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Bacteria Project

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Bacteria

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University of Puerto Rico Cayey Campus 2015 RISE Program Pérez-Ayala, Michelle C.1, Figueroa-Monsanto, Héctor L.2 , Maricelys3 , and Cruz, Giovanni4 Department of Biology, University of Puerto Rico at Cayey1, Department of Chemistry, University of Puerto Rico at Cayey2 , Hugher Hughes Program3, and RISE Program4 Introduction Microbiology is the field of science that focuses on the study of the morphology, application, and relevance of microorganisms, such as bacteria with the use of microscopes and technical procedures. These microorganisms or specimen,belong to the Bacteria Domain and Monera Kingdom and are found in moist areas. Among these places, bacteria can be located on epithelial surfaces, saliva, nail grime, as well as on top of desks, and even within soils. Actually, these diverse localizations have given these living organisms specific characteristics that permit them to be either heterotrophic or non-heterotrophic. Non-heterotrophic or autotrophic microorganisms play an eminent role in processes, such as nitrogen fixation benefiting plants, but not all bacteria have an optimistic symbiotic relationship or effect on living organisms. Heterotrophic organisms are adaptable to many organically formed compositions, such as humans???, acting positively or negatively. In contrast to the autotrophic individuals (I don’t think it is appropriate to refer to a bacteria as an individual.), heterotrophic organisms create negative outcomes on humans. For instance, the species Treponella palidium causes a skin disease called syphilis. This promotes the development of sores throughout the body by having contact with bodily fluids through sexual intercourse. Scientists have focused on not only the nourishment preference of these microorganisms, but also on their cellular wall composition, which makes them either gram positive or gram negative.
Gram-negative bacteria are more difficult to inhibit with antibiotics compared to gram- positive ones, due to the double layer of peptidoglycans in their cell wall. Gram-negative bacteria can be identified under the compound microscope because they retain pink or red stains from the conservation of safranin during the wet mount and gram staining methods. In contrast, if the stains are purple, they are classified as gram positive from crystal violet solution retention followed by the addition and rinse of both iodine and ethanol. This type of bacteria is more vulnerable to antibiotics because it has only one layer of peptidoglycan. Surprisingly, uncultured bacteria (gram positive/negative) methods of recompilation have permitted researchers to find bacterial compounds, such as teixobactin with the capacity to impede bacteria from emerging (Ling et al. 2015). Teixobactin is a compound that has shown to be more effective in terms of bacteria inhibition, compared with other antibiotics, such as ofloaxin (Ling et al. 2015). In addition, another type of antimicrobial chemical made of lipopeptide is called battacin. It was isolated from the soil bacterium Paenibacillus tianmuensis and has shown a potent inhibition effect. For instance, it has the capacity to eradicate bacteria in vitro or in cell culture, as well as gram-negative bacteria (Qian et al. 2012). Popowska et al. (2012), have compared the soil bacteria resistance, instead of contrasting antibiotic ability to inhibit these microrganisms. Specifically, exposing the bacteria to a soil located underneath animals that contained specific antibiotics with the purpose of testing their inhibition effects (This sentence lacks clarity.). In other words, uncultured bacterium can have a wide range of characteristics that can give it the capacity to create resistance to certain antibiotics. Both cultured and uncultured bacteria have been the precursors of many antibiotic chemical compounds that have inhibited disease-causing bacterium. These same antimicrobials have created resistance or mutations against the same antibiotics. The resistance effect may occurs 30 years after being placed on the market provoking or caused serious health issues. For this reason, there is an urgent need to find bacteria- generated compounds that will serve as long-term effective antimicrobials. The purpose of this study is to identify if harvested soil collected bacteria will develop a compound similar in capacity as the teixobactins. Also, in this study, soil cultured bacteria collected will be grown in order to identify only one type of bacteria genera with
the purpose of discovering an antibiotic that is able to inhibit the division capacity of the bacteria. expand this section. MATERIALS AND METHODS Soil Collection from Rhizosphere. Samples were collected from two types of soils rich in nutrients from the rhizosphere. In order to collect both soil samples, the rhizosphere digging areas were cleared and a small hole was made on each surface. Both samples were collected with two individual wrapped plastic spoons until 25% (1/4 parts) of two zip lock bags were filled, respectively. Pictures were also taken as evidence of the soil collection. The first collection was from a moist soil located in an urban area at 26˚C at 146˚ SE Caguas, PR 18˚14’25”N 66˚4’7” W. The area was surrounded by animals such as ducks, and chickens, among other. A second sample was collected from a rural area approximately 25 ˚C during the noon at 8:02a.m. in Patillas, PR 17˚53’31”N 65˚53’18” W. Weight and Dilution of Soil. One gram of the soil samples was weighted and diluted, in order to obtain a smaller number of bacteria. Each weighted soil was added to a 10mL saline H2O and NaCl (0.9%) solution containing test tube and then mixed on a Vortex, respectively. To diminish the concentration inside each tube and end up with a fewer number of bacteria, 200µL of each concentration was transferred to an individual 1.5mL centrifuge tube (100) and 20µl of NaCl were also added. Five different 1.5mL tubes (10-1, 10-2, 10-3, 10-4, 10-5) were filled with 180µL of NaCl. To complete the dilution, 20µL were transferred from the 100 to the 10-1 and the same process was repeated until 10-5. The TSA and R2A agar plates were smeared with 30µL of the 100 and 10-5 tubes to grow the bacteria at a temperature of 30˚C during twenty four hours incubation. Purification of Bacteria. The medium plates that showed bacterial growth were purified to eliminate unnecessary debris and to isolate one type of colony,
according to its morphology. In purification #1 to #5, an inoculator loop was used to swap a group of colonies off the R2A 100 plate onto three areas (North, East, and South) of a new R2A agar. Using a sterilized loop, the colonies were first smeared in a zig-zag motion on the North side of the plate. Then, the plate was closed, the loop was sterilized on the Bunsen burner, the plate cover was opened, the loop was pressed carefully on a corner of the plate where no bacteria was present, the bacteria were dragged from the previous section (North) to the next (East) several times, and at the last movement was zig-zag motion on the East. The same process was performed for the South. The new R2A plate was stored inside the incubator at 30˚C and the first R2A 100 plate was placed in the refrigerator. The same process was performed with the TSA 100 plate, prepared on the previous process using a new TSA plate. Gram Staining. An inoculator loop was used to swap one colony from a purified plate and rubbed and mixed with a drop of deionized water onto a microscope slide. Crystal violet was added followed by water to rinse off the excess purple dye. The same process was repeated with iodine, ethanol, and saphranin. The slide was then observed under the microscope to recover an image and determine the same colony morphology (color, margin, elevation, size, texture, appearance, pigmentation, and optical property). Freezing. This process is meant primarily to save a portion of the bacteria for further use. First, 1.5mL of the broth, equivalent liquid media, and 200µL of glycerol, which allows the bacteria colony to freeze but not to die at low temperatures, were deposited in a 2.0mL micro tube. Then the tubes were labeled for further usage and tests for other parts of investigation. Electrophoresis. This technique was utilized to characterize the DNA by band sizes, but in order to have an appreciable amount the DNA must be replicated by using PCR (polymerized chain reaction). This process seeks to replicate and amplify the DNA that is to be studied by setting it into different temperatures
specifically: 95˚C which denaturalizes the DNA breaking the chains of DNA, next a temperature of 60 ˚C for the process of annealing were the base pairing is taking place and finally extending the DNA chains at about 72 ˚C. After the replication proceeding to run the PCR adding the replicated DNA with an amount of dye because the DNA does not exhibit color and wouldn’t be visible in the gel. The DNA, RNA and proteins at the electrophoresis are measured based on a sample that runs the entire gel better referred to as the ladder. Once the electrophoresis is finished, it was read and the length of how far the DNA ran was determined identifying it by its size or charge. Antibiotic Resistance Test. Using the corresponding media plate with specific antibiotics randomly testing upon five of any antibiotics in order to detect if our bacteria has any resistance against any of those. Striking with the selected antibiotics and placing a test paper with the bacteria broth for easy identification of any resistance. It was verified after incubating it at 30 ˚C for a day. Antibiotic Production Test. The bacteria M.Luteous and E. Coli were each smeared in a media plate. A test paper was soaked with the bacteria broth and placed in the plates. The broth is a previously fixed mix with 1.5mL of the equivalent liquid media and left to stir and maintain an aqueous character. This test will result in the creation of a ring all around that will mean the bacteria does produce antibiotic, but if not it means it doesn’t present this particular characteristic. Oil Degradation. In order to test the susceptibility of the bacteria, a plate that has only a media of oil was made. The selected bacterium was streaked into the oiled plate for testing. The main purpose of this test is to verify if the bacteria will either feed of the oil surface or repel against it. An inoculator loop was used to swap one colony from a purified plate and rubbed and mixed with a drop of deionized water onto a microscope slide. Crystal violet was added followed by water to rinse off the excess purple dye. The same process was
repeated with iodine, ethanol, and saphranin. The slide was then observed under the microscope to recover an image and determine the same colony morphology including (color, margin, elevation, size, texture, appearance, pigmentation, and optical property). 2.5 Freezing This process was meant primarily to save a portion of the bacteria for further use. First, 1.5mL of the broth, an equivalentamount of liquid media, and 200µL of glycerol, which allows the bacteria colony to freeze but not die at low temperatures, were deposited in a 2.0mL micro tube. Then the tubes were labeled for further usage and tests for other parts of investigation. 2.6 Electrophoresis DNA was replicated and with the Polymerized Chain Recation (PCR). Electrophoresis was utilized to characterize the DNA by band sizes The PCR setting involved different temperatures specifically: 95˚C, which denaturalizes the DNA breaking the chains of DNA, next a temperature of 60 ˚C for the process of annealing were the base pairing takes place and finally extending the DNA chains at about 72 ˚C. After the replication, ethidium bromide was added to the DNA copies to work as the fluorescent tag. The DNA, RNA, and proteins in the electrophoresis were divided based on size. The DNA with the tag and the DNA ladder that reflects the base pairs were added the agarose gel. Once the electrophoresis was finished, the gel was observed to compare the DNA of the bacteria with the 16S gene that codifies for samples that are bacteria. 2.7 Antibiotic Production Test The bacteria M. luteous and E. coli were tested for antibiotic resistance caused by mutation by placing each bacterium on agar plates. Four test papers were soaked with the bacteria broth, previously fixed mix with 1.5mL of the equivalent liquid media and left to stirred for and maintain an aqueous character. Two papers were placed on each agar plate with the bacterium. 2.8 Oil Degradation To test if the bacteria would either feed off the oil surface or repel against it, the bacterium that was positive on the electrophoresis gel was streaked onto a plate of oil media for an incubation period of seven days at 30 ˚C. 3. Results 3.1 Soil collection from rhizosphere The first soil collection area is shown in Figure 1. it includes the flora and lake that surrounds it. The main animals that commonly pass through this area are chickens,
ducks, and dogs. Both this and the parameters included in Table1. show that there is a probability of finding bacteria in the gathered soil. Figure 1. a, Shows the tree next to the soil collection area where the animals, including humans tread roughly or calmly. b, The whole at the left of the bag less than a meter away from the tree trunk. c, The whole was about an inch deep surrounded by green grass and it contained roots from the same tree. The second soil collection area is shown in Figure 2. it, which includes the flora and shows absence of no water sources around. Only domestic animals such like dogs, cats, chickens, iguanas and humans pass through by this area. Figure 2 Both this and the parameters included in Table1. show that there is a probability of finding bacteria. Figure 2. a, Shows the soil collection area approximately near to many types of trees. b, The hole was a fairly deep one with an approximate radius of three inches. c, The hole within had grass roots, dirt pebbles, and small organisms worm like. Characteristics First soil collection Second soil collection 1. Temperature (˚C) 26˚C 25˚C 2. Coordinates 18˚14’25”N 66˚4’7” W 17˚53’31”N 65˚53’18” W 3. City, State 146˚ SE at Caguas, PR Patillas, PR 4. Soil Description It had a moist texture with visible grass and roots mixed with the soil particles It was moist during the morning, it lacked roots, and it had little organisms. 5. Surroundings The area was surrounded by animals such as ducks and chickens, among other The area included avocado cannon trees and a dog Table 1. These parameters reflect the circumstances of the collection area, as well as its location. a, b, c,
3.2 Weight and dilution of soil Approximately, 1.033±0.001 grams of the soil sample was weighted and diluted in six tubes (100 , 10-1 , 10-2 , 10-3 , 10-4 and 10-5 ) to obtain a smaller number of bacteria. Only the 100 tube previously spread in the TSA and R2A agar plates shown in Figure 2. Demonstrated showed bacteria colonies, after a weekend incubation at about 23˚C. These bacteria might be either registered in the DNA database or they may ight be a new genus or species. The 10-5 plate shown in Figure 3. had no bacteria growth and the plates were discarded. These might have been due to a higher presence of the aqueous NaCl. a, b, Figure 2. a, Shows the TSA 100 colonies with an extensive morphology explained in the Purification bacteria results. b, R2A 100 bacteria colonies were different from the TSA’s. a, b, Figure 3. a, Shows that the TSA 10-5 solution had no bacteria. b, R2A 10-5 had the same effect. 3.3 Purification of bacteria From the first soil collection, The TSA 100 colony morphology is shown in Table 2. and Table 3. shows the morphology for R2A 100 bacteria. TSA100 morphology Purr.#1 Purr.#2 Purr.#3
1. Shape Circular Circular Circular 2. Margin Curled Curled Entire 3. Elevation Flat Flat Convex 4. Size Moderate Punctiform, small and moderate Moderate 5. Texture Smooth Smooth Smooth 6. Appearance Dull Dull Dull 7. Pigmentation Cream Cream-yellow Cream 8. Optical property Opaque Opaque Opaque Table 2. TSA colony morphology. R2A 100 morphology Purr.#1 Purr.#2 Purr.#3 Purr.#4 Purr.#5 1. Shape Circular Circular Circular Circular and irregular Circular 2. Margin Entire and curled Curled Undulated and entire Curled Rhizoid 3. Elevation Flat Flat Raised Flat Flat 4. Size Punctiform and small Small or punctiform Punctiform, small, moderate and large Punctiform, small, moderate and large Punctiform, small and moderate 5. Texture Smooth Smooth Smooth Smooth Smooth 6. Appearance Dull Dull Dull Dull Dull 7. Pigmentatio n White White White White White 8. Optical property Opaque Opaque Opaque Opaque Opaque Table 3. R2A colony morphology. TSA 10-5 and colonies demonstrated different morphology when had a different purification.Purification #1 for TSA revealed a circular shape, curved margins , flat elevation, small, smooth texture, dull appearance, cream pigmentation, and an opaque optical property. The R2A 10-5 bacteria had more defined shape circular, curved with flat elevation, punctifor, with a smooth texture, dull appearance, white pigmentation, and the same optical property. For purification #2 the TSA 10-5 plate showed bacteria with irregular shape, curled margin, flat elevation with sizes that vary from a type of cloth that covers the whole plate, , smooth texture, dull appearance, a cream-yellow pigmentation, and an opaque optical property. The R2A colonies showed the same shape, margin, and
elevation. The sizes were small or linear due to the streaking. They , smooth texture, dull appearance, white pigmentation, and an opaque optical property. The R2A (puur3) bacteria colonies had a cloch like appearence, an undulated and entire margin, flat elevation, punctiform at the edges, small, moderate and large sizes, smooth texture, dull appearance, white pigmentation, and opaque optical property. The R2A (puur.4) showed irregular shape, curled margin, flat elevation, all sizes, smooth texture, dull appearance, white pigmentation and opaque optical property. R2A (purr.5) presented linear shape, an entire margin, flat elevation, punctiform size, smooth texture, dull appearance, cream pigmentation and opaque optical property. 3.4 Gram staining From the first soil collection, both the TSA and R2A colonies showed purple pigmentations. The colonies were Streptobacillus gram negative, according to Figure 4.
a, b, c, d, Figure 4. a,b, Shows that the R2A 100 colonies are gram negative and Streptobacillus. c,d, sShows the Streptobacillus gram negative bacteria for TSA 100 . From the second soil sample according to Figure 5. when doing Gram staining the TSA Streptococcus colored in purple therefore tested to be gram positive. Also the R2A was proven to be Streptobacillus pink therefore tested to be gram negative.
Figure 5. 3.5 Freezing From the first soil sample two tubes Figure 6. each with 1.5 mL of broth, 0.2 mL of glycerol and the R2A colonies. a, b, c, d, Figure 6. a, Freezing of TSA bacteria. b, TSA back up. c, R2A frozen bacteria. d, R2A back up. 3.6 Electrophoresis
The R2A copies of the PCR were positive for the 16S gene, according to the electrophoresis gel in Figure 7. This shows that the DNA copies belonged to bacteria. Figure 7. a, The R2A DNA in line 4, without counting the DNA ladder, was positive to the 16S gene. 3.7 Antibiotic production test M. Luteous was inhibited only by TSA 100 , according to Figure 6 a,b,. E. coli on Figure 8. c,d, was not inhibited neither by TSA nor by R2A. This shows that TSA bacteria might have an antibiotic property on M. luteous. a, b,
c, d, Figure 8. a, b, Show that TSA bacteria had an antibiotic resistance on M. luteus, but R2A did not. c, d, E. coli was had no inhibition. 3.8 Oil degradation The oil degradation test for the bacteria was negative, according to Figure 9. This shows that the bacteria will not be useful to degrade oil in the development of oil-derived products. Figure 9. The plate was from another oil test. It shows the same negative result that displayed both soil collection bacteria. 4. Cited Literature Ling LL, Schneider T, Peoples AJ, Spoering AL, Engels I, Conlon BP, Mueller A, Sch¨aberle TF, Hughes DE, Epstein S et al. 2015. A new antibiotic kills pathogens without detectable resistance. Nature 517, 455–459. doi: 10.1038/nature14098. Popowska M, Rzeczycka M, Miernik A, Krawczyk-Balska A, Walsh F, Duffy B. 2012. Influence of soil use on prevalence of tetracycline, streptomycin, and erythromycin resistance and associated resistance genes. Antimicrobial Agents and Chemotherapy 53 (3): 1434-43. doi: 10.1128/AAC.05766-11.
Qian CD, Wu XC, Teng Y, Zhao WP, Li O, Fang SG, Huang ZH, Gao HC. 2012. Battacin (octapeptin b5), a new cyclic lipopeptide antibiotic from Paenibacillus tianmuensis active against multidrug-resistant gram-negative bacteria. Antimicrobial Agents and Chemotherapy 56(3): 1458-1465. doi: 10.1128/AAC.05580-11.

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Bacteria Project

  • 1. University of Puerto Rico Cayey Campus 2015 RISE Program Pérez-Ayala, Michelle C.1, Figueroa-Monsanto, Héctor L.2 , Maricelys3 , and Cruz, Giovanni4 Department of Biology, University of Puerto Rico at Cayey1, Department of Chemistry, University of Puerto Rico at Cayey2 , Hugher Hughes Program3, and RISE Program4 Introduction Microbiology is the field of science that focuses on the study of the morphology, application, and relevance of microorganisms, such as bacteria with the use of microscopes and technical procedures. These microorganisms or specimen,belong to the Bacteria Domain and Monera Kingdom and are found in moist areas. Among these places, bacteria can be located on epithelial surfaces, saliva, nail grime, as well as on top of desks, and even within soils. Actually, these diverse localizations have given these living organisms specific characteristics that permit them to be either heterotrophic or non-heterotrophic. Non-heterotrophic or autotrophic microorganisms play an eminent role in processes, such as nitrogen fixation benefiting plants, but not all bacteria have an optimistic symbiotic relationship or effect on living organisms. Heterotrophic organisms are adaptable to many organically formed compositions, such as humans???, acting positively or negatively. In contrast to the autotrophic individuals (I don’t think it is appropriate to refer to a bacteria as an individual.), heterotrophic organisms create negative outcomes on humans. For instance, the species Treponella palidium causes a skin disease called syphilis. This promotes the development of sores throughout the body by having contact with bodily fluids through sexual intercourse. Scientists have focused on not only the nourishment preference of these microorganisms, but also on their cellular wall composition, which makes them either gram positive or gram negative.
  • 2. Gram-negative bacteria are more difficult to inhibit with antibiotics compared to gram- positive ones, due to the double layer of peptidoglycans in their cell wall. Gram-negative bacteria can be identified under the compound microscope because they retain pink or red stains from the conservation of safranin during the wet mount and gram staining methods. In contrast, if the stains are purple, they are classified as gram positive from crystal violet solution retention followed by the addition and rinse of both iodine and ethanol. This type of bacteria is more vulnerable to antibiotics because it has only one layer of peptidoglycan. Surprisingly, uncultured bacteria (gram positive/negative) methods of recompilation have permitted researchers to find bacterial compounds, such as teixobactin with the capacity to impede bacteria from emerging (Ling et al. 2015). Teixobactin is a compound that has shown to be more effective in terms of bacteria inhibition, compared with other antibiotics, such as ofloaxin (Ling et al. 2015). In addition, another type of antimicrobial chemical made of lipopeptide is called battacin. It was isolated from the soil bacterium Paenibacillus tianmuensis and has shown a potent inhibition effect. For instance, it has the capacity to eradicate bacteria in vitro or in cell culture, as well as gram-negative bacteria (Qian et al. 2012). Popowska et al. (2012), have compared the soil bacteria resistance, instead of contrasting antibiotic ability to inhibit these microrganisms. Specifically, exposing the bacteria to a soil located underneath animals that contained specific antibiotics with the purpose of testing their inhibition effects (This sentence lacks clarity.). In other words, uncultured bacterium can have a wide range of characteristics that can give it the capacity to create resistance to certain antibiotics. Both cultured and uncultured bacteria have been the precursors of many antibiotic chemical compounds that have inhibited disease-causing bacterium. These same antimicrobials have created resistance or mutations against the same antibiotics. The resistance effect may occurs 30 years after being placed on the market provoking or caused serious health issues. For this reason, there is an urgent need to find bacteria- generated compounds that will serve as long-term effective antimicrobials. The purpose of this study is to identify if harvested soil collected bacteria will develop a compound similar in capacity as the teixobactins. Also, in this study, soil cultured bacteria collected will be grown in order to identify only one type of bacteria genera with
  • 3. the purpose of discovering an antibiotic that is able to inhibit the division capacity of the bacteria. expand this section. MATERIALS AND METHODS Soil Collection from Rhizosphere. Samples were collected from two types of soils rich in nutrients from the rhizosphere. In order to collect both soil samples, the rhizosphere digging areas were cleared and a small hole was made on each surface. Both samples were collected with two individual wrapped plastic spoons until 25% (1/4 parts) of two zip lock bags were filled, respectively. Pictures were also taken as evidence of the soil collection. The first collection was from a moist soil located in an urban area at 26˚C at 146˚ SE Caguas, PR 18˚14’25”N 66˚4’7” W. The area was surrounded by animals such as ducks, and chickens, among other. A second sample was collected from a rural area approximately 25 ˚C during the noon at 8:02a.m. in Patillas, PR 17˚53’31”N 65˚53’18” W. Weight and Dilution of Soil. One gram of the soil samples was weighted and diluted, in order to obtain a smaller number of bacteria. Each weighted soil was added to a 10mL saline H2O and NaCl (0.9%) solution containing test tube and then mixed on a Vortex, respectively. To diminish the concentration inside each tube and end up with a fewer number of bacteria, 200µL of each concentration was transferred to an individual 1.5mL centrifuge tube (100) and 20µl of NaCl were also added. Five different 1.5mL tubes (10-1, 10-2, 10-3, 10-4, 10-5) were filled with 180µL of NaCl. To complete the dilution, 20µL were transferred from the 100 to the 10-1 and the same process was repeated until 10-5. The TSA and R2A agar plates were smeared with 30µL of the 100 and 10-5 tubes to grow the bacteria at a temperature of 30˚C during twenty four hours incubation. Purification of Bacteria. The medium plates that showed bacterial growth were purified to eliminate unnecessary debris and to isolate one type of colony,
  • 4. according to its morphology. In purification #1 to #5, an inoculator loop was used to swap a group of colonies off the R2A 100 plate onto three areas (North, East, and South) of a new R2A agar. Using a sterilized loop, the colonies were first smeared in a zig-zag motion on the North side of the plate. Then, the plate was closed, the loop was sterilized on the Bunsen burner, the plate cover was opened, the loop was pressed carefully on a corner of the plate where no bacteria was present, the bacteria were dragged from the previous section (North) to the next (East) several times, and at the last movement was zig-zag motion on the East. The same process was performed for the South. The new R2A plate was stored inside the incubator at 30˚C and the first R2A 100 plate was placed in the refrigerator. The same process was performed with the TSA 100 plate, prepared on the previous process using a new TSA plate. Gram Staining. An inoculator loop was used to swap one colony from a purified plate and rubbed and mixed with a drop of deionized water onto a microscope slide. Crystal violet was added followed by water to rinse off the excess purple dye. The same process was repeated with iodine, ethanol, and saphranin. The slide was then observed under the microscope to recover an image and determine the same colony morphology (color, margin, elevation, size, texture, appearance, pigmentation, and optical property). Freezing. This process is meant primarily to save a portion of the bacteria for further use. First, 1.5mL of the broth, equivalent liquid media, and 200µL of glycerol, which allows the bacteria colony to freeze but not to die at low temperatures, were deposited in a 2.0mL micro tube. Then the tubes were labeled for further usage and tests for other parts of investigation. Electrophoresis. This technique was utilized to characterize the DNA by band sizes, but in order to have an appreciable amount the DNA must be replicated by using PCR (polymerized chain reaction). This process seeks to replicate and amplify the DNA that is to be studied by setting it into different temperatures
  • 5. specifically: 95˚C which denaturalizes the DNA breaking the chains of DNA, next a temperature of 60 ˚C for the process of annealing were the base pairing is taking place and finally extending the DNA chains at about 72 ˚C. After the replication proceeding to run the PCR adding the replicated DNA with an amount of dye because the DNA does not exhibit color and wouldn’t be visible in the gel. The DNA, RNA and proteins at the electrophoresis are measured based on a sample that runs the entire gel better referred to as the ladder. Once the electrophoresis is finished, it was read and the length of how far the DNA ran was determined identifying it by its size or charge. Antibiotic Resistance Test. Using the corresponding media plate with specific antibiotics randomly testing upon five of any antibiotics in order to detect if our bacteria has any resistance against any of those. Striking with the selected antibiotics and placing a test paper with the bacteria broth for easy identification of any resistance. It was verified after incubating it at 30 ˚C for a day. Antibiotic Production Test. The bacteria M.Luteous and E. Coli were each smeared in a media plate. A test paper was soaked with the bacteria broth and placed in the plates. The broth is a previously fixed mix with 1.5mL of the equivalent liquid media and left to stir and maintain an aqueous character. This test will result in the creation of a ring all around that will mean the bacteria does produce antibiotic, but if not it means it doesn’t present this particular characteristic. Oil Degradation. In order to test the susceptibility of the bacteria, a plate that has only a media of oil was made. The selected bacterium was streaked into the oiled plate for testing. The main purpose of this test is to verify if the bacteria will either feed of the oil surface or repel against it. An inoculator loop was used to swap one colony from a purified plate and rubbed and mixed with a drop of deionized water onto a microscope slide. Crystal violet was added followed by water to rinse off the excess purple dye. The same process was
  • 6. repeated with iodine, ethanol, and saphranin. The slide was then observed under the microscope to recover an image and determine the same colony morphology including (color, margin, elevation, size, texture, appearance, pigmentation, and optical property). 2.5 Freezing This process was meant primarily to save a portion of the bacteria for further use. First, 1.5mL of the broth, an equivalentamount of liquid media, and 200µL of glycerol, which allows the bacteria colony to freeze but not die at low temperatures, were deposited in a 2.0mL micro tube. Then the tubes were labeled for further usage and tests for other parts of investigation. 2.6 Electrophoresis DNA was replicated and with the Polymerized Chain Recation (PCR). Electrophoresis was utilized to characterize the DNA by band sizes The PCR setting involved different temperatures specifically: 95˚C, which denaturalizes the DNA breaking the chains of DNA, next a temperature of 60 ˚C for the process of annealing were the base pairing takes place and finally extending the DNA chains at about 72 ˚C. After the replication, ethidium bromide was added to the DNA copies to work as the fluorescent tag. The DNA, RNA, and proteins in the electrophoresis were divided based on size. The DNA with the tag and the DNA ladder that reflects the base pairs were added the agarose gel. Once the electrophoresis was finished, the gel was observed to compare the DNA of the bacteria with the 16S gene that codifies for samples that are bacteria. 2.7 Antibiotic Production Test The bacteria M. luteous and E. coli were tested for antibiotic resistance caused by mutation by placing each bacterium on agar plates. Four test papers were soaked with the bacteria broth, previously fixed mix with 1.5mL of the equivalent liquid media and left to stirred for and maintain an aqueous character. Two papers were placed on each agar plate with the bacterium. 2.8 Oil Degradation To test if the bacteria would either feed off the oil surface or repel against it, the bacterium that was positive on the electrophoresis gel was streaked onto a plate of oil media for an incubation period of seven days at 30 ˚C. 3. Results 3.1 Soil collection from rhizosphere The first soil collection area is shown in Figure 1. it includes the flora and lake that surrounds it. The main animals that commonly pass through this area are chickens,
  • 7. ducks, and dogs. Both this and the parameters included in Table1. show that there is a probability of finding bacteria in the gathered soil. Figure 1. a, Shows the tree next to the soil collection area where the animals, including humans tread roughly or calmly. b, The whole at the left of the bag less than a meter away from the tree trunk. c, The whole was about an inch deep surrounded by green grass and it contained roots from the same tree. The second soil collection area is shown in Figure 2. it, which includes the flora and shows absence of no water sources around. Only domestic animals such like dogs, cats, chickens, iguanas and humans pass through by this area. Figure 2 Both this and the parameters included in Table1. show that there is a probability of finding bacteria. Figure 2. a, Shows the soil collection area approximately near to many types of trees. b, The hole was a fairly deep one with an approximate radius of three inches. c, The hole within had grass roots, dirt pebbles, and small organisms worm like. Characteristics First soil collection Second soil collection 1. Temperature (˚C) 26˚C 25˚C 2. Coordinates 18˚14’25”N 66˚4’7” W 17˚53’31”N 65˚53’18” W 3. City, State 146˚ SE at Caguas, PR Patillas, PR 4. Soil Description It had a moist texture with visible grass and roots mixed with the soil particles It was moist during the morning, it lacked roots, and it had little organisms. 5. Surroundings The area was surrounded by animals such as ducks and chickens, among other The area included avocado cannon trees and a dog Table 1. These parameters reflect the circumstances of the collection area, as well as its location. a, b, c,
  • 8. 3.2 Weight and dilution of soil Approximately, 1.033±0.001 grams of the soil sample was weighted and diluted in six tubes (100 , 10-1 , 10-2 , 10-3 , 10-4 and 10-5 ) to obtain a smaller number of bacteria. Only the 100 tube previously spread in the TSA and R2A agar plates shown in Figure 2. Demonstrated showed bacteria colonies, after a weekend incubation at about 23˚C. These bacteria might be either registered in the DNA database or they may ight be a new genus or species. The 10-5 plate shown in Figure 3. had no bacteria growth and the plates were discarded. These might have been due to a higher presence of the aqueous NaCl. a, b, Figure 2. a, Shows the TSA 100 colonies with an extensive morphology explained in the Purification bacteria results. b, R2A 100 bacteria colonies were different from the TSA’s. a, b, Figure 3. a, Shows that the TSA 10-5 solution had no bacteria. b, R2A 10-5 had the same effect. 3.3 Purification of bacteria From the first soil collection, The TSA 100 colony morphology is shown in Table 2. and Table 3. shows the morphology for R2A 100 bacteria. TSA100 morphology Purr.#1 Purr.#2 Purr.#3
  • 9. 1. Shape Circular Circular Circular 2. Margin Curled Curled Entire 3. Elevation Flat Flat Convex 4. Size Moderate Punctiform, small and moderate Moderate 5. Texture Smooth Smooth Smooth 6. Appearance Dull Dull Dull 7. Pigmentation Cream Cream-yellow Cream 8. Optical property Opaque Opaque Opaque Table 2. TSA colony morphology. R2A 100 morphology Purr.#1 Purr.#2 Purr.#3 Purr.#4 Purr.#5 1. Shape Circular Circular Circular Circular and irregular Circular 2. Margin Entire and curled Curled Undulated and entire Curled Rhizoid 3. Elevation Flat Flat Raised Flat Flat 4. Size Punctiform and small Small or punctiform Punctiform, small, moderate and large Punctiform, small, moderate and large Punctiform, small and moderate 5. Texture Smooth Smooth Smooth Smooth Smooth 6. Appearance Dull Dull Dull Dull Dull 7. Pigmentatio n White White White White White 8. Optical property Opaque Opaque Opaque Opaque Opaque Table 3. R2A colony morphology. TSA 10-5 and colonies demonstrated different morphology when had a different purification.Purification #1 for TSA revealed a circular shape, curved margins , flat elevation, small, smooth texture, dull appearance, cream pigmentation, and an opaque optical property. The R2A 10-5 bacteria had more defined shape circular, curved with flat elevation, punctifor, with a smooth texture, dull appearance, white pigmentation, and the same optical property. For purification #2 the TSA 10-5 plate showed bacteria with irregular shape, curled margin, flat elevation with sizes that vary from a type of cloth that covers the whole plate, , smooth texture, dull appearance, a cream-yellow pigmentation, and an opaque optical property. The R2A colonies showed the same shape, margin, and
  • 10. elevation. The sizes were small or linear due to the streaking. They , smooth texture, dull appearance, white pigmentation, and an opaque optical property. The R2A (puur3) bacteria colonies had a cloch like appearence, an undulated and entire margin, flat elevation, punctiform at the edges, small, moderate and large sizes, smooth texture, dull appearance, white pigmentation, and opaque optical property. The R2A (puur.4) showed irregular shape, curled margin, flat elevation, all sizes, smooth texture, dull appearance, white pigmentation and opaque optical property. R2A (purr.5) presented linear shape, an entire margin, flat elevation, punctiform size, smooth texture, dull appearance, cream pigmentation and opaque optical property. 3.4 Gram staining From the first soil collection, both the TSA and R2A colonies showed purple pigmentations. The colonies were Streptobacillus gram negative, according to Figure 4.
  • 11. a, b, c, d, Figure 4. a,b, Shows that the R2A 100 colonies are gram negative and Streptobacillus. c,d, sShows the Streptobacillus gram negative bacteria for TSA 100 . From the second soil sample according to Figure 5. when doing Gram staining the TSA Streptococcus colored in purple therefore tested to be gram positive. Also the R2A was proven to be Streptobacillus pink therefore tested to be gram negative.
  • 12. Figure 5. 3.5 Freezing From the first soil sample two tubes Figure 6. each with 1.5 mL of broth, 0.2 mL of glycerol and the R2A colonies. a, b, c, d, Figure 6. a, Freezing of TSA bacteria. b, TSA back up. c, R2A frozen bacteria. d, R2A back up. 3.6 Electrophoresis
  • 13. The R2A copies of the PCR were positive for the 16S gene, according to the electrophoresis gel in Figure 7. This shows that the DNA copies belonged to bacteria. Figure 7. a, The R2A DNA in line 4, without counting the DNA ladder, was positive to the 16S gene. 3.7 Antibiotic production test M. Luteous was inhibited only by TSA 100 , according to Figure 6 a,b,. E. coli on Figure 8. c,d, was not inhibited neither by TSA nor by R2A. This shows that TSA bacteria might have an antibiotic property on M. luteous. a, b,
  • 14. c, d, Figure 8. a, b, Show that TSA bacteria had an antibiotic resistance on M. luteus, but R2A did not. c, d, E. coli was had no inhibition. 3.8 Oil degradation The oil degradation test for the bacteria was negative, according to Figure 9. This shows that the bacteria will not be useful to degrade oil in the development of oil-derived products. Figure 9. The plate was from another oil test. It shows the same negative result that displayed both soil collection bacteria. 4. Cited Literature Ling LL, Schneider T, Peoples AJ, Spoering AL, Engels I, Conlon BP, Mueller A, Sch¨aberle TF, Hughes DE, Epstein S et al. 2015. A new antibiotic kills pathogens without detectable resistance. Nature 517, 455–459. doi: 10.1038/nature14098. Popowska M, Rzeczycka M, Miernik A, Krawczyk-Balska A, Walsh F, Duffy B. 2012. Influence of soil use on prevalence of tetracycline, streptomycin, and erythromycin resistance and associated resistance genes. Antimicrobial Agents and Chemotherapy 53 (3): 1434-43. doi: 10.1128/AAC.05766-11.
  • 15. Qian CD, Wu XC, Teng Y, Zhao WP, Li O, Fang SG, Huang ZH, Gao HC. 2012. Battacin (octapeptin b5), a new cyclic lipopeptide antibiotic from Paenibacillus tianmuensis active against multidrug-resistant gram-negative bacteria. Antimicrobial Agents and Chemotherapy 56(3): 1458-1465. doi: 10.1128/AAC.05580-11.