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Mycobacteriophage Isolation from Tropical Soil Sample: Serotinus Alejandra M. De Jesús-Soto1 , Kenny J. Colón-Colón2 1 Department of Mathematics, University of Puerto Rico at Cayey, Puerto Rico 2 Department of Biology, University of Puerto Rico at Cayey, Puerto Rico A B S T R A C T Mycobacteriophages are viruses that infect a specific type of bacteria. This abundant microorganism can be easily obtained from soil samples. Using Mycobacterium smegmatis as a host, a mycobacteriophage was isolated and purified from a soil sample. The goal is to obtain a pure phage population in order to analyze the information and then include it in the Mycobacteriophages Database. The first step was to collect a soil sample in order to make the enrichment and filtrate. Three plaque purifications followed this step in the process. A pure phage population was isolated from a tropical soil in Puerto Rico and named Serotinus. Future work includes performing the spot test, a process to identify the phage’s web pattern. Knowing the phages genetic information allows the identification of characteristics that may lead to important discoveries in modern medicine. Phages therapy seems to be an alternative medical treatment. 1. Introduction Mycobacteriophages are DNA viruses that infect a specific type of bacteria belonging to the mycobacteria genus. These are the most abundant type of microorganism in the biological universe. Mycobacteriophage infections may or may not lead to the death of the bacterium. This depends on its life style, which can be lytic or lysogenic. Lytic cycles results in the destruction of the infected bacteria and its membrane. It is used by temperate or virulent phages to achieve reproduction. The virulent phage infects bacteria with genetic material in order to undergo cell lysis. On the other hand, temperate phages undergo lysogenic cycle, in which the phage DNA first integrates into the bacterial chromosome to produce the prophage and make the host a lysogen. When the bacterium reproduces, the prophage is also copied. The prophage can be copied or activated, a process in which the prophage exits the chromosomal material to enter the lytic cycle. The findings of existent phage research have traversed many arenas of genetics and have even instigated the conception of new therapies and medical treatments (George 2013). A critical problem in heath arose due to the emergence of pathogen bacteria resistant to most currently available antimicrobial agents. The development of alternate anti-infection modalities is one of the highest priorities of modern medicine. Therefore, phage therapy seems to be a solution for this problem. Mycobacteriophages have been isolated from a variety of environments around the world. They can be easily obtained from soil samples. Using
Mycobacterium smegmatis as a host, we sought to determine the presence of mycobacteriophages in a soil sample. Therefore, we hypothesized that we can isolate a mycobacteriophage population from a tropical soil sample in Puerto Rico. The objectives of this research are to isolate, purify, and harvest a novel phage population while the ultimate goal is to identify the characteristics of the phage that may serve modern medicine. 2. Materials and Methods Figure 1.Flow chart of the experimental procedure. Steps to isolate, purify and characterize a mycobacteriophage population from a soil sample. Each of the stages of the experiment was carried out by using the Sea-phages Resource Guide (2012) of the Science Education Alliance. There were some adjustments on procedures that had to be executed throughout the process to ensure the isolation and harvest of the bacteriophage. For this reason, alterations made during the procedure are included. Note that all materials used underwent a sterilization process, either by chemical methods using ethanol at 70% and Lysol® or by physical method using autoclave in aseptic technique during their use. It is recommended not to talk while doing any of the procedures to further avoid contamination.
2.1. Sample Collection Soil sample was collected from optional locations such as in wet places or where there was decomposition. After digging a few centimeters the collected samples were maintained in a sterile container. Data regarding localization coordinates, environmental temperature, excavation depth and moisture content was recorded. 2.2. Enrichment In a 50 mL conical tube, 0.500 g of the soil sample was mixed with Master Mix, substance that contained 8 mL of sterilized water, 1 mL of 10x 7H9/glycerol broth and 1 mL of AD supplement and 0.1 mL of CaCl (Science Education Alliance. 2012). Finally, 1 mL of Mycobacterium smegmatis was added and the solution was incubated at 37°C and aerated at 220 rpm for 16-24 hours (Science Education Alliance 2012). 2.3. Filtration After completion of the incubation period, solution was centrifuged at 3,000 rpm for 15-20 minutes. Afterwards, supernatant was filter-sterilized and poured into a 15mL conical tube. Both the pellet and the supernatant were stored. 2.3.1 Centrifuge Another option to obtain a purer sample from the enrichment protocol after centrifuging the conical tube of the enrichment protocol was to take 1 mL of the supernatant from the conical tube and transfer it to a microtube. The microtube was centrifuged at 10,000 rpm for 10 minutes. Then, 500 µL of the supernatant of the centrifuged microtube was transferred to another microtube to obtain the filtrate. 2.4 Plate Streaking A sterile utensil (wooden stick) was moistened with the filter-sterilized supernatant once. It was then used to gently swipe streaks on the Luria medium agar plate in quadrants. Figure 2 shows the correct way of streaking a plate. The segment labeled as (1) was first streaked, and then, another sterile swab was used to drag part of sample segment (1) to segment (2). The process of taking a sample from segment (2) and dragging it to segment (3) was repeated. Then, 4.5 mL of ~55.0o C Top Agar and 0.5 mL of the Mycobacterium smegmatis were poured into the plate from quadrant 3 to quadrant 1. The plate was closed by placing the cap on top. Finally, after agar solidification the plate was placed in an incubator at 37°C for ~24 hours (Science Education Alliance 2012). After this part of the procedure, the presence of mycobacteriophages in the collected sample was finally determined. 2.5. Plaque purification Figure 2. Streaking Technique. Available source: http://faculty.mc3.edu/jearl/ML/streak1.gif After confirming the presence of mycobacteriophages, the next step consisted in the extraction of an isolated plaque using the wooden tip of a sterile swab. Part of the
plaque was transferred to a sterile microtube that contained 25 µL (microliters) of Phage Buffer (PB) which would help with the dilution and sustain the mycobacteriophages on the plaque. The plaque sample was streaked in a “smeg plate” (2.4 plate streaking protocol) and was left to rest from 16-24 hours until the next day. This plaque extraction procedure was progressively repeated with each plate until the third (3) plate was obtained. This was done to assure the pureness of a single type of phage from each plaque sample. The plaque purification samples of each three repetitions were placed in an environment temperature of 4°C (Science Education Alliance. 2012). 2.6 Phage-Titer Assay The third plaque purification sample went through another enrichment protocol (2.2). This was made for supplementing the purified mycobacteriophage. Eight (8) microtubes were labeled from 1 to 8. A volume of 90 µL (microliters) of PB was added to each microtube. In the microtube labeled (1), 10 µL (microliters) of the supernatant of the enrichment of the third plaque purification sample was added. Later, 10 µL (microliters) were extracted from microtube (1) to microtube (2). The same process was done going from the microtube (2) to microtube (3). This step was repeated successively until all 8 microtubes were diluted. 2.7 Empirical Test A smeg plate was prepared after labeling it and drawing eight (8) square divisions on the bottom of it with a number corresponding to the division on an edge for better plaque view. Before going to the important part of the empirical test, 4.5 mL of TA and 0.5 mL of Mycobacterium smegmatis were mixed and spread on top of the Luria medium Agar. Next, 10 µL of the sample of microtube (1) from the phage-titer dilutions was added to the square segment labeled with the same number. The process was repeated for each microtube sample on the corresponding numbered segment. The plate is then placed in an incubator at 37°C for 16-24 hours (Science Education Alliance 2012). 3. Results Twenty individual soil samples were collected and analyzed (Table 1). Positive results were obtained from sample #18 which was collected from an urban area in the city of Cayey. Location coordinates were: 18.11524 North, 66.137 West. The sample was collected 2.3 centimeters beneath the surface in an environment whose temperature skirted 25.0º Celsius. After collecting and enriching the sample, the presence of mycobacteriophages was confirmed. Then, after three plaques purifications, a phage with clear plaques was isolated (Figure 2). Currently, the process within this project is still in the MTPL, Medium Titter Phage Lysate. The next step was to perform a spot test in order to identify the mycobacteriophage’s web pattern and record results in the Mycobacteriophages Database. Figure 3. Clear plaques obtained after third purification.
4. Discussion This research on the collection and analysis of a soil sample for the isolation of a phage has been a worthwhile laboratory experience. Although the process was somewhat tedious and frustrating at the beginning due to all the negative results it was a learning experience that taught us patience, dedication and perseverance. Finally, after analyzing 20 samples, a mycobacteriophage was isolated and named Serotinus. After three purifications, the phage formed clear plaques on his host Mycobacterium Smegmatis, indicating that Serotinus is most likely a lytic phage. Future work would include completing the entire process of identifying and characterizing the phage in order to record and send the information to the Mycobactoriophages Database. The implications of isolating phages could lead to new and interesting developments in modern medicine. Currently, much research is being done related to phage therapy, and the study of novel phage populations could lead to promising discoveries. 5. Acknowledgments: This work was funded by the Howard Hughes Program and the RISE Program at the University of Puerto Rico at Cayey. The authors would like to thank Dr. Michael Rubin, Dr. Edwin Vazquez, Mr. Joseph Perez, Mr. Giovanni Cruz, Mr. Gustavo Martínez and Mr. Christopher Quintanal for their support during the entire process. 6. Literature Cited Alvarado EJ, Cruz-Arzón JA. 2013. Mycobacteriophage isolation from tropical soil sample: Mikriplithari and Ususindagari. Department of Mathematics- Physics, University of Puerto Rico at Cayey, Puerto RicoDepartment of Biology, University of Puerto Rico at Cayey, Puerto Rico. George MP. 2013. Mycobacteriophage Meru: Isolation and Characterization of a Novel Mycobacteriophage. [Internet]. [cited 2014 May 26], 5(10):1-3. Available from http://www.studentpulse.com/articles/770/m ycobacteriophage-meru-isolation-and- characterization-of-a-novel- mycobacteriophage Rubin M, Vázquez E. 2012. Mycobacteriophage Proteomics: From Genotype to Phenotype (There and Back Again)!.Howard Hughes Program, Department of Biology, University of Puerto Rico at Cayey. Science Education Alliance. 2012. SEA-PHAGES Resource Guide. Howard Hughes Medical Institute. Chevy Chase, Maryland
Table1. Soil samples tested in order to verify the presence of mycobacteriophage population. Table includes sample information: date of sampling, coordinates, ambient temperature, depth, moisture content, area and proximity. Sample Date Coordinates Temperature (ºC) Depth (cm) Moisture content Area Proximity 1 AMDS Feb / 4 / 14 Lat. 18.119793 Long. - 66.15790 23.33 2.54 Moist Urban UPR Cayey Campus Tree Dead Leafs 2 KJC Feb / 4 / 14 Lat. 18.119506 Long. - 66.157878 23.33 4.4 Dry Urban UPR Cayey Campus Dead tree Trunk 3 AMDS Feb / 18 / 14 Lat. 18.11801 Long. - 66.13711 26.11 3.3 Dry Urban. Coca Navas Street Cayey, P.R. 00736 Palm leaf House Cement 4 KJC Feb / 18 / 14 Lat. 18.187409 Long. - 66.140466 19.44 2.54 Dry Rural Urb. Campo Lago, Cidra, P.R. 00739 Sewage 5 AMDS Feb / 23 / 14 Lat. 18.11797 Long. - 66.13706 27.78 5.3 Saturated Urban Coca Navas Street Cayey, P.R. 00736 Under plant Roots 6 KJC Feb / 23 / 14 Lat. 18.119251 Long. - 66.161560 27.22 2.5 Dry Urban UPR Cayey Campus Mango Tree 7 AMDS Feb / 24 / 14 Lat. 18.11524 Long. - 66.16313 25.7 2.0 Moist Urban Antonio R. Barceló Street Cayey, P.R. 00736 Underneath a decaying fruit Fruit – tree 8 KJC Feb / 24 / 14 Lat.18.115079 Long. - 66.155562 24.44 3.8 Moist Urban Los Veteranos Avenue, Cayey, P.R. 00739 Garbage Dump 9 AMDS March / 9 / 14 Lat. 18.11529 Long. - 66.14004 27.06 3.1 Dry Urban Ciaprian Ortiz Rodriguez Avenue Cayey, P.R. 00736 Underneath sheep excrement Tree
10 AMDS Mar / 9 / 14 Lat. 18.12745 Long. - 66.12056 26.2 5.2 Saturated Rural Vegas Cayey, P.R. 00736 Dairy Cows excrement Cows 11 KJC Mar / 9 / 14 Lat. 18.187424 Long. -66.140468 17.78 4.4 Saturated Urban Urb. Campo Lago, Cidra, P.R. 00739 Water Drainage 12 KJC Mar / 9 / 14 Lat. 18.187581 Long. -66.140479 25.56 3.1 7 Dry Urban Urb. Campo Lago, Cidra, P.R. 00739 Cement Drainage 13 AMDS Mar / 16 / 14 Lat. 18.11402 Long. -66.16907 28.33 2.5 Saturated José De Diego Avenue Cayey, P.R. 00736 Septic tank Plantain trees 14 AMDS Mar / 16 / 14 Lat. 18.11746 Long. -66.17972 28.61 2.6 Moist Rural “Buena Vista Sur” Cayey, P.R. 00736 Stagnant water Plants 15 AMDS Mar / 16 / 14 Lat. 18.1174 Long. -66.17993 28.33 2.3 Moist Rural “Buena Vista Sur” Cayey, P.R. 00736 Under a plantain tree 16 KJC Mar / 16 / 14 Lat. 18.187940 Long. -66.140350 23.33 3.0 4 Moist Rural Lake shore, Cidra, P.R. 00739 Plantain Crop 17 AMDS Mar / 20 / 14 Lat. 18.1179 Long. -66.137 26.11 1.5 Dry Urban. Coca Navas Street, Cayey 00736 Coffee plant Cement House *** 18 AMDS Mar / 20 / 14 Lat. 18.11524 Long. -66.16313 25.0 2.3 Moist Urban Antonio R. Barceló Avenue, Cayey, P.R. 00736 Underneath a decaying fruit Fruit – tree 19 KJC Mar / 20 / 14 Lat. 18.119730 Long. -66.157776 28.89 5.7 1 Dry Urban UPR Cayey Campus Under plant Roots 20 KJC Mar / 20 / 14 Lat. 18.119564 Long. -66.158065 28.33 5.0 1 Dry Urban UPR Cayey Campus Under Rotten Fruit
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FFR COPY

  • 1. Mycobacteriophage Isolation from Tropical Soil Sample: Serotinus Alejandra M. De Jesús-Soto1 , Kenny J. Colón-Colón2 1 Department of Mathematics, University of Puerto Rico at Cayey, Puerto Rico 2 Department of Biology, University of Puerto Rico at Cayey, Puerto Rico A B S T R A C T Mycobacteriophages are viruses that infect a specific type of bacteria. This abundant microorganism can be easily obtained from soil samples. Using Mycobacterium smegmatis as a host, a mycobacteriophage was isolated and purified from a soil sample. The goal is to obtain a pure phage population in order to analyze the information and then include it in the Mycobacteriophages Database. The first step was to collect a soil sample in order to make the enrichment and filtrate. Three plaque purifications followed this step in the process. A pure phage population was isolated from a tropical soil in Puerto Rico and named Serotinus. Future work includes performing the spot test, a process to identify the phage’s web pattern. Knowing the phages genetic information allows the identification of characteristics that may lead to important discoveries in modern medicine. Phages therapy seems to be an alternative medical treatment. 1. Introduction Mycobacteriophages are DNA viruses that infect a specific type of bacteria belonging to the mycobacteria genus. These are the most abundant type of microorganism in the biological universe. Mycobacteriophage infections may or may not lead to the death of the bacterium. This depends on its life style, which can be lytic or lysogenic. Lytic cycles results in the destruction of the infected bacteria and its membrane. It is used by temperate or virulent phages to achieve reproduction. The virulent phage infects bacteria with genetic material in order to undergo cell lysis. On the other hand, temperate phages undergo lysogenic cycle, in which the phage DNA first integrates into the bacterial chromosome to produce the prophage and make the host a lysogen. When the bacterium reproduces, the prophage is also copied. The prophage can be copied or activated, a process in which the prophage exits the chromosomal material to enter the lytic cycle. The findings of existent phage research have traversed many arenas of genetics and have even instigated the conception of new therapies and medical treatments (George 2013). A critical problem in heath arose due to the emergence of pathogen bacteria resistant to most currently available antimicrobial agents. The development of alternate anti-infection modalities is one of the highest priorities of modern medicine. Therefore, phage therapy seems to be a solution for this problem. Mycobacteriophages have been isolated from a variety of environments around the world. They can be easily obtained from soil samples. Using
  • 2. Mycobacterium smegmatis as a host, we sought to determine the presence of mycobacteriophages in a soil sample. Therefore, we hypothesized that we can isolate a mycobacteriophage population from a tropical soil sample in Puerto Rico. The objectives of this research are to isolate, purify, and harvest a novel phage population while the ultimate goal is to identify the characteristics of the phage that may serve modern medicine. 2. Materials and Methods Figure 1.Flow chart of the experimental procedure. Steps to isolate, purify and characterize a mycobacteriophage population from a soil sample. Each of the stages of the experiment was carried out by using the Sea-phages Resource Guide (2012) of the Science Education Alliance. There were some adjustments on procedures that had to be executed throughout the process to ensure the isolation and harvest of the bacteriophage. For this reason, alterations made during the procedure are included. Note that all materials used underwent a sterilization process, either by chemical methods using ethanol at 70% and Lysol® or by physical method using autoclave in aseptic technique during their use. It is recommended not to talk while doing any of the procedures to further avoid contamination.
  • 3. 2.1. Sample Collection Soil sample was collected from optional locations such as in wet places or where there was decomposition. After digging a few centimeters the collected samples were maintained in a sterile container. Data regarding localization coordinates, environmental temperature, excavation depth and moisture content was recorded. 2.2. Enrichment In a 50 mL conical tube, 0.500 g of the soil sample was mixed with Master Mix, substance that contained 8 mL of sterilized water, 1 mL of 10x 7H9/glycerol broth and 1 mL of AD supplement and 0.1 mL of CaCl (Science Education Alliance. 2012). Finally, 1 mL of Mycobacterium smegmatis was added and the solution was incubated at 37°C and aerated at 220 rpm for 16-24 hours (Science Education Alliance 2012). 2.3. Filtration After completion of the incubation period, solution was centrifuged at 3,000 rpm for 15-20 minutes. Afterwards, supernatant was filter-sterilized and poured into a 15mL conical tube. Both the pellet and the supernatant were stored. 2.3.1 Centrifuge Another option to obtain a purer sample from the enrichment protocol after centrifuging the conical tube of the enrichment protocol was to take 1 mL of the supernatant from the conical tube and transfer it to a microtube. The microtube was centrifuged at 10,000 rpm for 10 minutes. Then, 500 µL of the supernatant of the centrifuged microtube was transferred to another microtube to obtain the filtrate. 2.4 Plate Streaking A sterile utensil (wooden stick) was moistened with the filter-sterilized supernatant once. It was then used to gently swipe streaks on the Luria medium agar plate in quadrants. Figure 2 shows the correct way of streaking a plate. The segment labeled as (1) was first streaked, and then, another sterile swab was used to drag part of sample segment (1) to segment (2). The process of taking a sample from segment (2) and dragging it to segment (3) was repeated. Then, 4.5 mL of ~55.0o C Top Agar and 0.5 mL of the Mycobacterium smegmatis were poured into the plate from quadrant 3 to quadrant 1. The plate was closed by placing the cap on top. Finally, after agar solidification the plate was placed in an incubator at 37°C for ~24 hours (Science Education Alliance 2012). After this part of the procedure, the presence of mycobacteriophages in the collected sample was finally determined. 2.5. Plaque purification Figure 2. Streaking Technique. Available source: http://faculty.mc3.edu/jearl/ML/streak1.gif After confirming the presence of mycobacteriophages, the next step consisted in the extraction of an isolated plaque using the wooden tip of a sterile swab. Part of the
  • 4. plaque was transferred to a sterile microtube that contained 25 µL (microliters) of Phage Buffer (PB) which would help with the dilution and sustain the mycobacteriophages on the plaque. The plaque sample was streaked in a “smeg plate” (2.4 plate streaking protocol) and was left to rest from 16-24 hours until the next day. This plaque extraction procedure was progressively repeated with each plate until the third (3) plate was obtained. This was done to assure the pureness of a single type of phage from each plaque sample. The plaque purification samples of each three repetitions were placed in an environment temperature of 4°C (Science Education Alliance. 2012). 2.6 Phage-Titer Assay The third plaque purification sample went through another enrichment protocol (2.2). This was made for supplementing the purified mycobacteriophage. Eight (8) microtubes were labeled from 1 to 8. A volume of 90 µL (microliters) of PB was added to each microtube. In the microtube labeled (1), 10 µL (microliters) of the supernatant of the enrichment of the third plaque purification sample was added. Later, 10 µL (microliters) were extracted from microtube (1) to microtube (2). The same process was done going from the microtube (2) to microtube (3). This step was repeated successively until all 8 microtubes were diluted. 2.7 Empirical Test A smeg plate was prepared after labeling it and drawing eight (8) square divisions on the bottom of it with a number corresponding to the division on an edge for better plaque view. Before going to the important part of the empirical test, 4.5 mL of TA and 0.5 mL of Mycobacterium smegmatis were mixed and spread on top of the Luria medium Agar. Next, 10 µL of the sample of microtube (1) from the phage-titer dilutions was added to the square segment labeled with the same number. The process was repeated for each microtube sample on the corresponding numbered segment. The plate is then placed in an incubator at 37°C for 16-24 hours (Science Education Alliance 2012). 3. Results Twenty individual soil samples were collected and analyzed (Table 1). Positive results were obtained from sample #18 which was collected from an urban area in the city of Cayey. Location coordinates were: 18.11524 North, 66.137 West. The sample was collected 2.3 centimeters beneath the surface in an environment whose temperature skirted 25.0º Celsius. After collecting and enriching the sample, the presence of mycobacteriophages was confirmed. Then, after three plaques purifications, a phage with clear plaques was isolated (Figure 2). Currently, the process within this project is still in the MTPL, Medium Titter Phage Lysate. The next step was to perform a spot test in order to identify the mycobacteriophage’s web pattern and record results in the Mycobacteriophages Database. Figure 3. Clear plaques obtained after third purification.
  • 5. 4. Discussion This research on the collection and analysis of a soil sample for the isolation of a phage has been a worthwhile laboratory experience. Although the process was somewhat tedious and frustrating at the beginning due to all the negative results it was a learning experience that taught us patience, dedication and perseverance. Finally, after analyzing 20 samples, a mycobacteriophage was isolated and named Serotinus. After three purifications, the phage formed clear plaques on his host Mycobacterium Smegmatis, indicating that Serotinus is most likely a lytic phage. Future work would include completing the entire process of identifying and characterizing the phage in order to record and send the information to the Mycobactoriophages Database. The implications of isolating phages could lead to new and interesting developments in modern medicine. Currently, much research is being done related to phage therapy, and the study of novel phage populations could lead to promising discoveries. 5. Acknowledgments: This work was funded by the Howard Hughes Program and the RISE Program at the University of Puerto Rico at Cayey. The authors would like to thank Dr. Michael Rubin, Dr. Edwin Vazquez, Mr. Joseph Perez, Mr. Giovanni Cruz, Mr. Gustavo Martínez and Mr. Christopher Quintanal for their support during the entire process. 6. Literature Cited Alvarado EJ, Cruz-Arzón JA. 2013. Mycobacteriophage isolation from tropical soil sample: Mikriplithari and Ususindagari. Department of Mathematics- Physics, University of Puerto Rico at Cayey, Puerto RicoDepartment of Biology, University of Puerto Rico at Cayey, Puerto Rico. George MP. 2013. Mycobacteriophage Meru: Isolation and Characterization of a Novel Mycobacteriophage. [Internet]. [cited 2014 May 26], 5(10):1-3. Available from http://www.studentpulse.com/articles/770/m ycobacteriophage-meru-isolation-and- characterization-of-a-novel- mycobacteriophage Rubin M, Vázquez E. 2012. Mycobacteriophage Proteomics: From Genotype to Phenotype (There and Back Again)!.Howard Hughes Program, Department of Biology, University of Puerto Rico at Cayey. Science Education Alliance. 2012. SEA-PHAGES Resource Guide. Howard Hughes Medical Institute. Chevy Chase, Maryland
  • 6. Table1. Soil samples tested in order to verify the presence of mycobacteriophage population. Table includes sample information: date of sampling, coordinates, ambient temperature, depth, moisture content, area and proximity. Sample Date Coordinates Temperature (ºC) Depth (cm) Moisture content Area Proximity 1 AMDS Feb / 4 / 14 Lat. 18.119793 Long. - 66.15790 23.33 2.54 Moist Urban UPR Cayey Campus Tree Dead Leafs 2 KJC Feb / 4 / 14 Lat. 18.119506 Long. - 66.157878 23.33 4.4 Dry Urban UPR Cayey Campus Dead tree Trunk 3 AMDS Feb / 18 / 14 Lat. 18.11801 Long. - 66.13711 26.11 3.3 Dry Urban. Coca Navas Street Cayey, P.R. 00736 Palm leaf House Cement 4 KJC Feb / 18 / 14 Lat. 18.187409 Long. - 66.140466 19.44 2.54 Dry Rural Urb. Campo Lago, Cidra, P.R. 00739 Sewage 5 AMDS Feb / 23 / 14 Lat. 18.11797 Long. - 66.13706 27.78 5.3 Saturated Urban Coca Navas Street Cayey, P.R. 00736 Under plant Roots 6 KJC Feb / 23 / 14 Lat. 18.119251 Long. - 66.161560 27.22 2.5 Dry Urban UPR Cayey Campus Mango Tree 7 AMDS Feb / 24 / 14 Lat. 18.11524 Long. - 66.16313 25.7 2.0 Moist Urban Antonio R. Barceló Street Cayey, P.R. 00736 Underneath a decaying fruit Fruit – tree 8 KJC Feb / 24 / 14 Lat.18.115079 Long. - 66.155562 24.44 3.8 Moist Urban Los Veteranos Avenue, Cayey, P.R. 00739 Garbage Dump 9 AMDS March / 9 / 14 Lat. 18.11529 Long. - 66.14004 27.06 3.1 Dry Urban Ciaprian Ortiz Rodriguez Avenue Cayey, P.R. 00736 Underneath sheep excrement Tree
  • 7. 10 AMDS Mar / 9 / 14 Lat. 18.12745 Long. - 66.12056 26.2 5.2 Saturated Rural Vegas Cayey, P.R. 00736 Dairy Cows excrement Cows 11 KJC Mar / 9 / 14 Lat. 18.187424 Long. -66.140468 17.78 4.4 Saturated Urban Urb. Campo Lago, Cidra, P.R. 00739 Water Drainage 12 KJC Mar / 9 / 14 Lat. 18.187581 Long. -66.140479 25.56 3.1 7 Dry Urban Urb. Campo Lago, Cidra, P.R. 00739 Cement Drainage 13 AMDS Mar / 16 / 14 Lat. 18.11402 Long. -66.16907 28.33 2.5 Saturated José De Diego Avenue Cayey, P.R. 00736 Septic tank Plantain trees 14 AMDS Mar / 16 / 14 Lat. 18.11746 Long. -66.17972 28.61 2.6 Moist Rural “Buena Vista Sur” Cayey, P.R. 00736 Stagnant water Plants 15 AMDS Mar / 16 / 14 Lat. 18.1174 Long. -66.17993 28.33 2.3 Moist Rural “Buena Vista Sur” Cayey, P.R. 00736 Under a plantain tree 16 KJC Mar / 16 / 14 Lat. 18.187940 Long. -66.140350 23.33 3.0 4 Moist Rural Lake shore, Cidra, P.R. 00739 Plantain Crop 17 AMDS Mar / 20 / 14 Lat. 18.1179 Long. -66.137 26.11 1.5 Dry Urban. Coca Navas Street, Cayey 00736 Coffee plant Cement House *** 18 AMDS Mar / 20 / 14 Lat. 18.11524 Long. -66.16313 25.0 2.3 Moist Urban Antonio R. Barceló Avenue, Cayey, P.R. 00736 Underneath a decaying fruit Fruit – tree 19 KJC Mar / 20 / 14 Lat. 18.119730 Long. -66.157776 28.89 5.7 1 Dry Urban UPR Cayey Campus Under plant Roots 20 KJC Mar / 20 / 14 Lat. 18.119564 Long. -66.158065 28.33 5.0 1 Dry Urban UPR Cayey Campus Under Rotten Fruit