1. H. Reza Soleimanpour (PhD) Culture of Mammalian Cells �The Basic Considerations
2. Outline of the lecture� What is tissue culture?
Equipments
Aseptic technique
Cell culture nutrients and supplemets
Tips
3. What is tissue culture?� A means to study biological systems in vitro
Doesnt really mean microorganisms
Refers mainly to mammalian cells and tissues
Cell lines
Primary cells
4. Brief history of tissue culture� Late 19th century: Methods established for the cyropreservation of semen for selective breeding of livestock.
1907: Experiments published showing frog embryo nerve fibre growth in vitro.
1912: Connective tissue cells cultured for extended periods.
1948:First clone of cell line; L-cells (mouse).
1952:HeLa cells established from cervical carcinoma, the first human cell line.
1955:Defined media developed
1961 to present: Experiments using tissue culture methods expands exponentially.
Absolute necessity for biological experimentation.
5. Equipments� Tissue culture hood
CO2 incubator
Refrigerator or cold cabinet
Freezer
Centrifuge
Microscope
6. Biological Containment Cabinets� (Hood)� Class I
Class II, type A
Class II, type B1
Class II, type B2
Class II, type B3
Class III
7. Class I hood� Protects worker
No product protection
Inward airflow away from operator
Should have HEPA filter
Similar to a fume hood
8. Class II hood� Personal protection
Product protection
Environmental protection
Inward airflow
HEPA filtered supply and exhaust air
4 designs
Recirculates most of the air Type A
Exhausts most of the air Type B1
Provides total exhaust Type B2 Level 3 containment
Cabinet can be a combination Type B3, MOST COMMON
9. Class II hood� Used with low to moderate risk biological agents, i.e., Level 2 and 3 pathogens
HBV
HIV
Tuberculosis
Toxic chemicals and trace quantities of radionuclides
10. Class III hood� Totally enclosed
Gas-tight
Negative air pressure
Supply air is HEPA filtered
Exhaust air is double HEPA filtered
Can be used with Level 4 pathogens
Ebola
Hantavirus
11. The 10 commandments of working with Biological Safety Cabinet� Preparation turn on, check air pressure, allow air to purge workspace for at least 5 min.
Disinfection-spray or swab all interior with appropriate disinfectant 70% Ethanol.
Assemble material only material required, everything sterilized.
Purge-continue air purge for a few minutes before working.
Personal procedures-gloves, protective clothing (lab coat), etc.
12. The 10 commandments of working with Biological Safety Cabinet� Perform procedures-introduce hands into work area, try not to remove hands from work area until all or most procedures complete, remove gloves into designated contaminated material container.
Purge-allow air purge with no activity inside for a few minutes.
Personal procedures-wash hands.
Terminal disinfection-put on new gloves, remove tissue flasks to incubator, biohazard bag, etc. Spray or swab all interior surfaces with appropriate disinfectant; 70% ethanol.
Shutdown-turn off blower and fluorescent lamp. Turn on UV lamp if applicable.
13. Incubator Temperature
37 C
Gas phase
CO2 usually 5%
Maintains pH (7.2-7.4)
Calibrate regularly
Humidity
Water tray
14. Centrifuge Spin down cells
Bench top
Temperature controlled
Usually 15 and 50 ml tubes
Balance!!!
15. Microscope Inverted/Stereo
Phase contrast
Photo capabilities
Regular cell stains, cell counting (hemocytometer)
Fluorescent
Electron
16. Fridges and freezers Refrigerator for media storage, solutions
-20C Freezer for FBS, antibiotics
-80C Freezer for growth factors, labile reagents
Liquid Nitrogen for cell lines
17. Water bath Warming media
Thawing frozen cells
Enzyme reactions
37C
Clean regularly
Dry bath not as efficient
18. Aseptic Techniques�Protect Your Experiments Gloves!!!!!
Sterilized media and serum, i.e., FBS.
Autoclave capabilities
Sterilized materials, i.e., pipettes, tips
Appropriate Hood
Swab all surfaces with 70% ethanol before and after working!
Dont Touch Anything to fingers!!
Dont Touch Anything to openings of containers!!
Clean up spills immediately!!
Dont put tube or flask caps on to hood surface! at least not inner side
down!!
If you think you contaminated a pipette or tip or flask YOU DID!!! get another one before you contaminate everything.
Dont bake bread with viable yeast the night before working!!
19. Cell Culture Nutrients and Supplements Sterile media
Many different media for different cultures
RPMI, IMDM, McCoys, Eagles,etc.
Serum requirements
FBS, Horse serum, Human serum
Screen small aliquots of various lots
Antibiotics
Check special requirements
L-glutamine
beta-mercaptoethanol
Growth factors
20. Tips Hoods
Certify each year
Clean regularly
Incubators
Check CO2 levels regularly
Check humidity
Clean regularly
Aseptic Technique
Common sense
Cell Culture
Dont use antibiotics in stock cultures
Check cultures daily, look for clear supernatant.
Yellow color may mean the needs for passage or contamination.
Use microscope to check cultures.
Check all cell lines for mycoplasma contamination routinely.
Balance centrifuge.
If yeast found, CLEAN EVERYTHING immediately!
