Results and Calculations
Direct cell count via hemocytometer
Average cell count per square- 304/15= 20.26
Each square has a volume of 6.25 × 10-3µl =0.00625 µl
Therefore, the total number of bacterial cells per ml of liquid is =
= average cells/square X 1000 = 20.26 X 1000 = 3241600 = 3.2 × 106 cells/ml
0.00625 0.00625
Direct cell count via heterotropic cell count
Average colonies on plate- 34.5 colonies
Dilution factor- 105
Volume of sample plated- 1.0 ml
Total no. of CFU/ml of sample is =
= (average no. of colonies X total dilution factor)/ volume plated
= (34.5 X 105)/ 1.0
= 34.5 X 105 CFU/ml =3.45 X 106 CFU/ml
Plate count of coliforms
Average colonies of coliform on plate- 50
Average colonies of E. coli on plate- 101
Dilution factor- 103
Volume of sample plated- 0.1 ml
Total no. of CFU/ml of sample (E. coli) is =
= (average no. of colonies X total dilution factor)/ volume plated
= (101 X 103)/0.1
=10 X 105 CFU/ml
Total no. of CFU/ml of sample (coliform) is =
= (50 X 103)/0.1
= 5 X 105 CFU/ml
Total no. of CFU/ml of sample (all coliform) is =
= (151 X 103)/0.1
= 15 X 105 CFU/ml
Most Probable number (MPN)
Thermotolerant coliform – 93 X 105
Discussion questions
Answer 1
Thus, it can be interpreted that the viable cell count method is more suitable for checking the water quality in Alice’s laboratory. It has been revealed from Canadian Drinking Water Quality Guidelines that no MAC is specific for HPC bacteria in water supplied by semi public, public and private drinking water system (Sen & Ashbolt, 2011). Increase in HPC concentrations more than baseline levels are undesirable conditions. The ideal HPC count is less than 10 CFU/ml. However, the count in Alice’s laboratory water is significantly higher than the ideal level.
Criteria for indicator organism
There is zero tolerance for faecal coliforms in treated drinking water and presence of these organisms above the level makes the water unacceptable for drinking. Thus, water industry uses these organisms as an indicator of health risk and use for monitoring the safety level of drinking water (Gunnarsdottir et al., 2012).
The thermotolerant coliform, i.e. E. coli is a better indicator of faecal contamination. Indicator value Escherichia coli is considered the most suitable index of faecal contamination (Hammes et al., 2012). As these organisms are more heat tolerant, thus are more resistant to the harsh environment, which indicates that their presence in water is more dangerous compared to the other coliforms, which can grow at 35 ºC -37 ºC.
In both of the colony counting methods, the coliform and thermotolerant coliform count have been done. However, comparison is justified, as it is helping in identifying the level of health risk upon consuming the contaminated water sample. Coliforms are the bacteria, which may harmful to the human body; however, the thermotolerat conliforms are more harmful as they can survive at high temperature, which enhances the chance of this organism to contaminate treated water in water treatment plant.
Thus, it is appropriate to compare the coliform and thermotolerant coliform count via two different methods. In layman’s terms, the experiments are done for comparing between apples to apple, not apple to orange (Payment & Locas, 2011). This is because, the characteristics of both the organisms are similar except some key difference including the ability of thermocoliform bacteria to ferment lactose and produce carbon dioxide within 48 hours at high temperature; tthereby indicating the importance of counting two different cell counts for these two sub categories of indicator organism.
For Alice’s future plan of water treatment, the quality of water needs to be assured, which can be done through various procedures including sampling, filtration, culturing and incubation. Filtration is a key step for maximizing recovery of microorganisms while avoiding exogenous contamination, which is performed by passing a known volume of water through a sterile membrane filter with a pore size small enough to retain bacterial cells, which is then transferred to an agar plate and allowed to develop into colonies.
Culture media includes the use of selective bacteria for detecting indicator organism, which have been earlier. In addition, the rapid methods can also be implemented; which include quantitative population. Biofilm is another potential process for testing the quality of water sample being tested in the laboratory. Biofilms are now recognised as complex microbial communities, forming on surfaces (Odonkor & Ampofo, 2013).
It has been revealed that most of the bacteria in drinking water distribution systems are present within biofilms rather than free living in the water itself. Salmonella Typhimurium, Campylobacter, Pseudomonas aeruginosa and Aeromonas hydrophila are the organisms identified from biofilms, which are potentially pathogens for human. High heterotropic plate count is suitable to identify the pool of microbial population in biofilms, thus it is a suitable method for testing water sample. Finally, the IMViC test is a significant microbial testing for testing the quality of water in laboratory.
It is a series of tests for identifying and confirming the presence of coliform group of bacteria in water. These include indole test, methyl red test, voges proskauer test and citrate test. In the first two tests, the faecal coliform like E. coli gives positive responses, whereas in last two tests, nonfaecal coliforms like Enterococcus gives positive results (Sen & Ashbolt, 2011). FLowcytometer is an advanced method for testing the quality of water also, which Alice can also use.
Reference List
Bain, R., Bartram, J., Elliott, M., Matthews, R., McMahan, L., Tung, R., … & Gundry, S. (2012). A summary catalogue of microbial drinking water tests for low and medium resource settings. International journal of environmental research and public health, 9(5), 1609-1625.
Bauman, R. W., Machunis-Masuoka, E., & Cosby, C. D. (2012). Microbiology: With diseases by body system. Benjamin Cummings.
Da Silva, N., Taniwaki, M. H., Junqueira, V. C. A., Silveira, N., & GOMES, R. A. R. (2013). Microbiological Examination Methods of Food and Water. CRC Press.
Gunnarsdottir, M. J., Gardarsson, S. M., Elliott, M., Sigmundsdottir, G., & Bartram, J. (2012). Benefits of water safety plans: microbiology, compliance, and public health. Environmental Science & Technology, 46(14), 7782-7789.
Hammes, F., Broger, T., Weilenmann, H. U., Vital, M., Helbing, J., Bosshart, U., … & Sonnleitner, B. (2012). Development and laboratory?scale testing of a fully automated online flow cytometer for drinking water analysis. Cytometry Part A, 81(6), 508-516.
McFeters, G. A. (Ed.). (2013). Drinking water microbiology: progress and recent developments. Springer Science & Business Media.
Odonkor, S. T., & Ampofo, J. K. (2013). Escherichia coli as an indicator of bacteriological quality of water: an overview. Microbiology research, 4(1).
Payment, P., & Locas, A. (2011). Pathogens in water: value and limits of correlation with microbial indicators. Ground Water, 49(1), 4-11.
Sen, K., & Ashbolt, N. J. (2011). Environmental microbiology: current technology and water applications. Horizon Scientific Press.
Yates, M. V., Nakatsu, C. H., Miller, R. V., & Pillai, S. D. (2016). Manual of environmental microbiology (No. Ed. 4). American Society for Microbiology (ASM).
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