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果蝇酸性脱氧核糖核酸酶是哺乳动物脱氧核糖核酸酶II的同源物。

Drosophila acid DNase is a homolog of mammalian DNase II.

作者信息

Evans Cory J, Merriam John R, Aguilera Renato J

机构信息

Department of Molecular, Cell and Developmental Biology, University of California, Los Angeles, CA 90095, USA.

出版信息

Gene. 2002 Jul 24;295(1):61-70. doi: 10.1016/s0378-1119(02)00819-3.

Abstract

Mammalian DNase II enzymes and the Caenorhabditis elegans homolog NUC-1 have recently been shown to be critically important during engulfment-mediated clearance of DNA. In this report, we describe the cloning and characterization of the gene encoding Drosophila DNase II. Database queries using the C. elegans NUC-1 protein sequence identified a highly homologous open reading frame in Drosophila (CG7780) that could encode a similar enzyme. Analysis of crude protein extracts revealed that wild-type Drosophila contain a potent acid endonuclease activity with cleavage preferences similar to DNase II/NUC1, while the same activity was markedly reduced in an acid DNase hypomorphic mutant line. Furthermore, the pattern of cleavage products generated from an end-labeled substrate by hypomorphic-line extracts was significantly altered in comparison to the pattern generated by wild-type extracts. Sequence analysis of CG7780 DNA and mRNA revealed that the hypomorphic line contains a missense mutation within the coding region of this gene. Additionally, Northern analysis demonstrated that CG7780 expression is normal in the mutant line, which in combination with the lowered/altered enzymatic activity and sequencing data suggested a defect in the CG7780 protein. To conclusively determine if CG7780 encoded the Drosophila equivalent of DNase II/NUC-1, transgenic lines expressing wild-type CG7780 in the mutant background were generated and subsequently shown to complement the mutant phenotype. Our results, therefore, provide compelling evidence that the predicted gene CG7780 encodes Drosophila DNase II (dDNase II), an enzyme related in sequence and activity to mammalian DNase II. Interestingly, overexpression of CG7780 both ubiquitously and in specific tissues failed to elicit any discernable phenotype.

摘要

最近研究表明,哺乳动物的脱氧核糖核酸酶II(DNase II)以及秀丽隐杆线虫的同源物NUC-1在DNA的吞噬介导清除过程中至关重要。在本报告中,我们描述了果蝇DNase II编码基因的克隆与特性分析。利用秀丽隐杆线虫NUC-1蛋白序列进行数据库查询,在果蝇中鉴定出一个高度同源的开放阅读框(CG7780),它可能编码一种类似的酶。对粗蛋白提取物的分析显示,野生型果蝇含有一种强大的酸性核酸内切酶活性,其切割偏好与DNase II/NUC1相似,而在酸性DNase功能减弱的突变品系中,相同活性明显降低。此外,与野生型提取物产生的切割产物模式相比,功能减弱品系提取物从末端标记底物产生的切割产物模式发生了显著改变。对CG7780 DNA和mRNA的序列分析表明,功能减弱品系在该基因的编码区域内存在一个错义突变。此外,Northern分析表明,CG7780在突变品系中的表达正常,这与降低/改变的酶活性和测序数据相结合,提示CG7780蛋白存在缺陷。为了最终确定CG7780是否编码果蝇的DNase II/NUC-1等同物,构建了在突变背景下表达野生型CG7780的转基因品系,随后证明其能够补充突变表型。因此,我们的结果提供了令人信服的证据,即预测基因CG7780编码果蝇DNase II(dDNase II),一种在序列和活性上与哺乳动物DNase II相关的酶。有趣的是,CG7780在全身和特定组织中的过表达均未引发任何可识别的表型。

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