Figure 1
Figure 1. Microarrays as a preliminary screen for useful surface epitopes. (A) Schematic of 2 protocols used to prepare human MSCs. (B) Phase-contrast photomicrographs of viable MSCs from passage 1/donor 1 plated at 100 cells/cm2 and incubated for 5 or 9 days to generate passage 2 MSCs. (C) Assay by forward and side scatter of light of MSCs from panel B. Vertical and horizontal lines were generated with microbeads to standardize the assay.10 (D) Microarray assays of mRNAs from viable MSCs from passage 1/donor 6 plated at 100 cells/cm2 and incubated for 5 days to approximately 50% confluency, 10 days to 100% confluency, and 15 days to overconfluency. The values were normalized to mRNA signals on day 15 (left) or on day 5 (right).

Microarrays as a preliminary screen for useful surface epitopes. (A) Schematic of 2 protocols used to prepare human MSCs. (B) Phase-contrast photomicrographs of viable MSCs from passage 1/donor 1 plated at 100 cells/cm2 and incubated for 5 or 9 days to generate passage 2 MSCs. (C) Assay by forward and side scatter of light of MSCs from panel B. Vertical and horizontal lines were generated with microbeads to standardize the assay.10  (D) Microarray assays of mRNAs from viable MSCs from passage 1/donor 6 plated at 100 cells/cm2 and incubated for 5 days to approximately 50% confluency, 10 days to 100% confluency, and 15 days to overconfluency. The values were normalized to mRNA signals on day 15 (left) or on day 5 (right).

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