| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 2067536 | Cell Biology International | 2008 | 6 Pages |
Abstract
Cyclic AMP-dependent proteolysis of GATA-6 was characterized by fusing GATA-6 with the carboxyl-terminal membrane domain of SREBP-2. When the fusion protein was stably expressed in CHO-K1 cells, it was recovered in the ER membrane. This protein was processed in a similar manner to SREBP-2 upon cholesterol starvation, and the GATA-6 moiety moved into the nucleus. The GATA-6 moiety on the membrane became undetectable in the presence of dbcAMP or cholera toxin. However, H-89, K-252a, MG115 and lactacystin inhibited this decrease, suggesting that the cytoplasmic GATA-6 moiety of the fusion protein was degraded by proteasomes though A-kinase upon elevation of the cellular cAMP concentration.
Keywords
PBS-TMG115A-kinaseGATA-6H-89CHO-K1dibutyryl cAMPTRISSREBPdbcAMPEEA1PDIPMSFhsp70PBSSDSHEPES4-(2-hydroxyethyl)-1-piperazineethane-sulfonic acidBSAcAMPDMSObovine serum albuminearly endosomal antigen 1immunoglobulin Dimethyl sulfoxidesodium dodecyl sulfateendoplasmic reticulumDIGphenylmethylsulfonyl fluorideProteolysisSterol regulatory element-binding proteinprotein disulfide isomeraseheat shock protein 70
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Authors
Takeshi Tsuge, Kae Uetani, Ryuichiro Sato, Ayako Ohashi-Kobayashi, Masatomo Maeda,