Recombinant lytic and GFP-CBD fusion proteins based on the Listeria phage endolysin Ply511

Recombinant lytic and GFP-CBD fusion proteins based on the Listeria phage endolysin Ply511 Diploma Thesis Lisa Conza Supervised by Mathias Schmelcher

Introduction Materials & Methods Results Overview Discussion & Outlook Recombinant endolysins • Introduction • Methods & Results • Conclusions • Outlook

Introduction Materials & Methods Results Overview Discussion & Outlook Listeria • Listeria are Gram-positive, non-spore forming, facultative anaerobic, short, rods • tolerates temperature between -0.4 - 50°C • pH optimum at pH 6-8 food borne pathogen causes epidemic or sporadic illness • motility performed by peritrichous flagella Listeria (Loessner, 2005)

Introduction Materials & Methods Results Overview Discussion & Outlook Bacteriophages • is a broad-host-range bacteriophage • is virulent, it can lyse approximately 95% of Listeria strains 1/2 and 4 • 96% of phages are tailed • classified in the order of the Caudovirales • subdivided into three families: Siphoviridae, Podoviridae, Myoviridae (A511) A511 Bacteriophage A511, the black bar is 50 nm (Ackermann, 2006)

Introduction Materials & Methods Results Overview Discussion & Outlook (Korndörfer et al., 2006) Endolysins • endolysins (bacteriophage lysins) are proteins which work as cell wall-hydrolyzing enzymes • produced in bacteriophage’s lytic cycle • with modular organization N C EAD CBD

Introduction Materials & Methods Results Overview Discussion & Outlook Dualistic model • The phage mediated cell lysis works in a dualistic system: -holin is inserted in the cytoplasmic membrane ->form hole (membrane disruption) ->endolysins can pass through (access the peptidoglycan layer) Loessner, 2005, modified.

Introduction Materials & Methods Results Overview Discussion & Outlook Alignment of three ply genes C Ply006 N C Ply118 N C Ply511 N • CBD118 and CBD006 have very similar binding range for serovars (1/2) and have high sequence homology at C-terminus • CBD511 and CBD118 are similar in sequence at N-terminus • Affinity to the cells of CBD006 is 100-fold lower then that of CBD118

Introduction Materials & Methods Results Overview Discussion & Outlook KPSTPAPKPSTPSTNLDKLGLVDYMNAKKMDSSYSNRDKLAK QYGIANYSSGTASQNTTLLSKIKGGAPKPSTPAPKPST EAD CBD Ply511 • Ply511 is an N-acetylmuramoyl-L-alanine amidase • molecular mass of 36.5kDa Loessner, 2005, modified.

Introduction Materials & Methods Results Overview Discussion & Outlook Aim of my work test for binding properties 1) HGFP_CBD constructs test for lytic activity 2) HEAD_CBD constructs

Introduction Materials & Methods Results Overview Discussion & Outlook Methods • Construction of pHGFP_CBD plasmids -fragments amplification and ligation in pHGFP -protein overexpression and purification -protein binding assays • Construction of pHEAD_CBD plasmids -EAD fragment instead of the GFP gene -proteins overexpression and purification -protein photometric lysis assays and overlay assays

Introduction Materials & Methods Results Overview Discussion & Outlook EAD S S CBD2 CBD1 S CBD1 S CBD2 S CBD2 CBD1 CBD1 S CBD1 S CBD1 CBD1 S S CBD2 S CBD2 CBD amplification

Introduction Materials & Methods Results Overview Discussion & Outlook 250 CBD fragment amplification M CBDS1 CBD2 Size [bp] • PCR amplifications • -line 1 M • -line 2 CBDS1 • -line 3 CBD2 500

Introduction Materials & Methods Results Overview Discussion & Outlook BamHI SphI SacI KpnI SmaI XmaI SalI PstI HindIII PT5 - lac O - lac O – RBS – ATG - 6xHis – MCS - Stop Codons pQE-30 3.4 kb Ampicillin Col E1 pQE-30 and pHGFP • pHGFP derived from pQE-30 vector (Loessner et al. 2002) • 4.159 kb cloning and expression vector • GFP gene inserted between BamHI and SacI • CBD fragments ligated downstream the GFP gene (Sacl/SalI)

Introduction Materials & Methods Results Overview Discussion & Outlook CBD1 CBD2 GFP SacI BamHI SalI MCS Ampicillin pHGFP Col E1 Construction of HGFP_CBD fusion proteins • pHGFP extraction from E.coli JM109 • SacI and SalI digestion of pHGFP and the CBD fragments • ligation of plasmids with fragmens • E.coli XL1-Blue electroporation • colony PCR

Introduction Materials & Methods Results Overview Discussion & Outlook CBD1 CBD2 GFP S S CBD1 CBD2 GFP S CBD1 GFP S CBD1 GFP CBD1 GFP S CBD1 GFP S S CBD2 GFP S CBD2 GFP HGFP_CBD constructs

Introduction Materials & Methods Results Overview Discussion & Outlook M 1 2 3 4 5 6 Size [bp] Size [bp] 750 1000 250 GFP_CBD plasmids CBD2 M CBD2 M pHGFP 4000 500 • Colony PCR of pHGFP_CBDS2 250 • SacI and SalIdigestion of pHGFP and of CBD2

Introduction Materials & Methods Results Overview Discussion & Outlook EAD HEAD_CBD constructs • PCR amplification of EAD511 coding region (BamHI/SacI sites) • excision of GFP fragment from HGFP_CBD constructs • insertion of EAD fragment CBD1 CBD2 GFP S S

Introduction Materials & Methods Results Overview Discussion & Outlook CBD2 CBD1 S S EAD S EAD CBD1 EAD CBD1 S CBD1 EAD S CBD1 S EAD CBD2 S EAD CBD2 EAD EAD HEAD_CBD constructs

Introduction Materials & Methods Results Overview Discussion & Outlook Size [bp] M EAD Size [bp] 4000 3500 2000 750 GFP 750 550 500 EAD amplified with PCR HEAD_CBD constructs pHGFP_CBD1S digestion with BamHI/SacI. For purification the plasmids are cut out from the gel

Introduction Materials & Methods Results Overview Discussion & Outlook tested in binding assay with Listeria strains tested in lysis assays with Listeria WSLC 1001 and in overlay assays with Listeria WSLC 1001 and WSLC 1020 Protein preparations • control of overexpression and purification • -activity test protein purification with IMAC (Ni-NTA gravity flow columns) E.coli overexpression cell disruption (French Press) HGFP_CBD fusion proteins HEAD constructs

Introduction Materials & Methods Results Overview Discussion & Outlook Results • HGFP_CBD fusion proteins • HEAD, HEAD_CBD fusion proteins

Introduction Materials & Methods Results Overview Discussion & Outlook M 0h 1h 2h 4h CE Flow Wash Elute c.E. Size [kDa] 116.0 66.2 37.5 kDa HGFP_CBDS1S 45.0 35.0 25.0 18.4 14.4 • SDS-PAGE analysis of 6x his-tagged HGFP_CBDS1S • Overexpression was performed in E.coli XL-1 Blue MRF’ and induced with IPTG SDS-PAGE

Introduction Materials & Methods Results Overview Discussion & Outlook Binding assay • ON cultures of Listeria cells • 100 µl of the centrifuged cells resuspended in 1 ml PBST were incubated with excess of fusion protein • 2 wash step with 500 µl PBST

Introduction Materials & Methods Results Overview Discussion & Outlook -binding assay of fusion protein HGFP_CBDS1S2to Listeria strain WSLC 1033. Binding assay

Introduction Materials & Methods Results Overview Discussion & Outlook Binding properties of different HGFP_CBD constructs Interpretation of binding properties: ++ cells displayed an intensive green fluorescence + cells visible with lower intensity (+)very weak signal - no signal

Introduction Materials & Methods Results Overview Discussion & Outlook Binding assay SacI CBDS1 Linker PSA GFP H kpnI SalI • HGFP_LPSA_CBD constructs with a PSA linker are tested in binding assays • results obtained are very similar of those displayed by the HGFP_CBD proteins

Introduction Materials & Methods Results Overview Discussion & Outlook Binding assay • HGFP_CBD “1” constructs don’t bind Listeria cells • HGFP_CBD “2” constructs bind the different Listeria cells • Confirmation of the idea that give the alignments of the three endolysins

Introduction Materials & Methods Results Overview Discussion & Outlook HEAD_CBD constructs • HEAD_CBD tested in -lysis assays -overlay assays

Introduction Materials & Methods Results Overview Discussion & Outlook Lysis assay • Equimolar amounts of all HEAD constucts • Positive control: HPL511 (Loessner et al., 1996) • Listeria WSLC 1001 • OD600 measurement in photometer after addition of enzyme • Steepest slope of the lysis curve corresponds to relative activity

Introduction Materials & Methods Results Overview Discussion & Outlook Lysis assay • Lysis curve of EAD_CBD1S is representative for all the CBD1 constructs • Lysis curve of EADS2 represent the all the CBD2 constructs • HPL511 used as positive control OD600 Time[seconds]

Introduction Materials & Methods Results Overview Discussion & Outlook Lysis assay • Lysis curves of HEAD_CBD“2“ constructs showed strong lytic activity • HEAD_CBD“1“ constructs: low activity • Lytic properties correspond to the binding properties of the CBD constructs

Introduction Materials & Methods Results Overview Discussion & Outlook Overlay assays • E.coli plated on IPTG plates • incubation 4 h • disruption of the cell membrane with chloroform • Plate overlayed with Listeria cells in soft agar

Introduction Materials & Methods Results Overview Discussion & Outlook Overlay assays -left: Listeria WSLC 1001; right:Listeria WSLC 1020

Introduction Materials & Methods Results Overview Discussion & Outlook Overlay assays -left: Listeria WSLC 1020 HEAD_CBD“1“ -right:Listeria WSLC1020 HEAD_CBD“2“

Introduction Materials & Methods Results Overview Discussion & Outlook Overlay assays • HEAD_CBD“1“: big lysis zone, unclear boundaries > protein is able to diffuse • HEAD_CBD“2“: smaller, well defined boundaries > higher affinity

Introduction Materials & Methods Results Overview Discussion & Outlook Conclusions 1 • The HGFP-CBD”1” fusion proteins don’t bind the different Listeria strains • Binding properties seem to be mainly located in the CBD”2” part • The isolated CBD”1” part seems not to play any role in binding • The HGFP-CBD proteins containing the PlyPSA linker show the same binding pattern of the proteins without linker

Introduction Materials & Methods Results Overview Discussion & Outlook Conclusions 2 • The lytic activity of HEAD_CBD”1” constructs is very low when compared with Ply511, HEAD_CBD”2” proteins show a stronger lytic activity • The lysis zones in overlay assays of HEAD_CBD”1” are big and diffuse, the ones of HEAD_CBD”2” and Ply511 are smaller and very definite -> difference in diffusion • The isolated CBD”1” part seems not to play any role in binding

Introduction Materials & Methods Results Overview Discussion & Outlook C Ply006 N C Ply118 N C Ply511 N Conclusions 3 • Both CBD subdomains are necessary for full functionality • Presence or absence of the repeated sequences does not seem to play a big role • Results obtained so far correspond to the situation in CBD118 and CBD006.

Introduction Materials & Methods Results Overview Discussion & Outlook Outlook • Biacore measurent of the affinity of binding of HGFP_CBD2 to the listerial cell wall compared to the complete CBD construct HGFP_CBD511 • New pictures of binding assays

Thank you to your attention! • I want to thank Mathias for the assistance and Professor Loessner to give me the possibility to perform my diploma thesis in its group.

Questions?

Introduction Materials & Methods Results Overview Discussion & Outlook HGFP_LPSA_CBD constructs • LPSA linker cloned between the GFP and the CBDs • Linker produced with overlapping primer (KpnI-SacI restriction site at their ends) • GFP gene amplifiedwith primer (BamHI-KpnI restriction site at their ends) SacI GFP H CBDS1 Linker PSA SalI kpnI • The two products were KpnI digested and ligated • Product was PCR amplified with a primers pair annealing to the linker sequence and the GFP gene • Sequencing for linker presence confirmation

Introduction Materials & Methods Results Overview Discussion & Outlook pH_CBD GFP_LPSA digestion BamHI-SacI digestion BamHI-SacI purification purification GFP SacI BamHI SalI ligation MCS E.coli electrophoration Ampicillin pH_GFP Colony PCR Col E1 GFP_LPSA_CBD plasmids already digested for EAD clonation

Introduction Materials & Methods Results Overview Discussion & Outlook BamHI SacI Size [bp] GFP Linker PSA kpnI 2000 750 GFP_LPSA Amplification of the GFP_LPSA Linker and GFP gene amplification Schema GFP_LPSA with restriction site

Introduction Materials & Methods Results Overview Discussion & Outlook Listeria strains and H_GFP_LPSA_CBDs tested in binding assay Interpretation of binding properties: ++ cells displayed an intensive green fluorescence + cells can see but with less intensity, difficult to see (+) very low signal, weak binding - any cells could be seen red: results different to there obtained by the GFP_CBD constructs

Recombinant lytic and GFP-CBD fusion proteins based on the Listeria phage endolysin Ply511

Recombinant lytic and GFP-CBD fusion proteins based on the Listeria phage endolysin Ply511

Presentation Transcript

Fusion Proteins and Mechanisms of Action

Production of recombinant proteins in E. coli by the heat inducible expression system based on the phage lambda pJ a

RECOMBINANT PROTEINS

Lytic Cycle

Phage

Phage

Class I and II Fusion Proteins

GFP – LacZ alpha fusion presentation

Purified proteins Recombinant proteins Whole inactivated or attenuated organisms

Phage

Chapter 8: Expression and Modification of Recombinant Proteins

Image Segmentation based on multicue fusion

Recombinant Proteins: What’s New in the Lab and the Clinic

refolding of recombinant proteins

Renaturation of Recombinant Proteins

High-throughput Screening of Soluble Recombinant Proteins

Phage

U.S Biosimilars Market by Product Type (Recombinant Non-Glycosylated Proteins, Recombinant Glycosylated Proteins); By Ap

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