Evaluation of the Potential Role of Bacillus altitudinis MT422188 in Nickel Bioremediation from Contaminated Industrial Efﬂuents

: The incessant pervasiveness of heavy metals in the environment is one of the precursory factors of pollution. This research study was endeavored upon to investigate the bioremediation potential of a nickel (Ni)-resistant bacterial isolate, identiﬁed as Bacillus altitudinis MT422188, whose optimum growth parameters were demonstrated at pH 7, temperature 32 ◦ C, and 1 mM phosphate. Minimal Inhibitory Concentration (MIC) and EC 50 for Ni were observed to be 20 and 11.5 mM, respectively, whereas the cross heavy-metal resistance was discerned as Cu 2+ (25 mM) > Zn 2+ (15 mM) > Cr 6+ (10 mM) > Pb 2+ (5 mM) > Co 2+ (8 mM) > Cd 2+ (3 mM) > Hg 2+ (0 mM). Ni biosorption studies by live and heat-killed bacterial cells were suggestive of Ni uptake being facilitated by an ATP-independent efﬂux system. A pilot-scale study displayed the effective removal of Ni (70 mg/L and 85 mg/L) at 4- and 8-day intervals, respectively. Moreover, chemotaxis and motility assays indicated the role of Ni as a chemoattractant for bacterial cells. The presence of Ni reduced the GR (0.001 ± 0.003 Ug − 1 FW), POX (0.001 ± 0.001 Ug − 1 FW), and SOD (0.091 ± 0.003 Ug − 1 FW) activity, whereas Sodium dodecyl sulphate—Polyacrylamide gel electrophoresis (SDS-PAGE) revealed the presence of metallothionein (60 kDa). Kinetic and isotherm studies suggested a pseudo second-order and Freundlich model to be better ﬁtted for our study. The thermodynamic parameters ( ∆ H ◦ = 3.0436 kJ/moL, ∆ S ◦ = 0.0224 kJ/moL/K) suggested the process to be endothermic, sponta-neous, and favorable in nature. FTIR analysis elucidated the interaction of hydroxyl and carboxyl groups with Ni. Scanning Electron Microscopy (SEM) and Energy Dispersive X-Ray Spectroscopy (EDS) demonstrated changes in the morphological and elemental composition of the bacterial cells, which afﬁrmed their interaction with Ni during biosorption. In summary, our study concludes the efﬁcient role of Bacillus altitudinis MT422188 in removing Ni from polluted industrial efﬂuents.


Introduction
Many natural and anthropogenic processes have introduced heavy metals into the environment, thus aggravating the problem of pollution, which poses serious threats to the sensitive and balanced ecological systems of the Earth [1]. The continuous emission of heavy metals ensures their persistence in the environment, due to which they do not tend to deteriorate or break down over time, thus rendering them hazardous for the environment and human health in exceedingly high concentrations [2,3]. The release of industrial wastewater leads to the interaction of contaminants with various types of living

Site Sampling and Isolation of Bacteria
The sampling of effluents was performed in the industrial area of Kala Shah Kaku, in the province of Punjab, where many steel, chemical, and textile industries are found. Samples were collected from several discharge points of different steel industries. Bottles were filled with 500 mL of wastewater, prior to which the bottles were rinsed with nitric acid (dilute). The samples, which were collected twice throughout the course of the study, were kept at 4 • C to regulate the temperature while transporting them to the microbiology laboratory for further analyses. The physicochemical features of the samples were determined according to standard protocol. The samples then proceeded to the isolation of Ni-resistant bacterial species on Luria-Bertani (LB) agar, augmented with 0.1 mM of Ni at 37 • C. Standard microbiological methods were followed for the isolation of bacteria, after which the morphological features of the selected bacterial isolate were observed [14].

Determination of MIC and Cross Heavy-Metal Resistance Pattern
The minimum inhibitory concentration (MIC) assay was performed using minimal salt agar medium [15] augmented with varying concentrations of Ni (0.1-30 mM). The cross heavy-metal resistance pattern was investigated via the test-tube dilation method, with different concentrations (0.1-30 mM) of several heavy-metal salts (CuSO 4 ·5H 2 O, K 2 Cr 2 O 7 , CdCl 2 ·H 2 O, HgCl 2 , PbCl 2 , ZnCl 2 ·6H 2 O, CoCl 2 ·6H 2 O) added to the salt medium, to which 1 mM phosphate and 4 g/L sodium succinate were added previously [16]. Results were observed in the form of optical density at 578 nm after incubating for 48 h at 37 • C.

Molecular Characterization of Selected Bacterial Isolate
The selected bacterial isolate on the basis of MIC was observed for its morphological and biochemical features, after which it was identified at the molecular level through 16 s rRNA sequencing. The obtained sequence was subjected to Basic Local Alignment Search Tool (BLAST) and submitted to the National Center for Biotechnology Information (NCBI).

Evaluation of Bacterial Growth and EC 50 in Presence of Ni
For this experiment, 1% fresh bacterial culture was added to sterile minimal salt broth to achieve the log phase of bacterial growth (OD 578 = 0.3-0.4), after which the experimental setup was supplemented with Ni (0.1 mM). Following an interval of 30 min, the optical density was recorded at 578 nm every 60 min for up to 9 h. The observed readings were then compared with the control setup and were plotted in graphical form [18]. In a similar manner, the experimental and control groups were set up for the determination of EC 50 . The experimental groups were supplemented with different concentrations of Ni (0, 0.25, 0.5, 0.75, 1.0, 1.25, 1.5, 1.75, 2. 2.5, 3, 3.5, 4 mM), followed by the absorbance obtained at regular intervals (OD = 578 nm). The results were plotted in graphical form [19].
2.6. Ni Biosorption Experiments 2.6.1. Determination of Ni Uptake The metal uptake analysis was performed by the method of Shamim et al. [18], whereby 1% bacterial culture was inoculated in sterile minimal salt medium previously augmented with 1 mM phosphate and 4 g/L sodium succinate. The flasks were incubated at 37 • C until OD 578 reached 0.3-0.4, after which 10 mgL −1 Ni were added to the experimental setup. After 30 min, 10 mL samples were harvested and the optical density (578 nm) was also recorded. This was termed as the first hour sample and reading, and the samples were harvested consecutively after 0, 1, 2, 3, 4, 5, 6, 7, 8, and 9 h. The pellet in the first falcon tube was then washed thrice with Milli-Q water (10 mL) and EDTA (0.1 mM), and centrifuged again at 12,000 rpm to obtain a pellet. The water was collected in a new falcon tube. The harvested pellets were then acid digested with the help of 0.2 N nitric acid (HNO 3 ) and incubated at 37 • C. The previously centrifuged supernatant samples, the water samples, and the pellet samples were then made ready for atomic absorption spectrometry (AAS) analysis at 228.8 nm the next day, prior to which the standards for the instrument were run to generate a calibration curve. The subsequent results were tabulated and graphs were plotted.

Ni Uptake in Presence of Inhibitors
This experiment was carried out likewise the previous method, along with the addition of two metabolic inhibitors, DNP (1 mM) and DCCD (100 µM), prior to the supplementation of Ni in the medium at the log phase of the bacterial cells. The rest of the procedure was carried out as before [18].

Ni Removal by Killed Bacterial Cells
The determination of metal uptake by killed bacterial cells was carried out by the method of Shamim et al. [18]. A total of 1% of bacterial culture was inoculated in experimental and control setups of sterile minimal salt broth medium, after which the logarithmic bacterial cells were killed via heat inactivation. Ni (10 mgL −1 ) was added to the killed cells, which were then incubated for 30 min. The rest of the procedure was followed according to the previous experimental setups.

Pilot-Scale Study for Ni Removal
The pilot-scale study was carried out by following the method of Shamim and Rehman [17]. The evaluation of Ni removal efficacy of the bacterial isolate from industrial effluents was carried out in three plastic containers, with the first being filled with tap water (10 L), and the other two with industrial effluents (10 L) (30 • C, pH 6.2, dissolved oxygen content 0.0134 ± 0.02 g L −1 , Ni 1.5 ± 0.01 g L −1 ). In the first two containers, fresh bacterial culture (1%) was added, following the addition of Ni in all containers. The samples from the containers placed at room temperature were collected after 4 and 8 days and were harvested at 15,000 rpm. The acid-digested supernatants were used to determine the Ni removal efficacy of the bacterial cells.

Profiling of Antioxidative Enzymes
For the evaluation of antioxidative enzymes, the preparation of the enzyme extract was performed by inoculating 1% bacterial culture in sterile minimal salt broth medium, which was incubated for 24 h at 37 • C, followed by the addition of Ni (0.1 mM) and incubation for another 24 h. Post 48 h of incubation, a sample (50 mL) was harvested for 10 min at 12,000 rpm. The supernatant was discarded and the pellet was homogenized in extraction buffer (5 mL) under cold conditions [20]. The solution was then homogenized at 12,000 rpm for 10 min. The supernatant was transferred to a new falcon tube labeled as the enzyme extract, which was used for the estimation of various antioxidative enzymes such as superoxide dismutase (SOD) [21], ascorbate peroxidase (APOX) [22], catalase (CAT) [23], peroxidase (POX) [24], and glutathione reductase (GR) [25].

Profiling of Proteins and Metallothioneins
The estimation of protein was carried out by plotting a curve of various concentrations of protein (1-30 µg) against a standard (bovine serum albumin). The samples for nonelucidated and elucidated protein content were prepared using Bradford reagent and the results were observed by taking the absorbance of samples (OD 595nm ) [26].
For the profiling of intracellular proteins (metallothioneins), the bacterial culture was inoculated in minimal salt broth medium in the presence and absence of Ni (0.1 mM) stress. Following an incubation of 24 h, the cell pellets were harvested at 15,000 rpm for 10 min. The pellets were homogenized and mixed in 1X gel-loading buffer, after which they were placed on a thermomixer for 5 min at 95 • C. Experimental and control samples were then resolved by SDS-PAGE using resolving gel (12%) and stacking gel (5%). After the subsequent stain and de-stain process, the gel was visualized and the bands were compared to the standard protein ladder [27].

Determination of Motility and Chemotactic Behavior
The evaluation of motility patterns (swim, swarm, twitch) of the bacterial cells in the presence and absence of Ni was conducted by the method of Murray et al. [28]. Likewise, the chemotactic behavior of the bacterial cells with and without Ni was elucidated using the capillary chemotaxis method [29].

Isothermic, Thermodynamics, and Adsorption Kinetic Studies
The isotherm studies to study the adsorption mechanism of the bacterial cells were performed using Langmuir and Freundlich isotherm models [30,31]. The Langmuir model was studied via the following non-linear (1) and linear (2) equations, respectively: Ce q e = Ce q max + 1 bq max (2) where C e = concentration of metal ions in solution at equilibrium (mM), q e = amount of metal ions adsorbed at equilibrium (mM/g), q max = Langmuir constant (mM/g), b = adsorption constant. The Freundlich model was studied via the following non-linear (3) and linear (4) equations, respectively [32]: The linear form of the equation is: where K f and n = Freundlich constants. The biosorption kinetic studies were evaluated using Lagergren's pseudo first-order and pseudo second-order kinetic models [33], where the linear equations of the pseudo first-order (5) and pseudo second-order (6) [34,35] are as follows: where q e and q t = amount of metals ions adsorbed at equilibrium, t = time, k 1 and k 2 = first-order and second-order rate constant, respectively. The thermodynamic studies were carried out using the Gibbs free energy change (∆G • ), enthalpy change (∆H • ), and entropy change (∆S • ) parameters with the following Equations (7) and (8): where R = universal gas constant, T = temperature in Kelvin (K), K D = value calculated from q e / C e .

Fourier Transform Infrared Spectroscopy (FTIR) Analysis of Bacterial Cells
FTIR analysis was utilized to obtain IR spectra for bacterial cells with and without Ni stress. For sample preparation, minimal broth medium was inoculated with 1% of bacterial culture with (experimental) and without (control) Ni (0.1 mM). The samples were incubated for 24 h at 37 • C, after which they were harvested and the resultant pellet was homogenized in deionized water (500 µL). FTIR (Bruker) analysis was then performed in the mid-IRF region of 4000-500 cm −1 [36].

Scanning Electron Microscopy (SEM) and Energy Dispersive Spectroscopy (EDS) Analysis
The SEM and EDS analyses were performed to study the pattern of Ni biosorption by bacterial cells. For both of the analyses, the method by Khan et al. [37] was adopted. Prepared samples were evaluated on SEM (JSM-IT-100, JEOL, Japan) coupled with EDS, under several magnifications.

Statistical Analysis
The experiments were carried out thrice to avoid error. All experimental setups were run with specific control setups under suitable and similar conditions. During result compilation, cumulative average and standard error was calculated using IBM SPSS (V. 24.0).

Enumeration of Ni-Resistant Bacterial Isolates
A total of 35 bacterial isolates were isolated from the collected samples, which were then subjected to an MIC assay for the selection of the most resistant isolate.

Selection and Molecular Identification of Bacterial Isolate
The most resistant bacterial isolate was selected on the basis of the MIC and cross heavy-metal resistance, which was then identified via 16s rRNA ribotyping. The isolate was identified as Bacillus altitudinis, and the accession number acquired from NCBI for the strain was MT422188.

Optimum Growth Conditions
The optimum growth was found to be at 32 • C, pH 7, and 1 mM phosphate for the bacterial cells, as depicted in Figure 1.

Bacterial Growth and EC 50
The growth curve demonstrated that the bacterial cells entered the log phase when they were introduced in the medium. The presence of Ni was observed to act as a stress for the bacterial cells, as observed from the overall reduction of the growth, as shown in Figure 2. The EC 50 of the bacterial cells was demonstrated to be 11.5 mM, which means that at this concentration about 50% of the cells were dead and 50% of the cells were live and functional, performing cellular functions, as shown in Figure 3.

Bacterial Growth and EC50
The growth curve demonstrated that the bacterial cells entered the log phase when they were introduced in the medium. The presence of Ni was observed to act as a stress for the bacterial cells, as observed from the overall reduction of the growth, as shown in Figure 2. The EC50 of the bacterial cells was demonstrated to be 11.5 mM, which means that at this concentration about 50% of the cells were dead and 50% of the cells were live and functional, performing cellular functions, as shown in Figure 3.

Bacterial Growth and EC50
The growth curve demonstrated that the bacterial cells entered the log pha they were introduced in the medium. The presence of Ni was observed to act as for the bacterial cells, as observed from the overall reduction of the growth, as s Figure 2. The EC50 of the bacterial cells was demonstrated to be 11.5 mM, which that at this concentration about 50% of the cells were dead and 50% of the cells w and functional, performing cellular functions, as shown in Figure 3.

Ni Uptake by Live Bacterial Cells
The bacterial cells entered log phase in the third hour, after which a steady in in the bacterial cells was observed. The cells also started to uptake Ni from the aq medium, which was evident from the decrease in Ni. The intracellular accumulatio adsorption also increased in the eight and ninth hours, where the concentration of N shown to be less, indicating the accumulation of Ni inside the bacterial cells (Figur (a)

Ni Uptake by Live Bacterial Cells
The bacterial cells entered log phase in the third hour, after which a steady increase in the bacterial cells was observed. The cells also started to uptake Ni from the aqueous medium, which was evident from the decrease in Ni. The intracellular accumulation and adsorption also increased in the eight and ninth hours, where the concentration of Ni was shown to be less, indicating the accumulation of Ni inside the bacterial cells (Figure 4a).

Ni Uptake by Live Bacterial Cells
The bacterial cells entered log phase in the third hour, after which a steady increase in the bacterial cells was observed. The cells also started to uptake Ni from the aqueous medium, which was evident from the decrease in Ni. The intracellular accumulation and adsorption also increased in the eight and ninth hours, where the concentration of Ni was shown to be less, indicating the accumulation of Ni inside the bacterial cells (Figure 4a). (a)

Ni Uptake in Presence of Inhibitors
The presence of DNP (inhibitor 1) reduced the overall growth of the bacterial cells, along with the presence of Ni in the aqueous medium. The growth of cells started to increase after the fourth hour, and kept steadily increasing until the ninth hour. The uptake of Ni from the medium was observed to be substantial from the sixth hour onwards, which also resulted in an increase in the adsorption and intracellular accumulation from the sixth to the ninth hour ( Figure 4b). DCCD (inhibitor 2) had a somewhat similar effect on the growth of bacterial cells as DNP. The growth of bacterial cells was seen to drastically increase in the ninth hour, with uptake of Ni from the aqueous medium starting from the seventh hour onwards. The intracellular accumulation and adsorption mechanism was also observed at the same hour, as depicted by Figure 4c. In the final inhibitor setup, the growth of bacterial cells decreased in the presence of three stress inducers used in combination (Ni, DNP, DCCD). The bacterial cells entered the log phase, but the growth was not as pronounced as in the other experimental setups. The presence of the inhibitors did not stop the cells from removing Ni from medium, as observed from the decrease of Ni in the ninth hour. The intracellular accumulation and adsorption of Ni was also observed minimally in the last two hours, as shown in Figure 4d.

Ni Removal by Killed Bacterial Cells
The killed bacterial cells failed to grow, as they did not reach the lag or log phase. The dead cells did not uptake any Ni from the aqueous medium, although the availability of bacterial cells (biomass) enabled the adsorption of Ni ions onto the bacterial cell surface ( Figure 5).

Ni Uptake in Presence of Inhibitors
The presence of DNP (inhibitor 1) reduced the overall growth of the bacterial cells, along with the presence of Ni in the aqueous medium. The growth of cells started to increase after the fourth hour, and kept steadily increasing until the ninth hour. The uptake of Ni from the medium was observed to be substantial from the sixth hour onwards, which also resulted in an increase in the adsorption and intracellular accumulation from the sixth to the ninth hour (Figure 4b). DCCD (inhibitor 2) had a somewhat similar effect on the growth of bacterial cells as DNP. The growth of bacterial cells was seen to drastically increase in the ninth hour, with uptake of Ni from the aqueous medium starting from the seventh hour onwards. The intracellular accumulation and adsorption mechanism was also observed at the same hour, as depicted by Figure 4c. In the final inhibitor setup, the growth of bacterial cells decreased in the presence of three stress inducers used in combination (Ni, DNP, DCCD). The bacterial cells entered the log phase, but the growth was not as pronounced as in the other experimental setups. The presence of the inhibitors did not stop the cells from removing Ni from medium, as observed from the decrease of Ni in the ninth hour. The intracellular accumulation and adsorption of Ni was also observed minimally in the last two hours, as shown in Figure 4d.

Ni Removal by Killed Bacterial Cells
The killed bacterial cells failed to grow, as they did not reach the lag or log phase. The dead cells did not uptake any Ni from the aqueous medium, although the availability of bacterial cells (biomass) enabled the adsorption of Ni ions onto the bacterial cell surface ( Figure 5).

Pilot-Scale Study for Ni Removal
In the pilot-scale study, B. altitudinis was observed to remove 70 and 85 mg/L after a time of 4 and 8 days, respectively, which was greater than the amount of Ni removed from other experimental setups, thus establishing its Ni bioremediation efficacy, as depicted in Figure 6.

Pilot-Scale Study for Ni Removal
In the pilot-scale study, B. altitudinis was observed to remove 70 and 85 mg/L after a time of 4 and 8 days, respectively, which was greater than the amount of Ni removed from other experimental setups, thus establishing its Ni bioremediation efficacy, as depicted in Figure 6.

Profiling of Antioxidative Enzymes
The evaluation of antioxidative enzymes demonstrated the reduced activity of G (0.001 ± 0.003 Ug -1 FW), POX (0.001 ± 0.001 Ug -1 FW), and SOD (0.091 ± 0.003 Ug -1 FW) a tivity in the presence of Ni in B. altitudinis cells. The presence of Ni failed to induce APO and CAT activities in measurable quantities, as shown in Table 1.

Profiling of Antioxidative Enzymes
The evaluation of antioxidative enzymes demonstrated the reduced activity of GR (0.001 ± 0.003 Ug −1 FW), POX (0.001 ± 0.001 Ug −1 FW), and SOD (0.091 ± 0.003 Ug −1 FW) activity in the presence of Ni in B. altitudinis cells. The presence of Ni failed to induce APOX and CAT activities in measurable quantities, as shown in Table 1.

Pattern of Motility and Chemotactic Behavior
The swimming, swarming, and twitching pattern of motility was observed in B. altitudinis cells in 0.3, 0.5, and 1% agar medium, which demonstrated remarkable motile behavior in the presence of Ni (Figure 8). The capillary chemotaxis experiment demonstrated the role of Ni as a chemoattractant for B. altitudinis, resulting in positive motility towards Ni in the medium (Figure 9). Sustainability 2021, 13, x FOR PEER REVIEW 12 of 22

Pattern of Motility and Chemotactic Behavior
The swimming, swarming, and twitching pattern of motility was observed in B. altitudinis cells in 0.3, 0.5, and 1% agar medium, which demonstrated remarkable motile behavior in the presence of Ni (Figure 8). The capillary chemotaxis experiment demonstrated the role of Ni as a chemoattractant for B. altitudinis, resulting in positive motility towards Ni in the medium (Figure 9).

Isothermic, Thermodynamic, and Adsorption Kinetic Studies
For the isotherm models, the graphs were plotted for both Langmuir and Freundlich isotherm models, respectively. The values for the Langmuir and Freundlich constants as well as the R 2 values are comprehensively provided in Table 2. For the Langmuir and Freundlich models, the R 2 values were observed to be in the range of 0.90-0.98 and 0.900-0.999, respectively, which therefore demonstrated the compatibility of the Freundlich model with our study. The pseudo first and second order of kinetics and their constants are shown in Table 3. The coefficient values (q exp and q cal ) of the first order were compared but were not compatible with each other. In the case of the second order, compatibility was positively observed between the two coefficients. Moreover, the comparison of the R 2 values of both orders demonstrated that pseudo second-order kinetics favored our study. The thermodynamic parameters of our study demonstrated the Gibbs free energy (∆G • ) for various temperatures, whereas the enthalpy change (∆H • ) and entropy change (∆S • ) were found to be 3.0436 KJ/mol and 0.0224 kJ/mol/K, respectively, as shown in Table 4.

Fourier Transform Infrared Spectroscopy (FTIR) Analysis
The FTIR analysis revealed the characteristic peaks of hydroxyl and carboxyl functional groups playing a role in the biosorption of Ni by B. altitudinis. The peak shifts were determined to be due to the interaction of Ni with bacterial cells (Table 5).

SEM and EDS Analyses
The SEM and EDS analyses demonstrated the positive physical and chemical changes in B. altitudinis cells, which were indicative of their biosorption and features in bacterial cells against Ni, as shown by Figure 10a,b and Figure 11a

SEM and EDS Analyses
The SEM and EDS analyses demonstrated the positive physical and chemical changes in B. altitudinis cells, which were indicative of their biosorption and features in bacterial cells against Ni, as shown by Figures 10a,b and 11a,b.

Discussion
Heavy metals are major contributors to pollution, as they are toxic substances that tend to accumulate over time in valuable resources around the world [38]. This research study was conducted to determine the efficacy and potential role of an Ni-resistant bacterial isolate in Ni bioremediation. The bacterial isolate, named ZBM-5, was selected on the basis of its MIC and cross heavy-metal resistance pattern. The isolate was identified as Bacillus altitudinis MT422188, and was used to remove Ni from aqueous media. The findings from our research are in agreement with the findings of Alboghobeish et al. [39], who in their work also reported the presence of Ni-resistant bacteria from heavy-metal contaminated wastewaters. Bacteria are dependent upon optimal temperatures, pH, and other parameters for their growth, which can decline or cease if they are allowed to grow at other temperatures. The growth conditions were examined, which demonstrated the optimum temperature, pH, and phosphate concentration of B. altitudinis to be 32 °C, 7, and 1 mM, respectively (Figure 1). The work of Zhenggang et al. [40] described the optimum temperature of Bacillus cereus to be 35 °C, which was determined over a range of other examined temperatures. Furthermore, another study reported the optimum temperature of another bacterial species, Sphaerotilus natans, to be 35 °C [41], demonstrating that

Discussion
Heavy metals are major contributors to pollution, as they are toxic substances that tend to accumulate over time in valuable resources around the world [38]. This research study was conducted to determine the efficacy and potential role of an Ni-resistant bacterial isolate in Ni bioremediation. The bacterial isolate, named ZBM-5, was selected on the basis of its MIC and cross heavy-metal resistance pattern. The isolate was identified as Bacillus altitudinis MT422188, and was used to remove Ni from aqueous media. The findings from our research are in agreement with the findings of Alboghobeish et al. [39], who in their work also reported the presence of Ni-resistant bacteria from heavy-metal contaminated wastewaters. Bacteria are dependent upon optimal temperatures, pH, and other parameters for their growth, which can decline or cease if they are allowed to grow at other temperatures. The growth conditions were examined, which demonstrated the optimum temperature, pH, and phosphate concentration of B. altitudinis to be 32 • C, 7, and 1 mM, respectively (Figure 1). The work of Zhenggang et al. [40] described the optimum temperature of Bacillus cereus to be 35 • C, which was determined over a range of other examined temperatures. Furthermore, another study reported the optimum temperature of another bacterial species, Sphaerotilus natans, to be 35 • C [41], demonstrating that most bacterial species are mesophilic in nature, functioning over a moderate range of temperatures that can be easily applied for optimum growth.
In this study, the MIC and the multiple metal resistance pattern of the bacteria were examined. The concentration that inhibited the growth of the bacterial isolate even after the desired incubation was termed "the effective MIC." In a similar manner, the cross heavymetal resistance pattern was checked for different heavy metals when their increasing concentrations were applied in solution. The concentration that failed to facilitate the growth of bacteria after the incubation period was termed "the inhibiting concentration of the respective metal." The MIC of B. altitudinis was observed to be 20 mM, whereas the multiple metal resistant behavior of the different metals was observed to be Cu 2+ > Zn 2+ > Cr 6+ > Pb 2+ > Co 2+ > Cd 2+ > Hg 2+ . In their study, Afzal et al. [42] also studied Ni-resistant bacterial isolates collected from wastewater samples from industrial effluents. The MIC of Ni was observed to be 8 mM in their study. Another study, conducted by Chowdhary et al. [43], stated the MIC of Ni resistant bacterial isolate to be 24 mM, which is in agreement with our results. The results are also similar to the results of Alboghobeish et al. [39], who reported the MBC of the Ni-resistant Klebsiella oxytoca species to be 24 mM. In agreement with previously reported works, another study reported the zone of inhibition of Niresistant bacteria to be 24 mM after it was treated and examined in a well-diffusion assay [44]. These results could establish the basis of resistance in bacterial species against Ni, whether chromosomal or plasmid mediated. This resistance is basically an adaptive mechanism that bacteria take up in order to ensure survival under stress conditions and high metal toxicity. The determination of EC 50 in the case of Ni was 11.5 mM (Figure 3), which means that at this concentration 50% of the bacterial cells were dead and 50% of the bacterial cells were live and functional, taking part in the cellular processes and responding to the metal toxicity in the environment. In the research findings by Speir et al. [45], the EC 20 value was examined for Zn, which was shown to be 330 mg kg −1 , in order to determine the metal toxicity in soil. The growth of bacteria was observed to be less in the presence of Ni in our research work, indicating the role of Ni as a stress for bacterial cells, though the growth followed the same pattern as seen in the absence of Ni (Figure 2). The findings by Afzal et al. [42] also reported a decrease in the bacterial growth in the presence of Ni, which demonstrates that the bacterial growth declined when it was compared with the growth pattern of the control (without stress).
The elevated concentration of pollutants such as heavy metals results in their contact with the surrounding microorganisms of the environment. Exposure to bacteria results in their interaction with bacterial cell walls, which leads to the production of harmful compounds and metabolites. The ingress of heavy metals inside bacterial cells is regulated by uptake systems that are specific to certain species of bacteria. These uptake systems are reported to be of two types, the first being a fast and unspecified system that occurs mostly across an osmotic gradient and is ATP independent, whereas the second uptake system is comparatively slower, specified, and dependent upon ATP. The entry of Ni is regulated by the ABC transporter family [46]. In this research work, the uptake mechanism of Ni by B. altitudinis was investigated. The reduced growth of cells in the presence of Ni indicated that the bacterial cells were in a stressful environment in the presence of Ni (Figure 4a). The presence of Ni and DNP demonstrated the uptake of Ni from the medium by the bacterial cells in the sixth hour, which also resulted in the intracellular accumulation and adsorption of Ni in the presence of DNP (Figure 4b). The second inhibitor, DCCD, had a similar effect on the uptake of Ni by bacterial cells, with almost identical uptake patterns (Figure 4c). The effect of Ni and both inhibitors combined demonstrated the growth pattern of the bacterial cells to be not as pronounced as compared to other experimental setups (Figure 4d), although the presence of both inhibitors did not cease the uptake of Ni from the medium, thereby indicating the role of an unspecified efflux system that is not dependent upon ATP. The uptake of Ni by killed bacterial cells was also investigated in the study, where it was observed that the killed cells were not able to uptake Ni from the medium, but adsorption was reported due to the availability of biosorbent sites that adsorb Ni from the environment without the aid of a specific uptake system ( Figure 5). Previous researchers have also reported on the biosorption ability of bacterial killed biomass [47,48]. The pilot-scale study was also conducted to determine the Ni removal efficacy of B. altitudinis, indicating it to be an effective agent of Ni bioremediation, as it was able to remove remarkable quantities of Ni (Figure 6), which was also reported by Rivas-Castillo et al. [49].
The motility of microorganisms is one of the main features that are essential for their survival. The requirement of nutrients and the search for them is enabled by the motile nature of the microorganisms. The same can be said about their escape from their surroundings if they encounter any stress in their surroundings, where their motility enables them to move away. This is achieved with the help of external features of microorganisms such as flagella and pili. The microorganisms, bacteria in particular, attain the help of various motility patterns in order to survive in various stressful conditions in their surroundings. The motion that is adapted by bacteria to move towards favorable conditions and vice versa is known as the phenomenon of chemotaxis. The migration of bacteria is directed under a chemical gradient, where they move away or towards it under conditions for their endurance and survival. The regulation of movement patterns in bacterial cells tends to cause a motion toward attractants or repellents in an environment. This stimulus in the environment is detected by bacterial chemoreceptors that aid in transmitting the signal of motion to the signal transduction system of the bacteria, after which the bacteria opt for a suitable movement pattern under stimulating conditions. The flagellar movements are controlled by the regulatory protein CheY. CheY-P, the phosphorylated form of CheY, binds to the flagellar motor, which leads to tumbling motions, whereas its non-phosphorylated form leads to running motions. The other regulatory proteins, CheA and CheW, act as a complex and a linker between the two proteins, respectively [50]. In this study, the mechanisms of motility and chemotaxis were investigated in a series of experiments. The presence of Ni demonstrated remarkable swimming, swarming, and twitching behavior in bacterial cells, which indicates that at a given concentration Ni acted as chemoattractant for the bacterial cells and they preferred to move freely in its presence (Figure 8). The chemotaxis experiments demonstrated that B. altitudinis demonstrated movement towards Ni when it was present in capillary tubes, as well as in the pond, resulting in more CFU/mL ( Figure 9). The positive chemotaxis for Ni affirmed that B. altitudinis was a metal lover ( Figure 9).
The presence of metallothioneins (MTs) in living beings is the basis of the important role they serve in many biological functions, as these proteins are reported to be highly conserved in living organisms, making them unchanged through many generations. The major function that MTs serve can be that of metal detoxification and conferring metal resistance among living organisms and bacteria. The MTs present in bacteria are majorly attributed to conferring resistance against various heavy metals, as demonstrated by the findings of many studies [18,37,51]. This work was also used to determine the presence of MTs in B. altitudinis with and without Ni stress (Figure 7). In agreement with our study, various other studies have also reported on the induction of MTs under heavy stress over the years [52,53]. The expression of antioxidative enzymes was also evaluated in this research study to gain better insight into the enzymes responsible for combating the generation of ROS in the system. The activity of GR, POX, and SOD enzymes was observed to decrease in the presence of Ni, whereas the activities of APOX and CAT were not observed in a quantifiable range, neither with nor without Ni stress (Table 1). Tammam et al. [54] reported an increase in SOD enzyme activity and a decline in GR enzyme activity under Ni stress.
The interactions between Ni ions and bacterial cells, resulting in the subsequent adsorption, was evaluated using isotherm models, pseudo-order kinetics, and thermodynamics (Tables 2-4). The isotherms of adsorption are the primary prerequisites in the design and development of adsorption systems [55]. Although several isotherm equations have been reported for studying adsorption models, Langmuir and Freundlich remain two of the most commonly used isotherms, where the former is of the assumption that adsorption occurs at particular sites homogenously (monolayer) inside the adsorbent, and the latter is suggestive of heterogenous (multilayer) systems. In both models, the R 2 values were reported to be above 0.92, indicating a good mathematical fit (Table 2). However, the greater coefficient values of the Freundlich model suggest it to be a better model fit for our study. Similar findings in Bacillus sp. were reported by Cai et al. [56]. The thermodynamic parameters were also investigated in order to evaluate the feasibility of the process. The Gibbs free energy (∆G • ) was observed to be negative, which indicates that the overall process of adsorption is feasible and spontaneous. Moreover, positive values of enthalpy change (∆H • ) and entropy change (∆S • ) demonstrated that the process was endothermic and favorable in nature. The results of our study are in agreement with Asare et al. [57].
The FTIR analysis was performed for the evaluation of bacterial functional groups associated with the adsorption of Ni ions by B. altitudinis ( Table 5). The FTIR spectra demonstrated broad peaks at 3279.39 cm −1 and 1637.22 cm −1 , where no Ni stress was added, which corresponded to the presence hydroxyl and carboxyl groups, respectively. The hydroxyl group demonstrated C-H stretching, due to which broad peaks were formed, whereas the carboxyl group demonstrated C=O stretching bonds in asymmetric and symmetric vibrations. In the presence of Ni, these peaks were observed to be shifted to 3272.11 cm −1 and 1636.97 cm −1 , respectively. The shift in the two peaks under Ni stress was observed to be due to the interaction and binding of Ni ions with the bacterial cells. The findings of Khan et al. [37] are in agreement with our study, where the involvement of various functional groups of bacteria were observed in biosorption by bacteria. The use of techniques like SEM and EDS aided in determining the biosorption and interaction of Ni ions with the bacterial cells at a microscopic level. The SEM images (Figure 10a,b) demonstrated the shape and structure of the bacterial cells before and after Ni biosorption. The size of the bacterial cells was observed to be changed after the biosorption of Ni ions, as the cells were observed to be bigger and swollen in size, indicating intracellular accumulation of Ni. Similarly, a morphological as well as elemental alteration of the bacterial cells after Ni biosorption was observed in the EDS images (Figure 11a,b), where the characteristic peak of Ni was only found after Ni biosorption. Our results were found to be similar to the findings of Rahman et al. [58].

Conclusions
This study was performed for the isolation and characterization of Ni-resistant bacteria which were isolated from Ni-polluted industrial effluents. The bacterial isolate was identified as Bacillus altitudinis, which was studied for its bioremediation potential against Ni. This study aimed to shed light through various experiments on the biosorption potential of Ni by B. altitudinis, proving it to be an efficient biosorbent. Further progress in investigating the molecular mechanisms of the bacterium in removing Ni from polluted industrial effluents can be helpful in gaining a better insight into the resistance and efflux systems that are responsible for bacterial resistance against Ni. Chemotaxis and motility assays demonstrated Ni to be a chemoattractant for B. altitudinis, thereby facilitating the movement of bacterial cells towards Ni in a stressful environment. The presence of Ni inducted a metallothionein of 60 kDa, whereas the FTIR analysis revealed the interaction of hydroxyl and carboxyl groups with Ni, with similar features observed in SEM and EDS. Equilibrium, kinetic, and thermodynamic studies depicted the adsorption of Ni onto bacterial cells to be in support of the Freundlich isotherm model, pseudo second-order kinetics, and endothermic, spontaneous, and feasible reaction, respectively. Therefore, these properties were helpful in elucidating the efficient role of B. altitudinis in Ni biosorption.