Mineralisation dans le sol de materiaux microbiens marques au carbone 14 et a l'azote 15: Quantification de l'azote de la biomasse microbienne

The mineralization of microbial material of different C-to-N ratios (5.2, 7.9, 10.2, 12.7) was followed in fumigated soil. The microbial materials used were from Aspergillus flavus cultures, grown in liquid media and labelled with [¹⁴C]glucose and (¹⁵NN4)3804. Three contrasting soils were used and the microbial materials incubated with the fumigated soils for 28 days at 28°C.The evolution of the added organic microbial C was fast: 80% of the [¹⁴C]CO₂ produced during the whole 28 days incubation was evolved in the first week. Microbial C mineralization was mainly related to soil type; the C-to-N ratio had small effect on the ratio (mineralized microbial carbon-to-added microbial carbon). Calculation of the K_c- coefficient (the fraction of the added microbial C mineralized in 7 days) shows that K_c values lie between 0.38 and 0.43 in the 3 soils.Organic N in the added microbial material also breaks down quickly: between 60 and 100% of the organic nitrogen mineralized was evolved during the first week of incubation. Mineralization kinetics are related to soil type and to the C-to-N ratio of the microbial material.The proportion of N mineralized in 7 days was lower in an acid soil than in near neutral soils and lower with high C-to-N ratio material than with low C-to-N ratio material. The ratio (mineralized microbial N-to-added microbial N) depends on soil type and is negatively correlated with the C-to-N ratio of the microbial material. The K_N value (the fraction of the added microbial N mineralized in 7 days) lies between 0.22 and 0.47 for the three soils and four materials investigated. The added microbial material induced a priming effect on soil native N: materials with C-to-N ratios of 10.2 and 12.7 produced negative priming effects whereas materials with C-to-N ratios of 5.2 and 7.9 sometimes produced a positive priming action.From the relationship between the C-to-N ratio of the added material and the (mineralized microbial C-to-mineralized microbial N) ratio, the soil native microbial biomass was estimated using the fiush-C-to-flush-N ratio. Biomass nitrogen was then calculated from the formula biomass-N = biomassC/(biomass C-to-N ratio). Calculated in this way, 2–4% of the total nitrogen in the three soils was in microbial biomass.     

STUDIES ON THE DECOMPOSITION OF PLANT MATERIAL IN SOIL

Soil samples taken during an experiment on the decomposition of ¹⁴C-labelled ryegrass in soil under field conditions (see Part I) were air-dried, irradiated, exposed to CHCl₃ or CH₃Br vapours, oven-dried or autoclaved. After these treatments the soils were inoculated, incubated, and the output of CO₂ measured. All these methods of partially (or, in some cases, completely) sterilizing soil rendered a small heavily labelled fraction of the soil organic matter decomposable. This fraction is postulated to be the soil biomass. Treatments involving heat or irradiation rendered small additional amounts of the soil organic matter decomposable (by processes other than the killing of organisms). Incubating unsterilized soil with partially sterilized soil did not decrease evolution of CO₂. This suggests that partial sterilization does not increase mineralization by destroying toxic substances that inhibit microbial growth, or by disturbing a host: predator balance in the unsterilized soil. The longer the labelled ryegrass was allowed to decompose in the field, the less labelled-CO₂ was evolved after partial sterilization. In contrast, the same amount of unlabelled-CO₂ was evolved from a soil that had been incubated 1 or 4 years with ryegrass. The labelled part of the biomass is considered to be largely zymogenic (with a half life of approximately 1.5 years), the unlabelled part largely autochthonous, remaining almost constant over the 3-year period. It is suggested that the size of the soil biomass can be roughly estimated from the size of the flush of CO₂ after CHCl₃ vapour treatment. Calculated on this basis, 2.3–3.5 Per cent the unlabelled-C in these soils (i.e. the C present in the soil before the labelled ryegrass was added) was in the biomass. Of the original ryegrass C added, 10–12 per cent was in the biomass after 1 year, decreasing to 4 per cent after 4 years.     

Chloroform fumigation and the release of soil nitrogen: A rapid direct extraction method to measure microbial biomass nitrogen in soil

A new “direct extraction” method for measuring soil microbial biomass nitrogen (biomass N) is described. The new method (fumigation-extraction) is based on CHC1₃ fumigation, followed by immediate extraction with 0.5 M K₂SO₄ and measurement of total N released by CHC1₃ in the soil extracts. The amounts of NH₄-N and total N extracted by K₂SO₄ immediately after fumigation increased with fumigation time up to 5 days. Total N released by CHC1₃ after 1 day fumigation (1 day CHC1₃-N) and after 5 days fumigation (5 day CHC1₃-N) were positively correlated with the flush of mineral N (F_N) in 37 soils that had been fumigated, the fumigant removed and the soils incubated for 10 days (fumigation-incubation). The regression equations were 1 day CHC1₃-N = (0.79 ± 0.022) F_N and 5 day CHC1₃-N = (1.01 ± 0.027) F_N, both regressions accounting for 92% of the variance in the data.In field soils previously treated with ¹⁵N-labelled fertilizer, the amounts of labelled N, measured after fumigation-extraction, were very similar to the amounts of labelled N mineralized during fumigation-incubation; both were about 4 times as heavily labelled as the soil N as a whole. These results suggest that fumigation-extraction and fumigation-incubation both measure the same fraction of the soil organic N (probably the cytoplasmic component of the soil microbial biomass) and that measurement of the total N released by CHC1₃ fumigation for 24 h provides a rapid method for measuring biomass N.     

Chemical fixation of ammonia to soil organic matter after application of urea

Chemical fixation of NH₃ to soil organic matter was studied in two Swedish soils with different contents of organic matter: a clay soil with 2.3% C and an organic soil with 36.6% C. ¹⁵N‐labelled urea was applied at different rates to both sterilized and non‐sterilized soils. After 10 days, the soils were extracted and washed with K₂SO₄ and determined for total N and atom% ¹⁵N excess. Urea N was recovered as non‐extractable N in sterilized soil corresponding to 9.7% of supplied ^l5N‐labelled urea in the organic soil and 2.2% in the clay soil. Since no biological immobilization is thought to occur in the sterile soil, this non‐extractable N is suggested to be chemically fixed to soil organic matter. Owing to urea hydrolysis in the clay soil, pH increased from 6.3 to 9.3 and in the organic soil from 5.7 to 6.9 and 8.8, respectively, at the low and high urea supply.     

Response of microbial biomass to alternate moist and dry conditions in a soil incubated with 14C- and 15N-labelled plant material

A red mediterranean soil was incubated for 1.5 yr, with ¹⁴C- and ¹⁵N-labelled plant material under constant temperature and moisture conditions. Then a portion of the soil was submitted to 4 rapid drying (at 40°C) and rewetting cycles. The duration of the dry periods ranged from 8 to 10 days and the wet periods from 15 to 20 days. Another portion of the soil was incubated under continuously moist conditions. At the end of each dry and moist period, biomass-C and -N were estimated, using the chloroform fumigation technique. The portion of biomass killed on drying and that restored after rewetting were calculated, by the difference between the sizes of biomass present after the dry and the moist periods.Soil drying destroyed $\text{1}\text{3}$ to $\text{1}\text{4}$ of biomass and at each cycle, after remoistening, the biomass was progressively restored to approximately the same size as before drying.The labelled-C to total-C ratio of the CO₂ released from undisturbed and continuously moist soil, ranged from 6 to 7%. In biomass, which survived the drying, the values ranged from 20 to 22%, whereas in the killed biomass they ranged between 7 and 8%, i.e. the same orders of magnitude as that of CO₂ evolved from undisturbed soil.A comparison of the labelled-C to total-C ratio of (1) CO₂C released from undisturbed and continuously moist soil, (2) the extra CO₂-C evolved as a result of alternate drying-remoistening conditions, (3) CO₂C released from the soil at the end of moist periods, (4) the C of microbial biomass which survived the drying, and (5) the C of the biomass present at the end of the moist periods, revealed that the calculated portion of biomass killed on drying essentially corresponded to a still relatively “active” fraction of biomass and that the biomass surviving rapid drying, essentially corresponded to a dormant and protected fraction.In contrast to the labelled-C to total-C ratio, the labelled-N to total-N ratio, in the fraction of biomass which was destroyed on drying, was not different from that of the surviving fraction. During incubation, labelled nitrates accumulated progressively in soil; transformations of N were probably affected by a remetabolization of the nitrates and of material made decomposable on drying, including destroyed microflora and non-biomass material.     

Microbial and soil parameters in relation to N mineralization in soils of diverse genesis under differing management systems

 Oregon soils from various management and genetic histories were used in a greenhouse study to determine the relationships between soil chemical and biological parameters and the uptake of soil mineralized nitrogen (N) by ryegrass (Lolium perenne L.). The soils were tested for asparaginase, amidase, urease, β-glucosidase, and dipeptidase activities and fluorescein diacetate hydrolysis. Microbial biomass carbon (C) and N as well as metabolic diversity using Biolog GN plates were measured, as were total soil N and C, pH, and absorbance of soil extracts at 270 nm and 210 nm. Potentially mineralizable N (N₀) and the mineralization rate constant (k) were calculated using a first order nonlinear regression model and these coefficients were used to calculate the initial potential rate of N mineralization (N₀ k). Except for Biolog GN plates, the other parameters were highly correlated to mineralized N uptake and each other. A model using total soil N and β-glucosidase as parameters provided the best predictor of mineralized N uptake by ryegrass (R ² =0.83). Chemical and biological parameters of soils with the same history of formation but under different management systems differed significantly from each other in most cases. The calculated values of the initial potential rate of mineralization in some cases revealed management differences within the same soil types. The results showed that management of soils is readily reflected in certain soil chemical and biological indicators and that some biological tests may be useful in predicting N mineralization in soils. Received: 31 January 1997     

Physical factors influencing decomposition of organic materials in soil aggregates

Glucose or starch labelled with ¹⁴C was mixed thoroughly into slurried soils. Aggregates of different sizes were obtained from the soils as they dried. The labelled substrates were considered to be distributed in both micro- and macropores in the aggregates. Control samples (labelled substrates in macropores only) were prepared by adding the labelled carbohydrates after the formation of the aggregates. The various samples were sterilized by γ-irradiation and stored at ?15°C.Samples were wetted to about ?20kPa, inoculated with soil organisms, and incubated for 4 weeks at 28°C in closed systems, which enabled regular measurement of ¹⁴CO₂ released.Based on the ¹⁴CO₂ released, it was concluded that starch was protected from microbial attack when present in micropores in aggregates made from fine sandy loam.After incubation samples were dried and rewetted. The flush of ¹⁴CO₂ released was twice as big for samples containing labelled starch compared with glucose, showing that disruption of aggregates, containing residual starch, and rearrangements of soil components are as important as chemical and biological factors in causing the flush of CO₂ resulting from wetting a soil. Mechanical disruption of the aggregates resulted in a similar flush of ¹⁴CO₂.     

Carbon-nitrogen relationships during the humification of cellulose in soils containing different amounts of clay

¹⁴C-labelled cellulose and ¹⁵N-labelled (NH₄)₂SO₄ were added to four soils with clay contents of 4, 11, 18 and 34%, respectively. Labelled cellulose was added to each soil in amounts corresponding to 1, 2 and 4 mg C g^?1 soil, respectively, and labelled NH₄⁺ at the rate of 1 mg N per 25 mg labelled C.After the first month of incubation at temperatures of 10, 20 and 30°C, respectively, from 38 to 65% of the labelled C added in cellulose had disappeared from the soils as CO₂, and from 60 to nearly 100% of the labelled N added as NH₄⁺ were incorporated into organic forms. The ratio of labelled C remaining in the soils to labelled N in organic forms was close to 25 after 10 days of incubation, decreasing to about 15 after 1 month and about 10 after 4 yr.The retention of total labelled C was largest in the soil with the highest content of clay where after 4 yr it was 25% of that added, compared to 12 in the soil with the lowest content of clay. The incorporation of labelled N in organic forms and its retention in these forms was not directly related to the content of clay in the soils, presumably because the two soils with the high content of clay had a relatively high content of available unlabelled soil-N which was used for synthesis of metabolic material.The proportionate retention of labelled C for a given soil was largely independent of the size of the amendments, whereas the proportionate amount of labelled N incorporated into organic forms increased in the clay-rich soils with increasing size of amendments. Presumably this is because the dilution with unlabelled soil-N was less with the large amendments.From 50 to 70% of the total labelled C remaining in the soils after the first month of incubation was acid hydrolyzable, as compared to 80–100% of the total remaining labelled organic N. This relationship held throughout the incubation and was independent of the size of the amendment and of the temperature of incubation.During the second, third and fourth year of incubation the half-life of labelled amino acid-N in the soils was longer than the half-life of labelled amino acid-C, presumably due to immobilization reactions. Some of the labelled organic N when mineralized was re-incorporated into organic compounds containing increasing proportions of native soil-C. whereas labelled C when mineralized as CO₂ disappeared from the soils.In general, native C and native organic N were less acid hydrolyzable and were accounted for less in amino acid form than labelled C and N.The amount of labelled amino acid-C, formed during decomposition of the labelled cellulose, and retained in the soil, was proportional to the clay content. This amount was about three times as large in the soil with the highest content of clay as in the soil with the lowest content. This difference between the soils was established during the first 10 days of incubation when biological activity was most intense, and it held throughout the 4 yr of incubation; proportionally it was independent of the amount of cellulose added and the temperature.In contrast, the labelled amino acid-N content was not directly related to the amount of clay in the soil, presumably because more unlabelled soil-N was available for synthesis of metabolic material in the two clay-rich soils than in those soils with less clay. The wider ratio between labelled amino acid-C and labelled amino acid-N in the two clay-rich soils as compared with those obtained with the soils with less clay indicates this.The effect of clay in increasing the content of organic matter in soil is possibly caused by newly synthesized matter, extracellular metabolites, as well as cellular material, forming biostable complexes and aggregates with clay. The higher the concentration of clay the more readily the interactions take place. The presence of clay may also increase the efficiency of using substrate for synthesis.     

Studies of nitrogen immobilization and mineralization in calcareous soils—II: Mineralization of immobilized nitrogen from soil fractions of different particle size and density

¹⁵NO^?₃ was immobilized in a calcareous sandy soil and a calcareous clay soil each incubated with glucose and wheat straw. Net mineralization of organic-¹⁵N was more rapid in the sandy soil, irrespective of C amendment, and in soils amended with glucose. Intermittent drying and wetting of soils during incubation stimulated mineralization of ¹⁵N-labelled and native soil organic-N in all treatments. The availability (percentage mineralization) of recently-immobilized ¹⁵N consistently exceeded that of the native soil N. Ratios of the availability of labelled and unlabelled N were similar in the sandy and clay soils but varied according to C amendment, drying and wetting cycle and incubation period.Changes in the distribution of immobilized N amongst soil extracts and soil fractions of different particle size and density were determined during periods of net N mineralization. In straw-amended soils, the organic-¹⁵N of a light fraction, sp.gr. < 1.59, decomposed relatively rapidly during the late mineralization period. Decreases of organic ¹⁵N of the fine clay fraction were also recorded. In glucose-amended soils, net N mineralization was accompanied by significant decreases in the concentrations of organic-¹⁵N of the silt and fine clay fractions.Drying and rewetting of soils hastened or magnified changes occurring in the organic-¹⁵N of soil fractions, but qualitatively, the pattern of change was similar to that observed with soils incubated under uniformly-moist conditions.The percentage distribution of labelled and unlabelled N suggested that in the long term, the silt fraction will accumulate an increasing proportion of the more stable nitrogenous residues.     

Nitrogen in particle size fractions of soils incubated for five years with 15N-ammonium and 14C-hemicellulose

Four soils with a range of clay and silt contents were incubated for 5 a with ¹⁵N-labelled (NH₄)SO₄ and ¹⁴C-labelled hemicellulose and then fractionated according to particle size by ultrasonic dispersion and sedimentation. The distribution of labelled and native N between clay, silt and sand fractions was determined and elated to previous results on the C distributions. Between 29% and 48% of the added N was found in organic form. The ¹⁵N atom percentage excess decreased in the order: clay > whole soil > silt > sand. For both clay and silt, the enrichment factor for labelled and native N decreased with increasing fraction weight. Clay enrichment was higher for labelled than for native N, the converse being true for silt. The distribution of whole soil labelled organic N was: clay 77–91%, silt 4–11%, and sand <0.5%. Corresponding values for native N were 69–74%, 16–22%, and 1–2%, respectively. All soils had higher proportions of labelled than of native N in the clay, the converse was true for the silt. The C/N ratio of the native silt organic matter was higher and that of clay organic matter lower than whole soil C/N ratios. Differences between the C/N ratio distributions of native and labelled organic matter were small. The relative distribution of labelled N and C was very similar confirming that the turnover of C and N in soil organic matter is closely interrelated.     

Degradation and humification of maize straw in soil microcosms inoculated with simple and complex microbial communities

Microbial communities are responsible for soil organic matter cycling and thus for maintaining soil fertility. A typical Orthic Luvisol was freed from organic carbon by thermal destruction at 600°C. Then the degradation and humification of ¹⁴C‐labelled maize straw by defined microbial communities was analysed. To study the role of microbial diversity on the humification of plant material, microcosms containing sterilized soil were inoculated with a natural microbial community or with microbial consortia consisting of bacterial and fungal soil isolates. Within 6 weeks, 41 ± 4% of applied ¹⁴C‐labelled maize straw was mineralized in the soil microcosms containing complex communities derived from a soil suspension, whilst the most efficient communities composed of soil isolates mineralized less than 35%. The humification products were analysed by solution state ¹³C‐NMR‐spectroscopy and gel permeation chromatography (GPC). The analyses of humic acids extracts by solution state ¹³C‐NMR‐spectroscopy revealed no difference in the development of typical chemical functional groups for humic substances during incubation. However, the increase in specific molecular size fractions of the extracted humic acids occurred only after inoculation with complex communities, but not with defined isolates. While it seems to be true that redundancy in soil microbial communities contributes to the resilience of soils, specific soil functions may no longer be performed if a microbial community is harshly affected in its diversity or growth conditions.     

Decomposition of straw in soil after stepwise repeated additions

Samples of a sandy soil, which had been incubated for 8 years in the field with [¹⁴C]labelled barley straw, were amended with 1, 2, 3 or 4 successive additions of [¹⁴C]labelled straw, respectively, applied at intervals of 3 months. The decomposition of the straw was studied over a 4-yr period of laboratory incubation, following the first repeated application, by determination of the total amount of labelled C in the soils and labelled C in the soil amino acids. The overall pattern of decomposition was similar whether the soil was amended with one or with several successive applications.Four years after the first repeated addition of labelled straw the soils were subjected to a number of “stress” treatments: addition of unlabelled glucose, air-drying, oven-drying, grinding and fumigation with vapour of chloroform, respectively. The CO₂ that developed during the first 10 days after the treatments, less the evolution from untreated samples, was taken as a measure of the effect of the treatments. The amount of biomass in the soils was calculated from the increase caused by the fumigation with chloroform. In soil incubated undisturbed in the field for 12 yr, biomass accounted for 2.6% of the labelled C in the soil, whereas it was only half this amount in the soil incubated for 8 yr in the field followed by 4 yr in the laboratory. In the soils amended with successive additions of labelled straw, the size of the biomass showed declining values with an increasing number of additions. Biomass thus accounted for 2.6% of the labelled C in the soil amended with one repeated addition, and 1.0% in the soil amended with 4 repeated additions.The increase in the evolution of labelled CO₂-C caused by the stress treatments ranged from 0.3 to 1.7% of the labelled C in the soil: air-drying had the least effect, grinding the most. The effect of each treatment declined with an increasing number of successive additions of straw. The ratio between CO₂ evolved after grinding and fumigation, respectively, revealed that grinding also exposed non-biomass material to accelerated decomposition.The effects of the stress treatments on the evolution of native CO₂-C was on the whole parallel to the effects on the evolution of labelled CO₂-C.     

Mineralization of soil organic nitrogen solubilized by aqua ammonia fertilizer

Organic N solubilized by NH_3(aq) was extracted from ¹⁵N-labelled or unlabelled soil, concentrated and added to non-extracted soil, which was incubated under aerobic conditions at 27±1°C. Gross N mineralization, gross N immobilization, and nitrification in soils with or without addition of unlabelled soluble organic N were estimated by models based on the dilution of the NH ₄ ⁺ or NO _inf3 ^sup- pools, which were labelled with ¹⁵N at the beginning of incubation. Mineralization of labelled organic N was measured by the appearance of label in the mineral N pool. Although gross N mineralization and gross N immobilization were increased in two soils between day 0 and day 7 following addition of unlabelled organic N solubilized by NH_3(aq), there was no increase in net N mineralization. Solubilization of ¹⁵N-labelled organic N increased and the ¹⁵N enrichment of the soluble organic N decereased as the concentration of NH_3(aq) added increased. A constant proportion of approximately one-quarter of the labelled organic N added at different rates to non-extracted soil was recovered in the mineral N pool after an incubation period of 14 days, and the availability ratios calculated from net N mineralization data were 1.1:1 and 2.1:1 for 111 and 186 mg added organic-N kg^-1 soil, respectively, indicating that the mineralization of organic N was increased by solubilization.     

Mineralization of bacteria and fungi in chloroform-fumigated soils

It has been suggested by others that the size of the flush of mineralization caused by CHC1₃ fumigation can be used to estimate the amount of microbial biomass in soils. Calculation of biomass from the flush requires that the proportion of CHCl₃-killed cell C mineralized be known. To determine this proportion, 15 species of [¹⁴C]labelled fungi and 12 species of [¹⁴C]labelled bacteria were added to four types of soil and these were fumigated for 24 h with CHC1₃, reinoculated with unfumigated soil, and incubated at 22°C for 10 days. The average percentage mineralization of the fungi was 43.7 ± 5.3, while the average for the bacteria was 33.3 ± 9.9. Using a 1:3 ratio for distribution of total biomass between the bacterial and fungal populations, respectively, it was calculated that the average mineralization of both types of cells was 41.1%. In experiments conducted to determine if CHC1₃ vapour alters stabilized microbial metabolites or dead microbial cells in a manner which makes them more susceptible to degradation, it was found that both fumigated and unfumigated dead fungal materials mineralized to the same extent in soil during 10 days of incubation.     

FORMATION OF MICROBIAL BIOMASS DURING THE DECOMPOSITION OF 14C LABELLED RYEGRASS IN SOIL

Ryegrass uniformly labelled with ^I4C was incubated aerobically at 25°C for 62 days in two contrasting soils, a near-neutral (pH 6.8) palcudalf from England and a strongly acid (pH 3.6) haplorthox from Brazil. Decomposition of the labelled plant material was faster in the near-neutral soil throughout the whole of the incubation period. In neither soil did the addition of fresh plant material significantly accelerate the evolution of CO₂ from organic matter already in the soil, i.e. there was no priming action. In the near-neutral soil there was a rapid build up of labelled microbial biomass in the first 6 days, followed by a much slower increase that continued throughout the whole incubation period. After 62 days 22.5% of the labelled C remaining in the near-neutral soil was in the biomass. The yield coefficient (the fraction of the incoming plant C converted to microbial C) of this stabilized or ‘resting’ biomass was 0.15. Much less labelled microbial biomass was formed in the acid soil than in the near-neutral soil. By the end of 62 days only 6.2% of the labelled carbon remaining in the acid soil was in the biomass. Biomass C measurements in strongly acid soils must however be treated with caution as the technique used has not yet been adequately validated for such soils.     

Nitrogen Fractions in Arable Soils in Relation to Nitrogen Mineralization and Plant Uptake

Abstract

Nitrogen (N) as a major constituent of all plants is one of the most important nutrients. Minimizing input of mineral nitrogen fertilizer is needed to avoid harm to the environment. Optimal input of mineral nitrogen should take the nitrogen supply of the soil into account. Many different soil tests have been proposed for determining soil nitrogen availability. In this article we present a new approach that is based on the measurement of nitrate, ammonium, and dissolved organic nitrogen (DON) in a 0.01 M CaCl₂ soil extract. Eighteen agricultural soils, differing widely in the availability of nitrogen were used, fertilized and unfertilized. It is shown that the nitrogen uptake by maize plants (Zea Mays L.) in both “N‐fertilized” and “N‐unfertilized” soils as measured in a pot experiment can be described with a simple model using the measured nitrogen fractions in the extract. The main source of nitrogen uptake by the plants is the mineralized organic nitrogen during the growing period. It is shown that the initial measured DON fraction is a good indicator of the nitrogen mineralized during plant growth.     

Effect of pH on nitrogen mineralization in crop-residue-treated soils

Summary This study compares N mineralization in soils treated with crop residues [corn (Zea mays L.), soybean (Glycine max (L.) Merr.), sorghum (Sorghum vulgare Pers.)] or alfalfa (Medicago sativa L.) at three adjusted soil pH values (4, 6, and 8); pH was adjusted with dilute H₂SO₄ or KOH. A sample of soil (20 g) was treated with 0.448 g plant material (equivalent to 50t ha^–1), mixed with 20 g silica sand adjusted to the pH of the soil, and packed in a leaching tube. The soil-sand mixture was leached with 100 ml 5 mM CaCl₂ adjusted to the same pH as that of the treated soil to remove the initial mineral N, and incubated at 30°C. The leaching procedure was repeated every 2 weeks for 20 weeks. Results from three soils showed that N mineralization increased as the soil pH increased. In one soil (Lester soil), significant amounts of NH ₄ ⁺ -N accumulated at pH 4 during the first 12 weeks. Treatment with corn and soybean residues resulted in a marked reduction in N mineralization, especially at pH 4. The percentage of organic N mineralized from sorghum residue and alfalfa added to soils increased as the soil pH increased; the values ranged from 7.7% to 37.0% for sorghum and from 17.2% to 30.1% for alfalfa.     

Mineralization of carbon and nitrogen from fresh and anaerobically stored sheep manure in soils of different texture

A sandy loam soil was mixed with three different amounts of quartz sand and incubated with (¹⁵NH₄)₂SO₄ (60 g N g^-1 soil) and fresh or anaerobically stored sheep manure (60 g g^-1 soil). The mineralization-immobilization of N and the mineralization of C were studied during 84 days of incubation at 20°C. After 7 days, the amount of unlabelled inorganic N in the manure-treated soils was 6–10 g N g^-1 soil higher than in soils amended with only (¹⁵NH₄)₂SO₄. However, due to immobilization of labelled inorganic N, the resulting net mineralization of N from manure was insignificant or slightly negative in the three soil-sand mixtures (100% soil+0% quartz sand; 50% soil+50% quartz sand; 25% soil+75% quartz sand). After 84 days, the cumulative CO₂ evolution and the net mineralization of N from the fresh manure were highest in the soil-sand mixutre with the lowest clay content (4% clay); 28% fo the manure C and 18% of the manure N were net mineralized. There was no significant difference between the soil-sand mixtures containing 8% and 16% clay, in which 24% of the manure C and -1% to 4% of the manure N were net mineralized. The higher net mineralization of N in the soil-sand mixture with the lowest clay content was probably caused by a higher remineralization of immobilized N in this soil-sand mixture. Anaerobic storage of the manure reduced the CO₂ evolution rates from the manure C in the three soil-sand mixtures during the initial weeks of decomposition. However, there was no effect of storage on net mineralization of N at the end of the incubation period. Hence, there was no apparent relationship between net mineralization of manure N and C.     

Arylamidase Activity as an Index of Nitrogen Mineralization in Soils

Abstract

The enzyme arylamidase [EC 3.4.11.2] catalyzes the hydrolysis of N‐terminal amino acids from arylamides. Because it has been proposed that this enzyme may play a major role in nitrogen (N) mineralization in soils, studies were carried out using short‐term laboratory incubations under aerobic and anaerobic conditions and chemical hydrolysis of soil organic N to assess the N mineralization in a range of 51 soils from six agroecological zones of the North Central region of the United States. The enzyme activity was assayed at its optimal pH value. With the exception of the values obtained for field‐moist soils incubated under anaerobic conditions, the amounts of N mineralized by all the biological and chemical methods studied were significantly correlated with arylamidase activity, with r values of 0.54*** for the amounts of inorganic N produced under aerobic incubation, of 0.44** for anaerobic incubation of air‐dried soils, of 0.53*** and 0.55*** for the amounts of ammonium (NH₄ ⁺)‐N released by steam distillation with PO₄‐B₄O₇ for 4 and 8 min, respectively; and of 0.49*** and 0.53*** for the amounts of NH₄ ⁺‐N released by steam distillation with disodium tetraborate (Na₂B₄O₇) for 4 min or 8 min, respectively. The amounts of N extractable with hot potassium chloride (KCl) were most significantly correlated with arylamidase activity (r=0.56***). Arylamidase activity was significantly correlated with organic carbon (C) (r=0.49***), organic N (r=0.55***), and fixed ammonium (NH₄ ⁺)‐N (r =0.42**).     

Kinetics and temperature relationships of mineralization and nitrification in Rothamsted soils with differing histories

Mineralization of soil organic nitrogen measured in laboratory incubation experiments on Rothamsted soils with contrasting histories was most appropriately expressed by the simple zero-order relationship N_t=kt in which N_t is the amount of N mineralized in time t. The rate constants (k) were well related to the absolute temperature by the Arrhenius equation. The approach in which ‘potentially mineralizable N’ (N₀) is mineralized with first-order kinetics could not be applied to these data. When the soils were incubated with added ammonium chloride, the increase in nitrate-N and the decline in ammonium-N were both linear with time, but were equal to each other in only one of the soils. These linear relationships did not reflect true zero-order kinetics because the rates of ammonium-N decline and nitrate-N production both depended on the initial ammonium concentration. The Arrhenius relationships showed no significant difference between mineralization and nitrification in their sensitivity to temperature.