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Intended Use
Gibco products for hybridoma culture have been designed and optimized for the serum-free growth of a variety of hybridoma cell lines and production of monoclonal antibodies.
Introduction
Traditional hybridoma culture media requiring serum supplementation have in recent years been replaced by a variety of commercially available serum-free formulations. Many serum-free formulations contain proteins (e.g., insulin, transferrin, albumin) and/or protein hydrolysates and lysates. As a result of a trend towards greater levels of media definition and the need for replacement of components of animal origin with non-animal derived materials, many serum free media formulations are considered unacceptable for certain applications. Hybridoma-SFM and PFHM II represent a spectrum of serum-free products for growth of hybridomas and monoclonal antibody production. Hybridoma-SFM is a serum-free, low protein (20 μg/mL protein as insulin and transferrin) medium that supports growth and monoclonal antibody production of a variety of hybridoma cell lines. PFHM II is a protein-free, chemically defined medium that is intended as a monoclonal antibody production medium, although it also has been used to grow a variety of hybridoma cell lines.
Features
PFHM II | Hybridoma-SFM | |
Protein-Free | X | |
Contains insulin and transferrin | X | |
Contains Phenol red | X | X |
Contains surfactant* | X | |
Contains inorganic iron carrier** | X |
Precautions
* PFHM II does not contain a surfactant. If used for agitated suspension culture, supplement with 0.1% PLURONIC F-68
** Medium should be pre-screened to determine potential interference of inorganic iron carrier(s) with antibody detection and/or purification method.
Hybridoma-SFM and PFHM II work well for a variety of hybridoma systems, but will not grow cholesterol dependen cell lines (e.g., NS0 and derivatives) without further supplementation. Supplementation with a lipoprotein preparation or other source of cholesterol will be required for cholesterol dependent cell lines. Addition of antibiotics should not be used as a substitute for proper sterile technique. In most instances, antibiotics are neither necessary nor advised. However, in those instances where antibiotics are desired, most general antibiotics are compatible with PFHM II including penicillin/streptomycin, gentamicin, anti-PPLO, lincocin and Fungizone. It is important not to use the following: kanamycin sulfates, neomycin sulfates or penicillin/streptomycin/neomycin mixtures
Physical Conditions
37° C + 0.5°C in a humidified atmosphere of 5 - 10% CO2 in air. Caps of flasks should be loosened to permit gas exchange. Cultures may be grown in stationary suspension culture (e.g., T-flask) or in agitated suspension culture (shaker or spinner flasks). Adequate headspace should be provided to facilitate gas exchange. (e.g., for a 125 mL shaker flask, use no more than 35 mL culture volume). Shaker flasks should be rotated at 125 - 135 rpm; agitation speed in spinner flasks will depend upon the impeller design. Protect cultures from light.
Adaptation of Cells to Serum-free or Protein-free Media
A sequential adaptation protocol may be necessary if direct adaptation does not work. In both cases, the cells should be in mid-logarithmic growth phase with high (>90%) viability. Success of the adaptation method will depend upon the particular hybridoma cell line and the culture conditions employed. It is recommended that backup cultures in the original medium be maintained until success with the new medium has been achieved.
A. Direct Adaptation
B. Sequential Adaptation
Cryopreservation
1 Note that conditioned medium should be obtained from a high viability, mid-log culture of cells.
Recovery from Cryopreservation
Quality Control
Gibco specialty media for hybridoma applications are performance tested using either a myeloma or hybridoma cell line. Additional standard evaluations are pH, osmolality and tests for the absence of bacterial and fungal contaminants.