AbstractThe total ammonium nitrogen

Abstract
The total ammonium nitrogen (TAN) concentration is often a key limiting water quality
parameter in intensive aquaculture systems. Removing ammonia (NH3) through biological activity is
thus an important objective in aquaria and aquaculture system designs. In this study, the performance
characteristics of a suspension of nitrifying cells (named ammonia binding inoculum liquid, ABIL)
have been explored. This aqueous suspension contains a highly active, nitrifying microbial
consortium that can be used to shorten the start-up period of a biofilter. Tests were performed in
freshwater at lab scale (70 l, 20 – 24 jC). Results showed that the application of the consortium at a
dose of 5 mg volatile suspended solids (VSS) l
1 assures a total removal of ammonium (NH4
+ ) and
nitrite species from 10 mg N l
1 to below the detection limit within a period of 4 days.
Experimentally, at a substrate level of 10 mg TAN l
1
, a rate of biological ammonium and nitrite
conversion of the order 0.3 – 0.5 g TAN g
1 VSS
1 day
1 could be achieved by the consortium in
the freshwater aquaria systems tested. Provided adequate aeration and dissolved oxygen (DO) levels
of 6 mg l
1 or more, no important intermediary nitrite concentrations were found. Only a small
amount of TAN was not recovered as nitrate and might have been lost through ammonia stripping.
Pre-inoculating the nitrifiers in polyurethane (PU) sponges and installation of such sponges in the
freshwater aquaria did not improve the effect compared to adding the consortium directly to the
water. After 12 months preservation of the inoculum at 4 jC, no important decrease in ammonium removal activity and only a minor decrease in the nitrite removal rate of the consortium were noticed.
1. Introduction
Fish stocking densities in aquaria and aquaculture systems are limited primarily by the
dissolved oxygen (DO) concentrations and often, also by the ammonia (NH3) concentrations
especially in systems with high hydraulic residence times (Meade, 1985).
Ammonia is formed as the principal end product from protein metabolism in fish. Fish
expel NH3 through their gills by branchial diffusion, and in freshwater fish, ammonium
(NH4
+ ) can also be branchially exchanged for a monovalent cation. Ammonia and
ammonium originating from the gills comprise 60– 90% of the total N excreted by fish
(Forster and Goldstein, 1969; Rychly, 1980). Urea is also expelled through the gills and
accounts for 9– 27% of the soluble N excreted (Clark et al., 1985). Another source of
ammonia in aquaria and aquaculture systems is microbial ammonification of organic
nitrogen in uneaten feed residues and in fish feces. This particulate matter only accounts
for 3.4 –4.2% of the total nitrogenous waste load in tank systems (Clark et al., 1985).
Ammonia exists in water in two forms, i.e., as ionized ammonium ions (NH4
+ ) and
unionized ammonia. The two species together are indicated as total ammonium nitrogen
(TAN). Unionized ammonia is the more toxic form. Levels above 0.1 mg NH3-N l
1 are
considered detrimental to fish (van Rijn et al., 1990) and in practical terms, fish should not
be chronically exposed to NH3-N levels of more than 50 AgNl
1 (Frances et al., 2000).
For larval culture, even more stringent conditions are required: Guillen et al. (1994)
reported high mortalities in groups of 1-day-old larvae of the Japanese croaker (Nibea
japonica) exposed to 2.7 and 27 Ag NH3-N l
1
.
Nitrification is the process in which ammonium is oxidized to nitrate in a two-step
process carried out by two different groups of chemolithoautotrophic bacteria. In the first
step, ammonium-oxidizing bacteria (AOB) oxidize ammonium to nitrite, which is
converted to nitrate by nitrite-oxidizing bacteria (NOB) in the second step (Focht and
Verstraete, 1977). Therefore, nitrification is an important process in fish culture, both in
home aquaria and commercial aquaculture systems, since it can convert toxic ammonia to
nitrate which is considered relatively harmless to fish and can be kept at safe levels with
regular water changes (Hargreaves, 1998).
Nitrite is formed in aquaria and aquaculture systems from the oxidation of ammonia
by chemolithoautotrophic AOB, but it can also be formed as a consequence of
denitrification activity in anoxic zones in the biofilter. The accumulation of nitrite can
be toxic to fish and other aquatic organisms. Nitrite reacts with hemoglobin to form
methemoglobin inhibiting the transport of oxygen resulting in methemoglobinemia or
brown blood disease (Frances et al., 1998). In the literature, different concentrations of
nitrite ranging from below 0.2 mg l
1 NO2

-N (Blancheton, 2000) up to 12 mg l
1
NO2

-N (Mazik et al., 1991; Chen and Lee, 1997) are being targeted as safe levels in aquaculture systems. Different parameters like exogenous chloride concentrations,
aquatic species, growth phase, exposure time, and pH affect the tolerance of the species
for nitrite.
Because of the ability to remove the ammonium ion and nitrite from water, the AOB
and NOB play an essential role in aquaria and aquaculture systems. Therefore, these
systems usually provide a solid matrix, often called a biological filter, to promote the
growth of AOB and NOB (Wheaton et al., 1994). However, AOB and especially NOB are
slow-growing organisms (Bock and Koops, 1992) with doubling times for NOB ranging
from 12 to 32 h (Ehrich et al., 1995). To shorten the time needed for the establishment of
the AOB and NOB, commercial preparations are available to seed the aquatic environment.
Past studies have generally shown these preparations to be poorly effective for
unknown reasons (Timmermans and Gerard, 1990).
Recently, a new approach for the growth and maintenance of nitrifying cultures has
resulted in the development of a product named ammonia binding inoculum liquid
(ABIL). This is a liquid-mixed microbial enrichment. In this study, the nitrification
performances of freshwater aquaria inoculated with this consortium were tested. It is
shown that application of the consortium as inoculum removes the TAN in a reliable and
reproducible way in a few days, with formation of low transient levels of nitrite.
2. Materials and methods
2.1. Growth of the consortium
The nitrifying suspension called ABIL was obtained from AVECOM (Belgium). It is
cultivated in a 500-l reactor in fed-batch mode at LabMET. The nitrifying culture was
obtained by gradual enrichment starting from natural surface water. The culture receives a
daily load of 88 g N (58.7 g TAN day
1 as ammonium chloride and 29.3 g NO2

-N
day
1 as sodium nitrite) to selectively support the growth of the nitrifying bacteria. The
feed also contains calcium carbonate as a carrier matrix, buffer, and carbon source. The pH
of the reactor is further controlled at pH 7.0 by addition of NaOH. Temperature is kept at
22 –24 jC. Compressed air is used to aerate the culture and maintain a dissolved oxygen
level of 6.0 mg O2 l

1 or higher. The cell density of the bacteria is maintained at 0.5 g
volatile suspended solids (VSS) l
1 by harvesting the culture on a regular basis. The
harvested cell suspension can be further concentrated to desirable cell densities by
sedimentation or centrifugation.
2.2. Specific activity of the consortium
The specific nitrifying activity of the ABIL consortium at different TAN concentrations
was determined as follows: 500-ml Erlenmeyer flasks filled with the consortium were
placed on a rotary shaker (115 rpm) after the addition of a specific volume of an ammonium
chloride solution (1 g TAN l
1
) to produce TAN concentrations in the range of 25 – 250 mg
l

1
. To prevent the cells from settling and to assure oxygen saturation, each Erlenmeyer
flask was equipped with a porous stone connected to an airblower. The nitrifying activity of the consortium was determined by measuring the concentration of TAN in the Erlenmeyer
flasks as a function of time. The concentration of TAN was determined with the distillation
method using a 2200 Kjeltec Auto Distillation apparatus (Foss Tecator, Sweden) (Bremner
and Keeney, 1965). The temperature of the room where the activity tests were done was
kept constant at 28 jC. For every TAN concentration, a blank test was performed to assess
the amount of nitrogen lost due to ammonia stripping. The blank test consisted of an
Erlenmeyer flask filled with tap water and a specific volume of an ammonium chloride
solution placed on the same rotary shaker and provided with a porous stone connected to an
airblower.