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EXPRESSION AND FUNCTIONAL CHARACTERIZATION OF ISOFORMS 4 OF THE PLASMA MEMBRANE CALCIUM PUMP

机译:等离子体膜钙泵的同工型4的表达和功能表征

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PMCA isoforms 4CII (generated by splicing at the C-terminus) and 4BICI (a pump version lacking the 10th transmembrane domain) were expressed in Sf9 cells using the baculovirus system. The purified PMCA4CII had a 20-fold lower affinity for calmodulin than the PMCA4CI, the PMCA4 isoform of the erythrocytes' membranes, but had a higher activity in the absence of calmodulin. The amount of phosphoenzyme intermediate formed by PMCA4CII in the presence of Ca2+ alone was almost 3 times higher than in PMCA I CI and was increased by La3+ less than in the PMCA4CI. The isoform lacking the 10th transmembrane domain (PMCA4BICI) had no Ca2+-dependent ATPase activity, but was still able to form the phosphoenzyme intermediate starting from phosphate. When expressed in COS cells, this isoform was retained in the endoplasmic reticulum; changes in membrane architecture apparently occurred during its expression; the C-terminal portion of the isoform was located in the cytosol, indicating that the deletion of the 10(th) transmembrane domain resulted in the loss of at least another transmembrane domain.
机译:使用杆状病毒系统,在Sf9细胞中表达了PMCA亚型4CII(通过在C端剪接生成)和4BICI(缺少第10个跨膜结构域的泵版本)。纯化的PMCA4CII对钙调蛋白的亲和力比红细胞膜PMCA4同工型PMCA4CI低20倍,但在没有钙调蛋白的情况下具有更高的活性。仅在Ca2 +存在下,PMCA4CII形成的磷酸酶中间体的量几乎是PMCA I CI的3倍,而La3 +的增加量则少于PMCA4CI。缺少第10个跨膜结构域(PMCA4BICI)的同工型没有依赖Ca2 +的ATPase活性,但仍然能够从磷酸盐开始形成磷酸酶中间体。当在COS细胞中表达时,这种同工型保留在内质网中。膜结构的变化显然在其表达过程中发生;同工型的C-末端部分位于胞质溶胶中,表明第10个跨膜结构域的缺失导致至少另一个跨膜结构域的丧失。

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