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Multiple splice variants of phosphodiesterase PDE4C cloned from human lung and testis

机译:从人肺和睾丸中克隆出磷酸二酯酶PDE4C的多个剪接变体

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Four closely related cyclic-nucleotide specific phosphodiesterase (PDE4) genes have been identified in both humans and rats: PDE4A, 4B, 4C and 4D. We have now cloned cDNAs for multiple splice variants of human PDE4C. Two splice variants, PDE4C-791 and PDE4C-426, were isolated from a fetal lung library. The longest open reading frame (ORF) of 791 amino acids (aa) is encoded by PDE4C-791, which is similar to a recently described cDNA [Engels, P., Sullivan, M., Muller, T. and Lübbert, H. FEBS Lett. 358 (1995) 305–10], except that an alternative 5′-end sequence upstream of the first methionine extends the PDE4C-791 ORF by 79 aa. The PDE4C-426 variant contains 3 insertions that are located 5′ to the catalytic domain and encode several in-frame stop codons. The predicted 426 aa protein initiates at a methionine 365 aa within PDE4C-791. A baculovirus clone starting at this methionine expressed an enzymatically active protein. Two additional splice variants, PDE4C-Δ54 and PDE4C-Δ109, were found in testis mRNA. PDE4C-Δ54 contained a novel 5′-end region and a deletion of 162 nt; the predicted protein deletes 54 aa from the amino-terminal region. The PDE4C-Δ54 protein produced in baculovirus-infected cells was enzymatically active and sensitive to PDE4-specific inhibitors. The PDE4C-Δ109 protein is similar to PDE4C-Δ54 but has an additional 55 aa deleted in the catalytic domain; it lacked enzymatic activity. Analysis of uncloned total mRNA from 4 tissue sources by polymerase chain reaction (PCR) confirmed the presence of mRNAs with the two deletions and three insertions that we observed in cDNA clones. The PDE4C-Δ54 variant was found only in testis and the 5′-extended region of PDE4C-791 was seen only in lung and the melanoma cell line G361. Hence, tissue-specific expression of various PDE4C isoforms should be considered in understanding how these gene products modulate cellular responses to cAMP.
机译:已在人类和大鼠中鉴定出四个紧密相关的环状核苷酸特异性磷酸二酯酶(PDE4)基因:PDE4A,4B,4C和4D。我们现在已经克隆了人类PDE4C多个剪接变体的cDNA。从胎儿肺文库中分离出两个剪接变体PDE4C-791和PDE4C-426。最长的791个氨基酸(aa)的开放阅读框(ORF)由PDE4C-791编码,与最近描述的cDNA相似[Engels,P.,Sullivan,M.,Muller,T. andLübbert,H. FEBS Lett。 358(1995)305-10],只是在第一个蛋氨酸上游的另一5'-末端序列使PDE4C-791 ORF延伸了79aa。 PDE4C-426变体包含3个插入,位于催化结构域的5'端,并编码几个框内终止密码子。预测的426aa蛋白起始于PDE4C-791中的甲硫氨酸365aa。从该蛋氨酸开始的杆状病毒克隆表达了一种酶活性蛋白。在睾丸mRNA中发现了另外两个剪接变体PDE4C-Δ54和PDE4C-Δ109。 PDE4C-Δ54含有一个新的5'末端区域和一个162 nt的缺失。预测的蛋白质从氨基末端区域删除了54个氨基酸。在杆状病毒感染的细胞中产生的PDE4C-Δ54蛋白具有酶活性,并且对PDE4特异性抑制剂敏感。 PDE4C-Δ109蛋白与PDE4C-Δ54相似,但在催化域中缺失了55个氨基酸;它缺乏酶活性。通过聚合酶链反应(PCR)分析来自4个组织来源的未克隆总mRNA,证实了我们在cDNA克隆中观察到的带有两个缺失和三个插入的mRNA。 PDE4C-Δ54变异仅在睾丸中发现,PDE4C-791的5'延伸区仅在肺和黑色素瘤细胞系G361中可见。因此,在理解这些基因产物如何调节细胞对cAMP的反应时,应考虑各种PDE4C亚型的组织特异性表达。

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