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Fig. 3.2 Laminar flow cabinet (class II)
Biosafety Levels ,[object Object],[object Object]
Biosafety levels contd. ,[object Object],[object Object]
Fig. 3.6 Tissue culture flasks (T-flasks)
Fig. 3.7 Multi-well plates
Fig. 3.10 Spinner bottle with suspended paddle
Fig. 3.11a Roller bottles of various sizes
Bottles in a roller system  Fig. 3.11b
Fig. 10.17 A confluent layer of BHK cells covers two microcarriers
Cell yield on microcarriers with varying charge
Non-porous microcarriers ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
Porous microcarriers ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],Amersham Biosciences
Fig. 10.18 Comparison of a unit system and a multiple system
Cell encapsulation Fig. 10.19
Typical  c ulture vessels suitable for cell growth Culture vessel Number of culture wells/ unit Max. culture volume (ml) Vessel size Growth surface (cm 2 ) Material Multiple well plate 96 0.37 10.8 x 6.4 mm (D x diam.) 0.32 plastic "  "  24 3.4 17.6 x 15.5 mm  " 1.88 plastic "  " 12 6.9 17.6 x 22.1 mm  " 3.8 plastic "  " 6 16.8 17.6 x 34.6 mm  " 9.4 plastic Medical flat bottle 10 125 ml 22 glass "  "  " 15 250 ml 30 glass Roux bottle 50 500 ml 200 glass T-flask, 25 5.0 50 ml 25 plastic "  , 75 15-30 250 ml 75 plastic "  , 150 75 600 ml 150 plastic "  , 175 50-100 750 ml 175 plastic
Typical  c ulture vessels suitable for cell growth continued Culture vessel 100-200 1250 ml 490 plastic Culture vessel 100-250 2200 ml 850 plastic Culture vessel 100-500 4900 ml 1750 plastic Culture vessel 100 250 ml glass Culture vessel 250 500 ml glass Culture vessel Number of culture wells/ unit Max. culture volume (ml) Vessel size Growth surface (cm 2 ) Material
Fig. 3.12a Inverted microscope
Fig. 3.12b Standard microscope
Lecture 4  Animal Cell Biotechnology Cell Culture Conditions and Media ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
Double chamber CO 2  incubator  Fig. 3.3
Butler, M.  2004.  Animal cell culture and technology 2nd ed. London and New York:Garland Science/BIOS Scientific Publishers. P 34.
[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]

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Lecture 4a culture equipment

  • 1. Fig. 3.2 Laminar flow cabinet (class II)
  • 2.
  • 3.
  • 4. Fig. 3.6 Tissue culture flasks (T-flasks)
  • 6. Fig. 3.10 Spinner bottle with suspended paddle
  • 7. Fig. 3.11a Roller bottles of various sizes
  • 8. Bottles in a roller system Fig. 3.11b
  • 9. Fig. 10.17 A confluent layer of BHK cells covers two microcarriers
  • 10. Cell yield on microcarriers with varying charge
  • 11.
  • 12.
  • 13. Fig. 10.18 Comparison of a unit system and a multiple system
  • 15. Typical c ulture vessels suitable for cell growth Culture vessel Number of culture wells/ unit Max. culture volume (ml) Vessel size Growth surface (cm 2 ) Material Multiple well plate 96 0.37 10.8 x 6.4 mm (D x diam.) 0.32 plastic " " 24 3.4 17.6 x 15.5 mm " 1.88 plastic " " 12 6.9 17.6 x 22.1 mm " 3.8 plastic " " 6 16.8 17.6 x 34.6 mm " 9.4 plastic Medical flat bottle 10 125 ml 22 glass " " " 15 250 ml 30 glass Roux bottle 50 500 ml 200 glass T-flask, 25 5.0 50 ml 25 plastic " , 75 15-30 250 ml 75 plastic " , 150 75 600 ml 150 plastic " , 175 50-100 750 ml 175 plastic
  • 16. Typical c ulture vessels suitable for cell growth continued Culture vessel 100-200 1250 ml 490 plastic Culture vessel 100-250 2200 ml 850 plastic Culture vessel 100-500 4900 ml 1750 plastic Culture vessel 100 250 ml glass Culture vessel 250 500 ml glass Culture vessel Number of culture wells/ unit Max. culture volume (ml) Vessel size Growth surface (cm 2 ) Material
  • 17. Fig. 3.12a Inverted microscope
  • 18. Fig. 3.12b Standard microscope
  • 19.
  • 20. Double chamber CO 2 incubator Fig. 3.3
  • 21. Butler, M. 2004. Animal cell culture and technology 2nd ed. London and New York:Garland Science/BIOS Scientific Publishers. P 34.
  • 22.

Hinweis der Redaktion

  1. Recirculates air through HEPA filters (High efficiency particulate air) Filter – series of glass fibres – particles in the air will be removed. remove 0.3 microns sterile environment – and air circulates – protects the operator Allows sterile manipulation and also protects the environment and operator Useful for Level 2 containment (Laboratory)
  2. Level 1. Examples: Bacillus subtilis , canine hepatitis , Escherichia coli , varicella ( chicken pox ), as well as some cell cultures and non-infectious bacteria. Level 2: or are difficult to contract via aerosol in a lab setting, such as hepatitis A , B , and C , influenza A , Lyme disease , salmonella , mumps , measles , HIV [3] , scrapie . Level 2 – primate cells Level 1 non-primate cells Level 3 – generally they are disease causing viruses (antharax, west nile virus, yellow fever, small pox) Sealed Cabinet and air locked storages.
  3. Level 3 : Includes various bacteria and viruses that can cause severe to fatal disease in humans, but for which vaccines or other treatment exist, such as anthrax , West Nile virus , Venezuelan equine encephalitis , Eastern Equine Encephalitis , SARS , smallpox , tuberculosis , typhus , Rift Valley fever , Rocky Mountain spotted fever , yellow fever . All procedures involving the manipulation of infectious materials are conducted within biological safety cabinets or other physical containment devices, or by personnel wearing appropriate personal protective clothing and equipment. Level 4: such as Bolivian and Argentine hemorrhagic fevers , dengue fever , Marburg virus , Ebola virus , hantaviruses , Lassa fever , Crimean-Congo hemorrhagic fever , and other various hemorrhagic diseases. When dealing with biological hazards at this level the use of a Hazmat suit and a self-contained oxygen supply is mandatory. The entrance and exit of a Level Four biolab will contain multiple showers, a vacuum room, an ultraviolet light room, designed to destroy all traces of the biohazard.
  4. Most labs use disposable flasks Generally sulfonated plastic – so that cells can grow in the inner surface containers are gamma radiated and sterile inside. loosen caps to allow gas exchanege Some manufacturers have covers that have holes that has a plastic inside to cover (no leaks) to allow gas exchange T-25, T-75, T-120 = numbers are square centimetres – surface area for cells to grow
  5. Could use a lot of replicate cultures Come in various sizes
  6. Autoclave sterilization Glass, screw cap on top that holds a column that contains a magnetic stir bar and teflon paddle stirs media Other arms can be used for sampling or probes depending on the size of bottle Max = 10 L Limitation is for 10L – power of stirring – efficiency of stirring is compromised. Stirred tank bioreactor (STB / STR) over 10 L – require a motor for stirring
  7. T 25 – surface area of 25 square cm, original were made out of glass 3 standard sizes (490, 850, 1750) Square centimetre required for anchorage dependent growth Bought as sterile units and are only meant for single use
  8. 5-60 rev /h Inner surface is constantly in contact with media ^ Simple lab setup, there are also machines that can hold 30 000 roller bottles
  9. BHA cells growing on the microcarriers (150 microns in diameter) about 250 cells on the surface of microcarrier Increase surface area = Suspend microcarriers in the stirred tank Each microcarrier needs to have clonal population on it Unit scale up: increase the volume in each flask – value: labour intensity is less i.e. Initial 1 L roller flask to an upgrade of 10 L bioreactor Multiple scale up: increase the number of rollers flasks – value: labour intensifies i.e. initial 4 roller flasks to an upgrade of 20 or more roller flasks
  10. Exchange capacity – miliequivalents/g – measure of the charge on the microcarrier Productivity = cell growth Very narrow window of charge where cells have high growth potential.
  11. Matrix in cytodex is dextran – polymer of glucose Cells only grow on the surface of the microcarrier Cytodex 1 is the most widely used Cytodex 3 has a good advantage – collagen – primary cells may require an attachment surface
  12. - Cytopore – dextra nmesh – larger pores – cells buries inside
  13. - Sodium alginate – liquid at room temperature mix with cells – drop a droplet in CaCl2 solution and bead hardens – cells therefore grows within the bead
  14. -Inverted microscope – stage is fairly wide – can fit a t flask on a stage and can be maginified through the microscope - Inverted – light source in on top
  15. - Stage is fairly narrow and cannot fit a t flask
  16. Bicarb-CO 2 system operates in blood in vivo. Balance between CO 2 from atmosphere and bicarbonate in the media. pKa of 6.3 is adequate, but not ideal. Buffering system +/- pKa value Relatively cheap system Concentration of CO 2 is important: if the concentration is too low, the pH increases. If the concentration is too high you get a drop in pH. Concentration of the CO 2 in the incubator ranges from 5 – 10%, supplied by a CO 2 cylinder, depends on the concentration of bicarbo in the media. Consequences of cells growing at a higher temperature is greater than growing cells in a lower than optimal temperature
  17. Magnetic stirring
  18. -Two CO 2 tanks attached in tandem. % of CO 2 is detected by an infrared gas analyzer to maintain an accuracy of +/- 0.1 %. - CO2 is filtered in, keeping CO2 sterile -Air filtered in to ensure an even temperature throughout the incubator chamber. - Temperature is controlled by a water jacket maintaining a temperature +/- 0.2  C. May also use heating elements. -Must keep incubator humid to prevent excessive evaporation from the media. A low concentration of disinfectant is kept in the water to prevent microbial growth.