Core practical - effect of antiseptics, antibiotics or plant extracts on microbial cultures The effectiveness of antibiotics Flashcards

1
Q

Method A - Preparing the agar plates of a colony of bacteria (6)

A

1- Glass Petri dishes and agar gel must be sterilised in an autoclave before use or pre-sterilised plastic Petri dishes can be bought.
2- Pour the sterile agar plates and allow to fully set.
3- Use a sterile pipette to add a few drops of the microorganism solution to the agar. Close the lid of the agar plate and place the pipette in disinfectant.
4- Unwrap a sterile spreader or sterilise a spreader in ethanol. Use the spreader to spread the microorganism solution, across the entire surface of the agar plate.
5- Label and invert the plate, and store upside down.
6- Incubate at a maximum temperature of 25°C in schools and colleges.

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2
Q

why must Glass Petri dishes and agar gel be sterilised?

A

this will kill any bacteria that are present in the solution or on the Petri dishes.

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3
Q

why do you need to Pour the sterile agar plates and allow to fully set.?

A

this provides the selected bacterium with all the nutrients needed to grow.

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4
Q

why do you need to ‘Use a sterile pipette to add a few drops of the microorganism solution to the agar. Close the lid of the agar plate and place the pipette in disinfectant.’?

A

this solution contains the bacteria that will grow on the agar.

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5
Q

why do you need to ‘Unwrap a sterile spreader or sterilise a spreader in ethanol. Use the spreader to spread the microorganism solution, across the entire surface of the agar plate.’?

A

this allows a lawn of bacteria to be produced across the whole of the plate. Replace the lid as soon as possible, secure with tape.

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6
Q

why do you need to ‘Label and invert the plate, and store upside down.’? (3)

A

-this stops additional unwanted bacteria in the air contaminating the plate.
-Do not fully seal the lid, as this will stop oxygen reaching the bacterium, and this may encourage harmful anaerobic bacteria to grow.
-Labels are important, as this identifies the growing bacterium.

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7
Q

why do you need to ‘Incubate at a maximum temperature of 25°C in schools and colleges’? (2)

A

-this reduces the chance of growing harmful pathogens.
-Hospital laboratories would incubate plates at 37°C (body temperature) to allow quick growth and identification.

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8
Q

what indicates that the bacteria have been killed?

A

A clear area (zone of inhibition)

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9
Q

Method B - Adding antibiotic or antiseptic soaked patches to pre-prepared agar plates + REASONS (4)

A

1- Soak filter paper disks in a variety of solutions, use either different concentrations of the same solution, or a variety of different solutions.
REASON: the effectiveness of the solutions at killing the bacteria can be tested.
2- Measure the clear area around the soaked filter paper disks. A control disk must be also included.
REASON: size of zone indicates the effect of the substance tested on the growth of the specific bacterium.

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10
Q

how could we calculate the effect of antibiotics or antiseptics on bacterial growth?

A

use ‘pie r squared’ to calculate the area of the clear zone

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