| Literature DB >> 26927156 |
Julija Svirskaitė1, Hanna M Oksanen2, Rimantas Daugelavičius3, Dennis H Bamford4.
Abstract
The slow rate of adsorption and non-synchronous release of some archaeal viruses have hindered more thorough analyses of the mechanisms of archaeal virus release. To address this deficit, we utilized four viruses that infect Haloarcula hispanica that represent the four virion morphotypes currently known for halophilic euryarchaeal viruses: (1) icosahedral internal membrane-containing SH1; (2) icosahedral tailed HHTV-1; (3) spindle-shaped His1; and (4) pleomorphic His2. To discern the events occurring as the progeny viruses exit, we monitored culture turbidity, as well as viable cell and progeny virus counts of infected and uninfected cultures. In addition to these traditional metrics, we measured three parameters associated with membrane integrity: the binding of the lipophilic anion phenyldicarbaundecaborane, oxygen consumption, and both intra- and extra-cellular ATP levels.Entities:
Keywords: Haloarcula hispanica; Pleolipoviridae; Sphaerolipoviridae; icosahedral membrane-containing virus SH1; icosahedral tailed virus HHTV-1; pleomorphic virus His2; potentiometry; spindle-shaped virus His1; virus life cycle
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Year: 2016 PMID: 26927156 PMCID: PMC4810249 DOI: 10.3390/v8030059
Source DB: PubMed Journal: Viruses ISSN: 1999-4915 Impact factor: 5.048
Haloarcula hispanica SH1, HHTV-1, His1, and His2 viruses used in the study: virion and virus life cycle properties.
| Virus | Virion Morphotype | Lipids 1 | Genome 3 (GenBank Acc. No.) | Virus Family 4 | Adsorption Rate Constant (mL/min) | Virus Release Starts (h p.i.) | Virus Exit | Progeny Viruses at 25 h p.i. (pfu/mL) | References |
|---|---|---|---|---|---|---|---|---|---|
| SH1 | Icosahedral | Internal membrane | 30,889 bp (AY950802) | 1.1 × 10−11 | ~6 | Lysis | 1.5 × 1011 | [ | |
| HHTV-1 | Icosahedral tailed | No lipids | 49,107 bp (KC292025) | Unclassified siphovirus | 2.9 × 10−13 | ~7 | Lysis | 7 × 1010 | [ |
| His1 | Spindle-shaped | Lipid modified MCP 2 | 14,462 bp (AF191796) | 1.9 × 10−12 | ~4 | No lysis | 3 × 1010 | [ | |
| His2 | Pleomorphic | Membrane envelope | 16,067 bp (AF191797) | “Pleolipoviridae” | 5.0 × 10−12 | ~4 | No lysis | 5 × 1011 | [ |
1 Membrane or lipids in the virion; 2 MCP, major capsid protein; 3 Linear dsDNA molecules; 4 International Committee on Taxonomy of Viruses (ICTV); 5 Unassigned family.
Figure 1Adsorption efficiency of His2 to Haloarcula hispanica cells at 37 °C with aeration. The number of unadsorbed viruses was determined by plaque assay. Linear regression was calculated for 0–150 min (r2 = 0.97). The last point (180 min) shows the effect of release of the first progeny viruses (see also Figure 3D).
Figure 2Growth parameters and physiological changes in Haloarcula hispanica during infection by (A–C) SH1 and (D,F) HHTV-1 (MOI of 20). Unadsorbed viruses were removed at 2 h p.i. and measurements were begun at 2 h 15 min p.i. (indicated by arrows) and were carried out in MGM medium at 37 °C with aeration. (A,D) Turbidities of the infected and uninfected cultures; the number of free progeny viruses (pfu/mL) in the infected cultures; and the number of viable cells (cfu/mL) at 25 h p.i. in the uninfected (black arrow head) and infected cultures (white arrow head); (B,E) PCB− binding in the presence of PCB− (calibrated with 3 µM PCB−) to infected, uninfected, and heat disrupted (showing the maximal binding) Har. hispanica cells (n = 3); (C,F) The level of dissolved oxygen in the medium of infected and uninfected Har. hispanica cells (n = 3).
Figure 3Growth parameters and physiological changes in Haloarcula hispanica during (A–C) His1 and (D,F) His2 virus infection (MOI of 20). For PBC− binding and oxygen consumption for the uninfected and heat disrupted control cells, see Figure 2A–C.
Figure 4The amount of the intracellular and extracellular ATP in uninfected and virus-infected (MOI of 20) cultures. Unadsorbed viruses were removed at 2 h p.i. and measurements (n = 3) were started at 2 h 15 min p.i. (marked by arrows).