRAPHIC analysis , *PAPER chromatography , *ALCOHOL - Abstract
From the lipopolysaccharide of Escherichia coli U41/14 (serotype 03 :K2ab(L) : H2) an unusual amino sugar was isolated. By sequential oxidation with periodate and hypoiodite and by oxidation with periodate, followed by detection of acetaldehyde formed, the ammo sugar was characterized as a 2-amino- dideoxyaldose. The hydrochloride of the amino sugar, in comparison to those of 2-amino-2, 6-dideoxy-D-glucose, 2-amino-2,6-dideoxy-L-galactose, 2-amino-2, 6-dideoxy-D-mannose, 2-amino-2, 6-di- deoxy-D-allose, and 2-amino-2, 6-dideoxy-D-gulose, was studied with aid of ion exchange column chromatography. The N-acetylated amino sugar was compared with the N-acetylated reference amino sugars with regard to their relative mobihties in paper chromatography. The ammo sugar alcohols and reference amino sugar alcohols were studied using paper electrophoresis in molybdate buffer. On the basis of the results obtained the unknown amino sugar was identified as 2-amino- 2,6-dideoxymannose (rhamnosamine). Its optical rotation showed it to be of the L-configuration. This is the first report on the natural occurrence of L-rhamnosamine. [ABSTRACT FROM AUTHOR]
- Published
- 1968
16. Cloning, expression and characterization of a Family 48 exocellulase, Cel48A, from Thermobifida fusca.
- Author
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Irwin, Diana C., Zhang, Sheng, and Wilson, David B.
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EXTRACELLULAR enzymes , *STREPTOMYCES , *ESCHERICHIA coli - Abstract
The gene for a 104-kDa exocellulase, Cel48A, formerly E6, was cloned from Thermobifida fusca into Escherichia coli and Streptomyces lividans. The DNA sequence revealed a type II cellulose-binding domain at the N-terminus, followed by a FNIII-like domain and ending with a glycosyl hydrolase Family 48 catalytic domain. The enzyme and catalytic domain alone were each expressed in and purified from S. lividans and had very low catalytic activity on swollen cellulose, carboxymethyl cellulose, bacterial microcrystalline cellulose and filter paper. However, in synergistic assays on filter paper, the addition of Cel48A to a balanced mixture of T. fusca endocellulase and exocellulase increased the specific activity from 7.9 to 11.7 µmol cellobiose·min-1·mL-1, more than 15-fold higher than any single enzyme alone. Cel48A retained > 50% of its maximum activity from pH 5 to 9 and from 40 to 60 °C. Using swissmodel, the amino-acid sequence of the Cel48Acd was modeled to the known structure of Clostridium cellulolyticum CelF. Family 48 enzymes are remarkably homologous at 35% identity for all their catalytic domains and some of the properties of the 10 members are discussed. [ABSTRACT FROM AUTHOR]
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- 2000
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17. Protein • Nucleic-Acid Reaction Kinetics.
- Author
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Giacomoni, Paolo U.
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NUCLEIC acids , *DNA polymerases , *RNA polymerases , *RNA synthesis , *ESCHERICHIA coli , *BINDING sites , *PYROPHOSPHATES - Abstract
This paper presents methods developed in order to analyze experimental results concerning the binding of Escherichia coli DNA-dependent RNA polymerase to DNA at high and at low DNA concentrations, using the filter retention assay. The basic hypotheses, under which the mathematical expressions for describing the kinetics of binding are derived, are as follows. (a) At low DNA concentration: equivalence and independence of the specific binding sites; first-order dependence of the binding reaction on both DNA and protein concentration. (b) At high DNA concentration: equivalence and independence of the non-specific binding sites; no direct transfer or one-dimensional sliding of the protein along the DNA. Comparison between theoretical predictions and experimental results at high DNA concentration will alow one to determine the relative value of the rates of binding of RNA polymerase to different promoters (between 1 and 2 in T5 DNA). Binding experiments performed at low DNA concentration are reported in this paper: these results and the analysis which is reported allow one to determine the value of the rate constant of formation of non-filterable complexes for the system fd DNA (replicative form) · RNA-polymerase (ka = 3.3 × 108 M-1 s-1 in 0.1 M NaCl, 0.01 M MgCl2). [ABSTRACT FROM AUTHOR]
- Published
- 1979
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18. Consequences of a Specific Cleavage <em>in situ</em> of 16-S Ribosomal RNA for Polypeptide Chain Elongation.
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Baan, Robert A., Frijmann, Marien, Van Knippenberg, Peter H., and Bosch, Leendert
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BACTERIOCINS , *ANTIBACTERIAL agents , *ESCHERICHIA coli , *RNA , *RIBOSOMES , *PROTEIN synthesis , *BIOCHEMISTRY - Abstract
In this paper the question was studied whether Escherichia coli ribosomes which have undergone a specific cleavage of their 16-S rRNA by treatment with the bacteriocin cloacin DF13, are able to enter and complete an elongation cycle. As we have shown in the preceding paper in this journal, these defective ribosomes can form 70-S initiation complexes with MS2 RNA as a messenger. Binding of the second aminoacyl-tRNA (alanyl-tRNA) to the latter complexes led to the formation of fMet-Ala-tRNA which was fully puromyein-sensitive. In addition to these aminoacyl-tRNAs also the third aminoacyl-tRNA (seryl-tRNA) can be bound to defective ribosomes. Dual-label experiments showed that puromycin released all radioactivity from the ribosomes. This indicates that fMet-Ala-Ser-tRNA is formed and is translocated from the A site to the P site. Control ribosomes bind the three aminoacyl-tRNAs in a 1:1:1 ratio. The defective particles bind fMet-tRNA, Ala-tRNA and Ser-tRNA in a ratio of 1:0.5:0.25. Kinetic experiments strongly suggest that at each binding of the ternary complex aminoacyt-tRNA · EF-Tu · GTP to the A site of defective ribosomes, about half of these particles undergo irreversible inactivation. Consequently polypeptide synthesis under our conditions will come to an end after incorporation of only four or five amino acids. The particles which temporarily survive ternary complex binding are fully capable of transpeptidation and translocation. [ABSTRACT FROM AUTHOR]
- Published
- 1978
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19. Biosynthesis of the O9 Antigen of <em>Escherichia coli</em>.
- Author
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Flemming, Hans-Curt and Jann, Klaus
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ESCHERICHIA coli , *BIOSYNTHESIS , *BIOCHEMISTRY , *ANTIGENS , *IMMUNITY , *ORGANIC synthesis - Abstract
`The O9-specific mannan of Escherichia coil was synthesized in vitro from GDP-[14C]mannose by membranes which were obtained from a phosphomannose isomerase-less mutant of E. coli O9:K29- :H-, Subsequent treatment of the membranes with dilute acid liberated a neutral product, whereas with aqueous phenol a charged product was obtained. Chromatography on DEAE-cellulose, incubation with alkaline phosphatase and microdetermination showed that the charged mannan was substituted with one phosphate per chain. The neutral 14C-labelled product of the incubation hr vitro was reduced with sodium boro[³H]hydride. After total acid hydrolysis, the radioactive material was chromatographed on paper in the presence of borate. It was found that [³H]glucitol, but no [³H, 14C]mannitol was present. When the neutral product, which was obtained after incubation of 14C-prelabelled membranes with nonradioactive GDP-mannose, was hydrolyzed with and without prior reduction with non-radioactive sodium borohydride, in subsequent paper chromatography, [14C]glucitol or [14C]glucose was found. The glucose was also converted enzymatically to gluconic acid, which was identified by paper electrophoresis. These results show that in the neutral O9-specific mannan glucose is at the reducing end and they indicate that the mannan chain grows at the non-reducing end. This is discussed with respect to the overall mechanism of the biosynthesis of the 09 antigen. [ABSTRACT FROM AUTHOR]
- Published
- 1978
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20. Immunochemical Studies on Lipopolysaccharides from Wild-Type and Mutants of Escherichia coli K-12.
- Author
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Mayer, Hubert, Rapin, Anette M. C., Schmidt, Günter, and Boman, Hans G.
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POLYSACCHARIDES , *ESCHERICHIA coli , *SACCHARIDES , *DISACCHARIDES , *SUGARS , *BIOCHEMISTRY - Abstract
Lipopolysaccharides from a number of mutants of Escherichia coil K-12 were investigated by means of chemical and serological methods. Inhibition of passive hemagglutination and inhibition of precipitation show that L-rhamnose is the immunodominant sugar in the lipopolysaccharide from wild-type E. coli K-12. The disaccharide rhamnosyl-KDO (where KDO is 3-deoxy-D-manno-octulosonic acid) was isolated and characterized after mild acid hydrolysis of the lipopolysaccharide. It is concluded that rhamnose is present in the innermost part of the core as a side-chain substituent on KDO. From crosses between an E. coli K-12 donor and E. coil O8, hybrids were obtained which contained either one or both of the donor rfa and rfb clusters. Serum absorption studies with lipopolysaccharides from these hybrids indicated that the histidine-linked rfb cluster is responsible for the presence of rhamnose in the K-12 core oligosaccharide. Using paper chromatography of 32p-labelled lipopolysaccharides we have found heterogeneous lipopolysaccharide in two strains as well as some differences between two wild-type strains. The latter difference is believed to be due to varying contents of KDO-linked ethanolamine phosphate. The overall results presented together with those described in the companion paper clearly show that the core oligosaccharide in E. coil K-12 has a structure different from the types previously described for other strains of E. coli (designed coli R1 to coil R4). [ABSTRACT FROM AUTHOR]
- Published
- 1976
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21. Identification of surface residues in the trp repressor of <em>Escherichia coli</em>.
- Author
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Lane, Andrew N. and Jardetzky, Oleg
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ESCHERICHIA coli , *NUCLEAR magnetic resonance , *AMINO acids , *BINDING sites , *BIOCHEMISTRY , *MOLECULAR biology - Abstract
A subset of the spin systems assigned in the ¹H NMR of the trp repressor in the first paper in this series (our penultimate preceding paper in this journal) can be identified as surface or buried residues on the basis of four independent types of measurement: (a) selective spin-lattice relaxation times; (b) the dependence of line widths on temperature and the concentration of manganous ion; (c) fluorescence quenching; and (d) titration behaviour. Criteria are developed for distinguishing surface and buried residues. The significance for the function of DNA biding proteins is discussed. [ABSTRACT FROM AUTHOR]
- Published
- 1985
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22. The O8 Antigen of <em>Escherichia coli</em> .
- Author
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Reske, Konrad and Jann, Klaus
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POLYSACCHARIDES , *ESCHERICHIA coli , *PHENOL , *MANNOSE , *MOLECULAR weights , *OLIGOSACCHARIDES , *HYDROLYSIS , *ELECTROPHORESIS , *MASS spectrometry - Abstract
The polysaccharide moiety of the lipopolysaccharide (polysaccharide I) from Escherichia coli F492 (08:K27-:H-) and the polysaccharide (polysaccharide II) from the rfa mutant F612 (derived from F492) were isolated by extraction with 450% aqueous phenol at 65 °C. Polysaccharide I was obtained in 1–2% yield (based on dry bacteria). It contained mannose (83.5%), glucose (5.7%), galactose (3.4%), heptose (4.6%) and 2-keto-3-deoxy-mannosulonic acid (0.8%). Polysaccharide II was obtained in 0.8–1% yield (based on dry bacteria). It contained 99.2% mannose. With the method of Yphantis it was found that the molecular weights of polysaccharides I and II were 12400 and 10400, respectively. The difference accounted for the core oligosaccharide which was present in polysaccharide I and absent in polysaccharide II. The specific optical rotation was 43 °C for polysaccharide I and 42 °C for polysaccharide II. Both polysaccharides were permethylated. Subsequent hydrolysis, reduction and acetylation, followed by gas-liquid chromatography and mass spectrometry indicated that in both polysaccharides two-thirds of the mannose units were substituted at C-2 and one-third at C-3. These results were confirmed by periodate oxidation. From polysaccharide II nine oligosaccharides were obtained after partial acid hydrolysis by chromatography on Biogel P2, paper chromatography and paper electrophoresis of the borate complexes. The oligosaccharides were reduced with sodium borodeuterate (which labelled the reducing mannose units) and methylated. After hydrolysis, reduction and acetylation the products were analyzed by gas chromatography and mass spectrometry. It is concluded that the poIysaccharides I and II contain about 20 repeating units of α-mannosyl-1,2-α-mannosyl-1,2-α-mannose which are joined through &alph;-1,3 linkages. [ABSTRACT FROM AUTHOR]
- Published
- 1972
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23. Propriétés des ribosomes et du RNA synthétisés par Escherichia coli cultivé en présence d'éthionine.
- Author
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Beaud, Georges and Hayes, Donal H.
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RIBOSOMES , *ESCHERICHIA coli , *ORGANELLES , *METHYLTRANSFERASES , *ADENOSYLMETHIONINE , *PROTEINS - Abstract
Two isogenic derivatives of Escherichia coli K12: strains EA 1 (Met-, Biot-, RCstr and EA 2 (Mei-, Biot-, RCrel) when grown in the presence of ethionine in place of methionine, synthesize ribosomes whose RNA is submethylated and whose proteins contain ethionine. Net ribosome synthesis in the presence of ethionine is greater in the RCrel strain than in the RCstr strain. The precedinig paper describes results obtained with the latter strain. Here we present further studies carried out with the isogenic RCrel strain EA 2 As in the case of the RCstr strain (previous paper) ribosomes synthesized by the RCrel strain grown in the presence of ethionine display defective association properties. A large fraction of these "ethionine" ribosomes is found as free subunits in crude extracts containing 10 mM Mg+ prepared from strain EA 2 grown in an ethionine-containing medium. These free "ethionine" subunits have sedimentation coefficients of 28 S and 45 S approximately while the "ethionine" subunits found associated as 70 S particles in crude bacterial extracts sediment at 30 S and 50 S respectively. Both classes of "ethionine" subunits (free, and associated) can be methylated in vitro in the presence of S-adenosyl methionine with or without the addition of an external source of methylases (100000 x g supernatant of a homologous crude bacterial extract) The latter observation shows that the "ethionine" subunits contain bound methylases. These enzymes do not seem to be normal ribosomal proteins nor to be bound specifically to "ethionine" ribosomes since (a) they are removed by washing the "ethionine" ribosomes with 1 M NH4Cl, and (b) they are found bound to normal methionine ribosomes from which they are also removed by washing with 1 M NH4Cl. [ABSTRACT FROM AUTHOR]
- Published
- 1971
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24. Generation and characterization of functional mutants in the translation initiation factor IF1 of Escherichia coli.
- Author
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Croitoru, Victor, Bucheli-Witschei, Margarete, Hägg, Peter, Abdulkarim, Farhad, and Isaksson, Leif A.
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PROKARYOTES , *ESCHERICHIA coli , *DNA replication , *MUTAGENESIS , *PHENOTYPES , *DNA synthesis - Abstract
Three protein factors IF1, IF2 and IF3 are involved in the initiation of translation in prokaryotes. No clear function has been assigned to the smallest of these three factors, IF1. Therefore, to investigate the role of this protein in the initiation process in Escherichia coli we have mutated the corresponding gene infA. Because IF1 is essential for cell viability and no mutant selection has so far been described, the infA gene in a plasmid was mutated by site-directed mutagenesis in a strain with a chromosomal infA+ gene, followed by deletion of this infA + gene. Using this approach, the six arginine residues of IF1 were altered to leucine or aspartate. Another set of plasmid-encoded IF1 mutants with a cold-sensitive phenotype was collected using localized random mutagenesis. All mutants with a mutated infA gene on a plasmid and a deletion of the chromosomal infA copy were viable, except for an R65D alteration. Differences in growth phenotypes of the mutants were observed in both minimal and rich media. Some of the mutated infA genes were successfully recombined into the chromosome thereby replacing the wild-type infA+ allele. Several of these recombinants showed reduced growth rate and a partial cold-sensitive phenotype. This paper presents a collection of IF1 mutants designed for in vivo and in vitro studies on the function of IF1. [ABSTRACT FROM AUTHOR]
- Published
- 2004
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25. Defective translocation of a signal sequence mutant in a prlA4 suppressor strain of Escherichia coli.
- Author
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Adams, Hendrik, Scotti, Pier A., Luirink, Joen, and Tommassen, Jan
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ESCHERICHIA coli , *CHROMOSOMAL translocation , *PROTEINS - Abstract
In the accompanying paper [Adams, H., Scotti, P.A., de Cock, H., Luirink, J. & Tommassen, J. (2002) Eur. J. Biochem. 269 , 5564–5571], we showed that the precursor of outer-membrane protein PhoE of Escherichia coli with a Gly to Leu substitution at position -10 in the signal sequence (G-10L) is targeted to the SecYEG translocon via the signal-recognition particle (SRP) route, instead of via the SecB pathway. Here, we studied the fate of the mutant precursor in a prlA4 mutant strain. prlA mutations, located in the secY gene, have been isolated as suppressors that restore the export of precursors with defective signal sequences. Remarkably, the G-10L mutant precursor, which is normally exported in a wild-type strain, accumulated strongly in a prlA4 mutant strain. In vitro cross-linking experiments revealed that the precursor is correctly targeted to the prlA4 mutant translocon. However, translocation across the cytoplasmic membrane was defective, as appeared from proteinase K-accessibility experiments in pulse-labeled cells. Furthermore, the mutant precursor was found to accumulate when expressed in a secY40 mutant, which is defective in the insertion of integral-membrane proteins but not in protein translocation. Together, these data suggest that SecB and SRP substrates are differently processed at the SecYEG translocon. [ABSTRACT FROM AUTHOR]
- Published
- 2002
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26. Liberation of the intramolecular interaction as the mechanism of heat-induced activation of HSP90 molecular chaperone.
- Author
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Tanaka, Etsuko, Nemoto, Takayuki K., and Ono, Toshio
- Subjects
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MOLECULAR chaperones , *ESCHERICHIA coli , *CITRATES - Abstract
The molecular chaperone function of HSP90 is activated under heat-stress conditions. In the present study, we investigated the role of the interactions in the heat-induced activation of HSP90 molecular chaperone. The preceding paper demonstrated two domain–domain interactions of HtpG, an Escherichia coli homologue of mammalian HSP90, i.e. an intra-molecular interaction between the N-terminal and middle domains and an intermolecular one between the middle and C-terminal domains. A bacterial two-hybrid system revealed that the two interactions also existed in human HSP90α. Partners of the interaction between the N-terminal and middle domains of human HSP90α could, but those between the middle and C-terminal domains could not, be replaced by the domains of HtpG. Thus, the interface between the N-terminal and middle domains is essentially unvaried from bacterial to human members of the HSP90-family proteins. The citrate synthase-binding activity of HtpG at an elevated temperature was solely localized in the N-terminal domain, but HSP90α possessed two sites in the N-terminal and other domains. The citrate-synthase-binding activity of the N-terminal domain was suppressed by the association of the middle domain. The complex between the N-terminal and middle domains is labile at elevated temperatures, but the other is stable even at 70 °C. Taken together, we propose the liberation of the N-terminal client-binding domain from the middle suppressor domain is involved in the temperature-dependent activation mechanism of HSP90 molecular chaperone. [ABSTRACT FROM AUTHOR]
- Published
- 2001
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27. The role of Asp42 in Escherichia coli inorganic pyrophosphatase functioning.
- Author
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Rodina, Elena V., Vainonen, Yuliya P., Vorobyeva, Nataliya N., Kurilova, Svetlana A., Nazarova, Tatjana I., and Avaeva, Svetlana M.
- Subjects
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MAGNESIUM ions , *PYROPHOSPHATES , *ESCHERICHIA coli , *ENZYMES - Abstract
Excess of Mg2+ ions is known to inhibit the soluble inorganic pyrophosphatases (PPases). In contrast, the mutant Escherichia coli inorganic pyrophosphatase Asp42→Asn is three times more active than native and retains its activity at high Mg2+ concentration. In this paper, another two mutant variants with Asp42 replaced by Ala or Glu were investigated to characterize the role of Asp42 in catalysis. pH-independent kinetic parameters of MgPPi hydrolysis and the dissociation constants for the activating and inhibitory Mg2+ ions were calculated. It was shown that Mg2+ inhibition of MgPPi hydrolysis by native PPase exhibited uncompetitive kinetics under the saturating substrate concentration. All three substitutions of Asp42 lead to a sharp decrease of inhibitory Mg2+ affinity to the enzyme. These findings allow determination of the sites of inhibitory and substrate Mg2+ ions binding to PPase. Common features of these mutants allow the conclusion that the function of Asp42 is to accurately coordinate the residues implicated in the substrate and the inhibitory Mg2+ ion binding to PPase active site. Structural analysis of PPase complexed with Mg2+ compared with PPase complexed with Mn2+ and reaction products confirms this supposition. [ABSTRACT FROM AUTHOR]
- Published
- 2001
- Full Text
- View/download PDF
28. NMR characterization of a single-cysteine mutant of Escherichia coli thioredoxin and a covalent thioredoxin-peptide complex.
- Author
-
Jeng, Mei-Fen, Reymond, Martine T., Tennant, Linda L., Holmgren, Arne, and Dyson, H. Jane
- Subjects
- *
THIOREDOXIN , *ESCHERICHIA coli , *NUCLEAR magnetic resonance - Abstract
The mechanism of disulfide reduction by thioredoxin in the cell is thought to occur through the formation and subsequent destruction of a mixed-disulfide intermediate between thioredoxin and the substrate. In order to model the interaction, we have prepared a mutant of Escherichia coli thioredoxin where the second cysteine residue of the active site has been replaced by an alanine residue. A specific covalent complex has been prepared between the remaining cysteine residue and a short cysteine-containing peptide. This paper describes the preparation and characterization of the mutant protein both free and in the peptide complex. [ABSTRACT FROM AUTHOR]
- Published
- 1998
- Full Text
- View/download PDF
29. Genomic organization, cDNA sequence, bacterial expression, and purification of human seryl-tRNA synthase.
- Author
-
Vincent, Christine, Tarbouriech, Nicolas, and Hártlein, Michael
- Subjects
- *
SERINE , *TRANSFER RNA , *INTRONS , *EXONS (Genetics) , *ESCHERICHIA coli , *SACCHAROMYCES cerevisiae - Abstract
In this paper, we report the cDNA sequence and deduced primary sequence for human cytosolic seryl-tRNA synthetase, and its expression in Escherichia coli. Two human brain eDNA clones of different origin, containing overlapping fragments coding for human seryl-tRNA synthetase were sequenced: HFBDN14 (fetal brain clone); and IB48 (infant brain clone). For both clones the 5′ region of the cDNA was missing. This 5′ region was obtained via PCR methods using a human brain 5′ RACE-Ready cDNA library. The complete cDNA sequence allowed us to define primers to isolate and characterize the intron/ exon structure of the serS gene, consisting of 10 introns and 11 exons. The introns' sizes range from 283 bp to more than 3000 bp and the size of the exons from 71 bp to 222 bp. The availability of the gone structure of the human enzyme could help to clarify some aspects of the molecular evolution of class-II aminoacyl-tRNA synthetases. The human seryl-tRNA synthetase has been expressed in E. coli, purified (95% pure as determined by SDS/PAGE) and kinetic parameters have been measured for its substrate tRNA. The human seryl-tRNA synthetase sequence (514 amino acid residues) shows significant sequence identity with seryl-tRNA synthetases from E. coli (25 %), Saccharomyces cerevisiae (40%), Arabidopsis thaliana (41%) and Caenorhabditis elegans (60%). The partial sequences from published mammalian seryl-tRNA synthetases are very similar to the human enzyme (94% and 92% identity for mouse and Chinese hamster seryl-tRNA synthetase, respectively). Human seryl-tRNA synthetase, similar to several other class-I and class-II human aminoacyl-tRNA synthetases, is clearly related to its bacterial counterparts, independent of an additional C-terminal domain and a N-terminal insertion identified in the human enzyme. In functional studies, the enzyme aminoacylates calf liver tRNA and prokaryotic E. coli tRNA. [ABSTRACT FROM AUTHOR]
- Published
- 1997
- Full Text
- View/download PDF
30. Different consequences of incorporating chloroplast ribosomal proteins L12 and S18 into the bacterial ribosomes of Escherichia coli.
- Author
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Weglöhner, Wolfgang, Jünemann, Ralf, von Knoblauch, Klaus, and Subramanian, Alap R.
- Subjects
- *
RIBOSOMES , *ESCHERICHIA coli , *CHLOROPLASTS , *AMINO acid sequence , *BIOLOGICAL divergence - Abstract
We have incorporated chloroplast ribosomal proteins (R-proteins) L12 and S18 into Escherichia coli ribosomes and examined the hybrid ribosomes for their ability to form polysomes in vivo and perform poly(U)-dependent poly(Phe) synthesis in vitro. The rye chloroplast S18 used for the experiment is a highly divergent protein (170 amino acid residues; E. coli S18, 74 residues), containing a repeating, chloroplast-specific, heptapeptide motif, and has amino acid sequence identity of only 35% to E. coli S18. When expressed in E. coli, chloroplast S18 was assembled in E. coli ribosomes. The latter formed polysomes in vivo at about the same rate as the host ribosomes, indicating that the replacement of E. coli S18 with its chloroplast homologue has only a minor, if any, effect on function. The L12 protein is much more conserved in sequence and chain length, and is known to have a very important function. The Arabidopsis chloroplast L12 used in the experiment was incorporated into E. coli 50S subunits that associated with the 30S subunits to form ribosomes, but the latter were unable to form polysomes. This result indicates functional inactivation of E. coli ribosomes by a chloroplast R-protein. To further confirm this result, we overproduced chloroplast L12 through the use of a secretion, vector and purified the protein to homogeneity. Chloroplast L12 could be efficiently incorporated in vitro into L7/12-1acking E. coli ribosomes, but the hybrid ribosomes were totally inactive in poly(U)-dependent poly(Phe) synthesis. Computer modeling of the spatial structure of all known chloroplast L12 proteins (using E. coli L12 coordinates) indicated a 'chloroplast loop' present only in chloroplast L12. The presence of this loop might have a role in the observed inactivation. Taken together with previously reported results (summarized in this paper), it would appear that the features of chloroplast R-proteins concerned with specific functions are more divergent than their assembly properties. We have previously described methods suitable for overproduction and purification of chloroplast Rproteins that are encoded in organellar DNA (≈20), but that gave poor yield for those encoded in the nuclear DNA (≈45). Here we describe a method that overcomes this problem and allows the purification of nucleus-encoded chloroplast R-proteins in milligram quantities. [ABSTRACT FROM AUTHOR]
- Published
- 1997
- Full Text
- View/download PDF
31. The predominant protein in peroxisomal cores of sunflower cotyledons in a catalase that differs in primary structure from the catalase in the peroxisomal matrix.
- Author
-
Kleff, Stefan, Sander, Stephanie, Mielke, Gregor, and Eising, Rainer
- Subjects
- *
PLANT cell microbodies , *SUNFLOWERS , *MOLECULAR structure , *AMINO acid sequence , *CATALASE , *ESCHERICHIA coli - Abstract
This paper describes a biochemical study on the protein composition of crystalline inclusions (cores) from plant peroxisomes. By SDS/PAGE and immunoblotting, a catalase of 59 kDa was identified as the predominant protein component in purified cores from sunflower (Helianthus annuus L.) cotyledons. A 55-kDa catalase was the only additional peptide detected. In contrast to in cores, the 55-kDa catalase was the major catalase protein in matrix fractions obtained from lysed peroxisomes. These findings suggested two peroxisomal populations of catalase differing in molecular structure and subperoxisomal compartmentation in sunflower cotyledons. Evidence for different amino acid sequences of the two catalases was found by peptide mapping with endoproteinase Glu-C, by expressing a eDNA encoding matrix catalase in Escherichia coli, and by partial amino acid sequencing of peptide fragments from 59-kDa core catalase. These results contradict the previous view that the formation of cores occurred via condensation of matrix catalase, and indicate that new concepts on the biogenesis and physiological function of plant peroxisomal cores need to be developed. [ABSTRACT FROM AUTHOR]
- Published
- 1997
- Full Text
- View/download PDF
32. L-Aspartate oxidase from <em>Escherichia coli</em> I. Characterization of coenzyme binding and product inhibition.
- Author
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Mortarino, Michele, Negri, Armando, Tedeschi, Gabriella, Simonic, Tatjana, Duga, Stefano, Gassen, Hans Gunther, and Ronchi, Severino
- Subjects
- *
FLAVOPROTEINS , *OXIDASES , *ESCHERICHIA coli , *PROTEINS , *MONOMERS , *ENZYMES , *MUTAGENESIS - Abstract
This paper reports the biochemical characterization of the flavoprotein L-aspartate oxidase from Escherichia coli. Modification of a previously published procedure allowed overexpression of the holoenzyme in an unproteolysed form. L-Aspartate oxidase is a monomer of 60 kDa containing 1 mol of non-covalently bound FAD/mol protein. A polarographic and two spectrophotometric coupled assays have been set up to monitor the enzymatic activity continuously. L-Aspartate oxidase was subjected to product inhibition since iminoaspartate, which results from the oxidation of L-aspartate, binds to the enzyme with a dissociation constant (Kd) equal to 1.4 μM. The enzyme binds FAD by a simple second-order process with Kd 0.67 μM. Site-directed mutagenesis of the residues E43, G44, S45, F47 and Y48 located in the putative binding site of the isoallossazinic portion of FAD reduces the affinity for the coenzyme. [ABSTRACT FROM AUTHOR]
- Published
- 1996
- Full Text
- View/download PDF
33. Use of T7 RNA polymerase in an optimized <em>Escherichia coli</em> coupled <em>in vitro</em> transcription-translation system.
- Author
-
Köhrer, Caroline, Mayer, Christine, Gröbner, Peter, and Piendl, Wolfgang
- Subjects
- *
TRANSFERASES , *PROMOTERS , *GENETIC transcription , *GENETIC translation , *ESCHERICHIA coli , *GENE expression - Abstract
An Escherichia coli coupled in vitro transcription-translation system has been modified to allow efficient expression of genes under the control of a T7 promoter. We describe both the characterization and use of two S30 crude extracts prepared from E. coli, namely S30 BL21 (DE3) (containing endogenous T7 RNA polymerase) and S30 BL21 (supplemented with exogenous T7 RNA polymerase). Since transcription by the highly active T7 RNA polymerase is known to overload the translational machinery of E. coli, the ratio betweent mRNA and ribosomes has to be regulated in the coupled in vitro systems. For this purpose, the level of mRNA is controlled by varying the amount of DNA template (S30 extract with endogenous T7 RNA polymerase) or by limited amounts of exogenously added T7 RNA polymerase. The couple in vitro system described in this paper provides two especially useful applications. First, it is most suitable for studying the regulation of gene expression in vitro, second, it can be used to express DNA templates carrying up to 10 genes. We show that genes which are not well expressed in E. coli in vivo because of unfavourable codon usage or plasmid instability are synthesized efficiently in the couple in vitro system. [ABSTRACT FROM AUTHOR]
- Published
- 1996
- Full Text
- View/download PDF
34. In vivo synthesis of ATPase complexes of Propionigenium modestum and Escherichia coli and analysis of their function.
- Author
-
Gerike, Ursula, Kaim, Georg, and Dimroth, Peter
- Subjects
- *
ADENOSINE triphosphatase gene expression , *GENE expression , *SODIUM , *HYDROLYSIS , *PLASMIDS , *ESCHERICHIA coli - Abstract
Expression studies of Propionigenium modestum ATPase genes in various combinations with Escherichia coli ATPase genes were performed in the unc deletion mutant strain E. coli DK8. Plasmids containing the whole unc operon from P. modestum were unable to complement the E. coli unc deletion mutant. Although all ATPase subunits were expressed from the plasmids, there was no detectable ATP hydrolysing activity, indicating that the F1 part was not functional. Transformants expressing an E. coli F1-P. modestum F0 hybrid exhibited considerable ATPase activities. Binding of the F1 part to the membrane was very weak, however, and the coupling between ATP hydrolysis and Na+ transport was impaired. After combining the genes for E. coli ATPase subunits α, β, γ, δ and epsilon and the hydrophilic part of subunit b with P. modestum ATPase subunits a and c and the hydrophobic part of subunit b on a plasmid, a non-functional hybrid ATPase was expressed in E. coli. The ATPase was only loosely bound to the membrane, from which it was solubilized with Triton X-100 and purified. Subunit b and a proteolytic degradation product were the only F0 subunits detectable in the purified enzyme. A stable F0 complex is thus not formed with the hybrid b subunit. The absence of a functional F0 complex was in accord with proton-conduction measurements with bacterial vesicles. The only functional Na+-translocating ATPase expressed in E. coli thus far consists of E. coli subunits α, β, γ and epsilon, and P. modestum subunits δ, a, b and c [Kaim, G. & Dimroth, P. (1993) Eur. J. Biochem. 218, 937-944]. During the cloning conducted in our present study, errors in the sequence entry into the EMBL data bank (accession no. X58461) for the P. modestum ATPase α and β subunits became evident, which are corrected in this paper. [ABSTRACT FROM AUTHOR]
- Published
- 1995
- Full Text
- View/download PDF
35. Evidence for a pyrimidine-nucleotide-specific initiation site (the i site) on Escherichia coli RNA polymerase.
- Author
-
Reddy, Padmalatha S. and Chatterji, Dipankar
- Subjects
- *
ESCHERICHIA coli , *RNA polymerases , *PYRIMIDINE nucleotides , *RIFAMPIN , *ESCHERICHIA , *TRANSFERASES - Abstract
Escherichia coli RNA polymerase has two sites, the i and i + 1, for the binding of the first two substrates. The i site is template- and Mg2+-independent and purine-nucleotide-specific, whereas the i + 1 site is template- and Mg2+-dependent and shows no nucleotide preference. The specificity of the i site for purine nucleotides is well in accord with the fact that most promoters initiate with a purine nucleotide. But there are a few promoters that initiate with a pyrimidine nucleotide. Dinucleotide synthesis at these promoters is completely inhibited by rifampicin. Earlier studies have failed to identify an i site for pyrimidine nucleotides. In this paper, using a fluorescent analog of UTP, namely uridine 5'-[γ-(5-sulfonic acid)naphthylamidate]-triphosphate, abbreviated as UTP[AmNS], we are able to show its binding to RNA polymerase, with a Kd of 0.8 μM, in the absence of Mg2+ and template. This suggests the presence of an i pyrimidine nucleotide site. The fact that UTP-[AmNS] is capable of initiating RNA synthesis from the i site is further evidenced by the abortive transcription analyses at the lac promoter. Fluorescence titration studies performed in the presence and absence of purine initiator molecules indicate that this site is different from the i purine site. Scatchard analysis of the above data indicates the presence of a single binding site for UTP[AmNS] in the absence of Mg2+. Moreover UTP[AmNS] binds to the core enzyme with a Kd of 3.0 μM implying that, unlike the i purine nucleotide site, the sigma protein confers a tighter binding of UTP-[AmNS] to the low-Kd site. Forster's energy transfer measurements using UTP[AmNS] as the donor and rifampicin as the acceptor have been used for estimation of the distance of the i pyrimidine nucleotide site from the rifampicin site. From these measurements, we infer that there is no direct interference of rifampicin with the first [ABSTRACT FROM AUTHOR]
- Published
- 1994
- Full Text
- View/download PDF
36. Regulatory Properties of Phosphofructokinase 2 from Escherichia coli.
- Author
-
Kotlarz, Denise and Buc, Henri
- Subjects
- *
ESCHERICHIA coli , *ALLOSTERIC enzymes , *ENZYMES , *BIOSYNTHESIS , *BIOCHEMICAL templates , *ADENOSINE triphosphate - Abstract
Escherichia coli K 12 appears to behave as an enzyme. We show in the present paper that, in fact, phosphofructokinase 2 also presents some regulatory properties in vitro: at high concentrations, ATP is an inhibitor of phosphofructokinase 2 and it provokes the tetramerization of the dimeric native enzyme. The binding of the two substrates to phosphofructokinase 2 is sequential and ordered as for phosphofructokinase 1, but in the former case fructose 6-phosphate is the first substrate to be bound and ADP the first product to be released. Each dimer of phosphofructokinase 2 binds two molecules of fructose 6-phosphate but only one molecule of the product fructose 1,6-bisphosphate. Although both phosphofructokinases of E. coli K 12 present regulatory properties in vitro, the mechanism of regulation of the activity of the two enzymes is strikingly different. It can be asked whether or not these mechanisms operate in vivo. [ABSTRACT FROM AUTHOR]
- Published
- 1981
- Full Text
- View/download PDF
37. A Proton NMR Study of Ribosomal Protein L25 from <em>Escherichia coli</em>.
- Author
-
Kime, Matthew J., Ratcliffe, R. George, Moore, Peter B., and Williams, Robert J. P.
- Subjects
- *
ESCHERICHIA coli , *PROTONS , *SOLUTION (Chemistry) , *METABOLISM , *URINALYSIS , *SOLVENTS - Abstract
A highly folded form of the ribosomal protein L25 from Escherichia coli can be obtained from urea-denatured preparations. Proton NMR data show that this form of the molecule must have a compact, globular tertiary structure. Spectroscopically it is indistinguishable from L25 prepared by methods which avoid denaturing solvents. Thus L25 is a protein which can be reversibly denatured. The stability and solubility of the folded form of the protein are discussed and primary assignments made for a number of resonances in its NMR spectrum. The paper shows that this folded form of the protein can be characterised using NMR spectroscopy. High-resolution NMR spectroscopy provides a sensitive and general way for the characterisation of protein folds. [ABSTRACT FROM AUTHOR]
- Published
- 1981
- Full Text
- View/download PDF
38. The Role of the Codon and the Initiation Factor IF-2 in the Selection of N-Blocked Aminoacyl-tRNA for Initiation.
- Author
-
van der Laken, Kees, Bakker-Steeneveld, Hanny, Berkhout, Ben, and van Knippenberg, Peter H.
- Subjects
- *
AMINOACYL-tRNA , *AMINO acids , *TRANSFER RNA , *RNA , *ESCHERICHIA coli , *ESCHERICHIA - Abstract
Poly(uridylic acid) [poly(U)] and poly(xanthidylic acid) [poly(X)] strongly stimulate the IF-2-dependent binding of fMet-tRNA to 30-S ribosomal subunits from Escherichia coli [Van der Laken et al. (1979) FEBS Lett. 100, 230–234]. The N-formylmethionine moiety is incorporated into poly(phenylalanine) upon subsequent addition of other components required for protein synthesis when poly(U) is used as template. This paper shows that N-acetylated Phe-tRNAPhe (AcPhe-tRNA), but not Phe-tRNAPhe or tRNAPhe, competes with fMet-tRNA for binding to poly(U)-programmed 30-S ribosomal subunits. The two species of N-blocked aminoacyl-tRNA are bound to poly(U)-programmed and poly(X)-programmed 30-S subunits in a ratio that is linearly dependent on the ratio of the two species added. With poly(U) as template there is no apparent preference for either fMet-tRNA or AcPhe-tRNA, whereas with poly(X) there is a 2–3-fold preference for fMet-tRNA. The initiation factor IF-2, which is strictly required for the binding of N-blocked aminoacyi-tRNAs, has a higher affinity for fMet-tRNA than for AcPhe-tRNA. It is concluded that (a) interaction of the 30-S ribosomal subunit with poly(U) or poly(X) leads to IF-2-dependent binding of N-blocked aminoacyl-tRNA; (b) the initiation factor IF-2 discriminates in favour of fMet-tRNA; (c) the presence of the cognate codon discriminates in favour of the corresponding N-blocked aminoacyl-tRNA. [ABSTRACT FROM AUTHOR]
- Published
- 1980
- Full Text
- View/download PDF
39. Complete Amino-Acid Sequences of DNA-Binding Proteins HU-1 and HU-2 from <em>Escherichia coli</em>.
- Author
-
Laine, Bernard, Kmiecik, Daniel, Sautiere, Pierre, Biserte, Gérard, and Cohen-Solal, Michel
- Subjects
- *
DNA-binding proteins , *ESCHERICHIA coli , *PEPTIDES , *AMINO acid sequence , *PROTEINS , *HOMOLOGY (Biology) , *HISTONES - Abstract
The DNA-binding protein HU from Escherichia coil is a heterodimer constituted of two poly- peptide chains termed HU-1 and HU-2, of 90 residues each. Their primary structures were established from structural data obtained from tryptic peptides of each monomer in addition to the structural data provided by the automated Edman degradation of the dimer and by peptides derived from cleavage of the dimer with trypsin, chymotrypsin, V8 staphylococcal protease and dilute acid. The results presented in this paper confirm the amino-terminal and carboxy-terminal sequences of the dimer HU reported previously [Laine et al. (1978) FEBS Lett. 89, 116–120]. The amino acid sequences of proteins HU-1 and HU-2 are identical to those of proteins NS-1 and NS-2 respectively, determined independently by Mende et al. [FEBS Lett. (1978) 96, 395–398]. The amino acid sequences of proteins HU-1 and HU-2 are closely related but differ by 28 residues. These proteins are characterized by their high content of hydrophobic residues represented mostly by alanine. In both proteins, half of the basic residues are scattered along the polypeptide chain and the remainder is found within two short sequences located in the carboxy-terminal part of the molecule. No sequence homology could be established between the proteins HU-1 and HU-2 and any one of the five histones from different eukaryotes. [ABSTRACT FROM AUTHOR]
- Published
- 1980
- Full Text
- View/download PDF
40. The Complete Nucleotide Sequence of the Ribosomal 16-S RNA <em>Escherichia coli</em>.
- Author
-
Carbon, Philippe, Ehresmann, Chantal, Ehresmann, Bernard, and Ebel, Jean-Pierre
- Subjects
- *
NUCLEOTIDE sequence , *RNA , *ESCHERICHIA coli , *DNA , *RIBOSOMES - Abstract
The complete nucleotide sequence of the 16-S RNA from Escherichia coli has been determined using rapid RNA-sequencing gel methods. The experimental data are fully described in this paper. The specificities of the ribonucleases, especially the ribonuclease PhyI are discussed and the consequences of the persistence of stable secondary structure are considered. The proposed sequence contains 1541 nucleotides and agrees completely with the DNA sequence of the rrnB cistron deduced by Brosius, J., Palmer, M. L., Kennedy, P.J., and Noller, H. F. [Proc. Natl Acad. Sci. U.S.A. (1978) 75, 4801–4805]. But there are several cistron heterogeneities of which we described 16 single-base heterogeneities, 7 of the deletion/insertion type and 9 of the transition or transversion type. Our observations suggest the existence, among the 7 ribosome RNA cistrons, of one or two mutated ones. The respective advantages and disadvantages of both RNA and DNA sequencing methods are discussed. [ABSTRACT FROM AUTHOR]
- Published
- 1979
- Full Text
- View/download PDF
41. Characterisation of the Binding of Virginiamycin S to <em>Escherichia coli</em> Ribosomes.
- Author
-
de Bethune, Marie-Pierre and Nierhaus, Knud H.
- Subjects
- *
ESCHERICHIA coli , *RIBOSOMES , *BIOCHEMISTRY , *BACTERIOLOGY , *MOLECULAR microbiology , *MOLECULAR biology , *BIOLOGY - Abstract
Virginiamycin S is an inhibitor of protein synthesis in vivo. In this paper we show by equilibrium dialysis that it binds specifically to the 50-S subunit of Escherichia coli ribosomes, with one binding site per subunit. This binding is not altered by the presence of chloramphenicol, tetracycline or puromycin but is competed for by erythromycin. Using the splitting-reconstitution method, it could be demonstrated that protein L16 is absolutely required for the binding of virginiamycin S to the 50-S subunit. [ABSTRACT FROM AUTHOR]
- Published
- 1978
- Full Text
- View/download PDF
42. DNA Unwinding Enzyme II of <em>Escherichia coli</em> 2. Characterization of the DNA Unwinding Activity.
- Author
-
Abdel-Monem, Mahmoud, Dorwald, Hildegard, and Hoffmann-Berling, Hartmut
- Subjects
- *
DNA , *ENZYMES , *ESCHERICHIA coli , *ADENOSINE triphosphate , *ADENINE nucleotides , *PHOSPHATES - Abstract
The DNA-stimulated 75 000-Mr ATPase described in the preceding paper is shown to be a further catalytic DNA unwinding principle (DNA unwinding enzyme II) made in Escherichia coli cells (the first being the 180 000-Mr ATPase of the cells: DNA unwinding enzyme I). Unwinding depends, strictly, on the supply of ATP. It occurs only under conditions permitting ATP dephosphorylation and it proceeds as long as enzyme molecules are permitted to enter the enzyme · DNA complex. The enzyme binds specifically to single-stranded DNA yielding a complex of only limited stability. These results are interpreted in terms of a distributive mode of action of the enzyme. It is argued that chain separation starts near a single-stranded DNA region and that, forced by continued adsorption of enzyme molecules to the DNA, it develops along the duplex. This mechanism is different from that deduced previously for DNA unwinding enzyme I. Complicated results were obtained using ATPase prepared from rep3 mutant cells. [ABSTRACT FROM AUTHOR]
- Published
- 1977
- Full Text
- View/download PDF
43. Cell-Wall Lipopolysaccharide of the '<em>Shigella</em>-like' <em>Escherichia coli</em> 058.
- Author
-
Dmitriev, Boris A., Knirel, Yuriy A., Kochetkov, Nikolay K., Jann, Barbara, and Jann, Klaus
- Subjects
- *
ENDOTOXINS , *ESCHERICHIA coli , *SHIGELLA , *POLYSACCHARIDES , *BIOPOLYMERS , *SACCHARIDES - Abstract
Two lipopolysaccharide preparations were obtained from Escherichia coli 058 by extraction with 45% aqueous phenol and fractional precipitation with cetyltrimethyl ammonium bromide (Cetavlon). Chemical analysis and polyacrylamide gel electrophoresis in the presence of sodium dodecylsulfate showed that the two preparations differed only in the extent of the O-specific polysaccharide moiety. The O-specific polysaccharide was characterized with proton magnetic resonance and infrared spectroscopy, optical rotation and paper electrophoresis. Using gas-liquid chromatography and ion-exchange chromatography, it was shown to contain D-mannose, 2-acetamido-2-deoxy-D-glucose, 3-O-(R-1'-carboxyethyl)-L-rhamnose (rhamnolactylic acid), and O-acetyl groups in the molar ratios of 2:1:1:1. The polysaccharide and oligosaccharides obtained from it were subjected to methylation and chromic acid oxidation. The results obtained indicated that the polysaccharide consists of tetrasaccharide repeating units in which the trisaccharide β-GlcNAc1-4αMan-1-4(2/3-O-Ac)-Man is substituted at C-3 of the non-acetylated mannose with rhamnolactylic acid. The repeating units are joined through α-mannosyl-1-3-glucosamine bonds. This structure is identical with that of the cell wall polysaccharide of Shigella dysenteriae type 5. [ABSTRACT FROM AUTHOR]
- Published
- 1977
- Full Text
- View/download PDF
44. Purification and Characterization of the Lytic Enzyme <em>N</em>-Acetylmuramyl-L-alanine Amidase of Bacteriophage T7.
- Author
-
Kleppe, Gunnar, Jensen, B., and Pryme, Ian F.
- Subjects
- *
CHROMATOGRAPHIC analysis , *POLYSACCHARIDES , *ANTIBACTERIAL agents , *ESCHERICHIA coli , *ENZYMES , *B cells , *COLLOIDS - Abstract
The lytic enzyme from bacteriophage T7 has been purified from T7-infected Escherichia coli B cells and characterized. In the purification procedure advantage was taken of the reversible binding of the enzyme to chitin. Molecular weight determinations of the enzyme by Sephadex G-75 chromatography and sodium dodecyl sulphate gel electrophoresis gave estimates of 21000 and 18000 respectively. Because the activity of the enzyme falls rapidly to 1-3% of that observed immediately after lysis of the cells, various means to stabilize the enzyme have been tried. Of the methods attempted only binding to the substrate analogue chitin was successful. The enzymic activity was found to be markedly dependent on ionic strength and pH, maximum activity was observed using 5 mM phosphate buffer pH 7.5. MgCl2 was found to enhance the lytic activity 2–3-fold, the optimal concentration being about 0.5 mM. The enzyme was not sensitive to penicillin G or spermine, but was specifically inhibited by p-chloromercuribenzoate. Following digestion of E. coli peptidoglycan the cell wall peptides L-Ala-D-Glu(A2pm), L-Ala-D-Glu(A2pm-D-Ala) and the dimer of the latter were formed, together with paper chromatographically immobile glycan strands. The enzyme, therefore, acts as an N-acetylmuramyl-L-alanine amidase by cleaving the bond between N-acetylmuramic acid and L-alanine in the E. coli peptidoglycan. The enzyme has apparently no effect on the peptidoglycan from Micrococcus luteus, and seems to have a preference for high-molecular-weight substrates. Thus the disaccharide-tetrapeptide GlcNAc-MurNAc-L-Ala-D-Glu(A2pm-D-Ala) and its dimer are not substrates for the enzyme. [ABSTRACT FROM AUTHOR]
- Published
- 1977
- Full Text
- View/download PDF
45. Characterisation of RNA Fragments Obtained by Mild Nuclease Digestion of 30-S Ribosomal Subunits from <em>Escherichia coli</em>.
- Author
-
Rinke, Jutta, Ross, Alexander, and Brimacombe, Richard
- Subjects
- *
ESCHERICHIA coli , *NUCLEASES , *RNA , *RIBOSOMES , *OLIGONUCLEOTIDES , *NUCLEOPROTEINS - Abstract
When Escherichia coli 30-S ribosomal subunits are hydrolysed under mild conditions, two ribonucleoprotein fragments of unequal size are produced. Knowledge of the RNA sequences contained in these hydrolysis products was required for the experiments described in the preceding paper, and the RNA sub-fragments have therefore been examined by oligonucleotide analysis. Two well-defined small fragments of free RNA, produced concomitantly with the ribonucleoprotein fragments, were also analysed. The larger ribonucleoprotein fragment, containing predominantly proteins S4, S5, S8, S15, S16 (17) and S20, contains a complex mixture of RNA sub-fragments varying from about 100 to 800 nucleotides in length. All these fragments arose from the 5′-terminal 900 nucleotides of 16-S RNA, corresponding to the well-known 12-S fragment. No long-range interactions could be detected within this RNA region in these experiments. The RNA from the smaller ribonucleoprotein fragment (containing proteins S7, S9, S10, S14 and S19) has been described in detail previously, and consists of about 450 nucleotides near the 3′ end of the 16-S RNA, but lacking the 3′-terminal 150 nucleotides. The two small free RNA fragments (above) partly account for these missing 150 nucleotides; both fragments arose from section A of the 16-S RNA, but section J (the 3′-terminal 50 nucleotides) was not found. This result suggests that the 3′ region of 16-S RNA is not involved in stable interactions with protein. [ABSTRACT FROM AUTHOR]
- Published
- 1977
- Full Text
- View/download PDF
46. Isolation of a Strong Suppressor of Nonsense Mutations in <em>Bacillus subtilis</em>.
- Author
-
Mellado, Rafael P., Viñuela, Eladio, and Salas, Margarita
- Subjects
- *
BACILLUS subtilis , *ESCHERICHIA coli , *OCHER , *GENES , *STOICHIOMETRY , *PROTEINS - Abstract
By treatment of Bacillus subtilis MO-101-P spoA- met thr- su- with ethyl methanesulfonate, a strong suppressor strain of nonsense mutations, B. subtilis MO-101-P spoA- [met-]+ thr- su+44, was isolated. This strain does not suppress phage Φ29 mutant susB47, selected on a B. subtilis strain containing the su+3 suppressor isolated by Georgopoulos. A revertant from this mutant, susB610, was isolated, being suppressed by both the su+3 and su+44 suppressor strains. The efficiency of suppression by strain su+44 is about 50%. The experiments shown in this paper suggest that strain su+44 contains an amber and strain su+3 an ochre suppressor. [ABSTRACT FROM AUTHOR]
- Published
- 1976
- Full Text
- View/download PDF
47. Cell-Wall Lipopolysaccharide of the <em>'Shigella</em>-Like' <em>Escherichia coli</em> 0124.
- Author
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Dmitriev, Boris A., Lvov, Vjacheslav L., Kochetkov, Nikolay K., Jann, Barbara, and Jann, Klaus
- Subjects
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GAS chromatography , *ESCHERICHIA coli , *ELECTROPHORESIS , *CHROMATOGRAPHIC analysis , *SPECTRUM analysis , *ELECTROCHEMISTRY , *MAGNETIC fields - Abstract
From Escherichia coli 0124 two lipopolysaccharide preparations were obtained with phenol/water extraction and cetavlon precipitation. Polyacrylamide gel electrophoresis in the presence of sodium dodecylsulfate and chemical analysis showed that the two preparations differed only in the extent of the O-specific polysaccharide moiety. In passive haemagglutination and gel precipitation the two lipopolysaccharide preparations from E. coli 0124 and the corresponding preparations from Shigella dysenteriae type 3 reacted alike. The O-specific polysaccharide moiety was characterized with proton magnetic resonance spectroscopy, optical rotation and paper electrophoresis. The constituents were determined by gas chromatography and ion-exchange chromatography. The polysaccharide contained glucose (Glc), gatactose (Gal), galactosamine (GalN) and 4-O-(1′-carboxyethyl)-D-glucopyranose (glucolactilic acid, GIcLA) in the molar ratios of 1 : 2 : 1 : 1. Glucolactilic acid, which has a structure similar to muramic acid, was first found in Sh. dysenteriae. The polysaccharide from E. coli 0124 and oligosaccharides obtained from it by partial acid hydrolysis were subjected to methylation analysis using the method of combined gas chromatography—mass spectrometry. The results indicated that the pentasaccharide repeating unit of the polysaccharide is[This symbol cannot be presented in ASCII format] In the polysaccharide the repeating units are joined through galactofuranosidic linkages. This structure is identical with that of the somatic polysaccharide of Sh. dysenterae type 3. [ABSTRACT FROM AUTHOR]
- Published
- 1976
- Full Text
- View/download PDF
48. Evidence for an Aminoendopeptidase Localized Near the Cell Surface of <em>Escherichia coli</em>.
- Author
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Lazdunski, Andrée, Murgier, Maryse, and Lazdunski, Claude
- Subjects
- *
ENZYMES , *ALKALINE phosphatase , *MALNUTRITION , *ENTEROBACTERIACEAE , *ESCHERICHIA coli , *ALANINE - Abstract
An enzyme capable of hydrolyzing the substrate L-alanine p-nitroanilide has been found in the various Escherichia coli strains tested. This enzyme has been called aminoendopeptidase since it shows both activities (see accompanying paper). It is released from the cells by osmotic shock and by lysozyme-EDTA spheroplasting treatment, and 50% of the total activity is directly detectable with suspensions of intact cells. However, the release by osmotic shock or spheroplasting is not as efficient as it is for alkaline phosphatase. This periplasmic aminoendopeptidase is constitutively produced but the differential rate of synthesis is increased 4-fold when the cell growth is limited by Pi. The occurrence of this 'derepression' is simultaneous with that of alkaline phosphatase. Increasing the concentration of inorganic phosphate in the medium has no effect on the constitutive aminoendopeptidase synthesis. The effect of phosphate starvation is specific since starvation for neither nitrogen nor carbon and energy source are effective in derepressing aminoendopeptidase. [ABSTRACT FROM AUTHOR]
- Published
- 1975
- Full Text
- View/download PDF
49. Altered α Subunits in Phenylalanyl-tRNA Synthetases from <em>p</em>-Fluorophenylalanine-Resistant Strains of <em>Escherichia coli</em>.
- Author
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Hennecke, Hauke and Böck, August
- Subjects
- *
TRANSFER RNA , *LIGASES , *ALANINE , *ENZYMES , *ESCHERICHIA coli , *ENTEROBACTERIACEAE , *PROTEINS - Abstract
Three different phenylalanyl-tRNA synthetases have been purified to near homogeneity, one from a wild-type strain of Escherichia coli and the others from two independently isolated p-fluorophenylalanine-resistant strains. The mutant enzymes were not able to use p-fluorophenylalanine as a substrate for activation and attachment to tRNA. They proved to be indistinguishable from the wild-type enzyme by several electrophoretic and immunological criteria. The α and β subunits of all three enzymes have been prepared by a method described in this paper. The isolated subunits per se did not reveal any significant enzyme activity, but combined they were able to form active phenylalanyl-tRNA synthetase after a defined reconstitution process. Mixed reconstitution experiments between wild-type and mutant subunits indicate that the mutant a subunit is responsible for p-fluorophenylalanine resistance and therefore seems to carry the phenylalanine-binding site or to participate in its formation. [ABSTRACT FROM AUTHOR]
- Published
- 1975
- Full Text
- View/download PDF
50. Relations between Structure and Function in Cytoplasmic Membrane Vesicles Isolated from an Escherichia coli Fatty-Acid Auxotroph.
- Author
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Shechter, Emanuel, Letellier, Lucienne, and Gulik-Krzywicki, Tadeusz
- Subjects
- *
CELL membranes , *FATTY acids , *ESCHERICHIA coli , *CELLS , *BIOCHEMISTRY - Abstract
The results presented in this paper establish relationships between structural morphological and functional properties of cytoplasmic membrane vesicles isolated from an Escherichia coli unsaturated fatty acid auxotroph. The membranes were isolated from cells grown in the presence of either oleic, linoleic, linolenic or elaidic acids. High-angle X-ray diffraction studies show that the order-disorder transitions induced by temperature variations and associated with the paraffin chains of the lipids are a function of the fatty acid composition of the membranes. In some cases "cocrystallization" of various lipid species takes place within a single type of ordered domains. In other cases there is segregation of various lipid species into more than one distinct type of ordered domain. The various order-disorder transitions observed induce morphological changes in the hydrophobic core of the membranes which can be detected by freeze-etch electron microscopy. A random distribution of particles on the fracture faces is observed when the paraffin chains of the lipids are disordered. Upon ordering of the paraffin chains, particles are excluded from the ordered domains and as a consequence, smooth areas and areas with densely packed particles are observed. The ratio of the smooth surface to particulated surface is proportional to the amount of ordered paraffin chains present. Moreover, the size of the smooth domains is a function of the fatty acid composition of the membranes. Discontinuities in the rate of D-lactate-dependent proline uptake as a function of temperature correlate with the order-disorder transitions observed. The high energies of activation at low temperatures are attributed to decreased mobility of the carrier proteins upon aggregation. In contrast, phosphoenolpyruvate-dependent vectorial phosphorylation does not respond to the ordering of the paraffin chains. [ABSTRACT FROM AUTHOR]
- Published
- 1974
- Full Text
- View/download PDF
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