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Antibody production by injection of living cells expressing non self antigens as cell surface type II transmembrane fusion protein
Authors:Nizet Yannick  Gillet Laurent  Schroeder Hélène  Lecuivre Corinne  Louahed J  Renauld J-C  Gianello Pierre  Vanderplasschen Alain
Affiliation:Bellbrook Labs, 5500 Nobel Dr., Ste. 250, Madison, WI 53711, USA. ivar.meyvantsson@bellbrooklabs.com
Abstract:Multi-well assays based on the Boyden chamber have enabled highly parallel studies of chemotaxis-the directional migration of cells in response to molecular gradients-while direct-viewing approaches have allowed more detailed questions to be asked at low throughput. Boyden-based plates provide a count of cells that pass through a membrane, but no information about cell appearance. In contrast, direct-viewing devices enable the observation of cells during chemotaxis, which allows measurement of many parameters including area, shape, and location. Here we show automated chemotaxis and cell morphology assays in a 96-unit direct-viewing plate. Using only 12000 primary human neutrophils per datum, we measured dose-dependent stimulation and inhibition of chemotaxis and quantified the effects of inhibitors on cell area and elongation. With 60 parallel conditions we demonstrated 5-fold increase in throughput compared to previously reported direct-viewing approaches.
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