BioRisk ig | 57-l 68 (2022) Apeer-reviewed open-access journal 

doi: 10.3897/biorisk.17.77463 RESEARCH ARTICLE & RB Ke) R IS k 

https://biorisk.pensoft.net 

Application of residual sludges from wastewater 
treatment technologies for construction of biofertiliser 

Mihaela Belouhova'*, Dobromira Yaneva'’, Yana Topalova'* 

| Department of General and Applied Hydrobiology, Faculty of Biology, Sofia University St. Kliment Ohridski, 
8 Dragan Tzankov Blvd, Sofia 1164, Bulgaria 2 Center of Competence “Clean technologies for sustainable 
environment — waters, wastes, energy for circular economy”, Sofia University St. Kliment Ohridski, 15 Tzar 
Osvoboditel Blud., Sofia 1504, Bulgaria 

Corresponding author: Mihaela Belouhova (mihaela.kirilova@uni-sofia.bg) 

Academic editor: Galina Radeva | Received 1 November 2021 | Accepted 28 November 2021 | Published 21 April 2022 

Citation: Belouhova M, Yaneva D, Topalova Y (2022) Application of residual sludges from wastewater treatment 
technologies for construction of biofertiliser. In: Chankova S, Peneva V, Metcheva R, Beltcheva M, Vassilev K, Radeva 
G, Danova K (Eds) Current trends of ecology. BioRisk 17: 157-168. https://doi.org/10.3897/biorisk.17.77463 

Abstract 

To stimulate plant development in phytoremediation or in the cultivation of non-food crops in potentially 
contaminated soils, a biotechnologically created product could be applied. The aim of this study was to ex- 
plore the possibility of creation of biofertiliser, based on activated sludge combined with bacterial strain with 
detoxifying and plant growth promoting properties. The presented study is focused on the effect of phenol in 
the following concentrations: 5 mg/l, 100 mg/l, 250 mg/l, 500 mg/l and 1000 mg/I on the metabolic activity 
of Brevibacillus laterosporus BT 271. The gradual increased concentration of phenol was used to study the met- 
abolic activity of mineralised activated sludge and B. laterosporus BT271. The CTC/DAPI staining showed 
high activity of the bacteria even at the highest concentration. The greatest amount of biomass was accumu- 
lated at 5 mg/I phenol (4.44 x 10’ cells/ml). At this toxicant concentration, a total dehydrogenase activity of 
5.72 x 10“ wg H+/ml*min was found. Studies of the metabolic activity of microorganisms in experiments 
involving a combination of mineralised activated sludge, B. /aterosporus BT271 and phenol at three concentra- 
tions (5 mg/l, 250 mg/l and 1000 mg/l) showed the highest value for dehydrogenase activity in the variant 
with average phenolic concentration (up to 6.39 x 10° ng H+/ml*min. The results proved the detoxification 
potential of B. laterosporus BT 271 when different concentrations of phenol were present. The combination of 
a mineralised activated sludge and selected highly active biodegrading B. /aterosporus BT271 showed valuable 
properties of detoxification and metabolic activity and keep these potentials up to 1000mg/I phenol. 

Keywords 
Bioremediation, Brevibacillus laterosporus BT271, mineralised activated sludge, phenol 

Copyright Mihaela Belouhova et al. This is an open access article distributed under the terms of the Creative Commons Attribution License (CC 
BY 4.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. 


158 Mihaela Belouhova et al. / BioRisk 17: 157-168 (2022) 

Introduction 

Soils are a key resource for the existence and maintenance of normal human life and 
the planet. They are, therefore, the focus of the EU’s Green Deal, adopted in 2019. 
According to this document and the European Commission's “Towards Zero Pollution 
for Air, Water and Soil’ action plan, Europe must have achieved zero soil pollution 
by 2050 (European Commission 2019, 2021). At the same time, in addition to the 
absence of pollution in the maintenance of soil fertility, the principles of the circular 
bio-economy need to be introduced (European Commission 2019). These ambitious 
goals will be difficult to achieve in the current economic and health crisis, combined 
with the lack of technology readiness in the various industries. Therefore, it is necessary 
to look for innovative solutions that allow environmentally-friendly treatment of soil 
resources and subsequent maintenance of fertility in them. One of the important direc- 
tions in this subject is the creation of a less toxic environment. When it comes to soils, 
this involves the elimination of toxic substances, such as pesticides. Another aspect is 
the use of treated water in irrigation in agriculture. This again carries risks for the entry 
of toxic substances, antibiotics, steroid hormones and other xenobiotics into the soil. 
They must be degraded by the soil microflora or by the addition of biofertilisers. ‘This 
requires a special focus on innovation activities related to the targeted management of 
detoxification processes in soils used for intensive or organic farming. 

Activated sludge is formed during the treatment of domestic wastewater and, after 
stabilisation and decontamination, can be used for soil treatment (Gray 2010; Dimkov 
et al. 2017). They are alternatives to conventional fertilisers and offer a circular solu- 
tion for solid waste from water treatment — stabilised sludge (Meuser 2013). These 
innovative and complex biofertilisers can be used for the reclamation of soils that are 
contaminated or damaged by human activity (Banov et al. 2020). The activated sludge 
is rich in both humic substances and micro-, macronutrients. It also contains microor- 
ganisms that are beneficial for the soil. 

However, the bacteria in the activated sludge for recovery have low detoxification 
activity and are adapted mainly to the biodegradation of only trivial contaminants. In 
the case of soil contamination with organic pollutants, it is necessary to enhance the 
target detoxification activity by adding highly active biodegradants, which perform the 
biodegradation of toxic contaminants at a high rate and with a minimum degree of in- 
hibition. This approach to bioaugmentation is used for contamination with petroleum 
products, pesticides, insecticides, pharmaceuticals, PFAS, antibiotics and other prod- 
ucts, xenobiotic soil contaminants and residues in recycled water for irrigation (Hong 
et al. 2020; Li et al. 2021). In these bioaugmentation procedures for the detoxification 
activity of biological fertilisers, consortia (Varjani and Upasani 2019; Laothamteep 
et al. 2022) or individual bacterial cultures belonging to various genera can be used - 
Pseudomonas (Ramadass et al. 2018), Enterobacter (Koolivand et al. 2020), Micrococcus 
(Nwankwegu and Onwosi 2017), Burkholderia (Morya et al. 2020), Bacillus (Banerjee 
et al. 2019), Shewanella (Zou et al. 2019), Xanthomonas (Xu et al. 2018) or Alcaligenes 
(Haouas et al. 2021). Of particular interest are the bacteria of the genus Brevibacillus 


Construction of residual sludge-based bioferilizer 159 

(Arya and K. Sharma 2015). They have pronounced bioremediation properties against 
various organic and inorganic pollutants (Wei et al. 2019; Jebril, Boden and Braun- 
gardt 2021). These microorganisms are also of particular interest due to the possibility 
of their bioremediation detoxification properties to be combined in microbial prepara- 
tions with the effect of protection against phytopathogens and enhancing plant growth 
(Ahmed et al. 2018). This study aims to explore the possibility of creating a bioferti- 
liser, based on activated sludge combined with a bacterial culture from g. Brevibacillus 
with detoxifying and possible plant growth-promoting properties. 

Materials and methods 

Experimental design 

The present study is focused on the exploration of the potential of a bacterial culture 
(Brevibacillus laterosporus BT271) for the creation of a biofertiliser with biodetoxifying 
properties. A combination of the highly-active bacteria with activated sludge that is 
conventionally used for the restoration of soil, will give added value to the future bio- 
product in the trend of the circular solutions. A waste (the residual activated sludge) 
will be transformed into a valuable biotechnological product. It can be applied for the 
restoration of the damaged environment. The here-described experiments include the 
first stages of development of such a product. The B. /aterosporus BT271 metabolic 
activity in the presence of a model xenobiotic (phenol) was evaluated. The volume of 
the used 14" hour bacterial culture in the experiments at this stage was 4%. Nutrient 
broth was used. The microorganisms were cultured at 30 °C and aerated. Phenol was 
added once at zero hour in the following five concentrations: 5 mg/l, 100 mg/l, 250 
mg/l, 500 mg/I and 1000 mg/l. Critical control points (CCPs) were set at 0 hour and 
6th hour. The metabolic activity of the combined residual activated sludge (rAS) and 
B. laterosporus BT271 was studied. Activated sludge weighing 0.5 g was used. Highly 
active biodegradant was added as fresh biomass, which is 10% of the weight of the 
activated sludge. The microorganism was cultured at 30 °C and aerated. Phenol was 
added once at zero hour in the following three concentrations: 5 mg/l, 250 mg/l and 
1000 mg/l. CCPs were also set at 0 hour and 6th hour. The metabolic activity of the 
combined residual activated sludge (rAS) and B. laterosporus BT271 was studied. The 
bacterial activity and the activity of the combination with rAS was estimated on the 
accumulation of the biomass, the total dehydrogenase activity of the microorganisms 
and the intoxication effects, determined with fluorescence and digital image analysis. 
Brevibacillus laterosporus BT271 — the bacterial culture was isolated from contami- 
nated soil close to an oil refinery (Lukoil Neftochim Burgas, Bulgaria) by Prof. Yana 
Topalova (Topalova 2009). This bacterial culture was adapted to the biodegradation of 
aryl-containing xenobiotics (phenol, nitrophenols, pentachlorophenol in high concen- 
tration). The culture possesses a broad spectrum of biodegradation activity towards 30 
different xenobiotics. The culture can survive in high percentage after lyophilisation and 
quickly recovered detoxification activity after re-hydration. The bacteria in our experi- 


160 Mihaela Belouhova et al. / BioRisk 17: 157-168 (2022) 

ments were kept as a lyophilised preparation prior to the experiments. They were culti- 
vated in Nutrient agar (HiMedia, India). For the experiments for the intoxication effects, 
18 h bacterial culture was used. 

Activated sludge 

The used activated sludge was residual activated sludge (rAS), treated with CaO (quick- 
lime) and ready for utilisation in agriculture. The rAS was taken from the WWTP on 
Sofia City, Bulgaria. 

Phenol 

The model toxicant used in the study was phenol since its derivatives are major envi- 
ronmental pollutants. It was supplied by Fluka Analytical (Switzerland). Five phenol 
concentrations in the range 5—1000 mg/I were used in the experiments. 

Methods 

The accumulation of the biomass was monitored by the optical density at 430 nm. The to- 
tal dehydrogenase activity was determined by the method of Lenhard (Lenhard et al. 1964). 
CTC/DAPI-based analysis was applied for determination of the bacterial metabolic 
activity and detection of changes in the morphology of the cells. It is based on the use of 
two fluorescent dyes. CTC or 5-cyano-2,3-ditolyl tetrazolium chloride is a tetrazolium 
salt that has no fluorescent properties. In the living cells, it is reduced to CT'C-formazan 
that emits a red fluorescence signal. In these experiments, it was used in 5 mM concen- 
tration. DAPI (4’,6-diamidino-2-phenylindole) is a fluorescent dye that binds DNA 
and emits a blue fluorescent signal. In concentration 1 ug/ml, it can be used as a staining 
method for all the biomass in the samples. By using CTC and DAPI simultaneously, 
information about the live cells in the whole sample was obtained. Fluorescence im- 
ages were taken by a “Leica” DMG6 B microscope. They were further processed with the 
software DAIME (Daims et al. 2006). The share of the live cells, their intensity and size 
(or the area of the cells) were calculated with the programme by using custom threshold 
segmentation. All the analyses were performed in three independent repetitions. 

Results 

In the experiments performed, the accumulation of biomass in B. laterosporus BT271 
under optimal conditions for development was studied. The Nutrient medium pro- 
vided a sufficient concentration of easily-degradable substrates and a lack of toxicants. 
The obtained results are illustrated in Fig. 1. The bacterial culture reaches its maximum 
number of cells at the 20" hour of its growth (3.25 x 107 cells/ml), after which it pass- 
es into a stationary phase of growth and a death phase. These data were also supported 
by the activity of dehydrogenase in the cells - the total dehydrogenase activity is highest 


Construction of residual sludge-based bioferilizer 161 

§ 3.50E-05 4.00E+07 
5 3.00E-05 § 
2 = 
= 2.00E-05 = 
Sh 2.00E+07 = 
= 1.50E-05 & 
A G 
Bee 1.00E+07 $ 
5.00E-06 Z. 
0.00E+00 0.00E+00 
0 2 4 6 8 10 12 14 16 18 20 22 24 
Time, h. 
mam D A487 em (1430 

Figure |. Biomass accumulation and total dehydrogenase activity (TDA) in B. laterosporus BT271 
(DA487 — dehydrogenase activity, measured at 487 nm; OD430 — optical density at 430 nm). 

at the 14" hour (exponential growth phase). The value of this indicator exceeds TDA 
at the beginning of cultivation by 69% and by 16% at the 24" hour of the culturing. 

In the further experiments for studying the detoxification properties of B. latero- 
sporus BT271, cultures in the late exponential phase (18 hours) were used. They had 
the maximum number of bacterial cells with the most active enzymes. 

In Fig. 2 A, the accumulation of biomass in B. daterosporus BT271 in the presence of 
five phenol concentrations is presented. The presented data show that the bacterial culture 
degrades phenol in wide range of concentrations - from 5 mg/l to 1000 mg/I. The number 
of cells in the presence of phenol reached 4.44 x 107 cells/ml in the presence of 5 mg/l 
phenol. The largest increase occurred when the microbial count was recorded at low con- 
centrations (16% for 5 mg/l and 13% for 100 mg/l). This is due to the lower inhibitory 
effect of the phenol in these concentrations. In contrast to the phenol experiments, in 
the cultivation of the bacterial culture in the absence of the phenol (control), a decrease 
of 3.25% was registered between the number of cells at 18 hours and 24 hours (Fig. 1). 

5 00E+07 m Oh. =6h. 1.00 BO0h. @6h. 
_34.00E+07 0.80 
§ 3.00E+07 % 0.60 ) 
8 2.00E+07 5 0.40 
~ 1.00E+07 v.20 iy 
0.00E+00 a ie eS 
‘ ° 2 
ws td i Ss s 
A B 

Figure 2. Change of the biomass accumulation in: A B. /aterosporus BT271 and B B. laterosporus BT271 
and rAS in presence of phenol in concentrations 5—1000 mg/I. 


162 Mihaela Belouhova et al. / BioRisk 17: 157-168 (2022) 

At the highest phenol concentrations, an increase in accumulated biomass was also 
found, although significantly less - 3.4% for 500 mg/l and 2.5% for 1000 mg/I phenol. 

In addition to determining the biomass accumulated from B. /aterosporus BT271 
in the presence of phenol, the change in absorbance when combining the bacterial 
culture with activated sludge for recovery was also investigated. This information can 
be used as an indirect indicator for the increase in biomass of the target detoxification 
culture. The obtained data are illustrated in Fig. 2B. At the high concentrations of the 
phenol, a significant increase was registered (average 34%). It is greatest at the addition 
of 250 mg/I phenol, but remains significant even at 1000 mg/l phenol. 

The metabolic activity of the bacteria in the presence of phenol was determined, 
based on the total dehydrogenase activity. The results obtained showed that, in B. lat- 
erosporus BT271, there is a significant activation of metabolic processes in the presence 
of phenol (Fig. 3A). At the beginning of the experiment, the measured TDA was from 
1.06 x 10° ng H*/ml*min to 1.06 x 10% pg H*/ml*min. After 6 hours of incubation, 
the values of this indicator increased from 7.58 x 10° ug H*/ml*min to 5.74 x 10% ug 
H*/ml*min. The highest increase was registered when 5 mg/| phenol was present - 7.3 
times. It was lowest when 1000 mg/! phenol was applied - 2.7 times. 

Fig. 3B represents the data on TDA for the combination of the highly active mi- 
croorganisms B. laterosporus BT271 with activated sludge for recovery. At the begin- 
ning of the experiment (0 h.), the values of this indicator were very low - they were at 
the lower limit of detection for this method. The only exception was the higher activity 
recorded in bacteria with the addition of 250 mg/l phenol. This is most likely due to 
the rapid activation of bacterial metabolism in the presence of this intermediate con- 
centration of the toxicant. 

After incubation for 6 hours, an increase in the activity of microorganisms was 
registered in all tested variants. ‘This is from 30% (at 250 mg/I phenol) to 32 times (at 
the highest concentration of the toxicant). The effect recorded in the activated sludge 
controls was most likely due to the rehydration of the cells in the activated sludge and 
their incubation at the optimum temperature (30 °C). 

The analysis of the metabolic activity, based on CTC, showed that, at most of the 
used concentrations, a slight decrease in the indicator was registered (on average by 14%) 

eae 8.00E-06 
3 = mOh. mh. a 
= 6.00E-04 E 6.00E-06 : 
i a wig 
@ 4.00E-04 E 4.00E-06 _—, 
= =m 2 = Ne 
e2.00E-04 3 2.00E-06 ra a 
"0.00E+00 LEN , 
| Vv & & Y ae SY Ss 
Ry Ss © © a) x zs ws $ 
oS RS oS S&S s& e y 6S 
va P ns Py 
A B 

Figure 3. Total dehydrogenase activity in A B. laterosporus BT271 and B B. laterosporus BT271 and rAS 
in presence of phenol in concentrations 5—1000 mg/l. 


Construction of residual sludge-based bioferilizer 163 

zB 200 m Oh. 6h. 250 0h. =6h. 
EF 150 —— i E 200 
E I z 150 ale af ds 
. fad a 
2 100 : Re | = 
S | (Hs | 5 100 Ea ia 
= & 50 be 
po Lo 
= " i 
AM mY e my Re rAS rAS+S5mg/L 250 1000 
2 ee ne ee BT271 mg/L mg/L 

Figure 4. Fluorescence intensity in A B. laterosporus BT271 and B B. laterosporus BT271 and rAS after 
6-hour incubation in presence of phenol. 

(Fig. 5). The difference in the fluorescence intensity of CTC varies from 3% (at 5 mg/| 
phenol) to 35% (at 1000 mg/l). An increase in fluorescence intensity (by 4%) was found 
only at a phenol concentration of 250 mg/l. The differences in the results obtained with 
the T[C-based method are most likely related to the differences in methodology. The 
CTC method provides information directly about the individual cells in the samples. The 
information from the TTC method represents the activity of all bacteria in the sample. 
It is based on the extracted formazan, the concentration of which is determined spectro- 
photometrically. Additionally, in the TTC-TDA analysis, an easily degradable substrate 
is added (glucose). This activates the metabolism of the cells. The data from this analysis 
can be considered as information about the metabolic activity of certain microorganisms 
at the optimal concentration of the dehydrogenase substrate. On the other hand, the 
CTC method shows the metabolic activity of the cells directly under the conditions of 
the experiment, i.e. not to what extent their metabolic functions are preserved (as in the 
TTC-TDA method), but to what extent they are active in the conditions of intoxication. 

Thus, it is clear that, in the presence of phenol in different concentrations, the bacte- 
rial culture B. laterosporus BT271 had high metabolic activity, estimated as TDA, based 
on the reduction of TTC. However, under the conditions of the experiment, the activity 
of the culture decreased slightly after the 6-hour incubation with phenol. An exception 
was the concentration of 250 mg/l, at which higher fluorescence intensity was detected 
(Fig. 4A). In addition, it showed an increase in the average cell size (by 44%). At the same 
time, at the highest concentration used (1000 mg/l), there was a decrease in intensity by 
34% and a decrease in cell area by 86% - an indication of intoxication changes in bacte- 
rial cells at this concentration. 

In Fig. 6, fluorescent pictures of CTC staining of the residual activated sludge before 
and after the inclusion of B. daterosporus BT271 bacteria are shown. ‘The images represent 
the increased number of living cells after the addition of bacteria. The data obtained were 
confirmed by the fluorescence intensity after 6 hours of incubation. It is 73% higher in 
the presence of 250 mg/I phenol. The highest concentration of the toxicant increased 
the metabolic activity of the microorganisms by 48% (Fig. 4B). These results were also 
confirmed by the TTC method for the determination of TDA. 


164 Mihaela Belouhova et al. / BioRisk 17: 157—168 (2022) 

Ee boo. 

Figure 5. CT'C/DAPI staining of B. laterosporus BT271 in the presence of 5 mg/I phenol: A 0 h; B after 

6 hours of incubation. 

; of 

Figure 6. CTC staining demonstrating the bacterial abundance and metabolic activity in: A residual 
activated sludge; B residual activated sludge with added B. /aterosporus BT271. 

In both methods used to study the metabolic activity of microorganisms in the 
combination of activated sludge and B. laterosporus BT271, the lowest effect was re- 
corded in the presence of 5 mg/I phenol. 

The results of the CTC analysis also show an increase in the metabolic activity of the 
sludge after rehydration (the control with activated sludge only). In this experimental 
result, an increase in metabolic activity by 36% was found. The data obtained showed 
that, when B. /aterosporus BT 271 was added to this sludge at the highest concentrations 
used (250 mg/l and 1000 mg/l), a significantly higher increase was achieved compared 
to the rehydrated sludge alone (61% on average). ‘This is indicative of the high biode- 
toxification potential of the combination of activated sludge and B. laterosporus BT271. 

Discussion 

The data discussed in the Results section showed that the combination of activated 
sludge and bacterial culture of Brevibacillus laterosporus BT271 has a high potential 
for use in biodetoxification procedures. These are required for environmental pollu- 
tion with various pollutants. Soils have been identified by the EU as a resource that 
must be protected and purified because of their critical importance for “human health, 
the state of the economy and the production of food and new medicines” (European 


Construction of residual sludge-based bioferilizer 165 

Commission 2020). One of the most common techniques for soil decontamination 
(bioremediation) is bioaugmentation - the addition of highly active biodegradants to 
eliminate the respective contamination. Numerous bacterial genera have been identi- 
fied as suitable for use in bioremediation procedures — Bacillus (Hsieh et al. 2020), 
Pseudomonas (Alhefeiti et al. 2021), Shewanella (Zou et al. 2019), Xanthomonas (Xu et 
al. 2018), Alcaligenes and Brevibacillus (Arya and K. Sharma 2015) and others. 

The high potential for application of Brevibacillus bacteria was also confirmed in 
the experiments of the present study. B. laterosporus BT271 increased in number de- 
spite the inhibitory effect of phenol applied in five increasing concentrations (5—1000 
mg/l) (Fig. 2). At the lowest concentrations of the toxicant, its inhibitory effect was the 
weakest and the increase in the quantity of the detoxification culture was up to 16%. At 
the highest concentration (1000 mg/l), it was 3%. At the same time, during the cultiva- 
tion on the Nutrient medium, a decrease of the biomass was registered at the 24" hour. 
The data obtained demonstrate that the culture can use the toxic phenol as a carbon 
source at all applied concentrations, which increases the number of cells, respectively 
the accumulation of the biomass of the detoxifying bacterial culture. Other authors 
also have established the applicability of Brevibacillus in the biodegradation and biore- 
mediation of phenol and phenolic derivatives (Abu Talha et al. 2018; Wei et al. 2019). 

In addition to specially-selected bacterial cultures, in practice, activated sludge 
from wastewater treatment plants is traditionally used as a biofertiliser. It is formed 
in the course of water purification after which it is subjected to stabilisation and de- 
contamination and can be applied directly to soil enrichment in agricultural and bi- 
oremediation procedures (Bitton et al. 2016). Activated sludge is traditionally used 
for fertilisation because it is a natural source of nutrients (Abdollahinejad et al. 2020). 
When these sludges are enriched with an appropriate amount of biomass from micro- 
bial cultures with detoxifying properties, biofertiliser with combined valuable proper- 
ties is obtained - for enrichment of the soil and soil fertility and simultaneous disposal 
of residual toxic contaminants in the soil. 

The targeted combination of mineralised sludge and the detoxification culture of 
B. laterosporus BT271 in the present study resulted in a very good result in terms of 
activity of the metabolic processes. As commented in the “Results”, the combination 
with activated sludge and B. laterosporus BT271 \ed to an increase in biomass accumu- 
lation by up to 47%. The low effect found in the controls and at 5 mg/I phenol is most 
likely due to the lack of sufficiently easily-degradable nutrient sources. 

The presence of phenol in different concentrations has an effect, not only on the ac- 
cumulation of biomass, but also on the activity of bacteria, both only on B. /aterosporus 
BT271 and in the combination of these microorganisms with the activated sludge. ‘The 
rate of metabolic transformations increased from 2.7 to 7.3 times in the presence of 
phenol. When combining the highly-active microorganisms with activated sludge and 
the effect of phenol in a concentration of 1000 mg/l, it causes an increase in metabolic 
activity by 32 times. This result, as well as the rapid activation of metabolic processes 
and the high value of TDA at 250 mg/I phenol, are an indication of the prospects for the 
combination of activated sludge and B. laterosporus BT271 for the creation of biofertilis- 
er with valuable combined properties for soil detoxification and increase in soil fertility. 


166 Mihaela Belouhova et al. / BioRisk 17: 157-168 (2022) 

Fluorescence analysis showed that, although the individual B. /aterosporus BT271 
cells decreased their activity after the addition of phenol, in the presence of activated 
sludge the total activity of the system increased by up to 73%. Thus, the use of prepara- 
tion with B. laterosporus BT271 and activated sludge in bioremediation activities could 
achieve a high rate of elimination of toxicants and, at the same time, would influence 
the soil fertility in a favourable direction in a way close to nature according to the rules 
of the circular economy and the principle “nature knows best”. 

Conclusion 

The results, presented so far, were focused on the study of the prospects for the creation of 
biofertiliser with combined activated sludge and specially-selected microorganisms with de- 
toxifying activity (B. laterosporus BT271). They showed that the accumulation of biomass 
and bacterial metabolic activity not only remain high, but also increased by 32 times in the 
presence of phenol in high concentrations (up to 1 g/l). This suggests that the application 
of the preparation with AS and B. laterosporus BT271 will have accelerated biodegradation 
in areas contaminated with xenobiotics with a cyclic structure (phenol and phenolic deriva- 
tives). It will be possible to use the synergistic effect of the introduction of nutrients (in the 
form of activated sludge) and specially-selected biodegradants of xenobiotics (B. laterospo- 
rus BT271), which also have protective properties against plants. Further experiments will 
be continued in the direction of testing the preparation in conditions close to the real ones. 

Acknowledgements 

This investigation has been supported financially by Operational Programme ‘Science and 
education for smart growth’, co-financed by the European Union through the European 
structural and investment funds, project BGO5M2OP001-1.002-0019: “Clean Technolo- 
gies for Sustainable Environment - Waters, Waste, Energy for a Circular Economy’. 

References 

Abdollahinejad B, Pasalari H, Jafari AJ, Esrafili A, Farzadkia M (2020) Bioremediation of diesel 
and gasoline-contaminated soil by co-vermicomposting amended with activated sludge: Die- 
sel and gasoline degradation and kinetics. Environmental Pollution 263: 114584. https://doi. 
org/10.1016/j.envpol.2020.114584 

Ahmed AIS, Omer AM, Ibrahim AI, Agha MK (2018) Brevibacillus spp. in agroecology: The 
beneficial impacts in biocontrol of plant pathogens and soil bioremediation. Fungal Genom- 
ics & Biology 08(02): e5. https://doi.org/10.4172/2165-8056. 1000157 

Alhefeiti AM, Athamneh K, Vijayan R, Ashraf SS (2021) Bioremediation of various aromatic and 
emerging pollutants by bacillus Cereus sp. isolated from petroleum sludge. Water Science and 

Technology 83(7): 1535-1547. https://doi.org/10.2166/wst.2021.065 


Construction of residual sludge-based bioferilizer 167 

Arya R, Sharma AK (2015) Bioremediation of Carbendazim, a benzimidazole fungicide using 
Brevibacillus Borstelensis and Streptomyces Albogriseolus together. Current Pharmaceutical 
Biotechnology 17(2): 185-189. https://doi.org/10.2174/1389201016666150930115737 

Banerjee S, Misra A, Chaudhury S, Dam B (2019) A bacillus strain tcl isolated from Jharia coalmine 
with remarkable stress responses, chromium reduction capability and bioremediation potential. 
Journal of Hazardous Materials 367: 215-223. https://doi.org/10.1016/j.jhazmat.2018.12.038 

Banov M, Rousseva S, Pavlov P (2020) Sustainable management and restoration of the fertility of 
damaged and contaminated lands and soils. In: Meena RS (Ed.) Soil Health Restoration and 
Management. Springer, Singapore, 113-59. https://doi.org/10.1007/978-98 1-13-8570-4_4 

Bitton G, Malek A, Zullo LC, Daoutidis P (2016) Wasterwater Microbiology. Industrial & Engi- 
neering Chemistry Research 55(12): 3327-3337. https://doi.org/10.102 1/acs.iecr.5b03209 

Daims H, Liicker $, Wagner M (2006) Daime, a novel image analysis program for microbi- 
al ecology and biofilm research. Environmental Microbiology 8(2): 200-213. https://doi. 
org/10.1111/.1462-2920.2005.00880.x 

Dimkov R, Topalova Y, Schneider I (2017) Ecological Biotechnology. Pensoft, Sofia, 376 pp. 

European Commission (2019) The European Green Deal. European Commission 53(9): 24. 
https://doi.org/10.1017/CBO978 1 107415324.004 

European Commission (2020) Communication from the Commission to the European Parlia- 
ment, the Council, the European Economic and Social Committee and the Committee of 
the Regions, EU Biodiversity Strategy for 2030. https://op.europa.eu/en/publication-detail/-/ 
publication/a3c806a6-9ab3-1 lea-9d2d-01aa75ed71al/language-en 

European Commission (2021) COM(2021) ANNEXES 1 to 2; EU Action Plan: “Towards Zero 
Pollution for Air, Water and Soil’. https://ec.europa.eu/environment/strategy/zero-pollution- 
action-plan_bg 

Gray NF (2010) Water technology. An introduction for environmental scientists and engineer. 
Elsevier, Netherlands, 768 pp. 

Haouas A, Modafar CE, Douira A, Ibnsouda-Koraichi S, Filali-Maltouf A, Moukhli A, Amir S 
(2021) Alcaligenes Aquatilis GTE53: Phosphate solubilising and bioremediation bacterium 
isolated from new biotope ‘phosphate sludge enriched-compost’. Saudi Journal of Biological 
Sciences 28(1): 371-379. https://doi.org/10.1016/j.sjbs.2020.10.015 

Hong X, Zhao Y, Zhuang R, Liu J, Guo G, Chen J, Yao Y (2020) Bioremediation of tetracycline 
antibiotics-contaminated soil by bioaugmentation. RSC Advances 10(55): 33086-33102. 
https://doi.org/10.1039/D0RA04705H 

Hsieh HY, Lin C, Hsu S, Stewart GC (2020) A bacillus spore-based display system for biore- 
mediation of atrazine. Applied and Environmental Microbiology 86(18): e13. https://doi. 
org/10.1128/AEM.01230-20 

Jebril N, Boden R, Braungardt C (2021) ‘The isolation and identification of cadmium-resistant 
Brevibacillus Agri C15. Journal of Physics: Conference Series 1879(2): 022015. https://doi. 
org/10.1088/1742-6596/1879/2/022015 

Koolivand A, Abtahi H, Villasefor J, Saeedi R, Godini K, Parhamfar M (2020) Effective scale- 
up of oily sludge bioremediation from a culture-based medium to a two-phase composting 
system using an isolated hydrocarbon-degrading bacterium: Effect of two-step bioaugmen- 
tation. Journal of Material Cycles and Waste Management 22(5): 1475-1483. https://doi. 
org/10.1007/s10163-020-01036-z 


168 Mihaela Belouhova et al. / BioRisk 17: 157-168 (2022) 

Laothamteep N, Naloka K, Pinyakong O (2022) Bioaugmentation with zeolite-immobilized bac- 
terial consortium OPK results in a bacterial community shift and enhances the bioremedia- 
tion of crude oil-polluted marine sandy soil microcosms. Environmental Pollution 292(Part 
A): e118309. https://doi.org/10.1016/j.envpol.2021.118309 

Lenhard G, Nourse LD, Scwartz M (1964) The measurement of dehydrogenase activity of acti- 
vated sludge. Proc. 2"4 International Conference on Water Pollution Research. 

Li H, Li Y, Bao M, Li S (2021) Solid inoculants as a practice for bioaugmentation to enhance 
bioremediation of hydrocarbon contaminated areas. Chemosphere 263: e128175. https:// 
doi.org/10.1016/j.chemosphere.2020.128175 

Meuser H (2013) Rehabilitation of soils in urban environments. In: Soil Remediation and 
Rehabilitation. Environmental Pollution, vol 23. Springer, Dordrecht, 5-36. https://doi. 
org/10.1007/978-94-007-5751-6_2 

Morya R, Salvachia D, Thakur IS (2020) Burkholderia: An untapped but promising bacterial 
genus for the conversion of aromatic compounds. Trends in Biotechnology 38(9): 963-975. 
https://doi.org/10.1016/j.tibtech.2020.02.008 

Nwankwegu AS, Onwosi CO (2017) Bioremediation of gasoline contaminated agricultural 
soil by bioaugmentation. Environmental Technology & Innovation 7: 1-11. https://doi. 
org/10.1016/j.eti.2016.11.003 

Ramadass K, Megharaj M, Venkateswarlu K, Naidu R (2018) Bioavailability of weathered hy- 
drocarbons in engine oil-contaminated soil: Impact of bioaugmentation mediated by Pseu- 
domonas spp. on bioremediation. The Science of the Total Environment 636: 968-974. 
https://doi.org/10.1016/j.scitotenv.2018.04.379 

Talha A, Goswami M, Giri BS, Sharma A, Rai BN, Singh RS (2018) Bioremediation of congo red 
dye in immobilized batch and continuous packed bed bioreactor by Brevibacillus Parabrevis 
using coconut shell bio-char. Bioresource Technology 252: 37—43. https://doi.org/10.1016/). 
biortech.2017.12.081 

Topalova Y (2009) Biological control and management of wastewater treatment. Pensoft, Sofia. 

Varjani S, Upasani VN (2019) Influence of abiotic factors, natural attenuation, bioaugmentation 
and nutrient supplementation on bioremediation of petroleum crude contaminated agricul- 
tural soil. Journal of Environmental Management 245: 358-366. https://doi.org/10.1016/). 
jenvman.2019.05.070 

Wei K, Hua Y, Hui P Guining L, Zhi D (2019) Bioremediation of triphenyl phosphate in river 
water microcosms: Proteome alteration of Brevibacillus Brevis and cytotoxicity assessments. 
The Science of the Total Environment 649: 563-570. https://doi.org/10.1016/j.scito- 
tenv.2018.08.342 

Xu X, Liu W, Tian S$, Wang W, Qi Q, Jiang P, Gao X, Li EK Li H, Hongwen Y (2018) Petroleum 
hydrocarbon-degrading bacteria for the remediation of oil pollution under aerobic condi- 
tions: A perspective analysis. Frontiers in Microbiology 9: e2885. https://doi.org/10.3389/ 
fmicb.2018.02885 

Zou L, Yun-hong H, Zhong-er L, Yan Q (2019) On-going applications of Shewanella species 
in microbial electrochemical system for bioenergy, bioremediation and biosensing. World 
Journal of Microbiology & Biotechnology 35(1): e9. https://doi.org/10.1007/s11274- 
018-2576-7