Your search keyword '"Clark, Kristina B."' showing total 2 results

1. Infection of bone marrow cells by dengue virus in vivo.

Author

Noisakran S, Onlamoon N, Hsiao HM, Clark KB, Villinger F, Ansari AA, and Perng GC

Subjects

Animals, Antigens, CD analysis, Blood Platelets ultrastructure, Blood Platelets virology, Bone Marrow Cells ultrastructure, Cell Lineage, Chlorocebus aethiops, Coculture Techniques, Dengue blood, Dengue pathology, Dengue Virus ultrastructure, Giant Cells virology, Immunophenotyping, Macaca mulatta, Megakaryocytes virology, Microscopy, Electron, Plasma virology, RNA, Viral analysis, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Vero Cells virology, Viral Load, Viremia virology, Bone Marrow Cells virology, Dengue virology, Dengue Virus physiology

Abstract

Abnormal bone marrow (BM) suppression is one of the hallmarks of dengue virus (DENV) infection in patients. Although the etiology remains unclear, direct viral targeting of the BM has been reasoned to be a contributing factor. The present studies were carried out in an effort to determine the potential effect of DENV infection on the cellularity of BM using a previously established nonhuman primate model of DENV-induced coagulopathy. BM aspirates were collected at various times from the infected nonhuman primate and cells were phenotypically defined and isolated using standard flow cytometry (fluorescence-activated cell sorting). These isolated cells were subjected to detection of DENV utilizing quantitative real-time reverse transcription polymerase chain reaction, electron microscopy, and immunostaining techniques. DENV RNA was detectable by quantitative real-time reverse transcription polymerase chain reaction in BM specimens and the presence of DENV-like particles within platelet was confirmed by electron microscopy. Enumeration of BM cells revealed a transient surge in cellularity at day 1, followed by a gradual decline from days 2 to 10 post infection. Detailed phenotypic studies showed similar kinetics in the frequencies of CD41(+)CD61(+) cells, regardless of CD34 and CD45 expression. The CD61(+) cells were not only the predominant cells that stained for DENV antigen but fluorescence-activated cell sorting-assisted isolation of CD61(+) cells from the BM were shown to contain infectious DENV by coculture with Vero cells. These data support the view that intravenous infection of nonhuman primate with DENV leads to direct infection of the BM, which is likely to be a contributing factor for transient cell suppression in the peripheral blood characteristic of acute DENV infection., (Copyright © 2012 ISEH - Society for Hematology and Stem Cells. All rights reserved.)

Published

2012

2. Multiploid CD61+ cells are the pre-dominant cell lineage infected during acute dengue virus infection in bone marrow.

Author

Clark KB, Noisakran S, Onlamoon N, Hsiao HM, Roback J, Villinger F, Ansari AA, and Perng GC

Subjects

Animals, Bone Marrow metabolism, Bone Marrow Cells metabolism, Colony-Forming Units Assay, Dengue metabolism, Dengue Virus, Humans, Macaca mulatta, Megakaryocytes metabolism, Megakaryocytes virology, Thrombocytopenia metabolism, Thrombocytopenia virology, p-Aminoazobenzene analogs & derivatives, p-Aminoazobenzene pharmacology, Bone Marrow virology, Bone Marrow Cells virology, Cell Lineage physiology, Dengue virology, Integrin beta3 metabolism

Abstract

Depression of the peripheral blood platelet count during acute infection is a hallmark of dengue. This thrombocytopenia has been attributed, in part, to an insufficient level of platelet production by megakaryocytes that reside in the bone marrow (BM). Interestingly, it was observed that dengue patients experience BM suppression at the onset of fever. However, few studies focus on the interaction between dengue virus (DENV) and megakaryocytes and how this interaction can lead to a reduction in platelets. In the studies reported herein, BM cells from normal healthy rhesus monkeys (RM) and humans were utilized to identify the cell lineage(s) that were capable of supporting virus infection and replication. A number of techniques were employed in efforts to address this issue. These included the use of viral RNA quantification, nonstructural protein and infectivity assays, phenotypic studies utilizing immunohistochemical staining, anti-differentiation DEAB treatment, and electron microscopy. Cumulative results from these studies revealed that cells in the BM were indeed highly permissive for DENV infection, with human BM having higher levels of viral production compared to RM. DENV-like particles were predominantly observed in multi-nucleated cells that expressed CD61+. These data suggest that megakaryocytes are likely the predominant cell type infected by DENV in BM, which provides one explanation for the thrombocytopenia and the dysfunctional platelets characteristic of dengue virus infection.

Published

2012