Production of Plant Growth-Promoting Bacteria Biofertilizer from Organic Waste Material and Evaluation of Its Performance on the Growth of Corn (Zea mays) ()
1. Introduction
Fertilizers play an important role in agricultural system mainly in increasing yield. Synthetic fertilizers were a part of the technology that contributed to the Green Revolution and millions of tons of chemical fertilizers have continued to be used the world over [1]. However, excessive application of chemical fertilizers has resulted in adverse environmental impacts and ecological challenges [2] [3]. Some of these negative impacts include: water body pollution/eutrophication and algal bloom, land degradation, food and food crop-products contamination, adverse human health effects, greenhouse effect/ozone layer depletion and general imbalance of the ecosystem [4]. These adverse effects have led to the introduction of microbial inoculants/biofertilizers for plant growth and development [5], which include Plant Growth-Promoting Microorganisms such as nitrogen fixing and phosphate solubilizing microorganisms [6]. Nitrogen is a very important factor that may limit plant growth and food production as it is an essential component of chlorophyll—a pigment that alongside amino acids, promote photosynthesis [7]. Nitrogen gas (N2), although one of the predominant elements in the atmosphere, can only be utilized by plants in reduced form, of ammonia and nitrate fertilizer or biological nitrogen fixation. Some of the soil nitrogen-fixing-bacteria include species of Azotobacter sp., Bacillus sp., Clostridium, and Klebsiella [7].
Phosphorus is the second most important element required for plant growth, next to Nitrogen [8]. Although large amount of phosphorus fertilizer are applied for soil fertility improvement, most of it (20% - 80%) are immobilized in the soil, making them unavailable for plant use [9]. It was reported that only 0.1% of the total Phosphorus is available for plant up-take due to Phosphorus fixation by some species of bacteria and fungi in the soil and rhizosphere [10]. [11] reported that bacteria solubilize phosphorus are more effectively than fungi. Strains from bacterial genera-Pseudomonas, Bacillus, Rhizobium and Enterobacter along with Penicillium and Aspergillus fungi are the most powerful Phosphorus solubilizers [12]. Researchers have discovered the development and use of biofertilizers as an environmentally-friendly, cost-effective and efficient fertilizer that can boost crop productivity as well as maintain the purity of the soil [12].
Biofertilizer is any substance which contains living microorganisms that can inhabit the rhizosphere or soil and promotes the growth of plant by promoting the availability of the primary plant nutrient when applied to the soil, surface of plant or seed [14] [15] [16], on the other hand, described biofertilizer as materials that include manure and plant extracts which contain microorganisms that promote plant growth. This group of microorganisms is known as plant growth promoting bacteria (PGPB), some of which promote plant growth by fixing atmospheric nitrogen and solubilizing phosphorus. Also, [17] defined biofertilizer as preparation containing live or latent cells of microorganisms or their metabolites, which when inoculated to seed, soil or roots of seedlings, promote plant growth and enhance harvestable yield. This definition separated biofertilizer from organic fertilizer which contains organic matters [17]. This application is based on the use of decomposing organic matters, crops remains, animal sewage and microorganisms, to enhance nutrients in the plant rhizosphere, soil stability, quick decomposition of organic matters and mycorrhiza symbiosis association [18].
The experiment was conducted at Isu-Aniocha, Awka North Local Government Area of Anambra State, Nigeria.
2. Materials
Fresh soil sample, from the soil rhizosphere, taken from 5 cm beneath the soil surface, dry grass, water hyacinth (Eichornia crassipes), leguminous plants (e.g. Leucaena leucocephala), rice chaff, wheat chaff, brown sugar, moringa leaves, orange, banana, grape, cucumber, poultry litter and sewage, microkjeldal flask, weighing balance, beakers, retort stand, burette, flat bottom flask, Bunsen burner, distillation column, conical flask.
3. Methods
The methods employed at the different stages of the production and the product testing, include: culturing of microorganisms, isolation of microorganisms, characterization of the experimental soil, biofertilizer and chemical/synthetic fertilizer.
4. Microorganism Culture
The microorganism was cultured, using 500 gm of the fresh soil sample from the soil rhizosphere, collected from 5 cm beneath the soil surface, 500 gm of wheat chaff and rice chaff, mixed with water until a homogenous mixture was obtained. The mixture was transferred into a covered container with a depression in the center to allow air circulation and ventilation. The container was kept under a shade and allowed to stand for seven days.
5. Production of Liquid Bio Fertilizer
Nine kilogramme (9 kg) of mixed fruits—oranges, cucumber, bananas, grape, moringa leaves were cut into tiny pieces and loaded into a container. 1 kg of brown sugar and 1 kg of the microorganism culture was added into the container in the ratio of 1:1.
The materials were mixed properly together, until the mixture became consistent. Sterile water was added into the container and stirred in one direction for few minutes. The container was tightly sealed and kept in a dark place for two weeks without any disturbance. The mixture was sieved and the liquid (biofertilizer) was transferred into a gallon and kept in a shady cool dry place ready for further analysis.
6. Isolation of Microorganisms
Nitrogen Fixing Bacteria, Phosphorus Solubilizing Bacteria (PSB)
The liquid (biofertilizer) produced above, was cultured using two selective media (for Azotobacter and Phosphorus Solubilizing Bacteria (PBS) respectively).
PSB bacteria, Pikovskaya agar medium [19] were prepared with the following quantity and components: glucose—2.5 g, Ca3 (PO4—1.25 g, NaCl—0.05 g, MgSO4∙7H2O—0.000625 g, MnSO4∙2H2O—0.000625 g, FeSO4∙7H2O—0.000625 g, yeast—1.25 g and 5 g of agar. The medium was diluted in 250 ml of distilled water and sterilized in an autoclave at the temperature of 121˚C for 15 minutes. The agar was poured into a plate (Petri dish) and was allowed to solidify at room temperature. Serial dilution was made and the sample was swabbed on the solidified agar with a swab stick and incubated at room temperature.
7. Isolation of Phosphorus Solubilizing Bacteria
7.1. Azotobacter spp.
Mannitol Ashby agar media was prepared with the following composition: 5 g of Mannitol, 0.05 g of Potassium Hydrogen Phosphate (K2HPO4), 0.05 g of Sodium Chloride (NaCl), 0.05 g of Magnesium Sulphate Heptahydrate (MgSO4∙7H2O), 0.025 g of Potassium Sulphate (K2SO4), 1.25 g of Calcium Carbonate (CaCO3) and 5 g of agar. The mixture was diluted in 250 ml of distilled water and sterilized in an autoclave at the temperature of 121˚C for 15 minutes. The agar was poured into a petri dish and allowed to solidify at room temperature. Serial dilution was made and the sample was swabbed on the solidified agar with a swab stick and incubated at room temperature.
7.2. Bacillus spp.
Hicrome Bacillus agar differential medium for identification of Bacillus species was used to isolate Bacillus subtilis, Bacillus megaterium and Bacillus thuringiensis.
8. Chemical Characterization of the Experimental Soil, Biofertilizer and Chemical Fertilizer
8.1. Soil Nutrient Analysis
The soil was characterized for Nitrogen, Potassium and Phosphorus nutrient content before the planting.
8.2. Nitrogen Content of the Biofertilizer
The microkjeldal method was used for the determination of Nitrogen. 1 gram of the soil sample weighed into a kjeldahl flask, and 10 gram of sodium sulphate was added into it, followed by 20 ml of concentrated sulphuric acid and 1 gram of copper (II) sulphate (pentahydrate). The flask containing the mixture was heated on a Bunsen burner at an angle of 60˚ until the solution was completely digested and the color changed from blackish color to bluish green. The solution was allowed to solidify for a period of 24 hours which changed the solution to white color. The solidified sample was dissolved with 200 ml of distilled water and 40% sodium hydroxide was added to it. The dissolved mixture was transferred into a 500 ml flat bottom flask and two to four pieces of zinc metal were introduced. The flask was connected to the distillation column. In the set-up, 100 ml of 4% boric acid was prepared in a conical flask and two drops of methyl red indicator was added into it of which a light pink color was obtained. The distillate was allowed to make contact with the boric acid which acts as an absorber. When the liquid in the absorber reached 200 ml marked on the conical flask, the distillation was stopped by disconnecting the distillation apparatus. The absorber was back titrated with 0.1 N sulphuric acid. The titration was stopped when the color of the distillate turned back to the initial color of the mixture of boric acid and methyl red indicator i.e. a light pink color.
8.3. The Nitrogen Content Was Calculated as Follows
100 × Titer value × 0.0014/weight of the sample used.
Where: 100 = percentage conversion.
0.0014 = the constant. This means that 0.0014 g of Nitrogen will be liberated by 1 ml of 0.1 N sulphuric acid.
8.4. Phosphorus Content of the Biofertilizer
The soil sample was digested with concentrated H2SO4 and HNO3 in the presence of CuSO4 and K2SO4. After digestion, the solution was neutralized with NaOH using phenolphthalein indicator. The solution was treated with ammonium molybdate and stannous chloride solution and was left to stand for 5 minutes. A blue color was obtained and its absorbance was measured with a spectrophotometer at 690 nm.
The phosphorus content was calculated as follows:
Absorbance × Volume of diluting flask × 100/1000 × Volume of sample used.
8.5. Potassium Content of the Biofertilizer
The soil sample was leached with ammonium acetate solution and the potassium content was estimated by flame photometry.
The potassium content was calculated as follows:
Absorbance × Volume of diluting flask × 100/1000 × Volume of sample used.
9. Application of the Fertilizers
The Nitrogen:Phosphorus:Potassium (NPK) ratio of the chemical fertilizer used was N:15, P:15, K:15, while the NPK composition of the biofertilizer was N:2.5, P:3.5, K:2.5. The planting beds (4 m2 in size) were prepared in triplicates for control, chemical fertilizer and biofertilizer respectively. Eight hundred grams (800 gm) of chemical fertilizer was applied on each of the three beds 2 weeks after the corns were cultivated. Ten (10 ml) of the concentrated biofertilizer solution was diluted in 1000 ml (1 litter) of distilled water before every application on the crop, which was applied to the corn plants daily, starting from the first day of their germination. Application was carried out at dawn to prevent the destruction of the resident microorganisms in the biofertilizer by the excess heat (sun rays) if applied during the day.
10. Results
Biofertilizer consistently and significantly increased the height of corn (Zea mays) compared to other treatments. At six weeks of planting, the height of corn treated with biofertilizer was observed to significantly (P < 0.05) increase to (193 cm) compared to NPK and the control. Also at 8 weeks after planting the height of the corn was observed to significantly (P < 0.05) increase to (225 cm) compared to other treatments (Table 3), with simultaneous higher increase in weight of yeild of plants treated with biofertilizer as against others (Table 6). As indicated in Table 4, the highest value of standard deviation of the biofertilizer showed the improved effect of this treatment on the growth performance of the plants over the other treatments.
Comparative analysis of the chemical compositions of the soil, synthetic/chemical fertilizer and the biofertilizer showed that the chemical fertilizer has equal ratio of nitrogen:phosphorus:potassium of 15:15:15, much higher than the ratio of the chemical composition of biological fertilizer of 2.46:3.49:2.5 and that of the soil—0.6:4.2:2.5 (Table 1). Comparing the above NPK values of the different fertilizers, it could be noticed that these values did not directly translate to the crop performance as shown in Table 4. In other words, it could not be said that the higher the NPK value in any given fertilizer the better the performance of the crop. Other factors have a role to play. Phosphate (P), as one of the most important elements for plant growth, is more abundant in chemical fertilizer than in biofertilizer (Table 1), but its availability is limited to plants [6] [11]. Phosphorus in agricultural soils is mostly present in form of insoluble phosphate and therefore unavailable for plant’s utilization (Tables 1-5).
The presence of microbes and other trace elements in the biofertilizer might have contributed to the improved performance of the corn plants treated with biofertilizer as against the performance of the crops treated chemical fertilizer and the control without microbial inoculum. [20] reported the complexity of the interactions of soil organisms and the target plants. A number of bacterial genera have been identified and used as Plant Growth-Promoting Biofertilizer (PGPB) and include Bacillus spp., Pseudomonas spp., and Azotobacter spp. Plant Growth Promoting Biofertilizer or microbial fertilizer has been defined as substance composed of living microorganisms and mixture of biodegradable substances applied to soil, seed or plant surfaces, which colonizes the interior
Table 1. Chemical composition of the experimental soil (control), chemical fertilizer and biofertilizer.
Table 2. Mode of treatments (triplicates): control, chemical fertilizer and biofertilizer.
Beds numbered from 1 - 3 were not treated with any type of fertilizer (Control), beds numbered from 4 - 6 were treated with chemical fertilizer (NPK) and beds numbered from 7 - 10 were treated with biofertilizer.
Table 3. The effect of application of chemical fertilizer and biofertilizer on corn plant growth (measured in height—cm).
Plant height was measured from the base of the plant to the tip of the plant.
part of the plant, via rhizosphere or intercellular spaces, that enhanced the growth and yields of the host plant by increasing availability of primary nutrients, such as nitrogen, phosphorus and potassium. They have been tested and reported as effective microbial inoculants used to improve soil and plant fertility
Table 4. Mean heights of corn plants treated with chemical fertilizer and biofertilizer (cm).
Table 5. Mean number of corn cobs at harvest per treatment.
Table 6. Weight of corn per treatment (gm).
Figure 1. Graphic representation of mean value of growth of corn (Zea mays) planted with the two fertilizers and the control.
[21] - [25] as observed in this work. Nitrogen, Phosphorus, Potassium (NPK) and other trace elements contained in fertilizers had been wrongly described as plant food; however, NPK are vital elements required for cell division and enzyme processes that allow photosynthesis and plant growth. Figures 3-5 above represent corn plants not treated with any fertilizer (control), those treated with chemical fertilizer and those treated with biofertilizer respectively; it could be noticed that while Figure 4 and Figure 5 demonstrated evidence of increased growth against the control plant (Figure 5), apart from increased growth also demonstrated protection against insect/pest attack as shown by the healthier leaves/blades of the plants (Figures 1-5).
Figure 2. Mean weight of corn per treatment (gm).
Figure 4. Corn plant treated with chemical fertilizer.
Figure 5. Corn plant treated with biofertilizer.
11. Conclusion
Based on the findings and the observations made, it was concluded that the biofertilizer has a higher crop performance efficiency than the chemical fertilizer. The Plant Growth Promoting Bacteria isolated and used as biofertilizer in this research work also demonstrated the ability to protect the corn plants from pathogen/insect attack and therefore can serve as both biofertilizer and biopesticide or biocontrol agent.
Acknowledgements
The authors are thankful to the Vice Chancellor of Godfrey Okoye University, Thinker’s Corner, Enugu, for the supply of the reagents and to the Director and staff of Masdevan Integrated Farming System (Songhai Model), Urum, Awka, Anambra State, Nigeria for their material and infrastructural provision.