土壤铁氧化物对有机质产甲烷过程的影响及其机制

甲烷(CH4)是重要的温室气体和清洁能源。土壤铁氧化物作为重要的环境因子对有机质产甲烷过程具有重要影响。强氧化性且易微生物还原的铁氧化物对产甲烷具有抑制作用,其抑制机理为:(1)铁还原菌与产甲烷菌竞争产甲烷底物(乙酸或H_2)抑制产甲烷过程;(2)产甲烷菌利用Fe(Ⅲ)氧化底物抑制甲烷产生;(3)铁氧化物提高体系氧化还原电势抑制产甲烷过程。然而,具有导电性且晶型较高的铁氧化物可作为电子导体促进互营菌与产甲烷菌之间的直接电子传递,加速产甲烷过程。本文系统阐述了不同类型铁氧化物对有机质互营产甲烷过程的抑制或促进效应及作用机制,并在此基础上探讨了铁氧化物影响产甲烷过程的研究趋势,以期推动铁氧化物在抑制温室气体和促进清洁能源生产方面的实际应用。     

产甲烷条件下岩溶湿地沉积物中古菌群落的变化规律

【背景】桂林会仙湿地位于喀斯特峰丛洼地和峰丛平原的过渡区,主要由岩溶地下河补给,水质呈现富钙偏碱特征,是一处典型的岩溶湿地环境,湿地沉积物以厌氧环境为主,独特的环境特征使之成为研究新型厌氧微生物的理想场所。氢型产甲烷菌和乙酸型产甲烷菌是环境中有机质厌氧降解的重要参与者,但目前会仙湿地产甲烷菌生理生态功能的研究十分有限。【目的】揭示乙酸盐营养型产甲烷条件和氢气营养型产甲烷条件下岩溶湿地环境古菌群落结构的变化规律和产甲烷菌的主要类群,探讨岩溶环境古菌的功能和相互关系。【方法】以会仙岩溶湿地沉积物为研究材料,分别以乙酸盐和氢气为唯一能源物进行富集培养,结合未添加任何能源底物的对照处理,动态监测产甲烷通量,分别构建了3个共包含146条古菌16S rRNA基因全长序列的文库,以及3个共包含138条甲基辅酶M还原酶基因mcr A基因序列的文库,通过构建系统发育树比较分析不同产甲烷底物培养条件下典型岩溶湿地古菌群落的变化规律。【结果】从乙酸型和氢型产甲烷条件培养物顶空气中都检测到了几乎等浓度的甲烷产生,甲烷八叠球菌是mcr A文库中主要的古菌类群,其中包含了Methanosarcina属古菌、Zoige Cluster I (ZC-I)和ANME-2d Cluster (AD)类群古菌,以及两个相对独立且不包含任何参考序列的分支KT-I和KT-II,可能代表产甲烷菌的新类群;经过两种产甲烷条件的富集培养后,ZC-I、AD和KT-II类群古菌的序列数占比有较为显著的增加(45%–155%);深古菌(Bathyarchaeota)是所有古菌16Sr RNA基因文库的优势类群,序列占比为88%–100%,其中MCG-11亚群最为丰富,占所有深古菌的84%,并且在乙酸盐产甲烷条件下增加了17%。【结论】会仙湿地沉积物中蕴涵着丰富的新型古菌序列,沉积物中主要的氢型产甲烷菌和乙酸型产甲烷菌都来自甲烷八叠球菌目,深古菌在岩溶环境和乙酸型产甲烷条件下可能都发挥着重要的作用。     

不同抑制剂对乙酸降解产甲烷及产甲烷菌群结构的影响

摘要:【目的】研究不同温度条件下的石油烃降解产甲烷菌系中是否存在乙酸互营氧化产甲烷代谢途径。【方法】以3个不同温度条件的正十六烷烃降解产甲烷菌系Y15(15℃)、M82(35℃)和SK(55℃)作为接种物,通过乙酸喂养实验、并添加乙酸营养型产甲烷古菌的选择性抑制剂NH4Cl和CH3F,结合末端限制性片段长度多态性(terminal restriction fragment length polymorphism,T-RFLP)和克隆文库技术,分析乙酸产甲烷潜力及产甲烷古菌群落的演替趋势,推测产甲烷代谢途径的变化趋势。【结果】无论是否添加NH4Cl和CH3 F,这3个菌系都可以利用乙酸生长并产生甲烷,但是添加NH4Cl和CH3 F后产甲烷延滞期增加,最大比甲烷增长速率降低;只添加乙酸后,3个不同温度的菌系的古菌群落主要由乙酸营养型产甲烷古菌甲烷鬃毛菌属(Methanosaeta)组成,其丰度分别为92.8±1.4%、97.3±2.4%和82.8±9.0%;当添加选择性抑制剂NH4Cl,3 个菌系中的Methanosaeta的丰度分别变为98.5±0.7%、87.4±4.8%和6.1±8.6%,中温菌系M82中氢营养型产甲烷古菌甲烷袋装菌属(Methanoculleus)的相对丰度增加到12. 6±4.0%,高温菌系SK中另一类氢营养型产甲烷古菌甲烷热杆菌属(Methanothermobacter)增至84.3±1.5%;当添加选择性抑制剂CH3 F,Methanosaeta丰度分别降至77.1 ± 14.5%,86.4±6.1%和35.8±7.8%,低温菌系Y15中的甲烷八叠球菌属(Methanosarcina)增高(15.7±21%),这类产甲烷古菌具有多种产甲烷代谢途径,M82中Methanoculleus丰度上升到13.6±13.1%,SK中Methanothermobacter丰度增大到48.5±11.2%。【结论】在低温条件下,菌系Y15可能主要通过乙酸裂解完成产甲烷代谢,在中高温条件下,菌系M82和SK中可能存在乙酸互营氧化产甲烷代谢途径,并且甲烷的产生分别通过不同种群的氢营养型产甲烷古菌来完成。     

滨海湿地甲烷产生途径和产甲烷菌研究进展

滨海湿地在全球碳循环中起着重要的作用,其甲烷排放量占全球海洋甲烷排放的75%.本文综述了滨海湿地主要甲烷产生途径、产甲烷菌种类及其影响因子.滨海湿地SO₄^2-含量丰富,乙酸发酵和H₂/CO₂途径产甲烷受抑制,乙酸营养型和氢营养型产甲烷菌丰度较低;而利用甲胺类等“非竞争性”底物的C1甲基化合物歧化途径不受硫酸还原菌竞争底物的限制,兼性营养型产甲烷菌成为产甲烷优势菌.盐度与SO₄^2-含量和植被类型密切相关,影响竞争性电子和产甲烷底物的种类和含量,对甲烷产生途径和产甲烷菌群落结构有重要影响.目前,滨海湿地产甲烷菌群落结构、甲烷产生途径的关键控制因素尚需明确,其对甲烷排放的影响有待进一步研究.     

稻鱼共生系统的土壤产甲烷和甲烷氧化微生物群落

稻鱼共生对稻田甲烷(CH₄)排放产生明显影响，但稻鱼共生是否影响与CH₄排放相关的产甲烷菌和甲烷氧化菌仍有待阐明。本研究以全球重要农业文化遗产——青田稻鱼系统为例，通过田间试验，比较研究了水稻单作系统(RM)、无饲料投放的稻鱼共生系统(RFN)和有饲料投放的稻鱼共生系统(RFF)水稻和田鱼的产量、土壤碳氮磷含量以及产甲烷和甲烷氧化微生物的特征。结果表明，RFF的水稻产量和土壤碳氮增量均显著高于RM。荧光定量PCR分析表明，稻鱼共生(RFN和RFF)的产甲烷菌和甲烷氧化菌丰度显著高于RM,且RFF的产甲烷菌丰度显著高于RFN。Illumina Miseq测序分析表明，稻鱼共生显著影响产甲烷菌群落结构，但对甲烷氧化菌群落结构的影响不显著；对于不同代谢类型的产甲烷菌，稻鱼共生(RFN和RFF)氢营养型产甲烷菌的丰度显著高于RM,且RFF的乙酸营养型产甲烷菌丰度显著高于RFN;对于不同代谢类型的甲烷氧化菌，RFN和RFF对类型Ⅰ的甲烷氧化菌丰度影响均不显著；RFF中类型Ⅱ的甲烷氧化菌丰度显著高于RM和RFN。可见，稻鱼共生可明显影响产甲烷菌和甲烷氧化...     

低温湿地甲烷古菌及其介导的甲烷产生途径

甲烷是重要的温室气体,低温湿地是大气甲烷的重要来源,因为湿地土壤中生活着大量的微生物包括甲烷古菌,它们将有机物降解转化为甲烷.本文总结了近年来低温湿地甲烷古菌群落组成、甲烷产生途径及其与环境的关系.研究显示,乙酸是低温湿地中主要的产甲烷物质,氢产甲烷过程主要发生在中温地区或酸性泥炭土中,而在盐碱水域中甲醇、甲胺是甲烷的重要底物.位于我国青藏高原的若尔盖湿地具有高海拔但低纬度的地理特征,我们的前期研究却显示甲醇在该湿地的甲烷排放中具有重要贡献.相应地,低温湿地中的甲烷古菌主要是利用甲基类化合物/乙酸的甲烷八叠球菌目和氢营养型的甲烷微球菌目.然而不同类型湿地甲烷排放途径及甲烷古菌的差异主要与环境的土壤类型、pH及植被类型相关,如刚毛荸荠生长的若尔盖湿地土壤中来源于甲醇的甲烷占全部甲烷的l7％;而木里苔草土壤中乙酸是产甲烷的主要前体物质.尽管已知冷适应的甲烷古菌在低温湿地的甲烷排放中发挥重要作用,但目前获得培养的嗜冷甲烷古菌却很少.冷响应的组学研究显示甲烷古菌的冷适应涉及到全局性生物学过程.     

增温对冻土区泥炭沼泽土壤孔隙水甲烷关联微生物和溶解性有机碳的影响

多年冻土区泥炭沼泽土壤孔隙水甲烷关联微生物及底物的研究有助于深入理解气候变化背景下寒区湿地生态系统甲烷循环过程。选取大兴安岭连续多年冻土区柴桦-泥炭藓和狭叶杜香-泥炭藓两种典型植被群落泥炭沼泽,设置开顶箱(Open Top Chamber,OTC)增温实验。于生长季(6月、7月、8月和9月)采集土壤孔隙水样品,对比分析OTC内外土壤孔隙水中产甲烷菌数量、甲烷氧化菌数量及溶解性有机碳(Dissolved Organic Carbon,DOC)浓度的动态变化特征,并探究土壤孔隙水甲烷关联微生物与DOC浓度的关系。结果表明:增温提高了生长季大兴安岭多年冻土区土壤孔隙水中产甲烷菌数量和DOC浓度,而对甲烷氧化菌数量的影响因月份而异。生长季柴桦-泥炭藓和狭叶杜香-泥炭藓泥炭沼泽土壤孔隙水中产甲烷菌数量的平均增加幅度分别为54.52%和44.97%,DOC浓度的平均增加幅度分别为34.16%和28.33%。增温使得生长季柴桦-泥炭藓和狭叶杜香-泥炭藓泥炭沼泽土壤孔隙水中甲烷氧化菌平均数量分别降低了46.20%和31.42%。一元线性回归分析结果表明,土壤孔隙水中DOC浓度可分别解释柴桦-泥炭藓和狭叶杜香-泥炭藓泥炭沼泽土壤孔隙水中产甲烷菌数量变化的29.00%和24.10%(P<0.01),而对两种植被群落下土壤孔隙水中甲烷氧化菌数量的影响并不显著(P>0.05)。     

长期不同施肥下水稻土甲烷氧化能力及甲烷氧化菌多样性的变化

稻田内源甲烷的氧化是稻田甲烷减排的重要途径。而甲烷氧化菌是土壤中甲烷氧化的主要施动者,在长期不同施肥条件下,土壤微生物群落的演变是否影响到土壤甲烷氧化菌群落结构及其活性,进而影响到田土壤CH4向大气的实际排放强度还不清楚。为此,选择太湖地区一个长期肥料试验的稻田土壤为研究对象,分析长期不同肥料施用对土壤甲烷氧化能力的影响及其与土壤中甲烷氧化菌群落结构变化的可能关系。结果表明,长期不同的施肥措施下稻田土壤对甲烷的氧化能力产生了明显差异,伴随着土壤中甲烷氧化菌（MOBI和MOBII）的基因群落多样性的显著变化。长期单一施用氮肥为主的化肥显著降低了土壤对甲烷的氧化能力,同时显著降低了稻田土壤甲烷氧化菌的多样性和丰富度;不同施肥下甲烷氧化菌多样性的变化与土壤的甲烷氧化能力的变化趋势相一致。因此,研究显示长期不同施肥处理下甲烷氧化菌群落结构的改变可能是引起水稻土甲烷氧化能力变化的一个主要因素,有机无机配合施用可以明显降低稻田土壤甲烷的大气释放潜能。但长期不同施肥处理下甲烷氧化菌活性的变化还有待于进一步研究。     

土壤大气甲烷氧化菌研究进展

土壤微生物催化是大气中痕量甲烷(约1.8ppmv)氧化的唯一生物途径。目前的研究表明好氧土壤中存在专性和选择性大气甲烷氧化菌2种类型:前者(USCα和USCγ)广泛分布于各种好氧旱地土壤,其甲烷氧化酶对低浓度甲烷亲和力极高,属真正的寡营养型,但至今尚未获得该种类的纯培养菌株。后者属于传统甲烷氧化菌Methylocystis/Methylosinus属,广泛分布于各种周期性排放高浓度甲烷的土壤环境中。该属大部分菌株含有亲和力不同的2套甲烷单加氧酶系统,其中的高亲和力甲烷单加氧酶使这些菌株可以在相当长的时间内(3个月)保持大气浓度甲烷氧化活性,但其生长和繁殖还需依赖于土壤内部阶段性产生的高浓度甲烷。本文详细阐述了2类大气甲烷氧化菌的发现历程及其可能的生存策略,最后系统梳理了几种关键的环境因子(土壤温度及湿度、土壤pH、植被、土地利用及氮输入)对大气甲烷氧化菌群落结构和甲烷氧化活性的影响,提出并展望了土壤大气甲烷氧化菌研究的重要方向。     

互花米草入侵对滩涂湿地甲烷排放的影响

在浙江省台州市附近滩涂湿地设置3个不同互花米草入侵密度梯度,即仅有本土植物样地、互花米草与本土植物混生样地和互花米草单优群落样地,研究互花米草入侵对滩涂湿地CH₄排放的影响.结果表明: 3个样地CH₄排放通量为0.68～5.88 mg·m^-2·h^-1,CH₄排放通量随着互花米草入侵梯度的增加而显著升高,互花米草单优群落样地CH₄排放通量分别为本土植物样地和混生样地的8.7和2.3倍.互花米草入侵显著提高了产甲烷菌数量、产甲烷潜力、甲烷氧化菌数量、甲烷氧化潜力、植物生物量、土壤有机碳含量和土壤pH,降低了土壤全氮含量.CH₄排放通量与土壤全氮呈显著负相关,与产甲烷菌数量、产甲烷潜力、甲烷氧化菌数量、甲烷氧化潜力、植物生物量和土壤pH呈显著正相关.互花米草的入侵提高了滩涂湿地植物群落生物量和土壤pH,促进了产甲烷菌数量和产甲烷潜力,从而提高了滩涂湿地的CH₄排放.     

Effect of temperature on carbon and electron flow and on the archaeal community in methanogenic rice field soil

Temperature is an important factor controlling CH(4) production in anoxic rice soils. Soil slurries, prepared from Italian rice field soil, were incubated anaerobically in the dark at six temperatures of between 10 to 37 degrees C or in a temperature gradient block covering the same temperature range at intervals of 1 degrees C. Methane production reached quasi-steady state after 60 to 90 days. Steady-state CH(4) production rates increased with temperature, with an apparent activation energy of 61 kJ mol(-1). Steady-state partial pressures of the methanogenic precursor H(2) also increased with increasing temperature from <0.5 to 3.5 Pa, so that the Gibbs free energy change of H(2) plus CO(2)-dependent methanogenesis was kept at -20 to -25 kJ mol of CH(4)(-1) over the whole temperature range. Steady-state concentrations of the methanogenic precursor acetate, on the other hand, increased with decreasing temperature from <5 to 50 microM. Simultaneously, the relative contribution of H(2) as methanogenic precursor decreased, as determined by the conversion of radioactive bicarbonate to (14)CH(4), so that the carbon and electron flow to CH(4) was increasingly dominated by acetate, indicating that psychrotolerant homoacetogenesis was important. The relative composition of the archaeal community was determined by terminal restriction fragment length polymorphism (T-RFLP) analysis of the 16S rRNA genes (16S rDNA). T-RFLP analysis differentiated the archaeal Methanobacteriaceae, Methanomicrobiaceae, Methanosaetaceae, Methanosarcinaceae, and Rice clusters I, III, IV, V, and VI, which were all present in the rice field soil incubated at different temperatures. The 16S rRNA genes of Rice cluster I and Methanosaetaceae were the most frequent methanogenic groups. The relative abundance of Rice cluster I decreased with temperature. The substrates used by this microbial cluster, and thus its function in the microbial community, are unknown. The relative abundance of acetoclastic methanogens, on the other hand, was consistent with their physiology and the acetate concentrations observed at the different temperatures, i.e., the high-acetate-requiring Methanosarcinaceae decreased and the more modest Methanosaetaceae increased with increasing temperature. Our results demonstrate that temperature not only affected the activity but also changed the structure and the function (carbon and electron flow) of a complex methanogenic system.     

Temperature Dependence of Methane Production in Tropical Rice Soils

Although CH 4 production is sensitive to temperature, it is not clear how temperature controls CH 4 production directly versus the production of organic substrates that methanogens convert into CH 4 . Therefore, this study was done to better understand how CH 4 production in rice paddy soil responded to temperature when the process was not limited by the availability of substrates. In a laboratory-incubation study using three Indian rice soils under flooded conditions, the effect of temperature on CH 4 production was examined. CH 4 production in acid sulphate, laterite, and alluvial soil samples under flooded conditions distinctly increased with increase in temperature from 15°C to 35°C. Laterite and acid sulphate soils produced distinctly less CH 4 than alluvial soils. CO 2 production increased with increase in temperature in all the soils. The readily mineralizable carbon C and Fe 2+ contents in soils were least at 15°C and highest at 35°C, irrespective of soil type. Likewise, a significant correlation existed between microbial population (methanogens and sulphate reducers) and CH 4 production. Comparing the temperature coefficients ( Q 10 ) for methane production within each soil type at low (15°C-25°C) and medium (25°C-35°C) temperature intervals revealed that these values were not uniform for both alluvial and laterite soils. But acid sulphate soil had Q 10 values that were near 2 at both temperature intervals. When these soil samples were amended with substrates (acetate, H 2 -CO 2 , and rice straw), there were stimulatory effects on methane production rates and consequently on the Q 10 values. The pattern of temperature coefficients was characteristic of the soil type and the nature of substrates used for amendment.     

Dynamics of the methanogenic archaeal community during plant residue decomposition in an anoxic rice field soil

Incorporation of plant residues strongly enhances the methane production and emission from flooded rice fields. Temperature and residue type are important factors that regulate residue decomposition and CH(4) production. However, the response of the methanogenic archaeal community to these factors in rice field soil is not well understood. In the present experiment, the structure of the archaeal community was determined during the decomposition of rice root and straw residues in anoxic rice field soil incubated at three temperatures (15 degrees C, 30 degrees C, and 45 degrees C). More CH(4) was produced in the straw treatment than root treatment. Increasing the temperature from 15 degrees C to 45 degrees C enhanced CH(4) production. Terminal restriction fragment length polymorphism analyses in combination with cloning and sequencing of 16S rRNA genes showed that Methanosarcinaceae developed early in the incubations, whereas Methanosaetaceae became more abundant in the later stages. Methanosarcinaceae and Methanosaetaceae seemed to be better adapted at 15 degrees C and 30 degrees C, respectively, while the thermophilic Methanobacteriales and rice cluster I methanogens were significantly enhanced at 45 degrees C. Straw residues promoted the growth of Methanosarcinaceae, whereas the root residues favored Methanosaetaceae. In conclusion, our study revealed a highly dynamic structure of the methanogenic archaeal community during plant residue decomposition. The in situ concentration of acetate (and possibly of H(2)) seems to be the key factor that regulates the shift of methanogenic community.     

温度对土壤氧化大气CH4的影响

讨论了温度对土壤氧化大气CH4的影响及其机理。当温度较低时土壤也具有一定的氧化大气CH4的能力,两者具有很高的相关关系,但是由于CH4氧化菌对大气CH4具有很强的亲和力以及大气CH4氧化所需活化能较低,因此土壤氧化大气CH4对温度的敏感度远低于产CH4,导致温度系数Q10较小。当大气CH4和O2扩散进入土壤的速率等于土壤中CH4和O2消耗的速率时,大气CH4氧化达到最大值,此时的土壤温度就是CH4氧化的最佳温度。如果温度继续升高并大于最佳温度,由于CH4氧化菌无法与利用O2能力更强的硝化细菌和其它微生物竞争利用土壤空气中有限的O2,使得土壤中CH4氧化菌的繁殖和活性降低。这一作用机理的提出较好地解释了为什么随着温度升高土壤氧化大气CH4能力呈低高低的态势。     

Effect of methanogenic substrates on anaerobic oxidation of methane and sulfate reduction by an anaerobic methanotrophic enrichment

Anaerobic oxidation of methane (AOM) coupled to sulfate reduction (SR) is assumed to be a syntrophic process, in which methanotrophic archaea produce an interspecies electron carrier (IEC), which is subsequently utilized by sulfate-reducing bacteria. In this paper, six methanogenic substrates are tested as candidate-IECs by assessing their effect on AOM and SR by an anaerobic methanotrophic enrichment. The presence of acetate, formate or hydrogen enhanced SR, but did not inhibit AOM, nor did these substrates trigger methanogenesis. Carbon monoxide also enhanced SR but slightly inhibited AOM. Methanol did not enhance SR nor did it inhibit AOM, and methanethiol inhibited both SR and AOM completely. Subsequently, it was calculated at which candidate-IEC concentrations no more Gibbs free energy can be conserved from their production from methane at the applied conditions. These concentrations were at least 1,000 times lower can the final candidate-IEC concentration in the bulk liquid. Therefore, the tested candidate-IECs could not have been produced from methane during the incubations. Hence, acetate, formate, methanol, carbon monoxide, and hydrogen can be excluded as sole IEC in AOM coupled to SR. Methanethiol did inhibit AOM and can therefore not be excluded as IEC by this study.     

In vitro methanol production from methyl coenzyme M using the Methanosarcina barkeri MtaABC protein complex

Methanol:coenzyme M methyltransferase is an enzyme complex composed of three subunits, MtaA, MtaB, and MtaC, found in methanogenic archaea and is needed for their growth on methanol ultimately producing methane. MtaABC catalyzes the energetically favorable methyl transfer from methanol to coenzyme M to form methyl coenzyme M. Here we demonstrate that this important reaction for possible production of methanol from the anaerobic oxidation of methane can be reversed in vitro. To this effect, we have expressed and purified the Methanosarcina barkeri MtaABC enzyme, and developed an in vitro functional assay that demonstrates MtaABC can catalyze the energetically unfavorable (ΔG° = 27 kJ/mol) reverse reaction starting from methyl coenzyme M and generating methanol as a product. Demonstration of an in vitro ability of MtaABC to produce methanol may ultimately enable the anaerobic oxidation of methane to produce methanol and from methanol alternative fuel or fuel‐precursor molecules. © 2017 American Institute of Chemical Engineers Biotechnol. Prog., 33:1243–1249, 2017     

植物在CH4产生、氧化和排放中的作用

综合评述了植物对CH4产生、内源CH4氧化和CH4排放的影响．不同植物释放根系分泌物能力的不同是造成CH4产生量差异的主要原因。而植物不同生育期分泌分泌物能力的差异是造成季节性变化的关键．植物泌O2能力的高低和季节性变化通过影响内源CH4的氧化来改变CH4的排放数量．植物问通气组织数量和密度的差异及其随生育期的变化,通过影响对CH4的传输能力来改变CH4的排放量．因此,植物排放CH4的通量及其季节性变化规律是由植物根系分泌分泌物能力、分泌O2能力和传输CH4能力综合决定的．     

水稻土中CH4氧化的研究

在实验室条件下研究了水稻土中CH₄氧化的特性.结果表明,在早稻种植前采集的水稻土不能氧化大气中的CH₄,但当所供给的CH₄浓度>10μl·L^-1时,能迅速氧化CH₄,所供给的CH₄浓度越高,氧化CH₄的速度越大.经高浓度(>1000μl·L^-1)的CH₄预培养10d,可使本来不具有氧化大气CH₄能力的土壤氧化大气CH_4.大田CH₄排放通量高的水稻土,氧化CH₄的能力较大.     

Methane formation and methane oxidation by methanogenic bacteria.

Methanogenic bacteria were found to form and oxidize methane at the same time. As compared to the quantity of methane formed, the amount of methane simultaneously oxidized varied between 0.3 and 0.001%, depending on the strain used. All the nine tested strains of methane producers (Methanobacterium ruminantium, Methanobacterium strain M.o.H., M. formicicum, M. thermoautotrophicum, M. arbophilicum, Methanobacterium strain AZ, Methanosarcina barkeri, Methanospirillum hungatii, and the "acetate organism") reoxidized methane to carbon dioxide. In addition, they assimilated a small part of the methane supplied into cell material. Methanol and acetate also occurred as oxidation products in M. barkeri cultures. Acetate was also formed by the "acetate organism," a methane bacterium unable to use methanogenic substrates other than acetate. Methane was the precursor of the methyl group of the acetate synthesized in the course of methane oxidation. Methane formation and its oxidation were inhibited equally by 2-bromoethanesulfonic acid. Short-term labeling experiments with M. thermoautotrophicum and M. hungatii clearly suggest that the pathway of methane oxidation is not identical with a simple back reaction of the methane formation process.     

Studies on an acetate-fermenting strain of Methanosarcina.

An acetate-fermenting strain of Methanosarcina was isolated from an acetate enrichment culture inoculated with anaerobic sludge from a waste treatment digestor. In pure culture, this organism fermented acetate in the absence of added hydrogen at rates comparable in magnitude to those found in digestor systems. This rate was significantly higher than previously obtained for pure cultures of this genus. Mineral components of yeast extract were highly stimulatory for cultures growing on methanol. Comparable stimulation was not observed for cultures growing on acetate. Labeling studies indicated that acetate was converted to methane and CO2 as predicted by previous studies on mixed cultures. Total oxidation or reduction of acetate was not the mechanism of conversion of acetate to methane by the pure culture. The ability of this strain to form colonies or to produce methane from acetate was apparently influenced by the choice of substrate and conditions used for growing the inoculum.