Your search keyword '"catabolite repression"' showing total 121 results

1. Draft genome sequencing of Sporolactobacillus terrae SBT-1, an efficient bacterium to ferment concentrated sugar to d-lactic acid.

Author

Thitiprasert, Sitanan, Piluk, Jirabhorn, Tolieng, Vasana, Tanaka, Naoto, Shiwa, Yuh, Fujita, Nobuyuki, Tanasupawat, Somboon, and Thongchul, Nuttha

Subjects

*LACTIC acid, *NUCLEOTIDE sequencing, *ENANTIOMERIC purity, *CATABOLITE repression, *ENZYMES, *SUCROSE, *SUGAR

Abstract

Recently, the industrial-scale development of microbial d-lactic acid production has been discussed. In this study, the efficiency of the new isolate Sporolactobacillus terrae SBT-1 for producing d-lactic acid under challenge conditions was investigated. The isolate SBT-1 exhibited superior activity in fermenting a very high glucose or sucrose concentration to d-lactic acid compared to the other S. terrae isolates previously reported in the literature; therefore, SBT-1 could overcome the limitations of effective lactic acid production. In batch cultivation using 360 g/L glucose, SBT-1 produced 290.30 g/L d-lactate with a sufficiently high glucose conversion yield of 86%, volumetric productivity of 3.02 g/L h, and optical purity of 96.80% enantiomer excess. SBT-1 could also effectively utilize 440 g/L sucrose as a sole carbon source to produce 276.50 g/L lactic acid with a conversion yield of 90%, a production rate of 2.88 g/L h, and an optical purity of 98%. d-Lactic acid fermentation by two other related producers, S. inulinus NRIC1133T and S. terrae NRIC0357T, was compared with fermentation by isolate SBT-1. The experimental data revealed that SBT-1 possessed the ability to ferment relatively high glucose or sucrose concentrations to d-lactic acid without obvious catabolite repression and byproduct formation compared to the two reference strains. In draft genome sequencing of S. terrae SBT-1, the results provided here can promote further study to overcome the current limitations for the industrial-scale production of d-lactic acid. [ABSTRACT FROM AUTHOR]

Published

2021

2. The role of stress in colicin regulation.

Author

Ghazaryan, Lusine, Tonoyan, Lilit, Ashhab, Ashraf, Soares, M., and Gillor, Osnat

Subjects

*COLICINS, *BACTERIOCINS, *ENTEROBACTERIACEAE, *MOLECULAR weights, *NUCLEIC acids, *CATABOLITE repression, *OXIDATIVE stress, *BACTERIA

Abstract

Bacteriocins produced by Enterobacteriaceae are high molecular weight toxic proteins that kill target cells through a variety of mechanisms, including pore formation and nucleic acid degradation. What is remarkable about these toxins is that their expression results in death to the producing cells and therefore bacteriocin induction have to be tightly regulated, often confined to times of stress. Information on the regulation of bacteriocins produced by enteric bacteria is sketchy as their expression has only been elucidated in a handful of bacteria. Here, we review the known regulatory mechanisms of enteric bacteriocins and explore the expression of 12 of them in response to various triggers: DNA-damaging agents, stringent response, catabolite repression, oxidative stress, growth phase, osmolarity, cold shock, nutrient deprivation, anaerobiosis and pH stress. Our results indicate that the expression of bacteriocins is mostly confined to mutagenic triggers, while all other triggers tested are limited inducers. [ABSTRACT FROM AUTHOR]

Published

2014

3. Draft genome sequencing of Sporolactobacillus terrae SBT-1, an efficient bacterium to ferment concentrated sugar to D-lactic acid

Author

Sitanan Thitiprasert, Nuttha Thongchul, Somboon Tanasupawat, Nobuyuki Fujita, Yuh Shiwa, Vasana Tolieng, Naoto Tanaka, and Jirabhorn Piluk

Subjects

Sucrose, Catabolite repression, Biochemistry, Microbiology, 03 medical and health sciences, chemistry.chemical_compound, Genetics, Food science, Lactic Acid, Enantiomeric excess, Sugar, Molecular Biology, 030304 developmental biology, 0303 health sciences, Bacillales, biology, 030306 microbiology, Chemistry, food and beverages, General Medicine, biology.organism_classification, Lactic acid, Glucose, Yield (chemistry), Fermentation, Sugars, Bacteria, Genome, Bacterial

Abstract

Recently, the industrial-scale development of microbial d-lactic acid production has been discussed. In this study, the efficiency of the new isolate Sporolactobacillus terrae SBT-1 for producing d-lactic acid under challenge conditions was investigated. The isolate SBT-1 exhibited superior activity in fermenting a very high glucose or sucrose concentration to d-lactic acid compared to the other S. terrae isolates previously reported in the literature; therefore, SBT-1 could overcome the limitations of effective lactic acid production. In batch cultivation using 360 g/L glucose, SBT-1 produced 290.30 g/L d-lactate with a sufficiently high glucose conversion yield of 86%, volumetric productivity of 3.02 g/L h, and optical purity of 96.80% enantiomer excess. SBT-1 could also effectively utilize 440 g/L sucrose as a sole carbon source to produce 276.50 g/L lactic acid with a conversion yield of 90%, a production rate of 2.88 g/L h, and an optical purity of 98%. d-Lactic acid fermentation by two other related producers, S. inulinus NRIC1133T and S. terrae NRIC0357T, was compared with fermentation by isolate SBT-1. The experimental data revealed that SBT-1 possessed the ability to ferment relatively high glucose or sucrose concentrations to d-lactic acid without obvious catabolite repression and byproduct formation compared to the two reference strains. In draft genome sequencing of S. terrae SBT-1, the results provided here can promote further study to overcome the current limitations for the industrial-scale production of d-lactic acid.

Published

2020

4. Succinate irrepressible periplasmic glucose dehydrogenase of Rhizobium sp. Td3 and SN1 contributes to its phosphate solubilization ability

Author

Bhagya Iyer and Shalini Rajkumar

Subjects

Calcium Phosphates, Succinic Acid, Catabolite repression, chemistry.chemical_element, Calcium, Gluconates, Biochemistry, Microbiology, Phosphates, Rhizobia, 03 medical and health sciences, chemistry.chemical_compound, Cajanus, Sesbania rostrata, Glucose dehydrogenase, Sesbania, Genetics, Molecular Biology, 030304 developmental biology, 0303 health sciences, biology, 030306 microbiology, Glucose 1-Dehydrogenase, General Medicine, Periplasmic space, biology.organism_classification, Phosphate, Glucose, chemistry, Gluconic acid, Rhizobium

Abstract

Td3 and SN1 are phosphate-solubilizing nodule rhizobia of Cajanus cajan and Sesbania rostrata, respectively. They solubilized 423 µg/mL and 428 µg/mL phosphate from tricalcium phosphate through the secretion of 19.2 mM and 29.6 mM gluconic acid, respectively, when grown in 100 mM glucose. However, 90% and 80% reduction in phosphate solubilization coupled to the production of 40 mM (Td3) and 28.2 mM (SN1) gluconic acid was observed when the two isolates were grown in 50 mM succinate + 50 mM glucose. Our results illustrate the role of succinate irrepressible glucose dehydrogenase (gcd) in phosphate solubilization and the role of succinate: proton symport in succinate-mediated repression of phosphate solubilization in these rhizobia. Calcium ion supplementation reduced the 88% and 72% repression in P solubilization to 18% and 9% in Td3 and SN1, respectively, coupled to a reduction in media pH from 6.8 to 4.9 in Td3 and 6.3 to 4.8 in SN1. Hence, repression had no genetic basis and is purely due to the biochemical interplay of protons and other cations.

Published

2019

5. Repression of oxalic acid-mediated mineral phosphate solubilization in rhizospheric isolates of Klebsiella pneumoniae by succinate.

Author

Rajput, Mahendrapal, Naresh Kumar, G., and Rajkumar, Shalini

Subjects

*OXALIC acid, *SOLUBILIZATION, *KLEBSIELLA, *ENTEROBACTERIACEAE, *CATABOLITE repression, *GLUCOSE

Abstract

Two strains of Klebsiella (SM6 and SM11) were isolated from rhizospheric soil that solubilized mineral phosphate by secretion of oxalic acid from glucose. Activities of enzymes for periplasmic glucose oxidation (glucose dehydrogenase) and glyoxylate shunt (isocitrate lyase and glyoxylate oxidase) responsible for oxalic acid production were estimated. In presence of succinate, phosphate solubilization was completely inhibited, and the enzymes glucose dehydrogenase and glyoxylate oxidase were repressed. Significant activity of isocitrate lyase, the key enzyme for carbon flux through glyoxylate shunt and oxalic acid production during growth on glucose suggested that it could be inducible in nature, and its inhibition by succinate appeared to be similar to catabolite repression. [ABSTRACT FROM AUTHOR]

Published

2013

6. Transcriptional analysis and functional characterization of XCC1294 gene encoding a GGDEF domain protein in Xanthomonas campestris pv. campestris.

Author

Hsiao, Yi-Min, Song, Wan-Ling, Liao, Chao-Tsai, Lin, I-Hsuan, Pan, Mei-Ying, and Lin, Ching-Fen

Subjects

*XANTHOMONAS campestris, *GENE expression, *CATABOLITE repression, *ESCHERICHIA coli, *POLYSTYRENE

Abstract

The nucleotide cyclic di-GMP is a second messenger in bacteria that regulates a range of cellular functions including the virulence of pathogens. GGDEF is a protein domain involved in the synthesis of cyclic di-GMP. The genome of the crucifer pathogen Xanthomonas campestris pv. campestris (Xcc) encodes 21 proteins with a GGDEF domain. Clp, a homolog of the model transcription factor Crp of Escherichia coli, is a global regulator in Xcc. The aim of this study is to identify genes encoding GGDEF domain proteins whose expression is regulated by Clp. Results of reporter assay and RT-PCR analysis suggested that Clp regulates the expression of a set of genes encoding proteins harboring GGDEF domain. The transcription initiation site of XCC1294, one of the Clp regulated gene encoding a GGDEF domain protein, was mapped. Promoter analysis and gel retardation assay indicated that the transcription of XCC1294 is positively and directly regulated by Clp. Furthermore, transcription of XCC1294 was subject to catabolite repression and affected by several stress conditions. We also showed that mutation of XCC1294 results in enhanced surface attachment. In addition, transcription of three putative adhesin genes ( xadA, fhaC, and yapH) was increased in the XCC1294 mutant. Taken together, the data presented here indicate that Clp positively regulates expression of XCC1294, and that XCC1294 serves a regulator of bacterial attachment and regulates different adhesin genes expression. [ABSTRACT FROM AUTHOR]

Published

2012

7. Transcriptional regulation of the acetyl-CoA synthetase gene acsA in Pseudomonas aeruginosa.

Author

Kretzschmar, Utta, Khodaverdi, Viola, and Adrian, Lorenz

Subjects

*PSEUDOMONAS aeruginosa, *ACETYLCOENZYME A, *GENES, *ENZYMES, *ALCOHOL

Abstract

Pseudomonas aeruginosa ATCC 17933 is able to oxidize ethanol to acetate under aerobic conditions. The P. aeruginosa acetyl-CoA synthetase (ACS) gene acsA was previously identified, and the ACS enzyme described to be required for growth on ethanol as the sole source of carbon and energy. Here, we investigated the transcriptional regulation of the acsA gene using an acsA:: lacZ fusion. Transcription of acsA was regulated by the carbon source, and expression was maximal on ethanol, acetate and propionate. In addition, the induction depended on the response regulator ErdR, which also regulates hierarchically arranged genes for ethanol oxidation. Transcription of the acsA gene was repressed by addition of succinate to an ethanol-containing medium. This repression required Crc, the product of the catabolite repression control gene crc. [ABSTRACT FROM AUTHOR]

Published

2010

8. The role of TrmB and TrmB-like transcriptional regulators for sugar transport and metabolism in the hyperthermophilic archaeon Pyrococcus furiosus.

Author

Sung-Jae Lee, Surma, Melanie, Hausner, Winfried, Thomm, Michael, and Boos, Winfried

Subjects

*GENES, *HEREDITY, *SUGARS, *ENZYMES, *PROTEINS, *ENZYMOLOGY, *CATALYSTS, *BIOCHEMISTRY, *SUCROSE

Abstract

TrmB of Pyrococcus furiosus was discovered as the trehalose/maltose-specific repressor for the genes encoding the trehalose/maltose high-affinity ABC transporter (the TM system). TrmB also represses the genes encoding the high affinity maltodextrin-specific ABC transporter (the MD system) with maltodextrin and sucrose as inducers. In addition, TrmB binds glucose leading to an increased repression of both, the TM and the MD system. Thus, TrmB recognizes different promoters and depending on the promoter it will be activated or inactivated for promoter binding by different sugar effectors. The TrmB-like protein TrmBL1 of P. furiosus is a global regulator and recognizes preferentially, but not exclusively, the TGM (for Thermococcales–glycolytic motif) sequence that is found upstream of the MD system as well as of genes encoding enzymes involved in the glycolytic and the gluconeogenic pathway. It responds to maltose and maltotriose as inducers and functions as repressor for the genes encoding the MD system and glycolytic enzymes, but as activator for genes encoding gluconeogenic enzymes. The TrmB-like protein TrmBL2 of P. furiosus lacks the sugar-binding domain that has been determined in TrmB. It recognizes the MD promoter, but not all TGM harboring promoters. It is evolutionary the most conserved among the Thermococcales. The regulatory range of TrmBL2 remains unclear. [ABSTRACT FROM AUTHOR]

Published

2008

9. Regulation of citB expression in Bacillus subtilis: integration of multiple metabolic signals in the citrate pool and by the general nitrogen regulatory system.

Author

Blencke, Hans-Matti, Reif, Irene, Commichau, Fabian M., Detsch, Christian, Wacker, Ingrid, Ludwig, Holger, and Stülke, Jörg

Subjects

*BACILLUS subtilis, *BACILLUS (Bacteria), *KREBS cycle, *METABOLISM, *CARBON, *GLUTAMINE

Abstract

The tricarboxylic acid (TCA) cycle is one of the major routes of carbon catabolism in Bacillus subtilis. The syntheses of the enzymes performing the initial reactions of the cycle, citrate synthase, and aconitase, are synergistically repressed by rapidly metabolizable carbon sources and glutamine. This regulation involves the general transcription factor CcpA and the specific repressor CcpC. In this study, we analyzed the expression and intracellular localization of CcpC. The synthesis of citrate, the effector of CcpC, requires acetyl-CoA. This metabolite is located at a branching point in metabolism. It can be converted to acetate in overflow metabolism or to citrate. Manipulations of the fate of acetyl-CoA revealed that efficient citrate synthesis is required for the expression of the citB gene encoding aconitase and that control of the two pathways utilizing acetyl-CoA converges in the control of citrate synthesis for the induction of the TCA cycle. The citrate pool seems also to be controlled by arginine catabolism. The presence of arginine results in a severe CcpC-dependent repression of citB. In addition to regulators involved in sensing the carbon status of the cell, the pleiotropic nitrogen-related transcription factor, TnrA, activates citB transcription in the absence of glutamine. [ABSTRACT FROM AUTHOR]

Published

2006

10. Xylose and some non-sugar carbon sources cause catabolite repression in Saccharomyces cerevisiae.

Author

Belinchón, Mónica M. and Gancedo, Juana M.

Subjects

*SACCHAROMYCES cerevisiae, *METABOLITES, *CARBON, *SACCHAROMYCETACEAE, *GLUCOSE, *MALTOSE

Abstract

Glucose and other sugars, such as galactose or maltose, are able to cause carbon catabolite repression in Saccharomyces cerevisiae. Although glycolytic intermediates have been suggested as signal for repression, no evidence for such a control mechanism is available. The establishment of a correlation between levels of intracellular metabolites and the extent of catabolite repression may facilitate the identification of potential signal molecules in the process. To set a framework for such a study, the repression produced by xylose, glycerol and dihydroxyacetone upon genes belonging to different repressible circuits was tested, using an engineered strain of S. cerevisiae able to metabolize xylose. Xylose decreased the derepression of various enzymes in the presence of ethanol by at least 10-fold; the corresponding mRNAs were not detected in these conditions. Xylose also impaired the derepression of galactokinase and invertase. Glycerol and dihydroxyacetone decreased 2- to 3-fold the derepression observed in ethanol or galactose but did not affect invertase derepression. For yeast cells grown in media with different carbon sources, no correlation was found between repression of fructose-1,6-bisphosphatase and intracellular levels of glucose 6-phosphate or fructose 1,6-bisphosphate. [ABSTRACT FROM AUTHOR]

Published

2003

11. Induction of butane consumption in Pseudomonas butanovora.

Author

Sayavedra-Soto, Luis A., Byrd, Chelsea M., and Arp, Daniel J.

Subjects

BUTANE, METABOLISM, PSEUDOMONAS, PSEUDOMONADACEAE, ENZYME induction, GENETIC regulation, MICROBIOLOGY, BIOLOGY

Abstract

The induction of the enzyme activities involved in butane metabolism in Pseudomonas butanovora was characterized. P. butanovora was grown on butane or its metabolites, both singly and in mixtures with other growth substrates. Cells grown in each of the butane metabolites readily consumed the growth substrate and downstream metabolites, but consumed the upstream butane metabolites more slowly. Upstream activities in the butane metabolism could be induced by downstream metabolites, but to much lower levels than with the primary substrate. The induction of butane oxidation was not repressed when P. butanovora was grown or incubated in a mixture of butane and 1-butanol, butyraldehyde or butyrate. However, no induction of butane consumption was observed in a mixture of butane and lactate, which is indicative of catabolite repression. In lactate-grown cells that were rid of the growth substrate and incubated with butane and acetylene (to inactivate newly formed butane monooxygenase), the consumption of butane, 1-butanol and butyraldehyde consumption was not induced. The overall results suggest an independent regulatory mechanism for each of the enzyme activities in butane metabolism. In addition, a low, constitutive butane oxidation was observed in cells grown on substrates other than butane metabolites. [ABSTRACT FROM AUTHOR]

Published

2001

12. Characterization of glucose-repression-resistant mutants of Bacillus subtilis: identification of the glcR gene.

Author

Stülke, Jörg, Martin-Verstraete, I., Glaser, P., and Rapoport, G.

Subjects

BACILLUS subtilis, BACILLUS (Bacteria), BACILLACEAE, GRAM-positive bacteria, METABOLISM, PHOSPHOTRANSFERASES, TRANSFERASES

Abstract

In Bacillus subtilis, carbon catabolite repression (CCR) is mediated by the pleiotropic repressor CcpA and by ATP-dependent phosphorylation of the HPr protein of the phosphotransferase system (PTS). In this study, we attempted to identify novel genes that are involved in the signal transduction pathway that ultimately results in CCR in the presence of repressing carbon sources such as glucose. Seven mutants resistant to glucose repression of the levanase operon were isolated and characterized. All mutations were trans-acting and pleiotropic as determined by analyzing CCR of β-xylosidase and of the sacPA and bglPH operon. Moreover, all mutations specifically affected repression exerted by glucose but not by other sugars. The mutations were mapped to three different loci on the genetic map, ptsG, glcR, and pgi. These three genes encode proteins involved in glucose metabolism. A novel repressor gene, glcR (ywpI), defined by two mutations, was studied in more detail. The glcR mutants exhibit loss of glucose repression of catabolic operons, a deficiency in glucose transport, and absence of expression of the ptsG gene. The mutant GlcR proteins act as super-repressors of ptsG expression. [ABSTRACT FROM AUTHOR]

Published

2001

13. Two distinct pathways for anaerobic degradation of aromatic compounds in the denitrifying bacterium Thauera aromatica strain AR-1.

Author

Philipp, Bodo and Schink, Bernhard

Subjects

DENITRIFYING bacteria, DENITRIFICATION, AROMATIC compounds, ANAEROBIOSIS, BIODEGRADATION, CHEMICAL reduction

Abstract

Denitrifying bacteria degrade many different aromatic compounds anaerobically via the well-described benzoyl-CoA pathway. We have shown recently that the denitrifiers Azoarcus anaerobius and Thauera aromatica strain AR-1 use a different pathway for anaerobic degradation of resorcinol (1,3-dihydroxybenzene) and 3,5-dihydroxybenzoate, respectively. Both substrates are converted to hydroxyhydroquinone (1,2,4-trihydroxybenzene). In the membrane fraction of T. aromatica strain AR-1 cells grown with 3,5-dihydroxybenzoate, a hydroxyhydroquinone-dehydrogenating activity of 74 nmol min–1(mg protein)–1 was found. This activity was significantly lower in benzoate-grown cells. Benzoate-grown cells were not induced for degradation of 3,5-dihydroxybenzoate, and cells grown with 3,5-dihydroxybenzoate degraded benzoate only at a very low rate. With a substrate mixture of benzoate plus 3,5-dihydroxybenzoate, the cells showed diauxic growth. Benzoate was degraded first, while complete degradation of 3,5-dihydroxybenzoate occurred only after a long lag phase. The 3,5-dihydroxybenzoate-oxidizing and the hydroxyhydroquinone-dehydrogenating activities were fully induced only during 3,5-dihydroxybenzoate degradation. Synthesis of benzoyl-CoA reductase appeared to be significantly lower in 3,5-dihydroxybenzoate-grown cells as shown by immunoblotting. These results confirm that T. aromatica strain AR-1 harbors, in addition to the benzoyl-CoA pathway, a second, mechanistically distinct pathway for anaerobic degradation of aromatic compounds. This pathway is inducible and subject to catabolite repression by benzoate. [ABSTRACT FROM AUTHOR]

Published

2000

14. The induction and repression of benzene and catechol oxidizing capacity of Pseudomonas putida ML2 studied in perturbed chemostat culture.

Author

Mason, Jeremy

Abstract

The oxidation of catechol, an intermediate in benzene catabolism, was studied using transient variations in dissolved oxygen tension (DOT) when a succinate limited steady state culture of Pseudomonas putida ML2 was perturbed with a pulse of another substrate. A model was developed and tested for the effect of fluctuations in oxidizing enzyme activity on DOT. It was found that the rate of induction of catechol oxidizing enzymes was independent of dilution rate up to a relative growth rate μ/μ of 0.75. Only at higher dilution rates was catabolite repression observed. [ABSTRACT FROM AUTHOR]

Published

1994

15. Release of glucose-mediated catabolite repression due to a defect in the membrane fraction of phosphoenolpyruvate: mannose phosphotransferase system in Pediococcus halophilus.

Author

Abe, Keietsu and Uchida, Kinji

Abstract

A spontaneous mutant 9R-4 resistant to 2-deoxyglucose (2DG) was derived from a wild-type strain Pediococcus halophilus I-13. Phosphoenolpyruvate (PEP)-dependent glucose-6-phosphate formation by the permeabilized 9R-4 cells was < 5% of that observed with the parent I-13. In vitro complementation of PEP-dependent 2DG-6-phosphate formation was assayed with combination of the cytoplasmic and membrane fractions prepared from the I-13 and the mutants (9R-4, and X-160 isolated from nature), which were defective in PEP: mannose phosphotransferase system (man:PTS). The defects in man:PTS of both the strain 9R-4 and X-160 were restricted to the membrane fraction (e.g. EII), not to the cytoplasmic one. Kinetic studies on the glucose transport with intact cells and iodoacetate-treated cells also supported the presence of two distinct transport systems in this bacterium as follows: (i) The wild-type I-13 possessed a high-affinity man:PTS ( K=11 μM) and a low-affinity proton motive force driven glucose permease (GP) ( K=170 μM). (ii) Both 9R-4 and X-160 had only the low-affinity system ( K=181 μM for 9R-4, 278 μM for X-160). In conclusion, a 2DG-induced selective defect in the membrane component (EII) of the man:PTS could partially release glucose-mediated catabolite repression but not frutose-mediated catabolite repression in soy pediococci. [ABSTRACT FROM AUTHOR]

Published

1991

16. Methanol and ethanol utilization in methylotrophic yeast Pichia pinus wild-type and mutant strains.

Author

Sibirny, A., Titorenko, V., Teslyar, G., Petrushko, V., and Kucher, M.

Abstract

In the wild-type strain of methylotrophic yeast Pichia pinus diauxic growth is observed during cultivation in medium containing a mixture of methanol and ethanol: firstly, 'slow' phase of ethanol utilization is revealed and, secondly, a 'fast' phase of methanol consumption is shown. Diauxic growth is observed also in ecr1 mutant, impaired in ethanol-induced catabolite repression of methylotrophic metabolism enzymes, but the order of utilization of the alcohols is inverted in this mutant. Such succession of alcohols utilization in both strains correlates well with the sequence of synthesis of microbody enzymes which catalyze key reactions of C- and C-metabolism. On the contrary, simultaneous utilization of methanol and ethanol from the mixture, as well as synchronous synthesis of both peroxisomal and glyoxisomal enzymes is observed in adh1 mutant which has reduced alcohol dehydrogenase activity. The strong differences between the wild-type strain and adh1 mutant were observed also in the kinetics of specific activity changes for C-metabolizing enzymes, localized in cytosol. In the wild-type strain during growth on methanol and ethanol mixture such changes correlate with the sequence of alcohol utilization. At the same time, in adh1 mutant the activities of formaldehyde dehydrogenase and formate dehydrogenase during the growth on the alcohols mixture are as high as during growth on methanol only, but the activity of dihydroxyacetone kinase is as low as under the growth on ethanol and is lower than on methanol. [ABSTRACT FROM AUTHOR]

Published

1991

17. Cloning and sequence of the mdh structural gene of Escherichia coli coding for malate dehydrogenase.

Author

Vogel, R., Entian, K., and Mecke, D.

Abstract

The malate dehydrogenase gene of Escherichia coli, which is susceptible to catabolite and anaerobic repression, has been cloned using plasmic pLC32-38 of Clarke and Carbon (1976). The nucleotide sequence was determined of a 2.47 kbp fragment, containing the mdh structural gene. All information necessary for expression of the mdh structural gene was mapped within a 1.3 kbp SphI-BstEII fragment. Compared with the untransformed wild type, transformations with pUC19 vector, containing this fragment, gave up to 40-fold more malate dehydrogenase activity in both E. coli wild type and mdh mutant recipients. Catabolite repression was not affected in the transformants. A possible CRP binding site in the promotor region of the mdh gene provides evidence for a co-regulation with fumA gene, the structural gene of fumarase, which is also subject to catabolite repression. The structures for transcription initiation and termination were similar to those previously described for E. coli. Amino acid sequence homologies between pro- and eucaryotic malate dehydrogenases are discussed. [ABSTRACT FROM AUTHOR]

Published

1987

18. On the role of cyclic AMP and the Fnr protein in Escherichia coli growing anaerobically.

Author

Unden, G. and Duchene, A.

Abstract

The role of adenosine 3′,5′-monophosphate (cAMP) and of the Fnr protein, a transcriptional regulator of anearobic electron transport, in the expression of anaerobic respiration of Escherichia coli was investigated. Under conditions of fermentation or anaerobic respiration intracellular cAMP was formed in concentrations up to 4.6 nmol/g protein. From the enzymes of the anaerobic electron transfer chain from glycerol-3-P to fumarate only the expression of glycerol-3-P dehydrogenase (Freedberg WB, Lin ECC (1973) J Bacteriol 115:816-823), but not that of fumarate reductase required cAMP. Isolated Fnr protein, which has been suggested to be an additional site of action of cAMP under anaerobic conditions did not bind cAMP. It is concluded that cAMP in anaerobic growth like in aerobic growth acts as the effector of CRP and that catabolite repression plays an important regulatory role in anaerobic catabolism. The Fnr protein was present in constant amounts (0.06 mg/g cellular protein) and in constant molar mass ( M 30000) in aerobically and in anaerobically grown bacteria. This result excluded regulation of the activity of the Fnr protein by a change of concentration or by processing of the protein. [ABSTRACT FROM AUTHOR]

Published

1987

19. Enterotoxin A production in Staphylococcus aureus: inhibition by glucose.

Author

Smith, J., Bencivengo, M., Buchanan, R., and Kunsch, C.

Abstract

In this study, we investigated the relationship between carbohydrate metabolism and repression of staphylococcus enterotoxin A (SEA) in Staphylococcus aureus 196E and a pleiotrophic mutant derived from strain 196E. The mutant, designated at strain 196E-MA, lacked a functional phosphoenolpyruvate phosphotransferase system (PTS). The mutant produced acid, under aerobic conditions, from only glucose and glycerol. The parent strain contained an active PTS, and aerobically produced acid from a large number of carbohydrates. Prior growth in glucose led to repression of SEA synthesis in the parent strain; addition to the casamino acids enterotoxin production medium (CAS) led to more severe repression of toxin synthesis. The repression was not related to pH decreases produced by glucose metabolism. When S. aureus 196E was grown in the absence of glucose, there was inhibition of toxin production as glucose level was increased in CAS. The inhibition was related to pH decrease and was unlike the repression observed with glucose-grown strain 196E. The inhibition of SEA synthesis in mutant strain 196E-MA was approximately the same in cells grown with or without glucose and was pH related. Repression of SEA synthesis similar to that seen with glucose-grown S. aureus 196E could not be demonstrated in the mutant. In addition, glucose-grown S. aureus 196E neither synthesized β-galactosidase nor showed respiratory activity with certain tricarboxylic acid (TCA) cycle compounds. Glucose-grown strain 196E-MA, however, did not show supressed respiration of TCA cycle compounds; β-galactosidase was not synthesized because the mutant lacked a functional PTS. Cyclic adenosine-3′, 5′-monophosphate did not reverse the repression by glucose of SEA or β-galactosidase synthesis in glucose-grown S. aureus 196E. An active PTS appears to be necessary to demonstrate glucose (catabolite) repression in S. aureus. [ABSTRACT FROM AUTHOR]

Published

1986

20. Differential sensitivities to glucose and galactose repression of gluconeogenic and respiratory enzymes from Saccharomyces cerevisiae.

Author

Herrero, P., Fernández, R., and Moreno, F.

Abstract

The synthesis of isocitrate lyase was induced by the presence of ethanol in the chemostat reaching a specific activity of 200 mU·mg at this induced state. In glucoselimited, derepressed cells, 20 mU·mg were detected and under repressed conditions isocitrate lyase activity was not detected. The sensitivity of gluconeogenic enzymes: cytoplasmic malate dehydrogenase; fructose 1,6-bisphosphatase and isocitrate lyase as well as the mitochondrial enzymes NADH dehydrogenase and succinate cytochrome c oxidase to glucose and galactose repression were studied in chemostat cultures. Our results show that galactose was less effective as a repressor than glucose. Malate dehydrogenase was completely inactivated by glucose, whereas galactose only produced a 78% decrease of specific activity. Fructose 1,6-bisphosphatase and isocitrate lyase were completely inactivated by both sugars but at different rate. Glucose produced an 85% decrease of specific activity of the mitochondrial enzymes whereas galactose only decrease an 67%. [ABSTRACT FROM AUTHOR]

Published

1985

21. Regulation of the β-ketoadipate pathway in Rhizobium japonicum and bacteroids by succinate.

Author

Röhm, Mechthild and Werner, Dietrich

Abstract

Rhizobium japonicum 61-A-101 and its bacteroids catabolize phenol and p-hydroxybenzoate. With phenol as a carbon source, utilization started only after a prolonged lag phase while p-hydroxybenzoate was almost instantancously metabolized. Succinate, which supports rapid growth of Rhizobium japonicum, completely repressed respication of phenol; the oxidation of p-hydroxybenzoate was partially inhibited. Pyruvate, supporting slower growth than succinate, retarded the onset of phenol consumption but did not affect its maximum rate. Catabolite repression of phenol utilization by succinate appears to be a characteristic feature of rhizobia. In Pseudomonas putida which also actively metabolizes phenol, succinate had no effect on phenol utilization. [ABSTRACT FROM AUTHOR]

Published

1985

22. The effect of gyrase inhibitors and cyclic AMP on induction and glucose repression of the 6-hydroxy-nicotine oxidases in Arthrobacter oxidans.

Author

Brandsch, Roderich and Decker, Karl

Abstract

The induction by d,l-nicotine of the enantiozymes 6-hydroxy- L-nicotine oxidase and 6-hydroxy- D-nicotine oxidase in Archrobacter oxidans was differently affected by the inhibitors of Escherichia coli gyrase, novobiocin and nalidixic acid. These compounds inhibited 6-hydroxy- L-nicotine oxidase induction slightly, but led to an increase in the level of 6-hydroxy- D-nicotine oxidase activity. Furthermore, the specific repression by glucose of 6-hydroxy- D-nicotine oxidase synthesis was not abolished by the addition of cAMP but by that of novobiocin. [ABSTRACT FROM AUTHOR]

Published

1982

23. Histidine utilization by Alcaligenes eutrophus: Regulation of histidase formation under heterotrophic conditions of growth.

Author

Schlesier, Michael and Friedrich, Bärbel

Abstract

Histidine supported good growth of Alcaligenes eutrophus strain H 16 as a nitrogen source, but only poor growth as a carbon and energy source. The facultative chemolithoautotrophic bacterium was also able to utilize urocanic acid, the first intermediate of histidine catabolism. The products of histidine degradation were ammonium, formate and glutamate. Three enzymes of the pathway, histidase, urocanase and formiminoglutamate hydrolase, were present in histidine-grown cells. Two types of spontaneous mutants, derived from the wild type, were characterized by an increased growth rate on histidine. One of these types was found to produce histidase constitutively and at a higher activity compared with the parental strain. The second type of mutant had apparently gained an improved histidine uptake system, which is supposed to be growth rate-limiting in the wild type. From the physiological studies the conclusion was drawn that the control of histidine-degrading enzymes is based on induction by urocanate and catabolite repression by carbon sources supporting fast growth, such as succinate or pyruvate. Ammonium was found not to affect catabolite repression, however, we obtained evidence that histidine uptake is subject to a nitrogen control. [ABSTRACT FROM AUTHOR]

Published

1982

24. Regulation of proline catabolism in Pseudomonas aeruginosa PAO.

Author

Meile, Leo, Soldati, Leda, and Leisinger, Thomas

Abstract

Mutants of Pseudomonas aeruginosa deficient in the utilization of l-proline as the only carbon and nitrogen source have been found to be defective either in proline dehydrogenase activity or in both proline dehydrogenase and Δ-pyrroline-5-carboxylate dehydrogenase activities of the bifunctional proline degradative enzyme. The latter type of mutants was unable to utilize l-ornithine, indicating that a single Δ-pyrroline-5-carboxylate dehydrogenase activity is involved in the degradation of ornithine and proline. Proline dehydrogenase and Δ-pyrroline-5-carboxylate dehydrogenase activities were strongly and coordinately induced by proline. It was excluded that Δ-pyrroline-5-carboxylate acted as an inducer of the bifunctional enzyme and it was shown that the low level induction observed during growth on ornithine was due to the intracellular formation of proline. The formation of the proline degradative enzyme was shown to be subject to catabolite repression by citrate and nitrogen control. [ABSTRACT FROM AUTHOR]

Published

1982

25. Characterization and synthesis regulation of Penicillium italicum 1,6-β-glucanase.

Author

Santos, T., Nombela, C., Villanueva, J., and Larriba, G.

Abstract

The filamentous fungus Penicillium italicum when grown in a synthetic medium, produced and secreted 1,6-β-glucanase into the culture medium. This enzyme has been partially purified by gel filtration. After this step the active fractions were free of 1,3-β-glucanase, α-amylase and β-glucosidase activities. Only four proteins, one associated with the enzyme, were found by polyacrylamide gel electrophoresis under non denaturing conditions. The enzyme behaves as an acidic protein (pI 4.65) with an optimum pH of 5 and an endohydrolytic mode of action. The activity was lost at pHs greater than 7. The enzyme was also found associated with the mycelium. Its synthesis was repressed by glucose or growth-promoting sugars. Derepression in low glucose containing medium required protein synthesis. 8-Hydroxyquinoline, an RNA synthesis inhibitor, added during the derepression period did permit some increase in the specific activity but prevented it when added at the beginning of that period. [ABSTRACT FROM AUTHOR]

Published

1979

26. Conditions for fruit body formation in the white rot basidiomycete Phanerochaete chrysosporium.

Author

Gold, Michael and Cheng, Therese

Abstract

In Phanerochaete chrysosporium fruit body formations is subject to strong catabolite repression by glucose in the presence of physiological levels of nitrogen. Walseth cellulose was found to be the best source of carbon for the induction of fruit body and consequent basidiospore synthesis. Ejected basidiospores collected from cultures grown under these conditions for two weeks are contaminated with neither conidia nor mycelial fragments and are therefore suitable for genetic analysis of recombination. Under conditions of nitrogen limitation, the glucose catabolite repression of fruit body synthesis was relieved. Exogenous adenosine 3′,5′-monophosphate but not other related nucleotides, also relieved glucose catabolite repression of fruit body formation. [ABSTRACT FROM AUTHOR]

Published

1979

27. Stimulation of growth and glucose catabolite enzymes by succinate in some thermophilic fungi.

Author

Wali, Anupam, Mattoo, Autar, and Modi, V.

Abstract

Thermophilic Humicola lanuginosa, Penicillium duponti, Sporotrichum thermophile and Mucor pusillus required succinate in addition to glucose for optimal growth. The requirement for succinate was concentration-dependent and the concentration needed for one half of the maximal growth was 6.14 mM. In the presence of succinate, glucose utilization from the medium was markedly increased and this was associated with increased levels of the enzymes of the glycolytic and Krebs cycle pathways. Addition of succinate to cultures growing in glucose at any stage of growth stimulated the growth with the resulting rate of growth remaining high if the addition was made within 3 days of inoculation. Cycloheximide (71.4 μM) prevented the succinate-mediated derepression of the enzymes suggesting that succinate may remove the catabolite repression in the presence of glucose. [ABSTRACT FROM AUTHOR]

Published

1978

28. Effect of cyclic AMP on catabolite repressed bacterial sporogenesis of an anaerobe.

Author

Emeruwa, A. and Hawirko, R.

Abstract

The sporulation of a high frequency sporogenic mutant of Clostridium botulinum was reduced to <30% in a medium containing 270 mM glucose. The repression was reversed from 30 to >80% sporulation by the addition of 10 or 10 M cyclic 3′,5′-adenosine monophosphate (cAMP) or monobutyryl cyclic AMP (B-cAMP). No difference was observed in amount of growth with the addition of either the cAMP or B-cAMP. Glucose consumption was enhanced by the addition of either of the cyclic nucleotides and corresponding changes in pH were observed. The catabolite repression by glucose was reversed by ATP or ADP. Except for GTP, guanine nucleotides were not effective. The intracellular cyclic AMP levels were high in vegetative, sporulating and derepressed cells, but low in glucose-repressed cells. The findings suggest that the sporulation of the anaerobe was sensitive to catabolite repression which was specifically reversed by cyclic AMP. [ABSTRACT FROM AUTHOR]

Published

1975

29. The non-metabolizable sucrose analog sucralose is a potent inhibitor of hormogonium differentiation in the filamentous cyanobacterium Nostoc punctiforme

Author

Samantha D. Splitt and Douglas D. Risser

Subjects

0301 basic medicine, Cyanobacteria, Sucrose, Sucralose, Nostoc, 030106 microbiology, Catabolite repression, Polysaccharide, Biochemistry, Microbiology, Magnoliopsida, 03 medical and health sciences, chemistry.chemical_compound, Genetics, Symbiosis, Hormogonium, Molecular Biology, chemistry.chemical_classification, biology, Nostoc punctiforme, Polysaccharides, Bacterial, General Medicine, biology.organism_classification, chemistry

Abstract

Nostoc punctiforme is a filamentous cyanobacterium which forms nitrogen-fixing symbioses with several different plants and fungi. Establishment of these symbioses requires the formation of motile hormogonium filaments. Once infected, the plant partner is thought to supply a hormogonium-repressing factor (HRF) to maintain the cyanobacteria in a vegetative, nitrogen-fixing state. Evidence implies that sucrose may serve as a HRF. Here, we tested the effects of sucralose, a non-metabolizable sucrose analog, on hormogonium differentiation. Sucralose inhibited hormogonium differentiation at a concentration approximately one-tenth that of sucrose. This result implies that: (1) sucrose, not a sucrose catabolite, is perceived by the cell and (2) inhibition is not due to a more general osmolarity-dependent effect. Additionally, both sucrose and sucralose induced the accrual of a polysaccharide sheath which bound specifically to the lectin ConA, indicating the presence of α-D-mannose and/or α-D-glucose. A ConA-specific polysaccharide was also found to be expressed in N. punctiforme colonies from tissue sections of the symbiotically grown hornwort Anthoceros punctatus. These findings imply that plant-derived sucrose or sucrose analogs may have multiple effects on N. punctiforme, including both repression of hormogonia and the induction of a polysaccharide sheath that may be essential to establish and maintain the symbiotic state.

Published

2015

30. Functional characterization and transcriptional analysis of icd2 gene encoding an isocitrate dehydrogenase of Xanthomonas campestris pv. campestris

Author

Ying-Chuan Chiang, Shin-Chiao Du, Yi-Min Hsiao, and Chao-Tsai Liao

Subjects

0301 basic medicine, 030106 microbiology, Catabolite repression, Brassica, Xanthomonas campestris, Biochemistry, Microbiology, Bacterial Adhesion, Xanthomonas campestris pv. campestris, 03 medical and health sciences, Start codon, Bacterial Proteins, Transcription (biology), Gene expression, Genetics, Promoter Regions, Genetic, Molecular Biology, Gene, Plant Diseases, biology, Virulence, General Medicine, Gene Expression Regulation, Bacterial, biology.organism_classification, Isocitrate Dehydrogenase, Isocitrate dehydrogenase, Ketoglutaric Acids, Transcription Initiation Site

Abstract

Isocitrate dehydrogenase (IDH) catalyzes the oxidative decarboxylation of isocitrate to alpha-ketoglutarate. In the genome of Xanthomonas campestris pv. campestris, the phytopathogen that causes black rot in cruciferous plants, two putative IDH genes, icd1 and icd2, have been annotated. Their physiological roles in X. campestris pv. campestris are unclear. In this study, the icd2 gene from X. campestris pv. campestris was characterized in detail. We demonstrated genetically that icd2 gene encodes a functional IDH, and is involved in virulence as well as bacterial attachment. Furthermore, the icd2 transcription initiation site was mapped at nucleotide G, 127 nucleotide upstream of the icd2 translation start codon. In addition, promoter analysis revealed that icd2 expression exhibits a distinct expression profile under different culture conditions, is subjected to catabolite repression, and is affected by acetate. This is the first time that the function and transcription of icd2 have been characterized in the crucifer pathogen X. campestris pv. campestris.

Published

2016

31. Characterization of genes involved in fructose utilization by Lactobacillus fermentum

Author

Matti Leisola, Antti Nyyssölä, Airi Palva, Miia Helanto, and Johannes Aarnikunnas

Subjects

Limosilactobacillus fermentum, Operon, Molecular Sequence Data, Fructose 1,6-bisphosphatase, Catabolite repression, lac operon, Electrophoretic Mobility Shift Assay, Fructose, Biochemistry, Microbiology, Fructokinase, trp operon, Fructokinases, Genetics, gal operon, RNA, Messenger, Cloning, Molecular, Phosphoenolpyruvate Sugar Phosphotransferase System, Molecular Biology, Base Sequence, biology, Glucose-6-Phosphate Isomerase, General Medicine, Molecular biology, biology.protein, bacteria, L-arabinose operon

Abstract

The genes encoding phosphoglucose isomerase (fruI) and fructokinase (fruK) of Lactobacillus fermentum NRRL-B-1932 were sequenced. They constituted an operon, which is involved in fructose metabolism of this strain by channeling intracellular fructose into the phosphoketolase pathway. A third open reading frame, unkR, upstream of the operon was identified as homologous to genes of LacI/GalR family repressors. The UnkR repressor’s role in transcriptional control of the fruIK operon could, however, not be established by electrophoretic mobility shift assay (EMSA) analysis. Sequence analysis revealed two putative catabolite responsive elements (cre) in the promoter region of fruIK suggesting that the fruIK operon is under negative regulatory control by carbon catabolite repression. Expression and enzyme activity data were compatible with the assumption that the fruIK operon is represessed by glucose. No sugar specific phosphoenolpyruvate sugar transferase system activity for the transport of fructose, glucose, sucrose or mannose could be detected in L. fermentum NRRL-B-1932 cells, which suggest that fructose is taken up by a permease system.

Published

2006

32. Anaerobiosis and low specific growth rates enhance hemolysin BL production by Bacillus cereus F4430/73

Author

Philippe Schmitt, Séverine Thomassin, Catherine Duport, Gérald Bourel, Sécurité et Qualité des Produits d'Origine Végétale (SQPOV), and Avignon Université (AU)-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE)

Subjects

[SDV]Life Sciences [q-bio], RT-PCR, Catabolite repression, Bacillus cereus, Chemostat, medicine.disease_cause, Biochemistry, Microbiology, Hemolysin Proteins, 03 medical and health sciences, Bacterial Proteins, [SDV.IDA]Life Sciences [q-bio]/Food engineering, Genetics, medicine, [SPI.GPROC]Engineering Sciences [physics]/Chemical and Process Engineering, Anaerobiosis, Molecular Biology, 030304 developmental biology, 0303 health sciences, Bacillaceae, biology, Reverse Transcriptase Polymerase Chain Reaction, 030306 microbiology, Toxin, Hemolysin, Gene Expression Regulation, Bacterial, General Medicine, biology.organism_classification, Bacillales, Glucose, Bacteria

Abstract

International audience; Bacillus cereus F4430/73 produced the highest levels of hemolysin BL (HBL) when grown under anaerobiosis in MOD medium. Anaerobic cells grown in a chemostat at low specific growth rate (0.1–0.2 h–1) expressed up to sevenfold more HBL than did cells held at a faster growth rate. At 0.2 h–1, the presence of 90 mM glucose resulted in inhibition of HBL production. Glucose was found to repress HBL induction at the mRNA level, indicating the potential involvement of catabolite repression in the regulation of HBL. Based on these data, it is suggested that growth rate could be an effector of catabolite regulation of HBL.

Published

2004

33. Characterization of glucose-repression-resistant mutants of Bacillus subtilis : identification of the glcR gene

Author

Philippe Glaser, Isabelle Martin-Verstraete, Jörg Stülke, and Georges Rapoport

Subjects

Glycoside Hydrolases, Operon, Mutant, Catabolite repression, Repressor, macromolecular substances, Biology, Biochemistry, Microbiology, Gene Expression Regulation, Enzymologic, Bacterial Proteins, Genetics, Cloning, Molecular, Phosphoenolpyruvate Sugar Phosphotransferase System, Molecular Biology, Psychological repression, Glucose transporter, Biological Transport, Gene Expression Regulation, Bacterial, General Medicine, PEP group translocation, Physical Chromosome Mapping, Fed-batch culture, DNA-Binding Proteins, Repressor Proteins, Glucose, Genes, Bacterial, Mutation, Mutagenesis, Site-Directed, bacteria, Bacillus subtilis

Abstract

In Bacillus subtilis, carbon catabolite repression (CCR) is mediated by the pleiotropic repressor CcpA and by ATP-dependent phosphorylation of the HPr protein of the phosphotransferase system (PTS). In this study, we attempted to identify novel genes that are involved in the signal transduction pathway that ultimately results in CCR in the presence of repressing carbon sources such as glucose. Seven mutants resistant to glucose repression of the levanase operon were isolated and characterized. All mutations were trans-acting and pleiotropic as determined by analyzing CCR of beta-xylosidase and of the sacPA and bglPH operon. Moreover, all mutations specifically affected repression exerted by glucose but not by other sugars. The mutations were mapped to three different loci on the genetic map, ptsG, glcR, and pgi. These three genes encode proteins involved in glucose metabolism. A novel repressor gene, glcR (ywpI), defined by two mutations, was studied in more detail. The glcR mutants exhibit loss of glucose repression of catabolic operons, a deficiency in glucose transport, and absence of expression of the ptsG gene. The mutant GlcR proteins act as super-repressors of ptsG expression.

Published

2001

34. Regulation of maltose transport in Saccharomyces cerevisae

Author

T.H C Brondijk, W.N Konings, Berend Poolman, GBB Cluster Microbiologie, Enzymologie, Faculty of Science and Engineering, Moleculaire Microbiologie, and Groningen Biomolecular Sciences and Biotechnology

Subjects

Post-translational regulation, Saccharomyces cerevisiae Proteins, Monosaccharide Transport Proteins, Saccharomyces cerevisiae, Catabolite repression, Glucose-6-Phosphate, Trans-inhibition, Biochemistry, Microbiology, chemistry.chemical_compound, Adenosine Triphosphate, Genetics, Maltose, GeneralLiterature_REFERENCE(e.g.,dictionaries,encyclopedias,glossaries), Molecular Biology, Maltose transport, chemistry.chemical_classification, Membrane transport, Symporters, biology, Chemistry, Biological Transport, General Medicine, biology.organism_classification, Yeast, Glucose, Enzyme, Catabolite inactivation, Symporter, ComputingMethodologies_DOCUMENTANDTEXTPROCESSING, Maltase

Abstract

Solute transport in Saccharomyces cerevisiae can be regulated through mechanisms such as trans-inhibition and/or catabolite inactivation by nitrogen or carbon sources. Studies in hybrid membranes of S. cerevisiae suggested that the maltose transport system Mal61p is fully reversible and capable of catalyzing both influx and efflux transport. This conclusion has now been confirmed by studies in a S. cerevisiae strain lacking the maltase enzyme. Whole cells of this strain, wherein the orientation of the maltose transporter is fully preserved, catalyze fully reversible maltose transport. Catabolite inactivation of the maltose transporter Mal61p was studied in the presence and absence of maltose metabolism and by the use of different glucose analogues. Catabolite inactivation of Mal61p could be triggered by maltose, provided the sugar was metabolized, and the rate of inactivation correlated with the rate of maltose influx. We also show that 2-deoxyglucose, unlike 6-deoxyglucose, can trigger catabolite inactivation of the maltose transporter. This suggests a role for early glycolytic intermediates in catabolite inactivation of the Mal61 protein. However, there was no correlation between intracellular glucose-6-phosphate or ATP levels and the rate of catabolite inactivation of Mal61p. On the basis of their identification in cell extracts, we speculate that (dideoxy)-trehalose and/or (deoxy)-trehalose-6-phosphate trigger catabolite inactivation of the maltose transporter.

Published

2001

35. The catabolite inactivation of Aspergillus nidulans isocitrate lyase occurs by specific autophagy of peroxisomes

Author

Fernando Laborda, A. I. Domínguez, J. Ramón De Lucas, and Cristina Amor

Subjects

IDH1, biology, Catabolite repression, Glyoxylate cycle, General Medicine, Isocitrate lyase, Peroxisome, biology.organism_classification, Isocitrate Lyase, Biochemistry, Microbiology, Aspergillus nidulans, Microscopy, Electron, Glucose, Endopeptidases, Autophagy, Peroxisomes, Genetics, Microbody, Microautophagy, Molecular Biology

Abstract

In Aspergillus nidulans, activity of the glyoxylate cycle enzyme isocitrate lyase is finely regulated. Isocitrate lyase is induced by growth on C2 compounds and long-chain fatty acids and repressed by glucose. In addition, activity of isocitrate lyase is subject to a second mechanism of catabolite control, glucose-induced inactivation. Here, we demonstrate that the catabolite inactivation of A. nidulans isocitrate lyase, a process that takes place during glucose adaptation of cells grown under gluconeogenic conditions, occurs by proteolysis of the enzyme. Ultrastructural analyses were carried out in order to investigate the cellular processes that govern the catabolite inactivation of this peroxisomal enzyme. Addition of glucose to oleate-induced cells triggered the specific engulfment and sequestration of peroxisomes by the vacuoles. Sequestration of various peroxisomes by a single vacuole was a frequently observed phenomenon. Results obtained by immunoelectron microscopy using antibodies against A. nidulans isocitrate lyase showed that degradation of this peroxisomal enzyme occurred inside the vacuole. In addition, ultrastructural studies demonstrated that microautophagy was the autophagic pathway involved in degradation of redundant peroxisomes during glucose adaptation of oleate-induced cells of A. nidulans.

Published

2000

36. Metabolism of aromatic aldehydes as cosubstrates by the acetogen Clostridium formicoaceticum

Author

Harold L. Drake, Carola Matthies, Claudia Frank, and Ulf Schwarz

Subjects

Time Factors, Catabolite repression, Fructose, Gluconates, Biochemistry, Microbiology, Aldehyde, chemistry.chemical_compound, Clostridium, Oxidoreductase, Genetics, Organic chemistry, Lactic Acid, Molecular Biology, chemistry.chemical_classification, biology, General Medicine, Acetogen, Metabolism, biology.organism_classification, Lactic acid, chemistry, Benzaldehydes

Abstract

When the acetogen Clostridium formicoaceticum was cultivated on mixtures of aromatic compounds (e.g., 4-hydroxybenzaldehyde plus vanillate), the oxidation of aromatic aldehyde groups occurred more rapidly than did O-demethylation. Likewise, when fructose and 4-hydroxybenzaldehyde were simultaneously provided as growth substrates, fructose was utilized only after the aromatic aldehyde group was oxidized to the carboxyl level. Aromatic aldehyde oxidoreductase activity was constitutive (activities approximated 0. 8 U mg-1), and when pulses of 4-hydroxybenzaldehyde were added during fructose-dependent growth, the rate at which fructose was utilized decreased until 4-hydroxybenzaldehyde was consumed. Although 4-hydroxybenzaldehyde inhibited the capacity of cells to metabolize fructose, lactate or gluconate were consumed simultaneously with 4-hydroxybenzaldehyde, and lactate or aromatic compounds lacking an aldehyde group were utilized concomitantly with fructose. These results demonstrate that (1) aromatic aldehydes can be utilized as cosubstrates and have negative effects on the homoacetogenic utilization of fructose by C. formicoaceticum, and (2) the consumption of certain substrates by this acetogen is not subject to catabolite repression by fructose.

Published

1998

37. The role of stress in colicin regulation

Author

Osnat Gillor, Lilit Tonoyan, Lusine Ghazaryan, Ashraf Al Ashhab, and M. Ines M. Soares

Subjects

Regulation of gene expression, biology, Stringent response, Catabolite repression, food and beverages, General Medicine, Gene Expression Regulation, Bacterial, Environment, biology.organism_classification, Biochemistry, Microbiology, Enterobacteriaceae, Bacteriocin, Bacteriocins, Stress, Physiological, Colicin, Genetics, Nucleic acid, Promoter Regions, Genetic, Molecular Biology, Bacteria, Mutagens

Abstract

Bacteriocins produced by Enterobacteriaceae are high molecular weight toxic proteins that kill target cells through a variety of mechanisms, including pore formation and nucleic acid degradation. What is remarkable about these toxins is that their expression results in death to the producing cells and therefore bacteriocin induction have to be tightly regulated, often confined to times of stress. Information on the regulation of bacteriocins produced by enteric bacteria is sketchy as their expression has only been elucidated in a handful of bacteria. Here, we review the known regulatory mechanisms of enteric bacteriocins and explore the expression of 12 of them in response to various triggers: DNA-damaging agents, stringent response, catabolite repression, oxidative stress, growth phase, osmolarity, cold shock, nutrient deprivation, anaerobiosis and pH stress. Our results indicate that the expression of bacteriocins is mostly confined to mutagenic triggers, while all other triggers tested are limited inducers.

Published

2014

38. Catabolite regulation of two Escherichia coli operons encoding nitrite reductases: role of the Cra protein

Author

J. A. Cole, Steve Busby, and Kerry L. Tyson

Subjects

Nitrite Reductases, Transcription, Genetic, genetic structures, Operon, Catabolite repression, Repressor, Biology, medicine.disease_cause, Biochemistry, Microbiology, Bacterial Proteins, Transcription (biology), Escherichia coli, Genetics, medicine, Electrophoretic mobility shift assay, Promoter Regions, Genetic, Molecular Biology, Nitrite Reductase (NAD(P)H), Escherichia coli Proteins, Fructosephosphates, technology, industry, and agriculture, Promoter, Gene Expression Regulation, Bacterial, General Medicine, equipment and supplies, Nitrite reductase, DNA-Binding Proteins, Repressor Proteins, Enzyme Repression, Protein Binding

Abstract

The Escherichia coli nir and nrf operons, which encode alternative nitrite reductases expressed during anaerobic growth, are subject to catabolite regulation. Transcription from the nir promoter is maximal when bacteria are grown in rich media such as Lennox broth supplemented with glucose. Conversely, expression of the nrf operon is suppressed by rich media, but stimulated during growth in minimal medium with glycerol and fumarate. The role of the catabolite repressor-activator (Cra) protein in catabolite regulation of the nir and nrf promoters was investigated. Transcription from the nir promoter was repressed by Cra when cells were grown in minimal medium with glycerol and fumarate. Crude protein extracts from a strain overproducing Cra encoded on a multicopy plasmid retarded a nir promoter fragment in a mobility shift assay, confirming that the observed Cra-dependent repression was due to the direct interaction of Cra with the regulatory region of the nir operon. Furthermore, the inclusion of fructose 1-phosphate, an effector of Cra DNA-binding activity, in the assay decreased the ability of Cra to retard the nir promoter fragment. In contrast, transcription from the nrf promoter was not regulated by Cra under any of the growth conditions tested.

Published

1997

39. Anaerobic citrate metabolism and its regulation in enterobacteria

Author

Michael Bott

Subjects

ATP citrate lyase, Carboxy-Lyases, Catabolite repression, Biological Transport, Active, Dehydrogenase, Formate dehydrogenase, Biochemistry, Microbiology, Enterobacteriaceae, Multienzyme Complexes, Genetics, Citrate synthase, Anaerobiosis, Citrates, Tartrates, Molecular Biology, biology, Oxo-Acid-Lyases, General Medicine, Citrate transport, NAD, Citric acid cycle, Oxaloacetate decarboxylase, Fermentation, biology.protein, Protons, Sodium-Potassium-Exchanging ATPase

Abstract

Several species of enterobacteria are able to utilize citrate as carbon and energy source. Under oxic conditions in the presence of a functional tricarboxylic acid cycle, growth on this compound solely depends on an appropriate transport system. During anaerobiosis, when 2-oxoglutarate dehydrogenase is repressed, some species such as Klebsiella pneumoniae and Salmonella typhimurium, but not Escherichia coli, are capable of growth on citrate by a Na+-dependent pathway forming acetate, formate, and CO2 as products. During the last decade, several novel features associated with this type of fermentation have been discovered in K. pneumoniae. The biotin protein oxaloacetate decarboxylase, one of the key enzymes of the pathway besides citrate lyase, is a Na+ pump. Recently it has been shown that the proton required for the decarboxylation of carboxybiotin is taken up from the side to which Na+ ions are pumped, and a membrane-embedded aspartate residue that is probably involved both in Na+ and in H+ transport was identified. The Na+ gradient established by oxaloacetate decarboxylase drives citrate uptake via CitS, a homodimeric carrier protein with a simultaneous-type reaction mechanism, and NADH formation by reversed electron transfer involving formate dehydrogenase, quinone, and a Na+-dependent NADH:quinone oxidoreductase. All enzymes specifically required for citrate fermentation are induced under anoxic conditions in the presence of citrate and Na+ ions. The corresponding genes form a cluster on the chromosome and are organized as two divergently transcribed operons. Their co-ordinate expression is dependent on a two-component system consisting of the sensor kinase CitA and the response regulator CitB. The citAB genes are part of the cluster and are positively autoregulated. In addition to CitA/CitB, the cAMP receptor protein (Crp) is involved in the regulation of the citrate fermentation enzymes, subjecting them to catabolite repression.

Published

1997

40. Extracellular arabinases in Aspergillus nidulans: the effect of different cre mutations on enzyme levels

Author

P. van der Veen, Herbert N. Arst, M.J.A. Flipphi, and Jantien Visser

Subjects

Molecular Genetics of Industrial Micro-organisms, Mutant, Catabolite repression, Reductase, Biochemistry, Microbiology, Gene Expression Regulation, Enzymologic, Aspergillus nidulans, Induction, Moleculaire genetica van industriële micro-organismen, Genetics, Molecular Biology, Derepression, VLAG, Regulator gene, biology, Structural gene, D-Xylulose Reductase, General Medicine, Carbon catabolite repression, biology.organism_classification, Arabinose, Carbon, Fed-batch culture, Enzyme Induction, Mutation, Arabinases, Enzyme Repression, Sugar Alcohol Dehydrogenases

Abstract

The regulation of the syntheses of two arabinan-degrading extracellular enzymes and several intracellular L-arabinose catabolic enzymes was examined in wild-type and carbon catabolite derepressed mutants of Aspergillus nidulans. alpha-L-Arabinofuranosidase B, endoarabinase, L-arabinose reductase, L-arabitol dehydrogenase, xylitol dehydrogenase, and L-xylulose reductase were all inducible to varying degrees by L-arabinose and L-arabitol and subject to carbon catabolite repression by D-glucose. With the exception of L-xylulose reductase, all were clearly under the control of creA, a negative-acting wide domain regulatory gene mediating carbon catabolite repression. Measurements of intracellular enzyme activities and of intracellular concentrations of arabitol and xylitol in mycelia grown on D-glucose in the presence of inducer indicated that carbon catabolite repression diminishes, but does not prevent uptake of inducer. Mutations in creA resulted in an apparently, in some instances very marked, elevated inducibility, perhaps reflecting an element of "self" catabolite repression by the inducing substrate. creA mutations also resulted in carbon catabolite derepression to varying degrees. The regulatory effects of a mutation in creB and in creC, two genes whose roles are unclear, but likely to be indirect, were, when observable, more modest. As with previous data showing the effect of creA mutations on structural gene expression, there were striking instances of phenotypic variation amongst creA mutant alleles and this variation followed no discernible pattern, i.e. it was non-hierarchical. This further supports molecular data obtained elsewhere, indicating a direct role for creA in regulating structural gene expression, and extends the range of activities under creA control.

Published

1994

41. The induction and repression of benzene and catechol oxidizing capacity of Pseudomonas putida ML2 studied in perturbed chemostat culture

Author

Jeremy R. Mason

Subjects

Stereochemistry, Catechols, Catabolite repression, Chemostat, Photochemistry, Models, Biological, Biochemistry, Microbiology, Dioxygenases, chemistry.chemical_compound, Oxidizing agent, Genetics, Catechol 1,2-dioxygenase, Molecular Biology, Catechol, biology, Pseudomonas putida, Benzene, General Medicine, biology.organism_classification, Catechol 1,2-Dioxygenase, Culture Media, Oxygen, chemistry, Enzyme Induction, Oxygenases, biology.protein, Steady state (chemistry), Enzyme Repression, Catechol dioxygenase

Abstract

The oxidation of catechol, an intermediate in benzene catabolism, was studied using transient variations in dissolved oxygen tension (DOT) when a succinate limited steady state culture of Pseudomonas putida ML2 was perturbed with a pulse of another substrate. A model was developed and tested for the effect of fluctuations in oxidizing enzyme activity on DOT. It was found that the rate of induction of catechol oxidizing enzymes was independent of dilution rate up to a relative growth rate (mu/mumax) of 0.75. Only at higher dilution rates was catabolite repression observed.

Published

1994

42. Role of altered rpoB alleles in Bacillus subtilis sporulation and spore resistance to heat, hydrogen peroxide, formaldehyde, and glutaraldehyde

Author

Ignacija Vlašić, Guenther Reitz, Wayne L. Nicholson, and Ralf Moeller

Subjects

Hot Temperature, Mutant, Catabolite repression, Bacillus subtilis, Biochemistry, Microbiology, chemistry.chemical_compound, Anti-Infective Agents, Transcription (biology), RNA polymerase, Formaldehyde, Drug Resistance, Bacterial, Genetics, polycyclic compounds, Spore resistance, Molecular Biology, Gene, Alleles, Spores, Bacterial, biology, fungi, sporulation, spore resistance, heat, chemicals, Water, General Medicine, DNA-Directed RNA Polymerases, Hydrogen Peroxide, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, rpoB, bacterial infections and mycoses, Heat, Spore, Glucose, chemistry, Sporulation, Glutaral, Mutation, bacteria, Chemicals

Abstract

Mutations in the RNA polymerase β-subunit gene rpoB causing resistance to rifampicin (Rif(R)) in Bacillus subtilis were previously shown to lead to alterations in the expression of a number of global phenotypes known to be under transcriptional control. To better understand the influence of rpoB mutations on sporulation and spore resistance to heat and chemicals, cells and spores of the wild-type and twelve distinct congenic Rif(R) mutant strains of B. subtilis were tested. Different levels of glucose catabolite repression during sporulation and spore resistance to heat and chemicals were observed in the Rif(R) mutants, indicating the important role played by the RNA polymerase β-subunit, not only in the catalytic aspect of transcription, but also in the initiation of sporulation and in the spore resistance properties of B. subtilis.

Published

2011

43. Metabolic effects of benzoate and sorbate in the yeast Saccharomyces cerevisiae at neutral pH

Author

Nedda Burlini, Paolo Tortora, Patrizia Facheris, Andrea Guerritore, and Rita Pellegrini

Subjects

Intracellular pH, Fructose 1,6-bisphosphatase, Catabolite repression, Saccharomyces cerevisiae, Benzoates, Biochemistry, Microbiology, Malate dehydrogenase, chemistry.chemical_compound, Fructosediphosphates, Genetics, Molecular Biology, biology, Gluconeogenesis, Fructose, General Medicine, Metabolism, Benzoic Acid, Hydrogen-Ion Concentration, Sorbic Acid, Fructose-Bisphosphatase, Kinetics, Glucose, chemistry, biology.protein, Phosphoenolpyruvate Carboxykinase (GTP), Sorbic acid, Phosphoenolpyruvate carboxykinase, Glycolysis

Abstract

Preincubation of yeast cells in the presence of benzoate or sorbate at an extracellular pH value of 6.8 elicited a set of metabolic effects on sugar metabolism, which became apparent after the subsequent glucose addition. They can be summarized as follows: a) reduced glucose consumption; b) inhibition of glucose- and fructose-phosphorylating activities; c) suppression of glucose-triggered peak of hexoses monophosphates; d) substantial reduction of glucose-triggered peak of fructose 2,6-bisphosphate; e) block of catabolite inactivation of fructose-1,6-bisphosphatase and phosphoenolpyruvate carboxy-kinase, but not of cytoplasmic malate dehydrogenase. On the whole this pattern resulted in prevention of glucose-induced switch of metabolism from a gluconeogenetic to a glycolytic state. Our data also show that, unlike former assumptions, intracellular acidification is not likely to mediate the bulk of metabolic effects of benzoate and sorbate, since under our working conditions intracellular pH kept close to neutrality.

Published

1993

44. Methanol and ethanol utilization in methylotrophic yeast Pichia pinus wild-type and mutant strains

Author

Andriy A. Sibirny, M. M. Kucher, V. I. Petrushko, V. I. Titorenko, and G. E. Teslyar

Subjects

Ethanol, Catabolite repression, General Medicine, Biology, Peroxisome, Formate dehydrogenase, Biochemistry, Microbiology, Yeast, chemistry.chemical_compound, Diauxic growth, chemistry, Genetics, Methanol, Molecular Biology, Formaldehyde dehydrogenase

Abstract

In the wild-type strain of methylotrophic yeast Pichia pinus diauxic growth is observed during cultivation in medium containing a mixture of methanol and ethanol: firstly, “slow” phase of ethanol utilization is revealed and, secondly, a “fast” phase of methanol consumption is shown. Diauxic growth is observed also in ecr1 mutant, impaired in ethanol-induced catabolite repression of methylotrophic metabolism enzymes, but the order of utilization of the alcohols is inverted in this mutant. Such succession of alcohols utilization in both strains correlates well with the sequence of synthesis of microbody enzymes which catalyze key reactions of C1- and C2-metabolism. On the contrary, simultaneous utilization of methanol and ethanol from the mixture, as well as synchronous synthesis of both peroxisomal and glyoxisomal enzymes is observed in adh1 mutant which has reduced alcohol dehydrogenase activity. The strong differences between the wild-type strain and adh1 mutant were observed also in the kinetics of specific activity changes for C1-metabolizing enzymes, localized in cytosol. In the wild-type strain during growth on methanol and ethanol mixture such changes correlate with the sequence of alcohol utilization. At the same time, in adh1 mutant the activities of formaldehyde dehydrogenase and formate dehydrogenase during the growth on the alcohols mixture are as high as during growth on methanol only, but the activity of dihydroxyacetone kinase is as low as under the growth on ethanol and is lower than on methanol.

Published

1991

45. Microbial degradation of acrylamide monomer

Author

Cherla Ramakrishna, Prahlad K. Seth, and Rishi Shanker

Subjects

Chemical Phenomena, Catabolite repression, Biochemistry, Microbiology, Amidohydrolases, Amidase, chemistry.chemical_compound, Hydrolysis, Pseudomonas, Genetics, Organic chemistry, Methacrylamide, Molecular Biology, Chromatography, High Pressure Liquid, Soil Microbiology, Acrylamides, biology, General Medicine, Biodegradation, biology.organism_classification, Chemistry, Biodegradation, Environmental, chemistry, Acrylamide, Acetamide

Abstract

Acrylamide, a neurotoxic monomer with extensive industrial applications was found to be degraded by the microorganisms present in a tropical garden soil. A bacterium capable of degrading acrylamide was isolated from this soil by enrichment. It was found to be aerobic, gram-negative, motile, short rod and identified as Pseudomonas sp. The bacterium degraded high concentrations of acrylamide (4 g/l) to acrylic acid and ammonia which were utilized as sole carbon and nitrogen source for growth. An amidase was involved in the hydrolysis of acrylamide, which could act on other short chain amides like formamide and acetamide but not on acrylamide analogues: methacrylamide and N,N-methylene bis-acrylamide. The enzyme was sensitive to catabolite repression by succinate both in presence as well as absence of nitrogen source.

Published

1990

46. Regulation of the chitobiose–phosphotransferase system in Vibrio cholerae

Author

Thorsten Berg, Stefan Schild, and Joachim Reidl

Subjects

Operon, Catabolite repression, macromolecular substances, Biology, Chitobiose, Disaccharides, medicine.disease_cause, Biochemistry, Microbiology, chemistry.chemical_compound, Bacterial Proteins, Vibrionaceae, Gene expression, Cyclic AMP, Genetics, medicine, ORFS, Vibrio cholerae, Molecular Biology, Chitosan, Escherichia coli Proteins, Phosphotransferases, Gene Expression Regulation, Bacterial, General Medicine, PEP group translocation, biology.organism_classification, Repressor Proteins, carbohydrates (lipids), chemistry

Abstract

Vibrio cholerae harbours a phosphotransferase system (PTS) enabling the organism to utilise chitosan oligosaccharide, e.g. derived from deacetylated chitin. As shown recently, this utilization system is encoded by the ORFs VC1281-1283 (Meibom et al. in Proc Natl Acad Sci USA, 101:2524-2529, 2004). By using a transcriptional reporter fusion technique, we identified the regulator of the system and characterised gene expression. Furthermore, we found that gene expression of this PTS system is influenced by catabolite regulation and also by an Mlc homologue (VC2007), which in E. coli is a global regulator of sugar metabolism.

Published

2007

47. Regulation of citB expression in Bacillus subtilis: integration of multiple metabolic signals in the citrate pool and by the general nitrogen regulatory system

Author

Ingrid Wacker, Hans-Matti Blencke, Irene Reif, Holger Ludwig, Fabian M. Commichau, Jörg Stülke, and Christian Detsch

Subjects

Nitrogen, Blotting, Western, Catabolite repression, Bacillus subtilis, Biology, Arginine, Biochemistry, Microbiology, Aconitase, Bacterial Proteins, Genetics, Citrate synthase, Citrates, Molecular Biology, Transcription factor, Aconitate Hydratase, General transcription factor, Catabolism, General Medicine, Gene Expression Regulation, Bacterial, biology.organism_classification, Blotting, Northern, Citric acid cycle, DNA-Binding Proteins, Repressor Proteins, Genes, Bacterial, biology.protein, Metabolic Networks and Pathways

Abstract

The tricarboxylic acid (TCA) cycle is one of the major routes of carbon catabolism in Bacillus subtilis. The syntheses of the enzymes performing the initial reactions of the cycle, citrate synthase, and aconitase, are synergistically repressed by rapidly metabolizable carbon sources and glutamine. This regulation involves the general transcription factor CcpA and the specific repressor CcpC. In this study, we analyzed the expression and intracellular localization of CcpC. The synthesis of citrate, the effector of CcpC, requires acetyl-CoA. This metabolite is located at a branching point in metabolism. It can be converted to acetate in overflow metabolism or to citrate. Manipulations of the fate of acetyl-CoA revealed that efficient citrate synthesis is required for the expression of the citB gene encoding aconitase and that control of the two pathways utilizing acetyl-CoA converges in the control of citrate synthesis for the induction of the TCA cycle. The citrate pool seems also to be controlled by arginine catabolism. The presence of arginine results in a severe CcpC-dependent repression of citB. In addition to regulators involved in sensing the carbon status of the cell, the pleiotropic nitrogen-related transcription factor, TnrA, activates citB transcription in the absence of glutamine.

Published

2005

48. Utilization of acidic amino acids and their amides by pseudomonads: role of periplasmic glutaminase-asparaginase

Author

Klaus-Heinrich Röhm, Christian Derst, Ute Klöppner, and Avinash Sonawane

Subjects

DNA, Bacterial, Asparaginase, Amino Acids, Acidic, Catabolite repression, Pseudomonas fluorescens, Biochemistry, Microbiology, chemistry.chemical_compound, Glutaminase, Pseudomonas, Genetics, Asparagine, Molecular Biology, chemistry.chemical_classification, biology, Base Sequence, Pseudomonas putida, Amino Acids, Basic, General Medicine, Metabolism, Periplasmic space, biology.organism_classification, Amino acid, Kinetics, chemistry, Genes, Bacterial, Mutation, Periplasm, Gene Deletion

Abstract

The acidic amino acids (Asp, Glu) and their amides (Asn, Gln) support rapid growth of a variety of Pseudomonas strains when provided as the sole source of carbon and nitrogen. All key enzymes of glutamate metabolism were detected in P. fluorescence, with glutaminase and asparaginase showing the highest specific activities. A periplasmic glutaminase/asparaginase activity (PGA) was found in all pseudomonads examined, including a number of root-colonizing biocontrol strains. The enzyme was purified and shown to be identical with the ansB gene product described previously. In addition to PGA, P. fluorescens contains a cytoplasmic asparaginase with marked specificity for Asn. PGA is strongly and specifically induced by its substrates (Asn, Gln) but also by the reaction products (Asp, Glu). In addition, PGA is subject to efficient carbon catabolite repression by glucose and by citrate cycle metabolites. A mutant of P. putida KT2440 with a disrupted ansB gene was unable to utilize Gln, whereas growth of the mutant on other amino acids was normal.

Published

2002

49. Regulation of formation of the intracellular beta-galactosidase activity of Aspergillus nidulans

Author

Sándor Biró, Erzsébet Fekete, Erzsébet Sándor, Levente Karaffa, Attila Szentirmai, Christian P. Kubicek, and Bernhard Seiboth

Subjects

Glycerol, Mutant, Catabolite repression, Lactose, Biológiai tudományok, Biochemistry, Microbiology, Aspergillus nidulans, chemistry.chemical_compound, Kluyveromyces, Természettudományok, Polysaccharides, Genetics, Transferase, Molecular Biology, biology, Kinase, Galactose, General Medicine, biology.organism_classification, beta-Galactosidase, Glucose, chemistry, Mutation, Intracellular

Abstract

The regulation of formation of the single intracellular beta-galactosidase activity of Aspergillus nidulans was investigated. beta-Galactosidase was not formed during growth on glucose or glycerol, but was rapidly induced during growth on lactose or D-galactose. L-Arabinose, and -- with lower efficacy -- D-xylose also induced beta-galactosidase activity. Addition of glucose to cultures growing on lactose led to a rapid decrease in beta-galactosidase activity. In contrast, in cultures growing on D-galactose, addition of glucose decreased the activity of beta-galactosidase only slightly. Glucose inhibited the uptake of lactose, but not of D-galactose, and required the carbon catabolite repressor CreA for this. In addition, CreA also repressed the formation of basal levels of beta-galactosidase and partially interfered with the induction of beta-galactosidase by D-galactose, L-arabinose, and D-xylose. D-Galactose phosphorylation was not necessary for beta-galactosidase induction, since induction by D-galactose occurred in an A. nidulans mutant defective in galactose kinase, and by the non-metabolizable D-galactose analogue fucose in the wild-type strain. Interestingly, a mutant in galactose-1-phosphate uridylyl transferase produced beta-galactosidase at a low, constitutive level even on glucose and glycerol and was no longer inducible by D-galactose, whereas it was still inducible by L-arabinose. We conclude that biosynthesis of the intracellular beta-galactosidase of A. nidulans is regulated by CreA, partially repressed by galactose-1-phosphate uridylyl transferase, and induced by D-galactose and L-arabinose in independent ways.

Published

2002

50. Induction of butane consumption in Pseudomonas butanovora

Author

Luis A. Sayavedra-Soto, Chelsea M. Byrd, and Daniel J. Arp

Subjects

Metabolite, Catabolite repression, Pseudomonas butanovora, Biochemistry, Microbiology, chemistry.chemical_compound, 1-Butanol, Pseudomonas, Genetics, Organic chemistry, Butyraldehyde, Molecular Biology, Aldehydes, biology, Chemistry, Substrate (chemistry), Butane, General Medicine, Metabolism, Monooxygenase, biology.organism_classification, Culture Media, Butyrates, Biodegradation, Environmental, Butanes, Oxidation-Reduction

Abstract

The induction of the enzyme activities involved in butane metabolism in Pseudomonas butanovora was characterized. P. butanovora was grown on butane or its metabolites, both singly and in mixtures with other growth substrates. Cells grown in each of the butane metabolites readily consumed the growth substrate and downstream metabolites, but consumed the upstream butane metabolites more slowly. Upstream activities in the butane metabolism could be induced by downstream metabolites, but to much lower levels than with the primary substrate. The induction of butane oxidation was not repressed when P. butanovora was grown or incubated in a mixture of butane and 1-butanol, butyraldehyde or butyrate. However, no induction of butane consumption was observed in a mixture of butane and lactate, which is indicative of catabolite repression. In lactate-grown cells that were rid of the growth substrate and incubated with butane and acetylene (to inactivate newly formed butane monooxygenase), the consumption of butane, 1-butanol and butyraldehyde consumption was not induced. The overall results suggest an independent regulatory mechanism for each of the enzyme activities in butane metabolism. In addition, a low, constitutive butane oxidation was observed in cells grown on substrates other than butane metabolites.

Published

2000