Characterization of the
 cydAB
 -Encoded Cytochrome
 bd
 Oxidase from
 Mycobacterium smegmatis

Kana, Bavesh D; Weinstein, Edwin A.; Avarbock, David; Dawes, Stephanie S.; Rubin, Harvey; Mizrahi, Valerie

doi:10.1128/jb.183.24.7076-7086.2001

Cited by 142 publications

(182 citation statements)

References 68 publications

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“…In addition, up-regulation of Rv1623c, a subunit of cytochrome D terminal oxidase complex, during NRP2 is indicative of ATP synthesis through electron transport chain. The homolog of this protein in E. coli is a component of the aerobic respiratory chain that is predominant when cells are grown under low aeration (37,38). Our study suggests that cytochrome D terminal oxidase of MTB also might perform a similar function when the bacterium gets ready to enter dormancy.…”

Section: Validation Of Quantitative Proteomic Data By Qpcr-tomentioning

confidence: 71%

Profiling the Proteome of Mycobacterium tuberculosis during Dormancy and Reactivation

Gopinath

Raghunandanan

Gomez

et al. 2015

Molecular & Cellular Proteomics

114

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Tuberculosis, caused by Mycobacterium tuberculosis, still remains a major global health problem. The main obstacle in eradicating this disease is the ability of this pathogen to remain dormant in macrophages, and then reactivate later under immuno-compromised conditions. The physiology of hypoxic nonreplicating M. tuberculosis is well-studied using many in vitro dormancy models. However, the physiological changes that take place during the shift from dormancy to aerobic growth (reactivation) have rarely been subjected to a detailed investigation. In this study, we developed an in vitro reactivation system by re-aerating the virulent laboratory strain of M. tuberculosis that was made dormant employing Wayne's dormancy model, and compared the proteome profiles of dormant and reactivated bacteria using label-free onedimensional LC/MS/MS analysis. The proteome of dormant bacteria was analyzed at nonreplicating persistent stage 1 (NRP1) and stage 2 (NRP2), whereas that of reactivated bacteria was analyzed at 6 and 24 h post reaeration. Proteome of normoxially grown bacteria served as the reference. In total, 1871 proteins comprising 47% of the M. tuberculosis proteome were identified, and many of them were observed to be expressed differentially or uniquely during dormancy and reactivation. The number of proteins detected at different stages of dormancy (764 at NRP1, 691 at NRP2) and reactivation (768 at R6 and 983 at R24) was very low compared with that of the control (1663). The number of unique proteins identified during normoxia, NRP1, NRP2, R6, and R24 were 597, 66, 56, 73, and 94, respectively. We analyzed various biological functions during these conditions. Fluctuation in the relative quantities of proteins involved in energy metabolism during dormancy and reactivation was the most significant observation we made in this study. Proteins that are up-regulated or uniquely expressed during reactivation from dormancy offer to be attractive targets for therapeutic intervention to

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Section: Validation Of Quantitative Proteomic Data By Qpcr-tomentioning

confidence: 71%

Profiling the Proteome of Mycobacterium tuberculosis during Dormancy and Reactivation

Gopinath

Raghunandanan

Gomez

et al. 2015

Molecular & Cellular Proteomics

114

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“…burnetii replication in ACCM is optimal in a 2.5% oxygen environment and the presence of genes encoding cytochrome bd (i.e., cydAB) with high affinity for oxygen provides a biochemical/ physiological explanation for the observed growth phenotype. Interestingly, the intracellular bacteria Mycobacterium tuberculosis (19), Chlamydia trachomatis (20), and Rickettsia rickettsii all encode cydAB, suggesting adaptation to microaerobic metabolism in intracellular bacteria may be underappreciated. Indeed, transcriptional analysis of M. tuberculosis during infection of macrophages indicates the organism adapts to a reduced oxygen environment (21), and improved growth of Chlamydia pneumoniae is observed under low oxygen conditions (22).…”

Section: Discussionmentioning

confidence: 99%

Host cell-free growth of the Q fever bacterium Coxiella burnetii

Omsland

Cockrell²,

Howe³

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

362

378

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The inability to propagate obligate intracellular pathogens under axenic (host cell-free) culture conditions imposes severe experimental constraints that have negatively impacted progress in understanding pathogen virulence and disease mechanisms. Coxiella burnetii, the causative agent of human Q (Query) fever, is an obligate intracellular bacterial pathogen that replicates exclusively in an acidified, lysosome-like vacuole. To define conditions that support C. burnetii growth, we systematically evaluated the organism's metabolic requirements using expression microarrays, genomic reconstruction, and metabolite typing. This led to development of a complex nutrient medium that supported substantial growth (approximately 3 log 10) of C. burnetii in a 2.5% oxygen environment. Importantly, axenically grown C. burnetii were highly infectious for Vero cells and exhibited developmental forms characteristic of in vivo grown organisms. Axenic cultivation of C. burnetii will facilitate studies of the organism's pathogenesis and genetics and aid development of Q fever preventatives such as an effective subunit vaccine. Furthermore, the systematic approach used here may be broadly applicable to development of axenic media that support growth of other medically important obligate intracellular pathogens.axenic growth ͉ metabolism ͉ microaerophile ͉ obligate intracellular pathogen

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“…The behavior of the 13032⌬cydAB mutant could be due to low dissolved oxygen concentrations at the end of the exponential growth phase, which strongly restrict the activity of the low-affinity cytochrome aa 3 oxidase but not that of the high-affinity cytochrome bd oxidase. In Mycobacterium smegmatis, like C. glutamicum a member of the suborder Corynebacterineae (36), cytochrome bd oxidase was recently shown to be important for growth under microaerobic conditions and to be induced two-to threefold upon reduction of the O 2 partial pressure in the growth medium from 21% to 0.5% air saturation (14).…”

Section: Discussionmentioning

confidence: 99%

Role of Cytochrome bd Oxidase from Corynebacterium glutamicum in Growth and Lysine Production

Kabus

Niebisch

Bott

2007

Appl Environ Microbiol

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Corynebacterium glutamicum possesses two terminal oxidases, cytochrome aa 3 and cytochrome bd. Cytochrome aa 3 forms a supercomplex with the cytochrome bc 1 complex, which contains an unusual diheme cytochrome c 1 . Both the bc 1 -aa 3 supercomplex and cytochrome bd transfer reducing equivalents from menaquinol to oxygen; however, they differ in their proton translocation efficiency by a factor of three. Here, we analyzed the role of cytochrome bd for growth and lysine production. When cultivated in glucose minimal medium, a cydAB deletion mutant of C. glutamicum ATCC 13032 grew like the wild type in the exponential phase, but growth thereafter was inhibited, leading to a biomass formation 40% less than that of the wild type. Constitutive overproduction of functional cytochrome bd oxidase in ATCC 13032 led to a reduction of the growth rate by ϳ45% and of the maximal biomass by ϳ35%, presumably as a consequence of increased electron flow through the inefficient cytochrome bd oxidase. In the L-lysine-producing C. glutamicum strain MH20-22B, deletion of the cydAB genes had only minor effects on growth rate and biomass formation, but lysine production was increased by ϳ12%. Thus, the respiratory chain was shown to be a target for improving amino acid production by C. glutamicum.

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Characterization of the cydAB -Encoded Cytochrome bd Oxidase from Mycobacterium smegmatis

Cited by 142 publications

References 68 publications

Profiling the Proteome of Mycobacterium tuberculosis during Dormancy and Reactivation

Profiling the Proteome of Mycobacterium tuberculosis during Dormancy and Reactivation

Host cell-free growth of the Q fever bacterium Coxiella burnetii

Role of Cytochrome bd Oxidase from Corynebacterium glutamicum in Growth and Lysine Production

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