培养看不见的东西:来自James Tiedje的经验

IF 4.5 Q1 MICROBIOLOGY mLife Pub Date : 2023-09-01 DOI:10.1002/mlf2.12083
Yoichi Kamagata
{"title":"培养看不见的东西:来自James Tiedje的经验","authors":"Yoichi Kamagata","doi":"10.1002/mlf2.12083","DOIUrl":null,"url":null,"abstract":"In recounting Dr. James M. Tiedje's outstanding research achievements spanning the past 55 years, it is easy to overlook his early and mid-career endeavors. Specifically, his contribution to the aerobic degradation of pesticides and other chemicals, as well as methanogenic degradation of those compounds retains their brilliance. Many researchers in environmental microbiology have gained invaluable knowledge from these studies, which have been applied to the elucidation of previously uncultivated microorganisms. Dr. Tiedje embarked on his career in soil microbiology at Cornell University in 1964 under the guidance of Martin Alexander. Motivated by Rachel Carson's Silent Spring published in 1962, he developed a keen interest in studying the degradation of 2,4-dichlorophenoxy acetic acid (2,4-D), widely used as a broad-leaf herbicide. Dr. Tiedje found that an Arthrobacter species converts 2,4-D into chlorocatechols, facilitated by a soluble ether linkage-cleaving enzyme1, 2. Subsequently, extensive investigations into the 2,4-D degradation by aerobic microorganisms were conducted, leading to the identification of α-ketoglutarate-dependent dioxygenase, the enzyme involved in the first step of 2,4-D metabolism3 (Figure 1). The story starts with my involvement in the “2,4-D project.” The project took place at the Center for Microbial Ecology, Michigan State University (MSU), where we focused on microbial evolution. 2,4-D, being an anthropogenic chemical with no analogous compounds found in nature, provided an excellent opportunity to explore how enzymes with different original functions were recruited and evolved to adapt to 2,4-D degradation. The project was initiated by Profs. James M. Tiedje and Keiji Yano (followed by Prof. Koki Horikoshi) in 1991 and received funding from Japan Science and Technology Agency (JST, formerly JRDC) and National Science Foundation USA. It involved numerous scientists and over 10 postdocs from various parts of the world. It was the mid-1990s, a time before high-throughput genome sequencing became available, and molecular biological studies were conducted using classical methods such as DNA sequencing using big gel plates. During this period, I had been working on methanogenic Archaea till I joined the project. To begin, we initiated genetic analysis of known 2,4-D-degraders, as well as search for previously unknown 2,4-D-degrading microbes4, 5. Meanwhile, Dr. Tiedje, who was supposed to lead the project, was on sabbatical, enjoying the warmer climate of Hawaii (quite different from Michigan) and collaborating with Hawaiian researchers. He learned that there were soils in Hawaii that had not been exposed to 2,4-D, and he brought those untouched soils back to Michigan. The underlying idea was to investigate whether the microorganisms capable of breaking down this widely used chemical, which was artificially synthesized and sprayed in large quantities, were absent in the Hawaiian soils, or there were microbes possessing the prototypic enzyme. I inoculated a liquid culture containing 2,4-D with Hawaiian soil and spent day after day monitoring its degradation by liquid chromatography. Our initial expectation was that 2,4-D decomposition would not occur so readily. Indeed, for a while, no 2,4-D degradation was observed. However, after a few weeks or perhaps a month, some soil samples began to show signs of degradation. I was secretly excited that the 2,4-D-degrading microorganisms might be present in these remote regions that had never been associated with 2,4-D. Are the 2,4-D-degrading microorganisms entirely novel or are they the same Alcaligenes (currently called Curpriavidus) species that Dr. Tiedje and his team as well as everyone here at MSU have been studying for years? However, it was not easy to clarify the true nature of the microorganisms that had emerged in the test tube. This was primarily due to their inability to readily form colonies on agar media. Although numerous colonies appeared on the agar medium containing 2,4-D, it was evident that this was a result of adding more yeast extract than 2,4-D. Moreover, it was also clear that 2,4-D was not degraded in liquid culture without yeast extract. In addition, the Hewlett-Packard liquid chromatograph frequently malfunctioned, causing delays in analysis and hindering our ability to identify the problem. To overcome these challenges, we decided to conduct an experiment in which we added radioactive 14C-labeled 2,4-D to visualize which colonies would show the highest concentration of radioactivity. Numerous microorganisms grew in a myriad of locations on the agar medium containing 2,4-D. Radioactive colonies were scattered among them in a hidden manner. It was obvious that the only way to eliminate microorganisms unrelated to 2,4-D degradation was to significantly reduce the concentration of yeast extract, which would also slow down the growth of 2,4-D degraders. After months of intensive culture and isolation operations, we successfully isolated five 2,4-D-degrading microorganisms. Surprisingly, these strains were not the known 2,4-D-degrading bacteria, but rather closely related to Bradyrhizobium, a soil-dwelling microbe that is ubiquitous6. Five years later, one of the isolates (obtained from soil covered for 4800 years beneath a lava flow, effectively isolated from human impact before the colonization of Hawaii) was found to harbor an aromatic ring-hydroxylation dioxygenase (i.e., Rieske nonheme iron oxygenase), which is quite different from previously known 2,4-D metabolic enzymes7, 8. Since then, this enzyme and its relatives have been discovered to be widely distributed among soil microorganisms. However, the evolutionary origin of this enzyme still remains enigmatic. Before my involvement in the 2,4-D project, my focus was on cultivating methanogenic archaea (methanogens) and relevant microorganisms to elucidate the functions of key microorganisms in methane fermentation processes. I encountered challenges in culturing these organisms. However, working on the 2,4-D project reminded me that the difficulty of isolating microorganisms extends beyond anaerobic microbes and is a universal challenge in microbiology. It highlighted the crucial importance of isolation and cultivation in obtaining knowledge about their functions and characteristics. During that time, massive sequencing and metagenomic analyses had not yet emerged. We were far from a time when we could gain insights from genome sequences. After concluding my research on 2,4-D, I redirected my attention to syntrophs and methanogens under anaerobic conditions, a field that had long captivated my interest. Methanogens produce methane from very limited low-molecule compounds, specifically, hydrogen + CO2, formate, acetate, alcohols, and methyl compounds. These substrates for methanogenesis are derived from fermentative microbes that utilize high-molecule organic matters9 (Figure 2). Among them, some organisms, commonly referred to as syntrophs, are specifically associated with methanogens. Syntrophs break down (i.e., anaerobically oxidize) fatty acids, alcohols, and aromatic compounds, which are extremely difficult to be degraded for most of anaerobic microbes that utilize higher-molecule organic compounds, and they produce hydrogen and acetate in the process. The accumulation of hydrogen and acetate is thermodynamically unfavorable, and syntrophs cannot survive unless such products are immediately eliminated from the system or metabolized by other microorganisms. Methanogens are making a major contribution as scavengers of hydrogen and acetate. While research on syntrophs had been in its infancy for a long time9, 10, it was in the 1980s that research into their entities really began to take off. The researchers leading the way in this research field from its inception were Marvin Bryant and his group at the University of Illinois at Urbana-Champaign11-14. Dr. Tiedje also embarked on important research on syntrophs during this period. In the early 1980s—over 40 years ago, he obtained a simplified microbial population that degraded 3-chlorobenzoate to produce methane15-17. The discovery of anaerobic degradation of halogenated aromatic compounds was groundbreaking at the time. That is why a short but important paper was published in Science in 198215. Dr. Tiedje and his colleagues made the initial discovery of how a model halogenated compound, 3-chlorobenzoate, could be converted into methane. They began thoroughly studying the microorganisms in the consortium. This was accomplished by culture, observation, and chemical analysis but no genetics at all as there was no genome information on the Earth16-24. The 3-chlorobenzoate study reached a significant milestone with the complete isolation of strain DCB-1, which was later named Desulfomonile tiedjei21. Until then, no one had ever imagined that anaerobic microorganisms can conserve energy by using halogenated compounds as the terminal electron acceptor. Eventually, Dr. Tiedje's team (including Joseph Suflita, Daniel Shelton, Jan Dolfing, William Mohn, and others) revealed that 3-chlorobenzoate is dechlorinated by reductive dehalogenation to benzoate, which is broken down into acetate and H2/CO2 by a syntrophic bacterium, and the H2/CO2 is converted into methane by a methanogenic archaeon, while the acetate is used as an electron donor for dechlorination25-28. The series of studies showed that anaerobic syntrophy is not only involved in degradation of simple fatty acids but also more complex compounds, for example, halogenated aromatic compounds. Returning to our research, the fact that most of the anaerobic microorganisms were yet to be cultivated and that syntrophic metabolism in methanogenic environments remained largely unknown was a major motivating factor for our research. In the late 1990s, microbial ecology had made significant advancements through the utilization of 16S ribosomal RNA/DNA sequencing and fluorescence in situ hybridization (FISH) analysis, thanks to the pioneering work of Amann et al., which became powerful tools29. In 1995–1997, the complete genomes of Haemophilus influenzae, Bacillus subtilis, Synechocystis sp., and Escherichia coli were sequenced, but it was still some time before the era of high-throughput genome/metagenome sequencing would emerge. We first attempted to isolate and cultivate syntrophs that degrade acetate, propionate, and butyrate under thermophilic conditions. It was known that methane fermentation at around 50°C was quite effective for degradation of a variety of chemical compounds. However, the isolation process proved to be quite challenging. Even when a stable enrichment culture could be obtained, it was not easy to isolate the protagonist even if FISH can identify them. A potential solution to this problem was already hinted at early studies of syntrophs, where they were found to be capable of growing on their own without a partner organism, given certain substrates, such as D. tiedjei in pure culture with pyruvate and rumen fluid20, or Syntrophomonas wolfei in pure culture with crotonate30. Indeed, this method sometimes worked. We were eventually able to isolate a wide variety of anaerobic syntrophic microorganisms and their partner organisms (mainly methanogens) over the past 20 years, as summarized in Table 1, which includes corresponding studies31, 32, 34-72. It is important to note that most of these microbes are fastidious or recalcitrant, and took a long time to be isolated and cultured. Fortunately, these microorganisms have now gained widespread recognition among researchers, and their names are commonly referenced in a number of metagenomics articles. Thermoacetogenium phaeum, an acetate-oxidizing and hydrogen-producing microbe, was the first syntroph that the author's group isolated31. We learnt a lot from this bacterium about how syntroph behaves and makes a living31, 32, 60-62. It can switch between acetogenesis and reverse acetogenesis under different conditions. The latter (i.e., syntrophic growth) was only observed when hydrogenotrophic methanogen exists as an H2 consumer. This microbe was also found to drive the Wood–Ljungdahl pathway in both directions62. As for acetate metabolism, it had been widely believed that aceticlastic (acetotrophic) methanogens play a primary role in methanogenic environments. However, many reports indicate the importance of syntrophic acetate oxidation coupled with H2-consuming methanogenesis. Shigematsu et al. investigated acetate conversion pathways of methanogenic consortia in acetate-fed chemostats at dilution rates of 0.025 and 0.6 day−1 and found that nonaceticlastic syntrophic oxidation by acetate-oxidizing syntrophs and hydrogenotrophic methanogens dominated over aceticlastic methanogens at the low dilution rate, whereas aceticlastic cleavage was suggested to occupy a primary pathway in total methanogenesis at the high dilution rate73. We found that deep subsurface environments harbor both thermophilic acetate-oxidizing syntrophs and aceticlastic methanogens. Furthermore, the population changes depending on CO2 concentrations33. Due to the limited availability of acetate-oxidizing syntroph strains, our isolate has become a valuable model organism to study the population dynamics over acetate metabolism. Phenol had long been known to be degraded under methanogenic conditions, but the microbes responsible for the degradation reaction were not known at all. At least, it was evident that phenol can be only syntrophically metabolized and it is very challenging to reveal the entity of the microbes. Syntrophorhabdus aromaticivorans was the first tangible, obligately anaerobic, syntrophic organism capable of oxidizing phenol in association with a H2-scavenging methanogen partner40-42. It could metabolize not only phenol but also p-cresol, 4-hydroxybenzoate, isophthalate, and benzoate. Since numerous reports based on metagenomic analyses indicate that Syntrophorhabdus type of bacteria is abundant in phenol-degrading methanogenic communities and there are no other possible microbes (except for denitrifying phenol degraders), the organism may monopolize phenol degradation. The whole-genome analysis showed that S. aromaticivorans syntrophic phenol-degrading phenylphosphate synthase (PpsAB) and phenylphosphate carboxylase (PpcABCD) catalyze the first two steps of phenol metabolism into benzoate. It also shows benzoate degradation through hydration of the dienoyl-coenzyme A (CoA) intermediate as reported in Syntrophus aciditrophicus. The conversion of benzoyl-CoA into dienoyl-CoA is an extremely endergonic reduction; thus, it may be catalyzed by electron-bifurcating reduction that involves benzoyl-CoA reductase, hydrogenase, and heterodisulfide reductase. Studies on syntrophy culminated in the discovery and isolation of archaeon whose ancestor might have been the closest relative to eukaryotes48. Imachi et al. took deep-sea methane-seep sediment samples and enriched microbes by a continuous down-flow reactor using sponge as a carrier. After 12 years of dedicated efforts and various attempts, the microbe was isolated in coculture with Methanogenium sp. The archaeon named Candidatus Prometheoarchaeum syntrophicum is an anaerobic, extremely slow-growing, small coccus capable of metabolizing amino acids through syntrophy. The reason that the isolate organism is referred to as “candidatus” is simply because it has not yet been deposited to public culture collections due to the difficulty in yielding sufficient amounts of biomass to maintain and distribute. The microbe was the first cultured Asgard archaeon, harboring 80 eukaryotic-like proteins, and has characteristic protrusions. Imachi et al. proposed an attractive hypothesis for eukaryogenesis, in which a primordial Asgard archaeon cell interacts with the ancestral beneficial bacterial cells and eventually endogenizes it, which is termed the entangle–engulf–endogenize (E3) model. The model has recently been reinforced by the discovery of another archaeon named Candidatus Lokiarchaeum ossiferum enriched from sediments from a small estuarine canal74. From the 1970s to the 1990s, microbiology focused on cultivation, biochemistry, physiology, and genetics. Dr. Tiedje was one of the greatest contributors to this era. With the arrival of the 21st century and the emergence of massive metagenome data, microbiology, and environmental microbiology have transitioned to a new stage. Despite this shift, most of the results obtained from this stage have been a continuation of previous research. It should be noted that microbiology still heavily relies on the process of isolation and cultivation to uncover the truth behind morphology, physiology, metabolism, and energetics. Data science will reinforce the future of microbiology. Dr. Tiedje, on the other hand, was one of the first researchers to recognize the importance of data science. In 1997, he and Jim Cole took over ribosomal database project (RDP) that had been run by Profs. Carl Woese, Gary Olsen, and colleagues at the University of Illinois Urbana-Champaign75. The RDP had 1687 aligned sequences (now millions!) and all sequences were curated by Carl Woese himself in 1993 when Dr. Tiedje made the decision to take it over. Today, microbial ecology heavily relies on this database and relevant ones. In addition, Dr. Tiedje has dedicated himself to studying global-scale microbiomes including wastewater treatment plants, rain forests, permafrost, nitrogen-fertilized soils, and antibiotic-contaminated environments, all within the context of human issues. He consistently remains at the forefront of his field. I would like to express my utmost respect and always remember his earlier studies, which tends to be overlooked by many. I would like to express my gratitude to Prof. James M. Tiedje and all my collaborators in his laboratory at Michigan State University for their valuable contributions. I thank Prof. Masao Fukuda at Nagaoka University of Technology for providing the detailed records of the Joint project between JST (JRDC) and NSF (International Collarborative Project in Microbial Evolution) (1991–1996). I am also grateful to all the collaborators who greatly contributed to the exploration of novel microbes and their functions. This research was supported by JSPS KAKENHI grant number JPH05295.","PeriodicalId":94145,"journal":{"name":"mLife","volume":null,"pages":null},"PeriodicalIF":4.5000,"publicationDate":"2023-09-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"Cultivating the unseen: Lessons from James Tiedje\",\"authors\":\"Yoichi Kamagata\",\"doi\":\"10.1002/mlf2.12083\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"In recounting Dr. James M. Tiedje's outstanding research achievements spanning the past 55 years, it is easy to overlook his early and mid-career endeavors. Specifically, his contribution to the aerobic degradation of pesticides and other chemicals, as well as methanogenic degradation of those compounds retains their brilliance. Many researchers in environmental microbiology have gained invaluable knowledge from these studies, which have been applied to the elucidation of previously uncultivated microorganisms. Dr. Tiedje embarked on his career in soil microbiology at Cornell University in 1964 under the guidance of Martin Alexander. Motivated by Rachel Carson's Silent Spring published in 1962, he developed a keen interest in studying the degradation of 2,4-dichlorophenoxy acetic acid (2,4-D), widely used as a broad-leaf herbicide. Dr. Tiedje found that an Arthrobacter species converts 2,4-D into chlorocatechols, facilitated by a soluble ether linkage-cleaving enzyme1, 2. Subsequently, extensive investigations into the 2,4-D degradation by aerobic microorganisms were conducted, leading to the identification of α-ketoglutarate-dependent dioxygenase, the enzyme involved in the first step of 2,4-D metabolism3 (Figure 1). The story starts with my involvement in the “2,4-D project.” The project took place at the Center for Microbial Ecology, Michigan State University (MSU), where we focused on microbial evolution. 2,4-D, being an anthropogenic chemical with no analogous compounds found in nature, provided an excellent opportunity to explore how enzymes with different original functions were recruited and evolved to adapt to 2,4-D degradation. The project was initiated by Profs. James M. Tiedje and Keiji Yano (followed by Prof. Koki Horikoshi) in 1991 and received funding from Japan Science and Technology Agency (JST, formerly JRDC) and National Science Foundation USA. It involved numerous scientists and over 10 postdocs from various parts of the world. It was the mid-1990s, a time before high-throughput genome sequencing became available, and molecular biological studies were conducted using classical methods such as DNA sequencing using big gel plates. During this period, I had been working on methanogenic Archaea till I joined the project. To begin, we initiated genetic analysis of known 2,4-D-degraders, as well as search for previously unknown 2,4-D-degrading microbes4, 5. Meanwhile, Dr. Tiedje, who was supposed to lead the project, was on sabbatical, enjoying the warmer climate of Hawaii (quite different from Michigan) and collaborating with Hawaiian researchers. He learned that there were soils in Hawaii that had not been exposed to 2,4-D, and he brought those untouched soils back to Michigan. The underlying idea was to investigate whether the microorganisms capable of breaking down this widely used chemical, which was artificially synthesized and sprayed in large quantities, were absent in the Hawaiian soils, or there were microbes possessing the prototypic enzyme. I inoculated a liquid culture containing 2,4-D with Hawaiian soil and spent day after day monitoring its degradation by liquid chromatography. Our initial expectation was that 2,4-D decomposition would not occur so readily. Indeed, for a while, no 2,4-D degradation was observed. However, after a few weeks or perhaps a month, some soil samples began to show signs of degradation. I was secretly excited that the 2,4-D-degrading microorganisms might be present in these remote regions that had never been associated with 2,4-D. Are the 2,4-D-degrading microorganisms entirely novel or are they the same Alcaligenes (currently called Curpriavidus) species that Dr. Tiedje and his team as well as everyone here at MSU have been studying for years? However, it was not easy to clarify the true nature of the microorganisms that had emerged in the test tube. This was primarily due to their inability to readily form colonies on agar media. Although numerous colonies appeared on the agar medium containing 2,4-D, it was evident that this was a result of adding more yeast extract than 2,4-D. Moreover, it was also clear that 2,4-D was not degraded in liquid culture without yeast extract. In addition, the Hewlett-Packard liquid chromatograph frequently malfunctioned, causing delays in analysis and hindering our ability to identify the problem. To overcome these challenges, we decided to conduct an experiment in which we added radioactive 14C-labeled 2,4-D to visualize which colonies would show the highest concentration of radioactivity. Numerous microorganisms grew in a myriad of locations on the agar medium containing 2,4-D. Radioactive colonies were scattered among them in a hidden manner. It was obvious that the only way to eliminate microorganisms unrelated to 2,4-D degradation was to significantly reduce the concentration of yeast extract, which would also slow down the growth of 2,4-D degraders. After months of intensive culture and isolation operations, we successfully isolated five 2,4-D-degrading microorganisms. Surprisingly, these strains were not the known 2,4-D-degrading bacteria, but rather closely related to Bradyrhizobium, a soil-dwelling microbe that is ubiquitous6. Five years later, one of the isolates (obtained from soil covered for 4800 years beneath a lava flow, effectively isolated from human impact before the colonization of Hawaii) was found to harbor an aromatic ring-hydroxylation dioxygenase (i.e., Rieske nonheme iron oxygenase), which is quite different from previously known 2,4-D metabolic enzymes7, 8. Since then, this enzyme and its relatives have been discovered to be widely distributed among soil microorganisms. However, the evolutionary origin of this enzyme still remains enigmatic. Before my involvement in the 2,4-D project, my focus was on cultivating methanogenic archaea (methanogens) and relevant microorganisms to elucidate the functions of key microorganisms in methane fermentation processes. I encountered challenges in culturing these organisms. However, working on the 2,4-D project reminded me that the difficulty of isolating microorganisms extends beyond anaerobic microbes and is a universal challenge in microbiology. It highlighted the crucial importance of isolation and cultivation in obtaining knowledge about their functions and characteristics. During that time, massive sequencing and metagenomic analyses had not yet emerged. We were far from a time when we could gain insights from genome sequences. After concluding my research on 2,4-D, I redirected my attention to syntrophs and methanogens under anaerobic conditions, a field that had long captivated my interest. Methanogens produce methane from very limited low-molecule compounds, specifically, hydrogen + CO2, formate, acetate, alcohols, and methyl compounds. These substrates for methanogenesis are derived from fermentative microbes that utilize high-molecule organic matters9 (Figure 2). Among them, some organisms, commonly referred to as syntrophs, are specifically associated with methanogens. Syntrophs break down (i.e., anaerobically oxidize) fatty acids, alcohols, and aromatic compounds, which are extremely difficult to be degraded for most of anaerobic microbes that utilize higher-molecule organic compounds, and they produce hydrogen and acetate in the process. The accumulation of hydrogen and acetate is thermodynamically unfavorable, and syntrophs cannot survive unless such products are immediately eliminated from the system or metabolized by other microorganisms. Methanogens are making a major contribution as scavengers of hydrogen and acetate. While research on syntrophs had been in its infancy for a long time9, 10, it was in the 1980s that research into their entities really began to take off. The researchers leading the way in this research field from its inception were Marvin Bryant and his group at the University of Illinois at Urbana-Champaign11-14. Dr. Tiedje also embarked on important research on syntrophs during this period. In the early 1980s—over 40 years ago, he obtained a simplified microbial population that degraded 3-chlorobenzoate to produce methane15-17. The discovery of anaerobic degradation of halogenated aromatic compounds was groundbreaking at the time. That is why a short but important paper was published in Science in 198215. Dr. Tiedje and his colleagues made the initial discovery of how a model halogenated compound, 3-chlorobenzoate, could be converted into methane. They began thoroughly studying the microorganisms in the consortium. This was accomplished by culture, observation, and chemical analysis but no genetics at all as there was no genome information on the Earth16-24. The 3-chlorobenzoate study reached a significant milestone with the complete isolation of strain DCB-1, which was later named Desulfomonile tiedjei21. Until then, no one had ever imagined that anaerobic microorganisms can conserve energy by using halogenated compounds as the terminal electron acceptor. Eventually, Dr. Tiedje's team (including Joseph Suflita, Daniel Shelton, Jan Dolfing, William Mohn, and others) revealed that 3-chlorobenzoate is dechlorinated by reductive dehalogenation to benzoate, which is broken down into acetate and H2/CO2 by a syntrophic bacterium, and the H2/CO2 is converted into methane by a methanogenic archaeon, while the acetate is used as an electron donor for dechlorination25-28. The series of studies showed that anaerobic syntrophy is not only involved in degradation of simple fatty acids but also more complex compounds, for example, halogenated aromatic compounds. Returning to our research, the fact that most of the anaerobic microorganisms were yet to be cultivated and that syntrophic metabolism in methanogenic environments remained largely unknown was a major motivating factor for our research. In the late 1990s, microbial ecology had made significant advancements through the utilization of 16S ribosomal RNA/DNA sequencing and fluorescence in situ hybridization (FISH) analysis, thanks to the pioneering work of Amann et al., which became powerful tools29. In 1995–1997, the complete genomes of Haemophilus influenzae, Bacillus subtilis, Synechocystis sp., and Escherichia coli were sequenced, but it was still some time before the era of high-throughput genome/metagenome sequencing would emerge. We first attempted to isolate and cultivate syntrophs that degrade acetate, propionate, and butyrate under thermophilic conditions. It was known that methane fermentation at around 50°C was quite effective for degradation of a variety of chemical compounds. However, the isolation process proved to be quite challenging. Even when a stable enrichment culture could be obtained, it was not easy to isolate the protagonist even if FISH can identify them. A potential solution to this problem was already hinted at early studies of syntrophs, where they were found to be capable of growing on their own without a partner organism, given certain substrates, such as D. tiedjei in pure culture with pyruvate and rumen fluid20, or Syntrophomonas wolfei in pure culture with crotonate30. Indeed, this method sometimes worked. We were eventually able to isolate a wide variety of anaerobic syntrophic microorganisms and their partner organisms (mainly methanogens) over the past 20 years, as summarized in Table 1, which includes corresponding studies31, 32, 34-72. It is important to note that most of these microbes are fastidious or recalcitrant, and took a long time to be isolated and cultured. Fortunately, these microorganisms have now gained widespread recognition among researchers, and their names are commonly referenced in a number of metagenomics articles. Thermoacetogenium phaeum, an acetate-oxidizing and hydrogen-producing microbe, was the first syntroph that the author's group isolated31. We learnt a lot from this bacterium about how syntroph behaves and makes a living31, 32, 60-62. It can switch between acetogenesis and reverse acetogenesis under different conditions. The latter (i.e., syntrophic growth) was only observed when hydrogenotrophic methanogen exists as an H2 consumer. This microbe was also found to drive the Wood–Ljungdahl pathway in both directions62. As for acetate metabolism, it had been widely believed that aceticlastic (acetotrophic) methanogens play a primary role in methanogenic environments. However, many reports indicate the importance of syntrophic acetate oxidation coupled with H2-consuming methanogenesis. Shigematsu et al. investigated acetate conversion pathways of methanogenic consortia in acetate-fed chemostats at dilution rates of 0.025 and 0.6 day−1 and found that nonaceticlastic syntrophic oxidation by acetate-oxidizing syntrophs and hydrogenotrophic methanogens dominated over aceticlastic methanogens at the low dilution rate, whereas aceticlastic cleavage was suggested to occupy a primary pathway in total methanogenesis at the high dilution rate73. We found that deep subsurface environments harbor both thermophilic acetate-oxidizing syntrophs and aceticlastic methanogens. Furthermore, the population changes depending on CO2 concentrations33. Due to the limited availability of acetate-oxidizing syntroph strains, our isolate has become a valuable model organism to study the population dynamics over acetate metabolism. Phenol had long been known to be degraded under methanogenic conditions, but the microbes responsible for the degradation reaction were not known at all. At least, it was evident that phenol can be only syntrophically metabolized and it is very challenging to reveal the entity of the microbes. Syntrophorhabdus aromaticivorans was the first tangible, obligately anaerobic, syntrophic organism capable of oxidizing phenol in association with a H2-scavenging methanogen partner40-42. It could metabolize not only phenol but also p-cresol, 4-hydroxybenzoate, isophthalate, and benzoate. Since numerous reports based on metagenomic analyses indicate that Syntrophorhabdus type of bacteria is abundant in phenol-degrading methanogenic communities and there are no other possible microbes (except for denitrifying phenol degraders), the organism may monopolize phenol degradation. The whole-genome analysis showed that S. aromaticivorans syntrophic phenol-degrading phenylphosphate synthase (PpsAB) and phenylphosphate carboxylase (PpcABCD) catalyze the first two steps of phenol metabolism into benzoate. It also shows benzoate degradation through hydration of the dienoyl-coenzyme A (CoA) intermediate as reported in Syntrophus aciditrophicus. The conversion of benzoyl-CoA into dienoyl-CoA is an extremely endergonic reduction; thus, it may be catalyzed by electron-bifurcating reduction that involves benzoyl-CoA reductase, hydrogenase, and heterodisulfide reductase. Studies on syntrophy culminated in the discovery and isolation of archaeon whose ancestor might have been the closest relative to eukaryotes48. Imachi et al. took deep-sea methane-seep sediment samples and enriched microbes by a continuous down-flow reactor using sponge as a carrier. After 12 years of dedicated efforts and various attempts, the microbe was isolated in coculture with Methanogenium sp. The archaeon named Candidatus Prometheoarchaeum syntrophicum is an anaerobic, extremely slow-growing, small coccus capable of metabolizing amino acids through syntrophy. The reason that the isolate organism is referred to as “candidatus” is simply because it has not yet been deposited to public culture collections due to the difficulty in yielding sufficient amounts of biomass to maintain and distribute. The microbe was the first cultured Asgard archaeon, harboring 80 eukaryotic-like proteins, and has characteristic protrusions. Imachi et al. proposed an attractive hypothesis for eukaryogenesis, in which a primordial Asgard archaeon cell interacts with the ancestral beneficial bacterial cells and eventually endogenizes it, which is termed the entangle–engulf–endogenize (E3) model. The model has recently been reinforced by the discovery of another archaeon named Candidatus Lokiarchaeum ossiferum enriched from sediments from a small estuarine canal74. From the 1970s to the 1990s, microbiology focused on cultivation, biochemistry, physiology, and genetics. Dr. Tiedje was one of the greatest contributors to this era. With the arrival of the 21st century and the emergence of massive metagenome data, microbiology, and environmental microbiology have transitioned to a new stage. Despite this shift, most of the results obtained from this stage have been a continuation of previous research. It should be noted that microbiology still heavily relies on the process of isolation and cultivation to uncover the truth behind morphology, physiology, metabolism, and energetics. Data science will reinforce the future of microbiology. Dr. Tiedje, on the other hand, was one of the first researchers to recognize the importance of data science. In 1997, he and Jim Cole took over ribosomal database project (RDP) that had been run by Profs. Carl Woese, Gary Olsen, and colleagues at the University of Illinois Urbana-Champaign75. The RDP had 1687 aligned sequences (now millions!) and all sequences were curated by Carl Woese himself in 1993 when Dr. Tiedje made the decision to take it over. Today, microbial ecology heavily relies on this database and relevant ones. In addition, Dr. Tiedje has dedicated himself to studying global-scale microbiomes including wastewater treatment plants, rain forests, permafrost, nitrogen-fertilized soils, and antibiotic-contaminated environments, all within the context of human issues. He consistently remains at the forefront of his field. I would like to express my utmost respect and always remember his earlier studies, which tends to be overlooked by many. I would like to express my gratitude to Prof. James M. Tiedje and all my collaborators in his laboratory at Michigan State University for their valuable contributions. I thank Prof. Masao Fukuda at Nagaoka University of Technology for providing the detailed records of the Joint project between JST (JRDC) and NSF (International Collarborative Project in Microbial Evolution) (1991–1996). I am also grateful to all the collaborators who greatly contributed to the exploration of novel microbes and their functions. This research was supported by JSPS KAKENHI grant number JPH05295.\",\"PeriodicalId\":94145,\"journal\":{\"name\":\"mLife\",\"volume\":null,\"pages\":null},\"PeriodicalIF\":4.5000,\"publicationDate\":\"2023-09-01\",\"publicationTypes\":\"Journal Article\",\"fieldsOfStudy\":null,\"isOpenAccess\":false,\"openAccessPdf\":\"\",\"citationCount\":\"0\",\"resultStr\":null,\"platform\":\"Semanticscholar\",\"paperid\":null,\"PeriodicalName\":\"mLife\",\"FirstCategoryId\":\"1085\",\"ListUrlMain\":\"https://doi.org/10.1002/mlf2.12083\",\"RegionNum\":0,\"RegionCategory\":null,\"ArticlePicture\":[],\"TitleCN\":null,\"AbstractTextCN\":null,\"PMCID\":null,\"EPubDate\":\"\",\"PubModel\":\"\",\"JCR\":\"Q1\",\"JCRName\":\"MICROBIOLOGY\",\"Score\":null,\"Total\":0}","platform":"Semanticscholar","paperid":null,"PeriodicalName":"mLife","FirstCategoryId":"1085","ListUrlMain":"https://doi.org/10.1002/mlf2.12083","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q1","JCRName":"MICROBIOLOGY","Score":null,"Total":0}
引用次数: 0

摘要

20世纪90年代末,由于Amann等人的开创性工作,微生物生态学通过利用16S核糖体RNA/DNA测序和荧光原位杂交(FISH)分析取得了重大进展,成为强有力的工具29。1995-1997年,流感嗜血杆菌、枯草芽孢杆菌、聚胞菌和大肠杆菌的全基因组测序完成,但距离高通量基因组/宏基因组测序时代的到来还有一段时间。我们首先尝试分离和培养在嗜热条件下降解醋酸盐、丙酸盐和丁酸盐的合养菌。众所周知,50℃左右的甲烷发酵对多种化合物的降解非常有效。然而,事实证明,隔离过程相当具有挑战性。即使可以获得稳定的富集培养物,即使FISH可以识别,也不容易分离出主角。在对共生菌的早期研究中已经暗示了这个问题的一个潜在解决方案,在研究中发现,在特定的基质下,它们能够在没有伴侣的情况下自行生长,例如用丙酮酸和瘤胃液纯培养的D. tiedjei,或用巴豆酸纯培养的狼共生单胞菌。事实上,这种方法有时是有效的。在过去的20年中,我们最终能够分离出各种厌氧合养微生物及其伴侣生物(主要是产甲烷菌),如表1所示,其中包括相应的研究31,32,34 -72。值得注意的是,这些微生物大多是挑剔的或顽固的,需要很长时间才能分离和培养。幸运的是,这些微生物现在已经得到了研究人员的广泛认可,它们的名字在一些宏基因组学文章中经常被引用。热醋酸菌(Thermoacetogenium phaeum)是一种醋酸盐氧化和产氢微生物,是作者小组分离到的第一个同质菌31。我们从这个细菌那里了解了很多关于同质菌的行为和生存的知识。在不同条件下可在丙酮生成和反丙酮生成之间切换。后者(即,合养生长)仅在氢营养产甲烷菌作为H2消费者存在时观察到。这种微生物也被发现在两个方向上驱动Wood-Ljungdahl通路62。在醋酸代谢方面,人们普遍认为产甲烷菌在产甲烷环境中起主要作用。然而,许多报告指出了醋酸合营养氧化与消耗h2的甲烷生成的重要性。Shigematsu等人研究了在稀释率为0.025和0.6 d−1的情况下,醋酸盐饲养的化生菌中产甲烷菌群的醋酸转化途径,发现在低稀释率下,醋酸盐氧化型合养菌和氢营养型产甲烷菌的非醋酸化合养氧化作用优于醋酸化产甲烷菌,而在高稀释率下,醋酸化裂解作用占据了总甲烷生成的主要途径73。我们发现深层地下环境中同时存在嗜热的醋酸氧化合养菌和醋酸产甲烷菌。此外,种群数量的变化取决于二氧化碳浓度。由于可获得的醋酸盐氧化合营养菌株有限,本分离菌株已成为研究醋酸盐代谢种群动态的有价值的模式生物。人们早就知道苯酚在产甲烷的条件下会被降解,但负责降解反应的微生物却根本不为人所知。至少,很明显,苯酚只能被共养代谢,而揭示微生物的实体是非常具有挑战性的。芳香合养菌是第一个能够与清除h2的甲烷菌伙伴一起氧化苯酚的有形的、专性厌氧的合养生物40-42。它不仅能代谢苯酚,还能代谢对甲酚、4-羟基苯甲酸酯、间苯二甲酸酯和苯甲酸酯。由于基于宏基因组分析的大量报道表明,在苯酚降解的产甲烷菌群落中,Syntrophorhabdus型细菌大量存在,并且没有其他可能的微生物(除反硝化苯酚降解菌外),因此该生物可能垄断了苯酚的降解。全基因组分析表明,S. aromaticivorans合成型苯酚降解苯磷酸合成酶(PpsAB)和苯磷酸羧化酶(PpcABCD)催化苯酚代谢为苯甲酸盐的前两步。它还显示苯甲酸酯的降解通过水合二烯酰辅酶A (CoA)中间体,如报道在合营养盐。苯甲酰辅酶a转化为二烯酰辅酶a是一个极耗氧还原过程;因此,它可以通过涉及苯甲酰辅酶a还原酶、氢化酶和异二硫还原酶的电子分叉还原催化。
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Cultivating the unseen: Lessons from James Tiedje
In recounting Dr. James M. Tiedje's outstanding research achievements spanning the past 55 years, it is easy to overlook his early and mid-career endeavors. Specifically, his contribution to the aerobic degradation of pesticides and other chemicals, as well as methanogenic degradation of those compounds retains their brilliance. Many researchers in environmental microbiology have gained invaluable knowledge from these studies, which have been applied to the elucidation of previously uncultivated microorganisms. Dr. Tiedje embarked on his career in soil microbiology at Cornell University in 1964 under the guidance of Martin Alexander. Motivated by Rachel Carson's Silent Spring published in 1962, he developed a keen interest in studying the degradation of 2,4-dichlorophenoxy acetic acid (2,4-D), widely used as a broad-leaf herbicide. Dr. Tiedje found that an Arthrobacter species converts 2,4-D into chlorocatechols, facilitated by a soluble ether linkage-cleaving enzyme1, 2. Subsequently, extensive investigations into the 2,4-D degradation by aerobic microorganisms were conducted, leading to the identification of α-ketoglutarate-dependent dioxygenase, the enzyme involved in the first step of 2,4-D metabolism3 (Figure 1). The story starts with my involvement in the “2,4-D project.” The project took place at the Center for Microbial Ecology, Michigan State University (MSU), where we focused on microbial evolution. 2,4-D, being an anthropogenic chemical with no analogous compounds found in nature, provided an excellent opportunity to explore how enzymes with different original functions were recruited and evolved to adapt to 2,4-D degradation. The project was initiated by Profs. James M. Tiedje and Keiji Yano (followed by Prof. Koki Horikoshi) in 1991 and received funding from Japan Science and Technology Agency (JST, formerly JRDC) and National Science Foundation USA. It involved numerous scientists and over 10 postdocs from various parts of the world. It was the mid-1990s, a time before high-throughput genome sequencing became available, and molecular biological studies were conducted using classical methods such as DNA sequencing using big gel plates. During this period, I had been working on methanogenic Archaea till I joined the project. To begin, we initiated genetic analysis of known 2,4-D-degraders, as well as search for previously unknown 2,4-D-degrading microbes4, 5. Meanwhile, Dr. Tiedje, who was supposed to lead the project, was on sabbatical, enjoying the warmer climate of Hawaii (quite different from Michigan) and collaborating with Hawaiian researchers. He learned that there were soils in Hawaii that had not been exposed to 2,4-D, and he brought those untouched soils back to Michigan. The underlying idea was to investigate whether the microorganisms capable of breaking down this widely used chemical, which was artificially synthesized and sprayed in large quantities, were absent in the Hawaiian soils, or there were microbes possessing the prototypic enzyme. I inoculated a liquid culture containing 2,4-D with Hawaiian soil and spent day after day monitoring its degradation by liquid chromatography. Our initial expectation was that 2,4-D decomposition would not occur so readily. Indeed, for a while, no 2,4-D degradation was observed. However, after a few weeks or perhaps a month, some soil samples began to show signs of degradation. I was secretly excited that the 2,4-D-degrading microorganisms might be present in these remote regions that had never been associated with 2,4-D. Are the 2,4-D-degrading microorganisms entirely novel or are they the same Alcaligenes (currently called Curpriavidus) species that Dr. Tiedje and his team as well as everyone here at MSU have been studying for years? However, it was not easy to clarify the true nature of the microorganisms that had emerged in the test tube. This was primarily due to their inability to readily form colonies on agar media. Although numerous colonies appeared on the agar medium containing 2,4-D, it was evident that this was a result of adding more yeast extract than 2,4-D. Moreover, it was also clear that 2,4-D was not degraded in liquid culture without yeast extract. In addition, the Hewlett-Packard liquid chromatograph frequently malfunctioned, causing delays in analysis and hindering our ability to identify the problem. To overcome these challenges, we decided to conduct an experiment in which we added radioactive 14C-labeled 2,4-D to visualize which colonies would show the highest concentration of radioactivity. Numerous microorganisms grew in a myriad of locations on the agar medium containing 2,4-D. Radioactive colonies were scattered among them in a hidden manner. It was obvious that the only way to eliminate microorganisms unrelated to 2,4-D degradation was to significantly reduce the concentration of yeast extract, which would also slow down the growth of 2,4-D degraders. After months of intensive culture and isolation operations, we successfully isolated five 2,4-D-degrading microorganisms. Surprisingly, these strains were not the known 2,4-D-degrading bacteria, but rather closely related to Bradyrhizobium, a soil-dwelling microbe that is ubiquitous6. Five years later, one of the isolates (obtained from soil covered for 4800 years beneath a lava flow, effectively isolated from human impact before the colonization of Hawaii) was found to harbor an aromatic ring-hydroxylation dioxygenase (i.e., Rieske nonheme iron oxygenase), which is quite different from previously known 2,4-D metabolic enzymes7, 8. Since then, this enzyme and its relatives have been discovered to be widely distributed among soil microorganisms. However, the evolutionary origin of this enzyme still remains enigmatic. Before my involvement in the 2,4-D project, my focus was on cultivating methanogenic archaea (methanogens) and relevant microorganisms to elucidate the functions of key microorganisms in methane fermentation processes. I encountered challenges in culturing these organisms. However, working on the 2,4-D project reminded me that the difficulty of isolating microorganisms extends beyond anaerobic microbes and is a universal challenge in microbiology. It highlighted the crucial importance of isolation and cultivation in obtaining knowledge about their functions and characteristics. During that time, massive sequencing and metagenomic analyses had not yet emerged. We were far from a time when we could gain insights from genome sequences. After concluding my research on 2,4-D, I redirected my attention to syntrophs and methanogens under anaerobic conditions, a field that had long captivated my interest. Methanogens produce methane from very limited low-molecule compounds, specifically, hydrogen + CO2, formate, acetate, alcohols, and methyl compounds. These substrates for methanogenesis are derived from fermentative microbes that utilize high-molecule organic matters9 (Figure 2). Among them, some organisms, commonly referred to as syntrophs, are specifically associated with methanogens. Syntrophs break down (i.e., anaerobically oxidize) fatty acids, alcohols, and aromatic compounds, which are extremely difficult to be degraded for most of anaerobic microbes that utilize higher-molecule organic compounds, and they produce hydrogen and acetate in the process. The accumulation of hydrogen and acetate is thermodynamically unfavorable, and syntrophs cannot survive unless such products are immediately eliminated from the system or metabolized by other microorganisms. Methanogens are making a major contribution as scavengers of hydrogen and acetate. While research on syntrophs had been in its infancy for a long time9, 10, it was in the 1980s that research into their entities really began to take off. The researchers leading the way in this research field from its inception were Marvin Bryant and his group at the University of Illinois at Urbana-Champaign11-14. Dr. Tiedje also embarked on important research on syntrophs during this period. In the early 1980s—over 40 years ago, he obtained a simplified microbial population that degraded 3-chlorobenzoate to produce methane15-17. The discovery of anaerobic degradation of halogenated aromatic compounds was groundbreaking at the time. That is why a short but important paper was published in Science in 198215. Dr. Tiedje and his colleagues made the initial discovery of how a model halogenated compound, 3-chlorobenzoate, could be converted into methane. They began thoroughly studying the microorganisms in the consortium. This was accomplished by culture, observation, and chemical analysis but no genetics at all as there was no genome information on the Earth16-24. The 3-chlorobenzoate study reached a significant milestone with the complete isolation of strain DCB-1, which was later named Desulfomonile tiedjei21. Until then, no one had ever imagined that anaerobic microorganisms can conserve energy by using halogenated compounds as the terminal electron acceptor. Eventually, Dr. Tiedje's team (including Joseph Suflita, Daniel Shelton, Jan Dolfing, William Mohn, and others) revealed that 3-chlorobenzoate is dechlorinated by reductive dehalogenation to benzoate, which is broken down into acetate and H2/CO2 by a syntrophic bacterium, and the H2/CO2 is converted into methane by a methanogenic archaeon, while the acetate is used as an electron donor for dechlorination25-28. The series of studies showed that anaerobic syntrophy is not only involved in degradation of simple fatty acids but also more complex compounds, for example, halogenated aromatic compounds. Returning to our research, the fact that most of the anaerobic microorganisms were yet to be cultivated and that syntrophic metabolism in methanogenic environments remained largely unknown was a major motivating factor for our research. In the late 1990s, microbial ecology had made significant advancements through the utilization of 16S ribosomal RNA/DNA sequencing and fluorescence in situ hybridization (FISH) analysis, thanks to the pioneering work of Amann et al., which became powerful tools29. In 1995–1997, the complete genomes of Haemophilus influenzae, Bacillus subtilis, Synechocystis sp., and Escherichia coli were sequenced, but it was still some time before the era of high-throughput genome/metagenome sequencing would emerge. We first attempted to isolate and cultivate syntrophs that degrade acetate, propionate, and butyrate under thermophilic conditions. It was known that methane fermentation at around 50°C was quite effective for degradation of a variety of chemical compounds. However, the isolation process proved to be quite challenging. Even when a stable enrichment culture could be obtained, it was not easy to isolate the protagonist even if FISH can identify them. A potential solution to this problem was already hinted at early studies of syntrophs, where they were found to be capable of growing on their own without a partner organism, given certain substrates, such as D. tiedjei in pure culture with pyruvate and rumen fluid20, or Syntrophomonas wolfei in pure culture with crotonate30. Indeed, this method sometimes worked. We were eventually able to isolate a wide variety of anaerobic syntrophic microorganisms and their partner organisms (mainly methanogens) over the past 20 years, as summarized in Table 1, which includes corresponding studies31, 32, 34-72. It is important to note that most of these microbes are fastidious or recalcitrant, and took a long time to be isolated and cultured. Fortunately, these microorganisms have now gained widespread recognition among researchers, and their names are commonly referenced in a number of metagenomics articles. Thermoacetogenium phaeum, an acetate-oxidizing and hydrogen-producing microbe, was the first syntroph that the author's group isolated31. We learnt a lot from this bacterium about how syntroph behaves and makes a living31, 32, 60-62. It can switch between acetogenesis and reverse acetogenesis under different conditions. The latter (i.e., syntrophic growth) was only observed when hydrogenotrophic methanogen exists as an H2 consumer. This microbe was also found to drive the Wood–Ljungdahl pathway in both directions62. As for acetate metabolism, it had been widely believed that aceticlastic (acetotrophic) methanogens play a primary role in methanogenic environments. However, many reports indicate the importance of syntrophic acetate oxidation coupled with H2-consuming methanogenesis. Shigematsu et al. investigated acetate conversion pathways of methanogenic consortia in acetate-fed chemostats at dilution rates of 0.025 and 0.6 day−1 and found that nonaceticlastic syntrophic oxidation by acetate-oxidizing syntrophs and hydrogenotrophic methanogens dominated over aceticlastic methanogens at the low dilution rate, whereas aceticlastic cleavage was suggested to occupy a primary pathway in total methanogenesis at the high dilution rate73. We found that deep subsurface environments harbor both thermophilic acetate-oxidizing syntrophs and aceticlastic methanogens. Furthermore, the population changes depending on CO2 concentrations33. Due to the limited availability of acetate-oxidizing syntroph strains, our isolate has become a valuable model organism to study the population dynamics over acetate metabolism. Phenol had long been known to be degraded under methanogenic conditions, but the microbes responsible for the degradation reaction were not known at all. At least, it was evident that phenol can be only syntrophically metabolized and it is very challenging to reveal the entity of the microbes. Syntrophorhabdus aromaticivorans was the first tangible, obligately anaerobic, syntrophic organism capable of oxidizing phenol in association with a H2-scavenging methanogen partner40-42. It could metabolize not only phenol but also p-cresol, 4-hydroxybenzoate, isophthalate, and benzoate. Since numerous reports based on metagenomic analyses indicate that Syntrophorhabdus type of bacteria is abundant in phenol-degrading methanogenic communities and there are no other possible microbes (except for denitrifying phenol degraders), the organism may monopolize phenol degradation. The whole-genome analysis showed that S. aromaticivorans syntrophic phenol-degrading phenylphosphate synthase (PpsAB) and phenylphosphate carboxylase (PpcABCD) catalyze the first two steps of phenol metabolism into benzoate. It also shows benzoate degradation through hydration of the dienoyl-coenzyme A (CoA) intermediate as reported in Syntrophus aciditrophicus. The conversion of benzoyl-CoA into dienoyl-CoA is an extremely endergonic reduction; thus, it may be catalyzed by electron-bifurcating reduction that involves benzoyl-CoA reductase, hydrogenase, and heterodisulfide reductase. Studies on syntrophy culminated in the discovery and isolation of archaeon whose ancestor might have been the closest relative to eukaryotes48. Imachi et al. took deep-sea methane-seep sediment samples and enriched microbes by a continuous down-flow reactor using sponge as a carrier. After 12 years of dedicated efforts and various attempts, the microbe was isolated in coculture with Methanogenium sp. The archaeon named Candidatus Prometheoarchaeum syntrophicum is an anaerobic, extremely slow-growing, small coccus capable of metabolizing amino acids through syntrophy. The reason that the isolate organism is referred to as “candidatus” is simply because it has not yet been deposited to public culture collections due to the difficulty in yielding sufficient amounts of biomass to maintain and distribute. The microbe was the first cultured Asgard archaeon, harboring 80 eukaryotic-like proteins, and has characteristic protrusions. Imachi et al. proposed an attractive hypothesis for eukaryogenesis, in which a primordial Asgard archaeon cell interacts with the ancestral beneficial bacterial cells and eventually endogenizes it, which is termed the entangle–engulf–endogenize (E3) model. The model has recently been reinforced by the discovery of another archaeon named Candidatus Lokiarchaeum ossiferum enriched from sediments from a small estuarine canal74. From the 1970s to the 1990s, microbiology focused on cultivation, biochemistry, physiology, and genetics. Dr. Tiedje was one of the greatest contributors to this era. With the arrival of the 21st century and the emergence of massive metagenome data, microbiology, and environmental microbiology have transitioned to a new stage. Despite this shift, most of the results obtained from this stage have been a continuation of previous research. It should be noted that microbiology still heavily relies on the process of isolation and cultivation to uncover the truth behind morphology, physiology, metabolism, and energetics. Data science will reinforce the future of microbiology. Dr. Tiedje, on the other hand, was one of the first researchers to recognize the importance of data science. In 1997, he and Jim Cole took over ribosomal database project (RDP) that had been run by Profs. Carl Woese, Gary Olsen, and colleagues at the University of Illinois Urbana-Champaign75. The RDP had 1687 aligned sequences (now millions!) and all sequences were curated by Carl Woese himself in 1993 when Dr. Tiedje made the decision to take it over. Today, microbial ecology heavily relies on this database and relevant ones. In addition, Dr. Tiedje has dedicated himself to studying global-scale microbiomes including wastewater treatment plants, rain forests, permafrost, nitrogen-fertilized soils, and antibiotic-contaminated environments, all within the context of human issues. He consistently remains at the forefront of his field. I would like to express my utmost respect and always remember his earlier studies, which tends to be overlooked by many. I would like to express my gratitude to Prof. James M. Tiedje and all my collaborators in his laboratory at Michigan State University for their valuable contributions. I thank Prof. Masao Fukuda at Nagaoka University of Technology for providing the detailed records of the Joint project between JST (JRDC) and NSF (International Collarborative Project in Microbial Evolution) (1991–1996). I am also grateful to all the collaborators who greatly contributed to the exploration of novel microbes and their functions. This research was supported by JSPS KAKENHI grant number JPH05295.
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