Biochemical and functional characterization of UDP-galactose 4-epimerase from Aeromonas hydrophila

Bacteria of genus Aeromonas, responsible for a variety of pathological conditions in humans and fish, are ubiquitous waterborne bacteria. Aeromonas produces several virulent factors including a complex of lipopolysaccharide and surface array protein, involved in colonization. UDP-galactose 4-epimerase (GalE) catalyzes the production of UDP-galactose, a precursor for lipopolysaccharide biosynthesis, and thus is an important drug target. GalE exhibits interspecies variation and heterogeneity at its structural and functional level and therefore, the differences between the GalE of the host and the pathogen can be exploited for drug designing. In the present study, we report biochemical and functional characterization of the recombinant GalE of Aeromonas hydrophila. Unlike GalE reported from all other species, the purified recombinant GalE of A. hydrophila was found to exist as a monomer. This is the first report of UDP-galactose 4-epimerase from any species being a monomer. The molecular mass of the 6xHis-rGalE was determined to be 38271.477 (m/z). The 6xHis-rGalE with a K(m) of 0.5 mM for UDP-galactose exhibited optimum activity at 37 degrees C and pH 8-9. Spectrofluorimetric and CD analysis confirmed that the thermal inactivation was due to structural changes and not due to the NAD-dissociation. A relatively more ordered structure of the enzyme at pH 8 and 9 as compared to that at pH 6 or 7 suggests a key role of the electrostatic interactions in maintaining its native tertiary structure.     

Characterization of RbmD (Glycosyltransferase in Ribostamycin Gene Cluster) through neomycin production reconstituted from the engineered <Emphasis Type="Italic">Streptomyces fradiae</Emphasis> BS1

Amino acid homology analysis predicted that rbmD, a putative glycosyltransferase from Streptomyces ribosidificus ATCC 21294, has the highest homology with neoD in neomycin biosynthesis. S. fradiae BS1, in which the production of neomycin was abolished, was generated by disruption of the neoD gene in the neomycin producer S. fradiae. The restoration of neomycin by self complementation suggested that there was no polar effect in the mutant. In addition, S. fradiae BS6 was created with complementation by rbmD in S. fradiae BS1, and secondary metabolite analysis by ESI/MS, LC/MS and MS/MS showed the restoration of neomycin production in S. fradiae BS6. These gene inactivation and complementation studies suggested that, like neoD, rbmD functions as a 2-N-acetlyglucosaminyltransferase and demonstrated the potential for the generation of novel aminoglycoside antibiotics using glycosyltransferases in vivo.     

Mitochondrial Alternative Oxidase Maintains Respiration and Preserves Photosynthetic Capacity during Moderate Drought in Nicotiana tabacum

The mitochondrial electron transport chain includes an alternative oxidase (AOX) that is hypothesized to aid photosynthetic metabolism, perhaps by acting as an additional electron sink for photogenerated reductant or by dampening the generation of reactive oxygen species. Gas exchange, chlorophyll fluorescence, photosystem I (PSI) absorbance, and biochemical and protein analyses were used to compare respiration and photosynthesis of Nicotiana tabacum ‘Petit Havana SR1’ wild-type plants with that of transgenic AOX knockdown (RNA interference) and overexpression lines, under both well-watered and moderate drought-stressed conditions. During drought, AOX knockdown lines displayed a lower rate of respiration in the light than the wild type, as confirmed by two independent methods. Furthermore, CO₂ and light response curves indicated a nonstomatal limitation of photosynthesis in the knockdowns during drought, relative to the wild type. Also relative to the wild type, the knockdowns under drought maintained PSI and PSII in a more reduced redox state, showed greater regulated nonphotochemical energy quenching by PSII, and displayed a higher relative rate of cyclic electron transport around PSI. The origin of these differences may lie in the chloroplast ATP synthase amount, which declined dramatically in the knockdowns in response to drought. None of these effects were seen in plants overexpressing AOX. The results show that AOX is necessary to maintain mitochondrial respiration during moderate drought. In its absence, respiration rate slows and the lack of this electron sink feeds back on the photosynthetic apparatus, resulting in a loss of chloroplast ATP synthase that then limits photosynthetic capacity.The plant mitochondrial electron transport chain (ETC) is bifurcated such that electrons in the ubiquinone pool partition between the cytochrome (cyt) pathway (consisting of Complex III, cyt c, and Complex IV) and alternative oxidase (AOX; Finnegan et al., 2004; Millar et al., 2011; Vanlerberghe, 2013). AOX directly couples ubiquinol oxidation with O₂ reduction to water. This reduces the energy yield of respiration because, unlike Complexes III and IV, AOX is not proton pumping. Hence, AOX is an electron sink, the capacity of which is little encumbered by rates of ATP turnover. In this way, AOX might be well suited to prevent cellular over-reduction. Supporting this, transgenic Nicotiana tabacum leaves with suppressed amounts of AOX have increased concentrations of mitochondrial-localized superoxide radical (O₂−) and nitric oxide, the products that can arise when an over-reduced ETC results in electron leakage to O₂ or nitrite (Cvetkovska and Vanlerberghe, 2012, 2013).In angiosperms, AOX is encoded by a small gene family (Considine et al., 2002). In Arabidopsis (Arabidopsis thaliana), mutation or knockdown of the stress-responsive AOX1a gene family member dramatically reduces AOX protein and the capacity of the AOX respiration pathway to consume O₂. Several studies have shown that this loss of AOX capacity in Arabidopsis aox1a plants affected processes such as growth, carbon and energy metabolism, and/or the cellular network of reactive oxygen species (ROS) scavengers (Fiorani et al., 2005; Umbach et al., 2005; Watanabe et al., 2008; Giraud et al., 2008; Skirycz et al., 2010). However, in studies in which respiration was measured, it was consistently reported that the lack of AOX capacity had no significant impact on the respiration rate in the dark (R_D; Umbach et al., 2005; Giraud et al., 2008; Strodtkötter et al., 2009; Florez-Sarasa et al., 2011; Yoshida et al., 2011b; Gandin et al., 2012). The exceptions are two reports that R_D was actually higher in aox1a than in the wild type under some conditions (Watanabe et al., 2008; Vishwakarma et al., 2014). To our knowledge, how the lack of AOX affects respiration rate in the light (R_L) is not reported in Arabidopsis or other species.Numerous studies have established the importance of mitochondrial metabolism in the light to optimize photosynthesis (Hoefnagel et al., 1998; Raghavendra and Padmasree, 2003). In recent years, the potential importance of specifically AOX respiration during photosynthesis has been examined using the Arabidopsis aox1a plants (Giraud et al., 2008; Strodtkötter et al., 2009; Zhang et al., 2010; Florez-Sarasa et al., 2011; Yoshida et al., 2011a, 2011b). In general, these studies reported small perturbations of photosynthesis in standard-grown aox1a plants, including slightly lower rates of CO₂ uptake or O₂ release (Gandin et al., 2012; Vishwakarma et al., 2014), slightly higher rates of cyclic electron transport (CET; Yoshida et al., 2011b), and slightly increased susceptibility to photoinhibition after a high light treatment (Florez-Sarasa et al., 2011). Generally, these studies concluded that aox1a plants exhibit a biochemical limitation of photosynthesis, in line with the hypothesis that AOX serves as a sink for excess photogenerated reducing power, with the reductant likely reaching the mitochondrion via the malate valve (Noguchi and Yoshida, 2008; Taniguchi and Miyake, 2012). Similar to these Arabidopsis studies, we recently reported that well-watered N. tabacum AOX knockdowns grown at moderate irradiance display a slight reduced rate of photosynthesis (approximately 10%–15%) when measured at high irradiance. However, we established that the lower photosynthetic rate was the result of a stomatal rather than biochemical limitation of photosynthesis, and provided evidence that this stomatal limitation resulted from disrupted nitric oxide homeostasis within the guard cells of AOX knockdown plants (Cvetkovska et al., 2014).Drought is a common abiotic stress that can substantially curtail photosynthesis because stomatal closure, meant to conserve water, also restricts CO₂ availability to the Calvin cycle. Besides this well established stomatal limitation of photosynthesis, there may also be water deficit-sensitive biochemical components that contribute to the reduction of photosynthesis during drought. However, the nature of this biochemical limitation and the degree to which it contributes to the curtailment of photosynthesis during drought remain areas of active debate (Flexas et al., 2004; Lawlor and Tezara, 2009; Pinheiro and Chaves, 2011). Additional factors, such as patchy stomatal closure (Sharkey and Seemann, 1989; Gunasekera and Berkowitz, 1992) or changes in the conductance to CO₂ of mesophyll cells (Perez-Martin et al., 2009), can further complicate analyses of photosynthesis during drought.Metabolism can experience energy imbalances, when there is a mismatch between rates of synthesis and rates of utilization of ATP and/or NADPH, and the importance of mechanisms to minimize such imbalances has been emphasized (Cruz et al., 2005; Kramer and Evans, 2011; Vanlerberghe, 2013). For example, such imbalances may occur in the chloroplast when the use of ATP and NADPH by the Calvin cycle does not keep pace with the harvesting of light energy (Hüner et al., 2012). This can result in excess excitation energy that can damage photosynthetic components, perhaps through the generation of ROS (Asada, 2006; Noctor et al., 2014). Such a scenario has been hypothesized to underlie the development of the biochemical limitations of photosynthesis reported during drought (Lawlor and Tezara, 2009).In this study, we find that N. tabacum AOX knockdowns show a compromised rate of mitochondrial respiration in the light during moderate drought. This corresponds with a strong nonstomatal limitation of photosynthesis in these plants relative to the wild type, and we describe a biochemical basis for this photosynthetic limitation. The results indicate that AOX is a necessary electron sink to support photosynthesis during drought, a condition when the major photosynthetic electron sink, the Calvin cycle, is becoming limited by CO₂ availability.     

Evaluation of the potential for sexual reproduction in field populations of Cercospora beticola from USA

Cercospora leaf spot, caused by the hemibiotrophic fungal pathogen Cercospora beticola, is the most economically damaging foliar disease of sugarbeet worldwide. Although most C. beticola populations display characteristics reminiscent of sexual recombination, no teleomorph has been described. To assess whether populations in northern United States have characteristics consistent with sexual reproduction, 1024 isolates collected over a 3-y period were analyzed for frequency and distribution of mating type genes. After clone correction, an approximately equal distribution of mating types was found for each sampling year. Mating type frequency was also assessed in individual lesions. Lesions always consisted of isolates with a single mating type and microsatellite haplotype, but both mating types and up to five microsatellite haplotypes could be found on an individual leaf. The MAT1-1-1 and MAT1-2-1 genes were sequenced from 28 MAT1-1 and 28 MAT1-2 isolates, respectively. Three MAT1-1-1 nucleotide haplotypes were identified that encoded a single amino acid sequence. For MAT1-2-1, five nucleotide haplotypes were identified that encoded four protein variants. MAT1-1-1 and MAT1-2-1 gene expression analyses were conducted on plants inoculated with either or both mating types. MAT1-1-1 expression remained low, but MAT1-2-1 spiked during late stages of colonization. A segment of the MAT1-2-1 coding sequence was also found in MAT1-1 isolates. Taken together, these results suggest that C. beticola has the potential for sexual reproduction.     

Global Genetic Determinants of Mitochondrial DNA Copy Number

Many human diseases including development of cancer is associated with depletion of mitochondrial DNA (mtDNA) content. These diseases are collectively described as mitochondrial DNA depletion syndrome (MDS). High similarity between yeast and human mitochondria allows genomic study of the budding yeast to be used to identify human disease genes. In this study, we systematically screened the pre-existing respiratory-deficient Saccharomyces cerevisiae yeast strains using fluorescent microscopy and identified 102 nuclear genes whose deletions result in a complete mtDNA loss, of which 52 are not reported previously. Strikingly, these genes mainly encode protein products involved in mitochondrial protein biosynthesis process (54.9%). The rest of these genes either encode protein products associated with nucleic acid metabolism (14.7%), oxidative phosphorylation (3.9%), or other protein products (13.7%) responsible for bud-site selection, mitochondrial intermembrane space protein import, assembly of cytochrome-c oxidase, vacuolar protein sorting, protein-nucleus import, calcium-mediated signaling, heme biosynthesis and iron homeostasis. Thirteen (12.7%) of the genes encode proteins of unknown function. We identified human orthologs of these genes, conducted the interaction between the gene products and linked them to human mitochondrial disorders and other pathologies. In addition, we screened for genes whose defects affect the nuclear genome integrity. Our data provide a systematic view of the nuclear genes involved in maintenance of mitochondrial DNA. Together, our studies i) provide a global view of the genes regulating mtDNA content; ii) provide compelling new evidence toward understanding novel mechanism involved in mitochondrial genome maintenance and iii) provide useful clues in understanding human diseases in which mitochondrial defect and in particular depletion of mitochondrial genome plays a critical role.     

Resistance of mitochondrial DNA-depleted cells against cell death: role of mitochondrial superoxide dismutase

We have shown that mitochondrial DNA-depleted (rho(0)) SK-Hep1 hepatoma cells are resistant to apoptosis, contrary to previous papers reporting normal apoptotic susceptibility of rho(0) cells. We studied the changes of gene expression in SK-Hep1 rho(0) cells. DNA chip analysis showed that MnSOD expression was profoundly increased in rho(0) cells. O(2)(.) contents increased during rho(0) cell derivation but became normalized after establishment of rho(0) phenotypes, suggesting that MnSOD induction is an adaptive process to increased O(2)(.). rho(0) cells were resistant to menadione, paraquat, or doxorubicin, and O(2)(.) contents after treatment with them were lower in rho(0) cells compared with parental cells because of MnSOD overexpression. Expression levels and activity of glutathione peroxidases were also increased in rho(0) cells, rendering them resistant to exogenous H(2)O(2). rho(0) cells were resistant to p53, and intracellular ROS contents after p53 expression were lower compared with parental cells. Other types of rho(0) cells also showed increased MnSOD expression and resistance against ROS. Heme oxygenase-1 expression was increased in rho(0) cells, and a heme oxygenase-1 inhibitor decreased the induction of MnSOD in rho(0) cells and their resistance against ROS donors. These results indicate that rho(0) cells are resistant to cell death contrary to previous reports and suggest that an adaptive increase in the expression of antioxidant enzymes renders cancer cells or aged cells with frequent mitochondrial DNA mutations to resist against oxidative stress, host anti-cancer surveillance, or chemotherapeutic agents, conferring survival advantage on them.     

Fibrinogen Induces Microglia-Mediated Spine Elimination and Cognitive Impairment in an Alzheimer’s Disease Model

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Clumping characteristics and hydrophobic behaviour of an isolated bacterial strain from sewage sludge

Summary A clump-forming bacterial strain was isolated from a sludge community derived from a waste water treatment plant. The Gram-negative bacterium is hydrophobic and forms an extensive capsule while clumping in dilute medium (0.1% bacto peptone). Emulsan, a capsule inhibitor, does not affect the clumping ability of this bacterium. Clumps are not dispersed with high and low pH, detergents or chelators. Bacterial clumping selected by the waste water treatment processes appears to be a complex set of interactions within and between the strains of bacteria. This study reveals some of the complexities.     

Mitochondria as determinant of nucleotide pools and chromosomal stability

Mitochondrial function plays an important role in multiple human diseases and mutations in the mitochondrial genome have been detected in nearly every type of cancer investigated to date. However, the mechanism underlying the interrelation is unknown. We used human cell lines depleted of mitochondrial DNA as models and analyzed the outcome of mitochondrial dysfunction on major cellular repair activities. We show that the deoxyribonucleoside triphosphate (dNTP) pools are affected, most prominently we detect a 3-fold reduction of the dTTP pool when normalized to the number of cells in S-phase. It is known that imbalanced dNTP pools are mutagenic and in accordance, we show that mitochondrial dysfunction results in chromosomal instability, which can explain its role in tumor development. We did not find any straightforward correlation between ATP levels and dNTP pools in cells with defective mitochondrial activity. Our results suggest that mitochondria are central players in maintaining genomic stability and in controlling essential nuclear processes such as upholding a balanced supply of nucleotides.