Ding Chuantian, Urabe Masashi, Bergoin Max, Kotin Robert M
Laboratory of Biochemical Genetics, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, Maryland 20892-1654, USA.
J Virol. 2002 Jan;76(1):338-45. doi: 10.1128/jvi.76.1.338-345.2002.
Junonia coenia densovirus (JcDNV) is an autonomous parvovirus that infects the larvae of the common buckeye butterfly, Junonia coenia. Unlike vertebrate parvoviruses, the genes encoding the structural protein and nonstructural (NS) proteins of JcDNV are in opposite orientations; thus, each strand contains a sense and antisense open reading frame (ORF). The promoter at map position 93 controls expression of NS ORFs 2, 3, and 4, which encode three NS proteins, NS-1, NS-2, and NS-3. These proteins are likely to be involved in viral DNA replication, among other functions. In contrast to the nonstructural proteins of the vertebrate parvoviruses, the NS proteins of the Densovirinae have not been characterized. Here, we describe biochemical properties of the NS-1 protein of JcDNV. The NS-1 ORF was cloned in frame with the Escherichia coli malE gene, which encodes the bacterial maltose binding protein (MBP). Using electrophoretic mobility shift and DNase I protection assays, we identified the region of the JcDNV terminal sequence that is recognized specifically by the MBP-NS-1 fusion protein. The site consists of (GAC)4 and is located on the A-A' region of the terminal palindrome. In addition, the MBP-NS-1 fusion protein catalyzes the cleavage of single-stranded DNA (ssDNA) substrates derived from the JcDNV putative origin of replication, primarily at two sites in the motif 5'-GTATTG-3'. One cleavage site is between the thymidine dinucleotide at positions 92 and 93 and the other site corresponds to thymidine at nucleotide 95; both sites are on the complementary strand of the sequence assigned GenBank accession number A12984. Cleavage of ssDNA is dependent on the presence of a divalent metal cofactor but does not require nucleoside triphosphate hydrolysis. Parvovirus NS proteins contain the phylogenically conserved Walker A- and B-site ATPase motifs. These sites in JcDNV NS-1 diverge from the consensus, yet despite these atypical motifs our analyses support that MBP-NS-1 has ATP-dependent helicase activity. These results indicate that JcDNV NS-1 possesses activities common to the superfamily of rolling-circle replication initiator proteins in general and the parvovirus replication proteins in particular, and they provide a basis for comparative analyses of the structure and function relationships among the parvovirus NS-1 equivalents.
苎麻珍蝶浓病毒(JcDNV)是一种自主细小病毒,可感染苎麻珍蝶(Junonia coenia)的幼虫。与脊椎动物细小病毒不同,JcDNV编码结构蛋白和非结构(NS)蛋白的基因方向相反;因此,每条链都包含一个正义和反义开放阅读框(ORF)。图谱位置93处的启动子控制NS ORF 2、3和4的表达,它们编码三种NS蛋白,即NS-1、NS-2和NS-3。这些蛋白可能参与病毒DNA复制以及其他功能。与脊椎动物细小病毒的非结构蛋白不同,浓病毒亚科的NS蛋白尚未得到表征。在此,我们描述了JcDNV的NS-1蛋白的生化特性。NS-1 ORF与编码细菌麦芽糖结合蛋白(MBP)的大肠杆菌malE基因框内克隆。使用电泳迁移率变动分析和DNase I保护分析,我们确定了JcDNV末端序列中被MBP-NS-1融合蛋白特异性识别的区域。该位点由(GAC)4组成,位于末端回文的A - A'区域。此外,MBP-NS-1融合蛋白催化源自JcDNV假定复制起点的单链DNA(ssDNA)底物的切割,主要在基序5'-GTATTG-3'的两个位点。一个切割位点在92和93位的胸腺嘧啶二核苷酸之间,另一个位点对应于95位的胸腺嘧啶;这两个位点都在GenBank登录号为A12984的序列的互补链上。ssDNA的切割依赖于二价金属辅因子的存在,但不需要核苷三磷酸水解。细小病毒NS蛋白包含系统发育上保守的沃克A和B位点ATP酶基序。JcDNV NS-1中的这些位点与共识不同,然而尽管有这些非典型基序,我们的分析支持MBP-NS-1具有ATP依赖性解旋酶活性。这些结果表明,JcDNV NS-1具有一般滚环复制起始蛋白超家族特别是细小病毒复制蛋白共有的活性,并且它们为细小病毒NS-1等同物之间的结构和功能关系的比较分析提供了基础。
