한빛사논문
Geon-Woo Kima, Jae-Su Moonb, and Aleem Siddiquia,1
aDivision of Infectious Diseases and Public Global Health, Department of Medicine, University of California San Diego, La Jolla, CA 92093; and bDivision of Endocrinology and Metabolism, Department of Medicine, University of California San Diego, La Jolla, CA 92093
1To whom correspondence may be addressed.
Abstract
Hepatitis B virus (HBV) contains a partially double-stranded DNA genome. During infection, its replication is mediated by reverse transcription (RT) of an RNA intermediate termed pregenomic RNA (pgRNA) within core particles in the cytoplasm. An epsilon structural element located in the 5′ end of the pgRNA primes the RT activity. We have previously identified the N6-methyladenosine (m6A)–modified DRACH motif at 1905 to 1909 nucleotides in the epsilon structure that affects myriad functions of the viral life cycle. In this study, we investigated the functional role of m6A modification of the 5′ ε (epsilon) structural element of the HBV pgRNA in the nucleocapsid assembly. Using the m6A site mutant in the HBV 5′ epsilon, we present evidence that m6A methylation of 5′ epsilon is necessary for its encapsidation. The m6A modification of 5′ epsilon increased the efficiency of viral RNA packaging, whereas the m6A of 3′ epsilon is dispensable for encapsidation. Similarly, depletion of methyltransferases (METTL3/14) decreased pgRNA and viral DNA levels within the core particles. Furthermore, the m6A modification at 5′ epsilon of HBV pgRNA promoted the interaction with core proteins, whereas the 5′ epsilon m6A site–mutated pgRNA failed to interact. HBV polymerase interaction with 5′ epsilon was independent of m6A modification of 5′ epsilon. This study highlights yet another pivotal role of m6A modification in dictating the key events of the HBV life cycle and provides avenues for investigating RNA–protein interactions in various biological processes, including viral RNA genome encapsidation in the context of m6A modification.
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