- 1Laboratory of Microbiology Signals and Microenvironment (LMSM), Normandie Université Rouen, Evreux, France
- 2Winogradsky Institute of Microbiology, Research Center of Biotechnology of Russian Academy of Science, Moscow, Russia
Neurohormones diffuse in sweat and epidermis leading skin bacterial microflora to be largely exposed to these host factors. Bacteria can sense a multitude of neurohormones, but their role in skin homeostasis was only investigated recently. The first study focused on substance P (SP), a neuropeptide produced in abundance by skin nerve terminals. SP is without effect on the growth of Gram-positive (Bacillus cereus, Staphylococcus aureus, and Staphylococcus epidermidis) and Gram-negative (Pseudomonas fluorescens) bacteria. However, SP is stimulating the virulence of Bacillus and Staphylococci. The action of SP is highly specific with a threshold below the nanomolar level. Mechanisms involved in the response to SP are different between bacteria although they are all leading to increased adhesion and/or virulence. The moonlighting protein EfTu was identified as the SP-binding site in B. cereus and Staphylococci. In skin nerve terminals, SP is co-secreted with the calcitonin gene-related peptide (CGRP), which was shown to modulate the virulence of S. epidermidis. This effect is antagonized by SP. Identification of the CGRP sensor, DnaK, allowed understanding this phenomenon as EfTu and DnaK are apparently exported from the bacterium through a common system before acting as SP and CGRP sensors. Many other neuropeptides are expressed in skin, and their potential effects on skin bacteria remain to be investigated. Integration of these host signals by the cutaneous microbiota now appears as a key parameter in skin homeostasis.
Introduction
Skin is a complex ecosystem hosting the second most numerous microbial population of the human body (1). Skin-associated bacteria, which represent the essential of this population, are classically divided into two categories, i.e., commensal and transient germs. While commensal bacteria are considered having protective functions, transient ones include opportunistic pathogens. However, this reductive vision is far from reality and germs such as Staphylococcus aureus, originally considered as pathogens, are chronically carried by 35–60% of the human population (2). Other bacterial pathogens, such as Bacillus cereus, Pseudomonas aeruginosa or even Neisseria meningitidis, can also be encountered on normal skin in a total absence of clinical signs (3). In fact, virulence is not a constant trait for the large majority of the bacterial species, and expression of virulence is closely controlled by bacterial communication designated under the general term of quorum sensing (QS) (4). The QS is triggered in Gram-negative bacteria by N-acyl homoserine lactones and in Gram-positive bacteria by cyclic or linear peptides. Sensing these molecules can lead pathogenic, but also non-pathogenic, bacteria to switch from harmless to aggressive by regulating the production of most of their virulence factors. However, communication is not solely based on intra- or interspecies bacterial QS, since bacteria also need adapting to their host, thereby sensing numerous eukaryotic signals, including skin neuropeptides. These mechanisms are acknowledged to be part of interkingdom communication.
Skin is the principal neuroendocrine organ of the human body (5), and since 1930 it is known that neurotransmitters such as catecholamines can modulate bacterial infection (6). However, at this time, bacteria were considered inert, and this observation was attributed to an unknown effect of adrenalin on the human physiology. It was necessary to wait for the work of Lyte and Ernst in 1992 to show that catecholamines can promote the growth of Escherichia coli (7) and also bacterial adhesion, biofilm formation, and expression of virulence factors (8, 9). Membrane proteins acting as specific bacterial sensors for catecholamines were identified, and it was then recognized that bacteria can sense human neurotransmitters (10). This concept was extended to neuropeptides and neurohormones, giving birth to microbial endocrinology, which is presently one of the more active fields in microbiology (11). Neuroendocrine factors have multiple effects on bacteria and can regulate their growth, adhesion, invasion, virulence, and/or biofilm formation activity (12). As almost 25% of the microbial population is located deeply into the skin, particularly in hair follicles and sweat or sebaceous glands (13), bacteria are in close contact with eukaryotic cells communication factors. Moreover, it has been shown that neuropeptides diffuse in significant amount in upper epidermal layers and sweat (14, 15). Cutaneous bacteria are then exposed largely to these host factors.
Effect of Substance P (SP) on Cutaneous Bacteria
In skin, SP is essentially released by sensory primary afferent C-fibers (16). This undecapeptide of the tachykinin family has multiple bioactivities other than neurotransmission, such as fibroblast and keratinocyte proliferation, mast cell degranulation, and capillary vasodilatation (5, 17). It is considered as a major mediator of neurogenic inflammation and has central functions in itch (5). Cutaneous neuropeptides, and particularly SP, are contributing to the pathogenesis of different skin diseases, including psoriasis (18), atopic dermatitis (19), immediate and delayed hypersensitivity (20), acne (21), or rosacea (22). These diseases are of multifactorial origin, and different studies suggest a contribution of the skin microflora but also an involvement of local host factors (23).
SP Sensing by B. cereus
In a first step, the effect of SP was studied on a strain of B. cereus (MFP01) isolated from normal human skin (23). Even at a micromolar concentration, SP was without effect on the growth kinetic of B. cereus. SP was also without effect of its swimming and swarming modes of motility. However, when B. cereus was grown in the presence of SP, the bacterium showed a strong increase of cytotoxicity on HaCaT keratinocytes (24). The threshold of SP activity was nanomolar and therefore in the range of the local concentration of the neuropeptide in skin during inflammation or stress. Bacteria were rinsed to remove any trace of free peptide prior to cell infection, and all the controls realized showed that this effect can only be explained by a direct effect of SP on the bacterium. Moreover, the SP reversed sequence peptide and neurokinin A, which in eukaryotes binds on the same receptor as SP, displayed no activity on cutaneous bacteria (24, 25). B. cereus is responding to SP by an over production of collagenase that can explain its effect on HaCaT cells (24). However, a massive cell death, as observed after exposure of keratinocytes to SP-treated bacteria, is associated with the release of high amounts of toxic-oxidizing compounds, and B. cereus also reacts to SP by an overproduction of superoxide dismutase (24). This can be considered as a defense reaction of the bacterium. When B. cereus was exposed to SP over a long period (13 h), an increase in the release of S-layer proteins was also noted (24). This result was correlated to a peel-off of the S-layer (the outer wall of the bacterium) and to a drop in bacterial surface polarity (24). These events can also be interpreted as a general defense reaction of the bacterium against SP as this peptide has structural homologies with cationic antimicrobial peptides, and S-layer monomers are known to complex and neutralize antimicrobial peptides (26). The response of B. cereus to SP being rapid (90.5% of the maximal response in less than 5 min) and the S-layer showing multiple pores allowing the passage of peptides (27), an SP surface binding site was postulated. By using an original immunoprecipitation technique, a 43 kDa protein, the thermo unstable ribosomal elongation factor EfTu, was identified as the SP sensor in the membrane of B. cereus (24) (Figure 1A). EfTu is not presenting sequence or structural similarities with the SP (NK1) receptor (Figure 1B). However, it was not surprising that EfTu was acting as a surface receptor on the bacterium because this molecule is present in large excess in bacteria (28), and it is now recognized as a “moonlighting protein” (29). These proteins are characterized by multiple functions in different locations between the bacterial stroma and the membrane. Because of their long evolution and history, bacteria have reached a high level of protein fitting (30); expression of moonlighting proteins should be an alternative strategy to counterbalance the absence of alternative splicing in these organisms.
Figure 1. Bacterial substance P (SP) and calcitonin gene-related peptide (CGRP) sensors. The thermo unstable ribosomal elongation factor EfTu identified as SP sensor is a 395 amino acids protein (43 kDa) characterized by three principal domains (A). Domain I is essentially organized in alpha helix whereas II and III form beta strands. No signal sequence or transmembrane domain signature is present. EfTu is not showing significant sequence or structural similarities with the NK1 SP human receptor (B). The Staphylococcus epidermidis chaperone DnaK identified as CGRP sensor is a 609 amino acids protein (70 kDa) (C). This protein is showing limited similarity with the human CGRP receptor component protein (CGRP-RCP) but higher similarity with an invertebrate (Ciona intestinalis) CGRP-RCP (124 amino acids) where DnaK was found covering 45% of its sequence with 40% identity (D). Sequence similarities were investigated by BlastP (https://blast.ncbi.nlm). 3D structures were calculated by RaptorX (31) and visualized using Python Molecular Viewer V1.5.6.
SP Sensing by Staphylococci
Further studies revealed that the ability to detect SP is shared by other Gram-positive bacteria such as S. aureus and Staphylococcus epidermidis. These bacteria react to SP by a marked increase in cytotoxicity and virulence on HaCaT keratinocytes and reconstructed human epithelium (RHE) (25). qRT-PCR arrays revealed that the response of RHE to S. aureus and S. epidermidis previously exposed to SP is notably different (25). SP-treated S. aureus induces an upregulation of CCL5 and CXCL1 chemokines and interleukin 8 expression by RHE suggesting the induction of an inflammatory response. Conversely, SP-treated S. epidermidis provoke overexpression of integrin α5 and chemokine ligand 10 CXCL10 (25), two markers of psoriasis (32). Postulating a link between the action of SP on S. epidermidis and psoriasis should be a premature conclusion, but this hypothesis is worthy consideration. To get further insights into the role of SP in promoting S. aureus and S. epidermidis virulence, the effects of the peptide on the adhesion and invasion potential of these bacteria were studied. Exposure of both Staphylococci to SP resulted in a marked increase in their adhesion potential on keratinocytes whereas their invasive activities were unchanged (25). Further studies, based on secretome analysis and biofilm formation activities revealed that S. aureus and S. epidermidis have very different responses to SP. Indeed, although SP has no effect on the release of exoproteins by S. epidermidis, this neuropeptide is stimulating the production of staphylococcal enterotoxin C2 by S. aureus (25). In addition, in S. aureus, SP induces a decrease in the production of lipase, apparently by inhibiting the processing of its precursor (25). Such a metabolic change should favor lipids’ accumulation, and it is well known that a hydrophobic environment is particularly important for the growth of S. aureus (33). Staphylococci also express the moonlighting protein EfTu and, as in B. cereus (24), EfTu was identified as the SP-binding site in S. aureus and S. epidermidis (25). These results suggest that EfTu should act as an SP sensor in a great variety of Gram-positive bacteria, and potentially also in other eubacteria.
SP Sensing by Gram-negative Bacteria
In agreement with this hypothesis, it was observed that Pseudomonas fluorescens, a typical Gram-negative bacterium and member of the commensal skin microflora (1), is also sensitive to SP (34). In this species, the effect of SP is more limited, as no variation of virulence was detected, but SP was found to increase the adhesion and invasive potentials of the bacterium on HaCaT cells (34). In addition, exposure of P. fluorescens to SP is associated with structural rearrangements of the biofilm. Although the SP-binding site was not identified until now in this species, it is interesting to note that, in Pseudomonas, EfTu is also known as an environmental sensor (35).
Effect of Calcitonin Gene-Related Peptide (CGRP) on Staphylococci
Calcitonin gene-related peptide is a neuropeptide abundantly expressed in the skin (9). CGRP is generally co-localized and co-released with SP (36). Two isoforms of this peptide, α-CGRP (or CGRP I) and β-CGRP (or CGRP II), are produced from the same gene by alternative splicing, but α-CGRP is the major form expressed in sensory skin fibers (5). CGRP is known to potentiate the effects of SP on vascular permeability and edema formation. In addition, CGRP exerts trophic effects on endothelial cells and melanocytes. A direct antimicrobial activity of CGRP has been described in E. coli and P. aeruginosa (37). This effect was explained by structural similarities between CGRP and antimicrobial peptides. However, the antimicrobial spectrum of CGRP is narrow, and this peptide was shown without effect on the viability of Staphylococci (37, 38).
Effect of CGRP on S. epidermidis Virulence
When S. epidermidis was exposed to CGRP, an important increase of cytotoxicity and virulence was observed on HaCaT keratinocytes and RHE (38). The threshold of CGRP activity on S. epidermidis is remarkably low (<10−12 M) suggesting a very specific action. Conversely, no effect of CGRP was found in S. aureus (38). As in nerve terminals CGRP is co-secreted with SP, S. epidermidis was exposed simultaneously to both neuropeptides, and it was observed that CGRP and SP have antagonistic activities suggesting the existence of a common step in response of the bacterium to these neuropeptides. After exposure to CGRP, S. epidermidis is leading to an upregulation of interleukin 8 secretion by keratinocytes and RHE, suggesting that CGRP-treated bacteria are activating an inflammatory response. Then, the normal tolerance of the skin to S. epidermidis should be decreased. Because in keratinocytes an inflammatory response is usually associated with the secretion of antimicrobial peptides (39), the production of cathelicidin LL37 and human β defensin 2 (HBD2) by keratinocytes was investigated. However, a limited increase in LL37 secretion and a decrease in HBD2 were observed, suggesting that the effect of CGRP on S. epidermidis is not mediated by antimicrobial peptides (38). Analysis of the secretome of CGRP-treated bacteria did not reveal significant variations in the production of known virulence factors. In fact, CGRP appears to modulate the surface properties of S. epidermidis as CGRP-treated bacteria showed increased adherence to keratinocytes and reduced internalization and biofilm formation activity. These changes appear be associated and may be attributed to an increase in surface hydrophobicity (38).
CGRP Sensing in S. epidermidis
Investigating the CGRP sensor in S. epidermidis was leading to the identification of the chaperone DnaK as a specific CGRP binding protein in this bacterium (38) (Figure 1C). In Staphylococci, this protein related to the heat shock protein Hsp70 is known for its multiple functions in environment and stress adaption (40) and was found as a receptor for endothelial cells (41). Moreover, DnaK is showing sequence similarities with the CGRP receptor component protein (CGRP-RCP), a subunit of the eukaryote CGRP receptor that is required for signal transduction (42) (Figure 1D). Altogether these data suggest that DnaK is another member of the moonlighting proteins family. Moreover, a functional relation has been shown between DnaK and EfTu, the SP sensor. Indeed, in E. coli, DnaK and EfTu are translocated through the inner membrane by the same large mechanosensitive channel MscL (43). The MscL channels are also expressed in the membrane of S. epidermidis, and it was observed that gadolinium chloride, an inhibitor of mechanosensitive channels’ activity, was blocking the response of the bacterium to CGRP (38). Complementary studies based on a ΔmscL mutant confirmed the involvement of MscL in the response of S. epidermidis to CGRP (44). These observations were leading to the hypothesis that the export of DnaK and EfTu through MscL is required for the response of the bacterium to CGRP and SP (38). The initial induction of this process remains a major question as the neuropeptides appear acting both as ligands and signals for the export of DnaK and EfTu. However, it was noted that, even in the absence of stimulation, a limited amount of EfTu (and presumably DnaK) is present in the periplasmic area of S. epidermidis (38), and this pool of proteins should be sufficient for the initial activation step and induction of the export process. In addition, such ionic channels were first characterized as sensors of membrane mechanical stresses, regulating especially the cell turgor. It could also be conceivable that the interaction of some neuropeptides with the bacterial membrane would lead to cell wall mechanical perturbations, and consequently to the activation of MscL and the export of EfTu and DnaK (Figure 2).
Figure 2. Potential mechanism of action of substance P (SP) and calcitonin gene-related peptide (CGRP) on Staphylococcus epidermidis. EfTu and DnaK, bacterial SP and CGRP sensor proteins, respectively, are exported in the periplasmic area through the large mechanosensitive channel MscL. In the periplasm or in the bacterial microenvironment, EfTu and DnaK are, respectively, binding to SP and CGRP. Following a mechanism potentially close to that of bacterial quorum-sensing factors, but that remains to be identified, EfTu-SP and DnaK-CGRP should trigger the bacterial response including increased adhesion to the target cell, biofilm formation, and expression of virulence factors.
Involvement of Other Skin Neuropeptides
As mentioned in Section “Introduction,” many neuropeptides are produced and released in skin but only a few have been evaluated for their potential effects on cutaneous bacteria. Neuropeptide Y, somatostatin, and even POMC-related peptides have been shown to modulate the growth and virulence of bacteria, but until now, not in the context of skin physiology (12). A particular attention should be given to natriuretic peptides produced locally by endothelial cells that have been studied for their effects on Gram-negative bacteria such as Pseudomonas. Indeed, capillary vessels are present in abundance in skin, and especially in a region of the hair follicle, the bulge, at the vicinity of local bacterial populations. Natriuretic peptides, and especially the C type natriuretic peptide (CNP), have been shown to modulate the virulence and adhesion properties of P. aeruginosa (45), a common cutaneous opportunistic pathogen, and P. fluorescens (46), a member of the commensal microflora. The CNP bacterial sensor was recently identified in P. aeruginosa as another moonlighting protein, the amidase AmiC, an ortholog of natriuretic peptide receptor C (47). In fact, cutaneous bacteria should integrate the signals from a multitude of skin neuropeptides and in response adapt their physiology and virulence. Such local effects are also suspected in the case of a bacterium such as Propionibacterium acnes whose acneic strains are particularly virulent in situ but appear without significant virulence when they are grown in vitro (48).
Conclusion
The physiological meaning of these observations and the reasons for the preservation or emergence of sensor systems for skin neuropeptides in cutaneous bacteria remain hypothetical. However, it appears nowadays that in gut, bacteria use hormones and neurotransmitters as signals for switching from a commensal to a pathogen behavior (49). It is interesting to note that, in skin, SP shows important variations of local concentration under the effect of pain, stress, or infection (15, 50, 51) and even in case of nervous breakdown (14). Then, local changes of SP concentration in skin, and presumably CGRP or other peptides, could trigger an increase in the virulence of cutaneous bacteria. These studies give consistence to the existence of a link between the central nervous system, the cutaneous microbiota, and skin homeostasis. Different products, including a polysaccharide rich in rhamnose and a thermal water of particular ionic composition, were found to be able to antagonize the effects of SP on B. cereus, S. aureus, and S. epidermidis (24). Dermocosmetic products have been developed nowadays on the basis of these observations, which also represent a new strategy for clinical applications in dermatology.
Author Contributions
MF wrote the review and designed the figures. MF, OM, and P-JR realized blasts and proteins 3D views. VB, AG, AN, JE, P-JR, VP, SC, and OL revised the manuscript.
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.
The handling Editor declared a shared affiliation, though no other collaboration, with several of the authors AN, AG, VB, JE, P-JR, SC, OL, MF and states that the process nevertheless met the standards of a fair and objective review.
Funding
LMSM is supported by the Communauté d’Agglomération d’Evreux, Conseil Départemental de l’Eure, Région Normandie, BPI (FUI programs), InterReg Program PeReNe, and UE (FEDER).
References
1. Grice EA, Segre JA. The skin microbiome. Nat Rev Microbiol (2011) 9(4):244–53. doi: 10.1038/nrmicro2537
2. Percival SL, Emanuel C, Cutting KF, Williams DW. Microbiology of the skin and the role of biofilms in infection. Int Wound J (2012) 9(1):14–32. doi:10.1111/j.1742-481X.2011.00836.x
3. Feuilloley MGJ, Doleans-Jordheim A, Freney J. Section III – Chapitre 12: Floremicrobienne de la peau saine. 3ème ed. In: de Riegel P, Favennec L, Paugam A, Pozzetto B, editors. Précis de Bactériologie Clinique. Paris: ESKA. (2015). p. 1–15.
4. De Kievit TR, Iglewski BH. Bacterial quorum sensing in pathogenic relationships. Infect Immun (2000) 68(9):4839–49. doi:10.1128/IAI.68.9.4839-4849.2000
5. Roosterman D, Goerge T, Schneider SW, Bunnett NW, Steinhoff M. Neuronal control of skin function: the skin as a neuroimmunoendocrine organ. Physiol Rev (2006) 86(4):1309–79. doi:10.1152/physrev.00026.2005
6. Renaud M, Miget A. Role favorisant des perturbations locales causes par l’adrénaline sur le développement des infections microbiennes. CR Soc Biol Fil (1930) 103:1052–4.
7. Lyte M, Ernst S. Catecholamine induced growth of Gram negative bacteria. Life Sci (1992) 50(3):203–12. doi:10.1016/0024-3205(92)90273-R
8. Lyte M, Freestone PP, Neal CP, Olson BA, Haigh RD, Bayston R, et al. Stimulation of Staphylococcus epidermidis growth and biofilm formation by catecholamine inotropes. Lancet (2003) 361(9352):130–5. doi:10.1016/S0140-6736(03)12231-3
9. Lyte M, Arulanandam BP, Frank CD. Production of Shiga-like toxins by Escherichia coli O157:H7 can be influenced by the neuroendocrine hormone norepinephrine. J Lab Clin Med (1996) 128(4):392–8. doi:10.1016/S0022-2143(96)80011-4
10. Sperandio V, Torres AG, Jarvis B, Nataro JP, Kaper JB. Bacteria-host communication: the language of hormones. Proc Natl Acad Sci U S A (2003) 100(15):8951–6. doi:10.1073/pnas.1537100100
11. Lyte M. Microbial endocrinology and infectious disease in the 21st century. Trends Microbiol (2004) 12(1):14–20. doi:10.1016/j.tim.2003.11.004
12. Lesouhaitier O, Veron W, Chapalain A, Madi A, Blier A-S, Dagorn A, et al. Gram-negative bacterial sensors for eukaryotic signal molecules. Sensors (Basel) (2009) 9(9):6967–90. doi:10.3390/s90906967
13. Lange-Asschenfeldt B, Marenbach D, Lang C, Patzelt A, Ulrich M, Maltusch A, et al. Distribution of bacteria in the epidermal layers and hair follicles of the human skin. Skin Pharmacol Physiol (2011) 24(6):305–11. doi:10.1159/000328728
14. Cizza G, Marques AH, Eskandari F, Christie IC, Torvik S, Silverman MN, et al. Elevated neuroimmune biomarkers in sweat patches and plasma of premenopausal women with major depressive disorder in remission: the POWER study. Biol Psychiatry (2008) 64(10):907–11. doi:10.1016/j.biopsych.2008.05.035
15. Harrison S, Geppetti P. Substance P. Int J Biochem Cell Biol (2001) 33(6):555–76. doi:10.1016/S1357-2725(01)00031-0
16. Severini C, Improta G, Falconieri-Erspamer G, Salvadori S, Erspamer V. The tachykinin peptide family. Pharmacol Rev (2002) 54(2):285–322. doi:10.1124/pr.54.2.285
17. Peters EM, Ericson ME, Hosoi J, Seiffert K, Hordinsky MK, Ansel JC, et al. Neuropeptide control mechanisms in cutaneous biology: physiological and clinical significance. J Invest Dermatol (2006) 126(9):1937–47. doi:10.1038/sj.jid.5700429
18. Ostrowski SM, Belkadi A, Loyd CM, Diaconu D, Ward NL. Cutaneous denervation of psoriasiform mouse skin improves acanthosis and inflammation in a sensory neuropeptide-dependent manner. J Invest Dermatol (2011) 131(7):1530–8. doi:10.1038/jid.2011.60
19. Misery L. Atopic dermatitis: new trends and perspectives. Clin Rev Allergy Immunol (2011) 41(3):296–7. doi:10.1007/s12016-010-8247-6
20. Wallengren J. Substance P antagonist inhibits immediate and delayed type cutaneous hypersensitivity reactions. Br J Dermatol (1991) 124(4):324–8. doi:10.1111/j.1365-2133.1991.tb00591.x
21. Toyoda M, Morohashi M. Pathogenesis of acne. Med Electron Microsc (2001) 34(1):29–40. doi:10.1007/s007950100002
22. Aubdool AA, Brain SD. Neurovascular aspects of skin neurogenic inflammation. J Investig Dermatol Symp Proc (2011) 15(1):33–9. doi:10.1038/jidsymp.2011.8
23. Hillion M, Mijouin L, Jaouen T, Barreau M, Meunier P, Lefeuvre L, et al. Comparative study of normal and sensitive skin aerobic bacterial populations. Microbiologyopen (2013) 2(6):953–61. doi:10.1002/mbo3.138
24. Mijouin L, Hillion M, Ramdani Y, Jaouen T, Duclairoir-Poc C, Follet-Gueye ML, et al. Effects of a neuropeptide (substance P) on cutaneous microflora. PLoS One (2013) 8(11):e78773. doi:10.1371/journal.pone.0078773
25. N’Diaye A, Mijouin L, Hillion M, Diaz S, Konto-Ghiorghi Y, Percoco G, et al. Effect of substance P in Staphylococcus aureus and Staphylococcus epidermidis virulence: implication for skin homeostasis. Front Microbiol (2016) 7:506. doi:10.3389/fmicb.2016.00506
26. De la Fuente-Nunez C, Mertens J, Smit J, Hancock REW. Bacterial surface layer protects against antimicrobial peptides. Appl Environ Microbiol (2012) 78(15):5452–6. doi:10.1128/AEM.01493-12
27. Egelseer E, Schocher I, Sára M, Sleytr UB. The S-layer from Bacillus stearothermophilus DSM 2358 functions as an adhesion site for a high-molecular-weight amylase. J Bacteriol (1995) 177(6):1444–51. doi:10.1128/jb.177.6.1444-1451.1995
28. Beck BD. Polymerization of the bacterial elongation factor for protein synthesis, EF-Tu. Eur J Biochem (1979) 97(2):495–502. doi:10.1111/j.1432-1033.1979.tb13137.x
29. Amblee V, Jeffery CJ. Physical features of intracellular proteins that moonlight on the cell surface. PLoS One (2015) 10(6):e0130575. doi:10.1371/journal.pone.0130575
30. Sela I, Wolf YI, Koonin EV. Theory of prokaryotic genome evolution. Proc Natl Acad Sci U S A (2016) 113(41):11399–407. doi:10.1073/pnas.1614083113
31. Källberg M, Wang H, Wang S, Peng J, Wang Z, Lu H, et al. Template-based protein structure modeling using the RaptorX web server. Nat Protoc (2012) 7(8):1511–22. doi:10.1038/nprot.2012.085
32. Ferrari SM, Ruffilli I, Colaci M, Antonelli A, Ferri C, Fallahi P. CXCL10 in psoriasis. Adv Med Sci (2015) 60:349–54. doi:10.1016/j.advms.2015.07.011
33. Wright JS, Lyon GJ, George EA, Muir TW, Novick RP. Hydrophobic interactions drive ligand-receptor recognition for activation and inhibition of staphylococcal quorum sensing. Proc Natl Acad Sci U S A (2004) 101:16168–73. doi:10.1073/pnas.0404039101
34. Hillion M, Mijouin L, N’Diaye A, Percoco G, Enault J, Follet-Gueye M-L, et al. Pseudomonas fluorescens, a forgotten member of the human cutaneous microflora sensible to skin communication and defense peptides. Int J Curr Microbiol Appl Sci (2014) 3(7):910–25.
35. Dagorn A, Hillion M, Chapalain A, Lesouhaitier O, Duclairoir-Poc C, Vieillard J, et al. Gamma-aminobutyric acid acts as a specific virulence regulator in Pseudomonas aeruginosa. Microbiology (2013) 159:339–51. doi:10.1099/mic.0.061267-0
36. Gibbins IL, Wattchow D, Coventry B. Two immunohistochemically identified populations of calcitonin gene-related peptide (CGRP)-immunoreactive axons in human skin. Brain Res (1987) 414(1):143–8. doi:10.1016/0006-8993(87)91335-7
37. El Karim IA, Linden GJ, Orr DF, Lundy FT. Antimicrobial activity of neuropeptides against a range of micro-organisms from skin, oral, respiratory and gastrointestinal tract sites. J Neuroimmunol (2008) 200(1–2):11–6. doi:10.1016/j.jneuroim.2008.05.014
38. N’Diaye AR, Leclerc C, Kentache T, Hardouin J, Duclairoir Poc C, Konto-Ghiorghi Y, et al. Skin-bacteria communication: involvement of the neurohormone calcitonin gene related peptide (CGRP) in the regulation of Staphylococcus epidermidis virulence. Sci Rep (2016) 6:35379. doi:10.1038/srep35379
39. Angrisano T, Pero R, Paoletti I, Keller S, Lembo L, Baroni A, et al. Epigenetic regulation of IL-8 and β-defensin genes in human keratinocytes in response to Malassezia furfur. J Invest Dermatol (2013) 133(8):2101–4. doi:10.1038/jid.2013.143
40. Singh VK, Syring M, Singh A, Singhal K, Dalecki A, Johansson T. An insight into the significance of the DnaK heat shock system in Staphylococcus aureus. Int J Med Microbiol (2012) 302(6):242–52. doi:10.1016/j.ijmm.2012.05.001
41. Hirschhausen N, Schlesier T, Schmidt MA, Götz F, Peters G, Heilmann C. A novel staphylococcal internalization mechanism involves the major autolysin Atl and heat shock cognate protein Hsc70 as host cell receptor. Cell Microbiol (2010) 12(12):1746–64. doi:10.1111/j.1462-5822.2010.01506.x
42. Evans BN, Rosenblatt MI, Mnayer LO, Oliver KR, Dickerson IM. CGRP-RCP, a novel protein required for signal transduction at calcitonin gene-related peptide and adrenomedullin receptors. J Biol Chem (2000) 275(40):31438–43. doi:10.1074/jbc.M005604200
43. Berrier C, Garrigues A, Richarme G, Ghazi A. Elongation factor Tu and DnaK are transferred from the cytoplasm to the periplasm of Escherichia coli during osmotic downshock presumably via the mechanosensitive channel MscL. J Bacteriol (2000) 182(1):248–51. doi:10.1128/JB.182.1.248-251.2000
44. N’Diaye AR. Skin microbial endocrinology: influence of endogenous peptides on the virulence of cutaneous microflora bacteria. PhD Thesis (2016).
45. Veron W, Lesouhaitier O, Pennanec X, Rehel K, Leroux P, Orange N, et al. Natriuretic peptides affect Pseudomonas aeruginosa and specifically modify lipopolysaccharide biosynthesis. FEBS J (2007) 274(22):5852–64. doi:10.1111/j.1742-4658.2007.06109.x
46. Veron W, Orange N, Feuilloley MG, Lesouhaitier O. Natriuretic peptides modify Pseudomonas fluorescens cytotoxicity by regulating cyclic nucleotides and modifying LPS structure. BMC Microbiol (2008) 8:114. doi:10.1186/1471-2180-8-114
47. Rosay T, Bazire A, Diaz S, Clamens T, Blier AS, Mijouin L, et al. Pseudomonas aeruginosa expresses a functional human natriuretic peptide receptor ortholog: involvement in biofilm formation. MBio (2015) 6(4):e1033–1015. doi:10.1128/mBio.01033-15
48. Ionescu MA, Feuilloley M, Enault J, Saguet T, Robert G, Lefeuvre L. La modulation du microbiofilm et du P. acnes ribotypes 4 et 5 dans l’acné polymorphe: étude microbiologique et clinique dans une série de 70 adultes acnéiques. Ann Dermato Venereo (2015) 142:S434–5. doi:10.1016/j.annder.2015.10.030
49. Sandrini S, Aldriwesh M, Alruways M, Freestone P. Microbial endocrinology: host-bacteria communication within the gut microbiome. J Endocrinol (2015) 225(2):R21–34. doi:10.1530/JOE-14-0615
50. Nakano Y. Stress-induced modulation of skin immune function: two types of antigen-presenting cells in the epidermis are differentially regulated by chronic stress. Br J Dermatol (2004) 151(1):50–64. doi:10.1111/j.1365-2133.2004.05980.x
Keywords: skin bacterial communication, substance P, calcitonin gene-related peptide, DnaK chaperone protein, EfTu thermo unstable ribosomal elongation factor, MscL mechanosensitive channel, moonlighting proteins, microbial endocrinology
Citation: N’Diaye A, Gannesen A, Borrel V, Maillot O, Enault J, Racine P-J, Plakunov V, Chevalier S, Lesouhaitier O and Feuilloley MGJ (2017) Substance P and Calcitonin Gene-Related Peptide: Key Regulators of Cutaneous Microbiota Homeostasis. Front. Endocrinol. 8:15. doi: 10.3389/fendo.2017.00015
Received: 03 November 2016; Accepted: 16 January 2017;
Published: 30 January 2017
Edited by:
Hubert Vaudry, University of Rouen, FranceReviewed by:
Kazuhiro Takahashi, Tohoku University, JapanJohn Michael Conlon, Ulster University, UK
Copyright: © 2017 N’Diaye, Gannesen, Borrel, Maillot, Enault, Racine, Plakunov, Chevalier, Lesouhaitier and Feuilloley. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Marc G. J. Feuilloley, bWFyYy5mZXVpbGxvbGV5JiN4MDAwNDA7dW5pdi1yb3Vlbi5mcg==