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Flupirtine and retigabine were essential drugs to combat pain and epilepsy. However, the Kv7 potassium channel openers are fraught with hepatotoxicity and tissue discoloration, respectively, limiting their therapeutic value. Both adverse events are likely due to reactive metabolites arising from oxidative metabolism. Designing safer analogues lacking the structural elements leading to described side effects is an active area of current research. One of the main metabolites of flupirtine is the biologically inactive 4-fluorohippuric acid. Hitherto unexplained, the proposed metabolic pathway leading to the formation of 4-fluorohippuric acid from flupirtine is verified here. Through the use of eighteen flupirtine analogues, mechanistic details of this pathway could be elucidated. A possible connection with the in vitro hepatotoxicity of the flupirtine analogues and the levels of 4-fluorobenzoic acid formed in enzyme incubations was examined by correlation analysis. These findings provide important information for the design of new flupirtine analogues as potential drug candidates.
Acidobacteria represents one of the most dominant bacterial groups across diverse ecosystems. However, insight into their ecology and physiology has been hampered by difficulties in cultivating members of this phylum. Previous cultivation efforts have suggested an important role of trace elements for the proliferation of Acidobacteria, however, the impact of these metals on their growth and metabolism is not known. In order to gain insight into this relationship, we evaluated the effect of trace element solution SL10 on the growth of two strains (5B5 and WH15) of Acidobacteria belonging to the genus Granulicella and studied the proteomic responses to manganese (Mn). Granulicella species had highest growth with the addition of Mn, as well as higher tolerance to this metal compared to seven other metal salts. Variations in tolerance to metal salt concentrations suggests that Granulicella sp. strains possess different mechanisms to deal with metal ion homeostasis and stress. Furthermore, Granulicella sp. 5B5 might be more adapted to survive in an environment with higher concentration of several metal ions when compared to Granulicella sp. WH15. The proteomic profiles of both strains indicated that Mn was more important in enhancing enzymatic activity than to protein expression regulation. In the genomic analyses, we did not find the most common transcriptional regulation of Mn homeostasis, but we found candidate transporters that could be potentially involved in Mn homeostasis for Granulicella species. The presence of such transporters might be involved in tolerance to higher Mn concentrations, improving the adaptability of bacteria to metal enriched environments, such as the decaying wood-rich Mn environment from which these two Granulicella strains were isolated.
The obligate anaerobe, spore forming bacterium Clostridioides difficile (formerly Clostridium difficile) causes nosocomial and community acquired diarrhea often associated with antibiotic therapy. Major virulence factors of the bacterium are the two large clostridial toxins TcdA and TcdB. The production of both toxins was found strongly connected to the metabolism and the nutritional status of the growth environment. Here, we systematically investigated the changes of the gene regulatory, proteomic and metabolic networks of C. difficile 630Δerm underlying the adaptation to the non-growing state in the stationary phase. Integrated data from time-resolved transcriptome, proteome and metabolome investigations performed under defined growth conditions uncovered multiple adaptation strategies. Overall changes in the cellular processes included the downregulation of ribosome production, lipid metabolism, cold shock proteins, spermine biosynthesis, and glycolysis and in the later stages of riboflavin and coenzyme A (CoA) biosynthesis. In contrast, different chaperones, several fermentation pathways, and cysteine, serine, and pantothenate biosynthesis were found upregulated. Focusing on the Stickland amino acid fermentation and the central carbon metabolism, we discovered the ability of C. difficile to replenish its favored amino acid cysteine by a pathway starting from the glycolytic 3-phosphoglycerate via L-serine as intermediate. Following the growth course, the reductive equivalent pathways used were sequentially shifted from proline via leucine/phenylalanine to the central carbon metabolism first to butanoate fermentation and then further to lactate fermentation. The toxin production was found correlated mainly to fluxes of the central carbon metabolism. Toxin formation in the supernatant was detected when the flux changed from butanoate to lactate synthesis in the late stationary phase. The holistic view derived from the combination of transcriptome, proteome and metabolome data allowed us to uncover the major metabolic strategies that are used by the clostridial cells to maintain its cellular homeostasis and ensure survival under starvation conditions.
Deciphering the influence of Streptococcus pneumoniae global regulators on fitness and virulence
(2019)
Streptococcus pneumoniae (S. pneumoniae; the pneumococcus) is a Gram-positive, aerotolerant, and opportunistic bacteria, which colonizes the upper respiratory tract of human. S. pneumoniae can further migrate to other sterile parts of the body, and causes local as well as fatal infections like, pneumonia, septicaemia and meningitis. Due to incomplete amino acid pathways, pneumococci are auxotrophic for eight different amino acids including glutamine and arginine. The pneumococcus has adapted to the various host environmental conditions and a number of systems are dedicated for the transport and utilization of nutrients such as monosaccharides, amino acids and oligopeptides.
In this study the amino acid metabolism was characterised by 15N-isotopologue profiling in two different pneumococcal strains, D39 and TIGR4. Efficient uptake of a labelled amino acids mixture of 15N-labelled amino acids showed that S. pneumoniae has a preference for the amino acids transport instead of a de novo biosynthesis. It is known that glutamine (Gln) serves as main nitrogen source for S. pneumoniae. The 15N-labelled Gln used in this study demonstrated an efficient 15N-enrichment of Glu, Ala, Pro and Thr. Minor enrichment was seen for the amino acids Asp, Ile, Leu, Phe, Tyr, and Val. Remarkably, labelled Gly and Ser could be determined in strain TIGR4, whereas for strain D39 these two labelled amino acids were not detected. This confirms earlier studies with 13C-labelled glucose, which showed the biosynthesis of Ser out of Gly. Strain TIGR4 was able to grow in chemically-defined medium depleted of Gly confirming that Gly can be synthesized out of serine by the action of the enzyme serine hydroxymethyltransferase (SHMT).
The transcriptional regulator GlnR controls the Gln and Glu metabolism in S. pneumoniae. Hence, the impact of the repressor GlnR on amino acids metabolism was also studied. An increased 15N-enrichment was determined for Ala and Glu in both used pneumococcal strains, while an increased level of Pro was only measured in the isogenic glnR-mutant of non-encapsulated D39.
Arginine can also serve as nitrogen source in strain TIGR4. The arginine deiminase system metabolizes Arg into ornithine, carbamoyl phosphate and CO2 by the generation of 1 ATP and 2 mol NH3. Because of the truncation of the arcA gene strain D39 lacks arginine deiminase activity and has thus no functional ADS system. When 15N-Arg was added for growth, only in strain TIGR4, thirteen (13) labelled amino acids were detected with the highest enrichment for Ala, Glu and Thr. Genes coding for the enzymes of the arginine metabolism and for arginine uptake are regulated by the activator ArgR2 in strain TIGR4. Inactivation of ArgR2 was not accompanied by an enrichment of labelled amino acids, when the argR2-mutant was grown with 15N-labelled Arg indicative of the important role of ArgR2.
The bicistronic operon arcDT encoding the arginine/ornithine transporter ArcD and a putative peptidase ArcT belong to the peptidase family M20. The in silico comparison of structures revealed a significant homology of ArcT to PepV of L. delbrueckii and to Sapep of S. aureus known as carboxypeptidase. ArcT was heterologously expressed in E. coli and purified under reducing conditions. An enzymatic reaction was established and several dipeptides like Ala-Arg, Arg-Ala, and Ala-Asp were used as substrates. In addition, the dependency on divalent cations was analysed. Cleavage of the dipeptide Ala-Arg was detected in the presence of Mn2+ as cofactor under reducing conditions. Reduced peptidase activity was observed when Zn2+ was added. No cleavage of the tripeptide Ala-Ala-Arg could be shown indicating that ArcT acts as dipeptidase with the preference to the Arg residue at the C-terminal end.
Bacterial meningitis caused by S. pneumoniae was studied in an in vivo proteomic analysis. In a mouse meningitis model S. pneumoniae was isolated from the cerebrospinal fluid (CSF) by a filter extraction step. The MS analysis identified AliB and ComDE only from CSF isolated pneumococci indicating that these proteins are expressed under infection conditions. Mice infected with D39 wild-type and isogenic aliB, comDE and aliB-comDE double knockout mutants showed significantly less number of pleocytosis in the CSF and lower bacterial load in the blood compared to the wild-type. The results indicate that AliB and ComDE play an important role during meningitis.
Phenotypic characterization was carried out to identify differences between the wild-type and the aliB-, comDE- and aliB-comDE double mutants. Oxidative stress conditions were induced by the application of hydrogen peroxide or paraquat during growth in a chemically-defined medium similar to the CSF. No alteration in growth and survival of these mutants compared to the wild-type was observed suggesting that oxygen radicals play not an important role during the progression of meningitis. In addition, no differences of AliB expression was detected in the ComDE deficient D39. No impact of aliB and comDE-mutation on the expression of different virulence factors like pneumolysin or proteins involved in capsular biosynthesis was detected.
In vitro proteome analysis was performed to compare the wild-type to the AliB, and ComDE deficient D39 in the early and mid logarithmic growth phase. More than 70 % of theoretically expressed proteins were identified. In the aliB-mutant 33 proteins were differentally expressed in the early growth phase and 50 proteins differed during mid log growth. For the comDE mutant 24 and 11 proteins differed in expression in these two growth phases. Interestingly, high level of AliA expression was identified in all samples. The aliB-mutant had a decreased abundance of the proteins resembling an oligopeptide ABC transporter (AmiA, AmiC, AmiD, AmiE). In addition, another ABC transporter for iron transport encoded by spd_1607 to spd_ 1610 was higher expressed in the aliB-mutant. In the ComDE deficient mutant lower abundance of the Ami transporter sytem was identified. An increased abundance of proteins involved in the pyrimidine metabolism (PyrF, PyrE, PyrDb, PyrB and PyrR) was recognized only in the early growth phase of the comDE-mutant. These analyses demonstrate the marginal changes in protein synthesis during growth of S. pneumoniae. These studies demonstrated the adaptation of the proteome of S. pneumoniae to different growth conditions and the impact of regulatory proteins on the availability of carbon and nitrogen sources.
Staphylococcus aureus (S. aureus) ist einer der meist gefürchtetsten pathogenen Mikroorganismen, der verantwortlich ist für eine Vielzahl von nosokomialen Infektionen und Krankheiten. S. aureus ist in der Lage, sich an verändernde Umweltbedingungen auf Ebene der Genexpression anzupassen, was zu unterschiedlichen Proteinzusammensetzungen und somit zu Veränderungen in der Metabolitenkomposition und metabolischen Aktivität führt. Außerdem stellt die Fähigkeit, Resistenzen gegen gegenwärtig genutzte Antibiotika zu entwickeln, eine Gefahr dar und macht diesen Keim in seiner Behandlung so schwierig. Für ein vollständiges Verstehen der Proteom-, Transkriptom- und Metabolomdaten ist die Untersuchung der Enzymaktivitäten ein entscheidendes Hilfsmittel. In der vorliegenden Arbeit wurden die enzymkatalytischen Eigenschaften sowie die spezifischen Enzymaktivitäten der Enzyme des Intermediär- und Fermentationsstoffwechsels untersucht. Aus Zellen der logarithmischen, transienten und stationären Wachstumsphase unter aeroben wie auch anaeroben Bedingungen wurden für die Enzyme das pH-Optimum, die maximale Reaktionsgeschwindigkeit (vmax) und die Substratkonzentration der halbmaximalen Reaktionsgeschwindigkeit (Km) bestimmt. In S. aureus COL wird die Glucose unter aeroben Bedingungen hauptsächlich über die Glycolyse metabolisiert. Glucose-6-phosphat wird weiter zu Pyruvat umgesetzt, welches wiederum durch die Pyruvat-Oxidase zu Acetylphosphat oder durch den Pyruvat-Dehydrogenase-Komplex zu Acetyl-CoA verstoffwechselt wird. Durch die Phosphatacetyl-Transferase wird das Acetyl-CoA im Folgenden ebenfalls zu Acetylphosphat umgesetzt und nicht dem Citrat-Zyklus zugeführt. Die Acetat-Kinase nutzt das Acetylphosphat zur Generierung von ATP. Geringe extrazelluläre Lactat-Konzentrationen weisen auf eine geringere Bedeutung der Lactat-Dehydrogenase unter aeroben Wachstumsbedingungen hin. Gleichwohl wird ein kleiner Teil des Pyruvates zur Regeneration von NAD+ durch die Lactat-Dehydrogenase genutzt. In der transienten und stationären Wachstumsphase werden die Gene der Enzyme für Gluconeogenese und Citrat-Zyklus vermehrt exprimiert. Lactat und Acetat werden als Kohlenstoff- und Energiequelle wieder aufgenommen und dienen der Bildung unterschiedlicher Intermediate, wie beispielsweise der Bildung von NADPH über Glucose-6-phosphat im Pentose-Phosphat-Weg. Lediglich die Citrat-Synthase, Isocitrat-Dehydrogenase und Fumarat-Hydratase des Citrat-Zyklus konnten enzymologisch untersucht werden, was auf eine geringe metabolische Aktivität im Citrat-Zyklus hinweist. Möglicherweise dient der erste Teil des Citrat-Zyklus nur der Einführung von Aminosäuren als Kohlen- und Stickstoffquelle in den Metabolismus. Unter anaeroben Bedingungen wird die Glucose in der Glycolyse und der gemischten Säuregärung zu Lactat und Ethanol umgesetzt. Hohe spezifische Enzymaktivitäten der Lactat- und Alkohol-Dehydrogenase konnten nachgewiesen werden. Die Energie in Form von ATP wird auch in dieser Phase des Wachstums durch Substratkettenphosphorylierung generiert. Bacillus subtilis 168 (B. subtilis 168) ist ein grampositives apathogenes Bakterium, das durch die Zugabe von Pyruvat auch zum Wachstum unter sauerstofffreien Bedingungen befähigt ist. Es exprimiert Enzyme der 2,3-Butandiol- und Lactatfermentation. In der hier vorliegenden Arbeit wurden die enzymkatalytischen Eigenschaften von Enzymen des Intermediär- und Fermentationsstoffwechsels untersucht. In der logarithmischen Wachstumsphase wird die Glucose über die Glycolyse verstoffwechselt. Wie bei S. aureus COL ist der Eintritt des Glucose-6-phosphates in den Pentose-Phosphat-Weg aufgrund einer höheren spezifischen Enzymaktivität der Glucose-6-phosphat-Isomerase limitiert. Die Energie in Form von ATP wird auch hier hauptsächlich über Substratkettenphosphorylierungsreaktionen generiert. Die Bedeutung der Lactat-Dehydrogenase-Aktivität unter aeroben Bedingungen ist noch nicht eindeutig geklärt, jedoch kann davon ausgegangen werden, dass auch hier ein Teil des Pyruvates zur Regeneration von NAD+ durch die Lactat-Dehydrogenase umgesetzt wird. Unter anaeroben Bedingungen wurden hohe Lactat-Dehydrogenasen-Aktivitäten gemessen. Außerdem wird die Glucose zur Regeneration von NAD+ zu D-2,3-Butandiol fermentiert. Zusammenfassend ist zu sagen, dass enzymologische Untersuchungen und die Erforschung der spezifischen Enzymaktivitäten unter bestimmten Bedingungen ein gutes Hilfsmittel für metabolische Studien ist und diese gut mit vorhandenen Proteom- und Metabolomdaten verglichen werden können. Enzymanalysen sind nicht einfach handhabbar, bieten aber die Möglichkeit, einen Blick in die Physiologie von Mikroorganismen zu werfen. Für ein allumfassendes Verständnis ist es wichtig, Enzymaktivitäten zu untersuchen.
Periodontitis is one of the most prevalent oral diseases worldwide and is caused by multifactorial interactions between host and oral bacteria. Altered cellular metabolism of host and microbes releases a number of intermediary end products known as metabolites. There is an increasing interest in identifying metabolites from oral fluids such as saliva to widen the understanding of the complex pathogenesis of periodontitis. It is believed that some metabolites might serve as indicators toward early detection and screening of periodontitis and perhaps even for monitoring its prognosis in the future. Because contemporary periodontal screening methods are deficient, there is an urgent need for novel approaches in periodontal screening procedures. To this end, we associated oral parameters (clinical attachment level, periodontal probing depth, supragingival plaque, supragingival calculus, number of missing teeth, and removable denture) with a large set of salivary metabolites (n = 284) obtained by mass spectrometry among a subsample (n = 909) of nondiabetic participants from the Study of Health in Pomerania (SHIP-Trend-0). Linear regression analyses were performed in age-stratified groups and adjusted for potential confounders. A multifaceted image of associated metabolites (n = 107) was revealed with considerable differences according to age groups. In the young (20 to 39 y) and middle-aged (40 to 59 y) groups, metabolites were predominantly associated with periodontal variables, whereas among the older subjects (≥60 y), tooth loss was strongly associated with metabolite levels. Metabolites associated with periodontal variables were clearly linked to tissue destruction, host defense mechanisms, and bacterial metabolism. Across all age groups, the bacterial metabolite phenylacetate was significantly associated with periodontal variables. Our results revealed alterations of the salivary metabolome in association with age and oral health status. Among our comprehensive panel of metabolites, periodontitis was significantly associated with the bacterial metabolite phenylacetate, a promising substance for further biomarker research.
The influence of regulatory proteins on the physiology and virulence of Streptococcus pneumoniae
(2015)
In conclusion, this work identifies the regulator ArgR2 as activator of the S. pneumoniae TIGR4 arginine deiminase system and arginine-ornithine transporter ArcD, which is needed for uptake of the essential amino acid arginine. Although ArgR2 activates ArcD expression and uptake of arginine is required to maintain pneumococcal fitness, the deficiency of ArgR2 increases TIGR4 virulence under in vivo conditions, suggesting that other factors regulated by ArgR2 counterbalance the reduced uptake of arginine by ArcD. Thus this works illustrates that the physiological homeostasis of pneumococci is complex and that ArgR2 plays a key role in maintaining bacterial fitness. Moreover, Rex was identified as a regulator of housekeeping genes including genes encoding glycolytic enzymes. In vitro studies and gene expression analyses suggested that the regulator Rex does not have an influence on the physiology of S. pneumoniae. However, a co-infection experiment demonstrated that Rex is involved in maintaining pneumococcal fitness and robustness under in vivo conditions.