Comprehensive analysis of human cytomegalovirus microRNA expression during lytic and quiescent infection

Zhang-Zhou Shen; Xing Pan; Ling-Feng Miao; Han-Qing Ye; Stéphane Chavanas; Christian Davrinche; Michael McVoy; Min-Hua Luo

doi:10.1371/journal.pone.0088531

Comprehensive analysis of human cytomegalovirus microRNA expression during lytic and quiescent infection

PLoS One. 2014 Feb 12;9(2):e88531. doi: 10.1371/journal.pone.0088531. eCollection 2014.

Authors

Zhang-Zhou Shen¹, Xing Pan¹, Ling-Feng Miao¹, Han-Qing Ye¹, Stéphane Chavanas², Christian Davrinche², Michael McVoy³, Min-Hua Luo¹

Affiliations

¹ State Key Laboratory of Virology, Wuhan Institute of Virology, Chinese Academy of Sciences, Wuhan, Hubei, China.
² INSERM-U1043/CNRS-U5282/Paul Sabatier University, Toulouse, France.
³ Department of Pediatrics, Virginia Commonwealth University, School of Medicine, Richmond, Virginia, United States of America.

Abstract

Background: Human cytomegalovirus (HCMV) encodes microRNAs (miRNAs) that function as post-transcriptional regulators of gene expression during lytic infection in permissive cells. Some miRNAs have been shown to suppress virus replication, which could help HCMV to establish or maintain latent infection. However, HCMV miRNA expression has not been comprehensively examined and compared using cell culture systems representing permissive (lytic) and semi-permissive vs. non-permissive (latent-like) infection.

Methods: Viral miRNAs levels and expression kinetics during HCMV infection were determined by miRNA-specific stem-loop RT-PCR. HCMV infected THP-1 (non-permissive), differentiated THP-1 (d-THP-1, semi-permissive) and human embryo lung fibroblasts (HELs, fully-permissive) were examined. The impact of selected miRNAs on HCMV infection (gene expression, genome replication and virus release) was determined by Western blotting, RT-PCR, qPCR, and plaque assay.

Results: Abundant expression of 15 HCMV miRNAs was observed during lytic infection in HELs; highest peak inductions (11- to 1502-fold) occurred at 48 hpi. In d-THP-1s, fourteen mRNAs were detected with moderate induction (3- to 288-fold), but kinetics of expression was generally delayed for 24 h relative to HELs. In contrast, only three miRNAs were induced to low levels (3- to 4-fold) during quiescent infection in THP-1s. Interestingly, miR-UL70-3p was poorly induced in HEL (1.5-fold), moderately in THP-1s (4-fold), and strongly (58-fold) in d-THP-1s, suggesting a potentially specific role for miR-UL70-3p in THP-1s and d-THP-1s. MiR-US33, -UL22A and -UL70 were further evaluated for their impact on HCMV replication in HELs. Ectopic expression of miR-UL22A and miR-UL70 did not affect HCMV replication in HELs, whereas miR-US33 inhibited HCMV replication and reduced levels of HCMV US29 mRNA, confirming that US29 is a target of miR-US33.

Conclusions: Viral miRNA expression kinetics differs between permissive, semi-permissive and quiescent infections, and miR-US33 down-regulates HCMV replication. These results suggest that miR-US33 may function to impair entry into lytic replication and hence promote establishment of latency.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cell Line
Cytomegalovirus / genetics*
Cytomegalovirus / physiology
Cytomegalovirus Infections / virology
Gene Expression Profiling*
Gene Expression Regulation, Viral*
Humans
Kinetics
Lentivirus / genetics
MicroRNAs / metabolism*
Plasmids / metabolism
RNA, Viral / metabolism*
Virus Replication / genetics

Substances

MicroRNAs
RNA, Viral

Grants and funding

This work was supported by the National Program on Key Basic Research Project (973 program 2011CB504804 and 2012CB519003), the National Natural Science Foundation of China (81071350, 81271850, 31170155, and 31000090), and the Scientific Innovation Project of the Chinese Academy of Sciences (XDB02050500, XDA0104107). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.