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索非布韦(β-D-2'-脱氧-2'-α-氟-2'-β-C-甲基尿苷)作为抗登革病毒复制的抑制剂的评价<sup/>。

Evaluation of Sofosbuvir (β-D-2'-deoxy-2'-α-fluoro-2'-β-C-methyluridine) as an inhibitor of Dengue virus replication<sup/>.

机构信息

McGill University AIDS Centre, Lady Davis Institute for Medical Research, Jewish General Hospital, Montreal, Quebec, Canada.

Department of Microbiology and Immunology, McGill University, Montreal, Quebec, Canada.

出版信息

Sci Rep. 2017 Jul 24;7(1):6345. doi: 10.1038/s41598-017-06612-2.

Abstract

We evaluated Sofosbuvir (SOF), the anti-hepatitis C virus prodrug of β-d-2'-deoxy-2'-α-fluoro-2'-β-C-methyluridine-5'-monophosphate, for potential inhibitory activity against DENV replication. Both cell-based and biochemical assays, based on use of purified DENV full-length NS5 enzyme, were studied. Cytopathic effect protection and virus yield reduction assays confirmed that SOF possessed anti-DENV activity in cell culture with a 50% effective concentration (EC) of 4.9 µM and 1.4 µM respectively. Real-time RT-PCR verified that SOF inhibits generation of viral RNA with an EC of 9.9 µM. Purified DENV NS5 incorporated the active triphosphate form (SOF-TP) into nascent RNA, causing chain-termination. Relative to the natural UTP, the incorporation efficiency of SOF-TP was low (discrimination value = 327.5). In a primer extension assay, SOF-TP was active against DENV NS5 wild-type polymerase activity with an IC of 14.7 ± 2.5 µM. The S600T substitution in the B Motif of DENV polymerase conferred 4.3-fold resistance to SOF-TP; this was due to decreased incorporation efficiency rather than enhanced excision of the incorporated SOF nucleotide. SOF has antiviral activity against DENV replication. The high discrimination value in favor of UTP in enzyme assays may not necessarily preclude antiviral activity in cells. SOF may be worthy of evaluation against severe DENV infections in humans.

摘要

我们评估了 Sofosbuvir(SOF),一种抗丙型肝炎病毒的前药,是β-d-2'-脱氧-2'-α-氟-2'-β-C-甲基尿苷-5'-单磷酸的类似物,以评估其对 DENV 复制的潜在抑制活性。我们研究了基于使用纯化的 DENV 全长 NS5 酶的细胞和生化测定。细胞病变效应保护和病毒产量减少测定证实 SOF 在细胞培养中具有抗 DENV 活性,其 50%有效浓度(EC)分别为 4.9μM 和 1.4μM。实时 RT-PCR 验证 SOF 抑制病毒 RNA 的生成,其 EC 为 9.9μM。纯化的 DENV NS5 将活性三磷酸形式(SOF-TP)掺入新生 RNA 中,导致链终止。与天然 UTP 相比,SOF-TP 的掺入效率较低(区分值=327.5)。在引物延伸测定中,SOF-TP 对 DENV NS5 野生型聚合酶活性具有活性,IC 为 14.7±2.5μM。DENV 聚合酶 B 基序中的 S600T 取代赋予 SOF-TP 对其 4.3 倍的抗性;这是由于掺入效率降低,而不是掺入的 SOF 核苷酸的增强切除。SOF 对 DENV 复制具有抗病毒活性。酶测定中有利于 UTP 的高区分值不一定排除细胞中的抗病毒活性。SOF 可能值得针对人类严重 DENV 感染进行评估。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6a97/5524696/624e2ad12b71/41598_2017_6612_Fig1_HTML.jpg

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