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The following protocols describe general procedures for subculturing mammalian cells in suspension culture. Note that the procedure for passaging insect cells differs from that for mammalian cells on several crucial steps. For more information, refer to Notes on Subculturing Insect Cells.
For passaging your own cell line, we recommend that you closely follow the instructions provided with each product you are using in your experiments. The consequences of deviating from the culture conditions required for a particular cell type can range from the expression of aberrant phenotypes to a complete failure of the cell culture.
Passaging Suspension Cultures
Subculturing suspension cells is somewhat less complicated than passaging adherent cells. Because the cells are already suspended in growth medium, there is no need to treat them enzymatically to detach them from the surface of the culture vessel, and the whole process is faster and less traumatic for the cells. Replacement of growth medium is not carried out in suspension cultures; instead, the cells are maintained by feeding them every 2 to 3 days until they reach confluency. This can be done by directly diluting the cells in the culture flask and continue expanding them, or by withdrawing a portion of the cells from the culture flask and diluting the remaining cells down to a seeding density appropriate for the cell line. Usually, the lag period following the passaging is shorter than that observed with adherent cultures.
Suspension Culture Vessels
Suspension cultures can be maintained in sterile culture flasks (e.g., shaker flasks without baffles) that are not tissue-culture treated; however, spinner flasks (i.e., stirrer bottles) specifically designed for suspension cell culture allow for superior gas exchange and permit higher volumes of cells to be cultured.
Spinner flasks have two basic designs; the medium is agitated (i.e., stirred) by a hanging stir-bar assembly or with a vertical impeller. The vertical impeller provides better aeration. The total culture volume in a spinner flask should not exceed half of the indicated volume of the spinner for proper aeration (e.g., a 500 mL spinner should never contain more than 250 mL of culture).
This video explains why, when and how to passage cells grown in both adherent and suspension cultures. This includes cell dissociation, counting cells, determining optimal seeding density and preparing new culture vessels for passaged cells.
All solutions and equipment that come in contact with the cells must be sterile.
Always use proper sterile technique and work in a laminar flow hood. Subculture cells when they are in log-phase growth before they reach confluency. When they reach confluency, cells in suspension clump together and the medium appears turbid when the culture flask is swirled. The maximum recommended cell density before passaging varies with cell lines; refer to the cell-specific product insert or manual for details.
Cells Grown in Shaker Flasks
The following protocol describes a general procedure for passaging mammalian cells grown in suspension culture using shaker flasks in a shaking incubator. For detailed protocols, always refer to the cell-specific product insert.
Note: Make sure that the shaker flask does not have baffles (i.e., the indents at the bottom of the flask designed to provide agitation), because they ruin the shaking rhythm.
Note: To minimize the accumulation of cell debris and metabolic waste by-products in shaker cultures, gently centrifuge the cell suspension at 100 × g for 5 to 10 minutes, and resuspend the cell pellet in fresh growth medium once every three weeks (or as needed).
Cells Grown in Spinner Flasks
The following protocol describes a general procedure for passaging mammalian cells in suspension grown using spinner flasks. For detailed protocols, always refer to the cell specific product insert.
Note that cells are sensitive to physical shearing. Ensure that impeller mechanisms rotate freely and do not contact vessel walls or the base. The top of the paddles should be slightly above the medium to ensure adequate aeration to the culture. Adjust the spinner mechanism so that paddles clear the sides and the bottom of the vessel. The table below lists the minimum volumes of media needed for different spinner flask sizes. |
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We do not recommend initiating a spinner culture into a spinner flask larger than 500 mL. We suggest scaling up from smaller spinners that have already been established.
Note: To minimize the accumulation of cell debris and metabolic waste by-products in spinner cultures, gently centrifuge the cell suspension at 100 × g for 5 to 10 minutes, and resuspend the cell pellet in fresh growth medium once every three weeks (or as needed).
While the general procedure for subculturing insect cells follows the same steps as mammalian cells, some key requirements of these culture systems are different. For best results, always follow the instructions provided with the insect cell lines you are using in your experiments.
Note: Sf-900 II SFM and Gibco Express Five SFM already contain surfactants.
For Research Use Only. Not for use in diagnostic procedures.
For Research Use Only. Not for use in diagnostic procedures.