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International Microbiology
Print version ISSN 1139-6709
INT. MICROBIOL. vol.8 n.1 Mar. 2005
REVIEW ARTICLE | |||
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| Soil health-a new challenge for microbiologists and chemists
Summary. Soil health refers to the biological, chemical, and physical features of soil that are essential to long-term, sustainable agricultural productivity with minimal environmental impact. Thus, soil health provides an overall picture of soil functionality. Although it cannot be measured directly, soil health can be inferred by measuring specific soil properties (e.g. organic matter content) and by observing soil status (e.g. fertility). There is also increased interest in studying soil microorganisms in their particular environments, as microbial diversity is intimately related to soil structure and function. One of the key objectives in determining soil health is to acquire indicators that can be used to evaluate the soil's current status and hence to develop sustainable agricultural systems. In this regard, significant progress has been made over the last few years in the development of specific biomarkers and macromolecular probes, enabling rapid and reliable measurements of soil microbial communities. In addition, modern molecular biological techniques, such as fluorescence in situ hybridization (FISH), reverse transcriptase polymerase chain reaction (RT-PCR), denaturing gradient gel electrophoresis (DGGE), and terminal restriction fragment length polymorphism (T-RFLP), have facilitated the analysis of microbial biodiversity and activity, whereas the application of modern analytical techniques, such as nuclear magnetic resonance (NMR) and pyrolysis-gas chromatography-mass spectrometry (Py-GC-MS), have provided data on soil chemistry. The combination of these two approaches offers promise in determining soil health status. [Int Microbiol 2005; 8(1):13-21] Key words: soil health · microbial indicators · chemical indicators · molecular methods · analytical methods | ||
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La salud del suelo-un nuevo reto para microbiólogos y químicos Resumen. El concepto de salud del suelo se relaciona con las características biológicas, químicas y físicas que son esenciales para una productividad agrícola sostenible a largo plazo con un mínimo impacto ambiental. La salud del suelo es el más fiel reflejo de su funcionalidad. Aunque no puede medirse directamente, se puede inferir a partir de la determinación de propiedades específicas del mismo suelo (p.e. el contenido en materia orgánica) y por la observación de su estado (p.e. la fertilidad). El interés por el estudio de los microorganismos del suelo en su propio medio está aumentando, puesto que la diversidad microbiana está estrechamente relacionada con la estructura y función del suelo. Un objetivo clave para determinar la salud de un suelo es la disponibilidad de indicadores factibles de ser utilizados en la evaluación de su estado y, a partir de aquí, implementar sistemas de agricultura sostenible. El desarrollo de biomarcadores específicos y sondas macromoleculares ha evolucionado considerablemente en los últimos años, lo cual ha permitido obtener medidas fiables y rápidas de las comunidades microbianas del suelo. Por otro lado, las modernas técnicas biomoleculares más recientes (p.e. la hibridación in situ mediante fluorescencia [FISH], la reacción en cadena de la polimerasa mediante transcriptasa inversa [RT-PCR], la electroforesis en gel con gradiente desnaturalizante [DGGE] y el análisis del polimorfismo en la longitud de los fragmentos de restricción terminales [T-RFLP]) permiten analizar la biodiversidad y actividad microbianas, mientras que la aplicación de técnicas analíticas modernas (p.e. resonancia magnética nuclear [NMR], pirólisis-cromatografía de gases-espectrometría de masas [Py-GC-MS]) proporciona datos sobre la química del suelo. La combinación de estas dos aproximaciones metodológicas ofrece buenas perspectivas en la determinación del estado de salud del suelo. [Int Microbiol 2005; 8(1):13-21] Palabras clave: salud del suelo · indicadores microbianos · indicadores químicos · métodos moleculares · métodos analíticos | A saúde do solo-um novo desafio para microbiologistas e químicos Resumo. O conceito de saúde do solo relaciona-se com suas características biológicas, químicas e físicas, essenciais para uma produtividade agrícola sustentável a longo prazo, com um mínimo de impacto ambiental. A saúde do solo é o mais fiel reflexo de sua funcionalidade. Ainda que não se possa medir diretamente, se pode inferir a partir da determinação das propriedades específicas do mesmo solo (p.e. o conteúdo da matéria orgânica) e pela observação de seu estado (p.e. a fertilidade). O interesse pelo estudo dos microrganismos do solo em seu meio está aumentando, uma vez que a diversidade microbiana está estreitamente relacionada com a estrutura e função do solo. Um dos objetivos chave para se determinar a saúde do solo é a disponibilidade de indicadores factíveis de serem utilizados na avaliação de seu estado e a partir daí implementar sistemas de agricultura sustentável. O desenvolvimento de biomarcadores específicos e sondas macromoleculares têm evoluído consideravelmente nos últimos anos, e através deles se pode obter medidas confiáveis e rápidas das comunidades microbianas do solo. Por outro lado, as modernas técnicas biomoleculares mais recentes (p.e. a hibridação in situ mediante fluorescência [FISH], a reação em cadeia da polimerase mediante transcriptase inversa [RT-PCR], a eletroforese em gel com gradiente desnaturalizante [DGGE] e a análise do polimorfismo no comprimento dos fragmentos de restrição terminais [T-RFLP]) permitem analisar a biodiversidade e a atividade microbiana, enquanto a aplicação de técnicas analíticas modernas (p.e. ressonância magnética nuclear [NMR], pirólise-cromatográfica de gases-espectrometria de massa [Py-GC-MS]) proporcionam dados sobre a química do solo. A combinação dessas duas abordagens oferece boas perspectivas na determinação do estado da saúde do solo. [Int Microbiol 2005; 8(1):13-21] Palavras chave: saúde do solo · indicadores microbianos · indicadores químicos · métodos moleculares · métodos analíticos |
Introduction
Soil represents the largest carbon pool on the Earth's surface (2157-2293 Pg), the amount of this element being twice as high in soil as in the atmosphere and two or three times larger than the amount in all living matter [6,48]. Because of the large quantity of C stored in soils, small modifications in soil C status may have a significant effect on the global C balance and therefore on climate change [31]. Soils contain an intricate network of plants and microbes in a heterogeneous solid medium in which chemical and physical conditions vary at the scale of the molecule and the cell. It is therefore difficult to understand the variations in soils in the absence of knowledge derived from both chemical and biological approaches, because microorganisms affect the environment and vice versa. Despite their small volume, soil microorganisms are key players in the global cycling of organic matter, reworking organic residues or mineralizing them to CO2, H2O, nitrogen, phosphorus, sulfur, and other nutrients [12]. Nutrients immobilized in microbial biomass are subsequently released when microbes are grazed by microbivores such as protozoa and nematodes. The purpose of this article is to give a current, multidisciplinary view of the study of soil health, with a brief description of the chemical and biological techniques now being used to analyze soil composition. We summarize current knowledge about the biological and chemical indicators of soil health, with particular emphasis on the classical and molecular techniques most widely used for its assessment.
Soil organic matter
Soil organic matter (SOM) can be seen as a mixture of biogenic components that include, in variable proportions and evolutionary stages, microorganisms and non-decomposed plant materials (1-10%). Depending on the turnover time in soil, SOM can be either active (fast recycling, corresponding mainly to carbohydrate, amino acid, and lipid fractions), remaining in the soil for months or even decades (10-40%), or passive or refractory (humic fraction), remaining in the soil for centuries to millennia (40-60%) [7]. SOM has taken on new significance because it correlates well with a number of important physical, chemical, and microbiological properties of soil. The SOM content of agricultural topsoil, for example, is usually in the range of 0.1-6%. From a qualitative point of view, SOM influences the physical and chemical properties of soil as well as the availability of nutrients for microbial and plant growth. It accumulates over long periods of time and its current distribution in a soil profile is the result of continuous reprocessing by microbes, recombination by chemical reactions, physical movement by soil animals, disturbances such as tree falls, and movement of the soil solution. Consequently, carbon cycling and its stabilization in soils are intimately associated with soil structure [40].
Intensive agriculture is practiced in many countries with adverse consequences on biodiversity and SOM status. Changes in the nutrient status of the soil, such as a decrease in the organic matter content, directly affect its microbial biodiversity. Some of the more resilient soils are found in grassland pastures, where bacteria are associated with root material and are attached to clay particles [43]. In well-drained soil sustained by a healthy bacterial microbiota, much of the space between soil aggregates is filled with air, which is necessary for soil productivity. Knowledge of the biodiversity of microbes in soil is therefore essential to maintaining agricultural productivity [19].
Biological indicators used for determining soil health, and standard analytical procedures
The concept of soil health refers to the biological, chemical, and physical features necessary for long-term, sustainable agricultural productivity with minimal environmental impact. Thus, soil health provides an overall picture of soil functionality. Healthy soils maintain a diverse community of soil organisms that help to: (i) control plant diseases as well as insect and weed pests; (ii) form beneficial symbiotic associations with plant roots (e.g. nitrogen-fixing bacteria and mycorrhizal fungi; (iii) recycle plant nutrients; (iv) improve soil structure with positive repercussions for its water- and nutrient-holding capacity; (v) improve crop production. One of the most important objectives in assessing the health of a soil is the establishment of indicators for evaluating its current status. These indicators are listed in Table 1, and several of them are discussed below.
Microbial biomass. Both direct and indirect methods have been used for the estimation of microbial biomass in the soil. Direct counting includes the use of staining techniques in conjunction with epifluorescence microscopy or automated image analysis [10,11]. The most common indirect methods are chloroform fumigation and substrate-induced respiration (SIR) [17]. In chloroform fumigation, the chloroform vapors kill the microorganisms in the soil and the size of the killed biomass is estimated either by quantification of respired CO2 (CFI) or by direct extraction of the soil immediately after the fumigation, followed by quantification of extractable carbon (CFE) (ISO-standard 14240-2:1997). SIR (ISO standard 14240-1:1997) measures the metabolically active portion of the microbial biomass by measuring the initial change in the soil respiration rate as a result of adding an easily decomposable substrate (e.g. glucose) [3]. Soil microbial biomass is subsequently calculated using a conversion factor [37].
Soil respiration is the biological oxidation of organic matter to CO2 by aerobic organisms, notably microorganisms [1]. It is positively correlated with SOM content, and often with microbial biomass and microbial activity, and can be determined as CO2 or O2 production using chemical titration, electrical conductivity, gas chromatography, or infrared spectroscopy [1]. The metabolic quotient (qCO2), also called the specific respiratory rate, is defined as the microbial respiration rate per unit microbial biomass [4].
Phospholipid fatty acids. Most soil microorganisms cannot be characterized by conventional cultivation techniques; indeed, it has been estimated that 80-99% of all species have not yet been cultured. Currently, the analysis of phospholipid fatty acids (PLFA), essential membrane components present in living organisms, can be used to overcome this limitation, thereby providing information on the trophic structure (at the phenotypic level) of microbial communities. The use of PLFA patterns for the characterization of microbial communities in soil has been reviewed by Zelles [60]. In general, PLFA analysis is a fast, reliable method for the detection of changes in the structure of soil microbial communities [27], and the variations detected can be related to changes in soil use and management [13].
Microbial activity
Measurements of microbial activity at the community level include the quantification of bacterial DNA and protein synthesis. The amount of DNA synthesis can be determined by measuring the incorporation of 3H- or 14C-thymidine into bacterial DNA [5]. Similarly, the amount of incorporation of 3H- or 14C-leucine, an amino acid that is incorporated only into proteins, reflects the level of bacterial protein synthesis [5].
There are a number of key indicators related to microbial activity, and some can be used to estimate both biomass and activity (e.g. soil respiration and the microbial quotient). Indicators of carbon cycling measure activity at the ecosystem level. For example, organic matter decomposition can be estimated using either litter bags [57], cotton strips, or wood sticks [34]. The information provided by each of these tests allows comparisons of the decomposition rates of different sites and ecosystems and at different times. In addition, well-documented assays are available for many soil-enzyme activities (e.g. cellulase, urease, phosphatase, and phenol oxidase) [20]. The mineralization of soil organic nitrogen through nitrate to gaseous nitrogen by soil microorganisms is a major component of global nitrogen cycling (Fig. 1). Therefore, measuring the activities of enzymes involved in these processes (e.g. urease) is an important aspect of determining overall microbial activity.
Microbial biodiversity and resilience
As in other well-studied ecosystems, the resilience of the soil is associated with biodiversity such that increasing the microbial diversity of the soil increases its resilience capacity. Thus, the aim of isolating viable microorganisms in soil is to estimate not only their numbers but also the diversity of the isolates. To do this, a medium satisfying the nutritional requirements of as many microorganisms in the soil as possible is required. The functional diversity of microbial populations in soils may be determined by measuring the expression of different enzymes, e.g. with respect to carbon utilization patterns [59]. Another aspect of soil biodiversity, soil suppressiveness, is an indicator of the capacity of soils to suppress specific plant pathogens through inherent biotic and abiotic factors [21]. Several methods are available for determining soil suppressiveness, including the inoculation of target plants seeds directly into the test soil or into a pathogen-infested test soil [14].
Bioavailability of environmental contaminants
Microorganisms can be used to determine the bioavailability of a given chemical compound in soil. Specifically, measurement of plasmid-containing bacteria, using either an endogenous or exogenous approach, serves as a general indicator of environmental contaminants. In the endogenous approach, plasmids are extracted from soil bacteria isolated on agar plates [16]. In the exogenous approach, a soil sample is mixed with plasmid-free bacteria, which, by conjugation, subsequently acquire naturally occurring plasmids from the soil bacteria [53]. If the number of plasmids is found to have increased at a given site, an investigation of the responsible stress factor can be initiated. Similarly, monitoring of antibiotic-resistant bacteria in soil can be used as an indicator of industrial and urban pollution.
Soil physical and chemical indicators
Among the variables proposed to assess soil health, physical indicators are of prime importance [22,56]. However, their site-specific interpretation with respect to soil quality will, in many instances, depend on specific land use and crop tolerance.
Water infiltration rate. Infiltration rates are subject to significant changes with soil use, management, and time. They are affected by the development of plant roots, earthworm burrows, soil aggregation, and overall increases in stable organic matter. Depending on the soil type, texture, structure, and soil water content, the water infiltration rate may improve immediately after tillage due to the loosening of surface crusts or compacted areas. Nonetheless, tillage also disrupts aggregates and soil structure, creating the potential for renewed compaction and surface crusting, and leading to a loss of continuous surface-connected pores.
Bulk density. Defined as the ratio of oven-dried soil (weight) to its bulk volume, soil bulk densities range, in general, from < 1.0 (in organic soils) to 1.7 g cm-3 and are dependent on the densities of the soil particles (sand, silt, clay, and organic matter) and their packing arrangement. Compacted soil layers have high bulk densities, restrict root growth, and inhibit the movement of air and water through the soil.
Soil pH. By estimating hydrogen-ion activity in a soil solution, the acidity or alkalinity of a soil can be measured. Soil pH affects the solubility of soil minerals, the availability of plant nutrients, and the activity of microorganisms. Acidity is generally associated with leached soils, whereas alkalinity generally occurs in drier regions. However, agricultural practices, such as liming or the addition of ammonium fertilizers, can alter soil pH. In general, pH values between 6 and 7.5 are optimal for crop growth.
Electrical conductivity. The electrical conductivity (EC) of a soil-water mixture is an indication of the amount of ions (dissolved salts) present in the soil solution. Excess salt content seriously affects plant growth and soil-water balance [26]. This may occur either naturally or as a result of inappropriate soil use and management. In general, electrical conductivity values between 0 and 0.8 dS m-1 are acceptable for general crop growth.
Ion-exchange capacity. The soil's ability to supply major plant nutrients, mainly calcium, magnesium and potassium, is reflected by its ion-exchange capacity. Specifically, the cation exchange capacity (CEC) is, to a large extent, related to the amount of soil colloids, organic matter, and clay, which are negatively charged and thus enable the soil to retain cations. Changes in pH and salt content affect the CEC. For example, aluminum toxicity occurs in certain soils at pH < 5, and soil dispersion with serious losses in structure may appear at high sodium concentrations (increasing salinity), both limiting factors for soil productivity and health.
Aggregate stability and soil slaking. An aggregate consists of several soil particles bound together and is usually formed by interactions of soil biota and the plant community and their products with soil mineral components. Aggregates play a major role in several aspects of soil health: the movement and storage of water, soil aeration, physical protection of SOM, the prevention of erosion, root development, and microbial community activity [54]. Aggregate stability is a measure of the vulnerability of soil aggregates to external destructive forces. Soil aggregation can naturally develop, disintegrate, and reform periodically [36]. Slaking is the process of fragmentation that occurs when aggregates are suddenly immersed in water [18] due to their inability to withstand the stresses of rapid water uptake. At fast rates of wetting, internal stresses arise from differential swelling and air entrapment in the soil aggregate [38]. Soil slaking can be used as a measure of the ability of the soil to maintain its structure and is affected by water content, rate of wetting, texture, clay mineralogy, and organic matter content.
Soil physical observations and estimations. Topsoil depth, root growth, and penetration resistance are also important indicators of soil health. Changes in topsoil thickness are usually the result of erosion processes accelerated by plowing, burning, overgrazing, and other management practices that remove the protective vegetative cover. These changes result in a loss of both the most fertile soil layer and its water-holding capacity as well as soil organic carbon content and productivity. Anomalies observed in root growth along a soil profile are indicators of physicochemical restraints in the soil, including compaction and the presence of areas with a higher penetration resistance, deficiencies in soil structure, high salt content, and low depth to bedrock, the stone layer, hard pan, the frozen layer, and the water table. All of these factors can result in plant stress and, eventually, in reduced crop growth and productivity [9]. Soil texture, i.e. the size distribution of primary soil particles smaller than 2 mm (sand, silt, and clay), is one of the most stable properties of soil. Texture is only slightly modified by cultivation and other practices that cause mixing of the different soil layers. Texture influences almost all other soil health indicators and helps determine water intake rates, water storage in the soil, ease of tillage, and soil aeration.
Molecular techniques to measure soil health: microbial biomass
An understanding of coupled biological and geochemical processes at the molecular level is fundamental for assessing the condition of the soil. Thus, a number of molecular and cellular techniques are currently being used in conjunction with biological and chemical indicators to increase our ability to evaluate soil health (Table 2).
Fluorescence microscopy. The number of bacteria in soil, their cell volumes, and the frequencies of dividing cells can be determined by fluorescence microscopy and computerized image analysis [10]. Soil microbial biomass can be estimated by staining with fluorescent dyes such as fluorescein isothiocyanate.
DNA measurement. Quantification of DNA following its extraction from soil may provide a simple and practicable method for estimating the amount of microbial biomass [29]. However, further work on correlating DNA measurements with a particular soil type is required.
Fluorescence in situ hybridization. FISH is a direct, cultivation-independent technique using rRNA-targeted oligonucleotide probes that is frequently used for the identification of microorganisms in soils. While this technique allows selective visualization of bacterial cells of different phylogenetic groups, it also has some limitations, particularly regarding quantitative analysis of complex samples [44].
RNA measurement. The composition of soil microbial communities can be estimated by reverse transcriptase polymerase chain reaction (RT-PCR) followed by gel electrophoresis of the amplified cDNA fragments [25]. The analysis of specific mRNAs reflects the expression of the corresponding gene in soil. Such measurements can also be done by real-time quantitative RT-PCR, which allows the detection and quantification of of mRNAs present in low amounts in environmental samples, including soils [47]. However, this method requires previous knowledge of the sequence of the mRNA of interest.
Stable isotope probing. SIP is a culture-independent technique that allows the identification of microorganisms directly involved in specific metabolic processes. In this method, labeled nucleic acids that were synthesized during assimilation of an isotopically enriched substrate are isolated and analyzed [50]. The technique has been used to study forest soils [51] and to identify the active components of an ammonia-oxidizing population in lake water [58].
Molecular techniques to measure soil health: genetic and functional biodiversity
Genetic diversity is most commonly studied by analyzing the diversity of genes encoding 16S rRNA (18S rRNA for eukaryotes). These genes occur in all microorganisms and show species-dependent variations in their base compositions. Three methods are commonly applied to examine the diversity of 16S (and 18S) rDNA sequences in total DNA extracted from soil microbial communities: denaturing gradient gel electrophoresis (DGGE), temperature gradient gel electrophoresis (TGGE), and terminal restriction fragment length polymorphisms (T-RFLP).
Denaturing gradient gel electrophoresis. Differences in the melting behavior of small DNA fragments (200–700 bp) that differ in as little as a single base substitution can be detected by DGGE [45]. The denaturants used are heat (a constant temperature of 60ºC) and a fixed ratio of formamide (ranging from 0–40%) and urea (ranging from 0–7 M). The position in the gradient where a domain of a DNA fragment melts and thus nearly stops migrating is dependent on the nucleotide sequence in the melted region. The benefit of this approach is that a molecular fingerprint of the community structure is generated for each soil. In fact, each band in each lane of the gel theoretically represents a different bacterial species. In addition, this technique enables the excision and subsequent sequencing of bands, allowing species identification using existing databases.
Temperature gradient gel electrophoresis. In contrast to DGGE, the separation of DNA by TGGE [35] does not depend on a chemical gradient of urea but instead on a precisely defined and controllable temperature gradient. This highly reproducible technique has the same advantages as DGGE. By designing species-specific in situ probes that hybridize to identified bacterial sequences, various species can be examined in even greater detail.
Terminal restriction fragment length polymorphism. Organisms can also be differentiated according to the patterns derived from cleavage of their DNA [41]. Thus, in T-RFLP, the specific fingerprint of a community is revealed by analyzing the polymorphism of a certain gene. T-RFLP is a high-throughput, reproducible method that allows the semi-quantitative analysis of the diversity of a particular gene in a community. It requires the extraction of DNA from a soil sample and its PCR amplification using a fluorescently labeled primer. T-RFLP yields a mixture of amplicons of the same or similar sizes with a fluorescent label at one end. After purification, the amplicon mixture is digested with a restriction enzyme, which generates fragments of different sizes that are separated by gel or capillary electrophoresis. The separated, labeled fragments are then densitometrically detected and a profile based on fragment lengths is generated. Recently, the potential of T-RFLP to discriminate soil bacterial communities in cultivated and non-cultivated soils was demonstrated [15].
BIOLOG™. Carbon utilization patterns can be measured by the BIOLOG™ assay [28]. In this test, a soil extract is incubated with up to 95 different carbon sources in a microtiter plate, and the redox dye tetrazolium blue is used to indicate microbial activity. Specific carbon sources have been selected for studies of soil microbial communities. The result of the assay is a qualitative physiological profile of the potential metabolic functions within the culturable portion of the microbial community. Differences in the profiles can then be analyzed by multivariate statistics.
Microbial resilience. The ability to estimate the relative abundance of each species of microorganisms in the soil, using the three techniques described above, has led to the suggestion that the "equitability index" (J) of numbers of individual species is an important estimation of the resilience of a soil. The use of statistical packages such as Phoretix enables quantification of both diversity indices and equitability [29,30].
Geochemical indicators
A number of analytical techniques are used for structural characterization of the SOM. In general, these involve the isolation of the free lipid and macromolecular fractions (humic substances and other recalcitrant organic fractions), which are among the most informative components of the SOM. The macromolecular fraction can be degraded by several means into small fragments that are chromatographically separated and then analyzed. This approach is aimed at obtaining environmental information based on the variable chemical composition of the SOM and it can be used to assess the impact of external disturbances. A review of the methods used can be found in [40].
Soil free lipids. This diverse group of hydrophobic substances includes simple compounds, ranging from fatty acids (which can be analyzed by the previously described PLFA techniques), to more complex molecules, such as sterols, terpenes, polynuclear hydrocarbons, chlorophylls, fats, waxes, and resins, which constitute the principal group of SOM biomarkers [39]. The extraction of soil lipids is frequently carried out using solvents with variable polarity in a Soxhlet apparatus, although alternative techniques, e.g. supercritical fluid extraction (SFE), are also available [8]. Total lipid extracts can be further fractionated by preparative chemical and chromatographic techniques, derivatized to enhance separation, or characterized by gas chromatography-mass spectrometry (GC-MS).
Humic fraction. Macromolecules with complex structures, including materials derived directly from the alteration of biogenic materials as well as structures formed de novo in the soil by biotic and abiotic factors [52], make up the humic fraction. The term humic substances (HS) is operational and several fractions are distinguished depending on their solubility in acid and alkaline media [24]. Recent progress in HS research has been made possible by the development of new approaches, methodologies, and instruments. A combination of different techniques appropriate for the study of complex matrices is used. Generally, a first estimation of the maturity or humification degree of the different HS fractions from SOM is obtained based on the results of both non-destructive and destructive methods. Among the non-destructive methods, solid-state 13C and 15N NMR spectroscopy is a valuable technique to quantify the different C and N structural groups: aromatic, aliphatic [alkyl-(waxes, alkanes, cutins and suberins)], o-alkyl (carbohydrates, tannins and altered carbohydrates), amide, amine, pyrrolic, etc. [33,49]. Infrared spectroscopy also provides valuable information on oxygen- and nitrogen-containing functionalities, while UV/visible spectroscopy is useful to establish humus maturity and the degree of HS aromaticness [55]. Among the destructive techniques, conventional analytical pyrolysis (Curie point or microfurnace), chemolysis in the presence of alkylating reagents ("thermally assisted hydrolysis-methylation") [32], and wet chemical degradation methods using specific reagents (CuO-NaOH, NaBO3, KMnO4, etc.) [2] generate fragments amenable to GC-MS analyses, which can be unambiguously used to identify to structures present in the HS.
Other methods used to characterize the HS include isotope ratio monitoring GC-MS (IRM-GC-MS), which provides both structural information and insight into the evolution and turnover times of different organic soil fractions [46]. Other emerging techniques are variants of traditional thermal analysis (TG-DSC) coupled with isotopic ratio monitoring (TA-IRM) [42].
Future prospects
There is a need for a holistic consideration of soil health as well as transdisciplinary soil management approaches that integrate biological, chemical, and physical strategies to achieve soils supporting a sustainable agriculture. The environmental and economic benefits of sustainable soils are enormous: increased resource efficiency, decomposition and nutrient cycling, nitrogen fixation, and water-holding capacity, as well as prevention of pollution and land degradation. Current agricultural practices reduce soil biodiversity, mainly as a result of the overuse of chemicals, leading to compaction or other disturbances and hence irreversible adverse ecological alterations, resulting in loss of agricultural productivity. A series of long-term comparative studies have shown that organic/sustainable systems can increase both SOM accumulation and microbial activity. Moreover, the organic C lost during intensive agriculture could be regained through sustainable management practices, thereby contributing to mitigating climate change.
The development of approaches that do not require the establishment of microbial cultures will undoubtedly enhance our knowledge of biodiversity and promote the discovery of new microorganisms with unique capacities for bioremediation, soil restoration, and therapeutic applications.
Acknowledgements. We thank Gonzalo Almendros from Centro de Ciencias Medioambientales (CSIC, Madrid, Spain) for his valuable revision of the article.
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