RNA-binding proteins involved in post-transcriptional regulation in bacteria.

Post-transcriptional regulation is a very important mechanism to control gene expression in changing environments. In the past decade, a lot of interest has been directed toward the role of small RNAs (sRNAs) in bacterial post-transcriptional regulation. However, sRNAs are not the only molecules controlling gene expression at this level, RNA-binding proteins (RBPs) play an important role as well. CsrA and Hfq are the two best studied bacterial proteins of this type, but recently, additional proteins involved in post-transcriptional control have been identified. This review focuses on the general working mechanisms of post-transcriptionally active RBPs, which include (i) adaptation of the susceptibility of mRNAs and sRNAs to RNases, (ii) modulating the accessibility of the ribosome binding site of mRNAs, (iii) recruiting and assisting in the interaction of mRNAs with other molecules and (iv) regulating transcription terminator/antiterminator formation, and gives an overview of both the well-studied and the newly identified proteins that are involved in post-transcriptional regulatory processes. Additionally, the post-transcriptional mechanisms by which the expression or the activity of these proteins is regulated, are described. For many of the newly identified proteins, however, mechanistic questions remain. Most likely, more post-transcriptionally active proteins will be identified in the future.

INTRODUCTION

Bacteria need to survive in constantly changing environments. Therefore, they must be able to alter their gene expression in response to environmental signals, causing protein levels to be adjusted according to the needs of the cell. This can be achieved by adjusting transcription initiation with sigma factors and proteins that activate or repress transcription. However, gene expression regulation also occurs after transcription is initiated (Perez-Rueda and Martinez-Nuñez, 2012). The importance of these post-transcriptional regulatory processes is highlighted by the weak correlation that has been observed between RNA and protein abundance (Picard et al., 2009).

Prokaryotic post-transcriptional regulators typically modulate RNA decay, translation initiation efficiency or transcript elongation. Different types of prokaryotic post-transcriptional regulators have been identified, including small RNAs (sRNAs) and RNA-binding proteins (RBPs). sRNAs are typically defined as non-coding RNA molecules that bind with limited complementarity near the ribosome binding site (RBS) of their target mRNA, causing competition with the ribosome for binding to this region. However, the number of sRNAs that deviate from this general definition is increasing (Liu and Camilli, 2010; Storz et al., 2011). The new insights into the post-transcriptional mechanisms of sRNAs and their role in gene expression regulation were reviewed recently (Desnoyers et al., 2013). Here, RBPs involved in post-transcriptional regulation are discussed. For some of these proteins, the mechanism of action and the targets are well described, as for CsrA and Hfq. Their post-transcriptional function in Escherichia coli was already reported almost 20 years ago (Liu et al., 1995; Muffler et al., 1996). Lately, more insight was gained into the diverse mechanisms these two well-studied proteins use to regulate the expression of their target genes and how they regulate their own expression or activity in E. coli and in other bacteria. Additional RBPs involved in post-transcriptional regulation have been identified only recently and not much is known about their post-transcriptional function. In this review, the general working mechanisms of RBPs are discussed first. Afterward, examples of well-known and recently identified proteins, from E. coli and from other bacteria, are described.

GENERAL MECHANISMS OF REGULATORY PROTEINS THAT ACT POST-TRANSCRIPTIONALLY

Bacterial post-transcriptionally active regulatory proteins typically bind RNA molecules and regulate translation initiation, stability, and transcript elongation of their RNA targets, using different regulatory mechanisms. These mechanisms include (i) adaptation of the susceptibility of the target RNAs to RNases, (ii) modulation of the accessibility of the RBS of mRNA targets for ribosome binding, (iii) acting as a chaperone for the interaction of the RNA target with other effector molecules, and (iv) modulation of transcription terminator/antiterminator structure formation, and will be described hereafter.

ADAPTATION OF THE SUSCEPTIBILITY TO RNases

Regulation of RNA stability is an important mechanism to post-transcriptionally control gene expression, as it affects the number of mRNAs that can be translated or the number of sRNAs that can execute their regulatory function. RNA stability is determined by intrinsic RNA elements, such as primary sequence and secondary structure, but can be affected by sRNAs or proteins that bind to the RNA molecule. These proteins are mainly ribonucleases (RNases). In E. coli, single-stranded RNA-specific endoribonucleases (e.g., RNaseE and RNaseG) or double-stranded RNA-specific endoribonucleases (e.g., RNaseIII) generally initiate mRNA decay by making endoribonucleolytic cleavages. This yields smaller products that are further degraded by a combination of endo- and exonucleases, like PNPase (polynucleotide phosphorylase), RNaseII, or occasionally RNaseR (reviewed in Kaberdin et al., 2011). sRNAs are mainly degraded by RNaseE and PNPase, or by RNaseIII if the sRNA is hybridized to an mRNA target (reviewed in Saramago et al., 2014). In addition to RNases, other RBPs can play a role in the regulation of RNA stability by modulating the susceptibility of mRNAs and sRNAs to these RNases. Regulatory RBPs can act by directly shielding the recognition sites of RNases involved in the decay of RNA molecules if they have a shared binding preference, e.g., proteins that bind to single stranded AU-rich regions which are also recognized by RNaseE in E. coli (Moll et al., 2003). Other regulatory RBPs are involved in the regulation of RNA stability and induce a change in the secondary structure of their mRNA targets upon binding. Consequently, RNase recognition sites become buried or more exposed in locally formed structures, which positively or negatively affects the RNA stability of these molecules, respectively (Barria et al., 2013; see Figure ).

Schematic overview of the working mechanism of RNA-binding proteins (RBPs) influencing RNase susceptibility. (A) By directly blocking RNase recognition sites or (B) by changing the secondary structure of the mRNAs they bind. Because the targets of RBPs can be both mRNAs and small RNAs (sRNAs) and sRNAs are not translated, the ribosome binding site (RBS) is surrounded by a dotted line. RBPs are depicted in yellow, endoribonucleases in blue, exoribonucleases in orange.

Although RNases are the proteins that are mainly involved in RNA degradation, mRNA modifying enzymes can facilitate mRNA turnover as well. Pyrophosphate removal at the 5′ end by RppH (pyrophosphate hydrolase) and addition of a single stranded poly(A) extension at the 3′ end of the mRNA by PAPI [Poly(A) polymerase I] both promote mRNA degradation. Additionally, the exonucleolytic decay of highly structured mRNAs can be facilitated by RhlB, which unwinds RNA structures in an ATP-dependent way (reviewed in Kaberdin et al., 2011). E. coli regulatory RBPs can interfere with the poly(A)-assisted decay of mRNA molecules by binding to the poly(A) tail and protecting the mRNA to which it is bound from degradation (Folichon, 2003). Other regulatory RBPs facilitate mRNA degradation by recruiting RNases or RNA modifying enzymes, e.g., PAPI (De Lay et al., 2013). Because these proteins form a platform for the interaction of RNA molecules and proteins, their mechanism of action is assumed to be different and will be described later.

Many components of the mRNA decay machinery, like the RNases RNaseIII, PNPase, RNaseII, and RNaseR as well as the polymerase PAPI are well conserved across the bacterial kingdom (Kaberdin et al., 2011). This is not the case for the major endonucleases RNaseE/G in E. coli. However, functional homologs of RNaseE/G were identified, e.g., RNase J1/J2 or RNaseY in Bacillus subtilis (Even et al., 2005; Shahbabian et al., 2009). Therefore, it is likely that the regulatory mechanisms identified for regulatory RBPs influencing the susceptibility to degrading or modifying enzymes in E. coli are conserved in other bacteria.

MODULATING RBS ACCESSIBILITY

Besides their involvement in the regulation of RNA stability, RBPs can post-transcriptionally control gene expression by altering the efficiency of translation initiation. Translation initiation of an mRNA requires ribosome binding to the RBS of the mRNA. This RBS contains the Shine–Dalgarno sequence, which is a sequence complementary to the 3′ end of the 16S rRNA. This sequence is important for the recruitment and the correct positioning of the ribosome on the mRNA (Shine and Dalgarno, 1974). The more efficient the pairing between the Shine–Dalgarno region of the mRNA and the 16S rRNA, the more efficient ribosomes are recruited. Although the Shine–Dalgarno region is very important, the interaction region of an initiating ribosome is larger than the Shine–Dalgarno sequence alone and comprises nucleotides -20 to +19 relative to the start codon of mRNAs broadening the region that needs to be accessible in order for ribosome binding to occur (Beyer et al., 1994; Huttenhofer and Fnolier, 1994; Mackay et al., 2011; Desnoyers and Masse, 2012). Regulatory RBPs can modulate the efficiency of translation initiation by directly competing with ribosomes for binding to the ribosome interaction region or by initiating a change in the secondary structure of the mRNA sequence near this region (see Figure ; Dubey et al., 2005; Baker et al., 2007; Irie et al., 2010). The resulting reduction in translation initiation efficiency often causes mRNA stability to be decreased as well. This can be explained by two mechanisms. Firstly, RNaseE can bind internally to a transcript (Mackie, 1998; Kime et al., 2010), but it can also interact with 5′ monophosphorylated transcripts with its 5′ binding pocket (Callaghan et al., 2005). When there is no ribosome bound, the mRNA is not protected from this kind of interaction with RNaseE. Secondly, when translation initiation efficiency is reduced, the spacing of the translating ribosomes on the mRNA is less compact. Consequently, it is more likely that RNase recognition sites in the mRNA become exposed causing transcript decay (Deana and Belasco, 2005).

Schematic overview of the working mechanisms of RBPs influencing the accessibility of the RBS. (A) By directly blocking this region and (B) by changing the secondary structure of the region surrounding the RBS. RBPs are depicted in yellow, the ribosomes in black, CDS, coding sequence.

RECRUITING AND ASSISTING IN THE INTERACTION WITH OTHER MOLECULES

RNA stability or translation initiation efficiency can also be affected by RBPs that form a platform to assist in the interaction of other molecules, which consequently affect RNA stability or translation efficiency (see Figure ). The mechanism of action of these RBPs is described here as different compared to the previous two, because they typically bind simultaneously to an RNA target and an effector molecule. The effector molecule bound by the regulatory protein can be an sRNA or a protein. As previously mentioned, sRNAs typically regulate translation efficiency and RNA stability by binding near the RBS of their mRNA targets. Intermolecular basepairing between the sRNAs and mRNAs is facilitated by regulatory RBPs that function as a chaperone (Herschlag, 1995; Soper et al., 2011). The proteins recruited by regulatory RBPs can be proteins facilitating mRNA degradation, e.g., PAPI, RNases, or the degradosome (De Lay et al., 2013). The degradosome is a multiprotein complex in which different components cooperate during mRNA decay. Often, it contains RNaseE as a scaffolding protein and the protein partners PNPase, enolase, and RhlB. However, its assembly is not essential for RNA decay in E. coli (Carpousis, 2007). The recruitment of these proteins by other RBPs negatively affects transcript stability.

Schematic overview of the working mechanism of RBPs that recruit and assist in the interaction with sRNAs and proteins. RBPs are depicted in yellow, endoribonucleases in blue, exoribonucleases in orange, and auxiliary factors of the degradosome in brown, CDS, coding sequence.

MODULATION OF TRANSCRIPTION TERMINATOR/ANTITERMINATOR STRUCTURE FORMATION

A last mechanism by which RBPs can post-transcriptionally affect gene expression is by modulating transcription elongation. After RNA polymerases initiate transcription, transcripts are elongated until a terminator is reached. There are two classes of terminators: intrinsic and factor-dependent terminators. At intrinsic terminators, dissociation of the elongation complex is dependent on the nucleic acid sequence and structure, while factor-dependent termination is dependent on the action of a protein factor, like the Rho-protein (Santangelo and Artsimovitch, 2011). Typically, these terminators are present at the end of the operon. However, some also exist within the 5′ leader region of the transcript. The presence of a terminator at this site prevents transcript elongation to full length. Premature termination can be abrogated by proteins that bind to the polymerase and allow transcription beyond the terminator signals or by the formation of an alternative secondary structure the enables transcription to progress (Stülke, 2002). In the latter process, RBPs can play a role. In the case of intrinsic termination, the RBPs can stabilize either the terminator structure or an alternative secondary structure, the antiterminator, which prevents the terminator form forming. Often the formation of both structures are mutually exclusive (Santangelo and Artsimovitch, 2011; see Figure ). In general, the activity of this type of RBPs is controlled by their phosphorylation state or by a bound ligand, which induces major conformational changes in the proteins (Santangelo and Artsimovitch, 2011), although there are exceptions (Tortosa et al., 1997; Bachem and Stülke, 1998). Furthermore, RBPs can play a role in rho-dependent termination by inducing a secondary structure change, exposing a rho utilization (rut) sequence that is normally inaccessible for the rho-factor. Protein binding enables access to this region and rho-dependent transcription termination takes place (Figueroa-Bossi et al., 2014).

Schematic overview of the working mechanism of RBPs that modulate transcription terminator/antitermator structure formation. (A) By stabilizing the antiterminator structure, (B) by stabilizing the terminator structure, and (C) by exposing a rho utilization site. RBPs are depicted in yellow, the sequences forming the terminator in red, the sequences forming the antiterminator in blue, and the rho utilization sequences (rut) en rho factor in green. RBS, ribosome binding site.

DIFFERENT RNA-BINDING PROTEINS THAT ACT POST-TRANSCRIPTIONALLY IN BACTERIA

A number of proteins involved in post-transcriptional regulation have been identified in E. coli as well as in other bacteria. They are listed in Table . From this list, the global regulatory proteins CsrA and Hfq are best described in literature. CsrA works predominantly by competing with the ribosome for binding to the RBS of its mRNA targets. Hfq is best known for its role in assisting interacting sRNAs and mRNAs, but the protein applies a variety of other mechanisms to post-transcriptionally control gene expression. Besides Hfq and CsrA, there are other proteins that regulate the expression of their mRNA targets using similar working mechanisms. Moreover, additional RBPs have been identified that specifically regulate sRNA stability. For other RBPs affecting translation efficiency or RNA stability, the exact working mechanism is still unknown. Possibly they do use analogous mechanisms compared to those described for the well-known proteins.

CsrA, AN RNA-BINDING PROTEIN PREDOMINANTLY ACTING BY CHANGING RBS ACCESSIBILITY FOR RIBOSOMES

CsrA from E. coli and its orthologs in other bacteria, are RBPs that predominantly regulate gene expression by competing with the ribosome for binding to the RBS. CsrA is a widely conserved protein that has been annotated in over 1500 species (Finn et al., 2014). The protein is a global regulator, as illustrated by the changed expression level of approximately 10% of the genes in a csrA mutant in different bacteria (Lawhon et al., 2003; Burrowes et al., 2006; Brencic and Lory, 2009). In general, CsrA activates exponential phase functions and represses stationary phase processes (reviewed in Romeo et al., 2013). This is caused by direct and indirect regulatory events, as some CsrA targets encode regulatory proteins themselves (Jonas et al., 2008; Edwards et al., 2011).

To determine the selectivity of the CsrA protein, a SELEX experiment was conducted, enabling the identification of the RNA ligands binding with the highest affinity to CsrA. The CsrA-binding consensus sequence was shown to be RUACARGGAUGU; with the ACA and GGA being 100% conserved. Besides by the presence of this sequence in the mRNA target, CsrA specificity is additionally determined by the secondary structure of the target, as CsrA preferentially binds to RNA molecules that have the binding motif in a hairpin structure, with GGA in the loops of the hairpin (Dubey et al., 2005). The similarity between the CsrA recognition sequence and the consensus sequence of the Shine–Dalgarno region, i.e., AGGAGG, explains why there can be competition between CsrA and the ribosome for binding at this region. However, there are examples of CsrA targets that have CsrA binding sites that do not overlap with the Shine–Dalgarno region. In these cases, one of the CsrA binding sites overlaps with the translation initiation codon (Jonas et al., 2008) or the binding sites are solely present within the coding region (Yakhnin et al., 2011a). In the latter case, CsrA still competes with ribosome binding (Yakhnin et al., 2011a). Generally, the reduced translation initiation efficiency that results from CsrA binding to an mRNA target, leads to mRNA degradation as well (Baker et al., 2002; Dubey et al., 2003; Wang et al., 2005), although there are exceptions (Baker et al., 2007).

While the predominant regulatory mechanism of CsrA is direct competition with the ribosome for RBS binding, the protein can also use other mechanisms. One example is the binding of RsmA, the CsrA ortholog in Pseudomonas aeruginosa, to one of its targets, psl, which causes a stabilization of a hairpin structure in the region spanning the RBS, blocking the Shine–Dalgarno region and preventing ribosome binding (Irie et al., 2010). Secondly, binding of CsrA can have a positive effect on gene expression by blocking RNaseE interaction sites at the 5′ region of the mRNA of flhDC in E. coli which has a positive effect on RNA stability (Yakhnin et al., 2014). Thirdly, CsrA has been implicated recently in promoting the translation of the moaA mRNA. CsrA binding influences the structure of the moaA mRNA, however, this does not affect moaA mRNA levels. The exact mechanism of translational activation therefore remains to be unraveled. Remarkably, the moaA mRNA region that contains one of the CsrA binding sites, can also form a molybdenum cofactor (MOCO) binding riboswitch. It is unclear whether MOCO and CsrA can bind simultaneously or whether MOCO prevents CsrA from binding (Patterson-Fortin et al., 2013). Lastly, CsrA induces premature transcription termination of the pgaA mRNA in E. coli by unfolding a secondary structure sequestering an entry site for transcription terminator factor Rho thereby regulating transcription elongation (Figueroa-Bossi et al., 2014). Although CsrA is predominantly involved in post-transcriptional regulation, the protein has recently been shown to affect transcription as well. In P. protegens, RsmA represses lipA transcription, although the mechanism remains unclear (Zha et al., 2014). Remarkably, lipA is additionally regulated by RsmE, which is one of the paralogs of RsmA in this species. RsmE blocks ribosome access by binding to the RBS of lipA.

Different Pseudomonas species indeed have three non-identical copies of RsmA, the CsrA ortholog in these bacteria. Although the expression profile of RsmE is slightly different from the one of RsmA, both proteins function in a largely redundant way (Reimmann et al., 2005). Another RsmA paralog is RsmN (also called RsmF). RsmN has a different structural organization of α-helices and β-sheets compared to RsmA and RsmE, but the tertiary structure is similar. This results in a conserved spatial organization of key residues within the dimeric structure, which is necessary for RNA-hairpin recognition (Marden et al., 2013; Morris et al., 2013). RsmA can bind to the mRNAs of its paralogs, thereby negatively influencing RsmE and RsmN protein expression (Reimmann et al., 2005; Marden et al., 2013). Altogether, these elements indicate that these proteins have a unique but overlapping regulatory role compared to RsmA. It has been suggested that variations in sequence, structure, RNA-binding affinities and specificities between these different paralogs facilitate tight gene-specific control at the global post-transcriptional level for Pseudomonads. The question remains why E. coli does not possess this wide array of CsrA paralogs (Morris et al., 2013).

Hfq USES DIFFERENT MECHANISMS TO POST-TRANSCRIPTIONALLY REGULATE TARGET GENE EXPRESSION

Hfq is another very well-studied post-transcriptional regulator. The protein is widespread but not ubiquitously present throughout the bacterial kingdom (Sobrero and Valverde, 2012). In general, a knockout in hfq reduces the fitness of bacteria to survive in stressful environments (Tsui et al., 1994; Christiansen et al., 2004; Liu et al., 2010; Wang et al., 2014). Its role in RNA metabolism is more limited in Gram-positive bacteria compared to Gram-negative bacteria, which is illustrated by the fact that an hfq deletion does not have the same global effect on the transcriptome of Bacillus, like it has on the transcriptome of E. coli or Salmonella (Hämmerle et al., 2014).

Hfq has three different sites that can bind RNA: the distal, proximal and lateral site (Sauer, 2013). The binding preferences of these different RNA-binding sites are probably not that strict, as a study performed in Listeria monocytogenes shows that RNA-binding sites of Hfq have the potential to bind a wider variety of RNA sequences than was previously thought (Kovach et al., 2014). However, in E. coli, the distal site of Hfq does have a preference for repetitions of ARN-triplets or poly(A) stretches (Mikulecky et al., 2004; Link et al., 2009; Lorenz et al., 2010). The proximal site, on the other hand, has a preference for AU-rich single stranded sequences or poly(U) stretches (Schumacher et al., 2002; Moll et al., 2003). Finally, the lateral site of Hfq binds U-rich sequences and double stranded elements (Sauer et al., 2012), although the function of this lateral site in RNA-binding is controversial (Sauer, 2013). Some of the Hfq binding specificities overlap with the binding preferences of certain RNases. Therefore, Hfq can influence the RNase susceptibility of an mRNA or an sRNA. The AU-rich binding preference of the proximal binding site of Hfq, for example, is similar to the sequence that is recognized by RNaseE. Therefore, Hfq and RNaseE can compete for binding to the same region, reducing RNA decay (Massé et al., 2003; Moll et al., 2003; Mohanty et al., 2004). In the same way, Hfq plays a role in poly(A)-assisted RNA degradation. With its distal binding site, Hfq can bind to the poly(A) tail of mRNAs. Consequently, this region becomes inaccessible for exonucleases, like PNPase and RNaseII. Hfq binding at the poly(A) tail also impairs RNaseE processing. Both processes increase mRNA stability. However, binding of Hfq can also promote polyadenylation and thus promote poly(A)-assisted decay (Hajnsdorf and Régnier, 2000; Le Derout, 2003; Régnier and Hajnsdorf, 2013). Altogether, these mechanisms indicate how Hfq is important for the stability of sRNAs and mRNAs. Although Hfq is present at high levels in the cell, there is not enough Hfq to stabilize all sRNAs and mRNAs. Therefore, there is constant competition amongst sRNAs and mRNAs for Hfq binding (Vogel and Luisi, 2011).

Next to its role in regulating RNA stability, Hfq can function as a chaperone to stimulate the interaction of mRNAs and sRNAs (Møller et al., 2002; Zhang et al., 2002; Geissmann and Touati, 2004; Rasmussen et al., 2005; Kawamoto et al., 2006). Because there are different RNA-binding sites present in a hexameric Hfq molecule, it is possible that an sRNA and an mRNA are simultaneously bound to one Hfq molecule. Such binding to Hfq brings sRNAs and mRNAs in close proximity, enhancing the likelihood of interaction (Soper et al., 2011). However, cobinding of sRNAs and mRNAs to Hfq is transient and insufficient for sRNA-dependent regulation (Hopkins et al., 2011). Therefore RNA restructuring is also an important function of Hfq in this process (Henderson et al., 2013). The protein can change the secondary structure of the RNA molecules, making some regions in the mRNA more accessible for base pairing (Soper et al., 2011).

In addition to assisting sRNA/mRNA interactions, Hfq can also form a platform for the interaction of these RNA molecules with other proteins, e.g., RNaseE. This RNA/protein complex can then further interact with the other subunits of the RNaseE-based degradosome, causing degradation of the mRNA, and often also of the sRNA, in the complex (Morita et al., 2005; Aiba, 2007). The interaction between Hfq and RNaseE is most likely a combination of direct protein interactions between RNaseE and Hfq, which occur at the RhlB recognition region of RNaseE in the canonical degradosome (Ikeda et al., 2011), and indirect interactions via the RNA molecules they bind (De Lay et al., 2013). Hfq can indirectly interact in this way with a number of other proteins, like the cold shock protein CspC in E. coli and RsmA in P. aeruginosa, a protein that was discussed previously in this review (Sorger-Domenigg et al., 2007; Cohen-Or et al., 2010). Another protein that may be recruited by Hfq is Crc, a protein involved in catabolite repression control in P. fluorescens and P. aeruginosa. Crc was originally identified as an RBP, able to bind short unpaired A-rich motifs (AAnAAnAA) at or near the RBS, thereby inhibiting translation initiation (Moreno et al., 2009; Sonnleitner et al., 2009; Browne et al., 2010). However, a recent study shows that Crc has no RNA-binding capacity and previous results on RNA-binding rely on contaminations of Crc protein samples with Hfq (Milojevic et al., 2013). Hfq and Crc are now assumed to cooperate for binding to RNAs that contain an A-rich motif, because both proteins form a cocomplex and are both necessary for catabolite repression. Possibly Hfq recruits Crc or Crc modifies Hfq in such a way that it can more efficiently bind to the A-rich stretches with its distal site, preventing translation (Moreno et al., 2014).

Next to its functions as a (de)stabilizing factor for RNA molecules and as an interaction platform for RNA/RNA an RNA/protein interactions, Hfq carries out other functions. One of these functions is competing with initiating ribosomes for access to the RBS by binding AU-rich regions close to the RBS which are acting as translational enhancers (Vytvytska et al., 2000; Desnoyers and Masse, 2012). These translational enhancers facilitate the interaction of an mRNA with protein S1 near the RBS, but this interaction is impaired when Hfq is bound. S1 is a protein, weakly associated to the 30S subunit of the ribosome that facilitates the recognition of mRNAs by ribosomes at the initial step of translation (Subramanian, 1983). Sometimes, sRNAs are involved in this regulatory process. Spot42, for example, recruits Hfq at the enhancer region (Desnoyers and Masse, 2012). In another case, Hfq binding takes place without an sRNA as a recruiting molecule. Oppositely, binding of the sRNA RyhB can prevent Hfq from binding to the enhancer region (Salvail et al., 2013). In addition, Hfq has a role in transcription regulation, by inhibiting the function of the Rho protein, which is involved in transcription termination (Le Derout et al., 2010; Rabhi et al., 2011).

While CsrA and Hfq use different mechanisms to globally regulate gene expression, there are proteins that have only been shown to use a confined number of these mechanisms or regulate a more limited number of genes. They will be described hereafter.

RNA-BINDING PROTEINS ADAPTING THE SUSCEPTIBILITY TO RNases

In addition to its role in facilitating ribosome interactions with the mRNA, protein S1 also has a function in post-transcriptional regulation. The protein can stabilize RNA molecules by directly shielding RNase recognition sites (Hajnsdorf and Boni, 2012). Although S1 has no strict sequence specificity, it does have a higher affinity for AU-rich mRNA sites. As RNaseE preferentially binds AU-rich single stranded regions as well, S1 can shield RNaseE recognition sites and protect mRNAs against cleavage (Komarova et al., 2005). Because S1 is capable of binding to sRNAs with the same affinity as Hfq, it has been suggested that S1 can theoretically regulate sRNA stability as well. However, the biological relevance of this suggestion still needs to be elucidated (Koleva et al., 2006; Windbichler et al., 2008).

S1 directly competes with RNases for binding to specific sequences. However, other proteins affect mRNA stability by promoting a change in the secondary structure of their mRNA targets. Consequently, RNase recognition sites become more or less available for RNases. An example of proteins that use this mechanism are cold shock proteins. These proteins are induced when bacteria encounter a temperature downshift. One of the physiological effects of cold is the stabilization of secondary structures that make RNase recognition sites inaccessible, which likewise impairs RNA degradation. Binding of the cold shock protein, CspA, to these mRNAs causes, together with the induced helicases, cold-induced secondary structures in the mRNA to be melted. Adversely, cold shock proteins can also prevent RNA degradation. CspE can bind poly(A) sites and can consequently interfere with either binding of PNPase or with internal cleavage by RNaseE (Feng et al., 2001). Additionally, cold shock proteins can assist in unwinding of secondary structures that sequester the RBS, which enhances translation efficiency (Barria et al., 2013).

RNA-BINDING PROTEINS THAT AFFECT sRNA STABILITY

Hfq is very well known for its role in regulating sRNA and mRNA stability. However, recently, other RBPs were identified that regulate the stability of specific sRNAs. A first example is CsrD (Suzuki et al., 2006). In E. coli, this protein is involved in the turnover of the sRNAs CsrB and CsrC. These sRNAs regulate the activity of CsrA, which is an RBP that was described earlier. Although CsrD destabilizes the sRNAs CsrB and CsrC in an RNaseE-dependent way, these sRNAs have no obvious RNaseE recognition sites and CsrD has no RNase activity itself. Therefore, it was suggested that CsrD might induce structural changes in the sRNA, making it more susceptible for RNaseE (Suzuki et al., 2006). CsrD does not bind specifically to CsrB or CsrC, however, the action of CsrD seems to be specific. This indicates that there are additional factors in the cell that determine the specificity of the process (Suzuki et al., 2006). A second example of an RBP specifically regulating sRNA stability is RapZ. RapZ is a protein identified in E. coli that functions as an adaptor protein guiding the processing of the sRNA, GlmZ. The protein has been reported to recruit RNaseE to the sRNA. It has been hypothesized that this occurs through changing the structure of the sRNA so it can be recognized by RNaseE, or by functioning as an interaction platform by delivering the sRNA to RNaseE (Göpel et al., 2013). Most likely, there are more proteins that bind sRNAs and target them for degradation, just like RapZ and CsrD.

RNA-BINDING PROTEINS THAT MODULATE RBS ACCESSIBILITY

TRAP (trp RNA-binding attenuation protein), a protein involved in the regulation of tryptophan metabolism of B. subtilis, acts through modulating RBS accessibility for ribosomes. The protein specifically binds multiple (9–11) NAG repeats, separated by non-conserved spacers. Because of the extended recognition sequence, TRAP can regulate a small subset of genes, all involved in tryptophan metabolism. TRAP can act as a post-transcriptional regulator by directly blocking ribosome access to the RBS (Babitzke et al., 1994; Yang et al., 1995; Du et al., 1997; Sarsero et al., 2000; Yakhnin et al., 2004). Although the protein binds multiple NAG repeats, it is sufficient that one repeat overlaps with the RBS to block ribosome access to this region (Babitzke et al., 1994; Babitzke et al., 1995). TRAP can also promote a change in secondary structure which influences the availability of the RBS for a subset of genes (Merino et al., 1995; Du and Babitzke, 1998). Additionally, the protein is involved in the regulation of transcription elongation, which will be described later.

The regulatory RBP BpuR from Borrelia burgdorferi possibly acts by competing with ribosome binding as well, as the protein has been shown to bind to the 5′ region of its mRNA target, thereby blocking translation. However, the only identified RNA target of this protein this far is its own mRNA. Most likely, BpuR is a post-transcriptional regulator of other genes in the Borrelia genome (Jutras et al., 2013b). BpuR can also act as a DNA binding protein, but it binds RNA with higher affinity (Jutras et al., 2013a).

PROTEINS ACTING AS AN INTERACTION PLATFORM WITH OTHER MOLECULES

YbeY is a widely conserved protein, known to influence the maturation of rRNAs and to be involved in the quality control of 70S ribosomes (Davies et al., 2011; Jacob et al., 2014). Although it is an essential RNase in some bacteria like Vibrio cholera, the protein is not essential and has weak RNase activity in E. coli and Sinorhizobium meliloti (Vercruysse et al., 2014). In these bacteria, both in silico and phenotypic indications exist, supporting the hypothesis that YbeY plays a role in sRNA regulation, although YbeY has not yet been shown to actually bind sRNAs in vivo in these species. In silico analyses show that YbeY displays high sequence and structural similarities to MID domains of Argonaut proteins, the central component of sRNA-mediated gene silencing in eukaryotes. Argonaut proteins bind sRNAs that function as sequence-specific guides to lead the Argonaut proteins to perfectly or partially complementary sequences (Mallory and Vaucheret, 2010). Additionally, structural models assigned a probable RNA-binding site for YbeY. Phenotypically, there are striking similarities between an smc01113 mutant, the ybeY ortholog in S. meliloti, and an hfq mutant (Pandey et al., 2011). Mutated YbeY indeed causes an increased sensitivity to various stresses, similarly to when Hfq is mutated. Moreover, YbeY modulates the levels of both already identified Hfq-dependent and Hfq-independent sRNAs and their targets in E. coli (Pandey et al., 2014), which suggests that YbeY has a central role in RNA metabolism. The exact working mechanism of the YbeY protein remains unknown. Besides the suggested role in the interaction of mRNAs and sRNAs, YbeY might still have a catalytic role as an RNase as a functional equivalent of RNaseE (Vercruysse et al., 2014).

While YbeY may play a central role in the general sRNA metabolism, there are some RBPs that form a platform of interaction for a more limited number of sRNAs. One example is the FinO family of bacterial chaperones. FinO is involved in the regulation of gene expression from the F-plasmid by facilitating the interaction between the sRNA FinP and the mRNA of the F plasmid transcription factor traJ. The protein facilitates sRNA-mRNA interactions by destabilizing internal hairpins in target RNAs (Arthur et al., 2003) and protects them from RNaseE (Jerome et al., 1999). However, contrary to Hfq, FinO does not simultaneously bind mRNA and sRNA molecules (Chaulk et al., 2010). Other proteins assigned to this FinO-family include NMB1681 in Neisseria meningitides and ProQ in E. coli. Although NMB1681 has been shown to restore phenotypes in an E. coli finO mutant, the role of this protein in Neisseria has not been unraveled (Chaulk et al., 2010). ProQ has an N-terminus homologous to FinO and a C-terminus homologous to the C-terminus of Hfq. Both the N- and the C-terminus facilitate sRNA-mRNA interactions. However, the Hfq-like domain most likely assists in sRNA–mRNA interaction, while the FinO-like domain confers sequence-specific properties to the protein (Chaulk et al., 2011; Sheidy and Zielke, 2013). ProQ also associates with the ribosome, which appears to be mediated by an interaction between ProQ and its targets being translated (Sheidy and Zielke, 2013).

A second example of an RBP possibly involved in assisting a limited number of sRNA–mRNA interactions is FbpB. FbpB is a small protein involved in the regulation of iron metabolism in B. subtilis. The protein is suggested to function as a coregulator of the translational repressor FsrA, by targeting the sRNA FsrA to specific transcripts and increasing the effectiveness of the sRNA. The phenotype of an fbpB mutant can indeed be restored by an upregulation of FsrA. FbpB is possibly involved in the recruitment of the degradation machinery of B. subtilis as well, thereby causing degradation of the sRNA–mRNA complex (Smaldone et al., 2012). Although this is still speculative, this would be consistent with the functions of Hfq in E. coli.

RNA-BINDING PROTEINS THAT MODULATE TRANSCRIPTION TERMINATOR/ANTITERMINATOR FORMATION

TRAP and cold shock proteins have been described earlier as they can induce a change in the secondary structure of their RNA target which modulates RNA stability or translation initiation efficiency. Additionally, these proteins can modulate transcription elongation by stabilizing a transcription terminator or antiterminator structure upon binding. TRAP, activated by tryptophan, binds to the Bacillus trp 5′ leader transcript and occludes the formation of the antiterminator. This antiterminator is located upstream of a terminator and the formation of both structures is mutually exclusive. Thereby, TRAP binding enables the terminator to be formed and transcription is prematurely stopped (Babitzke, 2004). The cold shock proteins CspA and homologs CspC and CspE from E. coli, work in the opposite way. These proteins prevent the formation of transcription terminators by stabilizing an antiterminator structure (Bae et al., 2000; Phadtare et al., 2002).

Another example of RBPs that stabilize an antiterminator structure upon binding is the Bgl/Sac family. These proteins are widely distributed and recognize a 23–30 nucleotide stretch called ribonucleotide antiterminator (RAT) that partially overlaps with the terminator sequence (Aymerich and Steinmetz, 1992). Similarly to cold shock proteins, binding of an RBP of the Bgl/Sac family causes this antiterminator region to fold in a stem-loop structure that occludes the formation of the terminator. The Bgl sytem of E. coli was the first mechanism that involves protein-mediated antitermination (Mahadevan and Wright, 1987; Schnetz and Rak, 1988). Members of this family have been identified in different bacteria such as E. coli, B. subtilis, Lactococcus lactis, and Erwinia chrysanthemi. They control the expression of genes required for the utilization of carbohydrates (Rutberg, 1997).

Lastly, PyrR of B. subtilis is involved in modulating transcription terminator/antiterminator formation, although its mechanism of action is a little different compared to the examples described above. PyrR, activated in the presence of uridine, stabilizes an anti-antiterminator structure. This structure sequesters nucleotides of the antiterminator by basepairing with sequences that lie further upstream, inducing terminator formation and preventing gene expression. Only in the absence of uridine the antiterminator can form and expression of the RNA target is possible (Lu et al., 1996).

POST-TRANSCRIPTIONALLY ACTIVE REGULATORY PROTEINS WITH AN UNKNOWN MECHANISM

Other post-transcriptionally active regulatory proteins have been identified. However, often their exact mechanism of action remains unclear. For example, YopD is a component of the type III secretion system (T3SS) of Yersinia species and is conserved in pathogens with a T3SS (Schiano and Lathem, 2012). It translocates virulence factors across the cell membrane of the host. Simultaneously, YopD post-transcriptionally regulates genes of the T3SS directly and specifically in complex with LcrH, a secretion chaperone (Schiano and Lathem, 2012). The specificity of YopD is thought to be based on the interaction of the protein with short AU-rich sequences, both up- and downstream of the start codon of the target genes. However, the interaction is more complex than YopD/LcrH and AU sequences alone. Other interaction partners are involved. The post-transcriptionally active complex of YopD, LcrH and other interacting components binds to the 5′UTR of its targets and represses their translation, but the mechanism remains unclear. YopD has been suggested to facilitate degradation of these targets by directly competing with ribosome binding or promoting degradation (Chen and Anderson, 2011). However, a recent report shows that YopD affects translation by modifying the ribosome itself (Kopaskie et al., 2013). It is remarkable that a protein with a structural function has a regulatory role as well.

In Shigella sonnei, RodZ was identified as a membrane-localized cytoskeletal protein that retains the rod-shaped morphology of the bacterium. Later, this protein was also shown to be involved in post-transcriptional regulation, as the protein has RNA-binding capacity and its expression leads to repression of InvE protein synthesis by means of a decreased stability of the mRNA. However, the working mechanism still needs to be resolved. Possibly it forms a platform where mRNAs and other putative regulatory factors coincide (Mitobe et al., 2011).

FlbT has been identified in Caulobacter crescentus and Brucella melitensis, where it is proposed to bind to the 5′UTR of the fliC mRNA. However, it is not clear how it post-transcriptionally regulates gene expression. In Caulobacter binding of FlbT promotes degradation of its mRNA targets, whereas in Brucella FlbT is proposed to be an activator of gene expression (Anderson and Gober, 2000; Ferooz et al., 2011).

The family of AmiR and NasR transcriptional antiterminator regulator (ANTAR) domain proteins is a last example of RBPs acting at the post-transcriptional level with an undefined regulatory mechanism. They are widely distributed among different species and are involved in transcription antitermination. These proteins recognize an RNA motif consisting of two tandem stem-loops. However the exact molecular mechanism of antitermination has not been determined (Ramesh et al., 2012). For NasR of Klebsiella oxytoca, it has been suggested that it does not involve the formation of an antitermination structure (Chai and Stewart, 1999).

POST-TRANSCRIPTIONAL REGULATION OF POST-TRANSCRIPTIONALLY ACTIVE REGULATORY PROTEINS

To ensure that gene expression is adjusted according to the needs of the cell, it is crucial that the expression and the activity of the regulatory RBPs themselves are tightly controlled as well. Remarkably, protein expression or protein activity is regulated itself by post-transcriptional regulatory processes. Proteins that modulate RBS accessibility, like CsrA and BpuR, have their recognition site present in the 5′UTR of their own mRNA. Protein binding to the mRNA consequently competes with ribosome binding, reducing translation initiation efficiency and the expression of the protein (Yakhnin et al., 2011b; Jutras et al., 2013b). Similarly, Hfq expression is autoregulated. The protein inhibits ribosome binding to its own mRNA, making it at the same time more vulnerable for cleavage by RNaseE. Two Hfq binding sites were identified upstream of the start codon, with one overlapping with the RBS. However, the other binding site is also necessary for translational repression together with a hairpin structure in the coding region. These elements possibly function as stabilizing elements for RNA/protein interaction (Vecerek et al., 2005).

Secondly, the activity of different RBPs is regulated with sRNAs. These sRNAs carry multiple high affinity sequences that are specifically recognized by a regulatory RBP. Binding of the sRNA sequesters the protein, resulting in a lower number of proteins available for binding to its mRNA targets. The best studied examples of sRNAs that regulate protein activity by mimicking the protein binding sequence are the sRNAs CsrB and CsrC (Liu et al., 1997; Weilbacher et al., 2003). They bind to the global regulator CsrA, which was discussed previously. CsrB and CsrC carry 18 and 9 CsrA binding sequences, respectively. Recently, another E. coli sRNA, McaS, was shown to bind CsrA. This sRNA has at least two CsrA binding sites (Jørgensen et al., 2013). The different sRNA molecules that regulate CsrA activity are differentially expressed in some conditions. Consequently, the activity of the RBP can be regulated in response to different environmental conditions (Jørgensen et al., 2013). Remarkably, CsrA activity is not only regulated by sRNAs. In Salmonella Typhimurium, for example, the fim mRNA can inhibit CsrA function as well. This mRNA carries the CsrA recognition sequence but the stability or the translation of fim mRNA is not affected by CsrA binding, excluding it from being a regulated CsrA target (Sterzenbach et al., 2013).

While CsrA is the best studied example of a protein that is regulated by sRNAs, more of them are known. The Hfq protein, which was extensively discussed above, is regulated by the sRNA CrcZ in E. coli. The sRNA has multiple A-rich stretches to which Hfq can potentially bind with its distal RNA-binding region. As Hfq has other RNA-binding sites it is possible that the protein can still bind and regulate other RNA molecules when CrcZ is bound to this distal site. However, this remains to be resolved (Sonnleitner and Bläsi, 2014). A last example is RapZ, which is sequestered by binding to the sRNA GlmY. This sRNA resembles the mRNA target of RapZ, i.e., GlmZ, by a conserved central stem-loop structure (Göpel et al., 2013). This shows that not only the global regulators, like CsrA and Hfq, are regulated through sRNA mimicry.

Although the activity of some RBPs is regulated by sRNAs, the activity of others is still regulated by proteins. This is the case for the TRAP protein, which is regulated by an anti-TRAP protein that binds near the RNA-binding pocket of the TRAP protein, preventing TRAP from binding to its mRNA targets (Snyder et al., 2004). CsrA from B. subtilis is another RBP that is regulated by a protein, FliW. This antagonistic protein binds near the active site of the protein. Remarkably, a CsrB-like sRNA has also been identified in B. subtilis (Mukherjee et al., 2011). Its regulatory role and the importance compared to FliW has not been unraveled yet (Kulkarni et al., 2006).

CONCLUSION AND PERSPECTIVES

Regulation of gene expression is very complex and takes place at different regulatory levels. At the post-transcriptional level, RBPs are important gene expression regulators. These proteins generally act by adapting RNA stability and mRNA translation efficiency. Hereto, they use different mechanisms, including (i) adaptation of the susceptibility of the target RNAs for RNases, (ii) modulation of the accessibility of the RBS for ribosome binding, (iii) acting as a chaperone for the interaction of the RNA target with other effector molecules, and (iv) modulation of transcription terminator/antiterminator formation. Different post-transcriptionally active RBPs have been identified in E. coli and in other bacteria, with Hfq and CsrA being the two best studied examples. These proteins apply different mechanisms to regulate the expression of their target genes. Recently, additional RBPs that affect mRNA and/or sRNA stability or translation efficiency have been identified. Although many mechanistic questions remain, they use mostly similar regulatory mechanisms to regulate the expression of their targets. Additionally, they are post-transcriptionally regulated themselves through autoregulation and regulation by sRNA mimicry.

A number of post-transcriptionally active RBPs have been identified. However, it is very likely that more RBPs are active as post-transcriptional regulators, given that some known regulatory RBPs have another function, e.g., as a transcription regulator or a structural protein. Moreover, proteins that specifically regulate sRNA stability have only recently been discovered. Therefore, most likely, more proteins of this class will be identified in the future. Additionally, relatively little is known about this type of regulatory proteins in other bacteria than E. coli. Therefore, methods have been developed to identify new RBPs. One of these methods is the in vitro or in vivo assembly of RNA and RBPs, followed by mass spectrometry (Tsai et al., 2011). This method has already been optimized for Helicobacter pylori, E. coli, Salmonella Typhimurium and P. aeruginosa (Windbichler et al., 2008; Said et al., 2009; Rieder et al., 2012; Osborne et al., 2014).

Further studies on well-known and newly identified post-transcriptionally active proteins will lead to a better understanding of how bacteria use this type of gene regulation to respond to changes in the environment and how different post-transcriptional networks interact with transcriptional regulons and with each other. This knowledge will create opportunities for new or improved biotechnological applications, e.g., in synthetic biology as a tool to control gene expression, complementing the current approaches of transcription control. Additionally, as many of these proteins play a central role in RNA metabolism, interfering with the expression or the function of these proteins can be interesting as an alternative antimicrobial strategy.

Conflict of Interest Statement

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Table 1

Bacterial RNA-binding proteins (RBPs) that influence gene expression post-transcriptionally.

RBP	Targets	Sequence selectivity	Predominant post-transcriptional working mechanism	Post-transcriptional regulators	Species	Reference
ANTAR containing proteins	Nitrate metabolism and other	Tandem stem-loop	Antitermination, mechanism unclear	/	Widely distributed	Ramesh et al. (2012)
Bgl/Sac family	Carbohydrate utilization genes	Ribonucleotide antiterminator (RAT)	Stabilizing antiterminator	/	Widely distributed	Rutberg (1997)
BpuR	bpuR mRNA	/	Inhibiting translation, exact mechanism unclear	/	Borrelia burgdorferi	Jutras et al. (2013b)
Csp	Global regulator	Hairpins	Promoting secondary structure change that changes availability for RBS or RNases - Blocking RNase interactions - Stabilizing antiterminator	/	Widely conserved	Barria et al. (2013)
CsrA (RsmA)	Global regulator	RUACARGGAUGU	Competing with ribosome binding - Blocking RNase interactions - Activation of translation by unknown mechanism	small RNAs (sRNAs) CsrB/C (RsmX/Y/Z) FliW protein	Widely conserved	Reviewed in reference Romeo et al. (2013)
CsrD	CsrB/C sRNAs	Unspecific, specificity by accessory proteins	Unclear, possibly by promoting secondary structure change that changes availability for RNases	CsrA protein	Enterobacteriacea	Suzuki et al. (2006)
FbpB	Iron metabolism	/	Unclear, possibly interaction platform sRNA/mRNA - Possibly recruiting RNase and degradosome	/	Bacillus subtilis	Gaballa et al. (2008), Smaldone et al. (2012)
FlbT	FliC	/	Unresolved	/	Rhizobiales Caulobacter crescentus	Anderson and Gober (2000), Ferooz et al. (2011)
Hfq	Global regulator	Poly(A)/ARN Poly(U)/AU-rich ssRNA U-rich dsRNA	Interaction platform sRNA/mRNA - Direct blocking of RNase recognition sites - Recruiting PAPI, Crc, RNaseE and degradosome - Competing with ribosome binding	Autoregulation sRNA CrcZ	Widely conserved	Reviewed in reference Sauer (2013)
ProQ	ProP, biofilm	Duplex with ss 5’ and 3’ end	Interaction platform sRNA/mRNA - ribosome association	/	Escherichia coli	Chaulk et al. (2011), Sheidy and Zielke (2013)
PyrR	Pyrimidine metabolism	/	Stabilizing anti-antiterminator		B. subtilis	Lu et al. (1996)
RapZ	GlmZ sRNA	/	Unclear, possibly recruiting RNaseE or promoting secondary structure change that changes availability for RNases	sRNA GlmY	E. coli	Göpel et al. (2013)
RNaseE	General RNA turnover	ss AU-rich region (A/GNAU)	RNase		Widely conserved	Reviewed in reference Mackie (2013)
RodZ	InvE (T3SS) + role in cell shape	/	Unresolved	/	Shigella sonnei	Mitobe et al. (2011)
RsmE	Global regulator	RUACARGGAUGU	Direct blocking of RBS	RsmA protein sRNAs RsmY/Z	Pseudomonads	Reimmann et al. (2005)
RsmN/F	Global regulator	RUACARGGAUGU	Direct blocking of RBS	RsmA protein sRNAs RsmY/Z	Pseudomonads	Marden et al. (2013); Morris et al. (2013)
S1	Global regulator	AU-rich ssRNA	Direct blocking of RNase restriction sites	/	Gram-positive bacteria	Hajnsdorf and Boni (2012)
TRAP	Tryptophan metabolism	(NAG)9-11	Direct blocking of RBS - Promoting secondary structure change that blocks RBS - Stabilizing terminator	Anti-TRAP protein	B. subtilis	Muto et al. (2000), Babitzke (2004), Gollnick et al. (2005)
YbeY	Global regulator sRNAs	/	RNase - Possibly interaction platform sRNA/mRNA	/	Widely conserved	Pandey et al. (2011, 2014)
YopD	T3SS + structural pore component	/	Modifying ribosome	/	Yersinia species	Chen and Anderson (2011)