Introduction

In many African countries where the livestock sector plays a prominent role in the economy especially for the rural population, animal diseases constitute one of the main hindrances (Mthi et al. 2018; Bolajoko et al. 2020). Animal diseases limit livestock production and productivity with significant impacts on animal health, public health and economies (McElwain and Thumbi 2017; Chakale et al. 2021). Indeed, in these regions, livestock act as a “bank” for the provision of cash derived from sales of their products or of the animals themselves in times of crisis, to raise funds needed to purchase food and meet other family needs.

In some areas of those countries (i.e. South Africa, Far North of Cameroon), because of the lack of access to veterinary drugs, and their mobility, many pastoralists use traditional medicines for preventing and managing animal diseases (Chitura et al. 2018). In fact, this traditional practice is continuing because pastoralists believe that medicinal plants are efficient, available and easily accessible and animal health is a prerequisite for higher productivity (FAO (Food and Agriculture Organization of the United Nations), 2013; Vougat et al. 2015). Researchers are working on this subject matter to actually confirm the potential of the plants used by livestock farmers (Mostafa et al. 2018; Nordin et al. 2019). The increasing focus on natural products might be due to their reduced or non-cytotoxicity or low side effects compared with chemically synthesized drugs (Hyun et al. 2013). In addition, plant extract usage represents an important alternative for the reduction of the use of drugs like antibiotics, known to be the main trigger of the development and spread of antimicrobial resistance, a major global threat to human health (Dadgostar, 2019; Varona et al. 2020). That is especially important for developing countries like Cameroon where stringent policies on antibiotic use are not fully in place (Mouiche et al. 2018).

Unfortunately, in Cameroon where livestock contributes significantly to the gross national product (MINEPIA 2009), no sufficient attention is focused on ethnoveterinary medicine. It is common knowledge that in the Far North region of Cameroon, the region that has the second highest cattle population in the country, many cattle farmers and specially pastoralists treat their animals with plant extracts (Vougat et al. 2015; MINEPIA, 2019 unpublished). Due to the increasing importance of such medicine to cattle farmers, our research team seeks to analyse the plants used to control and treat animal diseases. Our previous study in the Far North region of Cameroon consisted of investigating the plants used against one of the most common, frequent and recognizable infectious diseases (Foot and Mouth Disease or FMD) and evaluating the phytochemical composition and antioxidant potentials of the two mostly used (Boscia senegalensis and Tapinanthus dodoneifolius) (Vougat et al. 2015). Thus, this study aims to deepen the scope of analysis on these two plants which have a good phytochemical profile (Vougat et al. 2015; Idu et al. 2016). Both plants are also used in many countries to treat animal and human diseases (FMD, respiratory tract infections, stomach ache, diarrhoea, dysentery, diabetes, epilepsy, hepatitis in humans) (Vougat et al. 2015; Mamman et al. 2019; Mohamed et al. 2020a).

Therefore, with due knowledge of their profile and immense importance, this study was designed to evaluate the antibacterial, non-cytotoxic and antioxidant potentials of B. senegalensis and T. dodoneifolius. Antimicrobial activity is first screened because antibiotic drugs are the main veterinary medicine used by pastoralists in the study area (Vougat Ngom et al. 2017). The cytotoxic activity was evaluated to verify the safety of these plants.

Study area

The plants analyzed in this study were collected in the Far North region of Cameroon as previously described (Vougat et al. 2015). In Cameroon, pastoralists are mainly located in three regions (North West, Adamawa and Far North regions) (Kelly et al. 2016; Motta et al. 2018) where more than 80% of the national cattle, sheep and goat population are found (MINEPIA, 2009 Not published). However, due to its climate conditions, the Far North region has the majority of pastoralists of the country. This region is characterized by a Sudano-Sahelian climate. The average annual rainfall in this region is about 700 mm. The temperatures are generally low in the rainy season and the nights in the dry season between December and January (Dassou et al. 2015).

Methods

Preparation of plant extracts

T. dodoneifolius was collected from the host plant Acacia albida as a study has shown that the properties of T. dodoneifolius depended on its host plant (Idu et al. 2016). These plants were then identified and authenticated in the National Herbarium in Yaoundé (Cameroon) where the voucher specimens already existed under the reference numbers 23137 SRF/Cam and 50271 HNC respectively for B. senegalensis and T. dodoneifolius. The extraction of both plant samples was done according to the scheme below (Fig. 1). Each partition was obtained after washing three times with the solvent. Each dried fraction was kept in a freezer before biological tests.

Fig. 1
figure 1

Scheme of the extraction

Antibacterial assay

The antibacterial activity of both plants was evaluated by using both qualitative and quantitative methods.

Selected test bacteria

Three bacterial strains were used for the study: Escherichia coli (ATCC 25922), Staphylococcus aureus (ATCC 29213) and an in house fully characterized Salmonella typhimurium. These bacteria are among the most common foodborne bacteria in animal source food that cause a variety of diseases in humans and animals (Rortana et al. 2021). Bacterial strains were grown and maintained on Trypticase Soy Agar with 5% Sheep Blood plates (BD BBM™ Becton, Dickinson and Company, Sparks, USA). Bacterial suspensions of 0.5 McFarland were prepared with sterile saline solution to inoculate plates during the antibacterial assay.

Extracts re-suspension and paper disc preparation

Sterile saline solution was used to dissolve extracts of B. senegalensis obtained with methanol and water. For the other extracts (hexane and chloroform extracts of B. senegalensis and all the T. dodoneifolius extracts), 15% dimethyl sulfoxide (DMSO) (Thermo Fisher Scientific Inc., Pittsburgh, USA) was used (Kawo et al. 2011; Kpadonou-Kpoviessi et al. 2013). Each extract was prepared to yield a stock concentration of 100 mg/ml. After dilution of the stock solution, seven final concentrations (0.001, 0.01, 0.1, 1, 5, 10 and 20 mg/ml) of each sample were used to be tested against a bacterial suspension. Sterile filter paper discs of 6 mm in diameter (BD BBM™ Becton, Dickinson and Company, Sparks, USA) were impregnated with 50 μl of each concentration to give a respective final amount of 5 × 10−5, 5 × 10−4, 5 × 10−3, 5 × 10−2, 0.25, 0.5 and 1 mg/disc. A sterile paper disc prepared in the same condition with 50 μl of only solvent used for the corresponding extract was used as a negative control. Discs were allowed to dry at 37 °C for 24 h (so as to remove residual solvent, which might interfere with the determination).

Agar disk diffusion assay

Antimicrobial activities of the different extracts were screened for their inhibitory zone by the agar disc diffusion method as described elsewhere (Gautam et al. 2013). Briefly, Mueller Hinton Agar medium plates (BD Difco™ Becton, Dickinson and Company, Sparks, USA) were inoculated with a bacterial suspension at 0.5 McFarland, and discs with extract were placed on the surface of the agar. Plates were incubated at 37 °C for 24 h. The results were recorded by measuring the zone of growth inhibition (mm) surrounding the discs. Each concentration was tested in duplicate. The results of the diameters of the zones of inhibitions of extracts were interpreted as sensitive (> 18 mm), intermediate (14–17 mm), and resistant (< 14 mm) (Mohamed et al. 2020b).

Broth dilution method

The minimum inhibitory concentration (MIC), which is considered as the lowest concentration of the sample which inhibits the visible growth of a microbe, was determined by the broth dilution method. A dilution method (Elof 2004) was followed for the determination of MIC values with few modifications. Briefly, for each extract, different volumes of the stock solution were added to tubes containing different volumes of Trypticase Soy Broth (BD BBM™ Becton, Dickinson and Company, Sparks, USA) to obtain the concentrations of 0.001, 0.01, 0.1, 1, 5, 10 and 20 mg/ml. Thereafter, 20 μl inoculum (for bacteria 1 × 105 CFU/ml) was added to each tube. A tube containing 300 μl of TSB, 200 μl of solvent used for extract dilution and 20 μl inoculum was used as a negative control. Each concentration was assayed in duplicate. All the tubes were then incubated at 37 °C for 24 h. After incubation, the tubes were then examined for microbial growth by observing for turbidity. The MIC values were taken as the lowest extract concentration that showed no turbidity after incubation.

Cytotoxicity activity

Human colon cancer cells (HT-29) were obtained from the American Type Culture Collection (ATCC catalogue no. HTB-38). Colon cancer cells were cultured in RPMI 1640 medium (Hyclone) containing 100 μg/ml streptomycin, 100 units/ml penicillin, 0.25 μg/ml amphotericin B (Fungizone) and 10% fetal bovine serum (FBS). The cell line was cultured at 37 °C in a humidified incubator of an atmosphere of 95% air and 5% CO2. Cells were trypsinized and split for subculture when they reached near-confluent state (5 days). Cells are typically grown to 60–70% confluence, the medium was then changed and the cells were used for test procedure 1 day later according to the method described by Skehan et al. (1990) and Pan et al. (2010).

Antioxidative assay

The antioxidant assay was evaluated for the extracts that showed good results during antimicrobial and cytotoxicity analyses. The experiments were conducted in triplicate.

DPPH radical scavenging activity

The antioxidant activities of the samples were measured by determining the radical scavenging ability using the stable 2,2-diphenyl-1-picrylhydrazyl (DPPH) radical as described by Tepe et al. (2005). The activity of each extract was represented by the IC50 parameter (substrate concentration required to cause the loss of 50% of the initial concentration of DPPH), and vitamin C was used as standard.

Ferrous ion chelating capacity

The chelation of iron ions (II) was studied as described by Suter and Richter (2000) with minor modifications. The reaction solution containing 100 μl (2 mM) ferrous chloride and 400 μl (5 mM) potassium ferricyanide as reagent was prepared. A 200-μL test sample of the extract at various concentrations ranging from 2 to 10 mg/mL was prepared in different test tubes. Double distilled water was added to each test tube to a 1-ml level and mixed. The above reagent was then added, and the reaction mixture was incubated at 20 °C for 10 min. The formation of the potassium hexacyanoferrate complex was measured at 700 nm using a spectrophotometer. The assay was carried out at 20 °C to prevent Fe2+ oxidation. Lower absorbance indicated a higher iron chelating capacity. The negative control was without any chelating compound or test sample of extract. Ethylenediaminetetraacetic acid (EDTA) used as a control was prepared in the same way as the test samples and treated with the same reagent. The per cent of ferrous ion chelating capacity was calculated accordingly by comparing the absorbance of the test samples with that of the negative control.

Ferrous ion chelating capacity = [(A controlA extract)/A control] × 100

Acontrol is the absorbance of the negative control, and Aextract is the absorbance of the extract solution.

Statistical analysis

For the antioxidant activity of the plant extracts, data were presented as mean ± standard deviation. One-way analysis of variance followed by Duncan’s multiple range test was performed using Statgraphics 5.0. (Windows, www.statgraphics.com) to compare these data. But for the antimicrobial assay where a comparison was not needed, MIC are presented as mean. The IC50 (median growth inhibitory concentration) values of test samples for the cytotoxicity assay in serial dilutions were calculated using non-linear regression analysis (Table curve2Dv4; AISN Software, Inc., Mapleton, OR). The significance level was fixed at 0.05 for all the statistical analyses.

Results

Antibacterial activity of plant extracts

Tables 1 and 2 show the results of MIC determination of the test bacteria. At all the concentrations, chloroform, methanol and water extracts of B. senegalensis did not inhibit the growth of the bacteria studied. The same result was observed for all the extracts of T. dodoneifolius at 1, 0.1, 0.01 and 0.001 mg/ml. A conclusion of the bacterial growth in the tubes containing the hexane extract of B. senegalensis at 20, 10 and 5 mg/ml was not clear because before adding inoculum, the tubes were turbid. Therefore, this was not easy to know if they were the growth of bacteria or not. This was also observed in the tubes containing S. aureus and water or methanol extracts of T. dodoneifolius at 20, 10 and 5 mg/ml. The same results were found in the tubes containing S. aureus and hexane or chloroform extract of the same plant at 20 and 10 mg/ml.

Table 1 Minimum inhibitory concentration (MIC) of B. senegalensis on the test bacteria
Table 2 Minimum inhibitory concentration (MIC) of T. dodoneifolius on the test bacteria

The summarized results of the antibacterial susceptibility test of B. senegalensis and T. dodoneifolius against the test bacteria are presented in Tables 3 and 4, respectively. Hexane extract of B. senegalensis was the most effective, and the highest activity was demonstrated at 20 mg/ml (16 mm zone of inhibition), followed by 10 mg/ml (14.75 mm) and 5 mg/ml (13.25 mm) against Gram-positive bacteria. The methanol extract of T. dodoneifolius shows the highest activity against the same microorganism at 20 mg/ml (10 mm).

Table 3 Antibacterial activity of T. dodoneifolius on the test bacteria
Table 4 Antibacterial activity of B. senegalensis on the test bacteria

Cytotoxicity assay of the plant extracts

Four extracts of each plant sample were evaluated for their cytotoxicity against human colon cancer cells (HT-29) in vitro, and the results are presented in Table 5. All the extracts showed an IC50 significantly higher than 40 μg/ml.

Table 5 IC50 of T. dodoneifolius and B. senegalensis on human colon cancer cells (HT-29)

Antioxidant analysis

The antioxidant capacity of the extracts studied is shown in Table 6. From this table, it appears that the scavenging activity extract of B. senegalensis (28.80 ± 1.18 μg/ml) is significantly higher than that of vitamin C (107.65 ± 3.72 μg/ml) and T. dodoneifolius (767.28 ± 2.78 μg/ml).

Table 6 IC50 (μg/ml) value of different extracts

The chelating of Fe2+ by extracts was estimated, and the extent to which an extract can form complexes with the ferrous ion reflects its antioxidant activity. The IC50 of EDTA (0.50 ± 0.12 μg/ml) was significantly lower than that of the hexane extract of B. senegalensis (3.36 ± 0.10 μg/ml).

Discussion

The determination of the MIC of B. senegalensis showed that the chloroform, methanol and water extracts at all concentrations have no activity against the bacteria studied. The same result was found by Aliyu et al. (2008). However, this is in contradiction with Prashant et al.’s (2011) review. Indeed, according to them, these tree solvents are used for the extraction of antibacterial compounds in plant materials. However, the results of the hexane extract at 20, 10 and 5 mg/ml were difficult to be appreciated.

The results of the antibacterial activity of both plants showed that only one extract of each plant (hexane extract of B. senegalensis and methanol extract of T. dodoneifolius) has a significant activity against the strain of Gram-positive bacteria S. aureus. As this plant is commonly used again FMD in Far North of Cameroon, this result could suggest that the opportunistic bacterial diseases that affect animals infected by FMD could be due to Gram-positive bacteria. This is in correlation with the fact that the main veterinary drugs used by the pastoralists in this study area to manage cattle infected by the said disease consist of penicillin G (Vougat Ngom et al. 2017), an antibiotic belonging to the class with the action spectrum encompasses mainly Gram-positive bacteria (Lobanovska and Pilla 2017).

B. senegalensis activity against S. aureus demonstrated in this work is similar with the results found by Aliyu et al. (2008) who showed its activity against S. aureus resistant to methicillin, an antibiotic belonging to the class of penicillins M. This coherence of results could support the hypothesis that the hexane extract of B. senegalensis contain molecules which have the same mechanism of action like penicillins. This argument could be supported by the proximity between the diameter of the inhibition zone (16 mm) of B. senegalensis found in this work and those obtained by the authors cited above (19 mm). The similarity in the phytochemical composition of the extracts used during the study of Aliyu et al. (2008) is their compositions in tannins, saponins and alkaloids, compounds known to have antibacterial properties (Prashant et al. 2011). Taking into consideration the antioxidant properties found and the properties of the organic solvent used for the extraction, the antibacterial activity observed can be the result of those compounds.

The antibacterial activity of the methanol extract of T. dodoneifolius against S. aureus is similar with the finding of Deeni and Sadiq during the study they conducted in Northern Nigeria (Deeni and Sadiq 2002). This similarity could be justified by its high content of phenolic compounds and other compounds known for their antibacterial activities (Tavassoli and Djomeh 2011). Contrary to our results, the work of Ndamitso et al. (2013) showed that this methanol extract has a low activity. This difference could be referred to the different parts of the plants studied and their host plants. Indeed it has already been shown that the properties of this hemiparasitic plant depend on its host (Deeni and Sadiq 2002).

The non-cytotoxic effect of the methanol, hexane, water and chloroform extract of B. senegalensis and T. dodoneifolius was evaluated in vitro to assure their safety. This potential has been demonstrated using the colon cancer cells (HT-29) and four concentrations of each extract. The results clearly showed that all the extracts have a very significantly higher IC50 in comparison with 40 μg/ml. Taking into consideration the classification criteria of the extracts according to their cytotoxic potential as defined by the National Cancer Institute, we can say that apart from the hexane extracts of both plants and the aqueous extract of T. dodoneifolius considered moderately toxic, all the other extracts are not cytotoxic. Indeed, according to this institute, an extract that inhibits the proliferation of cells with an IC50 ≤ 20 μg/ml is considered as an active anticancer extract, and an extract with 20 μg/ml < IC50 < 100 μg/ml is indicated as moderately. The extracts with an IC50 > 100 μg/ml are inactive compounds (Tanamatayarat et al. 2003; Mutee et al. 2012). The non-toxic effect of different extracts of the plants studied may be due to their antioxidant activity as already highlighted by Kilani et al. (2008). This can justify the usage of these plants by people of various countries in Africa (Inuwa et al. 2012; Ndamitso et al. 2013; Bekoe et al. 2020).

The stable DPPH radical is widely used to evaluate the free radical scavenging activity of hydrogen donating antioxidants in many plant extracts (Talla et al. 2014). This scavenging activity was revealed to be higher for B. senegalensis than that of vitamin C and T. dodoneifolius. However, the activity of hexane extract of B. senegalensis found here is less than that of the methanolic and water extract of the same plant obtained in our previous study (Vougat et al. 2015). This difference can be explained by the polarity of the solvents used for the extraction (Ncube et al. 2008). Indeed, the non-polar solvent (hexane) used showed less activity than the polar protic solvent (water and methanol). Putting together this result and our previous finding (Vougat et al. 2015), it could be suggested that the antioxidant activity of B. senegalensis involved its hydrogen donating ability or the electron transfer reaction (Foti et al. 2004; Friaa et al. 2008). Indeed, DPPH is a stable free radical and accepts an electron or hydrogen radical to become a stable diamagnetic molecule (Soares et al. 1997).

One of the assays of antioxidative action is chelation of transition metal, thus preventing catalysis of hydroperoxide decomposition and fenotype reactions (Soares et al. 1997). The hexane extract of B. senegalensis showed a significantly high chelating effect than T. dodoneifolius. This finding is not due to the solvent used because generally extracts of solvents of low polarity show lower chelating capacity while those of higher polarity show higher chelating capacity (Talla et al. 2014). It is certainly the result of the phytochemical composition of both extracts as also observed by Ho et al. (2012). Indeed, it is well known that chelating capacity is attributed to flavonoids and phenolic compounds which use their redox properties to chelate transition metals (GülçinIlhami et al. 2004). However, the fact that the extract of B. senegalensis demonstrated a less chelating effect than EDTA suggest that this plant is a moderate metal chelating agent as compared to this standard.

Conclusions

In this study, several in vitro assays were applied to evaluate some properties of different extracts of B. senegalensis and of T. dodoneifolius, two plants most used by pastoralists in the Far North Region of Cameroon. The findings showed that the plant extracts are no toxic. Some bacteria tested were highly sensitive to these extracts. The observed bioactivities of B. senegalensis and T. dodoneifolius may support the traditional use of both plants for managing animal diseases in the Far North of Cameroon. The therapeutic properties of these plants could be due to their antioxidant and antibacterial effects of their secondary metabolilities. However, further studies are necessary to examine the in vivo effect of those extracts and to isolate the active compounds responsible for these pharmacological activities.