Bacterial metabolism in small temperate streams under contemporary and future climates

1. We examined the detailed temperature dependence (0–40 °C) of bacterial metabolism associated with fine sediment particles from three Danish lowland streams to test if temperature dependence varied between sites, seasons and quality of organic matter and to evaluate possible consequences of global warming. 2. A modified Arrhenius model with reversible denaturation at high temperatures could account for the temperature dependence of bacterial metabolism and the beginning of saturation above 35 °C and it was superior to the unmodified Arrhenius model. Both models overestimated respiration rates at very low temperatures (<5 °C), whereas Ratkowsky's model – the square root of respiration – provided an excellent linear fit between 0 and 30 °C. 3. There were no indications of differences in temperature dependence among samples dominated by slowly or easily degradable organic substrates. Optimum temperature, apparent minimum temperature, Q₁₀‐values for 0–40 °C and activation energies of bacterial respiration were independent of season, stream site and degradability of organic matter. 4. Q₁₀‐values of bacterial respiration declined significantly with temperature (e.g. 3.31 for 5–15 °C and 1.43 for 25–35 °C) and were independent of site and season. Q₁₀‐values of bacterial production behaved similarly, but were significantly lower than Q₁₀‐values of respiration implying that bacterial growth efficiency declined with temperature. 5. A regional warming scenario for 2071–2100 (IPCC A2) predicted that mean annual temperatures will increase by 3.5 °C in the air and 2.2–4.3 °C in the streams compared with the control scenario for 1961–1990. Temperature is expected to rise more in cool groundwater‐fed forest springs than in open, summer‐warm streams. Mean annual bacterial respiration is estimated to increase by 26–63% and production by 18–41% among streams assuming that established metabolism–temperature relationships and organic substrate availability remain the same. To improve predictions of future ecosystem behaviour, we further require coupled models of temperature, hydrology, organic production and decomposition.     

Soil respiration in a Mediterranean oak forest at different developmental stages after coppicing

To assess the variation of soil respiration at different forest stages we measured it in a coppiced oak (Quercus cerris L.) chronosequence in central Italy during two campaigns, spanning 2 successive years, in four stands at different stages of the rotation: 1 year (S1), 5 years (S5), 10 years (S10) and 17 years (S17) after coppicing. The contribution of the different components of soil respiration flux (aboveground litter, belowground decomposition soil organic matter and root respiration) was estimated by a paired comparison of manipulative experiments between the recently coppiced stand (S1) and mature stand (S17). Ninety percent of soil respiration values were between 1.7 and 7.8 μmol m^?2 s^?1, with an overall mean (±SD) of 4.0±2.7 μmol m^?2 s^?1. Spatial variation of soil respiration was high (CV=44.9%), with a mean range (i.e. patch size) of 4.8±2.7 m, as estimated from a semivariance analysis. In the absence of limitation by soil moisture, soil respiration was related to soil temperature with the exponential Q₁₀ model (average Q₁₀=2.25). During summer, soil moisture constrained soil respiration and masked its dependence on soil temperature. Soil respiration declined over the years after coppicing. Assuming a linear decline with stand age, we estimated a reduction of 24% over a 20‐year‐rotation cycle. The response of soil respiration to temperature also changed with age of the stands: the Q₁₀ was estimated to decrease from 2.90 in S1 to 2.42 in S17, suggesting that different components or processes may be involved at different developmental stages. The contribution of heterotrophic respiration to total soil respiration flux was relatively larger in the young S1 stand than in the mature S17 stand.     

土壤细菌呼吸对西双版纳热带森林恢复的响应

揭示不同恢复阶段热带森林土壤细菌呼吸季节变化及其主控因素,对于探明土壤细菌呼吸对热带森林恢复的响应机制具有重要的科学意义。以西双版纳不同恢复阶段热带森林(白背桐群落、崖豆藤群落和高檐蒲桃群落)为研究对象,运用真菌呼吸抑制法及高通量宏基因组测序技术分别测定土壤细菌呼吸速率和细菌多样性,并采用回归分析及结构方程模型揭示热带森林恢复过程中土壤细菌多样性、pH、土壤碳氮组分变化对土壤细菌呼吸速率的影响特征。结果表明：1)不同恢复阶段热带森林土壤细菌呼吸速率表现为：高檐蒲桃群落((1.51±0.62)CO₂ mg g^-1 h^-1)显著高于崖豆藤群落((1.16±0.56)CO₂ mg g^-1 h^-1)和白背桐群落((0.82±0.60)CO₂ mg g^-1 h^-1)(P<0.05)。2)不同恢复阶段土壤细菌呼吸速率呈显著的单峰型季节变化(P<0.05),最大值均出现在9月：高檐蒲桃群落((...     

Temperature effect on maintenance and growth respiration coefficients of young, field-grown hinoki cypress (Chamaecyparis obtusa)

Respiration measurements were made on the entire aboveground parts of young, field-grown hinoki cypress (Chamaecyparis obtusa) trees at monthly intervals over a 5-year period, to examine the effect of temperature on maintenance and growth respiration coefficients. The respiration rate of the trees was grouped on a monthly basis and then partitioned into maintenance and growth components. The maintenance respiration coefficient increased exponentially with air temperature. The maintenance respiration coefficient at a temperature of 0°C and itsQ ₁₀ value were 0.205 mmol CO₂ g⁻¹ d.w. month⁻¹ and 1.81, respectively. The growth respiration coefficient, which was virtually independent of temperature, had a mean value of 38.06±1.95 (SE) mmol CO₂g⁻¹ d.w. The growth rate increased exponentially with increasing temperature up to a peak at around 18°C, and thereafter declined, thereby resulting in the growth respiration rate being increasingly less sensitive to increasing air temperature. The reported decreases in theQ ₁₀ value of total respiration with increasing air temperature is due to the way in which the growth component of respiration responds to temperature.     

施肥对油茶园土壤呼吸和异养呼吸及其温度敏感性的影响

油茶是中国南方重要的木本食用油料树种,研究施肥对油茶园土壤呼吸及其温度敏感性的影响,对于估算中国南方典型种植园林温室气体排放及其对气候变化的响应具有重要意义。设置对照(CK)、施肥(OF)、断根(CK-T)和断根施肥(OF-T)4个处理,采用静态箱-气相色谱法,通过多年观测,分析探讨施肥对油茶园土壤呼吸和异养呼吸及其温度敏感性的影响。结果表明:(1)施肥对油茶园土壤呼吸和异养呼吸无显著影响。研究期间,各处理(OF、CK、OF-T、CK-T)土壤CO_2通量依次为(77.91±2.59)、(73.71±0.97)、(66.82±1.02)mg C m~(-2)h~(-1)和(66.84±3.94)mg C m~(-2)h~(-1);(2)各处理土壤呼吸温度敏感性(Q_(10))表现为OF-T(1.96±0.01)CK-T(1.79±0.03)OF(1.77±0.01)CK(1.75±0.03),其中,OF-T处理下Q_(10)显著高于其他3个处理,即施肥显著增加了断根处理土壤呼吸Q_(10);(3)施肥显著增加了土壤表层NH_4~+-N和NO_3~--N含量,Q_(10)与土壤表层NH_4~+-N和NO_3~--N含量表现出显著的正相关关系。     

A paired study of prairie carbon stocks, fluxes, and phenology: comparing the world's oldest prairie restoration with an adjacent remnant

We measured carbon (C) stocks and fluxes and vegetation phenology in the world's oldest prairie restoration (∼65 years) and an adjacent prairie remnant in southern Wisconsin from 2001–2004 to quantify structural and functional differences. While the species distributions and frequency differed, the number of species measured per 1 m² quadrat were not significantly different (15.8±4.4 and 14.1±2.1 for remnant and planted [order for all reported values in abstract]; P=0.29), and the annual average aboveground net primary productivity (271±51 and 330±55 g C m⁻²) and peak leaf area index (2.9–4.9 m² m⁻²) were comparable under similar fire management. Total root biomass was not significantly different in 2002 (1736±1062 and 1690±459 g dry matter m⁻²) or 2003 (3029±2081 and 2146±898 g m⁻²), but annual average soil respiration (1229±77 and 1428±24 g C m⁻² yr⁻¹) was significantly higher in the restoration (P<0.0001). However, the prairie remnant contained 37% greater soil C (P<0.0001) in the top 25 cm. Soil respiration response to 10 cm soil temperature (Q₁₀) varied with respect to prairie and soil moisture conditions as annual Q₁₀ values ranged from 2.5 to 3.6. We calculated a range of net ecosystem production (NEP) values using estimated heterotrophic respiration and three root turnover values. Average NEP varied from −1.4 to 1.9 and −2.3 to 1.3 Mg C ha⁻¹ yr⁻¹ for the remnant and planted prairies, respectively. While these two prairies share similar structural components and functional attributes, the large uncertainty in NEP casts doubt as to whether we can verify these prairies as C sources or sinks without direct measures of heterotrophic respiration and root turnover. We argue that quantitative studies of C exchange in prairies, which differ in restoration methodology, management intensity, and fire frequency, are needed to solidify the relationship between prairie structure and potentially desired functions such as C sequestration.     

Large seasonal changes in Q10 of soil respiration in a beech forest

We analyzed one year of continuous soil respiration measurements to assess variations in the temperature sensitivity of soil respiration at a Danish beech forest. A single temperature function derived from all measurements across the year (Q₁₀ = 4.2) was adequate for estimating the total annual soil respiration and its seasonal evolution. However, Q₁₀'s derived from weekly datasets ranged between three in summer (at a mean soil temperature of 14 °C) and 23 in winter (at 2 °C), indicating that the annual temperature function underestimated the synoptic variations in soil respiration during winter. These results highlight that empirical models should be parameterized at a time resolution similar to that required by the output of the model. If the objective of the model is to simulate the total annual soil respiration rate, annual parameterization suffices. If however, soil respiration needs to be simulated over time periods from days to weeks, as is the case when soil respiration is compared to total ecosystem respiration during synoptic weather patterns, more short‐term parameterization is required. Despite the higher wintertime Q₁₀'s, the absolute response of soil respiration to temperature was smaller in winter than in summer. This is mainly because in absolute numbers, the temperature sensitivity of soil respiration depends not only on Q₁₀, but also on the rate of soil respiration, which is highly reduced in winter. Nonetheless, the Q₁₀ of soil respiration in winter was larger than can be explained by the decreasing respiration rate only. Because the seasonal changes in Q₁₀ were negatively correlated with temperature and positively correlated with soil moisture, they could also be related to changing temperature and/or soil moisture conditions.     

Variability in temperature regulation of CO2 fluxes and N mineralization from five Hawaiian soils: implications for a changing climate

We examined the possibility that microbial adaptation to temperature could affect rates of CO₂, N₂O and CH₄ release from soils. Laboratory incubations were used to determine the functional relationship between temperature and CO₂, N₂O and CH₄ fluxes for five soils collected across an elevational range in Hawaii. Initial rates of CO2 production and net N mineralization increased exponentially from 15 °C to 55 °C; initial rates of CH₄ and N₂O release were more complex. No optimum temperature (in which rates decline at higher and lower temperatures) was apparent for any of the gases, but respiration declined with time at higher temperatures, suggesting rapid depletion of readily available substrate. Mean Q₁₀S for respiration varied from 1.4 to 2.0, a typical range for tropical soils. The functional relationship between CO₂ production and temperature was consistent among all five soils, despite the substantial differences in mean annual temperature, soils, and land-use among the sites. Temperature responses of N₂O and CH₄ fluxes did not follow simple Q₁₀ relationships suggesting that temperature functions developed for CO₂ release from heterotrophic respiration cannot be simply extrapolated. Expanding this study to tropical heterotrophic respiration, the flux is more sensitive to changes in Q₁₀ than to changes in temperature on a per unit basis: the partial derivative with respect to temperature is 2.4 Gt C ·° C^?1 with respect to Q₁₀, it is 3.5 Gt C · Q₁₀ unit^?1. Therefore, what appears to be minor variability might still produce substantial uncertainty in regional estimates of gas exchange.     

Temperature sensitivity of biomass‐specific microbial exo‐enzyme activities and CO2 efflux is resistant to change across short‐ and long‐term timescales

Accurate representation of temperature sensitivity (Q₁₀) of soil microbial activity across time is critical for projecting soil CO₂ efflux. As microorganisms mediate soil carbon (C) loss via exo‐enzyme activity and respiration, we explore temperature sensitivities of microbial exo‐enzyme activity and respiratory CO₂ loss across time and assess mechanisms associated with these potential changes in microbial temperature responses. We collected soils along a latitudinal boreal forest transect with different temperature regimes (long‐term timescale) and exposed these soils to laboratory temperature manipulations at 5, 15, and 25°C for 84 days (short‐term timescale). We quantified temperature sensitivity of microbial activity per g soil and per g microbial biomass at days 9, 34, 55, and 84, and determined bacterial and fungal community structure before the incubation and at days 9 and 84. All biomass‐specific rates exhibited temperature sensitivities resistant to change across short‐ and long‐term timescales (mean Q₁₀ = 2.77 ± 0.25, 2.63 ± 0.26, 1.78 ± 0.26, 2.27 ± 0.25, 3.28 ± 0.44, 2.89 ± 0.55 for β‐glucosidase, N‐acetyl‐β‐d ‐glucosaminidase, leucine amino peptidase, acid phosphatase, cellobiohydrolase, and CO₂ efflux, respectively). In contrast, temperature sensitivity of soil mass‐specific rates exhibited either resilience (the Q₁₀ value changed and returned to the original value over time) or resistance to change. Regardless of the microbial flux responses, bacterial and fungal community structure was susceptible to change with temperature, significantly differing with short‐ and long‐term exposure to different temperature regimes. Our results highlight that temperature responses of microbial resource allocation to exo‐enzyme production and associated respiratory CO₂ loss per unit biomass can remain invariant across time, and thus, that vulnerability of soil organic C stocks to rising temperatures may persist in the long term. Furthermore, resistant temperature sensitivities of biomass‐specific rates in spite of different community structures imply decoupling of community constituents and the temperature responses of soil microbial activities.     

Sorption of humic acids by bacteria

Capacity for sorption of humic acid (HA) from water solutions was shown for 38 bacterial strains. Isotherms of HA sorption were determined for the cells of 10 strains. The bonding strength between the cells and HA (k) and the terminal adsorption (Q _max) determined from the Langmuir equation for gram-positive and gram-negative bacteria were reliably different. Gram-positive bacteria sorbed greater amounts of HA than gram-negative ones (Q _max = 23 ± 10 and 5.6 ± 1.2 mg/m², respectively). The bonding strength between HA and the cells was higher in gram-negative bacteria than in gram-positive: k = 9 ± 5 and 3.3 ± 1.1 mL/mg, respectively.     

Nitrogen addition reduces soil respiration in a mature tropical forest in southern China

Response of soil respiration (CO₂ emission) to simulated nitrogen (N) deposition in a mature tropical forest in southern China was studied from October 2005 to September 2006. The objective was to test the hypothesis that N addition would reduce soil respiration in N saturated tropical forests. Static chamber and gas chromatography techniques were used to quantify the soil respiration, following four‐levels of N treatments (Control, no N addition; Low‐N, 5 g N m^?2 yr^?1; Medium‐N, 10 g N m^?2 yr^?1; and High‐N, 15 g N m^?2 yr^?1 experimental inputs), which had been applied for 26 months before and continued throughout the respiration measurement period. Results showed that soil respiration exhibited a strong seasonal pattern, with the highest rates found in the warm and wet growing season (April–September) and the lowest rates in the dry dormant season (December–February). Soil respiration rates showed a significant positive exponential relationship with soil temperature, whereas soil moisture only affect soil respiration at dry conditions in the dormant season. Annual accumulative soil respiration was 601±30 g CO₂‐C m^?2 yr^?1 in the Controls. Annual mean soil respiration rate in the Control, Low‐N and Medium‐N treatments (69±3, 72±3 and 63±1 mg CO₂‐C m^?2 h^?1, respectively) did not differ significantly, whereas it was 14% lower in the High‐N treatment (58±3 mg CO₂‐C m^?2 h^?1) compared with the Control treatment, also the temperature sensitivity of respiration, Q₁₀ was reduced from 2.6 in the Control with 2.2 in the High‐N treatment. The decrease in soil respiration occurred in the warm and wet growing season and were correlated with a decrease in soil microbial activities and in fine root biomass in the N‐treated plots. Our results suggest that response of soil respiration to atmospheric N deposition in tropical forests is a decline, but it may vary depending on the rate of N deposition.     

Thermal sensitivity of mitochondrial function in the Antarctic Notothenioid Lepidonotothen nudifrons

The thermal sensitivity of mitochondrial function was investigated in the stenothermal Antarctic fish Lepidonotothen nudifrons. State 3 respiration increases with increasing temperature between 0 °C and 18 °C with a Q ₁₀ of 2.43–2.63. State 4 respiration in the presence of oligomycin, an inhibitor of mitochondrial ATP synthase, quantifies the leakage of protons through the inner mitochondrial membrane, which causes oxygen consumption without concomitant ATP production. This parameter shows an unusually high Q ₁₀ of 4.21 ± 0.42 (0–18 °C), which indicates that proton leakage does not depend merely on ion diffusion but is an enzyme-catalysed process. The differential thermal sensitivity of oxidative phosphorylation (=state 3) and proton leakage (=state 4 in the presence of oligomycin) leads to progressive uncoupling of the mitochondria and decreased efficiency of oxidative phosphorylation under in vivo conditions if the body temperature of L. nudifrons increases. Accepted: 2 September 1999     

Improved in vivo measurement of alternative oxidase respiration in field‐collected pine roots

Cellular respiration via the alternative oxidase pathway (AOP) leads to a considerable loss in efficiency. Compared to the cytochrome pathway (COP), AOP produces 0–50% as much ATP per carbon (C) respired. Relative partitioning between the pathways can be measured in vivo based on their differing isotopic discriminations against ¹⁸O in O₂. Starting from published methods, we have refined and tested a new protocol to improve measurement precision and efficiency. The refinements detect an effect of tissue water content (P < 0.0001), which we have removed, and yield precise discrimination endpoints in the presence of pathway‐specific respiratory inhibitors [CN^? and salicylhydroxamic acid (SHAM)], which improves estimates of AOP/COP partitioning. Fresh roots of Pinus sylvestris were sealed in vials with a CO₂ trap. The air was replaced to ensure identical starting conditions. Headspace air was repeatedly sampled and isotopically analyzed using isotope‐ratio mass spectrometry. The method allows high‐precision measurement of the discrimination against ¹⁸O in O₂ because of repeated measurements of the same incubation vial. COP and AOP respiration discriminated against ¹⁸O by 15.1 ± 0.3‰ and 23.8 ± 0.4‰, respectively. AOP contributed to root respiration by 23 ± 0.2% of the total in an unfertilized stand. In a second, nitrogen‐fertilized, stand AOP contribution was only 14 ± 0.2% of the total. These results suggest the improved method can be used to assess the relative importance of COP and AOP activities in ecosystems, potentially yielding information on the role of each pathway for the carbon use efficiency of organisms.     

川中丘陵区冬水田种植模式转旱作土壤呼吸组分特征及碳平衡

冬水田-水稻是川中丘陵区传统的稻田种植模式,冬水田种植模式转变是实现多熟种植及机械化的重要途径。为探究冬水田-水稻种植模式转旱作过程中作物季及休闲期土壤呼吸速率及其组分构成,试验设置冬水田-水稻转旱作(FTD)、冬水田-水稻(FR)和冬闲田-玉米(FM)3种不同种植模式,采用根排除法和静态明箱-气相色谱法原位取样测定作物季及季后休闲期土壤呼吸及其组分,并通过测算净生态系统生产力(NEP)进而判断冬水田-水稻转旱作过程的农田系统碳汇强度。结果表明:(1)FTD显著提高了土壤总呼吸速率及其自养和异养呼吸速率,从而提高了其累积排放量(P<0.05)。与FR相比,FTD的土壤总呼吸及其自养和异养呼吸的累积排放量分别提高了13.14倍、11.32倍和15.56倍(P<0.05);与FM相比,FTD的土壤总呼吸及其自养和异养呼吸的累积排放量分别提高了70.56%、40.83%和115.47%(P<0.05)。(2)与FR和FM相比,FTD均降低了土壤呼吸及其组分的温度敏感性(Q₁₀),且土壤总呼吸的温度敏感性介于异养呼吸和自养呼吸之间。(3)FR,FM和FTD的净生态系统生产力(NEP)均为正值,其数值分别为7911.66 kg/hm²,5667.89 kg/hm²和1583.46 kg/hm²,均表现为大气CO₂的碳汇,但与FR与FM相比,FTD显著降低了其净生态系统生产力,呈现出较弱的碳汇。     

Respiration and glycolysis in the human diploid cell strain WI-38

Assessment of the respiratory and glycolytic capacity of non-growing WI-38 cells shows that, in the absence and presence of added glucose, the mean rates of oxygen consumption were 247 (QO₂ = 5.61) and 208 (QO₂ = 4.73) mμmoles/mg dry wt/hr., respectively. Mean glucose consumption was 225 mμmoles/mg dry wt/ hr. With uniformly labeled ¹⁴C glucose as substrate, 36 mμg atoms of carbon dioxide were produced, corresponding to 15–20% of the total cellular respiration. Mean values for lactate production in the presence and absence of glucose were 345 (Q_L^O2 = 7.85) and 196 (Q_L^O2 = 4.45) mμmoles/mg dry wt/hr., respectively. Human diploid cells in culture age, in the sense that their ability to proliferate decreases with time during serial subcultivation. Studies of their respiratory and glycolytic capacity as a function of the aging process showed that total respiration, glucose respiration and glycolytic capacity were relatively constant for cells in the middle and late passages and indicate that aging in this sense is not directly related to the respiratory and glycolytic capacity of the cell.     

Regulation of root respiration in two species of Plantago that differ in relative growth rate: the effect of short- and long-term changes in temperature

This study investigates the effect of short‐ and long‐term changesin temperature on the regulation of root respiratory O₂ uptakeby substrate supply, adenylate restriction and/or the capacityof the respiratory system. The species investigated were the lowland Plantagolanceolata L. and alpine Plantago euryphylla Briggs, Carolin& Pulley, which are inherently fast‐ and slow‐growing, respectively. Theplants were grown hydroponically in a controlled environment (constant23 °C). The effect of long‐term exposure to lowtemperature on regulation of respiration was also assessed in P.lanceolata using plants transferred to 15/10 °C(day/night) for 7 d. Exogenous glucose and uncoupler (CCCP)were used to assess the extent to which respiration rates were limitedby substrate supply and adenylates. The results suggest that adenylatesand/or substrate supply exert the greatest control overrespiration at moderate temperatures (e.g. 15–30 °C)in both species. At low temperatures (5–15 °C),CCCP and glucose had little effect on respiration, suggesting thatrespiration was limited by enzyme capacity alone. The Q₁₀ (proportionalincrease of respiration per 10 °C) of respirationwas increased following the addition of CCCP and/or exogenousglucose. The degree of stimulation by CCCP was considerably lowerin P. euryphylla than P. lanceolata. This suggeststhat respiration rates operate much closer to the maximum capacity in P.euryphylla than P. lanceolata. When P. lanceolata wastransferred to 15 °C for 7 d, respirationacclimated to the lower growth temperature (as demonstrated by an increasein respiration rates measured at 25 °C). In addition,the Q₁₀ was higher, and the stimulatory effectof exogenous glucose and CCCP lower, in the cold‐acclimated rootsin comparison with their warm‐grown counterparts. Acclimation of P.lanceolata to different day/night‐time temperatureregimes was also investigated. The low night‐time temperature wasfound to be the most important factor influencing acclimation. The Q₁₀ valueswere also higher in plants exposed to the lowest night‐time temperature.The results demonstrate that short‐ and long‐term changes in temperaturealter the importance of substrate supply, adenylates and capacityof respiratory enzymes in regulating respiratory flux.     

Foliar respiration acclimation to temperature and temperature variable Q10 alter ecosystem carbon balance

The response of respiration to temperature in plants can be considered at both short‐ and long‐term temporal scales. Short‐term temperature responses are not well described by a constant Q₁₀ of respiration, and longer‐term responses often include acclimation. Despite this, many carbon balance models use a static Q₁₀ of respiration to describe the short‐term temperature response and ignore temperature acclimation. We replaced static respiration parameters in the ecosystem model photosynthesis and evapo‐transpiration (PnET) with a temperature‐driven basal respiration algorithm (Rd_acclim) that accounts for temperature acclimation, and a temperature‐variable Q₁₀ algorithm (Q_10var). We ran PnET with the new algorithms individually and in combination for 5 years across a range of sites and vegetation types in order to examine the new algorithms' effects on modeled rates of mass‐ and area‐based foliar dark respiration, above ground net primary production (ANPP), and foliar respiration–photosynthesis ratios. The Rd_acclim algorithm adjusted dark respiration downwards at temperatures above 18°C, and adjusted rates up at temperatures below 5°C. The Q_10var algorithm adjusted dark respiration down at temperatures below 15°C. Using both algorithms simultaneously resulted in decreases in predicted annual foliar respiration that ranged from 31% at a tall‐grass prairie site to 41% at a boreal coniferous site. The use of the Rd_acclim and Q_10var algorithms resulted in increases in predicted ANPP ranging from 18% at the tall‐grass prairie site to 38% at a warm temperate hardwood forest site. The new foliar respiration algorithms resulted in substantial and variable effects on PnETs predicted estimates of C exchange and production in plants and ecosystems. Current models that use static parameters may over‐predict respiration and subsequently under‐predict and/or inappropriately allocate productivity estimates. Incorporating acclimation of basal respiration and temperature‐sensitive Q₁₀ have the potential to enhance the application of ecosystem models across broad spatial scales, or in climate change scenarios, where large temperature ranges may cause static respiration parameters to yield misleading results.     

全球陆地生态系统光合作用与呼吸作用的温度敏感性

基于全球647套通量数据,定量分析了全球尺度下生态系统光合作用和呼吸作用的温度敏感性(Q10)随纬度、气候和植被的分布规律。结果表明:在全球尺度下,光合作用和呼吸过程的温度敏感性(Q10,G和Q10,R)都随纬度的升高而增加,其中Q10,G和Q10,R的均值分别为3.99±0.21和2.28±0.074。除热带多树草原、常绿落叶林外,Q10,G均大于Q10,R值。不同植被类型的温度敏感性存在显著性差异,表现为:针叶林阔叶林;落叶林常绿林,其中生态系统的季节性变异是造成差异的主要原因。当植被类型和纬度区域共同影响Q10值时,植被类型对Q10值的总变异贡献更大。气候类型对Q10,G和Q10,R都有显著影响。在气候带上,干旱带的Q10,G最小,而冷温带的Q10,G最高。不同气候类型下(除温带草原气候外)的Q10,G都大于Q10,R。在极端条件下,温度可能不在是主导因素,而水分对温度敏感性的影响不可忽略,今后的研究需要更多的关注生态系统温度敏感性对水分变化的响应。     

Acclimation to temperature and temperature sensitivity of metabolism by ectomycorrhizal fungi

Ectomycorrhizal (ECM) fungi contribute significantly to ecosystem respiration, but little research has addressed the effect of temperature on ECM fungal respiration. Some plants have the ability to acclimate to temperature such that long‐term exposure to warmer conditions slows respiration at a given measurement temperature and long‐term exposure to cooler conditions increases respiration at a given measurement temperature. We examined acclimation to temperature and temperature sensitivity (Q₁₀) of respiration by ECM fungi by incubating them for a week at one of three temperatures and measuring respiration over a range of temperatures. Among the 12 ECM fungal isolates that were tested, Suillus intermedius, Cenococcum geophilum, and Lactarius cf. pubescens exhibited significant acclimation to temperature, exhibiting an average reduction in respiration of 20–45% when incubated at 23 °C compared with when incubated at 11 or 17 °C. The isolates differed significantly in their Q₁₀ values, which ranged from 1.67 to 2.56. We also found that half of the isolates significantly increased Q₁₀ with an increase in incubator temperature by an average of 15%. We conclude that substantial variation exists among ECM fungal isolates in their ability to acclimate to temperature and in their sensitivity to temperature. As soil temperatures increase, ECM fungi that acclimate may require less carbon from their host plants than fungi that do not acclimate. The ability of some ECM fungi to acclimate may partially ameliorate the anticipated positive feedback between soil respiration and temperature.     

Modeling soil CO<Subscript>2</Subscript> emissions from ecosystems

We present a new soil respiration model, describe a formal model testing procedure, and compare our model with five alternative models using an extensive data set of observed soil respiration. Gas flux data from rangeland soils that included a large number of measurements at low temperatures were used to model soil CO₂ emissions as a function of soil temperature and water content. Our arctangent temperature function predicts that Q₁₀ values vary inversely with temperature and that CO₂ fluxes are significant below 0 °C. Independent data representing a broad range of ecosystems and temperature values were used for model testing. The effects of plant phenology, differences in substrate availability among sites, and water limitation were accounted for so that the temperature equations could be fairly evaluated. Four of the six tested models did equally well at simulating the observed soil CO₂ respiration rates. However, the arctangent variable Q₁₀ model agreed closely with observed Q₁₀ values over a wide range of temperatures (r² = 0.94) and was superior to published variable Q₁₀ equations using the Akaike information criterion (AIC). The arctangent temperature equation explained 16–85% of the observed intra-site variability in CO₂ flux rates. Including a water stress factor yielded a stronger correlation than temperature alone only in the dryland soils. The observed change in Q₁₀ with increasing temperature was the same for data sets that included only heterotrophic respiration and data sets that included both heterotrophic and autotrophic respiration.