Haystead C M, Gailly P, Somlyo A P, Somlyo A V, Haystead T A
Department of Pharmacology, University of Virginia Health Sciences Center, Charlottesville 22908, USA.
FEBS Lett. 1995 Dec 18;377(2):123-7. doi: 10.1016/0014-5793(95)01318-0.
We have cloned a partial rat kidney cDNA that encodes a 72.5 kDa N terminal fragment of a third isoform of the M110 subunit of phosphatase 1. This new isoform contains an insert in the 542-597 position not present in the M110 previously cloned (Chen et al. (1994) FEBS Lett. 356, 51-55) from the same species. The encoded cDNA was expressed as a soluble GST-fusion protein in E. coli, and its ability to interact with native PP-1C was measured both in vitro and in permeabilized smooth muscle. In vitro, the fusion protein was capable of selectively binding PP-1C and increasing the substrate specificity of the phosphatase towards myosin 13.2 +/- 3.5-fold (S.E. of the mean, n = 3). In permeabilized smooth muscle pretreated with microcystin, the recombinant protein alone (1.0 microM) did not cause relaxation, but did significantly enhance the ability of PP-1C (0.3 microM) to relax the muscle. These findings show that the N terminal domain of the M110 subunit is the primary site for both PP-1C and myosin binding, and thereby determines myosin specificity. The presence of isoformic variation within this sequence may permit organ/cell specific regulation of phosphorylation sites.
我们克隆了一段大鼠肾脏cDNA,它编码磷酸酶1的M110亚基第三种同工型的72.5 kDa N端片段。这种新的同工型在542 - 597位含有一个插入序列,而之前从同一物种克隆的M110(Chen等人,(1994) FEBS Lett. 356, 51 - 55)中不存在该序列。编码的cDNA在大肠杆菌中表达为可溶性GST融合蛋白,并在体外和通透化的平滑肌中检测其与天然PP - 1C相互作用的能力。在体外,融合蛋白能够选择性结合PP - 1C,并使磷酸酶对肌球蛋白的底物特异性增加13.2 +/- 3.5倍(平均值的标准误,n = 3)。在用微囊藻毒素预处理的通透化平滑肌中,单独的重组蛋白(1.0 microM)不会引起舒张,但能显著增强PP - 1C(0.3 microM)舒张肌肉的能力。这些发现表明,M110亚基的N端结构域是PP - 1C和肌球蛋白结合的主要位点,从而决定了肌球蛋白的特异性。该序列中同工型变异的存在可能允许对磷酸化位点进行器官/细胞特异性调节。
