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Bacteria Classification By Gram Staining Essay Research

Bacteria Classification By Gram Staining Essay, Research Paper


Bacteria Classification By Gram Staining


THE AMERICAN UNIVERSITY IN CAIRO


BIOLOGY DEPARTMENT


SCIENCE 453 : BIOLOGY FOR ENGINEERS REPORT No.1


Presented By : Karim A. Zaklama 92-1509 Sci. 453-01


24/2/96


Objective:


To test a sample of laboratory prepared bacteria and categorise it


according to Christian?s gram positive and gram negative classes and also by


viewing it under a high powered microscope and oil immersions; classify its


shape and note any special characteristics.


Introduction:


Bacteria was categorised into two groups in 1884 by the Danish


Bacteriologist Christian, gram positive and gram negative by a staining


technique where the ability to avoid de-coloration of Crystal Violet solution


by alcohol would render the category of gram positive, and gram negative if the


bacteria is de-coloured. This could be noted by the final colour of the


bacteria: a violet colour where Gram positive and a pink colour of the Safranin


added pending the de-colouring process.


Materials:


1. Bacteria Sample 2. Microscope Slide 3. Gram Staining Kit and Wash Bottles


a. Crystal Violet Solution b. Iodine Solution c. 95% Ethyl Alcohol d.


Safranin e. Distilled Water 4. Bibulous Blotting Paper 5. Microscope 6. Oil


Procedure:


A. Preparation :


1. Bacteria is cultivated on agar jelly in an incubator at 25?C for 24 hours. 2.


Obtain a microscope slide and with a toothpick, smear a thin coat of the


bacteria sample onto the slide 3. Cover the smear with a drop Crystal Violet


and leave standing for 20 seconds 4. Wash off the stain with distilled water;


drain and blot off the excess with bibulous paper. 5. Apply Gram?s Iodine on


the smear and leave to stand for 1 minute. 6. Drain the excess iodine and apply


95% Ethyl alcohol for 20 second duration or till the alcohol runs clearly from


the slide. 7. The smear should rinsed for a few seconds with distilled water to


stop the action of the alcohol. 8. Drain and blot off the excess with bibulous


9. Introduce Safranin to the smear and leave standing for 20 seconds. 10. Wash


off the stain with distilled water; drain and blot off the excess with bibulous


paper. 11. Leave the slide to air dry.


B. Examination:


1. Place the slide under microscope on low powered lens. 2. Move the slide


using the apparatus until the sample can be seen as a blur under the microscope.


3. F

ocus the lens to ensure that there is a sample directly under the lens. 4.


Move to higher powered lens, repeat step 3. 5. Move to higher powered lens,


repeat step 3 6. Move microscope aside and add Oil immersion, leave for a few


seconds and re-examine the slide.


Note Shape and colour and any other observations.


Results and Observations:


It was evident by visual examination that the alcohol was de-colouring or a


least partially de-colouring the bacteria.


The sample appeared a dark pink or close to violet by the naked eye; a


microscope was needed to ensure results.


Under the low powered microscope shades of pink were noted.


Under the medium power, the shades were more clear but no shape could be made


out.


Under the high powered microscope clumps of pink rod (bacilli) shaped bacteria


cells could be observed.


Under Oil Immersion and high powered lens the cells could seen more spaced out


and thus a clearer indication of the pink colour, bacilli shape and spores could


be made out in the individual cells.


Conclusion:


The Shape was noted as Bacilli (Rod-like) shaped cells; a gram variable


shape, distinct in either Gram Negative or Gram positive bacteria.


The final colour of the cells were stained pink by the Safranin showing


the de-coloration of the crystal violet proving the bacteria is of the gram


negative class.


Under oil immersion the cells became more sparse and under the high


powered lens of the microscope spores could be seen, as little bubbles, in the


cells. This tells us that the bacteria was in its terminal state.


The presence of spores in the bacteria at its terminal state tells us


that the bacteria could be an old culture. Old bacteria cultures which are gram


positive tend to de-colour, yet more slowly than gram negative bacteria. The


speed of de-coloration was not inspected very clearly thus no further conclusion


could be reached, yet it is possible that this an old culture of Bacilli shaped


Gram Positive bacteria.


Recommendation:


It is recommended that the same sample be tested again for de-


coloration; focusing on de-coloration speed. If the de-coloration is fast then


the sample is definitely gram negative, slow de-coloration would tell us it is


gram positive. For future samples it would be recommended to keep the bacteria


sample for this specific test for only 16 hours as recommended to avoid the


presence of old cultures which are anomalous to this test.

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