Identification of novel human adenovirus candidates using the coxsackievirus and adenovirus receptor for cell entry

被引:6
作者
Mese, Kemal [1 ]
Bunz, Oskar [1 ]
Schellhorn, Sebastian [1 ]
Volkwein, Wolfram [2 ]
Jung, Dominik [1 ]
Gao, Jian [1 ]
Zhang, Wenli [1 ]
Baiker, Armin [2 ]
Ehrhardt, Anja [1 ]
机构
[1] Witten Herdecke Univ, Inst Virol & Microbiol, Ctr Biomed Educ & Res ZBAF, Stockumer Str 10, D-58453 Witten, Germany
[2] Bavarian Hlth & Food Safety Author LGL, Oberschleissheim, Germany
关键词
Adenovirus; Luciferase; Virus library; Receptor; CAR; USES SIALIC-ACID; SEROTYPES; 3; BINDING; CD46;
D O I
10.1186/s12985-020-01318-w
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
Background There are over 100 known human adenovirus (HAdV) types, which are able to cause a broad variety of different self-limiting but also lethal diseases especially in immunocompromised patients. Only limited information about the pathogenesis and biology of the majority of these virus types is available. In the present study, we performed a systematic screen for coxsackievirus and adenovirus receptor (CAR)-usage of a large spectrum of HAdV types. Methods To study receptor usage we utilized a recombinant HAdV library containing HAdV genomes tagged with a luciferase and GFP encoding transgene. We infected CHO-CAR cells stably expressing the CAR receptor and to much information with tagged viruses (HAdV3, 14, 16, 50, 10, 24, 27, 37 and 69) and measured luciferase expression levels 26 and for some viruses (AdV10, - 24 and - 27) 52 h post-infection. As positive control, we applied human adenovirus type 5 (HAdV5) known to use the CAR receptor for cell entry. For viruses replication studies on genome level we applied digital PCR. Results Infection of CHO-CAR and CHO-K1 cells at various virus particle numbers per cell (vpc) revealed that HAdV10, 24, and 27 showed similar or decreased luciferase expression levels in the presence of CAR. In contrast, HAdV3, 14, 16, 50, 37 and 69 resulted in increased luciferase expression levels in our initial screening experiments. CAR usage of HAdV3, 14, 50, and 69 was not studied before, and therefore we experimentally confirmed CAR usage for these HAdV as novel viruses utilizing CAR as a receptor. To rule out that replication of HAdV in transduced CHO cells is responsible for increased transduction rates we performed replication assays on virus genome level, which revealed that there is no HAdV replication. Conclusion In the present study, we screened a HAdV library and identified novel human HAdV using the CAR receptor. To our knowledge, this is the first description of CAR usage for HAdV 3, 14, 50, and 69.
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页数:7
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