Human parvovirus B19 causes cell cycle arrest of human erythroid progenitors via deregulation of the E2F family of transcription factors
Zhihong Wan, … , Sachiko Kajigaya, Neal S. Young
Zhihong Wan, … , Sachiko Kajigaya, Neal S. Young
Published September 20, 2010
Citation Information: J Clin Invest. 2010;120(10):3530-3544. https://doi.org/10.1172/JCI41805.
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Research Article Virology

Human parvovirus B19 causes cell cycle arrest of human erythroid progenitors via deregulation of the E2F family of transcription factors

Abstract

Human parvovirus B19 (B19V) is the only human pathogenic parvovirus. It causes a wide spectrum of human diseases, including fifth disease (erythema infectiosum) in children and pure red cell aplasia in immunocompromised patients. B19V is highly erythrotropic and preferentially replicates in erythroid progenitor cells (EPCs). Current understanding of how B19V interacts with cellular factors to regulate disease progression is limited, due to a lack of permissive cell lines and animal models. Here, we employed a recently developed primary human CD36+ EPC culture system that is highly permissive for B19V infection to identify cellular factors that lead to cell cycle arrest after B19V infection. We found that B19V exploited the E2F family of transcription factors by downregulating activating E2Fs (E2F1 to E2F3a) and upregulating repressive E2Fs (E2F4 to E2F8) in the primary CD36+ EPCs. B19V nonstructural protein 1 (NS1) was a key viral factor responsible for altering E2F1–E2F5 expression, but not E2F6–E2F8 expression. Interaction between NS1 and E2F4 or E2F5 enhanced the nuclear import of these repressive E2Fs and induced stable G2 arrest. NS1-induced G2 arrest was independent of p53 activation and increased viral replication. Downstream E2F4/E2F5 targets, which are potentially involved in the progression from G2 into M phase and erythroid differentiation, were identified by microarray analysis. These findings provide new insight into the molecular pathogenesis of B19V in highly permissive erythroid progenitors.

Authors

Zhihong Wan, Ning Zhi, Susan Wong, Keyvan Keyvanfar, Delong Liu, Nalini Raghavachari, Peter J. Munson, Su Su, Daniela Malide, Sachiko Kajigaya, Neal S. Young

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Figure 1

B19V NS1 protein induces stable G2 arrest in primary CD36+ EPCs.

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B19V NS1 protein induces stable G2 arrest in primary CD36+ EPCs. CD3...
CD36+ EPCs were B19V- or mock-infected (AC) or transduced with NS1 or control lentivirus (DF), followed by harvests at the indicated time points. (A and D) Cumulative proliferation was measured by counting live or dead cells in triplicate using the trypan blue exclusion method, and results are indicated as total and live cell numbers. Data are shown as mean ± SD of 3 independent experiments. (B and E) BrdU incorporation was analyzed by flow cytometry, and percentages of cells stained at the indicated time points are presented. (C and F) Cell cycle analysis was carried out by staining for DNA content, and percentages of cells in different cell cycle phases at indicated time points are presented on the right. Similar results were obtained in duplicate experiments.