Adenylate energy charge measurements in soil |
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| Institution: | 1. Consiglio per la Ricerca in Agricoltura e l''analisi dell''Economia agraria (CREA), Research Centre for Cereal and Industrial Crops, Laboratory of Caserta, Via Torrino, 2, 81100 Caserta, Italy;2. Consiglio per la Ricerca in Agricoltura e l''Analisi dell''Economia agraria (CREA), Research Centre for Agriculture and Environment, Unit of Firenze, Via di Lanciola, 12, 50125 Impruneta (FI), Italy;3. Consiglio per la Ricerca in Agricoltura e l''analisi dell''Economia agraria (CREA), Research Centre for Viticulture and Enology, Unit of Gorizia, Via Trieste 23, 4170 Gorizia, Italy;4. Department of Sustainable Crop Production, Università Cattolica del Sacro Cuore, via Emilia Parmense 84, Piacenza 29122, Italy;5. Department of Environmental, Biological, and Pharmaceutical Sciences and Technologies, University of Campania “Luigi Vanvitelli”, Via Vivaldi 43, 81100 Caserta, Italy;6. SOLIomics s.r.l., Via del Cotonificio, 129/B, 33100 Udine, Italy |
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| Abstract: | Adenosine 5'-triphosphate (ATP), adenosine 5'-diphosphatc (ADP) and adenosine 5'-monophosphate (AMP) were extracted from soil with either a solution of trichloroacetic acid, paraquat and phosphate (TCA reagent) or a mixture of chloroform, sodium hydrogen carbonate, phosphate and adenosine (NaHCO3 reagent). Standard enzymic procedures were used to convert ADP and AMP to ATP, which was measured by the fire-fly luciferin-luciferase system. The measured quantities of nucleotides were corrected for incomplete extraction using the percentage recoveries of added ATP, ADP and AMP. The adenylate energy charge ratio (AEC) was calculated from the formula AEC = (ATP] + 0.5 ADP])/(ATP] + ADP] + AMP]).Measurements were made on a grassland soil, following a conditioning incubation at 15°C and 50% WHC for 7 days. Additional measurements were made on the same soil after a further 50- or 100-day incubation at 25°C and 50% WHC, with or without an amendment of 1100 μg ryegrass Cg−1 soil, added at the end of the conditioning incubation. Biomass-ATP concentration, measured in TCA extracts, changed little, even on prolonged incubation, and was maintained at a level comparable to that observed in earlier work (about 10 p mol ATP g−1 biomass C). AEC values in TCA soil extracts were high (0.8–0.9) for all soil treatments and independent of substrate addition or length of incubation.In contrast, AEC was low (0.4) in fresh soil extracted with NaHCO3 reagent, but increased to 0.6 when ryegrass was incubated with the soil for 50 days. Although the total adenine nucleotide pool (i.e. ATP] + ADP] + AMP]) was similar as measured in NaHCO3 and in TCA soil extracts, both energy charge and ATP content were lower in the NaHCO3 extracts. It was therefore concluded that the main reason for the lower AECs observed with the NaHCO3 reagent was that microbial ATPases were still active during extraction and caused appreciable hydrolysis of microbial ATP to ADP and AMP. In contrast, the TCA reagent rapidly inactivates ATPases and is therefore preferable for extracting adenine nucleotides from soil.The results indicate that the soil microbial biomass, although a mainly dormant population, maintains both AEC and ATP at levels characteristic of exponentially growing organisms in vitro, even during prolonged incubation without fresh substrate. It was also concluded that roots make a negligible contribution to total ATP extracted from fresh sieved soil. |
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