Fig. 4.
Fig. 4. Physical association between GANP and MCM3. / (A) Association of MCM3 and GANP in cells in vivo. COS7 cells were transfected with complementary DNA (cDNA) constructs of both HA-MCM3 and FLAG-ganp. The NP-40 cell lysates were immunoprecipitated with anti-HA Ab, and Western blot analysis was carried out with anti-FLAG mAb to detect GANP. The transfectants with the single cDNA constructs were used as the negative control. (B) The cell lysate from WEHI-231 was immunoprecipitated with anti-GST, anti-GANP 42-23, or anti-MCM3 Ab. After separation by SDS-PAGE, the proteins were electrophoretically transferred to a membrane and probed with anti-MCM3 Ab. (C, left panel) In vitro kinase reactions were carried out with the anti-GANP immunoprecipitates washed with either NP-40 washing buffer or radioimmunoprotein-assay (RIPA) buffer. After the kinase reaction, the phosphorylated sample was washed further with the RIPA buffer and reimmunoprecipitated. The anti-GST immunoprecipitate was used as the negative control. (C, middle panel) Anti-GST, anti-GANP 42-23, and anti-MCM3 immunoprecipitates from WEHI-231 cell lysates were subjected to in vitro kinase assay. Normal rabbit serum was used as the control for anti-MCM3 Ab. The samples were separated by 7% SDS-PAGE. The bands corresponding to the sizes of GANP and MCM3 are indicated by arrows. (C, right panel) V8 cleavage mapping of 210-kd bands showed an identical cleavage pattern. As the control, an irrelevant V8-digested protein was separated in parallel. (D) Double staining with anti-MCM3 Ab and anti-CR1 mAb, or with PNA, was performed. The expression of MCM3 was up-regulated in the GC area.

Physical association between GANP and MCM3.

(A) Association of MCM3 and GANP in cells in vivo. COS7 cells were transfected with complementary DNA (cDNA) constructs of both HA-MCM3 and FLAG-ganp. The NP-40 cell lysates were immunoprecipitated with anti-HA Ab, and Western blot analysis was carried out with anti-FLAG mAb to detect GANP. The transfectants with the single cDNA constructs were used as the negative control. (B) The cell lysate from WEHI-231 was immunoprecipitated with anti-GST, anti-GANP 42-23, or anti-MCM3 Ab. After separation by SDS-PAGE, the proteins were electrophoretically transferred to a membrane and probed with anti-MCM3 Ab. (C, left panel) In vitro kinase reactions were carried out with the anti-GANP immunoprecipitates washed with either NP-40 washing buffer or radioimmunoprotein-assay (RIPA) buffer. After the kinase reaction, the phosphorylated sample was washed further with the RIPA buffer and reimmunoprecipitated. The anti-GST immunoprecipitate was used as the negative control. (C, middle panel) Anti-GST, anti-GANP 42-23, and anti-MCM3 immunoprecipitates from WEHI-231 cell lysates were subjected to in vitro kinase assay. Normal rabbit serum was used as the control for anti-MCM3 Ab. The samples were separated by 7% SDS-PAGE. The bands corresponding to the sizes of GANP and MCM3 are indicated by arrows. (C, right panel) V8 cleavage mapping of 210-kd bands showed an identical cleavage pattern. As the control, an irrelevant V8-digested protein was separated in parallel. (D) Double staining with anti-MCM3 Ab and anti-CR1 mAb, or with PNA, was performed. The expression of MCM3 was up-regulated in the GC area.

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