Indirect partitioning of soil respiration in a series of evergreen forest ecosystems

A simple estimation of heterotrophic respiration can be obtained analytically as the y-intercept of the linear regression between soil-surface CO₂ efflux and root biomass. In the present study, a development of this indirect methodology is presented by taking into consideration both the temporal variation and the spatial heterogeneity of heterotrophic respiration. For this purpose, soil CO₂ efflux, soil carbon content and main stand characteristics were estimated in seven evergreen forest ecosystems along an elevation gradient ranging from 250 to 1740 m. For each site and for each sampling date the measured soil CO₂ efflux (R _S) was predicted with the model R _S = a × S _C + b × R _D ± ε, where S _C is soil carbon content per unit area to a depth of 30 cm and R _D is the root density of the 2–5 mm root class. Regressions with statistically significant a and b coefficients allowed the indirect separation of the two components of soil CO₂ efflux. Considering that the different sampling dates were characterized by different soil temperature, it was possible to investigate the temporal and thermal dependency of autotrophic and heterotrophic respiration. It was estimated that annual autotrophic respiration accounts for 16–58% of total soil CO₂ efflux in the seven different evergreen ecosystems. In addition, our observations show a decrease of annual autotrophic respiration at increasing availability of soil nitrogen. Section Editor: A. Hodge     

冬小麦旺盛生长期间CO2浓度升高对根际呼吸的影响

依托FACE（free air carbon dioxide enrichment）技术平台,利用阻断根法,采用H6400红外气体分析仪（IRGA）-田间原位测定的方法,研究了大气CO2浓度升高和不同氮肥水平对水稻／小麦轮作制中冬小麦旺盛生长期间根际呼吸的影响。结果表明,在整个测定期间,大气CO2浓度升高增强了根际呼吸速率,提高了根际呼吸排放量。在高N和低N处理中,高CO2浓度下的根际呼吸总排放量分别比Ambient极显著增加117．0％和90．8％。根际呼吸速率在孕穗初期达到最大值;使根际呼吸在土壤呼吸中的比重由24．5％（LN）～26．7（HN）提高到39．8％（LN）～47．1％（HN）。CO2浓度升高与氮肥用量对根际呼吸产生交互效应。表明大气CO2浓度升高将加快土壤向大气的CO2排放,结果将有助于评价未来高CO2浓度背景下农田生态系统土壤碳的固定潜力。     

Coupling of canopy gas exchange with root and rhizosphere respiration in a semi-arid forest

The strength of coupling between canopy gas exchange and root respiration was examined in ~15-yr-old ponderosa pine (Pinus ponderosa Doug. Ex Laws.) growing under seasonally drought stressed conditions. By regularly watering part of the root system to reduce tree water stress and measuring soil CO₂ efflux on the dry, distant side of the tree, we were able to determine the strength of the relationship between soil autotrophic (root and rhizosphere) respiration and changes in canopy carbon uptake and water loss by comparison with control trees (no watering). After ~40 days the soil CO₂ efflux rate, relative to pre-treatment conditions, was twice that of the controls. This difference, attributable to root and rhizosphere respiration, was strongly correlated with differences in transpiration rates between treatments (r² = 0.73, p<0.01). By the end of the period, transpiration of the irrigated treatment was twice that of controls. Periodic measurements of photosynthesis under non-light limited conditions paralleled the patterns of transpiration and were systematically higher in the irrigated treatment. We observed no evidence for a greater sensitivity of soil autotrophic respiration to temperature compared to the response of heterotrophic respiration to temperature; the Q₁₀ for total soil respiration was 1.6 (p>0.99) for both treatments. At the ecosystem scale, daily soil CO₂ efflux rate was linearly related to gross primary productivity (GPP) as measured by eddy-covariance technique (r² = 0.55, p<0.01), suggesting patterns of soil CO₂ release appear strongly correlated to recent carbon assimilation in this young pine stand. Collectively the observed relationships suggest some consideration should be given to the inclusion of canopy processes in future models of soil respiration.     

Separating root and soil microbial contributions to soil respiration: A review of methods and observations

Forest soil respiration is the sum of heterotrophic (microbes, soil fauna) and autotrophic (root) respiration. The contribution of each group needs to be understood to evaluate implications of environmental change on soil carbon cycling and sequestration. Three primary methods have been used to distinguish hetero- versus autotrophic soil respiration including: integration of components contributing to in situ forest soil CO₂ efflux (i.e., litter, roots, soil), comparison of soils with and without root exclusion, and application of stable or radioactive isotope methods. Each approach has advantages and disadvantages, but isotope based methods provide quantitative answers with the least amount of disturbance to the soil and roots. Published data from all methods indicate that root/rhizosphere respiration can account for as little as 10 percent to greater than 90 percent of total in situ soil respiration depending on vegetation type and season of the year. Studies which have integrated percent root contribution to total soil respiration throughout an entire year or growing season show mean values of 45.8 and 60.4 percent for forest and nonforest vegetation, respectively. Such average annual values must be extrapolated with caution, however, because the root contribution to total soil respiration is commonly higher during the growing season and lower during the dormant periods of the year.     

CO2浓度增加和不同氮肥水平对冬小麦根系呼吸及生物量的影响

 依托FACE(Free-air CO₂ enrichment)研究平台, 利用特制分根集气生长箱, 采用静态箱-GC(Gas chromatography)法, 连续两年研究 了大气CO₂浓度升高和不同氮肥水平对冬小麦拔节期、孕穗抽穗期和灌浆末期的根系呼吸及生物量的影响。两季结果表明, CO₂浓度升高和高氮 肥量均不同程度地增加了3个阶段的地上部和地下部的生物量, 这有利于增加根茬的还田量; CO₂浓度升高对冬小麦不同生长阶段的根系呼吸影 响不同, 在拔节期影响较小;孕穗抽穗期显著增加了根系呼吸, 2004~2005季分别增加33.8%(148.1 mg N&;#8226;kg^-1 干土, HN)和43.9%(88.9 mg N&;#8226;kg^-1 干土, LN), 2005~2006季分别为23.8%(HN)和28.9%(LN); 而灌浆末期显著降低了根系呼吸, 2004~2005季分别降低31.4%(HN)和23.3% (LN), 2005~2006季分别为25.1%(HN)和18.5%(LN); 高施氮量比低施氮量促进了根系呼吸; 随着作物生长根系呼吸与地下生物量呈显著线性负相 关, 高CO₂环境中的R²变小,表明随着作物生长发育高CO₂浓度降低了作物根系呼吸与地下部生物量积累间的相关性.     

Interpreting,measuring, and modeling soil respiration

This paper reviews the role of soil respiration in determining ecosystem carbon balance, and the conceptual basis for measuring and modeling soil respiration. We developed it to provide background and context for this special issue on soil respiration and to synthesize the presentations and discussions at the workshop. Soil respiration is the largest component of ecosystem respiration. Because autotrophic and heterotrophic activity belowground is controlled by substrate availability, soil respiration is strongly linked to plant metabolism, photosynthesis and litterfall. This link dominates both base rates and short-term fluctuations in soil respiration and suggests many roles for soil respiration as an indicator of ecosystem metabolism. However, the strong links between above and belowground processes complicate using soil respiration to understand changes in ecosystem carbon storage. Root and associated mycorrhizal respiration produce roughly half of soil respiration, with much of the remainder derived from decomposition of recently produced root and leaf litter. Changes in the carbon stored in the soil generally contribute little to soil respiration, but these changes, together with shifts in plant carbon allocation, determine ecosystem carbon storage belowground and its exchange with the atmosphere. Identifying the small signal from changes in large, slow carbon pools in flux dominated by decomposition of recent material and autotrophic and mycorrhizal respiration is a significant challenge. A mechanistic understanding of the belowground carbon cycle and of the response of different components to the environment will aid in identifying this signal. Our workshop identified information needs to help build that understanding: (1) the mechanisms that control the coupling of canopy and belowground processes; (2) the responses of root and heterotrophic respiration to environment; (3) plant carbon allocation patterns, particularly in different forest developmental stages, and in response to treatments (warming, CO₂, nitrogen additions); and (4) coupling measurements of soil respiration with aboveground processes and changes in soil carbon. Multi-factor experiments need to be sufficiently long to allow the systems to adjust to the treatments. New technologies will be necessary to reduce uncertainty in estimates of carbon allocation, soil carbon pool sizes, and different responses of roots and microbes to environmental conditions.     

Spatial–temporal variation in soil respiration in an oak–grass savanna ecosystem in California and its partitioning into autotrophic and heterotrophic components

The spatial upscaling of soil respiration from field measurements to ecosystem levels will be biased without studying its spatial variation. We took advantage of the unique spatial gradients of an oak–grass savanna ecosystem in California, with widely spaced oak trees overlying a grass layer, to study the spatial variation in soil respiration and to use these natural gradients to partition soil respiration according to its autotrophic and heterotrophic components. We measured soil respiration along a 42.5 m transect between two oak trees in 2001 and 2002, and found that soil respiration under tree canopies decreased with distance from its base. In the open area, tree roots have no influence on soil respiration. Seasonally, soil respiration increased in spring until late April, and decreased in summer following the decrease in soil moisture content, despite the further increase in soil temperature. Soil respiration significantly increased following the rain events in autumn. During the grass growing season between November and mid-May, the average of CO₂ efflux under trees was 2.29 μmol m⁻² s⁻¹, while CO₂ efflux from the open area was 1.40 μmol m⁻² s⁻¹. We deduced that oak root respiration averaged as 0.89 μmol m⁻² s⁻¹, accounting for 39% of total soil respiration (oak root + grass root + microbes). During the dry season between mid-May and October, the average of CO₂ efflux under trees was 0.87 μmol m⁻² s⁻¹, while CO₂ efflux from the open areas was 0.51 μmol m⁻² s⁻¹. Oak root respiration was 0.36 μmol m⁻² s⁻¹, accounting for 41% of total soil respiration (oak root + microbes). The seasonal pattern of soil CO₂ efflux under trees and in open areas was simulated by a bi-variable model driven by soil temperature and moisture. The diurnal pattern was influenced by tree physiology as well. Based on the spatial gradient of soil respiration, spatial analysis of crown closure and the simulation model, we spatially and temporally upscaled chamber measurements to the ecosystem scale. We estimated that the cumulative soil respiration in 2002 was 394 gC m⁻² year⁻¹ in the open area and 616 gC m⁻² year⁻¹ under trees with a site-average of 488 gC m⁻² year⁻¹.     

CO2浓度升高和施氮条件下小麦根际呼吸对土壤呼吸的贡献

依托FACE技术平台,采用稳定13C同位素技术,通过将小麦(C3作物)种植于长期单作玉米(C4作物)的土壤上,研究了大气CO2浓度升高和不同氮肥水平对土壤排放CO2的δ13C值及根际呼吸的影响.结果表明:种植小麦后土壤排放CO2的δ13C值随作物生长逐渐降低,CO2浓度升高200 μmol·mol-1显著降低了孕穗、抽穗期(施氮量为250 kg·hm-2,HN)与拔节、孕穗期(施氮量为150 kg·hm-2,LN)土壤排放CO2的δ13C值,显著提高了孕穗、抽穗期的根际呼吸比例.拔节至成熟期,根际呼吸占土壤呼吸的比例在高CO2浓度下为24％～48％ (HN)和21％ ～48％ (LN),在正常CO2浓度下为20％ ～36％ (HN)和19％～32％(LN).不同CO2浓度下土壤排放CO2的δ13C值和根际呼吸对氮肥增加的响应不同,CO2浓度与氮肥用量在拔节期对根际呼吸的交互效应显著.     

CO2浓度升高和施氮条件下小麦根际呼吸对土壤呼吸的贡献

依托FACE技术平台, 采用稳定¹³C同位素技术, 通过将小麦(C₃作物)种植于长期单作玉米(C₄作物)的土壤上, 研究了大气CO₂浓度升高和不同氮肥水平对土壤排放CO₂的δ¹³C值及根际呼吸的影响. 结果表明: 种植小麦后土壤排放CO₂的δ¹³C值随作物生长逐渐降低, CO₂浓度升高200 μmol·mol^-1显著降低了孕穗、抽穗期(施氮量为250 kg·hm^-2, HN)与拔节、孕穗期(施氮量为150 kg·hm^-2, LN)土壤排放CO₂的δ¹³C值, 显著提高了孕穗、抽穗期的根际呼吸比例. 拔节至成熟期, 根际呼吸占土壤呼吸的比例在高CO₂浓度下为24%～48%(HN)和21%～48%(LN), 在正常CO₂浓度下为20%～36% (HN)和19%～32%(LN). 不同CO₂浓度下土壤排放CO₂的δ¹³C值和根际呼吸对氮肥增加的响应不同, CO₂浓度与氮肥用量在拔节期对根际呼吸的交互效应显著.     

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。     

神农架海拔梯度上4种典型森林的土壤呼吸组分及其对温度的敏感性

量化森林土壤呼吸及其组分对温度的响应对准确评估未来气候变化背景下陆地生态系统的碳平衡极其重要。该文通过对神农架海拔梯度上常绿阔叶林、常绿落叶阔叶混交林、落叶阔叶林以及亚高山针叶林4种典型森林土壤呼吸的研究发现: 4种森林类型的年平均土壤呼吸速率和年平均异养呼吸速率分别为1.63、1.79、1.74、1.35 μmol CO₂·m^-2·s^-1和1.13、1.12、1.12、0.80 μmol CO₂·m^-2·s^-1。该地区的土壤呼吸及其组分呈现出明显的季节动态, 夏季最高, 冬季最低。4种森林类型中, 阔叶林的土壤呼吸显著高于针叶林, 但阔叶林之间的土壤呼吸差异不显著。土壤温度是影响土壤呼吸及其组分的主要因素, 二者呈显著的指数关系; 土壤含水量与土壤呼吸之间没有显著的相关关系。4种典型森林土壤呼吸的Q₁₀值分别为2.38、2.68、2.99和4.24, 随海拔的升高土壤呼吸对温度的敏感性增强, Q₁₀值随海拔的升高而增加。     

Partitioning the components of soil respiration: a research challenge

Little is known about the respiratory components of CO₂ emitted from soils and attaining a reliable quantification of the contribution of root respiration remains one of the major challenges facing ecosystem research. Resolving this would provide major advances in our ability to predict ecosystem responses to climate change. The merits and technical and theoretical difficulties associated with different approaches adopted for partitioning respiration components are discussed here. The way forward is suggested to be the development of non-invasive regression analysis validated by stable isotope approaches to increase the sensitivity of model functions to include components of rhizosphere microbial activity, changing root biomass and the dynamics of a wide range of soil C pools. Section Editor: A. Hodge     

Soil respiration of Alaskan tundra at elevated atmospheric carbon dioxide concentrations

Summary CO₂ efflux from tussock tundra in Alaska that had been exposed to elevated CO₂ for 2.5 growing seasons was measured to assess the effect of long- and short-term CO₂ enrichment on soil respiration. Long-term treatments were: 348, 514, and 683 μll⁻¹ CO₂ and 680 μll⁻¹ CO₂+4°C above ambient. Measurements were made at 5 CO₂ concentrations between 87 and 680 μll⁻¹ CO₂. Neither long- or short-term CO₂ enrichment significantly affected soil CO₂ efflux. Tundra developed at elevated temperature and 680 μll⁻¹ CO₂ had slightly higher, but not statistically different, mean respiration rates compared to untreated tundra and to tundra under CO₂ control alone.     

Effect of carbon dioxide concentration on microbial respiration in soil

In order to assess the validity of conventional methods for measuring CO₂ flux from soil, the relationship between soil microbial respiration and ambient CO₂ concentration was studied using an open-flow infra-red gas analyser (IRGA) method. Andosol from an upland field in central Japan was used as a soil sample. Soil microbial respiration activity was depressed with the increase of CO₂ concentration in ventilated air from 0 to 1000 ppmv. At 1000 ppmv, the respiration rate was less than half of that at 0 ppmv. Thus, it is likely that soil respiration rate is overestimated by the alkali absorption method, because CO₂ concentration in the absorption chamber is much lower than the normal level. Metabolic responses to CO₂ concentration were different among groups of soil microorganisms. The bacteria actinomycetes group cultivated on agar medium showed a more sensitive response to the CO₂ concentration than the filamentous fungi group.     

Changes in soil CO2 and O2 concentrations when radiata pine is grown in competition with pasture or weeds and possible feedbacks with radiata pine root growth and respiration

This study examined the reciprocal effects of growing ryegrass, lotus and other weed species in competition with radiata pine on soil CO₂ and O₂ concentrations and on the growth and root respiration of the radiata pine. Soil O₂ concentrations decreased and soil CO₂ concentrations increased with increasing soil depth. Radiata pine plus competing species slightly reduced soil O₂ concentrations and markedly increased soil CO₂ concentrations (up to 40 mmol mol⁻¹) compared with radiata pine alone. The dry weights of shoots and roots, and the root respiration rates of radiata pine grown with competing vegetation were much less than those for radiata pine alone. This probably was not solely caused by competition for nutrients water or light since adequate water and nutrients were supplied to all treatments and the radiata pine overtopped the competing vegetation. When radiata pine roots were raised in NaHCO₃ solutions equivalent to a range of CO₂ concentrations, succinate dehydrogenase activity (a metabolic indicator of mitochondrial respiration) and elongation rates of roots decreased as CO₂ concentrations increased from 0 to 40 mmol mol⁻¹. This suggests that the elevated CO₂ concentrations found in the experiments in soil was the cause, at least in part, of the reduced growth of radiata pine in competition with other species. This revised version was published online in June 2006 with corrections to the Cover Date.     

Non-phototrophic CO 2 fixation by soil microorganisms

Although soils are generally known to be a net source of CO₂ due to microbial respiration, CO₂ fixation may also be an important process. The non-phototrophic fixation of CO₂ was investigated in a tracer experiment with ¹⁴CO₂ in order to obtain information about the extent and the mechanisms of this process. Soils were incubated for up to 91 days in the dark. In three independent incubation experiments, a significant transfer of radioactivity from ¹⁴CO₂ to soil organic matter was observed. The process was related to microbial activity and could be enhanced by the addition of readily available substrates such as acetate. CO₂ fixation exhibited biphasic kinetics and was linearly related to respiration during the first phase of incubation (about 20–40 days). The fixation amounted to 3–5% of the net respiration. After this phase, the CO₂ fixation decreased to 1–2% of the respiration. The amount of carbon fixed by an agricultural soil corresponded to 0.05% of the organic carbon present in the soil at the beginning of the experiment, and virtually all of the fixed CO₂ was converted to organic compounds. Many autotrophic and heterotrophic biochemical processes result in the fixation of CO₂. However, the enhancement of the fixation by addition of readily available substrates and the linear correlation with respiration suggested that the process is mainly driven by aerobic heterotrophic microorganisms. We conclude that heterotrophic CO₂ fixation represents a significant factor of microbial activity in soils.     

Soybean root respiration assessed from short-term14C-activity changes

During and immediately after labelling of soybeans (Glycine max. L.) in the field by exposure to¹⁴CO₂, its respiratory deposit into the soil atmosphere, and its liberation from the soil were used in conjunction with estimates of below-ground plant biomass to apportion total soil respiration. Root respiration of soybean plants at stage V₆ was estimated at 4 mg CO₂.(g root)^–1.h^–1. Soil biota, during the same time, contributed 35% of total soil respiration.Contribution from the Missouri Agricultural Experiment Station. Journal Series Number 10700. Funded in part by USDA Grant SE 83-CRSR-2-2309.     

Soil respiration response to three years of elevated CO2 and N fertilization in ponderosa pine (Pinus ponderosa Doug. ex Laws.)

We measured growing season soil CO₂ evolution under elevated atmospheric [CO₂] and soil nitrogen (N) additions. Our objectives were to determine treatment effects, quantify seasonal variation, and compare two measurement techniques. Elevated [CO₂] treatments were applied in open-top chambers containing ponderosa pine (Pinus ponderosa L.) seedlings. N applications were made annually in early spring. The experimental design was a replicated factorial combination of CO₂ (ambient, + 175, and +350 L L^–1 CO₂) and N (0, 10, and 20 g m^–2 N as ammonium sulphate). Soils were irrigated to maintain soil moisture at > 25 percent. Soil CO₂ evolution was measured over diurnal periods (20–22 hours) in October 1992, and April, June, and October 1993 and 1994 using a flow-through, infrared gas analyzer measurement system and corresponding pCO₂ measurements were made with gas wells. Significantly higher soil CO₂ evolution was observed in the elevated CO₂ treatments; N effects were not significant. Averaged across all measurement periods, fluxes, were 4.8, 8.0, and 6.5 for ambient + 175 CO₂, and +350 CO₂ respectively).Treatment variation was linearly related to fungal occurrence as observed in minirhizotron tubes. Seasonal variation in soil CO₂ evolution was non-linearly related to soil temperature; i.e., fluxes increased up to approximately soil temperature (10cm soil depth) and decreased dramatically at temperatures > 18°C. These patterns indicate exceeding optimal temperatures for biological activity. The dynamic, flow-through measurement system was weakly correlated (r = 0.57; p < 0.0001; n = 56) with the pCO₂ measurement method.     

Estimating respiration of roots in soil: Interactions with soil CO2, soil temperature and soil water content

Little information is available on the variability of the dynamics of the actual and observed root respiration rate in relation to abiotic factors. In this study, we describe I) interactions between soil CO₂ concentration, temperature, soil water content and root respiration, and II) the effect of short-term fluctuations of these three environmental factors on the relation between actual and observed root respiration rates. We designed an automated, open, gas-exchange system that allows continuous measurements on 12 chambers with intact roots in soil. By using three distinct chamber designs with each a different path for the air flow, we were able to measure root respiration over a 50-fold range of soil CO₂ concentrations (400 to 25000 ppm) and to separate the effect of irrigation on observed vs. actual root respiration rate. All respiration measurements were made on one-year-old citrus seedlings in sterilized sandy soil with minimal organic material.Root respiration was strongly affected by diurnal fluctuations in temperature (Q₁₀ = 2), which agrees well with the literature. In contrast to earlier findings for Douglas-fir (Qi et al., 1994), root respiration rates of citrus were not affected by soil CO₂ concentrations (400 to 25000 ppm CO₂; pH around 6). Soil CO₂ was strongly affected by soil water content but not by respiration measurements, unless the air flow for root respiration measurements was directed through the soil. The latter method of measuring root respiration reduced soil CO₂ concentration to that of incoming air. Irrigation caused a temporary reduction in CO₂ diffusion, decreasing the observed respiration rates obtained by techniques that depended on diffusion. This apparent drop in respiration rate did not occur if the air flow was directed through the soil. Our dynamic data are used to indicate the optimal method of measuring root respiration in soil, in relation to the objectives and limitations of the experimental conditions.     

施肥方式对紫色土土壤异养呼吸的影响

采用静态暗箱-气相色谱法于2010年12月至2011年10月对不同施肥方式下的紫色土土壤呼吸进行了研究,以揭示施肥方式对紫色土异养呼吸的影响。结果表明:施肥可对土壤异养呼吸产生激发效应。施肥后第5天出现峰值,猪厩肥处理的异养呼吸峰值为2356.8 mg CO2m-2h-1,显著高于秸秆配施氮磷钾(970.1 mgCO2m-2h-1)和常规氮磷钾处理(406.8 mgCO2m-2h-1)(P0.01);小麦季常规氮磷钾、猪厩肥和秸秆配施氮磷钾处理的平均土壤异养呼吸速率为212.9、285.8和305.8mgCO2m-2h-1,CO2排放量为255.1、342.3和369.5 gC/m2,玉米季为408.2、642.8和446.4 mgCO2m-2h-1,CO2排放量为344.7、542.8和376.9 gC/m2,玉米季土壤异养呼吸平均速率及CO2排放量均高于小麦季。全年平均土壤异养呼吸速率分别为310.6、446.3和377.4 mg CO2m-2h-1,CO2排放总量分别为599.8、885.1和746.4 gC/m2。猪厩肥对土壤异养呼吸速率和CO2排放量的影响最大,秸秆配施氮磷钾肥次之,氮磷钾肥最小,说明有机物料的投入是紫色土土壤异养呼吸速率的主要调控措施,低碳氮比的有机物料能促进土壤异养呼吸和CO2的排放。猪厩肥和秸秆配施氮磷钾肥处理相应地表和地下5 cm温度的Q10值分别为2.64、1.88和2.77、1.99,表明低碳氮比的有机物料还能增加土壤异养呼吸Q10值,使土壤异养呼吸速率对温度的敏感性加强。