3 antibiotic dicks | Distilled water | Culture of Serratia marcesans | Sterile filter-paper disks | Transparent tape | 1 sterile nutrient agar plate | Metric ruler | Forceps | 1 sterile cotton swab | Safety goggles | Lab apron | | Materials: Procedure: In the Antibiotic Resistant Bacteria lab‚ the effect of different antibiotics on the zone of inhibition on bacteria‚ Serratia marcesans‚ was measured in millimeters. The safety equipment‚ lab apron and goggles were worn at all times
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volume ratio. As the surface area of the Agar cube increases‚ the rate of conductivity will steadily increase‚ too. The trend line of the graph shows as an exponential graph because at one point there will be no more conductivity due to too small or too big Agar cubes. A difference can be seen in the average rate of conductivity depending on surface area because the Agar cubes with a larger total surface area are able to diffuse the ions faster. When the Agar cube has larger surface area‚ more area
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Some food in this world are made using microorganism to produce a desire flavour‚ taste and texture of the food. For examples: yogurt‚ tapai‚ cheese‚ bread and others. Starter cultures is used in these food production. A starter culture is a microbiological culture which actually perform fermentation. These starters usually consist of a cultivation medium‚ such as grains‚ seeds‚ or nutrient liquids that have been well colonized by the microorganisms used for the fermentation. These starters are formed
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designed Rainbow Agar O157 for the isolation and identification of EHEC. In this medium E. coli O157 was characterised by black colonies whereas O113 and some other EHEC strains were mauve‚ red or pink and indistinguishable from other strains of E. coli. Manafi and Kremsmaier (2001) evaluated the efficiency of different media for detecting Escherichia coli O157:H7. They found that SMAC agar had a sensitivity and specificity of 94.1 per cent and 91.6 per cent‚ Fluorocult HC agar
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correct‚ I carried out an experiment where I grew bacteria on 14 different agar plates and placed garlic on seven of the agar plates and then had no garlic present in the other seven agar plates. All 14 agar plates were kept under the same conditions while the bacteria colony was growing in order to ensure that all factors were kept constant. From the results‚ it was evidently clear that the size of the bacteria colony of the agar plates without garlic with an average of 115.29 mm² was much greater than
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causative bacteria or fungus. Potato dextrose agar is a good nutrient agar for mycelia to thrive on which is present in most fungal moulds.1 Standard nutrient agar is a general utility used for non-fastidious microorganisms.2 Aim The aim is to isolate fungi and bacteria colonies from diseased and healthy leaves. Materials and Methods Materials used for the experiment was two of each: standard nutrient agar plate and potato dextrose agar plate. To remove any epiphytic or saprophytic
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turn the agar plate over and divide the plate into four quadrants and label the agar plate whether you used the E. coli or B. megaterium and number the quadrants 1 through 4. Please keep in mind that one pair will test the E. coli and Environment 1 or 2‚ and one pair will test B. megaterium and Environment 1 or 2. After‚ you will need to swab the E. coli and B. megaterium on two different nutrient agar plates using a sterile disposable inoculating loop. Remember not to dig in into the agar or the
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INTRODUCTION Background Totipotency is the ability of a single cell to divide and produce all the differentiated cells in an organism‚ including extraembryonic tissues. Totipotent cells formed during sexual and asexual reproduction include spores and zygotes. Zygotes are the products of the fusion of two gametes. In some organisms‚ cells can dedifferentiate and regain totipotency. For example‚ a plant cutting or callus can be used to grow an entire plant. Human development begins when a sperm fertilizes
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Title: What is the effect of concentration of acid on the rate of diffusion in agar blocks? Aim: To investigate how the concentration affects the rate of diffusion of hydrochloric acid through agar blocks Research Question: To determine how will different concentrations (0.1M‚ 0.2M‚ 0.3M‚ 0.4M‚ 0.5M) of hydrochloric acid affect the rate of diffusion of sodium chloride through agar blocks? Introduction-include prediction; information you have researched before Diffusion refers to the passive movement
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source. Simmon’s citrate agar will be prepared by using Oxoid well-prepared Simmon’s citrate agar powder. The Simmon’s citrate agar was prepared by using Oxoid well-prepared Simmon’s citrate agar powder. The preparation was began by suspending 5.75g of the powder in 250 ml of distilled water and mixed thoroughly. The following shows the amount of each composition in 1 litre of Simmon’s citrate agar solution prepared using Simmon’s citrate agar powder. This Simmon’s citrate agar solution was then heated
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