Detection of inteins among diverse DNA polymerase genes of uncultivated members of the <i>Phycodnaviridae</i>

Culley, Alexander I.; Asuncion, Brenda F; Steward, Grieg F.

doi:10.1038/ismej.2008.120

Cited by 29 publications

(34 citation statements)

References 41 publications

Supporting

Mentioning

Contrasting

Unclassified

Order By: Relevance

“…polB identification and qPCR Phylogenetic analyses of AVS-amplified polB sequences from spring, summer and fall clone libraries revealed that, with the exception of a single sequence, they were all most closely related to cultivated prasinoviruses when compared with other phycodnaviruses. These results are consistent with those from previous studies demonstrating that all, or nearly all environmental sequences obtained with the AVS-1 and 2 primers cluster with polB genes from marine prasinoviruses (for example, Short and Suttle, 2002;Short and Short, 2008;Clasen and Suttle, 2009;Culley et al, 2009). It is known that these primers do not amplify polB genes from other phycodnaviruses, such as Emiliania huxleyi virus, Heterosigma akashiwo virus, Chrysochromulina ericina virus and Pyramimonas orientalis virus, for example, Larsen et al, 2008).…”

Section: Resultssupporting

confidence: 82%

Quantification of virus genes provides evidence for seed-bank populations of phycodnaviruses in Lake Ontario, Canada

2010

View full text Add to dashboard Cite

Using quantitative PCR, the abundances of six phytoplankton viruses DNA polymerase (polB) gene fragments were estimated in water samples collected from Lake Ontario, Canada over 26 months. Four of the polB fragments were most related to marine prasinoviruses, while the other two were most closely related to cultivated chloroviruses. Two Prasinovirus-related genes reached peak abundances of 41000 copies ml À1 and were considered 'high abundance', whereas the other two Prasinovirus-related genes peaked at abundances o1000 copies ml À1 and were considered 'low abundance'. Of the genes related to chloroviruses, one peaked at ca 1600 copies ml À1 , whereas the other reached only ca 300 copies ml À1 . Despite these differences in peak abundance, the abundances of all genes monitored were lowest during the late fall, winter and early spring; during these months the high abundance genes persisted at 100-1000 copies ml À1 while the low abundance Prasinovirus-and Chlorovirus-related genes persisted at fewer than ca 100 copies ml À1 . Clone libraries of psbA genes from Lake Ontario revealed numerous Chlorella-like algae and two prasinophytes demonstrating the presence of candidate hosts for all types of viruses monitored. Our results corroborate recent metagenomic analyses that suggest that aquatic virus communities are composed of only a few abundant populations and many low abundance populations. Thus, we speculate that an ecologically important characteristic of phycodnavirus communities is seed-bank populations with members that can become numerically dominant when their host abundances reach appropriate levels.

show abstract

Section: Resultssupporting

confidence: 82%

Quantification of virus genes provides evidence for seed-bank populations of phycodnaviruses in Lake Ontario, Canada

2010

View full text Add to dashboard Cite

show abstract

“…employed under nonoptimal conditions. No inteins were identified in these viral genomes, although inteins with homing endonucleases have been observed in prasinoviruses (62), including some Ostreococcus viruses (63), and in some green algae, including Bathycoccus, with viruses being a proposed mechanism for propagation (64).…”

Section: Discussionmentioning

confidence: 99%

Diversity of Viruses Infecting the Green Microalga Ostreococcus lucimarinus

Derelle

Monier

Cooke

et al. 2015

J Virol

View full text Add to dashboard Cite

The functional diversity of eukaryotic viruses infecting a single host strain from seawater samples originating from distant marine locations is unknown. To estimate this diversity, we used lysis plaque assays to detect viruses that infect the widespread species Ostreococcus lucimarinus, which is found in coastal and mesotrophic systems, and O. tauri, which was isolated from coastal and lagoon sites from the northwest Mediterranean Sea. Detection of viral lytic activities against O. tauri was not observed using seawater from most sites, except those close to the area where the host strain was isolated. In contrast, the more cosmopolitan O. lucimarinus species recovered viruses from locations in the Atlantic and Pacific Oceans and the Mediterranean Sea. Six new O. lucimarinus viruses (OlVs) then were characterized and their genomes sequenced. Two subgroups of OlVs were distinguished based on their genetic distances and on the inversion of a central 32-kb-long DNA fragment, but overall their genomes displayed a high level of synteny. The two groups did not correspond to proximity of isolation sites, and the phylogenetic distance between these subgroups was higher than the distances observed among viruses infecting O. tauri. Our study demonstrates that viruses originating from very distant sites are able to infect the same algal host strain and can be more diverse than those infecting different species of the same genus. Finally, distinctive features and evolutionary distances between these different viral subgroups does not appear to be linked to biogeography of the viral isolates. IMPORTANCEMarine eukaryotic phytoplankton virus diversity has yet to be addressed, and more specifically, it is unclear whether diversity is connected to geographical distance and whether differential infection and lysis patterns exist among such viruses that infect the same host strain. Here, we assessed the genetic distance of geographically segregated viruses that infect the ubiquitous green microalga Ostreococcus. This study provides the first glimpse into the diversity of predicted gene functions in Ostreococcus viruses originating from distant sites and provides new insights into potential host distributions and restrictions in the world oceans.

show abstract

“…Chen et al 1996, Short & Suttle 2002, Short & Short 2008, Clasen & Suttle 2009, Culley et al 2009, and by demonstrating the existence of polB fragments from unknown types of phycodnaviruses. Amplification with degenerate Chlorovirus-specific primers led to the recovery of Lake Ontario sequences that represent a new type of Chlorovirus.…”

Section: Resultsmentioning

confidence: 99%

“…For example, the algal virusspecific polB primers AVS1 and AVS2 have been used to amplify genes from different types of chloroviruses, prasinoviruses and prymnesioviruses (Chen & Suttle 1995, Brussaard et al 2004, Bellec et al 2009). However, with the exception of 1 operational taxonomic unit (OTU, or a DNA sequence ≤97% identical to any other) from the Gulf of Mexico (Chen et al 1996), and 2 from Kane'ohe Bay, O'ahu, Hawai'i, USA (Culley et al 2009), polB fragments amplified from natural environments using the AVS primers have all been most closely related to cultivated marine prasinoviruses (Short & Short 2008, Clasen & Suttle 2009, Culley et al 2009). …”

Section: Introductionmentioning

confidence: 99%

Novel phycodnavirus genes amplified from Canadian freshwater environments

Short

Rusanova²,

Staniewski³

2011

Aquat. Microb. Ecol.

View full text Add to dashboard Cite

Extant and newly designed primers for the polymerase chain reaction (PCR) were used to amplify phycodnavirus DNA polymerase ( polB) gene fragments from numerous samples collected at different times of the year from 3 freshwater environments in Ontario, Canada. Overall, a total of 143 cloned PCR fragments were sequenced and 106 putative phycodnavirus polB gene fragments were identified. Although most of these 106 gene fragments were very closely related (i.e. > 97% identical) to polB sequences from chloroviruses, or environmental sequences related to prasinoviruses, 16 represented 2 new types of phycodnavirus polB genes. More specifically, polB fragments that formed a new clade of chloroviruses were amplified from Lake Ontario using newly designed Chlorovirus-specific PCR primers, and a polB sequence most closely related to genes from the prymnesioviruses PgV-03T and CbV-PW1 was amplified from a pond sample from Mississauga, Ontario, using the degenerate algal virus-specific PCR primers AVS1 and AVS2. Thus, the results of the present study provide evidence for a new type of Chlorovirus, and the first observation of polB sequences from freshwater phycodnaviruses that are presumed to infect algae other than chlorophytes.

show abstract

Detection of inteins among diverse DNA polymerase genes of uncultivated members of the Phycodnaviridae

Cited by 29 publications

References 41 publications

Quantification of virus genes provides evidence for seed-bank populations of phycodnaviruses in Lake Ontario, Canada

Quantification of virus genes provides evidence for seed-bank populations of phycodnaviruses in Lake Ontario, Canada

Diversity of Viruses Infecting the Green Microalga Ostreococcus lucimarinus

Novel phycodnavirus genes amplified from Canadian freshwater environments

Contact Info

Product

Resources

About