Significance of temperature and water availability for soil phosphorus transformation and microbial community composition as affected by fertilizer sources

Little is known about the effects of temperature and drying–rewetting on soil phosphorus (P) fractions and microbial community composition in regard to different fertilizer sources. Soil P dynamics and microbial community properties were evaluated in a soil not fertilized or fertilized with KH₂PO₄ or swine manure at two temperatures (10 and 25 °C) and two soil water regimes (continuously moist and drying–rewetting cycles) in laboratory microcosm assays. The P source was the dominant factor determining the sizes of labile P fractions and microbial community properties. Manure fertilization increased the content of labile P, microbial biomass, alkaline phosphomonoesterase activity, and fatty acid contents, whereas KH₂PO₄ fertilization increased the content of labile inorganic P and microbial P. Water regimes, second to fertilization in importance, affected more labile P pools, microbial biomass, alkaline phosphomonoesterase activity, and fatty acid contents than temperature. Drying–rewetting cycles increased labile P pools, decreased microbial biomass and alkaline phosphomonoesterase activity, and shaped the composition of microbial communities towards those with greater percentages of unsaturated fatty acids, particularly at 25 °C in manure-fertilized soils. Microbial C and P dynamics responded differentially to drying–rewetting cycles in manure-fertilized soils but not in KH₂PO₄-fertilized soils, suggesting their decoupling because of P sources and water regimes. Phosphorus sources, temperature, and water regimes interactively affected the labile organic P pool in the middle of incubation. Overall, P sources and water availability had greater effects on P dynamics and microbial community properties than temperature.     

The extent of drying influences the flush of respiration after rewetting in non-saline and saline soils

Drying and rewetting are common events in soils during summer, particularly in Mediterranean climate where soil microbes may be further challenged by salinity. Previous studies in non-saline soils have shown that rewetting induces a flush of soil respiration, but little is known about how the extent of drying affects the size of the respiration flush or how drying and rewetting affects soil respiration in saline soils. Five sandy loam soils, ranging in electrical conductivity of the saturated soil extract (ECe) from 2 to 48 dS m⁻¹ (EC2, EC9, EC19, EC33 and EC48), were kept at soil water content optimal for respiration or dried for 1, 2, 3, 4 or 5 days (referred to 1D, 2D, 3D, 4D and 5D) and maintained at the achieved water content for 4 days. Then the soils were rewet to optimal water content and incubated moist for 5 days. Water potential decreased with increasing drying time; in the 5D treatment, the water potential ranged between −15 and −30 MPa, with the lowest potentials in soil EC33. In moist and dry conditions, respiration rates per unit soil organic C (SOC) were highest in soil EC19. Respiration rates decreased with increasing time of drying; when expressed relative to constantly moist soil, the decline was similar in all soils. Rewetting of soils only induced a flush of respiration compared to constantly moist soil when the soils were dried for 3 or more days. The flush in respiration was greatest in 5D and smallest in 3D, and greater in EC2 than in the saline soils. Cumulative respiration per unit SOC was highest in soil EC19 and lowest in soil EC2 Cumulative respiration decreased with increasing time of drying, but in a given soil, the relationship between water potential during the dry phase and cumulative respiration at the end of the experiment was weaker than that between respiration rate during drying and water potential. In conclusion, rewetting induced a flush in respiration only if the water potential of the soils was previously decreased at least 3-fold compared to the constantly moist soil. Hence, only marked increases in water potential induce a flush in respiration upon rewetting. The smaller flush in respiration upon rewetting of saline soils suggests that these soils may be less prone to lose C when exposed to drying and rewetting compared to non-saline soils.     

Carbon mineralization in saline soils as affected by residue composition and water potential

In saline soils under semi-arid climate, low matric and osmotic potential are the main stressors for microbes. But little is known about the impact of water potential (sum of matric and osmotic potential) and substrate composition on microbial activity and biomass in field collected saline soils. Three sandy loam soils with electrical conductivity of the saturated soil extract (EC_e) 3.8, 11 and 21 dS m^?1 (hereafter referred to EC3.8, EC11 and EC21) were kept at optimal water content for 14 days. After this pre-incubation, the soils were either left at optimal water content or dried to achieve water potentials of ?2.33, ?2.82, ?3.04 and ?4.04 MPa. Then, the soils were amended with 20 g?kg^?1 pea or wheat residue to increase nutrient supply. Carbon dioxide emission was measured over 14 days; microbial biomass C was measured at the end of the experiment. Cumulative respiration decreased with decreasing water potential and was significantly (P?<?0.05) lower in soils at water potential ?4 MPa than in soils at optimal water content. The effect of residue type on the response of cumulative respiration was inconsistent; with residue type having no effect in the saline soils (EC11 and EC21) whereas in the non-saline soil (EC3.8), the decrease in respiration with decreasing water potential was less with wheat than with pea residue. At a given water potential, the absolute and relative (in percentage of optimal water content) cumulative respiration was lower in the saline soils than in the non-saline soil. This can be explained by the lower osmotic potential and the smaller microbial biomass in the saline soils. However, even at a similar osmotic potential, cumulative respiration was higher in the non-saline soil. It can be concluded that high salt concentrations in the soil solution strongly reduce microbial activity even if the water content is relatively high. The stronger relative decrease in microbial activity in the saline soils at a given osmotic potential compared to the non-saline soil suggests that the small biomass in saline soils is less able to tolerate low osmotic potential. Hence, drying of soil will have a stronger negative effect on microbial activity in saline than in non-saline soils.     

Simple and Rapid Laboratory Method for Rewetting Dry Soil for Incubations

Soil microbial activity is greatly affected by soil water content. Determining the appropriate moisture content to rewet soils that have been dried in preparation for laboratory incubations to determine microbial activity can be laborious and time-consuming. The most common methods used achieve sufficient moisture content for peak microbial respiration are gravimetric water content, soil matric potential, or percentage of water-filled pore space (WFPS). Alternatively, a fast, simple, and accurate way to ensure that a given soil receives the appropriate amount of water for peak soil microbial respiration is to rely on natural capillary action for rewetting the dry soil. The capillary method is related to the gravimetric method for water uptake and has a strong correlation with WFPS. A microbial respiration test was conducted to compare rewetting methods. The 24-h carbon dioxide (CO₂) / carbon (C) results were very similar and strongly correlated using the gravimetric method and the capillary method for rewetting dried soil.     

Relationships of soil respiration to microbial biomass, substrate availability and clay content

The roles of microbial biomass (MBC) and substrate supply as well as their interaction with clay content in determining soil respiration rate were studied using a range of soils with contrasting properties. Total organic C (TOC), water-soluble organic carbon, 0.5 M K₂SO₄-extractable organic C and 33.3 mM KMnO₄-oxidisable organic carbon were determined as C availability indices. For air-dried soils, these indices showed close relationship with flush of CO₂ production following rewetting of the soils. In comparison, MBC determined with the chloroform fumigation-extraction technique had relatively weaker correlation with soil respiration rate. After 7 d pre-incubation, soil respiration was still closely correlated with the C availability indices in the pre-incubated soils, but poorly correlated with MBC determined with three different techniques—chloroform fumigation extraction, substrate-induced respiration, and chloroform fumigation-incubation methods. Results of multiple regression analyses, together with the above observations, suggested that soil respiration under favourable temperature and moisture conditions was principally determined by substrate supply rather than by the pool size of MBC. The specific respiratory activity of microorganisms (CO₂-C/MBC) following rewetting of air-dried soils or after 7 d pre-incubation was positively correlated with substrate availability, but negatively correlated with microbial pool size. Clay content had no significant effect on CO₂ production rate, relative C mineralization rate (CO₂-C/TOC) and specific respiratory activity of MBC during the first week incubation of rewetted dry soils. However, significant protective effect of clay on C mineralization was shown for the pre-incubated soils. These results suggested that the protective effect of clay on soil organic matter decomposition became significant as the substrate supply and microbial demand approached to an equilibrium state. Thereafter, soil respiration would be dependent on the replenishment of the labile substrate from the bulk organic C pool.     

Compaction effects on CO2 and N2O production during drying and rewetting of soil

The effects of compaction on soil porosity and soil water relations are likely to influence substrate availability and microbial activity under fluctuating soil moisture conditions. We conducted a short laboratory incubation to investigate the effects of soil compaction on substrate availability and biogenic gas (CO₂ and N₂O) production during the drying and rewetting of a fine-loamy soil. Prior to initiating the drying and wetting treatments, CO₂ production (−10 kPa soil water content) from uncompacted soil was 2.3 times that of compacted soil and corresponded with higher concentrations of microbial biomass C (MBC) and dissolved organic C (DOC). In contrast, N₂O production was 67 times higher in compacted than uncompacted soil at field capacity. Soil aeration rather than substrate availability (e.g. NO₃⁻ and DOC) appeared to be the most important factor affecting N₂O production during this phase. The drying of compacted soil resulted in an initial increase in CO₂ production and a nearly two-fold higher average rate of C mineralization at maximum dryness (owing to a higher water-filled pore space [WFPS]) compared to uncompacted soil. During the drying phase, N₂O production was markedly reduced (by 93-96%) in both soils, though total N₂O production remained slightly higher in compacted than uncompacted soil. The increase in CO₂ production during the first 24 h following rewetting of dry soil was about 2.5 times higher in uncompacted soil and corresponded with a much greater release of DOC than in compacted soil. MBC appeared to be the source of the DOC released from uncompacted soil but not from compacted soil. The production of N₂O during the first 24 h following rewetting of dry soil was nearly 20 times higher in compacted than uncompacted soil. Our results suggest that N₂O production from compacted soil was primarily the result of denitrification, which was limited by substrates (especially NO₃⁻) made available during drying and rewetting and occurred rapidly after the onset of anoxic conditions during the rewetting phase. In contrast, N₂O production from uncompacted soil appeared to be primarily the product of nitrification that was largely associated with an accumulation of NO₃⁻ following rewetting of dry soil. Irrespective of compaction, the response to drying and rewetting was greater for N₂O production than for CO₂ production.     

Carbon and nitrogen turnover in two acid forest soils of southeast Australia as affected by phosphorus addition and drying and rewetting cycles

The effects of adding P and of drying and rewetting were studied in two acid forest soils from southeast Australia. The soils were a yellow podzolic with a low soil organic matter content (3.75% C) and a red earth with a high organic matter content (13.5% C). C and N mineralization and microbial C and N contents were investigated in a laboratory incubation for 151 days. Microbial C and N were estimated by a hexanol fumigation-extraction technique. Microbial C was also determined by substrate-induced respiration combined with a selective inhibition technique to separate the fungal and the bacterial biomass. The results obtained by the selective inhibition technique were not conclusive. Adding P to the soil and drying and rewetting the soil reduced microbial N. This effect was more pronounced in rapidly and frequently dried soils. Microbial C was generally less affected by these treatments. Compared with the control, the addition of P caused a reduction in respiration in the red earth (-13%) but an increase in the yellow podzolic soil (+12%). In the red earth net N mineralization was highest following the addition of P. In the yellow podzolic soil highest N mineralization rates were obtained when the soil was subjected to drying and rewetting cycles. In both soils increased N mineralization was associated with a decrease in microbial N, indicating that the mineralized N was of microbial origin. Nitrification decreased with rapid drying and rewetting. The addition of P promoted heterotrophic nitrification in both soils.     

Substantial rewetting phenomena on soil respiration can be observed at low water availability

Although metabolic activity of soil organisms is determined by water accessibility, little attention was given to rewetting with different water potentials. Rapid water potential increase induced a respiration pulse in organic layers in laboratory experiments and significant effects could be observed when soil below −6300 hPa was rewetted.     

Rapid changes in carbon and phosphorus after rewetting of dry soil

Drying–rewetting (DRW) cycles are important for soil organic matter turnover; however, few studies have considered the short-term effects on nutrient availability. The pulses in soil respiration, extractable C, P and N pools were quantified after a single DRW cycle (ten sampling times over 49 h). Soil was pre-incubated with or without glucose (2.5 g kg⁻¹) for 10 days to induce differences in the size and activity of the microflora and then either subjected to a single DRW cycle (7-day drying period) or kept constantly moist. A resin extractable P (P_resin) method was used and compared to extraction of dissolved organic (DOP) and inorganic P (DIP) with a salt solution. The pulse in soil respiration, extractable organic C (EOC), P_resin, DOP and DIP was immediate and greatest in the first 2 h. The P_resin pulse was two to three times that measured by solution extraction (DIP). Also, P_resin quantified temporal changes in P not apparent in DIP, indicating the advantage of anion-exchange membranes in quantifying short-term changes in P availability. The P_resin pulse was smaller in the soil incubated with glucose showing that P pulses will be quantitatively smaller in a soil with an active microbial biomass. In contrast to P, pre-incubation with glucose did not alter EOC concentration or the pulse in EOC after rewetting. The P_resin pulse had disappeared by 49 h after DRW despite continued elevated rates of respiration. The sustained increase in DIP following DRW may have implications for plant availability or environmental losses.     

Effect of temperature on soil microbial biomass and its metabolic quotient in situ under different tillage systems

Variations in the microbial biomass and the in situ metabolic quotient (qCO₂) due to climatic conditions were determined in a typical soil from the Argentine Rolling Pampa. Microbial C was evaluated by fumigation-incubation and qCO₂ was calculated using soil respiration in the field. An inverse relationship between microbial C and soil temperature was fitted to a model (r ²=0.90, P=0.01). No significant association with the soil water content was detected because the soil was generally near field capacity and thus water availability did not limited microbial growth and activity. Values of qCO₂ increased (r ²=0.89, P=0.01) as the result of metabolic activatìon, likely induced by a higher maintenance energy requirement at high temperatures. The highest values of qCO₂ were obtained when microbial C was the lowest, which was attributed to self consumption of microbial C in the presence of high temperatures. Consequently, microbial C was generally higher (P=0.05) in winter than in summer. Therefore, when microbial C is used as an index of soil biological activity, the influence of temperature should be taken into account.     

Characterization of the water soluble soil organic pool following the rewetting of dry soil in a drought-prone tallgrass prairie

To better understand the nature of the C flush that follows the rewetting of dry soil, we chemically characterized the water soluble pools following rewetting of soil dried to several different water potentials. To assess the impact that historical soil water status has on the size of the rewetting labile soluble pool, a laboratory water stress gradient was applied to soils that were collected from drought-prone and irrigated tallgrass prairie soils. In the laboratory, soils were either incubated at −33 kPa or dried steadily over a 0.6, 1, 2, or 3 day period to −1.5, −4, −15, and −45 MPa respectively. On the 4th day, samples were wetted back to −33 kPa and immediately assayed for soluble, microbial, or respiratory pools of carbon. After extraction, samples were also assayed using NMR, GC-MS, and LC-MS to assess carbohydrate, amino acid, osmolyte and sugar pools. The greater the degree of drying before rewetting was associated with greater concentrations of microbial, soluble and respiratory pools of carbon, increasing by 50, 400 and 250%, respectively, in the most water stressed compared to continuously moist soil. Compared to drought-prone soils, the amount of soluble C released as a result of rewetting was 30 to 50% greater in soils that were irrigated for 11 years. The pool of organics was not completely characterized and only small amounts of TBDMS and TMS derived compounds accounting for 2-4% of the soluble C pool were detected. In contrast, oligosaccharides constituted approximately 20-25% of the sample C. Our results suggest that the flush of C following wetting of a dry soil is not dominated by common microbial osmolytes (e.g. proline, glycine betaine, ectoine, glycerol, mannitol, trehalose). In light of this finding more research is needed to better understand the adaptations that microbial communities utilize to respond to the rewetting of dried soil.     

Drying and rewetting effects on C and N mineralization and microbial activity in surface and subsurface California grassland soils

Rewetting a dry soil has long been known to cause a burst of respiration (the “Birch Effect”). Hypothesized mechanisms for this involve: (1) release of cellular materials as a result of the rapid increase in water potential stress and (2) stimulating C-supply to microbes via physical processes. The balance of these factors is still not well understood, particularly in the contexts of multiple dry/wet cycles and of how resource and stress patterns vary through the soil profile. We evaluated the effects of multiple dry/wet cycles on surface and subsurface soils from a California annual grassland. Treatments included 4, 6, and 12 cycles that varied the length of the drying period between rewetting events. Respiration was monitored after each wetting event while extractable C and N, microbial biomass, and microbial activity were assayed initially, after the first rewetting event, and at the end of the experiment. Initially, microbial biomass and activity (respiration, dehydrogenase, and N mineralization) in subsurface soils were ca. 10% and 20% of surface soil levels. After multiple cycles, however, subsurface soil microbial biomass and activity were enhanced by up to 8-fold, even in comparison to the constantly moist treatment. By comparison, surface soil microbial biomass and activity were either moderately (i.e. 1.5 times increase) or not affected by wetting and drying. Drying and rewetting led to a cascade of responses (soluble C release, biomass growth, and enhanced activity) that mobilized and metabolized otherwise unavailable soil carbon, particularly in subsurface soils.     

Carbon pulses but not phosphorus pulses are related to decreases in microbial biomass during repeated drying and rewetting of soils

Drying and rewetting cycles are known to be important for the turnover of carbon (C) in soil, but less is known about the turnover of phosphorus (P) and its relation to C cycling. In this study the effects of repeated drying-rewetting (DRW) cycles on phosphorus (P) and carbon (C) pulses and microbial biomass were investigated. Soil (Chromic Luvisol) was amended with different C substrates (glucose, cellulose, starch; 2.5 g C kg⁻¹) to manipulate the size and community composition of the microbial biomass, thereby altering P mineralisation and immobilisation and the forms and availability of P. Subsequently, soils were either subjected to three DRW cycles (1 week dry/1 week moist) or incubated at constant water content (70% water filled pore space). Rewetting dry soil always produced an immediate pulse in respiration, between 2 and 10 times the basal rates of the moist incubated controls, but respiration pulses decreased with consecutive DRW cycles. DRW increased total CO₂ production in glucose and starch amended and non-amended soils, but decreased it in cellulose amended soil. Large differences between the soils persisted when respiration was expressed per unit of microbial biomass. In all soils, a large reduction in microbial biomass (C and P) occurred after the first DRW event, and microbial C and P remained lower than in the moist control. Pulses in extractable organic C (EOC) after rewetting were related to changes in microbial C only during the first DRW cycle; EOC concentrations were similar in all soils despite large differences in microbial C and respiration rates. Up to 7 mg kg⁻¹ of resin extractable P (P_resin) was released after rewetting, representing a 35-40% increase in P availability. However, the pulse in P_resin had disappeared after 7 d of moist incubation. Unlike respiration and reductions in microbial P due to DRW, pulses in P_resin increased during subsequent DRW cycles, indicating that the source of the P pulse was probably not the microbial biomass. Microbial community composition as indicated by fatty acid methyl ester (FAME) analysis showed that in amended soils, DRW resulted in a reduction in fungi and an increase in Gram-positive bacteria. In contrast, the microbial community in the non-amended soil was not altered by DRW. The non-selective reduction in the microbial community in the non-amended soil suggests that indigenous microbial communities may be more resilient to DRW. In conclusion, DRW cycles result in C and P pulses and alter the microbial community composition. Carbon pulses but not phosphorus pulses are related to changes in microbial biomass. The transient pulses in available P could be important for P availability in soils under Mediterranean climates.     

Role of soil drying in nitrogen mineralization and microbial community function in semi-arid grasslands of north-west Australia

We examined effects of wetting and then progressive drying on nitrogen (N) mineralization rates and microbial community composition, biomass and activity of soils from spinifex (Triodia R. Br.) grasslands of the semi-arid Pilbara region of northern Australia. We compared soils under and between spinifex hummocks and also examined impacts of fire history on soils over a 28 d laboratory incubation. Soil water potentials were initially adjusted to −100 kPa and monitored as soils dried. We estimated N mineralization by measuring changes in amounts of nitrate (NO₃⁻-N) and ammonium (NH₄⁺-N) over time and with change in soil water potential. Microbial activity was assessed by amounts of CO₂ respired. Phospholipid fatty acid (PLFA) analyses were used to characterize shifts in microbial community composition during soil drying. Net N mineralized under hummocks was twice that of open spaces between hummocks and mineralization rates followed first-order kinetics. An initial N mineralization flush following re-wetting accounted for more than 90% of the total amount of N mineralized during the incubation. Initial microbial biomass under hummocks was twice that of open areas between hummocks, but after 28 d microbial biomass was<2 μ g⁻¹ ninhydrin N regardless of position. Respiration of CO₂ from soils under hummocks was more than double that of soils from between hummocks. N mineralization, microbial biomass and microbial activity were negligible once soils had dried to −1000 kPa. Microbial community composition was also significantly different between 0 and 28 d of the incubation but was not influenced by burning treatment or position. Regression analysis showed that soil water potential, microbial biomass N, NO₃⁻-N, % C and δ¹⁵N all explained significant proportions of the variance in microbial community composition when modelled individually. However, sequential multiple regression analysis determined only microbial biomass was significant in explaining variance of microbial community compositions. Nitrogen mineralization rates and microbial biomass did not differ between burned and unburned sites suggesting that any effects of fire are mostly short-lived. We conclude that the highly labile nature of much of soil organic N in these semi-arid grasslands provides a ready substrate for N mineralization. However, process rates are likely to be primarily limited by the amount of substrate available as well as water availability and less so by substrate quality or microbial community composition.     

干湿交替对土壤碳库和有机碳矿化的影响

水分是影响土壤活性碳库和惰性碳库周转过程的主导因子,而土壤有机碳的周转速率会对气候变化造成潜在的重要影响。以农田水稻土为供试土壤,通过培育试验研究了干湿交替过程对土壤有机碳矿化的影响,并利用两库叠加模型对土壤不同碳库及其降解动力学进行初步评估。结果表明:干湿交替激发了土壤呼吸,增加了土壤微生物代谢活性。三次湿润过程对土壤呼吸的激发量分别为119.3%、159.5%和87.3%,激发效应随干湿交替频率的增加先升高后降低。多次干湿交替后,土壤累积CO2释放量低于恒湿土壤,湿润所引起的激发的矿化量不足以弥补干旱期降低的矿化量。在湿润的数小时内,土壤溶解性有机碳含量先升高后降低。干湿交替提升了土壤活性碳库的降解速率,降低了惰性碳库的降解速率,湿润后土壤活性碳库显著增加。多次干湿交替降低了土壤真菌/细菌比,使土壤微生物群落结构发生变化,细菌成为优势种群。     

鄂尔多斯高原脉冲降雨对油蒿灌丛群落土壤碳排放的影响

Precipitation is the major driver of ecosystem functions and processes in semiarid and arid regions. In such water-limited ecosystems, pulsed water inputs directly control the belowground processes through a series of soil drying and rewetting cycles. To investigate the effects of sporadic addition of water on soil CO₂ efflux, an artificial precipitation event (3 mm) was applied to a desert shrub ecosystem in the Mu Us Sand Land of the Ordos Plateau in China. Soil respiration rate increased 2.8-4.1 times immediately after adding water in the field, and then it returned to background level within 48 h. During the experiment, soil CO₂ production was between 2 047.0 and 7 383.0 mg m^-2. In the shrubland, soil respiration responses showed spatial variations, having stronger pulse effects beneath the shrubs than in the interplant spaces. The spatial variation of the soil respiration responses was closely related with the heterogeneity of soil substrate availability. Apart from precipitation, soil organic carbon and total nitrogen pool were also identified as determinants of soil CO₂ loss in desert ecosystems.     

Prior exposure to diurnal heating influences soil respiration and N availability upon rewetting

On sunny summer days, the top 10 cm of soil in southern Australia are heated to temperatures between 50 and 80 °C for a few hours a day, often for several successive days. These extreme temperature events are likely to have profound effects on the microbiota in these soils, but we do not know how this recurrent heat exposure influences microbial dynamics and associated nutrient cycling. In this study, an air-dry soil from southern Australia was exposed to one or two diurnal heating events with maximum temperature of 50 or 70 °C. The control was left at ambient temperature (Amb). All soils were rapidly rewet. Soil respiration was measured for 7 days after rewetting; microbial biomass C, available N and P were determined before rewetting and 1 and 7 days after rewetting. After heating and before rewetting compared to Amb, microbial biomass C (MBC) was 50–80% lower, but available P was 25% higher in heated soils. Available N differed little between Amb and heated soils. Rewetting resulted in a flush of respiration in Amb and soils heated once, but there was no respiration flush in soils heated twice. Cumulative respiration compared to Amb was about 10% higher in soils heated once and about 25% lower in soils heated twice. In Amb, MBC 1 day after rewetting was similar as before rewetting. But in heated soils, MBC increased from before rewetting to 1 day after rewetting about fourfold. Compared to Amb, available N 1 day after rewetting was 20–30% higher in soils heated to 70 °C. Seven days after rewetting, available N was 10% higher than Amb only in soils heated twice to 70 °C. It can be concluded that diurnal heating kills a large proportion of the microbial biomass and influences soil respiration and nutrient availability after rewetting of soils. The effect of heating depends on both maximum temperature and number of events.     

Soil CO2 evolution: Response from arginine additions

Short-term response of soil C mineralization following drying/rewetting has been proposed as an indicator of soil microbial activity. Houston Black clay was amended with four rates of arginine to vary microbial responses and keep other soil properties constant. The evolution of CO₂ during 1 and 3 days following rewetting of dried soil was highly related to CO₂ evolution during 10 days following chloroform fumigation (r² = 0.92 and 0.93, respectively) which is a widely used method for soil microbial biomass C, which disrupts cellular membranes. This study suggest that the release of CO₂ following rewetting of dried soil with no amendments other than heat and water can be highly indicative of soil microbial activity and possibly be used as a quantitative measurement of soil biological quality in Houston Black soils.     

Response of microbial community composition and activity in agricultural and grassland soils after a simulated rainfall

Rainfall in Mediterranean climates may affect soil microbial processes and communities differently in agricultural vs. grassland soils. We explored the hypothesis that land use intensification decreases the resistance of microbial community composition and activity to perturbation. Soil carbon (C) and nitrogen (N) dynamics and microbial responses to a simulated Spring rainfall were measured in grassland and agricultural ecosystems. The California ecosystems consisted of two paired sets: annual vegetable crops and annual grassland in Salinas Valley, and perennial grass agriculture and native perennial grassland in Carmel Valley. Soil types of the respective ecosystem pairs were derived from granitic parent material and had sandy loam textures. Intact cores (30 cm deep) were collected in March 1999. After equilibration, dry soil cores (approx. −1 to −2 MPa) were exposed to a simulated Spring rainfall of 2.4 cm, and then were measured at 0, 6, 24, and 120 h after rewetting. Microbial biomass C (MBC) and inorganic N did not respond to rewetting. N₂O and CO₂ efflux and respiration increased after rewetting in all soils, with larger responses in the grassland than in the agricultural soils. Phospholipid fatty acid (PLFA) profiles indicated that changes in microbial community composition after rewetting were most pronounced in intensive vegetable production, followed by the relict perennial grassland. Changes in specific PLFA markers were not consistent across all sites. There were more similarities among microbial groups associated with PLFA markers in agricultural ecosystems than grassland ecosystems. Differences in responses of microbial communities may be related to the different plant species composition of the grasslands. Agricultural intensification appeared to decrease microbial diversity, as estimated from numbers of individual PLFA identified for each ecosystem, and reduce resistance to change in microbial community composition after rewetting. In the agricultural systems, reductions in both the measures of microbial diversity and the resistance of the microbial community composition to change after a perturbation were associated with lower ecosystem function, i.e. lower microbial responses to increased moisture availability.     

Addition of a clay subsoil to a sandy topsoil changes the response of microbial activity to drying and rewetting after residue addition – a model experiment

The effect of drying and rewetting (DRW) on C mineralization has been studied extensively but mostly in absence of freshly added residues. But in agricultural soils large amounts of residues can be present after harvest; therefore, the impact of DRW in soil after residue addition is of interest. Further, sandy soils may be ameliorated by adding clay‐rich subsoil which could change the response of microbes to DRW. The aim of this study was to investigate the effect of DRW on microbial activity and growth in soils that were modified by mixing clay subsoil into sandy top soil and wheat residues were added. We conducted an incubation experiment by mixing finely ground wheat residue (20 g kg^–1) into top loamy sand soil with clay‐rich subsoil at 0, 5, 10, 20, 30, and 40% (w/w). At each clay addition rate, two moisture treatments were imposed: constantly moist control (CM) at 75% WHC or dry and rewet. Soil respiration was measured continuously, and microbial biomass C (MBC) was determined on day 5 (before drying), when the soil was dried, after 5 d dry, and 5 d after rewetting. In the constantly moist treatment, increasing addition rate of clay subsoil decreased cumulative respiration per g soil, but had no effect on cumulative respiration per g total organic C (TOC), indicating that the lower respiration with clay subsoil was due to the low TOC content of the sand‐clay mixes. Clay subsoil addition did not affect the MBC concentration per g TOC but reduced the concentration of K₂SO₄ extractable C per g TOC. In the DRW treatment, cumulative respiration per g TOC during the dry phase increased with increasing clay subsoil addition rate. Rewetting of dry soil caused a flush of respiration in all soils but cumulative respiration at the end of the experiment remained lower than in the constantly moist soils. Respiration rates after rewetting were higher than at the corresponding days in constantly moist soils only at clay subsoil addition rates of 20 to 40%. We conclude that in presence of residues, addition of clay subsoil to a sandy top soil improves microbial activity during the dry phase and upon rewetting but has little effect on microbial biomass.