Standard Plate Count Method: By: Hafiza Asfa Shafique Microbiology BS Biotechnology V
Standard Plate Count Method: By: Hafiza Asfa Shafique Microbiology BS Biotechnology V
Standard Plate Count Method: By: Hafiza Asfa Shafique Microbiology BS Biotechnology V
method
• Definition: Viable Plate Count (also called a Standard Plate Count) is one of
the most common methods, for enumeration of bacteria.
• Enumeration of microorganisms is especially important in dairy
microbiology, food microbiology, and water microbiology.
• Knowing the bacterial count in drinking water, fresh milk, buttermilk,
yogurt, can be useful in many aspects of industrial microbiology.
• Bacteria are so small and numerous, counting them directly can be very
difficult. Some of the methods used involve diluting the sample to a point
at which the number of bacteria has been reduced to very small numbers.
VIABLE (STANDARD) PLATE COUNT
• The number of bacteria in a given sample is usually too great to be counted directly.
• The viable plate count method is an indirect measurement of cell density and
reveals information related only to live bacteria.
• However, if the sample is serially diluted and then plated out on an agar surface in
such a manner that single isolated bacteria form visible isolated colonies, the
number of colonies can be used as a measure of the number of viable (living) cells in
that known dilution.
• Normally, the bacterial sample is diluted by factors of 10 and plated on agar. After
incubation, the number of colonies on a dilution plate showing between 30 and 300
colonies is determined.
• A plate having 30-300 colonies is chosen because this range is considered statistically
significant.
Principle
• Serial dilutions of bacteria are plated onto an agar plate. Dilution procedure
influences overall counting process. The suspension is spread over the
surface of growth medium. The plates are incubated so that colonies are
formed. Multiplication of a bacterium on solid media results in the
formation of a macroscopic colony visible to naked eye.
• It is assumed that each colony arises from an individual viable cell. Total
number of colonies is counted and this number multiplied by the dilution
factor to find out concentration of cells in the original sample. Counting
plates should have 30-300 colonies at least. Since the enumeration of
microorganisms involves the use of extremely small dilutions and extremely
large numbers of cells, scientific notation is routinely used in calculations.
CFUs per milliliter (CFUs/ml)
• Generally, to determine the number of (colony forming units) CFUs per milliliter
(ml) of sample.
• To find this, the number of colonies (on a plate having 30-300 colonies) is
multiplied by the number of times the original ml of bacteria was diluted (the
dilution factor of the plate counted).
• For example, if a plate containing a 1/1,000,000 dilution of the original ml of
sample shows 150 colonies, then 150 represents 1/1,000,000 the number of CFUs
present in the original ml.
• Therefore the number of CFUs per ml in the original sample is found by
multiplying 150 x 1,000,000 as shown in the formula below:
• CFUs per ml of sample = The number of colonies counted X The dilution factor
of the plate counted
CFUs per milliliter (CFUs/ml)
• At the end of the incubation
period, select all of the agar
plates containing between 30
and 300 colonies.
• Plates with more than 300
colonies cannot be counted and
are designated "too numerous to
count" (TNTC).
• Plates with fewer than 30
colonies are designated "too few
to count" (TFTC).
PROCEDURE VIABLE PLATE COUNT
• Suppose, we will be testing two samples of water for the Viable
Count.
• The samples include:
1) water from a drinking fountain
2) boiled water from a drinking fountain
• You will need DATA TABLE 1 to input your data and calculate the
number of CFU per ml.
PROCEDURE VIABLE PLATE COUNT
1) Take 6 dilution tubes, each containing 9 ml of sterile saline water.
2) Dilute 1 ml of a sample by withdrawing 1 ml of the sample and
dispensing this 1 ml into the first dilution tube.
3) Using the same procedure, withdraw 1 ml from the first dilution
tube and dispense into the second dilution tube. Subsequently
withdraw 1 ml from the second dilution tube and dispense into the
third dilution tube. Continue doing this from tube to tube until the
dilution is completed.
9ml saline
4) Transfer 1 ml from each of only the last three dilution tubes onto the
surface of the corresponding agar plates.
5) Incubate the agar plates at 37°C for 48 hours. 6) Choose a plate that
appears to have between 30 and 300 colonies.
6) Choose a plate that appears to have between 30 and 300 colonies.
7) Count the exact number of colonies on that plate
8) Calculate the number of CFUs per ml of original sample as follows:
CFUs per ml of sample = The number of colonies X The dilution factor of the
plate counted
Overall procedure
Limitation
• A major limitation in this method is selectivity. The nature of the
growth medium and the incubation conditions determine which
bacteria can grow and thus be counted.
• Viable counting measures only those cells that are capable of growth
on the given medium under the set of conditions used for incubation.
• Sometimes cells are viable but non-culturable.