With interest we read the paper by Juste et al 1 proposing the amount of zymogen-granule membrane glycoprotein 2 (GP2) on the surface of intestinal bacteria as a Crohn\u27s disease (CD) marker. Indeed, a decreased GP2 level was found on microbes in patients with CD as compared to those of healthy controls. GP2 is a homologue to the urinary Tamm–Horsefall protein demonstrating an antimicrobial function by binding type 1-fimbriated uropathogenic Escherichia coli (UPEC). Likewise, GP2 seems to interact with intestinal bacteria as a specific receptor of bacterial type-1 fimbriae (FimH) on intestinal microfold cells that are partaking in immune responses against such microbes.2 GP2 is overexpressed in the inflamed intestine of patients with CD and has an immunomodulating role in innate and acquired immune responses.3 ,4Interestingly, GP2 was identified as autoantigen of pancreatic antibodies in CD.4 Altogether, these findings indicate two major GP2 sources (pancreatic/intestinal) and support a role for GP2 in the interaction between the immune system and intestinal microbiota.3 Thus, loss of tolerance to GP2 could play a role in CD\u27s pathophysiology supposed to be exacerbated by preceding intestinal infections. In general, the findings by Juste et al 1 may be explained by a lower pancreatic GP2 secretion, an impaired GP2 binding to bacteria, or by a higher prevalence of bacteria with poor or no GP2 binding in patients with CD

Berger, Enrico

Grzymajło, Krzysztof

Hiemann, Rico

Juretzek, Thomas

Kolenda, Rafal

Meissner, Dirk

Mydlak, Karsten

Nolan, Lisa

Reinhold, Dirk

Roggenbuck, Dirk

Rödiger, Stefan

Schierack, Peter

Swidsinski, Alexander

English

With interest we read the paper by Juste et al 1 proposing the amount of zymogen-granule membrane glycoprotein 2 (GP2) on the surface of intestinal bacteria as a Crohn's disease (CD) marker. Indeed, a decreased GP2 level was found on microbes in patients with CD as compared to those of healthy controls. GP2 is a homologue to the urinary Tamm–Horsefall protein demonstrating an antimicrobial function by binding type 1-fimbriated uropathogenic Escherichia coli (UPEC). Likewise, GP2 seems to interact with intestinal bacteria as a specific receptor of bacterial type-1 fimbriae (FimH) on intestinal microfold cells that are partaking in immune responses against such microbes.2 GP2 is overexpressed in the inflamed intestine of patients with CD and has an immunomodulating role in innate and acquired immune responses.3 ,4Interestingly, GP2 was identified as autoantigen of pancreatic antibodies in CD.4 Altogether, these findings indicate two major GP2 sources (pancreatic/intestinal) and support a role for GP2 in the interaction between the immune system and intestinal microbiota.3 Thus, loss of tolerance to GP2 could play a role in CD's pathophysiology supposed to be exacerbated by preceding intestinal infections. In general, the findings by Juste et al 1 may be explained by a lower pancreatic GP2 secretion, an impaired GP2 binding to bacteria, or by a higher prevalence of bacteria with poor or no GP2 binding in patients with CD.This article is from Gut 64 (2015): 517–519, doi:10.1136/gutjnl-2014-307854. Posted with permission.</p

Digital Repository @ Iowa State University (ISU)

response before measuring any drug orantidrug antibody levels. Without thecorrect context of loss of response, inter-pretation of drug and antidrug antibodylevels would be inappropriate, especiallyso when drug levels are found to be oftherapeutic levels. When properlydefined, customised treatment based ontherapeutic drug monitoring will avoidunhelpful dose-intensification of biologicsfor some patients and be cost-efficientfrom a macro-economic level.Nevertheless, I would like to congratu-late the authors for undertaking the taskof demonstrating the cost effectiveness ofindividualised biologic therapy forpatients with complicated CD in the eraof personalised medicine.Malcolm TanCorrespondence to Dr Malcolm Tan, Department ofGastroenterology and Hepatology, Changi GeneralHospital, 2 Simei Street 3, Singapore 529889,Singapore; dr.malcolm@gmail.comCompeting interests None.Provenance and peer review Not commissioned;internally peer reviewed.To cite Tan M. Gut 2015;64:516–517.Received 17 June 2014Accepted 1 July 2014Published Online First 16 July 2014Gut 2015;64:516–517.doi:10.1136/gutjnl-2014-307877REFERENCES1 Steenholdt C, Brynskov J, Thomsen OØ, et al.Individualised therapy is more cost-effective than doseintensification in patients with Crohn’s disease wholose response to anti-TNF treatment: a randomised,controlled trial. Gut 2014;63:919–27.2 Lahiff C, Safaie P, Awais A, et al. The Crohn’s diseaseactivity index (CDAI) is similarly elevated in patientswith Crohn’s disease and in patients with irritablebowel syndrome. Aliment Pharmacol Ther2013;37:786–94.3 Solberg IC, Vatn MH, Høie O, et al.; IBSEN StudyGroup. Clinical course in Crohn’s disease: results of aNorwegian population-based ten-year follow-up study.Clin Gastroenterol Hepatol 2007;5:1430–8.Species-specific andpathotype-specific bindingof bacteria to zymogengranule membraneglycoprotein 2 (GP2)Dear Editor,With interest we read the paper by Justeet al1 proposing the amount of zymogen-granule membrane glycoprotein 2 (GP2)on the surface of intestinal bacteria as aCrohn’s disease (CD) marker. Indeed, adecreased GP2 level was found onmicrobes in patients with CD as comparedto those of healthy controls. GP2 is ahomologue to the urinary Tamm–Horsefall protein demonstrating an anti-microbial function by binding type1-fimbriated uropathogenic Escherichiacoli (UPEC). Likewise, GP2 seems tointeract with intestinal bacteria as a spe-cific receptor of bacterial type-1 fimbriae(FimH) on intestinal microfold cells thatare partaking in immune responses againstsuch microbes.2 GP2 is overexpressed inthe inflamed intestine of patients with CDand has an immunomodulating role ininnate and acquired immune responses.3 4Interestingly, GP2 was identified as auto-antigen of pancreatic antibodies in CD.4Altogether, these findings indicate twomajor GP2 sources (pancreatic/intestinal)and support a role for GP2 in the inter-action between the immune system andintestinal microbiota.3 Thus, loss ofFigure 1 Binding of Escherichia coli pathotypes to GP2. Human recombinant GP2 expressedin Sf9 cells were immobilised on 96-well plates with anti-FimH antibodies used as positive, orhuman serum albumin as negative controls. After incubation of bacterial suspensions for 2 hfollowed by subsequent washing, bound bacteria were stained with a fluorescent dye andcounted with an automated fluorescence interpretation system (Aklides, Medipan, Dahlewitz,Germany). Bound bacteria are represented as bacteria per image (bpi, image=0.61 mm2). UPEC:human uropathogenic E. coli (n=24), HFEC: human intestinal commensal (fecal) E. coli (n=24),ETEC: human enterotoxigenic E. coli (n=24), EPEC: human enteropathogenic E. coli (n=24),SAEC: sepsis-associated human E. coli isolated from sepsis patients (n=24), EAEC: humanenteroaggregative E. coli (n=17), AFEC: chicken intestinal commensal (avian fecal) E. coli (n=24),CAEC: Crohn’s disease-associated E. coli isolated from patients with Crohn’s disease (n=20),Salmonella: Salmonella serovar (n=24), Klebsiella: Klebsiella pneumoniae (n=12), Proteus: Proteusmirabilis (n=12), Buttiauxella (n=6), Pantoea: Pantoea agglomerans (n=5), Raoultella: Raoultellaornithinolytica (n=7), Serratia: Serratia fonticola/liquefaciens (n=6), and methillicin-resistantStaphylococcus aureus: MRSA (n=24). Data are displayed as bpi in box-and-whisker plots with farout values, defined as values that are smaller than the lower quartile minus 3 times the IQR, orlarger than the upper quartile plus 3 times the IQR, displayed as solid triangles. Posthoc analysis,p<0.05 for the following comparisons: UPEC: ETEC, EAEC, Salmonella, Buttiauxella, Pantoea,Serratia, MRSA. HFEC: ETEC, EAEC, Salmonella, Proteus, Buttiauxella, Pantoea, Serratia, MRSA.ETEC: UPEC, HFEC, EPEC, SAEC, AFEC, CAEC, Salmonella, Klebsiella, Buttiauxella, Pantoea,MRSA. EPEC: ETEC, EAEC, Salmonella, Proteus, Buttiauxella, Pantoea, Serratia, MRSA. SAEC:ETEC, EAEC, Salmonella, Buttiauxella, Pantoea, Serratia, MRSA. EAEC: UPEC, HFEC, EPEC, SAEC,AFEC, CAEC, Salmonella, Klebsiella, Buttiauxella, Pantoea. AFEC: ETEC, EAEC, Salmonella,Buttiauxella, Pantoea, Serratia, MRSA. CAEC: ETEC, EAEC, Salmonella, Buttiauxella, Pantoea,Serratia, MRSA. Salmonella: UPEC, HFEC, ETEC, EPEC, SAEC, EAEC, AFEC, CAEC, Klebsiella,Proteus, Buttiauxella, Pantoea, Raoultella, Serratia, MRSA. Klebsiella: ETEC, EAEC, Salmonella,Buttiauxella, Pantoea, Serratia, MRSA. Proteus: HFEC, EPEC, Salmonella, Buttiauxella, Pantoea,MRSA. Buttiauxella: UPEC, HFEC, ETEC, EPEC, SAEC, EAEC, AFEC, CAEC, Salmonella, Klebsiella,Proteus, Raoultella. Pantoea: UPEC, HFEC, ETEC, EPEC, SAEC, EAEC, AFEC, CAEC, Salmonella,Klebsiella, Proteus, Raoultella. Raoultella: Salmonella, Buttiauxella, Pantoea, MRSA. Serratia:UPEC, HFEC, EPEC, SAEC, AFEC, CAEC, Salmonella, Klebsiella. MRSA: UPEC, HFEC, ETEC, EPEC,SAEC, AFEC, CAEC, Salmonella, Klebsiella, Proteus, Raoultella.PostScriptGut March 2015 Vol 64 No 3 517group.bmj.com on May 26, 2015 - Published by http://gut.bmj.com/Downloaded from tolerance to GP2 could play a role inCD’s pathophysiology supposed to beexacerbated by preceding intestinal infec-tions. In general, the findings by Justeet al1 may be explained by a lower pan-creatic GP2 secretion, an impaired GP2binding to bacteria, or by a higher preva-lence of bacteria with poor or no GP2binding in patients with CD.We have a longstanding interest in GP2’sintestinal function and, therefore, we eval-uated GP2 as receptor for intestinalbacterial pathotypes by testing the bindingof 284 bacteria in a novel binding assay.5These bacteria were of 8 E. coli patho-types, 8 Salmonella serovars, 6 otherEnterobacteriaceae genera (Klebsiella,Proteus, Buttiauxella, Pantoea, Raoultella,Serratia), and methicillin-resistantStaphylococcus aureus (MRSA) (figure 1).Binding rates of isolates ranged from 0 to2117 bacteria per image (bpi), andSalmonella isolates exhibited the signifi-cantly highest binding to GP2; whereas,Proteus, Buttiauxella, Pantoea, Raoultella,Serratia and MRSA isolates demonstratedlow binding (Kruskal–Wallis test,p<0.000001). E. coli pathotypes andKlebsiella expressed medium binding rates.CD-associated E. coli (CAEC) demon-strated no significantly different binding toGP2 than human commensal (fecal) E. coli(HFEC); sepsis-associated E. coli; UPEC,enteropathogenic E. coli (EPEC) or chickencommensal (avian fecal) E. coli, but ahigher binding than enterotoxigenic E. coliand human enteroaggregative E. coli(posthoc analysis, p<0.05, respectively).Nine out of 10 fimH-negative isolatesshowed low binding to GP2, andone HFEC isolate a high binding rate(473 bpi). GP2 binding of Salmonella,E. coli and other bacterial groupswas mannose-sensitive and not glucose-sensitive as shown by inhibition experi-ments proving a GP2-FimH interaction.To investigate the interaction betweenFimH-protein and GP2 at a molecularlevel, we sequenced fimH genes of 48E. coli isolates: six isolates of each patho-type including two isolates not bindingto GP2, two isolates showing mediumand two isolates showing strong binding.Thus, we defined 23 different FimH-amino acid sequences. Though there wasno specific FimH-amino acid sequencevariation for an E. coli pathotype, FimHsequences seem to correlate with thestrength of binding of GP2 to bacteria(figure 2). Additionally, bacterial bindingto GP2 correlated significantly with thatto anti-FimH antibodies, indicating thatFimH-expression levels are associatedwith GP2 binding (p<0.0001, see onlinesupplementary data).We conclude that GP2 is an intestinalepithelial receptor interacting with dis-tinct FimH-positive bacteria. This inter-action can be modulated by pancreaticGP2 secreted together with zymogensinto the intestine. GP2 binding is select-ive for bacterial species and pathotypesand, thus, may determine immuneresponses to the intestinal microbiota.CAEC do not differ in their bindingfrom most E. coli isolates supporting theFigure 2 Correlation between the FimH-amino acid sequences and binding to GP2. E. coliisolates with different binding characteristics to GP2 (n=48) were sequenced and clusteredaccording to the FimH-amino acid sequences. Data on each isolate are: isolate collection number,pathotype, binding to GP2 (low adhesion: <20 bpi; medium adhesion: 50–100 bpi; highadhesion: >300 bpi). UPEC: human uropathogenic E. coli, HFEC: human intestinal (fecal)commensal E. coli, ETEC: human enterotoxigenic E. coli, EPEC: human enteropathogenic E. coli,SAEC: sepsis-associated human E. coli isolated from patients with sepsis, EAEC: humanenteroaggregative E. coli, AFEC: chicken intestinal (avian fecal) commensal E. coli, CAEC: Crohn’sdisease-associated human intestinal E. coli from patients with Crohn’s disease.PostScript518 Gut March 2015 Vol 64 No 3group.bmj.com on May 26, 2015 - Published by http://gut.bmj.com/Downloaded from assumptions that other bacteria with lowGP2 binding are more abundant in CD,or the GP2 interaction with CAEC isimpaired.Peter Schierack,1 Stefan Rödiger,1Rafal Kolenda,1 Rico Hiemann,1 Enrico Berger,1Krzysztof Grzymajło,2 Alexander Swidsinski,3Thomas Juretzek,4 Dirk Meissner,5Karsten Mydlak,6 Dirk Reinhold,7 Lisa K Nolan,8Dirk Roggenbuck1,91Faculty of Natural Sciences, Brandenburg Universityof Technology Cottbus—Senftenberg, Senftenberg,Germany2University of Environmental and Life Sciences,Wroclaw, Poland3Innere Klinik, Gastroenterologie, Charité HumboldtUniversität, Berlin, Germany4Carl-Thiem-Klinikum, Cottbus, Germany5Labor Hameln Hildesheim, Hameln, Germany6Gemeinschaftslabor Cottbus, Cottbus, Germany7Institute of Molecular and Clinical Immunology,Otto-von-Guericke University Magdeburg, Magdeburg,Germany8Department of Veterinary Microbiology and PreventiveMedicine, College of Veterinary Medicine, Iowa StateUniversity, Ames, Iowa, USA9GA Generic Assays GmbH, Dahlewitz, GermanyCorrespondence to Professor Dirk Roggenbuck,Faculty of Natural Sciences, Brandenburg University ofTechnology Cottbus—Senftenberg, Großenhainer Str.57, Senftenberg 01968, Germany; dirk.roggenbuck@hs-lausitz.deContributors DRo, DRe and PS conceived of thestudy and participated in its design and coordinationand helped to draft the manuscript. SR, RK, EB, andKG carried out the experiments. RH developed thepattern recognition algorithms. LKN, DM, KM, AS, andTJ provided the bacterial isolates. All authors read andapproved the final manuscript.Competing interests DRo is a shareholder of GAGeneric Assays GmbH and Medipan GmbH. Theremaining authors declare that they have no competingfinancial interests.Provenance and peer review Not commissioned;internally peer reviewed.▸ Additional material is published online only. To viewplease visit the journal online (http://dx.doi.org/10.1136/gutjnl-2014-307854).Open Access This is an Open Access articledistributed in accordance with the Creative CommonsAttribution Non Commercial (CC BY-NC 4.0) license,which permits others to distribute, remix, adapt, buildupon this work non-commercially, and license theirderivative works on different terms, provided theoriginal work is properly cited and the use is non-commercial. See: http://creativecommons.org/licenses/by-nc/4.0/To cite Schierack P, Rödiger S, Kolenda R, et al. Gut2015;64:517–519.Received 14 June 2014Accepted 3 July 2014Published Online First 29 July 2014Gut 2015;64:517–519.doi:10.1136/gutjnl-2014-307854REFERENCES1 Juste C, Kreil DP, Beauvallet C, et al. Bacterial proteinsignals are associated with Crohn’s disease. Gut2014;63:1566–77.2 Hase K, Kawano K, Nochi T, et al. Uptake throughglycoprotein 2 of FimH(+) bacteria by M cellsinitiates mucosal immune response. Nature 2009;462:226–30.3 Roggenbuck D, Reinhold D, Schierack P, et al. Crohn’sdisease specific pancreatic antibodies: clinical andpathophysiological challenges. Clin Chem Lab Med2014;52:483–94.4 Roggenbuck D, Hausdorf G, Martinez-Gamboa L,et al. Identification of GP2, the major zymogengranule membrane glycoprotein, as the autoantigen ofpancreatic antibodies in Crohn’s disease. Gut2009;58:1620–8.5 Frommel U, Lehmann W, Rodiger S, et al. Adhesion ofhuman and animal Escherichia coli strains inassociation with their virulence-associated genes andphylogenetic origins. Appl Environ Microbiol2013;79:5814–29.The effect of exercise and dieton gut microbial diversityWe have read with great interest the studyby Clarke et al1 who in a very elegant andsophisticated manner documented theincrease in gut microbial diversity in associ-ation with exercise and dietary extremes inprofessional rugby players. The observedmicrobial shifts were accompanied by lowerinflammatory and healthier metabolic pro-files among athletes. Significantly higherproportions of the genus Akkermansiamuciniphila in athletes as well as in lowBody Mass Index control group werefound. As previously shown, the presenceof these bacteria in the human GI tract hasbeen associated with improved metabolicprofiles, possibly due to enhanced barrierfunction. However, from the study ofClarke et al it is difficult to draw the con-clusion and assess the impact of exerciseper se from dietary influences in groupsstudied for their gut microbial diversity. Asthe alterations of the microbial diversityhave already been linked to changes indietary habits, it is important to address animportant issue, which is the reported highprevalence of GI presentations among pro-fessional athletes. Endurance training hasbeen associated with reduced GI bloodflow, tissue hyperthermia and hypoxialeading to possible alterations of microbiotaand GI barrier. As documented in a well-designed and randomised, double-blinded,placebo-controlled trial, probiotic supple-mentation affected markers of intestinalbarrier, oxidation and inflammation intrained men. Lamprecht et al have shownthat a 14-week period of supplementationwith multi-species probiotics in trainedmen led to normalisation of stool zonulinconcentrations (a marker indicatingenhanced gut permeability) as comparedwith the placebo group. The researchersfound no effect of exercise on tumournecrosis factor-α serum concentrations.2Other studies with high endurance athletesdocumented beneficial effects of dietaryinterventions on improvements in cytokinesand immune-marker panels, positive effectson redox biology and lessening of GI symp-toms. As implicated in the study by Clarkeet al, the gut microbial diversity may beviewed as a new biomarker or indicator ofhealth. However, Wills et al3 in their recentprospective study using next-generationsequencing for examining the faecal micro-biota composition in patients with IBDduring a quiescent disease phase and a sub-sequent exacerbation could not demon-strate general changes in microbialcomposition or diversity in both groupsstudied. Of importance, a large increase inrelative abundance of Bacteroides fragilis orAkkermansia muciniphila during activephase of disease in some of patients wasreported.3 Other studies document thatprolonged strenuous exercise expands thepopulation of developmentally early stemcells in bone marrow and mobilises theminto peripheral blood (personal communi-cation, Dr Ratajczak, University ofLousiville, USA).4 The precise mechanismof this phenomenon is not known;however, it could play an important role intissue/organ rejuvenation after strenuousexercise. Our group has documented anincrease in mobilisation of stem and pro-genitor cells into peripheral blood inpatients with active IBD.5 It is difficult toexclude that these health effects are at leastin part mediated by gut derived bacteriallipopolysaccharides (endotoxins), whichenter the general circulation due toimpaired gut barrier integrity and increasedintestinal permeability—factors whichcould be considered more important healthdeterminants than microbial compositionitself. It would be very tempting to addressthe role of intestinal barrier (eg, by measur-ing intestinal markers such as intestinal-fattyacid binding protein or zonulin) or tomeasure the levels of serum endotoxin infuture studies investigating the effect ofexercise and diet on gut microbiota.Observations that antibiotic treatmentabolishes stem/progenitor cell mobilisationOpen AccessScan to access morefree contentPostScriptGut March 2015 Vol 64 No 3 519group.bmj.com on May 26, 2015 - Published by http://gut.bmj.com/Downloaded from membrane glycoprotein 2 (GP2)binding of bacteria to zymogen granule Species-specific and pathotype-specificRoggenbuckDirk Meissner, Karsten Mydlak, Dirk Reinhold, Lisa K Nolan and DirkBerger, Krzysztof Grzymajlo, Alexander Swidsinski, Thomas Juretzek, Peter Schierack, Stefan Rödiger, Rafal Kolenda, Rico Hiemann, Enricodoi: 10.1136/gutjnl-2014-3078542015 64: 517-519 originally published online July 29, 2014Gut  http://gut.bmj.com/content/64/3/517Updated information and services can be found at: These include:MaterialSupplementary htmlhttp://gut.bmj.com/content/suppl/2014/07/23/gutjnl-2014-307854.DC1.Supplementary material can be found at: References #BIBLhttp://gut.bmj.com/content/64/3/517This article cites 4 articles, 2 of which you can access for free at: serviceEmail alertingbox at the top right corner of the online article. Receive free email alerts when new articles cite this article. Sign up in theCollectionsTopic Articles on similar topics can be found in the following collections  (197)Open accessNoteshttp://group.bmj.com/group/rights-licensing/permissionsTo request permissions go to:http://journals.bmj.com/cgi/reprintformTo order reprints go to:http://group.bmj.com/subscribe/To subscribe to BMJ go to:group.bmj.com on May 26, 2015 - Published by http://gut.bmj.com/Downloaded from 

Species-specific and pathotype-specific binding of bacteria to zymogen granule membrane glycoprotein 2 (GP2)

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Species-specific and pathotype-specific binding of bacteria to zymogen granule membrane glycoprotein 2 (GP2)

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