User:Giovanna F: Difference between revisions
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Purpose: the propose of this lab is to identify and study unicellular eukarya and see the | Purpose: the propose of this lab is to identify and study unicellular eukarya and see the differentiation of algae and Protist characteristics and examine them in my transect | ||
Material and Methods: I used | Material and Methods: I used and observed products that were in a drop of my Hay Infusion Culture. We used the dichotomous key to identify organisms. To further study the organisms in our | ||
transect we had to inoculate nutrient agar petri dishes to look at prokayotes. I | transect we had to inoculate nutrient agar petri dishes to look at prokayotes. I carefully brought the culture to my area without disturbing it and took samples from the microscopic observation. Then, | ||
1:100 dilution. I had eight labeled tubes of 10mLs sterile broth. I had a 100microliters filled micropipettor and added it to the sterile broth. Then I mixed the tube. We pipetted 100uL to | I made a 1:100 dilution. I had eight labeled tubes of 10mLs sterile broth. I had a 100microliters filled micropipettor and added it to the sterile broth. Then I mixed the tube. We pipetted 100uL to | ||
dilutions from the tubes. I then put it onto its corresponding plate. I had four agar petri dishes with tetracycline and four without it. We left the dishes at room temperature for the bacteria | plate serial dilutions from the tubes. I then put it onto its corresponding plate. I had four agar petri dishes with tetracycline and four without it. We left the dishes at room temperature for the bacteria | ||
to grow. | |||
culture. | Data and Observations: The culture was dark brown and carried a very rough strong stench. There was nothing growing in it, but by the smell we knew that there were several living organisms in our | ||
culture. We had two different niches in our culture: the top and the bottom. From our transect we collected clovers, leaves, grass, woodchips, soil, snow, fallen leaves, and rocks covered in organic | |||
materials. These are the materials that were on our Hay culture. On the Bottom of the Hay infusion I identified Paramicum Bursaria. It was 37mm long, motile, a protozoa, and it does not | |||
photosynthesize but instead, engulfs its nutrients. The second organism on the botttom I found was Gonium. It was flat, green, 500mm long, non-motile, and was an algae. One of the organisms at | |||
the bottom was | |||
a Spirostomum which was 25mm long, had a long narrow body similar to that of worms, and had no apparent flagella or cilia. I saw two organisms that we were not able to identify. The first had a | |||
round dark colored head and long tail like a tadpole. This organism was not seen eating or interacting with other organisms. The second identified organism was 110mm in length and was clear in | |||
color, with a large mouth that consumed water. It seemed to be swimming in only one direction. | |||
Conclusion: I thought that organisms might differ in their niches. The organisms on the top would be more photosynthetic because they need to absorb sunlight to make their nutrients ,while the | |||
organisms at the bottom would need to be more motile because they would need to chase and consume their nutrients. If the organism grew for another two months I would expect there to be more | |||
organisms because they would multiply but there would be a low carrying capacity for the growth because our culture is so small. | |||
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Hay Infusion Culture Observations: | Hay Infusion Culture Observations: | ||
-smelled really bad and there appeared to be a top layer of film on the surface of the water | -smelled really bad and there appeared to be a top layer of film on the surface of the water | ||
-the grass and leaves appeared to float while the soil sunk to the bottom | -the grass and leaves appeared to float while the soil sunk to the bottom | ||
/Users/MissGiovanna/Desktop/52fc352a59f0b41b9a971803c29382c1.jpg | /Users/MissGiovanna/Desktop/52fc352a59f0b41b9a971803c29382c1.jpg | ||
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Purpose: The purpose of the lab was to examine and be able to tell the distinct characteristics of different types of bacteria within our transect and to test which bacteria are antibiotic resistant to | Purpose: The purpose of the lab was to examine and be able to tell the distinct characteristics of different types of bacteria within our transect and to test which bacteria are antibiotic resistant to | ||
Tetracycline. | Tetracycline. | ||
Revision as of 20:00, 25 March 2015
Giovanna Franklin
Matthew Lefauve
Observing Transect 5 on AU's Campus
Purpose: The purpose of this lab is to understand the biodiversity and the abiotic and biotic factors that appeared in our ecosystem
Data and Observations:
The are that my group was responsible for was transect 5. Transect 5 is located on the main quad outside of the Hurst building. My transect was 20 x 20 meters and was on flat land. Due to the cold
weather, there was no vegetation on our transect but there were a bunch of little brown bushes, soil, grass and snow.
Biotic: clover, grass, bush type 1, bush type 2, fern
Abiotic: woodchips, soil, snow, rocks, leaves
/Users/MissGiovanna/Desktop/99d958ecd2c5eda6cfd84037d250156f.jpg
/Users/MissGiovanna/Desktop/unnamed.jpg
Coding:
Green: represents grass
Purple: represents snow
Material and Methods:
We used a sterile 50mL tube to collect samples of the vegetation from our transect to bring back and analyze in lab. Although there weren't many live flowers or leaves, we still collected them along
with grass, soil, and clovers to put aside and use in our Hay Infusion Cultures. The Hay Infusion Culture was the first method to analyzing some of the organisms and vegetation within our transect. In
order to perform this, we took 10-20 grams of the sample we collected and placed it in a jar with 500 mLs of deer park water along with .1gm of dried milk.
/Users/MissGiovanna/Desktop/b3e482939a2d475cda0725511978d27f.jpg
Conclusions: Although there weren't many organisms that appeared to be alive when we collected the sample, I am assuming that there are lots of little bugs and critters that will be visible after we
let the Hay Infusion sit for a week and when we use the microscopes to examine it more closely.
Identifying Algae and Protists-Lab 2
Purpose: the propose of this lab is to identify and study unicellular eukarya and see the differentiation of algae and Protist characteristics and examine them in my transect
Material and Methods: I used and observed products that were in a drop of my Hay Infusion Culture. We used the dichotomous key to identify organisms. To further study the organisms in our
transect we had to inoculate nutrient agar petri dishes to look at prokayotes. I carefully brought the culture to my area without disturbing it and took samples from the microscopic observation. Then,
I made a 1:100 dilution. I had eight labeled tubes of 10mLs sterile broth. I had a 100microliters filled micropipettor and added it to the sterile broth. Then I mixed the tube. We pipetted 100uL to
plate serial dilutions from the tubes. I then put it onto its corresponding plate. I had four agar petri dishes with tetracycline and four without it. We left the dishes at room temperature for the bacteria
to grow.
Data and Observations: The culture was dark brown and carried a very rough strong stench. There was nothing growing in it, but by the smell we knew that there were several living organisms in our
culture. We had two different niches in our culture: the top and the bottom. From our transect we collected clovers, leaves, grass, woodchips, soil, snow, fallen leaves, and rocks covered in organic
materials. These are the materials that were on our Hay culture. On the Bottom of the Hay infusion I identified Paramicum Bursaria. It was 37mm long, motile, a protozoa, and it does not
photosynthesize but instead, engulfs its nutrients. The second organism on the botttom I found was Gonium. It was flat, green, 500mm long, non-motile, and was an algae. One of the organisms at
the bottom was
a Spirostomum which was 25mm long, had a long narrow body similar to that of worms, and had no apparent flagella or cilia. I saw two organisms that we were not able to identify. The first had a
round dark colored head and long tail like a tadpole. This organism was not seen eating or interacting with other organisms. The second identified organism was 110mm in length and was clear in
color, with a large mouth that consumed water. It seemed to be swimming in only one direction.
Conclusion: I thought that organisms might differ in their niches. The organisms on the top would be more photosynthetic because they need to absorb sunlight to make their nutrients ,while the
organisms at the bottom would need to be more motile because they would need to chase and consume their nutrients. If the organism grew for another two months I would expect there to be more
organisms because they would multiply but there would be a low carrying capacity for the growth because our culture is so small.
Microbiology and Identifying Bacteria with DNA Sequences-Lab 3
Hay Infusion Culture Observations:
-smelled really bad and there appeared to be a top layer of film on the surface of the water
-the grass and leaves appeared to float while the soil sunk to the bottom
/Users/MissGiovanna/Desktop/52fc352a59f0b41b9a971803c29382c1.jpg
Purpose: The purpose of the lab was to examine and be able to tell the distinct characteristics of different types of bacteria within our transect and to test which bacteria are antibiotic resistant to
Tetracycline.
