Maturation of the cytochrome <i>cd</i>1 nitrite reductase NirS from <i>Pseudomonas aeruginosa</i> requires transient interactions between the three proteins NirS, NirN and NirF

Nicke, Tristan; Schnitzer, Tobias; Münch, Karin; Adamczack, Julia; Haufschildt, Kristin; Buchmeier, Sabine; Kucklick, Martin; Felgenträger, Undine; Jänsch, Lothar; Riedel, Katharina; Layer, Gunhild

doi:10.1042/bsr20130043

Cited by 27 publications

(51 citation statements)

References 37 publications

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“…For the final insertion of heme d 1 into NirS, the system uses NirN, a structural homologue of NirS without nitrite reductase activity. NirS, NirF, and NirN form a stable complex during nitrite reductase maturation (26). In agreement, protein interactions of NorB and NorC with NirN were detected in our study (Table 3).…”

Section: Resultssupporting

confidence: 79%

“…The strongest interaction of NorBC (bait) for an isolated prey protein was detected for the periplasmic, membrane-attached lipoprotein NirF, the last enzyme in heme d 1 synthesis and a cofactor of nitrite reductases (26). For the final insertion of heme d 1 into NirS, the system uses NirN, a structural homologue of NirS without nitrite reductase activity.…”

Section: Resultsmentioning

confidence: 99%

“…The two c-type cytochromes NirM and NirC act as electron donors (25). NirN and NirF form a stable complex with the nitrite reductase NirS during enzyme maturation (26). NirF is involved in heme d 1 insertion (27).…”

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confidence: 99%

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Protein Network of the Pseudomonas aeruginosa Denitrification Apparatus

et al. 2016

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Oxidative phosphorylation using multiple-component, membrane-associated protein complexes is the most effective way for a cell to generate energy. Here, we systematically investigated the multiple protein-protein interactions of the denitrification apparatus of the pathogenic bacterium Pseudomonas aeruginosa. During denitrification, nitrate (Nar), nitrite (Nir), nitric oxide (Nor), and nitrous oxide (Nos) reductases catalyze the reaction cascade of NO 3؊ ¡ NO 2؊ ¡ NO ¡ N 2 O ¡ N 2 . Genetic experiments suggested that the nitric oxide reductase NorBC and the regulatory protein NosR are the nucleus of the denitrification protein network. We utilized membrane interactomics in combination with electron microscopy colocalization studies to elucidate the corresponding protein-protein interactions. The integral membrane proteins NorC, NorB, and NosR form the core assembly platform that binds the nitrate reductase NarGHI and the periplasmic nitrite reductase NirS via its maturation factor NirF. The periplasmic nitrous oxide reductase NosZ is linked via NosR. The nitrate transporter NarK2, the nitrate regulatory system NarXL, various nitrite reductase maturation proteins, NirEJMNQ, and the Nos assembly lipoproteins NosFL were also found to be attached. A number of proteins associated with energy generation, including electron-donating dehydrogenases, the complete ATP synthase, almost all enzymes of the tricarboxylic acid (TCA) cycle, and the Sec system of protein transport, among many other proteins, were found to interact with the denitrification proteins. This deduced nitrate respirasome is presumably only one part of an extensive cytoplasmic membrane-anchored protein network connecting cytoplasmic, inner membrane, and periplasmic proteins to mediate key activities occurring at the barrier/interface between the cytoplasm and the external environment. IMPORTANCEThe processes of cellular energy generation are catalyzed by large multiprotein enzyme complexes. The molecular basis for the interaction of these complexes is poorly understood. We employed membrane interactomics and electron microscopy to determine the protein-protein interactions involved. The well-investigated enzyme complexes of denitrification of the pathogenic bacterium Pseudomonas aeruginosa served as a model. Denitrification is one essential step of the universal N cycle and provides the bacterium with an effective alternative to oxygen respiration. This process allows the bacterium to form biofilms, which create low-oxygen habitats and which are a key in the infection mechanism. Our results provide new insights into the molecular basis of respiration, as well as opening a new window into the infection strategies of this pathogen.

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Section: Resultssupporting

confidence: 79%

Section: Resultsmentioning

confidence: 99%

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Protein Network of the Pseudomonas aeruginosa Denitrification Apparatus

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“…In line with this proposal it has been shown that NirN from P. aeruginosa interacts with both NirS and NirF in vivo. However, in that study it was also observed by UV-visible absorption spectroscopy of periplasmic protein fractions that the cofactor content of NirS in the P. aeruginosa ⌬nirN strain was different from that in the P. aeruginosa WT strain (15). Later, the same observation was reported for a ⌬nirN strain of Magnetospirillum gryphiswaldense (17).…”

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confidence: 55%

“…Depending on the organism, NirF is either a soluble periplasmic protein or attached to the outer face of the cytoplasmic membrane, most likely by a lipid anchor (14,15). In addition to its periplasmic location, purified recombinant NirF from Paracoccus pantotrophus has been shown to bind heme d 1 in vitro (13).…”

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confidence: 99%

NirN Protein from Pseudomonas aeruginosa is a Novel Electron-bifurcating Dehydrogenase Catalyzing the Last Step of Heme d1 Biosynthesis

Adamczack

Hoffmann

Papke

et al. 2014

Journal of Biological Chemistry

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Heme d1 plays an important role in denitrification as the essential cofactor of the cytochrome cd1 nitrite reductase NirS. At present, the biosynthesis of heme d1 is only partially understood. The last step of heme d1 biosynthesis requires a so far unknown enzyme that catalyzes the introduction of a double bond into one of the propionate side chains of the tetrapyrrole yielding the corresponding acrylate side chain. In this study, we show that a Pseudomonas aeruginosa PAO1 strain lacking the NirN protein does not produce heme d1. Instead, the NirS purified from this strain contains the heme d1 precursor dihydro-heme d1 lacking the acrylic double bond, as indicated by UV-visible absorption spectroscopy and resonance Raman spectroscopy. Furthermore, the dihydro-heme d1 was extracted from purified NirS and characterized by UV-visible absorption spectroscopy and finally identified by high-resolution electrospray ionization mass spectrometry. Moreover, we show that purified NirN from P. aeruginosa binds the dihydro-heme d1 and catalyzes the introduction of the acrylic double bond in vitro. Strikingly, NirN uses an electron bifurcation mechanism for the two-electron oxidation reaction, during which one electron ends up on its heme c cofactor and the second electron reduces the substrate/product from the ferric to the ferrous state. On the basis of our results, we propose novel roles for the proteins NirN and NirF during the biosynthesis of heme d1.

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Redox control of magnetosome biomineralization

2021

J. Ocean. Limnol.

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Maturation of the cytochrome cd1 nitrite reductase NirS from Pseudomonas aeruginosa requires transient interactions between the three proteins NirS, NirN and NirF

Cited by 27 publications

References 37 publications

Protein Network of the Pseudomonas aeruginosa Denitrification Apparatus

Protein Network of the Pseudomonas aeruginosa Denitrification Apparatus

NirN Protein from Pseudomonas aeruginosa is a Novel Electron-bifurcating Dehydrogenase Catalyzing the Last Step of Heme d1 Biosynthesis

Redox control of magnetosome biomineralization

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