Abstract
Viruses that infect bacteria (phages) can influence bacterial community dynamics, bacterial genome evolution and ecosystem biogeochemistry. These influences differ depending on whether phages establish lytic, chronic or lysogenic infections. Although the first two produce virion progeny, with lytic infections resulting in cell destruction, phages undergoing lysogenic infections replicate with cells without producing virions. The impacts of lysogeny are numerous and well-studied at the cellular level, but ecosystem-level consequences remain underexplored compared to those of lytic infections. Here, we review lysogeny from molecular mechanisms to ecological patterns to emerging approaches of investigation. Our goal is to highlight both its diversity and importance in complex communities. Altogether, using a combined viral ecology toolkit that is applied across broad model systems and environments will help us understand more of the diverse lifestyles and ecological impacts of lysogens in nature.
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Why study lysogeny?
Bacteria significantly alter the biosphere, affecting global biogeochemical cycles and the biology of other organisms biology (Alivisatos et al., 2015), but do so under the constraints of bacteriophage (phage) infection. Such phage infections range from productive to lysogenic (see Concept Box and Figure 1a) dependent on, for example, phage genetics, host genetics, phage concentration, host physiology and environmental conditions. Temperate phages in particular can replicate either lysogenically as prophages or, instead, produce virions. Although prophages in lysogenic cycles largely have been viewed as dormant entities, both prophages and their subsequent productive cycles can affect individual cells as well as entire communities. The phenomenon of lysogeny is well known, early reviews of lysogeny date to over half a century ago (Lwoff, 1953), though mostly temperate phages infecting E. coli have been characterized in depth including λ, Mu, P1 or N15. In nature, phages have been detected wherever their host microbes exist (Weinbauer, 2004), with reviews focusing on total viral communities from soil, aquatic and host-associated systems (Chibani-Chennoufi et al., 2004; Suttle, 2005; Sawstrom et al., 2008; Srinivasiah et al., 2008; Williamson, 2011; Marcó et al., 2012; Reyes et al., 2012; Abeles and Pride, 2014; Sime-Ngando, 2014; Virgin, 2014; Ogilvie and Jones, 2015; Zablocki et al., 2016). Assessing predominant infection dynamics and associated driving factors, however, can be challenging due to difficulties in determining lysogeny abundance, diversity and ecology (Paul and Weinbauer, 2010).
Here, we complement efforts to specifically review lysogeny which have largely focused on prophage genomics and impacts of lysogeny on either microbial cells (Casjens, 2003; Brussow et al., 2004; Canchaya et al., 2004; Abedon and LeJeune, 2005; Fortier and Sekulovic, 2013; Hargreaves et al., 2014; Feiner et al., 2015; Menouni et al., 2015; Davies et al., 2016) or particular environments (for example, aquatic (Paul, 2008)). We aim to establish an integrative view across model systems and environments, whereas also highlighting emerging tools for the study of lysogeny in nature.
Lysogeny mechanistic diversity
Most molecular knowledge of lysogeny has been derived from a handful of E. coli phages, such as λ and Mu, which integrate into the bacterial chromosome via site-specific recombination (Casjens and Hendrix, 2015) or random transposition (Harshey, 2014), respectively. In contrast, other phages are maintained extrachromosomally with either circular (for example, P1, (Lobocka et al., 2004) or linear (for example, N15, (Ravin, 2015)) genomes. Some temperate phages, such as satellite phage P4, require other temperate phages, such as P2, to complete infection cycles (Christie and Calendar, 2016). Other temperate phages, for example,Vibrio cholera phage CTXphi, chronically infect their host during productive cycles and integrate during lysogenic cycles (McLeod et al., 2005). Although infection details differ, lysogeny generally proceeds through three steps: (i) establishment, (ii) maintenance and also, potentially, (iii) induction of productive cycles (Figure 1). Focusing on λ as a reference, we highlight how these mechanistic factors both serve as a knowledge baseline for further study and can contribute to lysogen ecology.
Establishment
Given evasion of host resistance mechanisms (Samson et al., 2013), temperate phages ‘decide’ whether to produce virions (productive cycle) or instead establish lysogenic cycles as prophages. In λ, the ‘decision’ to enter lysogeny is driven by genetic compatibility (for example, host attB integration sites), host physiological state (for example, nutrient depletion increases lysogeny) and phage density (for example, higher MOIs increase lysogeny) (Casjens and Hendrix, 2015). Integration is driven via recombinases acting on phage (attP) and bacterial (attB) attachment site sequences that determine specificity (Fogg et al., 2014), or prophages may integrate randomly (for example, Mu) or not at all (for example, P1).
Maintenance
Once established, integrated prophages replicate as part of the bacterial chromosome, whereas extrachromosomal prophages require genes for plasmid inheritance (for example, ParA/ParB in P1 or SopA/SopB in N15) and persistence (for example, toxin–antitoxin proteins that kill plasmid-lacking cells) (Casjens and Hendrix, 2015; Ravin, 2015). Either state has the potential to impact on host gene regulation and resulting biology, including growth rate, development and phenotype (Feiner et al., 2015). In λ, maintenance is tightly regulated by its repressor, CI, via a complex genetic feedback circuit (Bednarz et al., 2014). During this stage, prophages not only can alter cellular processes, but are subject to evolutionary change, with selection presumably balancing phage versus cell needs (Bobay et al., 2013).
Induction
Activation of the lytic-lysogenic switch occurs either spontaneously at low frequency (10−8–10−5 per cell for λ (Czyz et al., 2001)) or as a result of external stressors such as those triggering the cell’s DNA damage response (the SOS response) (Casjens and Hendrix, 2015), leading to inactivation of CI. Stressors include changes in nutrients, pH or temperature, and exposure to antibiotics, hydrogen peroxide, foreign DNA (Banks et al., 2003; Mell and Redfield, 2014; Casjens and Hendrix, 2015) or DNA damaging agents (Cochran et al., 1998). Alternatively, prophages can influence the induction of other phages. For example, satellite temperate phage P4 is induced via Cox, an anti-repressor encoded by temperate phage P2 (Christie and Dokland, 2012), whereas Enterococcus prophages pp1, pp3 and pp5 inhibit the induction of co-infecting prophages pp4 and pp6 (Matos et al., 2013). This view of intracellular phage-mediated competition highlights the complexity of interactions among phages of likely ecological relevance.
Once induced, prophages replicate either episomally (for example, λ, P1, N15) or by transposition (for example, Mu). Later, virion particles assemble and are packaged with phage DNA via endonucleolytic enzymes that either cut DNA at specific sites (for example, cos phages) or non-specifically after filling up the capsid (for example, headful packaging by pac phages) (Rao and Feiss, 2015). Specialized transduction (by cos temperate phages) and generalized transduction (by pac phages generally) can differentially impact bacterial genome evolution (Rao and Feiss, 2015).
Such models of temperate phage infection (Figure 1) offer a comparative baseline for discovering variations in lysogeny in nature. For example, as observed in Staphylococcus aureus, temperate phage can integrate into one host genome but exist extrachromosomally in others (Utter et al., 2014), or as found in Salmonella, be asymmetrically inherited by only one daughter cell (Cenens et al., 2013a). As conditions in nature are highly variable, it is also critical to distinguish lysogeny from delayed or inefficient lytic infections (Dang et al., 2015), as well as determine how natural infections can differ from those in the laboratory (Chibani-Chennoufi et al., 2004). Establishment of new phage-host model systems also will be instrumental towards furthering our understanding of lysogen ecology.
Benefits and consequences of lysogeny
Temperate phages alter the biology of their hosts and, in turn, influence the surrounding community of host and non-host cells (Figure 1c). We briefly summarize four such effects, which have been previously reviewed. First, integrating prophages can engineer a host’s genome (Menouni et al., 2015) and help to regulate gene expression and function such that integration and excision alters cellular processes (Feiner et al., 2015). Second, prophages can change cell physiology by introducing novel functions or altering pre-existing ones, such as virulence factor production, metabolism, cell development and immunity to phages (Hargreaves et al., 2014). Third, through transduction, temperate phages can facilitate the transfer of bacterial DNA that potentially confer new phenotypes such as antibiotic resistance (Davies et al., 2016). Fourth, induced and released temperate phages can modify bacterial communities by lysing competitor bacterial strains (Duerkop et al., 2012), lysogenizing other cells (Gama et al., 2013), and liberating intracellular contents for neighboring cells to use as nutrients (Nanda et al., 2015).
Prophages can be ‘domesticated’ by losing genes, including those necessary for virion production (Wang et al., 2010; Bobay et al., 2014). Resulting prophage-derived genomic elements can be selectively maintained by cells should they still confer some advantage. Such cryptic prophages also can directly impact the wider ecosystem. R-type bacteriocins, which resemble phage tail-like particles, can, for example, kill neighboring competitor bacteria (Gebhart et al., 2012). Phage tail-like metamorphosis-associated contractile structures in the biofilm formed by Pseudoaltermonas luteoviolacae, by contrast, can trigger the settlement of eukaryotic tube worm larvae to surfaces (Shikuma et al., 2014), though exactly how P. luteoviolacae might benefit from this process is unclear. Prophage decay also can result in repetitive sequences that facilitate chromosomal insertions, creating niche-defining genomic islands. In Cyanobacteria, these have been hypothesized to influence expression of adjacent nitrogen stress response genes (Sullivan et al., 2009). Decayed prophages can still be inducible as well as capable of lysing their host cell, as illustrated by R-type bacteriocins (Gebhart et al., 2012), and their genes may re-enter the virus gene pool via recombination during co-infection with other phages (De Paepe et al., 2014a).
Genetic, ecological and functional insights into lysogeny
Viral ecology has been extensively studied and reviewed, providing insights into lysogeny and its influencing factors that we synthesize here (Figure 2). Genetically, temperate phages have been identified in ~40–50% of microbial genomes (Canchaya et al., 2003; Casjens, 2003; Fouts, 2006; Paul, 2008; Touchon et al., 2016), and more recently from 21/30 phyla for which complete isolate genomes were available (Touchon et al., 2016). Ecologically, lysogens are widespread (Chibani-Chennoufi et al., 2004), occurring in terrestrial (Williamson et al., 2007; Srinivasiah et al., 2008), aquatic (Wommack and Colwell, 2000; Weinbauer, 2004; Suttle, 2005; Paul, 2008; Sawstrom et al., 2008; Paul and Weinbauer, 2010; Sime-Ngando, 2014) and host-associated ecosystems (Reyes et al., 2012; Abeles and Pride, 2014; De Paepe et al., 2014b; Virgin, 2014; Edlund et al., 2015; Ogilvie and Jones, 2015), though frequencies vary.
Functionally, a paradigm of lysogeny is that it enhances phage and host survival, particularly under adverse conditions, with most data deriving from aquatic and soil environments (Paul, 2008; Sawstrom et al., 2008; Srinivasiah et al., 2008; Williamson, 2011; Sime-Ngando, 2014). Specifically, lysogen frequency generally is inversely correlated with primary microbial productivity levels during specific seasons or environments (Sawstrom et al., 2008). Modeling (Stewart and Levin, 1984) suggests that the lysogenic state should be favored under conditions that cause reduced host cell number and activity (for example, low productivity, low nutrients or reduced host fitness) or when viral particle decay rates are high (for example, from heat or UV exposure), as postulated in soil and aquatic environments (Sime-Ngando, 2014).
Virus-to-microbe-ratios (VMR) have been associated with lysogeny such that lower VMRs (due to, for example, high rates of virion decay and/or low virion production) may be indicative of conditions that could favor lysogeny (Williamson, 2011). VMRs vary considerably, from 1.4 to 160 in marine waters (Wigington et al., 2016) and between ~0.001 and >1000 in different soils (Williamson, 2011). Generally where lower VMRs occur, for example, human gut lumen (0.019 to 0.209; (Kim et al., 2011)) and some soils (for example, ⩾12 in wetland soils; (Williamson et al., 2007)), lysogeny is hypothesized to be common. Conversely, where higher VMRs occur, for example, marine oligotrophic waters and cold desert soils, lysogeny is considered to be less prevalent (Paul, 2008; Zablocki et al., 2016). Recent research builds on this, finding that low VMRs occurred where microbial cell numbers are most abundant (Knowles et al., 2016). How specific virus-host abundances fit into either the previous view of where low host cell numbers would increase lysogeny over lytic infections, to the alternative that high host cell numbers promotes lysogeny, invites renewed effort to develop experimental hypothesis-testing approaches, as exemplified by the few but important mesocosm experiments available (Srinivasiah et al., 2008; Pradeep Ram and Sime-Ngando, 2010).
Where to explore lysogeny next
Next-generation sequencing is beginning to map viral diversity across less-explored ecosystems, using genomes derived from viral particles (Reyes et al., 2012) or total microbial communities (Paez-Espino et al., 2016). The abundance, diversity and activity of lysogeny in many systems, however, remains underexplored.
In applied settings, understanding lytic-lysogenic dynamics may aid in improving biotechnological processes, such as in agricultural or food production, but such knowledge is in its infancy. For example, prophages are diverse among lactic acid bacteria responsible for fermentation processes such as wine (for example, Oenococcus) or dairy (for example, Lactococcus and Lactobacillus) (Marcó et al., 2012; Kot et al., 2014). These offer models of microbial succession during fermentations that are both ecologically and economically interesting given that prophages can be both beneficial (improving host fitness) and detrimental (lysing cells upon induction).
In host-associated systems, lysogeny studies have largely focused on microbial virulence (Brussow et al., 2004; Abedon and LeJeune, 2005; Fortier and Sekulovic, 2013; Hargreaves et al., 2014; Feiner et al., 2015; Davies et al., 2016). In humans, temperate phages appear common (Abeles and Pride, 2014; De Paepe et al., 2014b; Edlund et al., 2015; Ogilvie and Jones, 2015). In addition, infection dynamics of the human gut virome (Waller et al., 2014) show low host cell abundances when temperate phages are in lytic cycles, presumably lysing those hosts. Another study found increased expression of phage genes involved in lytic cycles during periodontal disease (Santiago-Rodriguez et al., 2015), suggesting a connection between phages and disease, though it was not confirmed that these genes were associated with temperate phages. Given the importance of microbiota in health and disease (Alivisatos et al., 2015), and the added consequences of the use of antibiotics, which are stressors that impact on lysogen induction (Allen et al., 2011), host-associated systems are ideal for exploring the implications of the lytic-lysogenic switch. Further, investigation of specific temperate phage–host interaction dynamics can reveal key players driving ecosystem change (Allen et al., 2011; Waller et al., 2014).
Across host genomes, patterns are emerging in both the types of bacteria that are commonly lysogenized and prophage diversity. For example, the detection of λ-like, P1-like or Mu-like phages varies across microbial genomes, with Mu-like and P1-like being least reported (Casjens, 2003; Fouts, 2006; Bobay et al., 2013; Roux et al., 2015b). In addition, prophages appear to predominate across some microbial phyla (for example, 74% of Firmicutes, 41% of Actinobacteria and 22% of Cyanobacteria), but not others (for example, 0% of Chlamydiae) (Touchon et al., 2016). Correlations between prophage frequency and bacterial growth rates, genome size and pathogenicity have been found (Touchon et al., 2016) and could be driven by a microbe’s ecology. For example, prophages have been associated only with invasive Staphylococcus aureus strains (Goerke et al., 2009), and are absent from the intracellular pathogen, Chlamydiae (Touchon et al., 2016).
Emerging approaches to study lysogeny in nature
A combination of approaches for investigating lysogeny in bacterial isolates and complex communities (Figure 3) can be used to assess its abundance, diversity and activity. Experimental methods for detecting lysogeny have provided foundational mechanistic and ecological knowledge, but are recognized to have methodological issues. First, they often require exposure to stressors or lysogen dilution (Paul and Weinbauer, 2010), which can have variable induction efficiencies (Braid et al., 2004; Hanh et al., 2015; Niu et al., 2015). Second, quantifying induction is problematic as virion enumeration is challenging on field samples (Forterre et al., 2013) and highly sensitive to burst size estimates (Parada et al., 2006). Here, we focus on how sequencing-based methods can complement more traditional experimental approaches and help formulate hypotheses to experimentally test.
Sequencing-enabled approaches for identifying and quantifying temperate phages:
Prophage sequences can be identified from whole or draft microbial isolate genomes (Lima-Mendez et al., 2008; Zhou et al., 2011; Akhter et al., 2012; Roux et al., 2015a); theoretically from single-cell genomes (Roux et al., 2014; Labonte et al., 2015b); or from microbial metagenomes (Waller et al., 2014; Roux et al., 2015a). From viromes, temperate phages can be identified by marker genes (for example, integrases or ParA/B genes (Emerson et al., 2012)); phylogenic analysis of conserved genes (for example, DNA polymerase gene (Schmidt et al., 2014)); similarity to isolate phages or by cross-comparing viral and bacterial sequence datasets (Waller et al., 2014); and by predicting phage/host lifestyle through in silico genome analysis (for example, with PHACTS (McNair et al., 2012)). Such sequence-based approaches can even help identify hosts (Waller et al., 2014; Hannigan et al., 2015; Labonte et al., 2015a, b; Edwards et al., 2016) and the relative proportions of temperate phages undergoing lysogenic or lytic infections (Waller et al., 2014). Prophage functionality, however, from in silico prediction requires experimental validation. In addition, activity can be inferred from presence in metatranscriptomes (Dupont et al., 2015; Engelhardt et al., 2015; Santiago-Rodriguez et al., 2015) and metaproteomes (Ogilvie et al., 2013) or by coupling viromics to induction experiments (McDaniel et al., 2008). Although confirming activity depends on experimental induction, this latter approach revealed seasonal patterns in lysogen frequency, inversely correlated to bacterial productivity in Antarctic Ocean waters (Brum et al., 2015).
Improving sequence-based and experimental characterization of lysogeny:
Sequence-based approaches can be improved with better technology to obtain (Brown et al., 2014), assemble (Bankevich et al., 2012) and identify temperate phages either by circumventing reference database limitations (for example, via k-mer analysis (Hurwitz et al., 2014)) or expanding known prophage sequence diversity (Roux et al., 2015b; Paez-Espino et al., 2016).
Experimentally, there is critical need for developing both additional experimental approaches that can help test in silico-derived hypotheses, and new model systems that can capture the diversity of lysogenic infections in nature. Here, methods for gene marker-based approaches are emerging for single-cell resolution including microfluidic digital PCR (Tadmor et al., 2011), fluorescently labeled probes (Allers et al., 2013), fluorescently labeled phages (Zeng et al., 2010)), and fluorescent reporters of prophage gene expression and genome inheritance (Cenens et al., 2013b). These can help discriminate between lysogeny and poorly characterized lysogenic (Abedon, 2009) or inefficiently lytic (Dang et al., 2015) infections. Although such methods could be improved, as discussed in (Dang and Sullivan, 2014), they nevertheless still should be helpful for characterizing lysogenic infections.
Conclusions
Temperate phages can switch between infection modes that have different but significant affects on microbial communities. Lytic cycles both kill and solubilize host bacteria, whereas lysogenic cycles impact host cells more subtly, both physiologically and genetically. Though lysogeny has been long recognized, fundamental questions nonetheless remain: (i) How do lysogen abundances change across space, time and taxa? (ii) What are the consequences and impacts on prophage-host interaction dynamics and ecosystem function? (iii) What drives these patterns? (iv) From the phage perspective, what types of prophages predominate, and why? (v) From the host perspective, why are some bacteria more prone to lysogeny than others? Numerous emerging approaches offer opportunities to develop model systems, as well as study the diverse ecological roles that lysogens have in natural microbial communities. Given these new approaches, we posit that as lytic phages have dominated the viral ecology literature to date, temperate phages should soon share the spotlight.
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Acknowledgements
Anca Segall, Bob Blasdel, Claudia Igler, Bentley Fane, Martha Clokie and members of the OSU VirusLab, especially Simon Roux, Joanne Emerson and Sheri Floge, are thanked for shaping our thinking on temperate phage biology, although the latter are also thanked for comments on the manuscript. Support for this synthesis effort was provided by a Gordon and Betty Moore Foundation Investigator Award (#3790) and National Science Foundation award (OCE# 1536989) to MBS.
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Howard-Varona, C., Hargreaves, K., Abedon, S. et al. Lysogeny in nature: mechanisms, impact and ecology of temperate phages. ISME J 11, 1511–1520 (2017). https://doi.org/10.1038/ismej.2017.16
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DOI: https://doi.org/10.1038/ismej.2017.16
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