Program in Emerging Infectious Diseases, DUKE-NUS Graduate Medical School, Singapore, Singapore.
PLoS Negl Trop Dis. 2010 Nov 9;4(11):e881. doi: 10.1371/journal.pntd.0000881.
The enzyme activities catalysed by flavivirus non-structural protein 3 (NS3) are essential for virus replication. They are distributed between the N-terminal protease domain in the first one-third and the C-terminal ATPase/helicase and nucleoside 5' triphosphatase domain which forms the remainder of the 618-aa long protein.
METHODOLOGY/PRINCIPAL FINDINGS: In this study, dengue full-length NS3 protein with residues 49 to 66 of NS2B covalently attached via a flexible linker, was used as bait in biopanning with a naïve human Fab phage-display library. Using a range of truncated constructs spanning the NS2B cofactor region and the full-length NS3, 10 unique Fab were identified and characterized. Of these, monoclonal Fab 3F8 was shown to bind α3″ (residues 526 through 531) within subdomain III of the helicase domain. The antibody inhibits the ATPase and helicase activites of NS3 in biochemical assays and reduces DENV replication in HEK293 cells that were previously transfected with Fab 3F8 compared with mock transfected cells.
CONCLUSIONS/SIGNIFICANCE: Antibodies such as 3F8 are valuable tools for studying the molecular mechanisms of flaviviral replication and for the monospecific detection of replicating dengue virus in vivo.
黄病毒非结构蛋白 3(NS3)催化的酶活性对病毒复制至关重要。它们分布在 N 端蛋白酶结构域的前三分之一和 C 端 ATP 酶/解旋酶和核苷 5'三磷酸酶结构域之间,该结构域形成 618 个氨基酸长的蛋白质的其余部分。
方法/主要发现:在这项研究中,使用全长 NS3 蛋白(NS2B 的残基 49 到 66 之间通过柔性接头共价连接)作为诱饵,通过幼稚的人类 Fab 噬菌体展示文库进行生物淘选。使用跨越 NS2B 辅助因子区域和全长 NS3 的一系列截断构建体,鉴定并表征了 10 个独特的 Fab。其中,单克隆 Fab 3F8 被证明与螺旋酶结构域的亚结构域 III 内的 α3″(残基 526 到 531)结合。该抗体在生化测定中抑制 NS3 的 ATP 酶和解旋酶活性,并降低先前用 Fab 3F8 转染的 HEK293 细胞中的 DENV 复制,与模拟转染细胞相比。
结论/意义:像 3F8 这样的抗体是研究黄病毒复制的分子机制和在体内单特异性检测复制性登革热病毒的有价值的工具。
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