| Cloning by Limiting Dilution of Hybridoma | | 点击: 作者: 来源: 时间: 2007-04-10 本站论坛 |
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Cloning by Limiting Dilution of Hybridoma |
| Author: Nanci Donacki |
| Source: Contributed by Nanci Donacki |
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Materials
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DMEM, high glucose (Life Technologies, Inc. #10313-021 or equivalent)
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Fetal Bovine Serum (Life Technologies, Inc. #16000-044 or equivalent)
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L-glutamine (Life Technologies, Inc. #25030-149 or equivalent)
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Hybridoma Cloning Factor (Fisher # IG50-0615)
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50 ml sterile centrifuge tubes (Falcon #2070)
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15 ml sterile centrifuge tubes (Falcon # 2099)
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96 well culture plates (Falcon #3072))
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Hemocytometer
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Trypan Blue, 0.4% (Life Technologies, Inc. # 630-5150AG)
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Multi-channel pipettor and sterile tips
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Reagent Reservoir
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HT (Life Technologies, Inc. #11067-030)
Procedure
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The day before the cloning, refeed 24-well plates or flasks with fresh medium.
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Prepare the cloning medium DMEM 4 mM L-glutamine 20% FBS 10% Hybridoma Cloning Factor
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Resuspend the cells to be cloned. Transfer 1 ml to a sterile 15 ml tube. Transfer 50 ml of this suspension to a clean tube for cell and viability counts.
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Count the cells and determine the viability. NOTE: The viability must be greater than 80% to continue.
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For each hybridoma cell line, calculate the dilutions to give 4 cells/ml, 2 cells/ml and 1 cell/ml in cloning medium.
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Label 50 ml tubes for each clone and dilution.
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Add medium to each tube according to the calculated dilutions.
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Serially dilute each clone to 4, 2, and 1 cell/ml. The final dilution tube should contain 50 ml of cloning medium at 1 cell/ml.
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Pour each of the dilutions into a sterile reagent reservoir. Plate 250 ml/well into 96-well plates - 1 plate at 4 cells/ml, 1 plate at 2 cells/ml and 2 plates at 1 cell/ml.
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Complete dilutions and plating for each hybridoma cell line.
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Place all plates at 37oC, 8-10% CO2. Incubate for 5-7 days.
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Microscopically examine all plates to ensure cloning and plating efficiency before refeeding the plates. |
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