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Defined Media and Supplements Chapter 9 Reasons for development of media Cells cultured in natural media  Cells cultured in chemically defined media based on analyses of body fluids and nutritional biochemistry  Eagle’s basal Medium, Eagle’s Minimal Essential medium (MEM), Dulbecco’s modification of Eagle’s medium (DMEM) etc  Physicochemical properties  Most cell lines grow well at pH 7.4  Transformed cell lines @ pH 7.0-7.4  Phenol red is used as an indicator Role of Co2, Bicarbonate ions and pH Requires both - optimum cell growth  Table 9.1 shows the amount of Co2, HCO3- and HEPES  Inclusion of pyruvate in medium enables cells to increase their endogenous production of CO2 making them independent of exogenous CO2 as well as HCO3 Co2, Bicarbonate and pH - Co2 in gas phase dissolves in medium Establishes equilibrium with HCO3- ions and lowers pH. H2O + CO2 H2CO3 H+ + HCO3- - Balanced by bicarbonate concentration from a base.  - - Reduction of Oxygen Toxicity In vivo – oxygen required for respiration  In vitro – glutathione  Cell cultures – require low oxygen tensions  Organ cultures – late-stage embryos, newborns or adults require 95% O2  Selenium tolerance is provided  Reduction of Viscosity  Cell damage can be reduced by – Carboxymethylcellulose (CMC) or Polyvinylpyrrolidone (PVP) Reduction of surface tension and foaming Foaming can lead to Protein Denaturation  Contamination  Limit gaseous diffusion  Arises in suspension cultures in stirrer vessels or bioreactors  Silicone antifoam or Pluronic F68 – 0.01-0.1% prevents foaming  Prevents foaming by reducing surface tension and may protect cells against shear stress from bubbles  What is Balanced Salt Solutions? BSS is composed of inorganic salts, may include sodium bicarbonate and glucose  Forms basis of complete media  BSS recipes are modified  PBS without Ca2+ and Mg2+ = known as PBS solution A  D-PBSA  Usage of BSS  Depends on CO2 tension  Tissue disaggregation or monolayer dispersal  Suspension or adherent cell culture What is Complete Media? media – all constituents (glutamine) and supplements (serum, growth factors or hormones)  Complete 9.4.1 Amino acids Essential amino acids – cysteine, arginine, glutamine and tyrosine  Individual requirements vary with cell type  Responsible for cell growth and survival  Other nonessential amino acids are added  9.4.2 Vitamins Eagle MEM - Water soluble vitamins – B group, choline, folic acid, inositol and nicotinamide  M199 - Fat soluble vitamins (A,D, E and K)  LHC-9 has Vitamin A  MCDB 110 has Vitamin E  Individual requirements vary with cell type  9.4.3 Salts Na+, K+, Mg 2+, Ca2+, Cl-, SO4, PO4 and HCO3- maintain osmolality of medium  Ca2+ - signal transduction process, whether proliferate or differentiate  Na+, K+ and Cl- regulate membrane potential  SO4, PO4- and HCO3- act as nutritional precursors for macromolecules and regulate intracellular charge  9.4.4 Glucose Source of energy  Metabolism of glucose – by Glycolysis to form Pyruvate  Pyruvate - converted to lactate or acetoacetate – enters into citric acid cycle  More energy derived from glutamine than glucose  9.4.5 Organic Supplements  Proteins, Peptides, Nucleosides, Citric acid cycle intermediates, Pyruvate and Lipids  Help in cloning and maintaining certain specialized cells (in presence or absence of serum) 9.4.7 Antibiotics Disadvantages: Encourage development of antibiotic-resistant organisms  Hide cryptic contaminants  Hide mycoplasma infections  Antimetabolic effects that can cross-react with mammalian cells  9.5 Serum Commonly used : bovine calf, fetal bovine, adult horse and human serum  Calf (CS) and fetal bovine (FBS) – used for cell lines and cloning  Human serum – used for human cell lines  Horse serum is consistent from batch to batch - Less polyamines  9.5.1 Protein Albumin – important carrier of lipids, minerals and globulins  Fibronectin – promote cell attachment  Fetutin – enhance cell attachment  Transferrin – binds iron  Increases viscosity of medium, reducing shear stress during pipetting and stirring and adds to medium’s buffering capacity  9.5.2 Growth Factors Platelet-derived growth factor (PDGF)  Fibroblast growth factor (FGFs)  Epidermal growth factor (EGF)  Insulin-like growth factors IGF-I and IGF-II  Help in Mitogenic activity and stability  9.5.3 Hormones  Hydrocortisone – present in fetal bovine serum – can promote cell attachment and proliferation or cell differentiation  Insulin – uptake of glucose and amino acids – binds to IGF receptors Selection of medium and serum     RPMI 1640, DMEM and MEM – 75 % sales DMEM/F12 – 4% DMEM has twice the amino acid concentration of MEM, four times the vitamin concentrations and twice the HCO3and CO2 concentrations to achieve better buffering MEM has additional amino acids, vitamins, nucleosides and lipoic acids Testing serum  - - Plating efficiency: check growth of cells in Cloning, count them Stain and count colonies Plating efficiency (survival) and colony size (cell proliferation) Tested at a range 2-20% Testing serum Growth curve: lag period, doubling time and saturation density - Lag period – culture has to adapt to serum - Saturation density – more cells will grow in a given amount of serum  Preservation of cell culture characteristics  Sterility     This project is funded by a grant awarded under the President’s Community Based Job Training Grant as implemented by the U.S. Department of Labor’s Employment and Training Administration (CB-15-162-06-60). 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