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Suspension culture

A cell suspension or suspension culture is a type of cell culture in which single cells or small aggregates of cells are allowed to function and multiply in an agitated growth medium, thus forming a suspension. Suspension culture is one of the two classical types of cell culture, the other being adherent culture. The history of suspension cell culture closely aligns with the history of cell culture overall, but differs in maintenance methods and commercial applications. The cells themselves can either be derived from homogenized tissue or from heterogenous cell solutions. Suspension cell culture is commonly used to culture nonadhesive cell lines like hematopoietic cells, plant cells, and insect cells.[1] While some cell lines are cultured in suspension, the majority of commercially available mammalian cell lines are adherent.[2][3] Suspension cell cultures must be agitated to maintain cells in suspension, and may require specialized equipment (e.g. magnetic stir plate, orbital shakers, incubators) and flasks (e.g. culture flasks, spinner flasks, shaker flasks).[4] These cultures need to be maintained with nutrient containing media and cultured in a specific cell density range to avoid cell death.[5]

CHO cells in suspension

History edit

 
SH-SY5Y cells adhered to a surface

The history of suspension cell culture is closely tied to the overall history of cell and tissue culture. In 1885, Wilhelm Roux laid the groundwork for future tissue culture, by developing a saline buffer that was used to maintain living cells (chicken embryos) for a few days.[6] Ross Granville Harrison in 1907 then developed in vitro cell culture techniques, including modifying the hanging drop technique for nerve cells and introducing aseptic technique to the culture process.[7] Later in 1910, Montrose Thomas Burrows adapted Harrison's technique and collaborated with Alexis Carrel to establish multiple tissue cultures that could be maintained in vitro using fresh plasma combined with saline solutions.[8] Carrel went on to develop the first known cell line, a line derived from chicken embryo heart which was maintained continuously for 34 years.[9] Though the "immortality" of the cell line was later challenged by Leonard Hayflick, this was a major breakthrough and inspired others to pursue creating other cell lines.[10] Notably in 1952, George Otto Gay and his assistant Mary Kubicek cultured the first human derived immortalized cell line - HeLa. While the other cell lines were adherent, HeLa cells were able to be maintained in suspension.[11]

Methods and maintenance edit

Isolating cells and starting a culture edit

All primary cells (cells derived directly from a subject) must first be removed from a subject, isolated (using digestion enzymes), and suspended in media before being cultured.[1] However, this does not mean that these cells are compatible with suspension culture, as most mammalian cells are adherent and need to attach to a surface to divide. White blood cells can be taken from a subject and cultured in suspension, since they naturally exist in suspension in blood.[12] Adhesion of white blood cells in vivo is typically the result of an inflammatory immune response and requires specific cell-cell interactions that should not occur in a suspension of a single type of white blood cell.[13]

Immortalized mammalian cell lines (cells that are able to replicate indefinitely), plant cells, and insect cells can be obtained cryopreserved from manufacturers and used to start a suspension culture.[14] To start a culture from cryopreserved cells, the cells must first be thawed and added to a flask or bioreactor containing media. Depending upon the cryoprotectant agent, the cells might need to be washed to avoid deleterious effects from the agent.[3]

Suspension cell culture maintenance for laboratories edit

Suspension cell cultures are similar to adherent cultures in a number of ways. Both require specialized nutrient containing media, containers that allow for gas transfer, aseptic conditions to avoid contamination, and frequent passaging to prevent overcrowding of cells. However, even within these similarities there are a few key differences between these culture methods. For example, though both adherent and suspension cell cultures can be maintained in standard flasks such as the T-75 tissue culture flask, suspension cultures need to be agitated to avoid settling to the bottom of the flask. While adherent cell cultures can be maintained in flat flasks with a lot of surface area (to promote cell adhesion), suspension cultures require agitation otherwise the cells will fall to the bottom of a flask, greatly impacting their access to nutrients and oxygen, eventually resulting in cell death.[4] For this reason, specialized flasks (including the spinner flask and shaker flask, discussed below) have been developed to agitate media and keep the cells in suspension. However, the agitation of media subjects the cells to shear forces which can stress the cells and negatively impact growth. Although both adherent and suspension cell cultures require media, media used in suspension culture may contain a surfactant to protect cells from shear forces in addition to the amino acids, vitamins and salt solution contained in culture media such as DMEM.[5]

Spinner flasks edit

Spinner flasks, which are used for suspension cultures, contain a magnetic spinner bar which circulates the media throughout the flask and keeps cells in suspension.[15] Spinner flasks contain one central capped opening flanked by two protruding arms which are also capped and allow for additional gas exchange. The magnetic spinner bar itself is typically suspended from a rod attached to the central cap so that it maximizes media circulation in the cell suspension. When culturing cells, the spinner flask containing cells is placed on a magnetic stir plate, inside of an incubator and the spinner parameters need to be adjusted carefully to avoid killing cells with shear forces.[16]

 
Orbital laboratory shaker.

Shaker flasks edit

Shaker flasks are also used for suspension cultures, and appear similar to typical Erlenmeyer flasks but have a semi-permeable lid to allow for gas exchange.[17] During suspension cell culturing, shaker flasks are loaded with cells and the appropriate media before they are placed on an orbital shaker. To optimize cell culture proliferation, the revolutions per minute of the orbital shaker must be adjusted within an acceptable range depending on the cells and media used. The media must be allowed to stir, but cannot disturb the cells too much causing them excessive stress. Shaker flasks are often used for fermentation cultures with microorganisms such as yeast.[18]

Passaging (subculturing) cells edit

Passaging, or subculturing, suspension cell cultures is more straightforward than passaging adherent cells. While adherent cells require initial processing with a digestion enzyme, to remove them from the culture flask surface, suspension cells are floating freely in media.[19] A sample from the culture can then be taken and analyzed to determine the ratio of living to dead cells (using a stain such as trypan blue) and the total concentration of cells in the flask (using a hemocytometer). Using this information, a portion of the current suspension culture will be transferred to fresh flask and supplemented with media. The passage number should be recorded, particularly if the cells are primary and not immortalized as primary cell lines will eventually undergo senescence.[20] Suspension cells are often passaged outright without changing the media. In order to change the media for a suspension culture, all cells from the current container should be removed and centrifuged into a pellet. The excess media is then removed from the centrifuged sample, and the flask is refilled with fresh media before re-adding the cells to the flask. Media changes and subculturing are important to maintain cell lines, since cells will consume nutrients in media to expand. Cells will also grow exponentially until the environment becomes inhospitable due to lack of nutrients, extreme pH, or lack of space to grow.

Commercial applications of suspension cell culture edit

Unlike adherent cultures, which are limited by the surface area provided for them to expand on, suspension cultures are limited by the volume of their container. Meaning, suspension cells can exist in much larger quantities in a given flask and are preferred when using cells to make products including proteins, antibodies, metabolites or just to produce a high volume of cells. However, there are far fewer mammalian suspension cell lines than mammalian adhesive cell lines. Most large scale suspension culture involves non-mammalian cells and takes place in bioreactors.

Some examples of suspension cell culture:

  • Antibody production by hybridomas[21]
  • Fermentation cultures for beer[22]
  • Therapeutic protein production by CHO cells[23]
  • Secondary metabolite production for drugs in plant cells[24]
  • Recombinant protein production in insect cells[25]
  • Bulk protein production for enzyme and vaccine research[26]
  • Producing cell suspension cultures to support oncolytic adenovirus used in cancer immunotherapy [27]

List of suspension cell lines edit

Cell line Meaning Organism Origin tissue Morphology Links
CHO Chinese Hamster Ovary Hamster Ovary Epithelial ECACC Cellosaurus
HeLa "Henrietta Lacks" Human Cervix epithelium Cervical carcinoma ECACC Cellosaurus
H-9 Human Embryonic stem cells Lymphoblast Cellosaurus
Jurkat Human White blood cells Lymphoblast ECACC Cellosaurus
C6/36 Insect - Asian tiger mosquito Larval tissue ECACC Cellosaurus
High Five Insect (moth) - Trichoplusia ni Ovary Cellosaurus
S2 Schneider 2 Insect - Drosophila melanogaster Late stage (20–24 hours old) embryos ATCC Cellosaurus
Sf21 Spodoptera frugiperda 21 Insect (moth) - Spodoptera frugiperda Ovary ECACC Cellosaurus
Sf9 Spodoptera frugiperda 9 Insect (moth) - Spodoptera frugiperda Ovary Epithelial ECACC Cellosaurus
SH-SY5Y Human Bone marrow Epithelial Cellosaurus
PC-3 Human Prostate Epithelial Cellosaurus

See also edit

References edit

  1. ^ a b Gibco Cell Culture Basics Handbook. www.invitrogen.com/cellculturebasics: Thermofisher Scientific.
  2. ^ "Cell Culture Basics: Equipment, Fundamentals and Protocols". Cell Science from Technology Networks. Retrieved 2021-11-08.
  3. ^ a b Sigma Aldrich. "Fundamental Techniques in Cell Culture - Laboratory Handbook 3rd Edition" (PDF). Retrieved 2021-11-07.
  4. ^ a b Taya, M.; Kino-oka, M. (2011-01-01), Moo-Young, Murray (ed.), "2.27 - Bioreactors for Animal Cell Cultures", Comprehensive Biotechnology (Second Edition), Burlington: Academic Press, pp. 373–382, ISBN 978-0-08-088504-9, retrieved 2021-10-30
  5. ^ a b "Subculturing Suspension Cells - US". www.thermofisher.com. Retrieved 2021-10-30.
  6. ^ Hoffman, R.M. (September 26, 2016). "The Beginning of Tissue Culture". Elsevier SciTech Connect. Retrieved November 29, 2022.
  7. ^ "Ross Granville Harrison (1870-1959) | The Embryo Project Encyclopedia". embryo.asu.edu. Retrieved 2022-11-29.
  8. ^ "Alexis Carrel's Tissue Culture Techniques | The Embryo Project Encyclopedia". embryo.asu.edu. Retrieved 2022-11-29.
  9. ^ Jedrzejczak-Silicka, Magdalena (2017-05-10). History of Cell Culture. IntechOpen. ISBN 978-953-51-3134-2.
  10. ^ Jiang, Lijing. ""Alexis Carrel's Tissue Culture Techniques." The Embryo Project Encyclopedia". embryo.asu.edu. Retrieved 2021-10-18.
  11. ^ Skloot, Rebecca (2010). The immortal life of Henrietta Lacks. New York: Crown Publishers. ISBN 978-1-4000-5217-2. OCLC 326529053.
  12. ^ Granger, D. Neil; Senchenkova, Elena (2010). Leukocyte–Endothelial Cell Adhesion. Morgan & Claypool Life Sciences.
  13. ^ Alberts, Bruce; Johnson, Alexander; Lewis, Julian; Raff, Martin; Roberts, Keith; Walter, Peter (2002). "Cell-Cell Adhesion". Molecular Biology of the Cell. 4th Edition.
  14. ^ "Cryopreservation of Mammalian Cells - US". www.thermofisher.com. Retrieved 2022-12-02.
  15. ^ Freed, Lisa E.; Guilak, Farshid (2007-01-01), Lanza, Robert; Langer, Robert; Vacanti, Joseph (eds.), "Chapter Eleven - Engineering Functional Tissues", Principles of Tissue Engineering (Third Edition), Burlington: Academic Press, pp. 137–153, ISBN 978-0-12-370615-7, retrieved 2021-10-30
  16. ^ Kurtis Kasper, Milind Singh, F.; Mikos, Antonios G. (2013-01-01), Ratner, Buddy D.; Hoffman, Allan S.; Schoen, Frederick J.; Lemons, Jack E. (eds.), "Chapter II.6.3 - Tissue Engineering Scaffolds", Biomaterials Science (Third Edition), Academic Press, pp. 1138–1159, ISBN 978-0-12-374626-9, retrieved 2021-10-30{{citation}}: CS1 maint: multiple names: authors list (link)
  17. ^ Klöckner, W.; Büchs, J. (2011-01-01), Moo-Young, Murray (ed.), "2.17 - Shake-Flask Bioreactors", Comprehensive Biotechnology (Second Edition), Burlington: Academic Press, pp. 213–226, ISBN 978-0-08-088504-9, retrieved 2021-10-30
  18. ^ Link, H.; Weuster-Botz, D. (2011-01-01), Moo-Young, Murray (ed.), "2.11 - Medium Formulation and Development", Comprehensive Biotechnology (Second Edition), Burlington: Academic Press, pp. 119–134, ISBN 978-0-08-088504-9, retrieved 2021-10-30
  19. ^ Gibco Cell Culture Basics Handbook. www.invitrogen.com/cellculturebasics: Thermofisher Scientific.
  20. ^ Sigma Aldrich. "Fundamental Techniques in Cell Culture - Laboratory Handbook 3rd Edition" (PDF). Retrieved 2021-11-07.
  21. ^ Li, Feng; Vijayasankaran, Natarajan; Shen, Amy (Yijuan); Kiss, Robert; Amanullah, Ashraf (2010). "Cell culture processes for monoclonal antibody production". mAbs. 2 (5): 466–477. doi:10.4161/mabs.2.5.12720. ISSN 1942-0862. PMC 2958569. PMID 20622510.
  22. ^ Pilkington, P. H.; Margaritis, A.; Mensour, N. A.; Russell, I. (1998). "Fundamentals of Immobilised Yeast Cells for Continuous Beer Fermentation: A Review". Journal of the Institute of Brewing. 104 (1): 19–31. doi:10.1002/j.2050-0416.1998.tb00970.x. ISSN 2050-0416.
  23. ^ Matasci, Mattia; Hacker, David L.; Baldi, Lucia; Wurm, Florian M. (2008-09-01). "Recombinant therapeutic protein production in cultivated mammalian cells: current status and future prospects". Drug Discovery Today: Technologies. Protein therapeutics. 5 (2): e37–e42. doi:10.1016/j.ddtec.2008.12.003. ISSN 1740-6749. PMID 24981089.
  24. ^ Verpoorte, R.; van der Heijden, R.; Memelink, J. (2000-07-01). "Engineering the plant cell factory for secondary metabolite production". Transgenic Research. 9 (4): 323–343. doi:10.1023/A:1008966404981. ISSN 1573-9368. PMID 11131010. S2CID 25185714.
  25. ^ Scott, Robert I.; Blanchard, John H.; Ferguson, Clare H. R. (1992-10-01). "Effects of oxygen on recombinant protein production by suspension cultures of Spodoptera frugiperda (Sf-9) insect cells". Enzyme and Microbial Technology. 14 (10): 798–804. doi:10.1016/0141-0229(92)90095-6. ISSN 0141-0229. PMID 1369406.
  26. ^ admin.facellitate (2022-06-08). "In vitro cell culture techniques: Adherent culture Vs. Suspension culture". faCellitate. Retrieved 2022-11-29.
  27. ^ Moreira, Ana Sofia; Silva, Ana Carina; Sousa, Marcos F. Q.; Hagner-McWhirterc, Åsa; Ahlénc, Gustaf; Lundgren, Mats; Coroadinha, Ana S.; Alves, Paula M.; Peixoto, Cristina; Carrondo, Manuel J. T. (April 2020). "Establishing Suspension Cell Cultures for Improved Manufacturing of Oncolytic Adenovirus". Biotechnology Journal. 15 (4): e1900411. doi:10.1002/biot.201900411. ISSN 1860-7314. PMID 31950598. S2CID 210700489.

suspension, culture, cell, suspension, suspension, culture, type, cell, culture, which, single, cells, small, aggregates, cells, allowed, function, multiply, agitated, growth, medium, thus, forming, suspension, classical, types, cell, culture, other, being, ad. A cell suspension or suspension culture is a type of cell culture in which single cells or small aggregates of cells are allowed to function and multiply in an agitated growth medium thus forming a suspension Suspension culture is one of the two classical types of cell culture the other being adherent culture The history of suspension cell culture closely aligns with the history of cell culture overall but differs in maintenance methods and commercial applications The cells themselves can either be derived from homogenized tissue or from heterogenous cell solutions Suspension cell culture is commonly used to culture nonadhesive cell lines like hematopoietic cells plant cells and insect cells 1 While some cell lines are cultured in suspension the majority of commercially available mammalian cell lines are adherent 2 3 Suspension cell cultures must be agitated to maintain cells in suspension and may require specialized equipment e g magnetic stir plate orbital shakers incubators and flasks e g culture flasks spinner flasks shaker flasks 4 These cultures need to be maintained with nutrient containing media and cultured in a specific cell density range to avoid cell death 5 CHO cells in suspension Contents 1 History 2 Methods and maintenance 2 1 Isolating cells and starting a culture 2 2 Suspension cell culture maintenance for laboratories 2 2 1 Spinner flasks 2 2 2 Shaker flasks 2 2 3 Passaging subculturing cells 3 Commercial applications of suspension cell culture 4 List of suspension cell lines 5 See also 6 ReferencesHistory edit nbsp SH SY5Y cells adhered to a surfaceThe history of suspension cell culture is closely tied to the overall history of cell and tissue culture In 1885 Wilhelm Roux laid the groundwork for future tissue culture by developing a saline buffer that was used to maintain living cells chicken embryos for a few days 6 Ross Granville Harrison in 1907 then developed in vitro cell culture techniques including modifying the hanging drop technique for nerve cells and introducing aseptic technique to the culture process 7 Later in 1910 Montrose Thomas Burrows adapted Harrison s technique and collaborated with Alexis Carrel to establish multiple tissue cultures that could be maintained in vitro using fresh plasma combined with saline solutions 8 Carrel went on to develop the first known cell line a line derived from chicken embryo heart which was maintained continuously for 34 years 9 Though the immortality of the cell line was later challenged by Leonard Hayflick this was a major breakthrough and inspired others to pursue creating other cell lines 10 Notably in 1952 George Otto Gay and his assistant Mary Kubicek cultured the first human derived immortalized cell line HeLa While the other cell lines were adherent HeLa cells were able to be maintained in suspension 11 Methods and maintenance editIsolating cells and starting a culture edit Main article Cell isolation All primary cells cells derived directly from a subject must first be removed from a subject isolated using digestion enzymes and suspended in media before being cultured 1 However this does not mean that these cells are compatible with suspension culture as most mammalian cells are adherent and need to attach to a surface to divide White blood cells can be taken from a subject and cultured in suspension since they naturally exist in suspension in blood 12 Adhesion of white blood cells in vivo is typically the result of an inflammatory immune response and requires specific cell cell interactions that should not occur in a suspension of a single type of white blood cell 13 Immortalized mammalian cell lines cells that are able to replicate indefinitely plant cells and insect cells can be obtained cryopreserved from manufacturers and used to start a suspension culture 14 To start a culture from cryopreserved cells the cells must first be thawed and added to a flask or bioreactor containing media Depending upon the cryoprotectant agent the cells might need to be washed to avoid deleterious effects from the agent 3 Suspension cell culture maintenance for laboratories edit Suspension cell cultures are similar to adherent cultures in a number of ways Both require specialized nutrient containing media containers that allow for gas transfer aseptic conditions to avoid contamination and frequent passaging to prevent overcrowding of cells However even within these similarities there are a few key differences between these culture methods For example though both adherent and suspension cell cultures can be maintained in standard flasks such as the T 75 tissue culture flask suspension cultures need to be agitated to avoid settling to the bottom of the flask While adherent cell cultures can be maintained in flat flasks with a lot of surface area to promote cell adhesion suspension cultures require agitation otherwise the cells will fall to the bottom of a flask greatly impacting their access to nutrients and oxygen eventually resulting in cell death 4 For this reason specialized flasks including the spinner flask and shaker flask discussed below have been developed to agitate media and keep the cells in suspension However the agitation of media subjects the cells to shear forces which can stress the cells and negatively impact growth Although both adherent and suspension cell cultures require media media used in suspension culture may contain a surfactant to protect cells from shear forces in addition to the amino acids vitamins and salt solution contained in culture media such as DMEM 5 Spinner flasks edit Spinner flasks which are used for suspension cultures contain a magnetic spinner bar which circulates the media throughout the flask and keeps cells in suspension 15 Spinner flasks contain one central capped opening flanked by two protruding arms which are also capped and allow for additional gas exchange The magnetic spinner bar itself is typically suspended from a rod attached to the central cap so that it maximizes media circulation in the cell suspension When culturing cells the spinner flask containing cells is placed on a magnetic stir plate inside of an incubator and the spinner parameters need to be adjusted carefully to avoid killing cells with shear forces 16 nbsp Orbital laboratory shaker Shaker flasks edit Shaker flasks are also used for suspension cultures and appear similar to typical Erlenmeyer flasks but have a semi permeable lid to allow for gas exchange 17 During suspension cell culturing shaker flasks are loaded with cells and the appropriate media before they are placed on an orbital shaker To optimize cell culture proliferation the revolutions per minute of the orbital shaker must be adjusted within an acceptable range depending on the cells and media used The media must be allowed to stir but cannot disturb the cells too much causing them excessive stress Shaker flasks are often used for fermentation cultures with microorganisms such as yeast 18 Passaging subculturing cells edit Passaging or subculturing suspension cell cultures is more straightforward than passaging adherent cells While adherent cells require initial processing with a digestion enzyme to remove them from the culture flask surface suspension cells are floating freely in media 19 A sample from the culture can then be taken and analyzed to determine the ratio of living to dead cells using a stain such as trypan blue and the total concentration of cells in the flask using a hemocytometer Using this information a portion of the current suspension culture will be transferred to fresh flask and supplemented with media The passage number should be recorded particularly if the cells are primary and not immortalized as primary cell lines will eventually undergo senescence 20 Suspension cells are often passaged outright without changing the media In order to change the media for a suspension culture all cells from the current container should be removed and centrifuged into a pellet The excess media is then removed from the centrifuged sample and the flask is refilled with fresh media before re adding the cells to the flask Media changes and subculturing are important to maintain cell lines since cells will consume nutrients in media to expand Cells will also grow exponentially until the environment becomes inhospitable due to lack of nutrients extreme pH or lack of space to grow Commercial applications of suspension cell culture editUnlike adherent cultures which are limited by the surface area provided for them to expand on suspension cultures are limited by the volume of their container Meaning suspension cells can exist in much larger quantities in a given flask and are preferred when using cells to make products including proteins antibodies metabolites or just to produce a high volume of cells However there are far fewer mammalian suspension cell lines than mammalian adhesive cell lines Most large scale suspension culture involves non mammalian cells and takes place in bioreactors Some examples of suspension cell culture Antibody production by hybridomas 21 Fermentation cultures for beer 22 Therapeutic protein production by CHO cells 23 Secondary metabolite production for drugs in plant cells 24 Recombinant protein production in insect cells 25 Bulk protein production for enzyme and vaccine research 26 Producing cell suspension cultures to support oncolytic adenovirus used in cancer immunotherapy 27 List of suspension cell lines editCell line Meaning Organism Origin tissue Morphology LinksCHO Chinese Hamster Ovary Hamster Ovary Epithelial ECACC CellosaurusHeLa Henrietta Lacks Human Cervix epithelium Cervical carcinoma ECACC CellosaurusH 9 Human Embryonic stem cells Lymphoblast CellosaurusJurkat Human White blood cells Lymphoblast ECACC CellosaurusC6 36 Insect Asian tiger mosquito Larval tissue ECACC CellosaurusHigh Five Insect moth Trichoplusia ni Ovary CellosaurusS2 Schneider 2 Insect Drosophila melanogaster Late stage 20 24 hours old embryos ATCC CellosaurusSf21 Spodoptera frugiperda 21 Insect moth Spodoptera frugiperda Ovary ECACC CellosaurusSf9 Spodoptera frugiperda 9 Insect moth Spodoptera frugiperda Ovary Epithelial ECACC CellosaurusSH SY5Y Human Bone marrow Epithelial CellosaurusPC 3 Human Prostate Epithelial CellosaurusSee also editCell culture Adherent culture Bio MEMS Cell adhesion Cell adhesion moleculeReferences edit a b Gibco Cell Culture Basics Handbook www invitrogen com cellculturebasics Thermofisher Scientific Cell Culture Basics Equipment Fundamentals and Protocols Cell Science from Technology Networks Retrieved 2021 11 08 a b Sigma Aldrich Fundamental Techniques in Cell Culture Laboratory Handbook 3rd Edition PDF Retrieved 2021 11 07 a b Taya M Kino oka M 2011 01 01 Moo Young Murray ed 2 27 Bioreactors for Animal Cell Cultures Comprehensive Biotechnology Second Edition Burlington Academic Press pp 373 382 ISBN 978 0 08 088504 9 retrieved 2021 10 30 a b Subculturing Suspension Cells US www thermofisher com Retrieved 2021 10 30 Hoffman R M September 26 2016 The Beginning of Tissue Culture Elsevier SciTech Connect Retrieved November 29 2022 Ross Granville Harrison 1870 1959 The Embryo Project Encyclopedia embryo asu edu Retrieved 2022 11 29 Alexis Carrel s Tissue Culture Techniques The Embryo Project Encyclopedia embryo asu edu Retrieved 2022 11 29 Jedrzejczak Silicka Magdalena 2017 05 10 History of Cell Culture IntechOpen ISBN 978 953 51 3134 2 Jiang Lijing Alexis Carrel s Tissue Culture Techniques The Embryo Project Encyclopedia embryo asu edu Retrieved 2021 10 18 Skloot Rebecca 2010 The immortal life of Henrietta Lacks New York Crown Publishers ISBN 978 1 4000 5217 2 OCLC 326529053 Granger D Neil Senchenkova Elena 2010 Leukocyte Endothelial Cell Adhesion Morgan amp Claypool Life Sciences Alberts Bruce Johnson Alexander Lewis Julian Raff Martin Roberts Keith Walter Peter 2002 Cell Cell Adhesion Molecular Biology of the Cell 4th Edition Cryopreservation of Mammalian Cells US www thermofisher com Retrieved 2022 12 02 Freed Lisa E Guilak Farshid 2007 01 01 Lanza Robert Langer Robert Vacanti Joseph eds Chapter Eleven Engineering Functional Tissues Principles of Tissue Engineering Third Edition Burlington Academic Press pp 137 153 ISBN 978 0 12 370615 7 retrieved 2021 10 30 Kurtis Kasper Milind Singh F Mikos Antonios G 2013 01 01 Ratner Buddy D Hoffman Allan S Schoen Frederick J Lemons Jack E eds Chapter II 6 3 Tissue Engineering Scaffolds Biomaterials Science Third Edition Academic Press pp 1138 1159 ISBN 978 0 12 374626 9 retrieved 2021 10 30 a href Template Citation html title Template Citation citation a CS1 maint multiple names authors list link Klockner W Buchs J 2011 01 01 Moo Young Murray ed 2 17 Shake Flask Bioreactors Comprehensive Biotechnology Second Edition Burlington Academic Press pp 213 226 ISBN 978 0 08 088504 9 retrieved 2021 10 30 Link H Weuster Botz D 2011 01 01 Moo Young Murray ed 2 11 Medium Formulation and Development Comprehensive Biotechnology Second Edition Burlington Academic Press pp 119 134 ISBN 978 0 08 088504 9 retrieved 2021 10 30 Gibco Cell Culture Basics Handbook www invitrogen com cellculturebasics Thermofisher Scientific Sigma Aldrich Fundamental Techniques in Cell Culture Laboratory Handbook 3rd Edition PDF Retrieved 2021 11 07 Li Feng Vijayasankaran Natarajan Shen Amy Yijuan Kiss Robert Amanullah Ashraf 2010 Cell culture processes for monoclonal antibody production mAbs 2 5 466 477 doi 10 4161 mabs 2 5 12720 ISSN 1942 0862 PMC 2958569 PMID 20622510 Pilkington P H Margaritis A Mensour N A Russell I 1998 Fundamentals of Immobilised Yeast Cells for Continuous Beer Fermentation A Review Journal of the Institute of Brewing 104 1 19 31 doi 10 1002 j 2050 0416 1998 tb00970 x ISSN 2050 0416 Matasci Mattia Hacker David L Baldi Lucia Wurm Florian M 2008 09 01 Recombinant therapeutic protein production in cultivated mammalian cells current status and future prospects Drug Discovery Today Technologies Protein therapeutics 5 2 e37 e42 doi 10 1016 j ddtec 2008 12 003 ISSN 1740 6749 PMID 24981089 Verpoorte R van der Heijden R Memelink J 2000 07 01 Engineering the plant cell factory for secondary metabolite production Transgenic Research 9 4 323 343 doi 10 1023 A 1008966404981 ISSN 1573 9368 PMID 11131010 S2CID 25185714 Scott Robert I Blanchard John H Ferguson Clare H R 1992 10 01 Effects of oxygen on recombinant protein production by suspension cultures of Spodoptera frugiperda Sf 9 insect cells Enzyme and Microbial Technology 14 10 798 804 doi 10 1016 0141 0229 92 90095 6 ISSN 0141 0229 PMID 1369406 admin facellitate 2022 06 08 In vitro cell culture techniques Adherent culture Vs Suspension culture faCellitate Retrieved 2022 11 29 Moreira Ana Sofia Silva Ana Carina Sousa Marcos F Q Hagner McWhirterc Asa Ahlenc Gustaf Lundgren Mats Coroadinha Ana S Alves Paula M Peixoto Cristina Carrondo Manuel J T April 2020 Establishing Suspension Cell Cultures for Improved Manufacturing of Oncolytic Adenovirus Biotechnology Journal 15 4 e1900411 doi 10 1002 biot 201900411 ISSN 1860 7314 PMID 31950598 S2CID 210700489 Retrieved from https en wikipedia org w index php title Suspension culture amp oldid 1177472562, wikipedia, wiki, book, books, library,

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