23 Mar 2015 02 May 2017
Total and viable counts of microorganisms
There are several methods for determining total and viable counts of microorganisms
Total Cell counting is used
Viable counting are used
Details of uses of cell counting, including their advantages and disadvantages.
There are several methods for determining total and viable counts of microorganisms
Include other methods and include references to your source
Brief detail of your actual experiment, mentioning the organism and which techniques will be used
Total Viable Count - This involves counting the colonies produced by viable cells under favourable growth conditions. In pour-plate method, an aliquot of suitably diluted sample is mixed with nutrient agar at a temperature where it is liquid. Then the mixture is poured into petridishes and allowed to set.
Alternatively an aliquot of the sample is spread over the agar surface of a Petridis using a sterile spreader. Membrane filters can also be used to determine the bacterial numbers. In this method cells are filtered onto membrane filter which is then placed over nutrient agar surface.
Total Cell Count - The most common method of enumerating the total microbial cells is the direct counting of cell suspension in a counting chamber of known volume using a microscope. One such counting chamber is Neubauer counting chamber. Another method involves an electronic instrument, Coulter counter.
http://www.microbiologyprocedure.com/aquatic-environment-microbiology/total-cell-count.htm
http://www.mansfield.ohio-state.edu/~sabedon//biol4038.htm
http://www.rapidmicrobiology.com/test-methods/Total-Viable-Count.php
http://www.biochemj.org/bj/021/0104/0210104.pdf
Explain the procedure where cells crosses gridlines of the haemocytometer
In this discussion you should discuss the errors associated with measurement of viability. Discuss ways of improving the experiment and whether this could be achieved with the material provided
The experiment could be improved by:
The main source of error occurred during experiment was leaving the agar plate lid open to transfer the dilutions for a long time which could of contaminated the agar plate by air.
(Madigan, 2009)
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