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Manual cell counting

To count the cells manually you need to use a hemocytometer. A hemocytometer is a microscope slide that is specially designed to enable cell counting. The slide has a sink in its middle; the area of the sink is marked with a grid. A drop of a cell culture is placed in the sink. Looking at the sample under the microscope, the researcher uses the grid to manually count the number of cells in a certain area. The depth of the sink is predefined. Thus the volume of the counted culture can be calculated and with it the concentration of the cells.

The hemocytometer is a rectangled-shaped piece of glass which contains a small sink shaped as a square in the middle. The zoom of this sink is shown: it is divided in nine smaller squares where the four squares located in the corners are divided by sixteen even smaller squares. The other five squares are divided in smaller sections by multiple lines that cross the sink from side to side horizontally and vertically.

Figure 1: Manual hemocytometer, showing in detail the grid to count cells.

Use the following procedure:

  • Focus on the grid lines of the hemocytometer with a 10X objective.
  • Using a hand tally counter, count the cells in one set of 16 squares. When counting, employ a system whereby cells are only counted when they are set within a square or on the right-hand or bottom boundary line.
  • Move the hemocytometer to the next set of 16 corner squares and carry on counting until all four sets of 16 corners are counted.
  • Take the average cell count from each of the sets of 16 corner squares and multiply by 10,000 (104).
  • If you dilute the cells (using medium or trypan blue) you need to multiply by the dilution factor as well.
  • The final value is the number of viable cells/mL in the original cell suspension.

Referred from:

Article
Cell counting