Figure 4
Figure 4. Lnk domains and Y536 contribute differently to the proliferation of hematopoietic progenitors in vitro. (A) Total RNA was extracted from wild-type (+/+) or Lnk−/− Lin−GFP+ progenitor cells transduced with either vector alone, WT or mutant forms of Lnk and subjected to RT-PCR with specific primers for Lnk (top panel) or HPRT (bottom panel) as control. (B) Wild-type or Lnk−/− Lin−GFP+ transduced cells were assessed for their in vitro proliferative capacity in methylcellulose media containing IL-7 and SCF. Data represent the mean plus or minus SD (error bars) of number of colonies per 103 Lin−GFP+ cells from triplicate samples from 3 independent assays using 3 to 5 mice of each genotype. Statistical significance was determined using the Student t test: ***P ≤ .01. (C) Typical appearance of GFP+ pre-B colonies from Lin− transduced progenitor cells in response to IL-7 + SCF after 7 days of incubation in methylcellulose media. GFP+ colonies were acquired with a 40×/0.55 NA dry objective and a charge-coupled device (CCD) camera (MicroMax 13004, Princeton Instruments, Trenton, NJ). Images were processed with MetaMorph software (Molecular Devices, Downingtown, PA). Scale bar equals 20 μm.

Lnk domains and Y536 contribute differently to the proliferation of hematopoietic progenitors in vitro. (A) Total RNA was extracted from wild-type (+/+) or Lnk−/− LinGFP+ progenitor cells transduced with either vector alone, WT or mutant forms of Lnk and subjected to RT-PCR with specific primers for Lnk (top panel) or HPRT (bottom panel) as control. (B) Wild-type or Lnk−/− LinGFP+ transduced cells were assessed for their in vitro proliferative capacity in methylcellulose media containing IL-7 and SCF. Data represent the mean plus or minus SD (error bars) of number of colonies per 103 LinGFP+ cells from triplicate samples from 3 independent assays using 3 to 5 mice of each genotype. Statistical significance was determined using the Student t test: ***P ≤ .01. (C) Typical appearance of GFP+ pre-B colonies from Lin transduced progenitor cells in response to IL-7 + SCF after 7 days of incubation in methylcellulose media. GFP+ colonies were acquired with a 40×/0.55 NA dry objective and a charge-coupled device (CCD) camera (MicroMax 13004, Princeton Instruments, Trenton, NJ). Images were processed with MetaMorph software (Molecular Devices, Downingtown, PA). Scale bar equals 20 μm.

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