Identification of virion-associated transcriptional transactivator (VATT) of SGIV ICP46 promoter and their binding site on promoter

Li-Qun Xia; Jian-Lin Chen; Hong-Lian Zhang; Jia Cai; Sheng Zhou; Yi-Shan Lu

doi:10.1186/s12985-019-1210-0

Virology Journal (Sep 2019)

Identification of virion-associated transcriptional transactivator (VATT) of SGIV ICP46 promoter and their binding site on promoter

Li-Qun Xia,
Jian-Lin Chen,
Hong-Lian Zhang,
Jia Cai,
Sheng Zhou,
Yi-Shan Lu

Affiliations

Li-Qun Xia: Shenzhen Institute of Guangdong Ocean University
Jian-Lin Chen: Shenzhen Institute of Guangdong Ocean University
Hong-Lian Zhang: Shenzhen Institute of Guangdong Ocean University
Jia Cai: Shenzhen Institute of Guangdong Ocean University
Sheng Zhou: Guangdong Provincial Key Laboratory of Pathogenic Biology and Epidemiology for Aquatic Economic Animal, Guangdong Ocean University
Yi-Shan Lu: Shenzhen Institute of Guangdong Ocean University

DOI: https://doi.org/10.1186/s12985-019-1210-0
Journal volume & issue: Vol. 16, no. 1
pp. 1 – 14

Abstract

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Abstract Background Iridoviruses are large DNA viruses that cause diseases in fish, amphibians and insects. Singapore grouper iridovirus (SGIV) is isolated from cultured grouper and characterized as a ranavirus. ICP46 is defined to be a core gene of the family Iridoviridae and SGIV ICP46 was demonstrated to be an immediate-early (IE) gene associated with cell growth control and could contribute to virus replication in previous research. Methods The transcription start site (TSS) and 5′-untranslated region (5′-UTR) of SGIV ICP46 were determined using 5′ RACE. The core promoter elements of ICP46s were analyzed by bioinformatics analysis. The core promoter region and the regulation model of SGIV ICP46 promoter were revealed by the construction of serially deleted promoter plasmids, transfections, drug treat and luciferase reporter assays. The identification of virion-associated transcriptional transactivator (VATT) that interact with SGIV ICP46 promoter and their binding site on promoter were performed by electrophoretic mobility shift assays (EMSA), DNA pull-down assays and mass spectrometry (MS). Results SGIV ICP46 was found to have short 5′-UTR and a presumptive downstream promoter element (DPE), AGACA, which locates at + 36 to + 39 nt downstream of the TSS. The core promoter region of SGIV ICP46 located from − 22 to + 42 nt relative to the TSS. VATTs were involved in the promoter activation of SGIV ICP46 and further identified to be VP12, VP39, VP57 and MCP. A 10-base DNA sequence “ATGGCTTTCG” between the TSS and presumptive DPE was determined to be the binding site of the VATTs. Conclusion Our study showed that four VAATs (VP12, VP39, VP57 and MCP) might bind with the SGIV ICP46 promoter and be involved in the promoter activation. Further, the binding site of the VATTs on promoter was a 10-base DNA sequence between the TSS and presumptive DPE.

Published in Virology Journal

ISSN: 1743-422X (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Internal medicine: Infectious and parasitic diseases
Website: http://virologyj.biomedcentral.com

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