Taken from Darby et al. (in revision) Soil Biology and
Biochemistry, with modest edits for brevity:
Soils were collected in July 2014 from three sites at and near the
Hubbard Brook Experimental Forest (see Geographic Location, above). At
each site, eight soil cores were collected from within a 900
m2 plot; half (n = 4 cores per site) were
randomly selected for the microbial analyses described here. The
forest floor (Oe/Oa) was collected by removing loose leaf litter (Oi),
then using a knife to collect a block of the Oe and Oa horizons from
within a 15 x 15 cm wooden frame. A diamond bit rotary corer (Rau et
al., 2011) with a 9.5 cm internal diameter enabled quantitative
collection of the underlying mineral soil in 10 or 20 cm increments to
50 cm depth (0-10, 10-20, 20-30, and 30-50 cm). All analyses described
here were performed on all 60 soil samples (3 sites × 4 cores per site
× 5 depths per core), with minor exceptions noted below. Samples were
stored on ice packs during transport and at 4 °C in the laboratory
until processing. Soils were sieved within 24 hours of collection,
using a coarse sieve (4 mm) to quickly homogenize the sample and
remove large rocks and roots. Sub-samples of sieved soil were stored
at -20 °C for later use in enzyme activity assays. The remaining soil
was stored at 4 °C for up to 2 more days for the N cycling assays.
Bulk density and soil C and N stocks were determined from the
quantitative soil samples following Rau et al. (2011). Briefly, 10 g
subsamples of sieved soil were taken for moisture determination by
drying for 1 day at 110 oC, and for C and N
analysis after grinding to a fine powder with a ball mill (Retsch
mixer mill MM200; Verder Scientific, Newtown, Pennsylvania, USA). Soil
C and N concentration and isotopic composition were measured at the
Cornell Stable Isotope Laboratory in Ithaca, NY, using a Finnigan MAT
Delta Plus mass spectrometer following combustion with an elemental
analyzer (Carlo Erba NC2500; Thermo Finnigan, San Jose, CA, USA).
Surface mineral soil pH was measured with an Accumet AB15 pH meter
(ThermoFisher Scientific, Waltham, MA, USA) with a 1:2 ratio of dry
soil to water.
Rates of gross N mineralization and nitrification were assessed using
the isotope pool dilution method (Davidson et al., 1991; Hart et al.,
1994), in which a known amount of
15NH4
+
or
15NO3
-
is added to a soil sample, and its rate of dilution by mineralization
or nitrification of unlabeled N is measured over 24 hours. To quantify
rates of gross N mineralization and
15NH4
+
consumption, 7.53 μg N of 98 atom%
(15NH4)2SO4
were added to a pair of 15 g field-moist sub-samples, each in a 125 mL
HDPE bottle. The label, along with 1 mL of deionized water, was
distributed within each sub-sample using a 250 μg syringe. One
sub-sample from each pair was extracted with 50 mL of 2M KCl within 15
minutes of labeling, and the second sub-sample was extracted after
incubation in the dark for 24 hours at room temperature. The KCl
extracts were stored in 60 mL HDPE bottles and frozen at -20 °C until
chemical analysis. The same procedure was used to estimate rates of
gross nitrification and
15NO3
-
consumption in another pair of subsamples using 1.63 μg N of 98%
K15NO3
-
per subsample.
The KCl extracts were analyzed with colorimetric methods for
NH4
+ (alkaline
phenate) and NO3
- +
NO2
- (cadmium
reduction) concentrations using a Quikchem 8100 flow injection
analyzer (Lachat Instruments, Milwaukee, WI, USA) at the Cary
Institute of Ecosystem Studies in Millbrook, NY. The N diffusion
method (Brooks et al. 1989) was used to determine
15N in the extract
NH4
+ or
NO3
-. Extracts with
small concentrations of extractable
NH4
+ or
NO3
- were spiked
with known amounts (50 or 100 μg N) of unlabeled
NH4
+ or
NO3
- to ensure that
each sample contained sufficient N for diffusion and
15N analysis. For the diffusions, two small
glass fiber filters were acidified with 20 μL
KHSO4, then sealed in a Teflon tape packet that
was floated on each KCl extract in a 125 ml HDPE bottle that was
placed on a shaker table for seven days. MgO was added to all samples
to increase pH and convert
NH4
+ to
NH3, which is trapped on the acidified filters.
Devarda’s alloy was also added to the
15NO3
--labeled
extracts to convert
NO3
- to
NH4
+; filters in
these extracts collected both
NH4
+ and
NO3
-. Filter
15N contents were analyzed at the Cornell
Stable Isotope Laboratory as described above. Pre-spike
15NH4
+
and
15NO3
-
extract concentrations were computed using mean
15N measurements of the unlabeled spike
solutions, and assuming that 15N values of
the unlabeled NH4
+
in the extracts for gross nitrification matched the natural abundance
15N measured in corresponding soil samples
(Högberg 1997).
Gross N cycling rates were calculated using the differences in atom
percent 15N enrichment above background
(APE) and in inorganic N concentrations between the pre- and
post-incubated samples using the equations in Hart et al. (1994),
originally developed by Kirkham and Bartholomew (1954). Lack of
15N enrichment for four of the 240
diffusions prevented calculation of two each of the 60 gross
mineralization and nitrification rates. One-day net N mineralization
and nitrification rates were calculated using the pre- and post-
incubation extractable inorganic N measurements collected during the
gross N mineralization assay. Net N mineralization was calculated as
([NH4
+-N]+[
NO3
--N])incubation
- ([NH4
+-N]+[
NO3
--N])initial
and net nitrification was calculated as
[NO3
--N]incubation-
[NO3
--N]initial.
For the enzyme assay, two soil slurries were created for each soil
sample, each using two grams of soil in 150 mL of a 50 mM sodium
acetate buffer (pH 5.0) homogenized with a hand blender. One slurry
was used for measurements of hydrolytic enzyme activity and the other
for oxidative enzyme activity. Lack of material precluded analysis of
oxidative enzyme activity for one sample at the old-growth site and
eight samples at the mature site, including all four of its forest
floor samples. For both sets of enzyme analyses, 50 µL of each sample
slurry was added to 8 replicate wells in a column of a 96-well plate.
Potential activities of six hydrolytic enzymes used for microbial
acquisition of C-, N-, and P were quantified with fluorometric assays
using the method outlined in German et al. (2011). These enzymes
included two used to degrade cellulose, β-glucosidase (BG) and
cellobiohydrolase (CB); one to degrade hemicellulose, β-xylosidase
(BX); one to acquire phosphorus, acid phosphatase (AP); and two used
to acquire N, NAG for amino sugars and LAP for amino acids. A
fluorescent substrate specific to each enzyme function was added to
the plate, which was then incubated in the dark at room temperature.
Fluorescence was measured on a microplate reader set at 365 nm
excitation and 450 nm emission. Assays were run alongside a standard
curve containing soil homogenate with an increasing concentration of
methylumbelliferone (MUB), except for the LAP analyses which used
amidomethylcoumarin (AMC) standards (Table 2). Fluorescence was
converted to units of potential enzyme activity per unit dry mass
(nmol g-1 h-1)
as in German et al. (2011). Potential activity of the lignolytic
oxidative enzyme phenol oxidase (POX), was assessed using two
different enzyme substrates, ABTS
(2,20-azino-bis(3-ethylbenzthiazoline-6-sulfonic acid)) and L-DOPA
(L-3,4-dihydroxyphenylalanine), as suggested by Bach et al. (2013) on
account of the variability of these assays. These activities are
referred to here as POXABTS and
POXLDOPA, respectively. Plates were incubated
in the dark for 24 hours at room temperature after adding the L-DOPA
or ABTS substrates. Before measurement, 150 µL of each well was
transferred onto a clear reading plate with transparent well bottoms.
Bach, C.E., Warnock, D.D., Van Horn, D.J., Weintraub, M.N.,
Sinsabaugh, R.L., Allison, S.D., German, D.P., 2013 .Measuring phenol
oxidase and peroxidase activities with pyrogallol, L-DOPA, and ABTS:
effect of assay conditions and soil type. Soil Biology Biochemistry,
67, 183-191.
Brooks, P.D., Stark, J.M., McInteer, B.B., Preston. T., 1989.
Diffusion method to prepare soil extracts for automated N-15 analysis.
Soil Science Society of America Journal 53, 1707-1711.
Davidson, E.A., Hart S.C., Shanks C.A., Firestone, M.K., 1991.
Measuring gross nitrogen mineralization, immobilization, and
nitrification by 15N isotopic pool dilution
in intact soil cores, Journal of Soil Science 42, 335-349.
German, D.P., Weintraub, M.N., Grandy, A. S., Lauber, C.L., Rinkes,
Z.L., Allison. S.D., 2011. Optimization of hydrolytic and oxidative
enzyme methods for ecosystem studies. Soil Biology and Biochemistry
43, 1387-1397.
Hart, S.C., Nason, G.E., Myrold, D.D., Perry, D.A., 1994. Dynamics of
gross nitrogen transformations in an old-growth forest: The carbon
connection. Ecology 75, 880-891.
Högberg, P. 1997. Tansley Review No. 95:
15N natural abundance in soil-plant
systems. New Phytologist 137, 179-203.
Kirkham, D., Bartholomew, W.V., 1955. Equations for following nutrient
transformations in soil, utilizing tracer data. Soil Science Society
of America Proceedings 19, 189-192.
Rau, B.M., Melvin, A.M., Johnson, D.W., Goodale, C.L., Blank, R.R.,
Fredriksen, G., Miller W.W., Murphy, J.D., Todd D.E., Walker, R.F.,
2011. Revisiting soil carbon and nitrogen sampling: quantitative pits
versus rotary cores. Soil Science 176, 273-279.
