Figure 3
Figure 3. Transfection of AQP9 into Hep3B and K562 cells. (A) K562EGFP-C2 cells examined under fluorescent microscopy showed even cellular distribution of green fluorescence; however, K562EGFR-AQP9 cells showed selective localization of green fluorescence to the plasma membrane. Images were visualized using an Olympus IX70 microscope equipped with a C plan semi-apochromat 60×/0.7 numerical aperture lens (Olympus, Tokyo, Japan). A Nikon Coolpix 4500 camera (Nikon, Tokyo, Japan) was used to capture the images. (B) Western-blot analysis of Hep3B cells. In anti-GFP immunoblotting, EGFP (30 kDa) and EGFP-AQP9 (61 kDa) were detected in Hep3BEGFP and Hep3BEGFP-AQP9 cells, respectively. With anti-AQP9 immunoblotting, only the protein band of EGFP-AQP9 (61 kDa) was detected in Hep3BEGFP-AQP9 cells, showing that Hep3BEGFP cells did not express detectable levels of AQP9. (C) Western-blot analysis of K562 cells. In anti-GFP immunoblotting, protein bands of EGFP (30 kDa) and EGFP-AQP9 (61 kDa) were detected in K562EGFP and K562EGFP-AQP9 cells. An additional band (30-31 kDa) was observed in the K562EGFP-AQP9 sample. This might be due to degradation of EGFP-AQP9 fusion protein into EGFP and AQP9 fractions. In anti-AQP9 immunoblotting, a predominant band of EGFP-AQP9 (61 kDa) was detected in K562EGFP-AQP9 cells. At the anti-AQP9 antibody concentration and exposure time used to avoid overexposure of the K562EGFP-AQP9 lysate, K562EGFR lysate did not show detectable AQP9, as was shown previously in Figure 2.

Transfection of AQP9 into Hep3B and K562 cells. (A) K562EGFP-C2 cells examined under fluorescent microscopy showed even cellular distribution of green fluorescence; however, K562EGFR-AQP9 cells showed selective localization of green fluorescence to the plasma membrane. Images were visualized using an Olympus IX70 microscope equipped with a C plan semi-apochromat 60×/0.7 numerical aperture lens (Olympus, Tokyo, Japan). A Nikon Coolpix 4500 camera (Nikon, Tokyo, Japan) was used to capture the images. (B) Western-blot analysis of Hep3B cells. In anti-GFP immunoblotting, EGFP (30 kDa) and EGFP-AQP9 (61 kDa) were detected in Hep3BEGFP and Hep3BEGFP-AQP9 cells, respectively. With anti-AQP9 immunoblotting, only the protein band of EGFP-AQP9 (61 kDa) was detected in Hep3BEGFP-AQP9 cells, showing that Hep3BEGFP cells did not express detectable levels of AQP9. (C) Western-blot analysis of K562 cells. In anti-GFP immunoblotting, protein bands of EGFP (30 kDa) and EGFP-AQP9 (61 kDa) were detected in K562EGFP and K562EGFP-AQP9 cells. An additional band (30-31 kDa) was observed in the K562EGFP-AQP9 sample. This might be due to degradation of EGFP-AQP9 fusion protein into EGFP and AQP9 fractions. In anti-AQP9 immunoblotting, a predominant band of EGFP-AQP9 (61 kDa) was detected in K562EGFP-AQP9 cells. At the anti-AQP9 antibody concentration and exposure time used to avoid overexposure of the K562EGFP-AQP9 lysate, K562EGFR lysate did not show detectable AQP9, as was shown previously in Figure 2.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal