Anammox

Anammox, an abbreviation for anaerobic ammonium oxidation, is a globally important microbial process of the nitrogen cycle that takes place in many natural environments. The bacteria mediating this process were identified in 1999, and were a great surprise for the scientific community. 'Anammox' is also the trademarked name for an anammox-based ammonium removal technology developed by the Delft University of Technology. Anammox, an abbreviation for anaerobic ammonium oxidation, is a globally important microbial process of the nitrogen cycle that takes place in many natural environments. The bacteria mediating this process were identified in 1999, and were a great surprise for the scientific community. 'Anammox' is also the trademarked name for an anammox-based ammonium removal technology developed by the Delft University of Technology. In this biological process, which is a comproportionation reaction, nitrite and ammonium ions are converted directly into diatomic nitrogen and water. Globally, this process may be responsible for 30-50% of the N2 gas produced in the oceans. It is thus a major sink for fixed nitrogen and so limits oceanic primary productivity. The bacteria that perform the anammox process belong to the bacterial phylum Planctomycetes. Currently, five anammox genera have been discovered: Brocadia, Kuenenia, Anammoxoglobus, Jettenia (all fresh water species), and Scalindua (marine species). The anammox bacteria are characterized by several striking properties: they all possess one anammoxosome, a membrane bound compartment inside the cytoplasm which is the locus of anammox catabolism. Further, the membranes of these bacteria mainly consist of ladderane lipids so far unique in biology. Of special interest is the conversion to hydrazine (normally used as a high-energy rocket fuel, and poisonous to most living organisms) as an intermediate. A final striking feature of the organism is the extremely slow growth rate. The doubling time is anywhere from 7–22 days. The anammox bacteria are geared towards converting their substrates at very low concentrations; in other words, they have a very high affinity to their substrates ammonium and nitrite (sub-micromolar range). Anammox cells are packed with cytochrome c type proteins (≈30% of the protein complement), including the enzymes that perform the key catabolic reactions of the anammox process, making the cells remarkably red. The anammox process was originally found to occur only from 20 °C to 43 °C but more recently, anammox has been observed at temperatures from 36 °C to 52 °C in hot springs and 60 °C to 85 °C at hydrothermal vents located along the Mid-Atlantic Ridge. In 1932, it was reported that dinitrogen gas was generated via an unknown mechanism during fermentation in the sediments of Lake Mendota, Wisconsin, USA. In 1965, F. A. Richards noticed that most of the ammonium that should be produced during the anaerobic remineralization of organic matter was unaccounted for. As there was no known biological pathway for this transformation, biological anaerobic oxidation of ammonium received little further attention. In 1977, Engelbert Broda predicted the existence of two chemolithoautotrophic microorganisms capable of oxidizing ammonium to dinitrogen gas on the basis of thermodynamic calculations. It was thought that anaerobic oxidation of ammonium would not be feasible, assuming that the predecessors had tried and failed to establish a biological basis for those reactions. By the 1990s, Arnold Mulder's observations were just consistent with Richard's suggestion. In their anoxic denitrifying pilot reactor, ammonium disappeared at the expense of nitrite with a clear nitrogen production. The reactor used the effluent from a methanogenic pilot reactor, which contained ammonium, sulphide and other compounds, and nitrate from a nitrifying plant as the influent. The process was named 'anammox,' and was realized to have great significance in the removal of unwanted ammonium. The discovery of the anammox process was first publicly presented at the 5th European congress on biotechnology. By the mid-1990s, the discovery of anammox in the fluidized bed reactor was published. A maximum ammonium removal rate of 0.4 kg N/m3/d was achieved. It was shown that for every mole of ammonium consumed, 0.6 mol of nitrate was required, resulting in the formation of 0.8 mol of N2 gas. In the same year, the biological nature of anammox was identified. Labeling experiments with 15NH4+ in combination with 14NO3− showed that 14-15N2 was the dominant product making up 98.2% of the total labeled N2. It was realized that, instead of nitrate, nitrite was assumed as the oxidizing agent of ammonium in anammox reaction. Based on a previous study, Strous et al. calculated the stoichiometry of anammox process by mass balancing, which is widely accepted by other groups. Later, anammox bacteria were identified as planctomycetes, and the first identified anammox organism was named Candidatus 'Brocadia anammoxidans.' Before 2002, anammox was assumed to be a minor player in the nitrogen cycle within natural ecosystems. In 2002 however, anammox was found to play an important part in the biological nitrogen cycle, accounting for 24-67% of the total N2 production in the continental shelf sediments that were studied. The discovery of anammox process modified the concept of biological nitrogen cycle, as depicted in Figure 2. According to 15N labeling experiments carried out in 1997, ammonium is biologically oxidized by hydroxylamine, most likely derived from nitrite, as the probable electron acceptor. The conversion of hydrazine to dinitrogen gas is hypothesized to be the reaction that generates the electron equivalents for the reduction of nitrite to hydroxylamine. In general, two possible reaction mechanisms are addressed. One mechanism hypothesizes that a membrane-bound enzyme complex converts ammonium and hydroxylamine to hydrazine first, followed by the oxidation of hydrazine to dinitrogen gas in the periplasm. At the same time, nitrite is reduced to hydroxylamine at the cytoplasmic site of the same enzyme complex responsible for hydrazine oxidation with an internal electron transport (Figure 3a). The other mechanism postulates the following: ammonium and hydroxylamine are converted to hydrazine by a membrane-bound enzyme complex, hydrazine is oxidized in the periplasm to dinitrogen gas, and the generated electrons are transferred via an electron transport chain to nitrite reducing enzyme in the cytoplasm where nitrite is reduced to hydroxylamine (Figure 3b). Whether the reduction of nitrite and the oxidation of hydrazine occur at different sites of the same enzyme or the reactions are catalyzed by different enzyme systems connected via an electron transport chain remains to be investigated. In microbial nitrogen metabolism, the occurrence of hydrazine as an intermediate is rare. Hydrazine has been proposed as an enzyme-bound intermediate in the nitrogenase reaction.Recently, using detailed molecular analyses and combining complementary methods, Kartal and coworkers published strong evidence supporting the latter mechanism.Furthermore, the enzyme producing hydrazine, hydrazine synthase was purified and shown to produce hydrazine from NO and ammonium. The production of hydrazine from ammonium and NO was also supported by the resolution of the crystal structure of the enzyme hydrazine sythase. A possible role of nitric oxide (NO) or nitroxyl (HNO) in anammox was proposed by Hooper et al. by way of condensation of NO or HNO and ammonium on an enzyme related to the ammonium monooxygenase family. The formed hydrazine or imine could subsequently be converted by the enzyme hydroxylamine oxidase to dinitrogen gas, and the reducing equivalents produced in the reaction are required to combine NO or HNO and ammonium or to reduce nitrite to NO. Environmental genomics analysis of the species Candidatus Kuenenia stuttgartiensis, through a slightly different and complementary metabolism mechanism, suggested NO to be the intermediate instead of hydroxylamine (Figure 4). However, this hypothesis also agreed that hydrazine was an important intermediate in the process. In this pathway (Figure 4), there are two enzymes unique to anammox bacteria: hydrazine synthase (hzs) and hydrazine dehydrogenase (hdh). The HZS produces hydrazine from nitric oxide and ammonium, and HDH transfer the electrons from hydrazine to ferredoxin. Few new genes, such as some known fatty acid biosynthesis and S-adenosylmethionine radical enzyme genes, containing domains involved in electron transfer and catalysis have been detected. Anammox microorganisms can also directly couple NO reduction to ammonia oxidation, without the need for nitrite supply. Another, still unexplored, reaction mechanism involves anaerobic ammonium oxidation on anodes of bio-electrical systems. Such systems can be microbial fuel cells or microbial electrolysis cells. In the absence of dissolved oxygen, nitrite, or nitrate, microbes living in the anode compartment are able to oxidize ammonium to dinitrogen gas (N2) just as in the classical anammox process. At the same time, they unload the liberated electrons onto the anode, producing electrical current. This electrical current can be used either directly in fuel cell mode or for hydrogen and methane gas production in electrolysis mode. While there is no clarity on the reaction mechanism behind, one hypothesis is that nitrite, nitrate, or dinitrogen oxide play a role as intermediates. However, since the process occurs at very low electrochemical potentials, other, more speculative, reaction mechanisms seem possible as well. Until now, ten anammox species have been described, including seven that are available in laboratory enrichment cultures. All have the taxonomical status of Candidatus, as none were obtained as classical pure cultures. Known species are divided over five genera: (1) Kuenenia, represented by Kuenenia stuttgartiensis, (2) Brocadia (three species: B. anammoxidans, B. fulgida, and B. sinica), (3) Anammoxoglobus (one species: A. propionicus, (4) Jettenia (one species: J. asiatica, and (5) Scalindua (four species: S. brodae, S. sorokinii, S. wagneri, and S. profunda Representatives of the first four genera were enriched from sludge from wastewater treatment plants; K. stuttgartiensis, B. anammoxidans, B. fulgida, and A. propionicus were even obtained from the same inoculum. Scalindua dominates the marine environment, but is also found in some freshwater ecosystems and wastewater treatment plants. Together, these 10 species likely only represent a minute fraction of anammox biodiversity. For instance, there are currently over 2000 16S rRNA gene sequences affiliated with anammox bacteria that have been deposited to the Genbank (https://www.ncbi.nlm.nih.gov/genbank/), representing an overlooked continuum of species, subspecies, and strains, each apparently having found its specific niche in the wide variety of habitats where anammox bacteria are encountered. Species microdiversity is particularly impressive for the marine representative Scalindua. A question that remains to be investigated is which environmental factors determine species differentiation among anammox bacteria.