Hybridomas

1. Hybridomas

3. Hybrid Cell Lines Normal Cells Are Fused With A Cancerous Cell Line • E.x myeloma, lymphoma • Fusion Is Accomplished With PEG (polyethylene glycol) • The New Hybrid Cell Exhibits Properties Of Both Cell Types • Unlimited growth • Secretes monoclonal antibody • Or Secretes cytokines

4. Normal Cell • For Monoclonal Antibody Production • Animal Is Immunized With Antigen • Spleen Cells Are Isolated • Intraperitoneal Immunization • Balb/c Mouse • Day 0: 50 g of Ag In Complete Freund’s Adjuvant • Day 14: 25 g of Ag In Incomplete Freund’s Adjuvant • Day 28: 25 g of Ag In D-PBSA • Bleed Animal Test Reactivity To Antigen • Serum Is Diluted 1:30 • Final Boost of 10 g Antigen i.v or i.p 3 days before fusion • Aseptically Isolate Spleen Cells

5. P3.653 Myeloma • This Cell Line Is Deficient In HGPRT (hypoxantine guanine phosphoribosyl transferase) • Alternatively TK (thymidine kinase deficient) • Cell Line Cannot Survive In Selection Medium • Aminopterin Inhibits “De novo Pathway”, “Salvage Pathway” Is Not Possibe Due To HGPRT or TK Deficiency • It Is Also Ig Deficient • It can not secret any immunoglobulins • Aminopterin (folic acid antagonist) Blocks De novo Pathway • P3.653 cells die in the presence of aminopterin • They cannot utilize the “salvage pathway” because they are HGPRT deficient

7. Possible Fusion Products Myeloma HGPRT Deficient And Ig Deficient Plasma Cells From Immunized Animal +  Senescence  Can Use Salvage Pathway No Senescence  Senescence  HAT Medium  HAT Medium

12. Fusing Spleen Cells With Myeloma • Purify Spleen cells • T-cell Depletion (anti-Thy 1.2 followed by complement lysis) • MACS purification (CD138) • Fusion • Mix spleen cells and myeloma in 50 mL tube (4:1) • Spin and resuspend pellet with 1 mL PEG over 15 s • Mix by swirling for 75 s • Add 1 mL of SFM (serum free medium) over 15s, swirl for 45s • Add 2 mL SFM over 30s, swirl 90s • Add 4 mL HAT over 30s, swirl 90s • Add 8 mL HAT over 30s, swirl 90s • Add Above volume in a new container, add HAT till cell concentration is 1x106 cells/mL • Add 200 L per well 96 well/plate (200,000 cells/well)

13. Selection Of Hybridomas • Selecting Clones • Feed Wells With New HAT Medium (remove old, add 150 L new) • Feed Cells Twice A Week • After about 2 weeks Test Supernatants Of Potential Clones Using Elisa • Retest +ve Clones in 48 hrs • Expand Clones In New 96-well plate with HT NOT HAT • Retest Sups, Expand In 24-well Plate, Switch To Normal Medium, Retest • Expand in 4-well Plate • Cryopreserve

14. Ensuring Monoclonality • To Ensure Monoclonality Sub-clone Hybridoma • Serially dilute @ 1 cell per 3 wells • Use a spleen cells as feeder cells • Feeder cells concentration @ 1x106 cells/mL • 96 well plate, 2x105 cells/well • Colonies are observed at 5 days • Replenish with fresh medium @ day 7 • Screening Is done at day 10 and 14 • Clones are cryopreserved same way as parental clones

15. Antibody Production • Large Amounts Of Antibody Can Be Produced Using Animals • Prime Balb/c animal with IFA • Inject clone i.p • Collect peritoneal ascites • Alternatively Bioreactors Are Used • Cells are cultured in hollow fibers • Fresh media and waste are recircuilated • High concentrations of Ab produced in cell compartment • Collected at different time points