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Periplasm

The periplasm is the aqueous compartment situated between the inner cytoplasmic and the outer in , forming a gel-like matrix that typically occupies 20% to 40% of the cell's total volume. This space is bounded by the two membranes and contains a layer that provides , along with a high concentration of proteins, including enzymes, binding proteins, and chaperones. In , a narrower periplasmic space exists between the cytoplasmic membrane and the thick layer, but it is less pronounced and functionally distinct. The periplasm serves as a multipurpose essential for bacterial , featuring an oxidizing that facilitates protein oxidation, folding, and through specialized chaperones and bond-forming enzymes. It houses binding proteins that aid in the uptake of nutrients such as , sugars, vitamins, and iron via transporters, as well as enzymes like for hydrolysis and for acquisition. Additionally, membrane-derived oligosaccharides (MDOs) within the periplasm regulate cellular osmolarity by counteracting external variations, while detoxification enzymes such as β-lactamases protect against antibiotics. The size and integrity of the periplasm are tightly controlled by lipoproteins, such as Lpp, which anchor the outer membrane to the layer, maintaining an intermembrane distance critical for functions like environmental sensing and the assembly of nanomachines such as the flagellar rotor. This compartment also acts as a reservoir for factors that reflect the bacterium's metabolic status and responses to external conditions, influencing pathogenicity and adaptation. Disruptions in periplasmic , such as alterations in size or protein composition, can impair , resistance, and overall cell envelope integrity, making it a potential target for novel strategies.

Definition and Context

Definition

The periplasm refers to the specialized compartment situated between the inner cytoplasmic membrane and the outer membrane in diderm bacteria, which include Gram-negative species, or between the plasma membrane and the cell wall in monoderm bacteria, such as Gram-positive species. This space functions as a distinct aqueous within the bacterial cell envelope, housing the peptidoglycan layer that provides structural integrity. Characterized as a gel-like, viscous matrix, the periplasm is densely populated with soluble proteins, enzymes, and binding proteins that contribute to its crowded and dynamic nature. The terminology has evolved from its initial focus on the "Gram-negative periplasm" to a broader application encompassing diderm and monoderm configurations, as proposed in Gupta's phylogenomic analyses of prokaryotic cell envelopes (1998, 2009). Unlike the , the periplasm contains no ribosomes or ATP-generating systems, relying instead on and electrochemical gradients, such as the Donnan potential, to facilitate protein transport and enzymatic activities.

Occurrence in Bacteria

The periplasm is primarily found in diderm bacteria, which possess both an inner cytoplasmic membrane and an outer membrane, creating a distinct compartment between them. This structure is typical of , such as those in the Proteobacteria, including the model organism , though some (e.g., Negativicutes in Firmicutes) also exhibit diderm configurations. In these bacteria, the periplasm contains a thin layer, typically 2-3 nm thick, which anchors the outer membrane to the inner membrane and contributes to cell shape maintenance. In monoderm bacteria, which lack an outer membrane and are exemplified by many such as in the phylum Firmicutes (though some Firmicutes members are diderm), the periplasm is not a well-defined space but is represented by an inner-wall zone (IWZ). This zone lies between the cytoplasmic membrane and the thicker layer of the , serving a comparable role in protein localization and transport. The in these bacteria is substantially thicker, ranging from 20-80 nm, forming a robust multilayered network that constitutes the bulk of the . The distinction between diderm and monoderm configurations reflects ancient evolutionary divergences in bacterial lineages, with phylogenetic analyses suggesting that monoderms may represent the ancestral state from which diderms arose under selective pressures, such as exposure favoring outer development. However, this view is debated, with some phylogenomic studies proposing that diderms were ancestral and monoderms arose through outer loss in certain lineages. Studies using conserved protein signatures, including chaperonins like Hsp60 and , support this transition as a key event in bacterial diversification, with diderms emerging later in . While the periplasm is absent in most and eukaryotes, some with outer -like structures, such as certain hyperthermophiles in the phylum Crenarchaeota, exhibit a quasi-periplasmic space between their cytoplasmic and surface layers, lacking but potentially fulfilling analogous compartmental functions. Eukaryotes generally do not possess a direct homolog, though intracellular compartments like the lumen share some biochemical similarities in protein processing.

Physical and Chemical Properties

Composition

The periplasm of is primarily composed of soluble proteins, which can constitute up to 30% of the total cellular protein content, as revealed by proteomic analyses. These proteins are diverse and include several key classes essential for periplasmic functions: chaperones such as SurA and Skp that assist in , enzymes like alkaline phosphatases and hydrolases that perform degradative or catalytic roles, and binding proteins that facilitate nutrient uptake through systems. Structurally, the periplasm contains the peptidoglycan sacculus, a thin meshwork of cross-linked polysaccharides and peptides that provides rigidity and anchors the outer membrane. The outer leaflet of the outer membrane, bounding the periplasm, is dominated by lipopolysaccharides (LPS), amphipathic molecules consisting of lipid A, core oligosaccharide, and O-antigen chains that contribute to the compartment's barrier properties. Divalent cations, particularly Mg²⁺ and Ca²⁺, are abundant in the periplasm, where they stabilize LPS aggregates by screening negative charges on phosphate and carboxyl groups within the lipid A and core regions. The periplasmic environment is characterized by a mildly acidic ranging from 6 to 7, which closely tracks the external in neutral conditions, and oxidizing conditions that promote the formation of bonds in proteins. These properties are maintained by enzymatic systems like DsbA, enabling proper folding of secreted proteins. Additionally, structural elements such as the bases of motility organelles, including the P ring of flagella, are anchored within the layer of the periplasm, securing the flagellar motor to the cell envelope.

Volume and Dynamics

The periplasm in diderm , such as , occupies 20-40% of the total cellular volume, accommodating a significant portion of the cell's proteins and serving as a dynamic compartment between the inner and outer membranes. In contrast, monoderm , including most Gram-positive species, possess a much smaller analogous periplasmic space due to the absence of an outer membrane and the dominance of a thick layer. This disparity in volume underscores the periplasm's role as a specialized feature primarily in diderms, where it is anchored by acting as a structural scaffold. The periplasm exhibits dynamic volume changes in response to cellular growth, division, and environmental stresses, including osmotic shifts that can cause expansion or contraction to maintain envelope integrity. For instance, hypoosmotic conditions increase , leading to periplasmic expansion, while hyperosmotic induces contraction. Recent studies have shown that alterations in width, such as those induced by in the actin homolog MreB, result in corresponding reductions in periplasmic volume; in wider E. coli mutants, the periplasm thins by approximately 3 compared to wild-type s, activating envelope responses via the Rcs phosphorelay system. In vivo measurements of periplasmic volume and width rely on advanced imaging techniques like cryo-electron , which provides high-resolution visualizations of the intact without fixation artifacts. These methods have revealed typical periplasmic widths of 20-40 nm in , with precise quantifications showing wild-type E. coli at around 30-32 nm. plays a key role in modulating this width, as it exerts mechanical force on the membranes and , influencing periplasmic dimensions during osmotic adaptations and growth phases.

Biological Functions

Protein Processing and Quality Control

Proteins destined for the periplasm in are primarily exported from the via two major pathways: the (general secretory) pathway and the Tat (twin-arginine translocation) pathway. The pathway translocates unfolded precursor proteins across the inner membrane in a post-translational manner, relying on the SecYEG translocon and chaperone-assisted unfolding to prevent premature folding in the . In contrast, the Tat pathway exports fully folded proteins, often those requiring cofactors for stability, using a distinct translocon that recognizes a twin-arginine in the . These pathways ensure that proteins enter the periplasm in states amenable to subsequent maturation, with the pathway handling the majority of periplasmic proteins and the Tat pathway specialized for a subset of cofactor-containing enzymes. Upon translocation into the oxidizing environment of the periplasm, many exported proteins require disulfide bond formation for proper folding and stability. This process is catalyzed primarily by the DsbA enzyme, a soluble periplasmic with a thioredoxin-like fold featuring an active-site motif (CXXC) that enables rapid disulfide exchange. DsbA introduces non-native disulfide bonds into incoming polypeptide chains by attacking their free thiols with its oxidized cysteine pair, thereby transferring its disulfide and becoming reduced itself; this is reoxidized by the membrane-bound DsbB, which links the process to the respiratory . For proteins with incorrect disulfide pairings, the DsbC corrects them through similar thiol-disulfide exchange, using its own CXXC motif within a domain, while DsbD maintains DsbC in its reduced state by shuttling electrons from the . These enzymes collectively ensure vectorial disulfide formation, promoting the structural integrity of periplasmic proteins like factors and enzymes. To prevent aggregation of unfolded outer membrane proteins (OMPs) during transit, periplasmic chaperones such as Skp and SurA play essential roles. Skp, a 17-kDa trimeric chaperone, encapsulates hydrophobic OMP precursors in a cage-like structure, shielding exposed transmembrane regions and dynamically expanding to accommodate chain elongation for proteins exported via the pathway. SurA, the primary chaperone for most OMPs, binds unfolded substrates via its peptidyl-prolyl isomerase domains and delivers them to the β-barrel assembly machinery (BAM) complex at the outer membrane, with genetic studies showing it handles the bulk of OMP biogenesis while Skp supports a parallel, partially redundant pathway. Misfolded or aggregated proteins are targeted for degradation by proteases, notably DegP (also known as HtrA), a temperature-dependent that functions as a chaperone below 28°C to protect substrates from irreversible aggregation and switches to proteolytic activity at higher temperatures to degrade them into peptides. DegP's oligomeric cage structure sequesters misfolded OMPs and periplasmic proteins, using a PDZ as a molecular to ensure processive cleavage into defined fragments, thus maintaining periplasmic under stress.

Transport and Secretion

The periplasm in serves as a critical compartment for the translocation of molecules across the cell envelope, enabling the import of essential nutrients and the export of proteins and other cargoes to the extracellular environment. This space facilitates high-affinity uptake systems and pathways that are essential for bacterial survival, , and environmental . Soluble periplasmic proteins play a key role in binding and delivering substrates to membrane-embedded transporters, while specialized multiprotein complexes drive the directional movement of folded macromolecules. Nutrient uptake in the periplasm is primarily mediated by ATP-binding cassette (ABC) importers, which rely on periplasmic binding proteins (PBPs) to capture scarce substrates with high specificity and deliver them to transmembrane transporters. For instance, the (MBP) in binds maltose in the periplasm and interacts with the MalFGK2 to facilitate its ATP-dependent import across the inner membrane, allowing efficient scavenging of oligosaccharides in nutrient-limited conditions. These PBPs undergo conformational changes upon substrate binding, promoting interaction with the importer's substrate-binding site and ensuring selective transport of sugars, , and ions. Similar mechanisms operate for peptide uptake via DppA and OppA proteins, underscoring the periplasm's role in concentrating low-abundance nutrients for cytoplasmic assimilation. Secretion through the periplasm involves dedicated systems that translocate folded exoproteins from the periplasm across the outer membrane. The type II secretion system (T2SS), also known as the general secretory pathway, assembles a pseudopilus apparatus in the periplasm to push substrates like lipases, proteases, and toxins outward, as exemplified by the Gsp machinery in Vibrio cholerae and Pseudomonas aeruginosa, where periplasmic components such as GspL and GspM form a platform for pilus extension and retraction. This system exports over 40 different proteins in some species, contributing to virulence by delivering hydrolytic enzymes that degrade host tissues. Complementing T2SS, outer membrane vesicles (OMVs) bud from the outer membrane, encapsulating periplasmic contents including proteins, lipids, and DNA for targeted delivery to recipient cells or host environments. In Neisseria gonorrhoeae, OMVs transport virulence factors like IgA protease, enhancing immune evasion and biofilm formation without direct cell-cell contact. The periplasm also supports ion and DNA transport, particularly during bacterial competence for genetic transformation. In competent Bacillus subtilis, transforming DNA is threaded through the cell wall into the periplasm via the ComEA protein, which binds and stabilizes single-stranded DNA, conferring DNase resistance and enabling subsequent translocation to the cytoplasm by ComFA helicase. This process, detailed in studies showing periplasmic accumulation as the initial barrier to transformation, allows horizontal gene transfer under stress conditions. Ion homeostasis is maintained by periplasmic chaperones and transporters, such as those in ABC systems for metal ions, preventing toxicity while supporting enzymatic functions. In , the periplasm is integral to assembly and function, housing components that span the cell envelope for transmission. The flagellar embeds in the inner membrane with periplasmic rings (P-ring and L-ring) formed by FlgI and FlgH proteins, which anchor the rod structure and facilitate hook-filament in the periplasm before . During , stator units like MotA/MotB complexes interact with periplasmic domains of the (FliG), generating up to 1,500 · to drive the helical filament for . In , these periplasmic interactions ensure efficient assembly and switching between counterclockwise and clockwise , essential for directed movement.

Cell Wall Maintenance

The periplasm plays a crucial role in the final stages of (PG) synthesis, where (PBPs) catalyze the cross-linking of PG precursors to form the mature meshwork. These membrane-anchored enzymes, primarily class A and B PBPs, perform transglycosylation to polymerize strands and transpeptidation to link cross-bridges, occurring in the periplasmic space to ensure proper envelope assembly during cell growth and division. The AmpG transporter facilitates the uptake of PG precursors, such as anhydromuropeptides, from the periplasm into the , enabling their reuse in ongoing PG biogenesis and maintaining precursor pools for sustained wall synthesis. PG recycling in the periplasm involves the degradation and recovery of wall fragments, with enzymes like NagZ (a β-N-acetylglucosaminidase) and AmpD (an anhydromuramyl-L-alanine amidase) processing imported GlcNAc-anhMurNAc-peptide units to salvage (GlcNAc), N-acetylmuramic acid (MurNAc), and peptide components. This pathway, conserved in , prevents the wasteful accumulation of turnover products and supports efficient resource utilization during envelope remodeling. Recent analyses highlight how disruptions in this recycling, such as AmpG deficiencies, lead to muropeptide buildup in the periplasm, compromising wall integrity. Periplasmic modifications of enhance bacterial resilience, including O-acetylation at the C6 position of MurNAc residues, which sterically hinders of the backbone, and amidation of stems (e.g., on D-isoglutamate or D-alanine), which alters charge and reduces susceptibility to host-derived muramidases. These post-synthetic adjustments, mediated by periplasmic acetyltransferases like PatA/PatB and amidotransferases, are vital for evading innate immune defenses in pathogenic contexts. Envelope stress responses in the periplasm are coordinated by the Rcs phosphorelay system, where the outer membrane RcsF acts as a for PG damage or assembly defects, transmitting signals through periplasmic interactions to activate the histidine kinase RcsC and downstream regulators like RcsB. This pathway induces adaptive responses, such as capsule production and repression, to restore upon detecting periplasmic perturbations.

Significance

Clinical and Pathogenic Roles

The periplasm plays a crucial role in bacterial by facilitating the assembly and secretion of key factors essential for . In Gram-negative pathogens, the Type V secretion system, also known as the autotransporter pathway, enables the translocation of passenger domains—such as adhesins and toxins—across the outer membrane after initial export to the periplasm via the machinery. For instance, adhesins like those in the YadA family promote host cell attachment and formation, while toxins such as the autotransporter of (EspC) contribute to tissue invasion. Additionally, periplasmic chaperones and the P-ring structure support flagella assembly, allowing motility that aids in host colonization and dissemination during infection, as seen in spirochetes like where periplasmic flagella drive unique undulatory movement. The periplasm is a primary site for action and resistance in , influencing clinical outcomes in infections. , including penicillins and cephalosporins, target (PBPs) localized in the periplasmic space, where they inhibit cross-linking essential for integrity, leading to bacteriolysis. , a last-resort polymyxin, disrupts the by lipopolysaccharides, causing periplasmic leakage and subsequent inner damage. Efflux pumps like AcrAB-TolC, spanning the inner , periplasm, and outer , actively export a broad range of antibiotics from the periplasm, contributing to intrinsic multidrug resistance in pathogens such as and . Periplasmic enzymes, particularly , confer by hydrolyzing before they reach PBPs, a mechanism prevalent in extended-spectrum beta-lactamase (ESBL)-producing . These enzymes are secreted into the periplasm, where they efficiently degrade incoming drugs, enabling survival in clinical settings like urinary tract infections. Emerging research highlights the periplasm's role in broader multidrug , including novel enzymes and efflux modulation that exacerbate to carbapenems and fluoroquinolones, as detailed in recent reviews on Gram-negative pathogens. In , the periplasm supports pathogenesis through outer membrane vesicles (OMVs) that package and deliver effectors, promoting intestinal invasion and immune evasion during .

Biotechnological Applications

The periplasm of serves as a key compartment for recombinant , particularly for proteins requiring disulfide bonds, such as fragments and hormones, due to its oxidative that facilitates proper folding. Strategies to enhance yields include the use of signal peptides like the , which directs proteins to the periplasm via the pathway, achieving high-level expression of functional disulfide-bonded therapeutics. For instance, periplasmic expression systems have been optimized for production, where co-expression of disulfide isomerases like DsbA and DsbC further improves assembly and solubility, enabling scalable manufacturing for diagnostic and therapeutic applications. Outer membrane vesicles (OMVs) derived from , which bud from the periplasmic space, have been engineered for targeted delivery of therapeutic proteins, addressing challenges in . A notable advance involves the type zero secretion system (T0SS), where proteins are packaged into OMVs for protection against gastric degradation, enabling effective mucosal uptake. In a 2025 study, Wang and colleagues demonstrated this approach by engineering E. coli OMVs to deliver and antigens orally, achieving up to 20-fold higher in animal models compared to direct of the proteins, with potential for and enzyme replacement therapies. Periplasmic engineering has expanded to biocatalytic applications, where compartmentalization enhances enzyme stability and product purity for pharmaceutical and synthesis. By targeting enzymes to the periplasm, bacterial cells act as whole-cell factories, minimizing intracellular interference. Recent efforts have transformed the periplasm into tunable "factories" by co-expressing molecular chaperones, such as Skp, FkpA, and Dsb proteins, to boost folding efficiency and mitigate aggregation of recombinant proteins. These multi-chaperone systems increase soluble yields by up to fourfold for complex therapeutics like single-chain variable fragments (scFvs), while integrating modulators maintains periplasmic during high-density . In 2024 platforms, such designs have enabled efficient production of disulfide-bonded peptides, paving the way for customizable periplasmic cascades in sustainable .

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