Abstract. In contrast to mineral topsoils, in subsoils the origin and processes leading to the formation and stabilization of organic matter (OM) are still not well known. This study addresses the fate of litter-derived carbon (C) in whole soil profiles with regard to the conceptual cascade model, which proposes that OM formation in subsoils is linked to sorption–microbial processing–remobilization cycles during the downward migration of dissolved organic carbon (DOC). Our main objectives were to quantify the contribution of recent litter to subsoil C stocks via DOC translocation and to evaluate the stability of litter-derived OM in different functional OM fractions. A plot-scale stable isotope-labeling experiment was conducted in a temperate beech forest by replacing the natural litter layer with 13C enriched litter on an area of 20 m2 above a Dystric Cambisol. After 22 months of field exposure, the labeled litter was replaced again by natural litter and soil cores were drilled down to 180 cm soil depth. Water extraction and density fractionation were combined with stable isotope measurements in order to link the fluxes of recent litter-derived C to its allocation into different functional OM fractions. A second sampling was conducted 18 months later to further account for the stability of translocated young litter-derived C. Almost no litter-derived particulate OM (POM) entered the subsoil, suggesting root biomass as the major source of subsoil POM. The contribution of aboveground litter to the formation of mineral-associated OM (MAOM) in topsoils (0–10 cm) was 1.88±0.83 g C m−2 and decreased to 0.69±0.19 g C m−2 in the upper subsoil (10–50 cm) and 0.01±0.02 g C m−2 in the deep subsoil >100 cm soil depth during the 22 months. This finding suggests a subordinate importance of recent litter layer inputs via DOC translocation to subsoil C stocks, and implies that most of the OM in the subsoil is of older age. Smaller losses of litter-derived C within MAOM of about 66 % compared to POM (77 %–89 %) over 18 months indicate that recent carbon can be stabilized by interaction with mineral surfaces; although the overall stabilization in the sandy study soils is limited. Our isotope-labeling approach supports the concept of OM undergoing a sequence of cycles of sorption, microbial processing, and desorption while migrating down a soil profile, which needs to be considered in models of soil OM formation and subsoil C cycling.
Thermal analysis techniques have been used to differentiate soil organic carbon (SOC) pools with differing thermal stability. A correlation between thermal and biological stability has been indicated in some studies, while others reported inconsistent relationships. Despite these controversial findings and no standardized method, several recently published studies used thermal analysis techniques to determine the biological stability and quality of SOC in mineral soils. This study examined whether thermal oxidation at temperature levels between 200°C and 400°C, combined with evolving gas analysis and isotope ratio mass spectrometry, is capable of identifying SOC pools with differing biological stability in mineral soils. Soil samples from three sites being under Miscanthus (C4‐plant) cultivation for more than 17 years following former agricultural cropland (only C3‐plant) cultivation were used. Due to natural shifts in 13C content, young and labile Miscanthus‐derived SOC could be distinguished from stable and old C3‐plant‐derived SOC. The proportion of Miscanthus‐derived SOC increased significantly with increasing temperatures up to 350°C in bulk soil samples, indicating increasing oxidation of labile and young SOC with increasing temperatures. Use of density fractions to validate the thermally oxidized SOC from bulk soil samples revealed that the thermal oxidation patterns did not reflect the biological stability of SOC. The suggested biologically labile particulate organic carbon (light fraction from density fractionation) was clearly enriched in Miscanthus‐derived young SOC. The thermal oxidation patterns, however, revealed preferential oxidation of these biologically labile fractions not at low temperatures, but rather at higher temperatures. The reverse was found for the biologically stable mineral‐associated density fraction (heavy fraction). Based on different soil types, it was concluded that the thermal stability of SOC between 200°C and 400°C is not a suitable indicator of the biological stability of SOC and, thus, thermal oxidation is not capable of fractionating SOC pools with differing biological stability.
Abstract. Large amounts of total organic carbon are temporarily stored in soils, which makes soil respiration one of the major sources of terrestrial CO2 fluxes within the global carbon cycle. More than half of global soil organic carbon (SOC) is stored in subsoils (below 30 cm), which represent a significant carbon (C) pool. Although several studies and models have investigated soil respiration, little is known about the quantitative contribution of subsoils to total soil respiration or about the sources of CO2 production in subsoils. In a 2-year field study in a European beech forest in northern Germany, vertical CO2 concentration profiles were continuously measured at three locations, and CO2 production was quantified in the topsoil and the subsoil. To determine the contribution of fresh litter-derived C to CO2 production in the three soil profiles, an isotopic labelling experiment, using 13C-enriched leaf litter, was performed. Additionally, radiocarbon measurements of CO2 in the soil atmosphere were used to obtain information about the age of the C source in the CO2 production. At the study site, it was found that 90 % of total soil respiration was produced in the first 30 cm of the soil profile, where 53 % of the SOC stock is stored. Freshly labelled litter inputs in the form of dissolved organic matter were only a minor source for CO2 production below a depth of 10 cm. In the first 2 months after litter application, fresh litter-derived C contributed, on average, 1 % at 10 cm depth and 0.1 % at 150 cm depth to CO2 in the soil profile. Thereafter, its contribution was less than 0.3 % and 0.05 % at 10 and 150 cm depths, respectively. Furthermore CO2 in the soil profile had the same modern radiocarbon signature at all depths, indicating that CO2 in the subsoil originated from young C sources despite a radiocarbon age bulk SOC in the subsoil. This suggests that fresh C inputs in subsoils, in the form of roots and root exudates, are rapidly respired, and that other subsoil SOC seems to be relatively stable. The field labelling experiment also revealed a downward diffusion of 13CO2 in the soil profile against the total CO2 gradient. This isotopic dependency should be taken into account when using labelled 13C and 14C isotope data as an age proxy for CO2 sources in the soil.
scite is a Brooklyn-based organization that helps researchers better discover and understand research articles through Smart Citations–citations that display the context of the citation and describe whether the article provides supporting or contrasting evidence. scite is used by students and researchers from around the world and is funded in part by the National Science Foundation and the National Institute on Drug Abuse of the National Institutes of Health.
hi@scite.ai
10624 S. Eastern Ave., Ste. A-614
Henderson, NV 89052, USA
Copyright © 2024 scite LLC. All rights reserved.
Made with 💙 for researchers
Part of the Research Solutions Family.