4 cm in diameter) to a bulk density of 1.4 g cm−3. The major characteristics of the research site are given in Table 1 according to Gerwin et al. (2009). Five grams of labelled litter material (L. corniculatus or C. epigejos) was mixed into the first centimetre of the soil in each microcosm. Microcosms without litter application served as controls. In total, 75 microcosms were randomly placed and incubated at 10 °C in the dark. The soil water content was estimated by weekly weighing and was maintained Enzalutamide chemical structure at 55% of the maximum water-holding capacity throughout the experiment. For each treatment (L. corniculatus, C. epigejos, control), 15 microcosms

were prepared for harvests with five independent replicates after 4, 12 and 40 weeks of litter incubation. For microbial analyses, the detritusphere in the first 2 cm of each column was harvested. To quantify the litter degradation rates, additional 15 microcosms for L. corniculatus

and C. epigejos were incubated under the same conditions. Five grams of the labelled litter material (L. corniculatus or C. epigejos) was filled into nylon bags (10 × 10 cm, mesh size 40 μm) and placed into these microcosms, 1 cm below soil surface. At all sampling times, individual litter bags were removed from five independent microcosms; the total amount of litter was air-dried and weighed in order to calculate the litter degradation rates. The total 13C, C and N contents at individual harvesting times were analysed using an Euro EA (Eurovector, PI3K Inhibitor Library concentration Milan, Italy) coupled with an isotope ratio mass spectrometer MAT 253 (Thermo Electron, Bremen, Germany). Microbial biomass C was estimated after chloroform fumigation–extraction (Cmic) according to Joergensen (1995). The total organic C content and the δ13C in the CaCl2 Adenosine triphosphate extracts were measured

using on-line coupling of liquid chromatography and stable isotope ratio MS (Thermo Electron), according to Krummen et al. (2004). PLFA analyses were based on Zelles et al. (1995) and have been described in detail elsewhere (Esperschütz et al., 2009). Fatty acids are presented by the number of C atoms, followed by the number of double bonds. The positions of double bonds are indicated by ‘ω’ and the number of the first double-bonded C atoms from the ω end of the C chain. Anteiso- and iso-branched fatty acids are indicated by ‘ant’ and ‘iso’, followed by the number of C atoms. Branched fatty acids in which the position of the double bond was unknown were indicated by the prefix ‘br’. Methyl groups on the 10th C atom from the carboxyl end of the molecule were indicated by ‘10ME’. Cyclopropane fatty acids were indicated by the prefix ‘cyc’, while dicyclopropylic PLFA were indicated by ‘dic’. Even-chained, saturated fatty acids were abbreviated with the prefix ‘nor’. A univariate anova was carried out using spss 11.