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Identification of Members of the Protein Phosphatase 1 Gene Family in the Rat and Enhanced Expression of Protein Phosphatase 1α Gene in Rat Hepatocellular Carcinomas

机译:大鼠磷酸化酶1基因家族成员的鉴定及大鼠肝细胞癌中磷酸化酶1α基因的增强表达

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摘要

We isolated four kinds of cDNA clones of isotypes of catalytic subunits of protein phosphatase >1 (PP‐1) from rat liver and testis cDNA libraries. For the cloning, cDNA fragments of dis2ml and dis2m2, which encode mouse PP‐1 catalytic subunits, were used as probes. Two of the four isotypes were thought to be derived from the same gene and produced by alternative splicing. Based on the comparative study of their nucleotide and deduced amino acid sequences with those reported, these cDNA clones were named rat PP‐1α, PP‐1γ1, PP‐1γ2 and PP‐δ. The deduced amino acid sequences of these four cDNA clones showed about 90% identity. Their amino‐terminal regions were highly conserved, and their differences were mainly in the carboxy‐terminal regions. Furthermore, several amino acids located in the middle regions of the peptides were conserved in all the isotypes of the catalytic subunits of PP‐1, PP‐2A, PP‐2B and PP‐2C. These conserved regions are suggested to be the functional domains of the catalytic subunits of protein phosphatases. Rat hepatocellular carcinomas induced by a food mutagen, 2‐amino‐3,8‐dimethylimidazo[4,5‐f]quinoxaline showed increased expression of PP‐1α, but no increased expression of PP‐1γ1, PP‐1γ2 or PP‐1δ. Involvement of PP‐1α in hepatocarcinogenesis or in hepatic cell proliferation was suspected.
机译:我们从大鼠肝脏和睾丸cDNA文库中分离了4种蛋白磷酸酶> 1 (PP-1)催化亚基同型的cDNA克隆。为了克隆,使用编码小鼠PP-1催化亚基的dis2ml和dis2m2 cDNA片段作为探针。四个同种型中的两个被认为源自相同的基因,并通过选择性剪接产生。根据与已报道的核苷酸和推导氨基酸序列的比较研究,这些cDNA克隆被命名为大鼠PP-1α,PP-1γ1,PP-1γ2和PPδ。这四个cDNA克隆的推导的氨基酸序列显示出约90%的同一性。它们的氨基末端区域是高度保守的,它们的差异主要在羧基末端区域。此外,位于肽中间区域的几个氨基酸在PP-1,PP-2A,PP-2B和PP-2C催化亚基的所有同种型中都是保守的。这些保守的区域被认为是蛋白质磷酸酶催化亚基的功能域。食物诱变剂2-氨基-3,8-二甲基咪唑并[4,5-f]喹喔啉诱导的大鼠肝细胞癌中PP-1α的表达增加,但PP-1γ1,PP-1γ2或PP-1δ的表达没有增加。怀疑PP-1α参与肝癌发生或肝细胞增殖。

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