Fig. 1.
Fig. 1. Characterization of the functional promoter for CCR3 in human T cells. / (A) Map of the upstream region of the human CCR3 gene. Black boxes and angle dashed lines represent exons and splicing patterns, respectively. Exon 1 contains the main 5′ UTR part and exon 2 contains the ATG coding region. Grey arrows represent primers subsequently used for PCR in Figure 2A. H and K, respectively, indicate the position ofHindIII and KpnI sites. The 1, 2, and 3 located with gray lines indicate the regions analyzed by ChIP and DNaseI HS experiments. (B) Identification of the T-cell minimal promoter region for CCR3. Construct maps and data for relative luciferase expression in Jurkat human T cells (filled bars) and 721.221 human B cells (open bars). PCR fragments of variable sizes of the CCR3 5′-flanking region were generated and cloned in the Firefly luciferase pGL3 Basic vector. Exon 1 (gray box) and Luciferase (open box) are represented on the maps. Plasmids were transiently transfected by electroporation with a control plasmid pRL-TK (Renillaluciferase) into Jurkat and 721.221 cells. Relative luciferase activities of the cell lysates are representative of at least 5 independent experiments performed with different clones for each construct. Errors bars indicate SDs. (-) indicates not tested. (C) Identification of an NRE located in the flanking intronic region. An intronic PCR fragment (+134 to +237) was cloned either in sense (pGL3 C NRE S) or antisense orientation (pGL3 C NRE AS) into theFirefly luciferase vector pGL3 control containing the SV40 promoter and enhancer. Relative luciferase activities were determined as described in (B).

Characterization of the functional promoter for CCR3 in human T cells.

(A) Map of the upstream region of the human CCR3 gene. Black boxes and angle dashed lines represent exons and splicing patterns, respectively. Exon 1 contains the main 5′ UTR part and exon 2 contains the ATG coding region. Grey arrows represent primers subsequently used for PCR in Figure 2A. H and K, respectively, indicate the position ofHindIII and KpnI sites. The 1, 2, and 3 located with gray lines indicate the regions analyzed by ChIP and DNaseI HS experiments. (B) Identification of the T-cell minimal promoter region for CCR3. Construct maps and data for relative luciferase expression in Jurkat human T cells (filled bars) and 721.221 human B cells (open bars). PCR fragments of variable sizes of the CCR3 5′-flanking region were generated and cloned in the Firefly luciferase pGL3 Basic vector. Exon 1 (gray box) and Luciferase (open box) are represented on the maps. Plasmids were transiently transfected by electroporation with a control plasmid pRL-TK (Renillaluciferase) into Jurkat and 721.221 cells. Relative luciferase activities of the cell lysates are representative of at least 5 independent experiments performed with different clones for each construct. Errors bars indicate SDs. (-) indicates not tested. (C) Identification of an NRE located in the flanking intronic region. An intronic PCR fragment (+134 to +237) was cloned either in sense (pGL3 C NRE S) or antisense orientation (pGL3 C NRE AS) into theFirefly luciferase vector pGL3 control containing the SV40 promoter and enhancer. Relative luciferase activities were determined as described in (B).

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal