WO2016007943A1 - Composition and methods for tethering bioactive peptides to metal oxide surfaces - Google Patents

Composition and methods for tethering bioactive peptides to metal oxide surfaces Download PDF

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Publication number
WO2016007943A1
WO2016007943A1 PCT/US2015/040112 US2015040112W WO2016007943A1 WO 2016007943 A1 WO2016007943 A1 WO 2016007943A1 US 2015040112 W US2015040112 W US 2015040112W WO 2016007943 A1 WO2016007943 A1 WO 2016007943A1
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Prior art keywords
ogp
cat
multivalent
catechol
peptide
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PCT/US2015/040112
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French (fr)
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Matthew Becker
Wen Tang
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The University Of Akron
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Priority to CA2954555A priority Critical patent/CA2954555A1/en
Priority to EP15818436.6A priority patent/EP3166553A4/en
Priority to US15/325,218 priority patent/US10765748B2/en
Publication of WO2016007943A1 publication Critical patent/WO2016007943A1/en

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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/06Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite
    • A61K47/08Organic compounds, e.g. natural or synthetic hydrocarbons, polyolefins, mineral oil, petrolatum or ozokerite containing oxygen, e.g. ethers, acetals, ketones, quinones, aldehydes, peroxides
    • A61K47/10Alcohols; Phenols; Salts thereof, e.g. glycerol; Polyethylene glycols [PEG]; Poloxamers; PEG/POE alkyl ethers
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K14/00Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • C07K14/435Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • C07K14/475Growth factors; Growth regulators
    • C07K14/51Bone morphogenetic factor; Osteogenins; Osteogenic factor; Bone-inducing factor
    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K7/00Peptides having 5 to 20 amino acids in a fully defined sequence; Derivatives thereof
    • C07K7/04Linear peptides containing only normal peptide links
    • C07K7/08Linear peptides containing only normal peptide links having 12 to 20 amino acids

Definitions

  • One or more embodiments of the present invention relate to a molecule for the attachment of bioactive peptides to metal oxide and other surfaces.
  • the present invention relates a multivalent amino acid-based Dendron having a bioactive peptide at its focal point and one or more surface-binding catechol groups.
  • Titanium is the most widely used material in bone implants and dental fixations due to its low density, high strength and high resistance to erosion.
  • the oxide passivation layer of 2-20 nm Ti0 2 is quickly formed on titanium implants.
  • Several methods have been developed to decorate titanium implants with bioactive peptides/proteins. Modifications can be achieved through physical interactions, such as protein-encapsulated coating, erosion and subject protein adsorption, and peptide-grafted polycation adsorption.
  • the diffusion of loaded bioactive components may require high doses, and lead to low drug efficiency, and other adverse reactions.
  • DOPA 3,4-dihydroxyphenylalanine
  • Anti-fouling ethylene glycol dendrons and glycocalyx layers have been successfully coated onto titanium oxide surfaces with catechol-functionalized oligomers as the surface- anchoring domain.
  • catechol-functionalized oligomers as the surface- anchoring domain.
  • sequestering bioactive moieties, such as peptides that are known to direct cell behaviors, using catechol-bearing molecules on the surfaces of biomaterials has not been reported.
  • Modular peptides are conjugated molecules containing several different peptide sequences that are known to have specific bio -functionality.
  • the surface-binding peptide that sequesters the whole molecule on the surface and the bioactive subunit that influences the cell behavior.
  • the loading concentration and retention time of the peptides on the surface are critical parameters that determine whether molecular signaling in the cell will be triggered.
  • concentration-dependent concentration-dependent.
  • concentrations that are required to trigger and sustain the cell response are less understood. Strong adsorption is the prerequisite to realize efficient immobilization with bioconjugate solutions at low concentration, and to retain the peptides on the surfaces over extended periods.
  • Osteogenic growth peptide is an endogenous regulatory tetradecapeptide presents in mammalian serum with concentrations at the micromolar scale. Native or synthetic OGP regulates proliferation, alkaline phosphatase activity and matrix mineralization in studies of osteoblastic cell lines derived from human and other mammalian species. As its active portion, the carboxy- terminal pentapeptide, OGP(10-14) directs rat bone marrow mesenchymal stem cells to differentiate to osteoblasts. OGP or OGP(10-14)-functionalized biomaterials, including scaffolds for bone tissue engineering, gradient substrates, and peptide nanofibers, have been prepared, and shown to promote both cell proliferation and osteogenic differentiation, in vitro and in vivo.
  • embodiments of the present invention are directed to a series of multivalent dendrons containing a bioactive peptide domain and surface- binding catechol domains.
  • these multivalent dendrons were obtained through solid phase synthesis and have a strong binding affinity to metal oxide surfaces such as, Ti0 2 , Zr0 2 , Ce0 2 , Fe 3 0 4 , and Si0 2 , as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold.
  • These catechol-bearing dendrons provide a fast and efficient method to functionalize a wide range of inorganic materials with bioactive peptides and have the potential to be used in coating orthopaedic implants and fixation devices.
  • the present invention is directed to a multivalent dendron comprising a bioactive peptide domain and one or more surface-binding catechol domains.
  • the multivalent dendrons of the present invention further comprise a flexible linkage between said bioactive peptide domain and said one or more surface-binding catechol domains.
  • the multivalent dendron of the present invention may comprise any of the above- described embodiments wherein said bioactive peptide domain comprises a bioactive peptide selected from the group consisting of: — NH-KIPKASSVPTELSAISTLYL- COOH, BMP-2, OGP, OGP C-terminal sequence (YGFGG), and combinations thereof.
  • the multivalent dendron of the present invention may comprise any of the above-described embodiments wherein said bioactive peptide is less than 30 amino acids in length. In some embodiments, the multivalent dendron of the present invention may comprise any of the above-described embodiments wherein said bioactive peptide is less than 20 amino acids in length. In some embodiments, the multivalent dendron of the present invention may comprise any of the above-described embodiments wherein said bioactive peptide is OGP C- terminal sequence (YGFGG) .
  • YGFGG OGP C- terminal sequence
  • the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the multivalent dendron has a valence of from 1 to 8. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above- described embodiments wherein the multivalent dendron has a valence of 1. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the multivalent dendron has a valence of 2. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the multivalent dendron has a valence of 4.
  • the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the flexible linkage comprises an oligomer of polyethylene glycol, polyethylene glycol, polypropylene glycol, or polyethylene. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the flexible linkage comprises a polyethylene glycol oligomer having from 1 to 20 ethylene glycol units.
  • the multivalent dendrons of the present invention may comprise any of the above-described embodiments having the formula:
  • PEP is a bioactive peptide
  • the multivalent dendrons of the present invention may comprise any of the above-described embodiments having the formula:
  • PEP is a bioactive peptide
  • a is an integer from 1 to 20 and m is 0 or 1.
  • the multivalent dendrons of the present invention may comprise any of the above-described embodiments having the formula:
  • PEP is a bioactive peptide
  • a is an integer from 1 to 20
  • m is 0 or 1.
  • ESI electrospray ionization
  • FIG. 2 is a graph showing the adsorption of catechol-functionalized dendrons, OGP-Cat, OGP-(Cat) 4 and OGP-PEG-(Cat) 4 onto Ti0 2 surfaces generated by quartz crystal microbalance with dissipation (QCM-d).
  • the experiment contained three processes: i) baseline in HEPES buffer; ii) adsorption of ligands; iii) buffer washing the adsorbed ligands, as indicated by the small peak due to the stop of flow.
  • tetravalent ligands OGP-(Cat) 4 and OGP- PEG-(Cat) 4 requires solution at much lower concentration compared to monovalent ligand, OGP-Cat, indicating a stronger binding affinity.
  • FIG. 3A is a graph generated by QCM-d showing the adsorption of OGP- Cat onto Ti0 2 surface.
  • the adsorbed layer was then washed with 25 mM HEPES buffer. The flow rate was 0.150 mL/min. Three independent measurements (Sensors 1-3) are shown.
  • FIG. 3B is a graph showing that the disassociation constant of OGP-Cat was 5.7 ⁇ 0.2 ⁇ by fitting the adsorption isotherm with single-site specific binding model, as representing with the dash line.
  • the adsorbed area mass was calculated from the Sauerbrey Equation.
  • Each dot with error bar was calculated based on three independent measurements.
  • FIG. 4A-F are adsorption isotherms of catechol-functionalized dendrons according to one or more embodiments of the present invention. Each dot with an error bar was calculated based on three independent measurements. The lines represent fitting with single-site specific binding model.
  • OGP-(Cat) 4 as weakly adsorbed onto Si0 2 , Al 2 03, and HA, and relatively strongly adsorbed onto Au, as measured by QCM-d.
  • FIG. 7 is an X-Ray Photoelectron Spectroscopy (XPS) characterization of Ti0 2 deposition after RF sputtering coating for lh.
  • XPS X-Ray Photoelectron Spectroscopy
  • FIG. 8 is a height image and associated Image Statistics showing the surface roughness of Ti0 2 deposition measured by atomic force microscopy (AFM). The Ti0 2 layer was formed on the top of Si wafer after lh deposition.
  • AFM atomic force microscopy
  • FIGS. 9A-D confirm the successful immobilization of OGP-(Cat) 4 on a Ti0 2 surface.
  • FIG. 9A is a survey scan of bare Ti0 2 surface and OGP-(Cat) 4 immobilized Ti0 2 . The Nls signal comes from amide bonds in peptides.
  • FIG. 9B is a graph showing the results of 1 minute of Ar + plasma treatment to the OGP-(Cat) 4 immobilized Ti0 2 surface removed the adsorbed OGP- (Cat) 4 layer. The Nls peaks are normalized to the highest intensity (Ols) for comparison of the signal to noise ratio.
  • FIGS. 9C and D The multiple peaks in the high resolution XPS spectra of FIGS. 9C and D were fitted with a Gaussian model. The atomic ratios of C2/C1, C3/C1, 02/01, 03/01 and C3/N of respective surfaces were calculated based on the integrated area of each peak.
  • Ti0 2 substrates were incubated in the solution of 0.5 mM FITC-labeled OGP-Cat and FITC overnight, then thoroughly washed with water and dried with N 2 .
  • FITC- labeled OGP-Cat immobilized Ti0 2 pattern on glass slides observed under (FIG. 10A) bright field microscope and (FIG. 10B) fluorescence microscope.
  • the scale bar is 50 ⁇ .
  • FIGS. 11 is a graph of the mean intensity of a FITC-labeled OGP-Cat immobilized surface after incubation for different durations.
  • the control sample is a Ti0 2 substrate incubated in the solution of FITC for overnight.
  • the mean intensity was calculated based on 10 randomly chosen sites observed under the same conditions.
  • the immobilized OGP-(Cat) 4 preserved on the surface for more than 2 weeks in buffer at physiological pH, in comparison, the diffusion of monovalent ligand OGP-Cat was detected after 12 hours.
  • the control is taken after incubation of Ti0 2 substrates in 25 mM HEPES buffer. To compare the signal to noise ratio, all spectra were normalized to the peak of highest intensity (Ols).
  • FIG. 14 is a graph showing that the immobilized OGP-PEG-(Cat) 4 promoted the cell proliferation, and that this effect was dose-dependent. Cell number on substrates after day 1 and day 3 were evaluated by PrestoBlue Assay. The error bar was calculated from three replicates.
  • FIGS. 15A-C are graphs showing the immobilized OGP(10-14) peptide on OGP-99% substrates up-regulated the alkaline phosphatase (ALP) activity and mineralization of MC3T3 cells.
  • FIG. 15 A is a graph showing ALP activity of MC3T3 cells cultured on substrates having 99% OGP coverage (OGP-99%), substrates having 50% OGP coverage (OGP-50%), and Ti0 2 substrates, respectively, on day 18.
  • FIG. 15B is a graph showing mRNA levels of transcription factor gene of ALP, in MC3T3- El cells measured by real-time PCR after cell culture for 18 days.
  • FIG. 15C is a graph showing Ca 2+ accumulation in the cell films quantified with ICP-OES and normalized with total amount of protein.
  • the cell films on OGP-99% exhibited 2-fold higher content of Ca 2+ compared with those on other substrates.
  • the error bar was calculated from three replicates.
  • FIGS. 16A-C are images showing mineralization of MC3T3-E1 cells on substrates studied by Alizarin Red S. staining on day 14 and Ca 2+ quantification by ICP-AES on day 18. Larger sized calcified nodules were observed on OGP-99%, indicating promoted mineralization results from the higher concentration of OGP(10- 14). Images of cell films on OGP-99% (FIG. 16A), OGP-50% (FIG. 16B), and Ti0 2 (FIG. 16C) substrates after Alizarin Red S. observed under bight field microscope. The mineralized osteoids, the spherulites with dark color, ranging from 0.5 to 2 ⁇ , were observed on all the three kinds of substrates. And only cell films on OGP-99% showed the dark mineralized chunks, ranging from 2 to 10 ⁇ .
  • FIG. 17A is a XPS spectra showing preferential adsorption of OGP-(Cat) 4 to the Ti0 2 region of a partially Ti0 2 -coated glass slide observed with XPS.
  • the stronger signal of Nls in the Ti0 2 region compared with that of the Si0 2 region indicates peptides preferentially adsorbed to the Ti0 2 surface.
  • the XPS signals were normalized with the strongest peak intensity (Ols).
  • the atomic percentage of nitrogen in Ti0 2 and Si0 2 region were 8 ⁇ 1% and 1.7 ⁇ 0.8%, respectively.
  • FIG. 18 is a graph showing mRNA levels of transcription factor genes of BSP and OCN, in MC3T3-E1 cells measured by real-time PCR after cell culture for 18 days. Data represent relative expression to the level of the control (cells on Ti0 2 ), set at 1, and mean value and standard deviation calculated from triplicates. The cells having 99% OGP coverage (OGP-99% substrate) expressed a much higher gene level of BSP and OCN, compare to cells on bare Ti0 2 .
  • the various embodiments of the present invention relate to an amino acid based multivalent binding dendron having a bioactive peptide at its focal point and one or more surface-binding catechol domains. These multivalent dendrons are useful for binding bioactive peptides to metal oxide and other surfaces.
  • the multivalent amino acid-based dendrons of the present invention will have a bioactive peptide domain located at its focal point and one or more surface-binding catechol domains at its periphery.
  • amino acid based multivalent binding dendron of one or more embodiments of the present invention may bond to metal oxide and other surfaces by coordination bonding
  • the terms "ligand,” “catechol-bearing multivalent binding ligands,” “catechol bearing ligand,” “multivalent ligand,” “tetravalent ligand,” may also be used herein to refer to these compounds.
  • bioactive peptide domain of the multivalent surface-binding dendrons of the present invention will contain a bioactive peptide that may be connected to the focal point of the dendron either directly, or through a flexible linkage.
  • a bioactive peptide refers to any peptide sequence having 30 amino acids or less with a specific biological function, and is not particularly limited. Any bioactive peptide having 30 amino acids or less may be used.
  • the bioactive peptide may be an osteoinductive, osteoconductive, antimicrobial, morphogenic, homing or immunostimulatory peptide.
  • Suitable bioactive peptides may include, without limitation, — NH- KIPKASSVPTELSAISTLYL-COOH (Seq. I.D. No. 1), bone moiphogenetic protein 2 (BMP-2), osteoconductive peptide (OGP), OGP C-terminal sequence (YGFGG), GRGDS and combinations thereof.
  • BMP-2 bone moiphogenetic protein 2
  • OFGP osteoconductive peptide
  • YGFGG OGP C-terminal sequence
  • GRGDS GRGDS and combinations thereof.
  • the bioactive peptide may be OGP C-terminal sequence (YGFGG).
  • the bioactive peptide may be OGP.
  • the bioactive peptide may be less than 20 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 22 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 20 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 15 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 10 amino acids in length. In some embodiments, the bioactive peptide may be from 10 to 20 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 5 amino acids in length.
  • the multivalent dendrons of the present invention comprise one or more surface-binding catechol domains.
  • each one of these surface-binding catechol domains will have a catechol functional group.
  • These catechol groups are known to form bonds with metal oxide surfaces such as, Ti0 2 , Zr0 2 , Ce0 2 , and Fe 3 0 4 , Si0 2 , as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold.
  • the number of surface- binding catechol domains is a function of the valence of the dendron.
  • the "valence" of a dendron refers to the number of catechol units that are present on the molecule.
  • a dendron having a valence or 4 will have four catechol units.
  • the multivalent dendrons of the present invention may have a valence as high as 16, but valences of from 1 to 8 are preferred.
  • the multivalent dendrons of the present invention may have a valence of from 2 to 8.
  • the multivalent dendrons of the present invention may have a valence of from 4 to 8.
  • the multivalent dendrons of the present invention may have a valence of from 1 to 6. In some embodiments, the multivalent dendrons of the present invention may have a valence of from 1 to 4. In some embodiments, the multivalent dendrons of the present invention may have a valence of 2. In some embodiments, the multivalent dendrons of the present invention may have a valence of 4.
  • the multivalent dendrons of the present invention are amino acid-based and the dendron body (the portion of the dendron the between the bioactive peptide or flexible linkage and the catechol domains) comprises one or more amino acids.
  • the dendron body may comprise the residue of any a-amino acid other than proline.
  • the term "residue(s)" is used to refer generally to the part of a monomer or other chemical unit that has been incorporated into a polymer or large molecule.
  • residue of an amino acid and “amino acid residue” are used interchangeably to refer to part of the amino acids that is incorporated into a larger molecule such as a peptide or the multivalent surface-binding dendrons of the present invention.
  • the dendron body may comprise the residue of alanine (ala - A), arginine (arg - R), asparagine (asn - N), aspartic acid (asp - D), cysteine (cys - C), glutamine (gin - Q), glutamic acid (glu - E), glycine (gly - G), histidine (his - H), isoleucine (ile - I), leucine (leu - L), lysine (lys - K), methionine (met - M), phenylalanine (phe - F), serine (ser - S), threonine (thr - T), tryptophan (trp - W), tyrosine (tyr - Y), or valine (val - V). or any combination thereof
  • the multivalent dendron of the present invention may have the formula:
  • PEP is a bioactive peptide
  • the dendron body will comprise one or more lysine residues.
  • the amino acid lysine presents two amine groups for binding.
  • the catechol functional groups are separated from the dendron body by from 2 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 4 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 6 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 8 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 4 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 6 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 8 carbon atoms.
  • the multivalent dendron of the present invention may have the formula:
  • PEP is a bioactive peptide
  • a is an integer from 1 to 20
  • m is 0 or 1.
  • one of the two amine groups on these forming dendrons may be reacted with one additional lysine molecule to form a dendron body having 3 amino groups available for bonding.
  • both of the amine groups on these forming dendrons may be reacted with an additional lysine molecules to form a dendron body having 4 amino groups available for bonding.
  • each time these dendrons are reacted with an excess of lysine molecules the number of amino groups available for bonding will double. In this way, the valence of the surface- binding dendrons of the present invention may be controlled.
  • These dendrons are then functionalized with catechol groups to form multivalent dendrons having a number of surface-binding catechol domains that corresponds to the number of amino groups available for bonding, as will be discussed in more detail below.
  • the multivalent dendrons of the present invention may have the formula:
  • PEP is a bioactive peptide
  • a is an integer from 1 to 20
  • m is 0 or 1.
  • the bioactive peptide in these embodiments may be attached directly, or indirectly through a flexible linkage, to the C-terminus of the amino acid at the focal point of the dendron.
  • the flexible linkage may be formed from any flexible material capable of bonding to the N-terminal end of a bioactive peptide and the C-terminal end of the amino acid at the focal point of the dendron.
  • the flexible linkage may comprise an oligomer of polyethylene glycol, polypropylene glycol, or polyethylene.
  • flexible linkage comprises a polyethylene glycol oligomer having from 1 to 20 polyethylene glycol units.
  • the flexible linkages may comprise a hexaethylene glycol oligomer.
  • the flexible linker may be comprised of repeating units of polypropylene glycol, polyethylene glycol or polyethylene.
  • a may be an integer from 2 to 20. In some embodiments, a may be an integer from 4 to 20. In some embodiments, a may be an integer from 6 to 20. In some embodiments, a may be an integer from 8 to 20. In some embodiments, a may be an integer from 10 to 20. In some embodiments, a may be an integer from 1 to 18. In some embodiments, a may be an integer from 1 to 16. In some embodiments, a may be an integer from 1 to 14. In some embodiments, a may be an integer from 1 to 12. In some embodiments, a may be an integer from 1 to 10. In some embodiments, a may be an integer from 1 to 8. In some embodiments, a may be an integer from 1 to 5. In some embodiments, a may be an integer from 3 to 8. In some embodiments, a may be 6.
  • the multivalent dendron of the present invention may have the formula:
  • the multivalent dendrons of the present invention may be formed using any methods known in the art.
  • dendrons of the present invention may be formed using simple solid phase protein synthesis techniques as shown in Scheme 1 below.
  • the bioactive peptide is first synthesized on a solid phase polymer resin by conventional solid phase peptide synthesis methods. These methods are well known in the art and need not be described in detail.
  • an OGP(10-14) peptide is formed by solid phase peptide synthesis from a Fmoc protected glycine connected at its C-terminus to a solid phase resin VII.
  • solid phase peptide synthesis may be accomplished using any conventional solid phase CEM Discovery Microwave peptide synthesizer with microwave assistance functionality.
  • the phase peptide synthesizer may be a Liberty 1 peptide microwave synthesizer (CEM Corporation, Matthews, NC).
  • bioactive peptide may be may be synthesized by any other suitable peptide synthesizer or by hand using FMOC chemistry.
  • bioactive peptide shown in Scheme 1 is OGP(10-14), it should be understood that any of the bioactive proteins describe above may also be formed in this manner and used in Scheme 1.
  • Addition of the flexible linkage to the bioactive peptide may be accomplished by any suitable means.
  • addition of the flexible linkage IX to the peptide VII is accomplished by (i) a microwave assisted reaction with a coupling agent and a base in a suitable solvent and (ii) a microwave assisted reaction with a base in a suitable solvent.
  • a microwave assisted reaction with a coupling agent and a base in a suitable solvent
  • a microwave assisted reaction with a base in a suitable solvent.
  • Suitable coupling agents may include, without limitation, 2- (IH-benzotriazol-l -yl) - 1, 1,3,3 ⁇ tetramethyluronium hexafluorophosphate (HBTU), (benzotriazol-1- yloxy)tris(dimethylamino)phosphonium hexafluorophosphate (BOP), bis-(2-oxo-3- oxazolidinyl)phosphinic chloride (BOP-Cl), (l-cyano-2-ethoxy-2- oxoethylidenaminooxy)dimethylamino-mo holino-carbenium hexafluorophosphate (COMUTM), dicyclohexylcarbodiimide (DCC), diisopropylcarbodiimide (DIC), 3- (diethoxyphosphoryloxy)-l,2,3-benzotriazin-4(3H)-one (DEPBT), N-(3- dimethyla
  • TOTU [(ethoxycarbonyl)cyanomethylenamino]-N,N,N',N'-tetra methyluronium tetrafluoroborate
  • TPTU 2- (2-pyridon- 1 -yl) - 1 , 1 ,3 ,3 -tetramethyluronium tetrafluoroborate
  • TSTU N,N,N'N'-tetramethyl-0-(N-succinimidyl)uronium tetrafluoroborate
  • the coupling agent is HBTU.
  • Suitable bases may include, without limitation, iV,A r -DiisopiOpylethylamine (D1PEA or Himig's base), in the embodiment shown in Scheme 1 above, the base is D1PEA.
  • Suitable base may include, without limitation, piperidine, or morpholme. In the embodiment shown in Scheme 1 above, the base is piperidine.
  • Suitable solvents for the coupling agent and base may include, without limitation, N,N dimethylformamide (DMF), -methyl pyrolidone (NMP) and combinations thereof.
  • Suitable solvents for the coupling reaction may include, without limitation, DMF and/or NMP.
  • the amino acid is lysine, but it should be understood that if only a single surface-binding catechol domain is desired, any a- amino acid other than proline may be used.
  • the lysine is added to the amine end group of the PEG by an amidation reaction. The resulting molecule will have one (if an amino acid other than lysine was used) or two (if lysine was used) amine functional groups.
  • the amine functional groups on the dendron are functionalized with a protected catechol group.
  • the protected catechol groups may be added to the amine functional group or groups on the dendron by reacting it with a protected carboxy functionalized catechol compound.
  • the catechol functional group is attached to the amino acid chain at the N-terminal end by means of an amide bond between the amine group and a carboxyl group connected to the catechol functional group.
  • the carboxyl functional group may be separated from the catechol group by from 1 to 20 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 15 carbon atoms.
  • the carboxyl functional group may be separated from the catechol group by from 2 to 10 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 6 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 4 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 5 to 10 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 5 to 20 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 10 to 20 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by 2 carbon atoms.
  • the catechol compound may be the deamino form of the naturally occurring 3,4-dihydroxyphenylalanine (DOPA).
  • DOPA 3,4-dihydroxyphenylalanine
  • the catechol compound may be 3,4-dihydroxyhydrocinnamic acid and is commercially available from Sigma Aldrich Company LLC (St. Louis, Missouri) or Alfa Aesar (Ward Hill, Massachusetts).
  • the catechol groups of the protected catechol compounds may be protected in any manner known in the art for that purpose provided that removal of the protecting group does not cause degradation of the parent compound.
  • acetonide protection mechanisms known in the art may be utilized to protect the catechol groups.
  • these carboxyl functionalized acetonide protected catechol compounds may have the formula:
  • b is an integer from about 0 to about 20. In some embodiments b may be an integer from about 0 to 15. In some embodiments b may be an integer from about 0 to 10. In some embodiments b may be an integer from about 0 to 6. In some embodiments b may be an integer from about 1 to 4. In some embodiments b may be an integer from about 2 to 20. In some embodiments b may be an integer from about 6 to 20. In some embodiments b may be an integer from about 10 to 20. In some embodiments b may be an integer from about 15 to 20. In some embodiments b may be an integer from about 3 to 6. In some embodiments b may be an integer from about 2 to 5. In some embodiments b may be an integer from about 2 to 4.
  • the carboxyl functionalized protected catechol compound may comprise 2,2-dimethyl-l,3-benzodioxole-5- propanoic acid, 2,2-dimethyl-l,3-benzodioxole-5-butanoic acid, 2,2-dimethyl-l,3- benzodioxole-5-petnanoic acid, 2,2-dimethyl-l,3-benzodioxole-5-hexanoic acid, 2,2- dimethyl-l,3-benzodioxole-5-heptanoic acid, or 2,2-dimethyl-l,3-benzodioxole-5- octanoic acid.
  • the carboxyl functionalized protected catechol compounds may be prepared from the corresponding carboxyl functionalized catechol compound by reaction with acetone under basic conditions. In some embodiments, the carboxyl functionalized protected catechol compounds may be prepared as described in Example 4, below.
  • the protected catechol groups were added to the two amine groups of the lysine by the formation of an amine bond between the carboxyl functionalized end group of an acetonide-protected 3,4- dihydroxyhydrocinnamic acid XII with amine groups of the lysine using an additive such as hydroxybenzotriazole (HOBt) and a peptide coupling reagent such as ⁇ , ⁇ '- diisopropylcarbodiimide (DIC).
  • HABt hydroxybenzotriazole
  • DIC peptide coupling reagent
  • the step of coupling of acetonide-protected 3,4-dihydroxyhydrocinnamic acids XII with amines in the peptide chain terminus cannot tolerate microwave-assisted conditions, and the protection of catechol groups is essential for successful synthesis.
  • Suitable additives may include, without limitation, HOBt, 1-hydroxybenzotriazole hydrate (HOBt H20), l-hydroxy-7- azabenzotriazole (HOAt), l-hydrox-6-chloro-triazole (6-Cl-HOBt), 3-hydroxy, 1,2,3- benzotriazin-4(3H)-one (HOOBt), N-hydroxysuccinimide (HOSu), and combinations thereof.
  • the addative is HOBt.
  • One of ordinary skill in the art will likewise be able to select a suitable coupling agent without undue experimentation.
  • Suitable peptide coupling reagent may include, without limitation, HBTU, BOP, COMUTM, DCC, DIC, DEPBT, EDC, HATU, HBTU, HCTU, PyAOP, PyBOP, PyBrOP, TATU, TBTU, TDBTU, TNTU, TOTU, TPTU, TSTU, and combinations thereof, in the embodiment shown in Scheme 1 above, the coupling agent is DIC.
  • the protected catechol group on the resulting dendron is then deprotected, before being cleaved from the resin to form the multivalent dendron of one or more embodiments of the present invention.
  • the method selected for deprotecting the catechol functionalized groups will, of course, depend upon the way in which the catechol group has been protected. In some embodiments, like that shown in Scheme 1 above, an acetonide protected catechol compound may be used and methods for deprotecting such compounds are well known in the art.
  • the catechol groups on the dendron may be deprotected by reacting them with an aqueous solution containing a strong acid such as triflouroacetic acid (TFA) and a proton scavenger such as triisopropylsilyl (TIPS) to obtain free catechol groups.
  • a strong acid such as triflouroacetic acid (TFA) and a proton scavenger such as triisopropylsilyl (TIPS)
  • TFA triflouroacetic acid
  • TIPS triisopropylsilyl
  • the acid is TFA.
  • the acetonide protected catechol groups may be deprotected as described in Example 5.
  • the multivalent dendrons of various embodiments of the present invention may be attached to metal oxide surfaces such as, Ti0 2 , Zr0 2 , Ce0 2 , and Fe 3 0 4 , Si0 2 , as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold by any suitable method.
  • the multivalent dendrons may be dissolved in a suitable aqueous or organic solvent and then contacted to the substrate surface in any convenient manner.
  • the surface may subsequently be rinsed with a buffered solution to remove any unattached dendrons.
  • a series of multivalent catechol-bearing modular peptides may be generated to providing a simple and efficient method of functionalizing metal-oxide based orthopaedic implants with bioactive peptides.
  • tetravalent dendrons according to embodiments of the present invention were shown to persist on the metal oxide surfaces in vitro beyond two weeks under near physiological conditions.
  • the bioactivity of immobilized peptides was demonstrated in an in vitro cell culture study and it was found that the tethered OGP(10-14) promoted the proliferation, osteogenic differentiation and mineralization of MC3T3-E1 cells.
  • the multivalent dendrons of various embodiments of the present invention represent a substantial improvement over prior art systems and a large step toward the development of translational implants with improved bioactivity.
  • lysine-based dendrons were used as the platform to construct the catechol-bearing multivalent binding ligands with a bioactive peptide at the core as shown in Formulas I, II, and III, above.
  • tunable numbers of catechol (Cat) functional groups were attached with a valence of 1, 2 or 4.
  • an osteoconductive peptide, OGP(10-14) was linked. (See PEP in Formulas I, II, and III).
  • the embodiments without the hexaethylene glycol flexible linkage are generally referred to herein as OGP-(Cat) n and the embodiments with the hexaethylene glycol flexible linkage are generally referred to herein as OGP-PEG- (Cat) n , wherein n is 1, 2, or 4.
  • OGP-(Cat) n and OGP-PEG-(Cat) n were carried out using Fmoc based solid phase synthesis as described above, and in particular, OGP-PEG-(Cat) 2 was synthesized as shown in Scheme 1 as an example.
  • Scheme 1 See, Examples 1-5)
  • the last coupling step of acetonide-protected 3,4-dihydroxyhydrocinnamic acids XII with amines in the peptide chain terminus cannot tolerate microwave-assisted conditions, and the protection of catechol groups is essential for successful synthesis. No intervening purification was required, and synthetic process only took 6 hours in all.
  • OGP(10-14) peptide- functionalized catechol-bearing dendrons were achieved with high purity with the yield of 9%-25% as shown in electrospray ionization (ESI) or matrix-assisted laser desorption/ionization time-of-flight (MALDI-ToF) mass spectrometry (FIG. 1).
  • ESI electrospray ionization
  • MALDI-ToF matrix-assisted laser desorption/ionization time-of-flight
  • Binding affinity and maximum adsorption Binding affinity and maximum adsorption.
  • Am - ⁇ — where Am is the amount of adsorbed analyte, c is the
  • B max is the maximum adsorption
  • K d is the apparent dissociation constant
  • OGP-(Cat) 4 Limited adsorption of OGP-(Cat) 4 with materials of compounds from main group elements, including Si0 2 , Al 2 0 3 and hydroxyapatite (HA), was confirmed even when applying a solution at 10-times higher concentration (FIG. 6) . Stronger adsorption was observed for transition metal and transition metal oxide, which was attributed to coordination bonding. Despite the strong binding with Ti0 2 , OGP-(Cat) 4 showed similar strong binding affinity and persistence under buffer washing to other biomaterial-related surfaces, including zirconia, Zr0 2 , a widely used material in prosthetic devices, cerium oxide, Ce0 2 , and iron oxide, Fe 3 0 4 . Therefore, it is believed that OGP-(Cat) 4 will be highly useful for the functionalization of transition metal oxides.
  • T1O2 layer was prepared by RF sputter coating on glass slides or silica wafers.
  • the thickness of T1O2 layer was measured to be around 36 nm with O/Ti ratio equaling to 2.0 (FIG. 7).
  • the surfaces roughness of deposited T1O2 was measured by atomic force microscopy (AFM) with an RMS roughness around 1 nm (FIG. 8).
  • AFM atomic force microscopy
  • RMS roughness refers to a root mean square average of the profile height deviations from the mean line, recorded within the evaluation length RMS.
  • Immobilization of peptides onto Ti0 2 surface was accomplished by immersing the Ti0 2 substrates into the corresponding modular peptide solution and incubating it overnight at ambient temperature.
  • the successful immobilization of OGP-Cat and OGP-(Cat) 4 onto Ti0 2 -coated substrates were confirmed by XPS.
  • Nitrogen is the element contained only in the modular peptides while not in bare Ti0 2 , as shown in the XPS survey scan of bare Ti0 2 and OGP-(Cat) 4 in FIG. 9A.
  • Nls signal at 400.3 eV corresponding to the amide in peptides can be used to prove the immobilization of OGP-(Cat) 4 onto Ti0 2 surfaces (FIG. 9A).
  • the adsorbed OGP- (Cat) 4 layer was readily removed with Ar + plasma treatment for 1 min, indicating that the Nls indeed came from the very top adsorbed peptides layer (FIG. 9B). It is noted that the Nls peaks in FIG. 9B are normalized to the highest intensity (Ols) for comparison of the signal to noise ratio.
  • Standard deviations are typically below 10% relative.
  • OGP-(Cat) n (n 1,4) immobilization without incubation in buffer.
  • the N/Ti ratio increased from 0.03 (Ti0 2 control) to around 0.4 (OGP-Cat: Oh incubation in buffer, OGP-(Cat) 4 : 0 day incubation).
  • the presence of modular peptide OGP-(Cat) 4 was further proven by the significant change of Cls and Ols signatures in high resolution XPS spectra before and after the immobilization. In FIGS.
  • the Cls signals were fit with Gaussian model into three components based on their respective binding energy, including carbon of C-C bond (CI, 284.8 eV), of C-0 bond (C2, 286.1 eV), and of amide bond (C3, 287.8 eV).
  • the significant increase in the atomic ratios of C2/C1, C3/C1, 02/01, and 03/01 indicates the amide bonds and phenol rings contained in the OGP-(Cat) 4 .
  • the C3/N ratio, from amide bond of OGP-(Cat) 4 is 0.93, which is close to the theoretical value of 1.
  • Fluorescein-labeled modular peptide (FITC-labeled OGP-Cat) was also synthesized to visualize the presence of the immobilized peptides on Ti0 2 surface using fluorescence microscopy. (See, Example 13). After immobilization of FITC- labeled OGP-Cat onto Ti0 2 surfaces, the fluorescence intensity was much stronger compared to the control sample, which incubating Ti0 2 -coated substrates in a solution of FITC at identical concentration. When a Ti0 2 pattern was present on the glass slides, it was observed that the Ti0 2 region showed a significantly stronger fluorescence signal due to the stronger binding affinity of FITC-labeled OGP-Cat to Ti0 2 compared with Si0 2 . See, FIGS. 10A-B.
  • the mean intensity of FITC-labeled OGP-Cat immobilized Ti0 2 substrates after incubation was quantified to detect the diffusion of FITC-labeled OGP-Cat into surrounding solution. (See FIG. 11). After 3 days incubation, the intensity deceased by about a half of the original intensity coming from FITC-labeled OGP-Cat on surfaces, indicating the dissociation of monovalent ligand.
  • the decrease of Nls corresponds to the dissociation of adsorbed peptides from Ti0 2 surface.
  • the tetravalent ligand OGP-(Cat) 4 showed a longer retention time on the targeted surface (the decrease of Nls signal was not detected until after 14 days), while the monovalent ligand OGP- Cat showed a reduction in the Nls signal after only 12 hours.
  • the atomic ratio of N/Ti for each was calculated and, as shown in Table 2, the half-life of the immobilized OGP-Cat and OGP-(Cat) 4 present on Ti0 2 surface was around 36 hours and 14 days, respectively.
  • the toxicity of the dendron of the embodiments of the present invention was tested using mouse calvarial pre-osteoblast cells (MCZTZ El ) cells.
  • the MC3T3- El cells were seeded on the Ti0 2 substrates with immobilized FITC-labeled OGP-Cat and cultured for 24 hours.
  • the dominant green fluorescence (viability > 98%) from live cells in the live/dead cell staining demonstrated that the modular peptide bioconjugates are not toxic when tethered to the surface.
  • the cells were well spread on the peptide-bearing surfaces, which is a consistent with an adherent proliferating cell population. See also, Example 17.
  • the loading amount was calculated based on the adsorption isotherm fitted with signal site specific model as shown in Table 1, above.
  • the XPS characterization was applied to detect the immobilized peptides from the Nls signal, which is an element only contained in the amide bond in OGP-PEG-(Cat) 4 for Ti0 2 .
  • substrates having 99% OGP-PEG-(Cat) 4 coverage OGP-99% substrates
  • 50% OGP-PEG-(Cat) 4 coverage OGP-50%).
  • the nitrogen content normalized with total amount of elements on surface was 5.8 ⁇ 0.3 for OGP-99% substrates, while that of OGP-50% were not distinguished from noise due to low content. See also, Example 15 below.
  • the MC3T3-E1 cells were fluorescently stained to visualize actin and vinculin proteins, to assess the organization of cytoskeleton and the spatial distribution of focal adhesion contacts respectively. After 24 hours, the MC3T3-E1 cells were attached on both OGP-99% and bare Ti0 2 substrates and the focal adhesion contacts between cells and substrates formed. As expected, there was there was no statistical difference in cell area and aspect ratio for the cell adhesion to OGP- 99% and bare Ti0 2 substrates as it is known that OGP peptides, immobilized or dissolved, show no effects in the adhesion of MC3T3-E1 cells.
  • the OGP-99%, OGP-50% and Ti0 2 substrates were seeded with preosteoblast MC3T3-E1 cells with a cell density of 18 cell/mm 2 .
  • the cells were mostly attaching to the surface and adjusting to the new environment, therefore, the cell number after 1 day for all three substrates was comparable.
  • the MC3T3-E1 cells on OGP-99% substrates showed the highest cell number compared with the others, indicating that the OGP(10-14) peptide promoted a faster cell proliferation rate in a concentration dependent manner, as shown in FIG. 14. (See also, Examples 16 and 17, below).
  • Bone sialoprotein constitutes approximately 8% of all non- collagenous proteins found in bone, and is important in the nucleation process of hydroxyapatite formation.
  • Osteocalcin OCN
  • OCN Osteocalcin
  • the fluorescent staining of BSP and OCN, the maker proteins of osteogenic differentiation revealed that the MC3T3-E1 cells on the OGP-99%, OGP-50% and Ti0 2 substrates secreted abundant amounts of BSP and OCN after 2 weeks, as indicated by the strong fluorescence of red (OCN) and green (BSP) on the substrates. Similar results were observed for OGP-50% and Ti0 2 substrates.
  • Alkaline phosphatase plays a critical role in the process of mineral formation in tissues such as bone, cartilage, and dentin.
  • ALP activity is a widely recognized biochemical marker for bone forming ability.
  • a standard colorimetric assay was performed to quantify the ALP activity after culture for 18 days, and the values were normalized with total amount of protein to account for the difference of cell number content in samples.
  • the immobilized OGP(10-14) at high concentrations exhibited an enhancement effect on the ALP activity (FIG. 15A).
  • MC3T3-E1 cells on OGP-99% showed a 3-fold higher ALP level compared with those on OGP-50% and Ti0 2 .
  • This up-regulation of ALP activity indicates the immobilized OGP(10-14) preserves its ability to stimulate the dephosphorylation, which is an essential activity involved in the mineralization process.
  • the mRNA expression level of ALP in cells on OGP-99% is also higher in comparison with those on OGP-50% and Ti0 2 as indicated in RT-PCR (FIG. 15B).
  • the appearance of calcium deposition is the phenotypic marker for the last stage of mature osteoblast.
  • ECM extracellular matrix
  • the cell films on all three substrates were positively stained red, indicating the MC3T3-E1 cells differentiated to osteoblast and secreted mineralized ECM.
  • Fmoc-protected amino acids were purchased from Novabiochem (San Diego, CA).
  • Fmoc-NH-PEG6-Propionic acid was purchased from AAPPTec (Louisville, KY).
  • Solvents were purchased from Sigma-Aldrich (St. Louis, MO). Unless otherwise stated, all solvents used were reagent grade and all chemicals were used as supplied.
  • the peptide synthesis was performed on a Liberty 1 peptide microwave synthesizer (CEM Cooperation, Matthews, NC). Reserved-phase high performance liquid chromatography (RP-HPLC) was performed on an Akta Purifier HPLC system by using a ZORBA 300SB-C18 column (5 ⁇ , 9.4x250 mm).
  • the HPLC-grade solvent was degassed before usage, with recipes as A: 0.1 % trifluoroacetic acid in H 2 0 and B: 0.085% trifluoroacetic acid in 95% acetonitrile and 5% H 2 0.
  • the flow rate was 4 mL/min with the pressure around 13 MPa. Fluorescence images were viewed on an 1X81 Microscope (Olympus, Center Valley, PA). Quantification of the adsorption of catechol-bearing peptides onto surfaces was performed by a Q-sense E4 system (Biolin Scientific AB, Sweden).
  • Electrospray ionization mass spectrometry (ESI-MS) spectra were recorded on a Waters Synapt HDMS quadrupole/time-of-flight (Q/ToF) instrument in positive mode.
  • Matrix-assisted laser desorption/ionization time-of-flight (MALDI-ToF) mass spectra were recorded on a Bruker Ultraflex III ToF/ToF mass spectrometer (Bruker Daltonics, Billerica, MA) equipped with Nd:YAG laser which emits at 355 nm.
  • XPS measurements were performed on a Kratos AXIS Ultra DLD spectrometer (Manchester, U.K.) using silicon wafers or glass as substrates.
  • a customized deposition system equipped with DC and RF magnetron sputtering sources was used to do the RF sputter coating. Thickness measurement was measured with NewViewTM 7100 3D Optical Surface Profiler (Zygo, Middlefield, CT, USA) . AFM images were achieved with a Veeco Nanoscope IIIA Atomic Force Microscope (Plainview, NY, USA) . Absorbance or fluorescence was measured using a monochromator-based multi-mode microplate reader (Biotek, Winooski, VT).
  • RNA extraction kit was all purchased from Life technologies (Grand Island, NY).
  • concentration of calcium ions in the supernatant was measured with inductively coupled plasma optical emission spectrometry (ICP-OES) (Agilent Technologies 700 series, Santa Clara, CA, USA) .
  • ICP-OES inductively coupled plasma optical emission spectrometry
  • Real time polymerase chain reaction was performed in the Applied Biosystems Real-Time PCR Instruments - 7500 Fast System (Life technologies, Grand Island, NY).
  • the Lys-based dendron was conjugated to the OGP(10-14) peptide of Example 1, above by using Fmoc-Lys(Fmoc)-OH XV in the coupling step as shown in Schme 3, below.
  • the resins with peptides 1-4 were each transferred into a peptide reaction vessle.
  • the resins were firstly swelled in DMF for 15 minutes. After aspiration, 20 mL DMF was added into each reaction vessle. With nitrogen boubling the solution, acetonide-protected 3,4-dihydroxyhydrocinnamic acid (4 equiv. to each amine), HOBt (10 equiv. to each amine), and DIC (10 equiv. to each amine) were added sequetially to each reaction vessel. Each reaction was carried out at ambient temperature with nitrogen boubling for 4 hours.
  • each reaction vessel was washed by DMF, DCM and MeOH, three times each for 2 minutes. Then, each of the resins were immersed in 30 mL cleavage cocktail (trifluoroacetic acid 95%, triisopropylsilane 2.5%, H 2 0 2.5%, v/v) for 0.5 hour with nitrogen boubling. The solutions were collected and concentrated to ⁇ 3 mL with Roto Vapor. The peptides were precipitated in cold ether three times.
  • cleavage cocktail trifluoroacetic acid 95%, triisopropylsilane 2.5%, H 2 0 2.5%, v/v
  • the catechol-bearing peptides were characterized with either Electrospray Ionization Mass Spectrometry (ESI-MS) or MALDI-ToF mass spectrometry, depending on their molecular weight.
  • ESI-MS Electrospray Ionization Mass Spectrometry
  • MALDI-ToF mass spectrometry
  • OGP-Cat [M+ H] + m/z was calculated to be 792.4 and measured at 792.6.
  • OGP-(Cat) 2 [M + H] + m/z was calculated to be 956.4 and measured at 956.5.
  • OGP-(Cat) 4 [M+Na] + m/z was calculated to be 1562.7 and measured at 1562.7.
  • OGP-PEG-Cat [M+ H] + m/z was calculated to be 1127.5 and measured at 1127.6.
  • OGP-PEG-(Cat) 2 [M+Na] + m/z was calculated to be 1313.6 and measured at 1313.7.
  • OGP-PEG-(Cat) 4 [M+Na] + m/z was calculated to be 1897.9 and measured at 1898.3. See FIGS. 1A-F.
  • the total yield calculated from the staring Fmoc-Gly-Wang Resin (0.25mmol) was: OGP-Cat: 25%, OGP-(Cat) 2 : 23%, OGP-(Cat) 4 : 12%, OGP-PEG-Cat: 20%, OGP-PEG-(Cat) 2 : 15%, and OGP-PEG-(Cat) 4 : 9%.
  • FITC-labeled OGP-Cat was synthesized as set forth in Scheme 7, below.
  • FITC-labeled OGP-Cat [M + H] + m/z was calculated to be 1181.4 and found in 1181.6.
  • the solution of FITC-labeled OGP-Cat (0.5 mM) was used directly to immobilize onto Ti0 2 surface without further purification.
  • Quartz crystal microbalance with dissipation (QCM-d) measurement Quartz crystal microbalance with dissipation (QCM-d) measurement.
  • Quartz crystal microbalance with dissipation was used to determine the binding isotherm for OGP-(Cat) 4 on Ti0 2 , Fe 2 0 3 , Fe 3 0 4 , Zr0 2 , Ce0 2 , Si0 2 , and Au substrates.
  • the AT cut sensors were purchased from Biolin Scientific AB (Sweden) and cleaned before use according to the protocol provided by the company. The sensor was excited at 5 MHz as its fundamental frequency. The frequency shift (Af) and dissipation (AD) were measured at 3 rd , 5 th , 7 th , 9 th , 11 th and 13 th overtones.
  • the QCM-d measurements in Example 7 above may be used to calculate the adsorbed area mass.
  • the adsorbed area mass was proportional to the frequency shift (Af) and calculated by the Sauerbrey Equation.
  • C the mass sensitivity constant with the value of 17.7 ng Hz "1 cm "2 for 5 MHz fundamental frequency crystal
  • n is the frequency overtone number
  • Adsorbed area mass measured from QCM-d includes water contained in the adhering layer.
  • AD Adsorbed area mass measured from QCM-d
  • For adsorptions of OGP-(Cat) n and OGP-PEG-(Cat) n (n 1, 2, 4) onto substrates, AD were below l x lO "6 per 10 Hz, and measurements from multiple overtones were close to each other, indicating adsorbed films were rigid, and the effect from content of water was slight.
  • Am - J ⁇ — , where Am is the amount of adsorbed analyte, c is the concentration of
  • B max is the maximum adsorption of analyte on the surface
  • K d is the apparent dissociation constant
  • Ti0 2 substrates used herein glass slides and silicon wafers were cleaned by sonication in 2% SDS solution for 30 minutes followed by thoroughly rinsing with water, dried with nitrogen and UV-ozone treatment for 20 minutes.
  • the Ti0 2 target 99.99% pure, 2.00" diameter x 0.125" thickness
  • 300 mesh Cu grids were placed on the top of glass.
  • OGP-(Cat) n and OGP-PEG-(Cat) n were dissolved in HEPES buffer at concentrations of 50 ⁇ /L. Substrates were immersed into the solution (800 ⁇ , for 20 mm x 20 mm glass slides, 500 ⁇ , for 5 mm x 5 mm silica wafer) and incubated at ambient temperature overnight. After that, the substrates were rinsed thoroughly with water to wash away the unbounded molecules, dried with nitrogen and subjected to further study.
  • XPS X-ray photoelectron spectroscopy
  • X-ray photoelectron spectroscopy was used to confirm the presence of the OGP peptide on the surface of the substrate by the presence of nitrogen.
  • the XPS measurements were performed on a Kratos AXIS Ultra DLD spectrometer.
  • the X- ray source was monochromated Al Ka, scanning over a binding-energy range of (0 to 700) eV with a dwell time of 100 ms.
  • the analyzer pass energy was 110 eV for the survey spectra and 11 eV for the high-resolution Cls, Nls, and Ols scans. Each spectrum was collected over a 300 x 700 ⁇ sample area. The results are reported in FIGS. 7, 9A-D, 12, 13, and 17. .
  • the Ti0 2 -coated glass slides were sterilized by washing with ethanol and UV irradiation for 30 minutes.
  • the OGP-PEG-(Cat) 4 in HEPES buffer solution was sterilized by filtration through a 0.2 ⁇ sterile syringe filter (EMD Millipore Millex).
  • K d is the apparent dissociation constant.
  • K d is 0.028 + 0.008 ⁇ /L
  • B max is 196 + 23 ng/cm 2 , as characterized in the previous work.
  • MC3T3-E1 mouse preosteoblast (passage 17) were expanded and cultured in a-MEM media (Gibco, Life Technoligies, Grand Island, NY) supplemented with 10% fetal bovine serum (FBS) (Invitrogen), 100 units/mL penicillin (Invitrogen), and 100 ⁇ g/mL streptomycin (Invitrogen) at 37°C in a 5% C0 2 humidified atmosphere.
  • FBS fetal bovine serum
  • penicillin Invitrogen
  • streptomycin Invitrogen
  • the cells were subcultured every 3 days in the presence of 0.25% (w/v) trypsin and 0.5 % (w/v) ethylenediaminetetraacetic acid tetrasodium salt (EDTA) solution. Cells were seeded on substrates at 18 cells/mm 2 and fed every two days.
  • EDTA ethylenediaminetetraacetic acid tetrasodium salt
  • Viability of the cell culture of Example 16 above was evaluated using a Live/Dead viability/cyto toxicity kit (Invitrogen, UK) . Briefly, 5 ⁇ , of the 4 mM Calcein-AM stock solution and 10 ⁇ , of the 2 mM ethidium homodimer-1 (EtmD-1) stock solution were added to 10 mL of cell culture medium to prepare the Live/Dead staining solution. 1 mL of staining solution was added into each well in a 6-well plate, after aspiration of the old medium. The samples were incubated for 10 min in Live/Dead staining solution.
  • EtmD-1 2 mM ethidium homodimer-1
  • Freshly made 0.1 wt% NaBH 4 in lxPBS was then added for 10 minutes at r.t. to quench the aldehyde fluorescence, followed by aspiration and incubation in 5% donkey serum for 20 minutes at r.t. to block the non-specific binding.
  • the substrates were incubated in vinculin primary antibody Mouse in l xPBS (v/v 1 :200) at 4°C overnight. After washing with 1% donkey serum 3 times, the substrates were stained in a solution of rhodamine phalloidin (v/v 1 :40) and Alexa Flour 488 secondary antibody Mouse (v/v 1 :200) for 1 hour at r.t., avoiding light.
  • the nuclei were stained with DAPI in l xPBS (6 ⁇ / 10 mL) for 20 minutes at r.t. in the dark. After washing with lxPBS 3 times to remove excess staining, the samples were mounted and viewed under an 1X81 Microscope (Olympus, Center Valley, PA) with mercury bulb excitation and the filters of FITC, TRITC and DAPI. The images showed the differences in cell morphology imparted by each concentration.
  • BSP bone sialoprotein
  • OCN osteocalcin
  • the substrates were incubated in bone sialoprotein (BSP) primary antibody Mouse (v/v 1:400) and osteocalcin (OCN) primary antibody Goat in IxPBS (v/v 1:100) overnight at 4°C. After washing with 1% donkey serum 3 times, the substrates were stained by incubation in a solution of Alexa Flour 488 secondary antibody Mouse (v/v 1:200) and Alexa Flour 546 secondary antibody Goat (v/v 1:200) in IxPBS for 1 hour at r.t. in the dark. After washing with 1% donkey serum 3 times, the nuclei were stained with DAPI in IxPBS (6 ⁇ , / 10 mL) for 20 minutes at r.t. avoiding light.
  • BSP bone sialoprotein
  • OCN osteocalcin
  • Samples of cell coated substrates (Examples 16 and 17)were pre-fixed in pre-warmed 0.8 mL cell culture media and 1.2 mL 3.7% paraformaldehyde (PFA) in CS buffer for 5 minutes on a dry block at 37°C. After aspiration, samples were fixed in 3.7 % PFA solution at 37°C for 5 minutes. Freshly made Alizarin Red S. solution (0.8 g in 40 mL dd H 2 0, pH adjusted to 4.2), was added into substrates that are washed 3 times with dd H 2 0 to remove soluble calcium. After incubation at r.t. for 40 minutes, the Alizarin Red S. solution was carefully removed. The substrates were washed with double distilled H 2 0 4 times, mounted and observed under bright field microscope. These images showed significantly higher Ca +2 levels for the OGP-99% than the OGP- 50% or Ti0 2 substrates. See FIG. 15C.
  • ALP activity was measured by SensoLyte pNPP ALP Assay Kit (AnaSpec Inc, San Jose, CA, USA) following the provided protocol.
  • the MC3T3-E1 cells on OGP-99%, OGP-50% and Ti0 2 substrates were washed with lx Assay Buffer twice. (See FIG. 15A).
  • the cell film was peeled from the substrates and transferred into a 1.5 mL centrifuge tube, followed by addition of 0.5 mL lysis buffer (20 ⁇ , Triton X- 100 in 10 mL l x Assay Buffer) .
  • the cells was resuspended and incubated in the lysis buffer for 10 min at 2500 xg at 4°C.
  • the emission wavelength was set at 393.366 nm to quantify Ca 2+ .
  • a standard curve was measured with solutions of c(Ca 2+ ) equal to 0.125, 0.25, 0.5, 1, and 2 ppm. Triplicate measurements were carried out for each sample.
  • the calcium amount of each sample was normalized with total protein amount, which was done in the same way as set forth above for the ALP activity assay. See FIG. 15C.
  • RT-PCT Real time-polymerase chain reaction
  • RNA was isolated from the cell coated substrates (See, Examples 16 and 17) on day 18 with an RNA extraction and isolation kit (Applied Biosystems, Life Technologies), following the provided protocol, and was quantified by ultraviolet spectroscopy.
  • the synthesis of complementary DNA (cDNA) was performed with a high-capacity cDNA reverse transcription kit with RNase inhibitor (Applied Biosystems, Life Technologies) using 800 ng total RNA as the template in a 100 ⁇ reaction following the provided protocol.
  • RT-PCR was performed with non-specific detection fluorescence, SYBR Green, or double-dye probe detection, and TaqMan probes system (Applied Biosystems, Life Technologies) .
  • SYBR Green system 10 ng of cDNA product and lx SYBR Green master mixture (Applied Biosystems, Life Technologies) were included in 50 ⁇ , reaction mixture (209.4 nM each primer).
  • TaqMan system 24 ng of cDNA product and lxTaqMan master mixture (Applied Biosystems, Life Technologies) were included in 25 ⁇ , reaction mixture.
  • the housekeeping gene was glyceraldehyde-3-phosphate dehydrogenase (GAPDH). All oligonucleotide primers (See Table 5, below) were purchased from Applied Biosystems (Life Technologies).
  • the ALP primer alpl gene from Mouse was also purchased from Applied Biosystems (Life Technologies) .
  • RT-PCR was performed in the Applied Biosystems Real-Time PCR Instruments - 7500 Fast System (Life technologies, Grand Island, NY) with recommended programs by the supplier.
  • FIGS. 15B and 18 The results are shown in FIGS. 15B and 18.
  • the data reported in FIG. 18 represents relative expression to the level of the control (cells on Ti0 2 ), set at 1, and mean value and standard deviation calculated from triplicates.

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Abstract

In various aspects, embodiments of the present invention are directed to a series of multivalent dendrons containing a bioactive peptide domain and surface-binding catechol domains. In some embodiments, these multivalent dendrons were obtained through solid phase synthesis and have a strong binding affinity to metal oxide surfaces such as, TiO2, ZrO2, CeO2, and Fe3O4, SiO2, as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold. These catechol-bearing dendrons provide a fast and efficient method to functionalize a wide range of inorganic materials with bioactive peptides and have the potential to be used in coating orthopaedic implants and fixation devices.

Description

COMPOSITION AND METHODS FOR TETHERING BIOACTIVE PEPTIDES TO METAL OXIDE SURFACES
CROSS REFERENCE TO RELATED APPLICATIONS
[0001] This application claims the benefit of U.S. provisional patent application serial number 62/023,292 entitled "Methods and Molecules for Tethering Bioactive Peptides to Metal Oxide Surfaces," filed July 11, 2014, and incorporated herein by reference in its entirety.
FIELD OF THE INVENTION
[0002] One or more embodiments of the present invention relate to a molecule for the attachment of bioactive peptides to metal oxide and other surfaces. In certain embodiments, the present invention relates a multivalent amino acid-based Dendron having a bioactive peptide at its focal point and one or more surface-binding catechol groups.
REFERENCE TO GOVERNMENT SUPPORT
[0003] The invention was developed at least in part with the support of National Science Foundation grant number DMR-1105329. The government may have certain rights in the invention.
SEQUENCE LISTING
[0004] The Sequence Listing file entitled "UOA.1147 Sequence Listing_ST25.txt" having a size of 2,235 bytes and creation date of July 7, 2015, that was electronically filed with the patent application is incorporated herein by reference in its entirety.
BACKGROUND OF THE INVENTION
[0005] Immobilization of bioactive peptides onto surfaces has been proven to be an effective avenue to improve cell attachment, influence proliferation, and direct differentiation in tissue engineering. Physical adsorption/encapsulation and chemical conjugation have both been applied to derivatize tissue engineering scaffolds with bioactive peptides. Most of these methods were developed for polymeric materials, while the surface decoration of inorganic surfaces has received less attention, due to the lack of diversity in presenting functional groups for highly efficient chemical reactions. However, many inorganic materials are useful in the medical applications field. For instance, titanium and zirconia are widely used in prosthetic devices and dental implants; cerium oxide nanoparticles are potent antioxidants in therapeutics; and iron oxide magnetic nanoparticles are used to enhance the magnetic resonance imaging contrast in disease diagnostics. Thus the development of efficient and convenient methods to immobilize bioactive peptides onto the surface of metal oxide materials (Ti02, Zr02, Ce02, Fe304, etc.) will not only influence the cell behavior locally, but will also contribute to the improvement of diagnostic and therapeutic techniques in the clinic.
[0006] Titanium is the most widely used material in bone implants and dental fixations due to its low density, high strength and high resistance to erosion. In physiological conditions, the oxide passivation layer of 2-20 nm Ti02 is quickly formed on titanium implants. Several methods have been developed to decorate titanium implants with bioactive peptides/proteins. Modifications can be achieved through physical interactions, such as protein-encapsulated coating, erosion and subject protein adsorption, and peptide-grafted polycation adsorption. However, the diffusion of loaded bioactive components may require high doses, and lead to low drug efficiency, and other adverse reactions. Chemical conjugation by generating reactive functional groups using electrochemical anodization, acid-etching, and oxidation, have been utilized to covalently conjugate the bioactive moieties onto the titanium implant surface, but the methods require complicated procedures and change the surface properties of the device during fabrication.
[0007] The presence of 3,4-dihydroxyphenylalanine (DOPA), which is found abundantly in mussel adhesive proteins, has been connected to the strong adhesion of mussels onto multiple surfaces in wet conditions. Catechol group is the functional group of DOPA, which is known to interact with titanium oxide surface through coordination bond or H-bond with pH sensitivity. Catechol is also crosslinked together under oxidative or basic conditions to form coating layers on surfaces. Thus it has been served as adhesive building blocks in the surface coating of variety of materials, including metal oxides, and organic polymers. Besides titanium oxide, the interaction of catechol with other metal oxides has also been studied, including iron oxide, chromium(III) oxide manganese dioxide, aluminium oxide and zirconia. Anti-fouling ethylene glycol dendrons and glycocalyx layers have been successfully coated onto titanium oxide surfaces with catechol-functionalized oligomers as the surface- anchoring domain. However, sequestering bioactive moieties, such as peptides that are known to direct cell behaviors, using catechol-bearing molecules on the surfaces of biomaterials has not been reported.
[0008] Modular peptides are conjugated molecules containing several different peptide sequences that are known to have specific bio -functionality. In the modular peptides, there are two active components, the surface-binding peptide that sequesters the whole molecule on the surface and the bioactive subunit that influences the cell behavior. The loading concentration and retention time of the peptides on the surface are critical parameters that determine whether molecular signaling in the cell will be triggered. In many studies it was shown that the cell response to specific peptides is concentration-dependent. However, in most applications, the concentrations that are required to trigger and sustain the cell response are less understood. Strong adsorption is the prerequisite to realize efficient immobilization with bioconjugate solutions at low concentration, and to retain the peptides on the surfaces over extended periods.
[0009] It is known that if there are more than one pair of ligand-receptor interactions binding simultaneously, a synergistic augment rises in binding affinity with an order of magnitude enhancement over the corresponding monovalent ligand. This multivalent binding strategy has been used extensively in nature and with synthetic molecules to enhance their binding affinity. Dendrimers are ideal platforms to construct multivalent binding ligands due to their abundant functional groups in the periphery region. Studies have shown that the molecular structure of the multivalent ligands, including binding valency, the flexible linkage units, molecular architecture and receptor density all play significant roles in the ultimate association constant of the multivalent ligand with its receptor.
[0010] Osteogenic growth peptide (OGP) is an endogenous regulatory tetradecapeptide presents in mammalian serum with concentrations at the micromolar scale. Native or synthetic OGP regulates proliferation, alkaline phosphatase activity and matrix mineralization in studies of osteoblastic cell lines derived from human and other mammalian species. As its active portion, the carboxy- terminal pentapeptide, OGP(10-14) directs rat bone marrow mesenchymal stem cells to differentiate to osteoblasts. OGP or OGP(10-14)-functionalized biomaterials, including scaffolds for bone tissue engineering, gradient substrates, and peptide nanofibers, have been prepared, and shown to promote both cell proliferation and osteogenic differentiation, in vitro and in vivo.
[0011] What is needed in the art is a versatile molecule that will tether bioactive molecules to a variety of surfaces in such a way that their inherent biological function is preserved.
SUMMARY OF THE INVENTION
[0012] In various aspects, embodiments of the present invention are directed to a series of multivalent dendrons containing a bioactive peptide domain and surface- binding catechol domains. In some embodiments, these multivalent dendrons were obtained through solid phase synthesis and have a strong binding affinity to metal oxide surfaces such as, Ti02, Zr02, Ce02, Fe304, and Si02, as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold. These catechol-bearing dendrons provide a fast and efficient method to functionalize a wide range of inorganic materials with bioactive peptides and have the potential to be used in coating orthopaedic implants and fixation devices.
[0013] In various aspects, the present invention is directed to a multivalent dendron comprising a bioactive peptide domain and one or more surface-binding catechol domains. In some embodiments, the multivalent dendrons of the present invention further comprise a flexible linkage between said bioactive peptide domain and said one or more surface-binding catechol domains. In some embodiments, the multivalent dendron of the present invention may comprise any of the above- described embodiments wherein said bioactive peptide domain comprises a bioactive peptide selected from the group consisting of: — NH-KIPKASSVPTELSAISTLYL- COOH, BMP-2, OGP, OGP C-terminal sequence (YGFGG), and combinations thereof.
[0014] In some embodiments, the multivalent dendron of the present invention may comprise any of the above-described embodiments wherein said bioactive peptide is less than 30 amino acids in length. In some embodiments, the multivalent dendron of the present invention may comprise any of the above-described embodiments wherein said bioactive peptide is less than 20 amino acids in length. In some embodiments, the multivalent dendron of the present invention may comprise any of the above-described embodiments wherein said bioactive peptide is OGP C- terminal sequence (YGFGG) .
[0015] In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the multivalent dendron has a valence of from 1 to 8. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above- described embodiments wherein the multivalent dendron has a valence of 1. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the multivalent dendron has a valence of 2. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the multivalent dendron has a valence of 4.
[0016] In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the flexible linkage comprises an oligomer of polyethylene glycol, polyethylene glycol, polypropylene glycol, or polyethylene. In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments wherein the flexible linkage comprises a polyethylene glycol oligomer having from 1 to 20 ethylene glycol units.
[0017] In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments having the formula:
Figure imgf000006_0001
wherein PEP is a bioactive peptide; R is selected from the group consisting of -CH3, - (CH2)3NHC(NH2)C=NH, -CH2CONH2,-CH2COOH, -CH2SH, -(CH2)2COOH, - (CH2)2CONH2, -Ni l ,, -CH2C = CH-N = CH-NH, -CH(CH3)CH2CH3, -CH2CH(CH3)2, - (CH2)4NH2, -(CH2)2SCH3, -CH2Ph, -CH2OH, -CH(OH}CH3, -CH2-C = CH-NH-Ph, - CH2-Ph-OH, -CH(CH3)2, and combinations thereof; a is an integer from 1 to 20; and m is 0 or 1.
[0018] In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments having the formula:
Figure imgf000007_0001
wherein PEP is a bioactive peptide; a is an integer from 1 to 20 and m is 0 or 1.
[0019] In some embodiments, the multivalent dendrons of the present invention may comprise any of the above-described embodiments having the formula:
Figure imgf000007_0002
wherein PEP is a bioactive peptide; a is an integer from 1 to 20; and m is 0 or 1.
BRIEF DESCRIPTION OF THE DRAWINGS
[0020] For a more complete understanding of the features and advantages of the present invention, reference is now made to the detailed description of the invention along with the accompanying figures in which:
[0021] FIGS. 1A-F are electrospray ionization (ESI) of OGP-(Cat)n (FIGS. 1A-C) and OGP-PEG-(Cat)n (FIGS. 1D-F) (n = 1, 2, 4).
[0022] FIG. 2 is a graph showing the adsorption of catechol-functionalized dendrons, OGP-Cat, OGP-(Cat)4 and OGP-PEG-(Cat)4 onto Ti02 surfaces generated by quartz crystal microbalance with dissipation (QCM-d). The experiment contained three processes: i) baseline in HEPES buffer; ii) adsorption of ligands; iii) buffer washing the adsorbed ligands, as indicated by the small peak due to the stop of flow. To reach similar level of frequency shift, tetravalent ligands OGP-(Cat)4 and OGP- PEG-(Cat)4 requires solution at much lower concentration compared to monovalent ligand, OGP-Cat, indicating a stronger binding affinity.
[0023] FIG. 3A is a graph generated by QCM-d showing the adsorption of OGP- Cat onto Ti02 surface. The adsorption of OGP-Cat onto Ti02 surface at different concentrations was measured by QCM-d, while the concentration was increased sequentially ( = 0.068 μιηοΙ/L, c2 = 0.34 μιηοΙ/L, c3 = 1.8 μιηοΙ/L, c4 = 7.3 μιηοΙ/L, cs = 13 μιηοΙ/L, and c6 = 34 μιηοΙ/L). The adsorbed layer was then washed with 25 mM HEPES buffer. The flow rate was 0.150 mL/min. Three independent measurements (Sensors 1-3) are shown.
[0024] FIG. 3B is a graph showing that the disassociation constant of OGP-Cat was 5.7±0.2 μΜ by fitting the adsorption isotherm with single-site specific binding model, as representing with the dash line. The adsorbed area mass was calculated from the Sauerbrey Equation. Each dot with error bar was calculated based on three independent measurements.
[0025] FIG. 4A-F are adsorption isotherms of catechol-functionalized dendrons according to one or more embodiments of the present invention. Each dot with an error bar was calculated based on three independent measurements. The lines represent fitting with single-site specific binding model.
[0026] FIG. 5 is a graph showing tetravalent binding ligand OGP-(Cat)4 (c= 1 μΜ) binding affinities to Fe203, Fe304, Zr02, Ti02, Ce02, Si02, Au surfaces, as measured by QCM-d.
[0027] FIG. 6 is a graph showing tetravalent binding ligand OGP-(Cat)4 (c = 10 μΜ) binding affinities to Si02, Al203, hydroxyapatite (HA) and Au surfaces, as measured by QCM-d. OGP-(Cat)4 as weakly adsorbed onto Si02, Al203, and HA, and relatively strongly adsorbed onto Au, as measured by QCM-d.
[0028] FIG. 7 is an X-Ray Photoelectron Spectroscopy (XPS) characterization of Ti02 deposition after RF sputtering coating for lh. The obtained Ti02 shows the O/Ti ratio of 2, matching with the theoretical stoichiometry. Some carbon and fluorine contamination exists.
[0029] FIG. 8 is a height image and associated Image Statistics showing the surface roughness of Ti02 deposition measured by atomic force microscopy (AFM). The Ti02 layer was formed on the top of Si wafer after lh deposition.
[0030] FIGS. 9A-D confirm the successful immobilization of OGP-(Cat)4 on a Ti02 surface. FIG. 9A is a survey scan of bare Ti02 surface and OGP-(Cat)4 immobilized Ti02. The Nls signal comes from amide bonds in peptides. FIG. 9B is a graph showing the results of 1 minute of Ar+ plasma treatment to the OGP-(Cat)4 immobilized Ti02 surface removed the adsorbed OGP- (Cat) 4 layer. The Nls peaks are normalized to the highest intensity (Ols) for comparison of the signal to noise ratio. FIG. 9C and D graphs showing the signal changes in high resolution XPS spectra of Ols (FIG. 9C) and Cls (FIG. 9D) demonstrating the successful immobilization of OGP-(Cat)4 on Ti02 substrates. The multiple peaks in the high resolution XPS spectra of FIGS. 9C and D were fitted with a Gaussian model. The atomic ratios of C2/C1, C3/C1, 02/01, 03/01 and C3/N of respective surfaces were calculated based on the integrated area of each peak.
[0031] FIGS. 10A-B are images showing the immobilization of modular peptides as viewed by labeling the peptide with fluorescein. Due to multivalent binding effect, the retention time of OGP-(Cat)4 on titanium oxide surface in buffer at physiological pH was longer than 2 weeks, which is long enough to trigger the cell responses. The immobilized FITC-labeled OGP-Cat on Ti02 surface was observed under fluorescence microscope, and the mean intensity of fluorescence decreased after incubating the substrates in pH=7.4 25 mM HEPES buffer due to the diffusion of FITC-labeled OGP- Cat. Ti02 substrates were incubated in the solution of 0.5 mM FITC-labeled OGP-Cat and FITC overnight, then thoroughly washed with water and dried with N2. FITC- labeled OGP-Cat immobilized Ti02 pattern on glass slides observed under (FIG. 10A) bright field microscope and (FIG. 10B) fluorescence microscope. The scale bar is 50 μπι.
[0032] FIGS. 11 is a graph of the mean intensity of a FITC-labeled OGP-Cat immobilized surface after incubation for different durations. The control sample is a Ti02 substrate incubated in the solution of FITC for overnight. The mean intensity was calculated based on 10 randomly chosen sites observed under the same conditions.
[0033] FIGS. 12 and 13 are XPS spectra of Nls signals taken after incubation of OGP-(Cat)4 (FIG. 12) and OGP-Cat (FIG. 13) immobilized Ti02 substrates in HEPES buffer (pH = 7.4) for different durations. The immobilized OGP-(Cat)4 preserved on the surface for more than 2 weeks in buffer at physiological pH, in comparison, the diffusion of monovalent ligand OGP-Cat was detected after 12 hours. The control is taken after incubation of Ti02 substrates in 25 mM HEPES buffer. To compare the signal to noise ratio, all spectra were normalized to the peak of highest intensity (Ols).
[0034] FIG. 14 is a graph showing that the immobilized OGP-PEG-(Cat)4 promoted the cell proliferation, and that this effect was dose-dependent. Cell number on substrates after day 1 and day 3 were evaluated by PrestoBlue Assay. The error bar was calculated from three replicates.
[0035] FIGS. 15A-C are graphs showing the immobilized OGP(10-14) peptide on OGP-99% substrates up-regulated the alkaline phosphatase (ALP) activity and mineralization of MC3T3 cells. FIG. 15 A is a graph showing ALP activity of MC3T3 cells cultured on substrates having 99% OGP coverage (OGP-99%), substrates having 50% OGP coverage (OGP-50%), and Ti02 substrates, respectively, on day 18. FIG. 15B is a graph showing mRNA levels of transcription factor gene of ALP, in MC3T3- El cells measured by real-time PCR after cell culture for 18 days. The ALP activity and its mRNA level of MC3T3 cells on OGP-99% substrate was significantly higher compared to substrates with lower concentration or none. FIG. 15C is a graph showing Ca2+ accumulation in the cell films quantified with ICP-OES and normalized with total amount of protein. The cell films on OGP-99% exhibited 2-fold higher content of Ca2+ compared with those on other substrates. The error bar was calculated from three replicates.
[0036] FIGS. 16A-C are images showing mineralization of MC3T3-E1 cells on substrates studied by Alizarin Red S. staining on day 14 and Ca2+ quantification by ICP-AES on day 18. Larger sized calcified nodules were observed on OGP-99%, indicating promoted mineralization results from the higher concentration of OGP(10- 14). Images of cell films on OGP-99% (FIG. 16A), OGP-50% (FIG. 16B), and Ti02 (FIG. 16C) substrates after Alizarin Red S. observed under bight field microscope. The mineralized osteoids, the spherulites with dark color, ranging from 0.5 to 2 μπι, were observed on all the three kinds of substrates. And only cell films on OGP-99% showed the dark mineralized chunks, ranging from 2 to 10 μπι.
[0037] FIG. 17A is a XPS spectra showing preferential adsorption of OGP-(Cat)4 to the Ti02 region of a partially Ti02-coated glass slide observed with XPS. The stronger signal of Nls in the Ti02 region compared with that of the Si02 region indicates peptides preferentially adsorbed to the Ti02 surface. The XPS signals were normalized with the strongest peak intensity (Ols). The atomic percentage of nitrogen in Ti02 and Si02 region were 8 ± 1% and 1.7 ± 0.8%, respectively.
[0038] FIG. 18 is a graph showing mRNA levels of transcription factor genes of BSP and OCN, in MC3T3-E1 cells measured by real-time PCR after cell culture for 18 days. Data represent relative expression to the level of the control (cells on Ti02), set at 1, and mean value and standard deviation calculated from triplicates. The cells having 99% OGP coverage (OGP-99% substrate) expressed a much higher gene level of BSP and OCN, compare to cells on bare Ti02.
DETAILED DESCRIPTION OF THE ILLUSTRATIVE EMBODIMENTS
[0039] In general outline, the various embodiments of the present invention relate to an amino acid based multivalent binding dendron having a bioactive peptide at its focal point and one or more surface-binding catechol domains. These multivalent dendrons are useful for binding bioactive peptides to metal oxide and other surfaces. In one or more embodiments, the multivalent amino acid-based dendrons of the present invention will have a bioactive peptide domain located at its focal point and one or more surface-binding catechol domains at its periphery. As the amino acid based multivalent binding dendron of one or more embodiments of the present invention may bond to metal oxide and other surfaces by coordination bonding, the terms "ligand," "catechol-bearing multivalent binding ligands," "catechol bearing ligand," "multivalent ligand," "tetravalent ligand," may also be used herein to refer to these compounds.
[0040] The bioactive peptide domain of the multivalent surface-binding dendrons of the present invention will contain a bioactive peptide that may be connected to the focal point of the dendron either directly, or through a flexible linkage. As used herein, a "bioactive peptide" refers to any peptide sequence having 30 amino acids or less with a specific biological function, and is not particularly limited. Any bioactive peptide having 30 amino acids or less may be used.
[0041] In some embodiments, the bioactive peptide may be an osteoinductive, osteoconductive, antimicrobial, morphogenic, homing or immunostimulatory peptide. Suitable bioactive peptides may include, without limitation, — NH- KIPKASSVPTELSAISTLYL-COOH (Seq. I.D. No. 1), bone moiphogenetic protein 2 (BMP-2), osteoconductive peptide (OGP), OGP C-terminal sequence (YGFGG), GRGDS and combinations thereof. In some embodiments, the bioactive peptide may be OGP C-terminal sequence (YGFGG). In some embodiments, the bioactive peptide may be OGP.
[0042] In some embodiments, the bioactive peptide may be less than 20 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 22 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 20 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 15 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 10 amino acids in length. In some embodiments, the bioactive peptide may be from 10 to 20 amino acids in length. In some embodiments, the bioactive peptide may be from 2 to 5 amino acids in length.
[0043] As set forth above, the multivalent dendrons of the present invention comprise one or more surface-binding catechol domains. As should be apparent, each one of these surface-binding catechol domains will have a catechol functional group. These catechol groups are known to form bonds with metal oxide surfaces such as, Ti02, Zr02, Ce02, and Fe304, Si02, as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold.
[0044] As will be appreciated by those of skill in the art, the number of surface- binding catechol domains is a function of the valence of the dendron. As used herein, the "valence" of a dendron refers to the number of catechol units that are present on the molecule. A dendron having a valence or 4, for example, will have four catechol units. In some embodiments, the multivalent dendrons of the present invention may have a valence as high as 16, but valences of from 1 to 8 are preferred. In some embodiments, the multivalent dendrons of the present invention may have a valence of from 2 to 8. In some embodiments, the multivalent dendrons of the present invention may have a valence of from 4 to 8. In some embodiments, the multivalent dendrons of the present invention may have a valence of from 1 to 6. In some embodiments, the multivalent dendrons of the present invention may have a valence of from 1 to 4. In some embodiments, the multivalent dendrons of the present invention may have a valence of 2. In some embodiments, the multivalent dendrons of the present invention may have a valence of 4.
[0045] The multivalent dendrons of the present invention are amino acid-based and the dendron body (the portion of the dendron the between the bioactive peptide or flexible linkage and the catechol domains) comprises one or more amino acids. In embodiments where the valence is 1 and there is a single catechol domain, the dendron body may comprise the residue of any a-amino acid other than proline. As used herein, the term "residue(s)" is used to refer generally to the part of a monomer or other chemical unit that has been incorporated into a polymer or large molecule. By extension, the terms "residue of an amino acid" and "amino acid residue" are used interchangeably to refer to part of the amino acids that is incorporated into a larger molecule such as a peptide or the multivalent surface-binding dendrons of the present invention. In some of these embodiments, the dendron body may comprise the residue of alanine (ala - A), arginine (arg - R), asparagine (asn - N), aspartic acid (asp - D), cysteine (cys - C), glutamine (gin - Q), glutamic acid (glu - E), glycine (gly - G), histidine (his - H), isoleucine (ile - I), leucine (leu - L), lysine (lys - K), methionine (met - M), phenylalanine (phe - F), serine (ser - S), threonine (thr - T), tryptophan (trp - W), tyrosine (tyr - Y), or valine (val - V). or any combination thereof
[0046] In some embodiments, the multivalent dendron of the present invention may have the formula:
Figure imgf000013_0001
wherein PEP is a bioactive peptide; R is-CH3, -(CH2)3NHC(NH2)C=NH, -CH2CONH2 - CH2COOH, -CH2SH, -(CH2)2COOH, -(CH2)2CONH2, -NH2, -CH2C = CH-N=CH-NH, -
CH(CH3)CH2CH3, -CH2CH(CH3)2, -(CH2)4NH2, -(CH2)2SCH3, -CH2Ph, -CI 1 ,0! I, - CH(OH)CH3, -CH. -C- C! I- H-I'h, -CH2-Ph-OH, or -CH(CH3)2; a is an integer from 1 to 20; and m is 0 or 1.
[0047] In embodiments where the valence is two or more, the dendron body will comprise one or more lysine residues. As will be apparent to those of ordinary skill in the art, the amino acid lysine presents two amine groups for binding. In some embodiments, both of these amine groups may be functionalized with catechol groups to produce a multivalent dendron having two surface-binding catechol domains (valence = 2).
[0048] In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 4 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 6 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 8 to 10 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 4 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 6 carbon atoms. In some embodiments, the catechol functional groups are separated from the dendron body by from 2 to 8 carbon atoms.
[0049] In some embodiments, the multivalent dendron of the present invention may have the formula:
Figure imgf000014_0001
(ID wherein PEP is a bioactive peptide; a is an integer from 1 to 20; and m is 0 or 1.
[0050] In some other embodiments, one of the two amine groups on these forming dendrons may be reacted with one additional lysine molecule to form a dendron body having 3 amino groups available for bonding. In some other embodiments, both of the amine groups on these forming dendrons may be reacted with an additional lysine molecules to form a dendron body having 4 amino groups available for bonding. As should be apparent to those of skill in the art, each time these dendrons are reacted with an excess of lysine molecules the number of amino groups available for bonding will double. In this way, the valence of the surface- binding dendrons of the present invention may be controlled. These dendrons are then functionalized with catechol groups to form multivalent dendrons having a number of surface-binding catechol domains that corresponds to the number of amino groups available for bonding, as will be discussed in more detail below.
[0051] In some embodiments, the multivalent dendrons of the present invention may have the formula:
Figure imgf000015_0001
wherein PEP is a bioactive peptide; a is an integer from 1 to 20; and m is 0 or 1. In this way, it is possible to form a multivalent dendron having a desired number of surface -binding catechol domains.
[0052] As set forth above, the bioactive peptide in these embodiments may be attached directly, or indirectly through a flexible linkage, to the C-terminus of the amino acid at the focal point of the dendron. The flexible linkage may be formed from any flexible material capable of bonding to the N-terminal end of a bioactive peptide and the C-terminal end of the amino acid at the focal point of the dendron. In some embodiments, the flexible linkage may comprise an oligomer of polyethylene glycol, polypropylene glycol, or polyethylene. In some embodiments, flexible linkage comprises a polyethylene glycol oligomer having from 1 to 20 polyethylene glycol units. In some embodiments, the flexible linkages may comprise a hexaethylene glycol oligomer.
[0053] With reference to formulas (I), (II), and (III), above, "m" corresponds to the presence or absence of the flexible linkage. If m= l, there is a flexible linkage. If m=0, there is no flexible linkage and the bioactive peptide will be bonded directly to the focal point of the dendron. Similarly, in the embodiments show in formulas I, II, and III, "a" represents the length of the flexible linkage measured in terms of the number of repeating polyethylene glycol units in the flexible linkage when m= l. Once again, while the flexible linker shown in formulas (I), (II), and (III) is comprised of repeating polyethylene glycol units, the invention is to be so limited. In some embodiments, the flexible linker may be comprised of repeating units of polypropylene glycol, polyethylene glycol or polyethylene. In some embodiments, a may be an integer from 2 to 20. In some embodiments, a may be an integer from 4 to 20. In some embodiments, a may be an integer from 6 to 20. In some embodiments, a may be an integer from 8 to 20. In some embodiments, a may be an integer from 10 to 20. In some embodiments, a may be an integer from 1 to 18. In some embodiments, a may be an integer from 1 to 16. In some embodiments, a may be an integer from 1 to 14. In some embodiments, a may be an integer from 1 to 12. In some embodiments, a may be an integer from 1 to 10. In some embodiments, a may be an integer from 1 to 8. In some embodiments, a may be an integer from 1 to 5. In some embodiments, a may be an integer from 3 to 8. In some embodiments, a may be 6.
[0054] In some embodiments, the multivalent dendron of the present invention may have the formula:
Figure imgf000017_0001
(V), or
Figure imgf000017_0002
(VI), wherein m is 0 or 1 as set forth above.
[0055] The multivalent dendrons of the present invention may be formed using any methods known in the art. In some embodiments, dendrons of the present invention may be formed using simple solid phase protein synthesis techniques as shown in Scheme 1 below.
Scheme 1
Figure imgf000018_0001
[0056] In these embodiments, the bioactive peptide is first synthesized on a solid phase polymer resin by conventional solid phase peptide synthesis methods. These methods are well known in the art and need not be described in detail. In the reaction shown in Scheme 1, an OGP(10-14) peptide is formed by solid phase peptide synthesis from a Fmoc protected glycine connected at its C-terminus to a solid phase resin VII. In some of these embodiments, solid phase peptide synthesis may be accomplished using any conventional solid phase CEM Discovery Microwave peptide synthesizer with microwave assistance functionality. In some embodiments, the phase peptide synthesizer may be a Liberty 1 peptide microwave synthesizer (CEM Corporation, Matthews, NC). In these methods, amino acids are sequentially added to the N-terminus of a forming peptide chain through a series of deprotection and coupling steps by FMOC chemistry. In some other embodiments, the bioactive peptide may be may be synthesized by any other suitable peptide synthesizer or by hand using FMOC chemistry. And while the bioactive peptide shown in Scheme 1 is OGP(10-14), it should be understood that any of the bioactive proteins describe above may also be formed in this manner and used in Scheme 1. [0057] Once the desired peptide has been formed, it is bonded either to a flexible linkage or directly to the dendron body. Again, it should be understood that the invention is not to be limited to the flexible linkage shown in Scheme 1, and any of the materials described above with respect to the flexible linkage could also have been used in place of the hexaethylene glycol shown in Scheme 1, or if no flexible linkage is desired (m=0), this step may be omitted altogether. In the embodiment shown in Scheme 1, the C-terminal end of the bioactive peptide is left attached to and protected by the a solid phase resin and the N-terminal end of the peptide is reacted with an Fmoc protected polyethylene glycol (PEG) IX having six ethylene glycol units (a = 6), thereby adding the PEG to the N-terminal end of the bioactive peptide to form the PEG-PEP molecule X.
[0058] Addition of the flexible linkage to the bioactive peptide may be accomplished by any suitable means. In the embodiment shown in Scheme 1, addition of the flexible linkage IX to the peptide VII is accomplished by (i) a microwave assisted reaction with a coupling agent and a base in a suitable solvent and (ii) a microwave assisted reaction with a base in a suitable solvent. One of ordinary skill in the art will be able to select a suitable coupling agent, base, amino acid and the necessary solvents without undue experimentation. Suitable coupling agents may include, without limitation, 2- (IH-benzotriazol-l -yl) - 1, 1,3,3 tetramethyluronium hexafluorophosphate (HBTU), (benzotriazol-1- yloxy)tris(dimethylamino)phosphonium hexafluorophosphate (BOP), bis-(2-oxo-3- oxazolidinyl)phosphinic chloride (BOP-Cl), (l-cyano-2-ethoxy-2- oxoethylidenaminooxy)dimethylamino-mo holino-carbenium hexafluorophosphate (COMU™), dicyclohexylcarbodiimide (DCC), diisopropylcarbodiimide (DIC), 3- (diethoxyphosphoryloxy)-l,2,3-benzotriazin-4(3H)-one (DEPBT), N-(3- dimethylaminopropyl)-:¥'-ethylcarbodiimide hydrochloride (EDC), 2-(lH-7- azabenzotriazol-l-yl)-l,l,3,3-tetramethyl uronium hexafluorophosphate (HATU), O- benzotriazole-N,N,N',N'-tetramethyl-uronium-hexafluoro-phosphate (HBTU), 2-(6- Chloro- 1 H-benzotriazole- 1 -yl) - 1 , 1 ,3,3-tetramethylaminium hexafluorophosphate (HCTU) , (7-azabenzotriazol- 1 -yloxy) tripyrrolidinophosphonium hexafluorophosphate (PyAOP) , (benzotriazol- 1 -yloxy) tripyrrolidinophosphonium hexafluorophosphate (PyBOP), bromotripyrrolidinophosphonium hexafluorophosphate (PyBrOP), 0-(7- azabenzotriazole-l-yl)-N,N,N',N'-tetramethyluronium tetrafluoroborate (TATU), O- (benzotriazol- 1 -yl) -Ν,Ν,Ν',Ν'-tetramethyluronium tetrafluoroborate (TBTU) , N,N,N^N'-tetramethyl-0-(3,4-dihydro-4-oxo-l,2,3-benzotriazin-3-yl)uranium tetrafluoroborate (TDBTU), 2-(5-norborene-2,3-dicarboximido)-l, 1,3,3- tetramethyluronium tetrafluoroborate (TNTU), O-
[(ethoxycarbonyl)cyanomethylenamino]-N,N,N',N'-tetra methyluronium tetrafluoroborate (TOTU) , 2- (2-pyridon- 1 -yl) - 1 , 1 ,3 ,3 -tetramethyluronium tetrafluoroborate (TPTU), or N,N,N'N'-tetramethyl-0-(N-succinimidyl)uronium tetrafluoroborate (TSTU) .
[0059] in the embodiment shown in Scheme 1 above, the coupling agent is HBTU. Suitable bases may include, without limitation, iV,Ar-DiisopiOpylethylamine (D1PEA or Himig's base), in the embodiment shown in Scheme 1 above, the base is D1PEA. Suitable base may include, without limitation, piperidine, or morpholme. In the embodiment shown in Scheme 1 above, the base is piperidine. Suitable solvents for the coupling agent and base may include, without limitation, N,N dimethylformamide (DMF), -methyl pyrolidone (NMP) and combinations thereof. Suitable solvents for the coupling reaction may include, without limitation, DMF and/or NMP.
[0060] Next, the peptide (m=0) or peptide-PEG complex (m= l) may be reacted with an amino acid that will form the focal point of the dendron body. In the embodiment shown in Scheme 1, the amino acid is lysine, but it should be understood that if only a single surface-binding catechol domain is desired, any a- amino acid other than proline may be used. In the embodiment of Scheme 1, the lysine is added to the amine end group of the PEG by an amidation reaction. The resulting molecule will have one (if an amino acid other than lysine was used) or two (if lysine was used) amine functional groups.
[0061] Next, the amine functional groups on the dendron are functionalized with a protected catechol group. In some embodiments, the protected catechol groups may be added to the amine functional group or groups on the dendron by reacting it with a protected carboxy functionalized catechol compound. In these embodiments, the catechol functional group is attached to the amino acid chain at the N-terminal end by means of an amide bond between the amine group and a carboxyl group connected to the catechol functional group. [0062] In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 1 to 20 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 15 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 10 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 6 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 2 to 4 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 5 to 10 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 5 to 20 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by from 10 to 20 carbon atoms. In some of these embodiments, the carboxyl functional group may be separated from the catechol group by 2 carbon atoms.
[0063] In some embodiments, the catechol compound may be the deamino form of the naturally occurring 3,4-dihydroxyphenylalanine (DOPA). In some embodiments, the catechol compound may be 3,4-dihydroxyhydrocinnamic acid and is commercially available from Sigma Aldrich Company LLC (St. Louis, Missouri) or Alfa Aesar (Ward Hill, Massachusetts).
[0064] The catechol groups of the protected catechol compounds may be protected in any manner known in the art for that purpose provided that removal of the protecting group does not cause degradation of the parent compound. In some embodiments, acetonide protection mechanisms known in the art may be utilized to protect the catechol groups. In some embodiments, these carboxyl functionalized acetonide protected catechol compounds may have the formula:
Figure imgf000021_0001
wherein b is an integer from about 0 to about 20. In some embodiments b may be an integer from about 0 to 15. In some embodiments b may be an integer from about 0 to 10. In some embodiments b may be an integer from about 0 to 6. In some embodiments b may be an integer from about 1 to 4. In some embodiments b may be an integer from about 2 to 20. In some embodiments b may be an integer from about 6 to 20. In some embodiments b may be an integer from about 10 to 20. In some embodiments b may be an integer from about 15 to 20. In some embodiments b may be an integer from about 3 to 6. In some embodiments b may be an integer from about 2 to 5. In some embodiments b may be an integer from about 2 to 4. In some embodiments b may be 1. In some embodiments, the carboxyl functionalized protected catechol compound may comprise 2,2-dimethyl-l,3-benzodioxole-5- propanoic acid, 2,2-dimethyl-l,3-benzodioxole-5-butanoic acid, 2,2-dimethyl-l,3- benzodioxole-5-petnanoic acid, 2,2-dimethyl-l,3-benzodioxole-5-hexanoic acid, 2,2- dimethyl-l,3-benzodioxole-5-heptanoic acid, or 2,2-dimethyl-l,3-benzodioxole-5- octanoic acid.
[0065] In some embodiments, the carboxyl functionalized protected catechol compounds may be prepared from the corresponding carboxyl functionalized catechol compound by reaction with acetone under basic conditions. In some embodiments, the carboxyl functionalized protected catechol compounds may be prepared as described in Example 4, below.
[0066] In the embodiment shown in Scheme 1, the protected catechol groups were added to the two amine groups of the lysine by the formation of an amine bond between the carboxyl functionalized end group of an acetonide-protected 3,4- dihydroxyhydrocinnamic acid XII with amine groups of the lysine using an additive such as hydroxybenzotriazole (HOBt) and a peptide coupling reagent such as Ν,Ν'- diisopropylcarbodiimide (DIC). It should be noted that in these embodiments, the step of coupling of acetonide-protected 3,4-dihydroxyhydrocinnamic acids XII with amines in the peptide chain terminus cannot tolerate microwave-assisted conditions, and the protection of catechol groups is essential for successful synthesis.
[0067] One of ordinary skill in the art will be able to select a suitable additive and coupling agent without undue experimentation. Suitable additives may include, without limitation, HOBt, 1-hydroxybenzotriazole hydrate (HOBt H20), l-hydroxy-7- azabenzotriazole (HOAt), l-hydrox-6-chloro-triazole (6-Cl-HOBt), 3-hydroxy, 1,2,3- benzotriazin-4(3H)-one (HOOBt), N-hydroxysuccinimide (HOSu), and combinations thereof. In the embodiment shown in Scheme 1 above, the addative is HOBt. One of ordinary skill in the art will likewise be able to select a suitable coupling agent without undue experimentation. Suitable peptide coupling reagent may include, without limitation, HBTU, BOP, COMU™, DCC, DIC, DEPBT, EDC, HATU, HBTU, HCTU, PyAOP, PyBOP, PyBrOP, TATU, TBTU, TDBTU, TNTU, TOTU, TPTU, TSTU, and combinations thereof, in the embodiment shown in Scheme 1 above, the coupling agent is DIC.
[0068] The protected catechol group on the resulting dendron is then deprotected, before being cleaved from the resin to form the multivalent dendron of one or more embodiments of the present invention. The method selected for deprotecting the catechol functionalized groups will, of course, depend upon the way in which the catechol group has been protected. In some embodiments, like that shown in Scheme 1 above, an acetonide protected catechol compound may be used and methods for deprotecting such compounds are well known in the art. In these embodiments, the catechol groups on the dendron may be deprotected by reacting them with an aqueous solution containing a strong acid such as triflouroacetic acid (TFA) and a proton scavenger such as triisopropylsilyl (TIPS) to obtain free catechol groups. Again, these methods are well known in the art and one of ordinary skill in the art will be able to select a suitable acid and proton scavenger without undue experimentation. In the embodiment shown in Scheme 1 above, the acid is TFA. One of ordinary skill in the art will likewise be able to select a suitable proton scavenger without undue experimentation. In some embodiments, the acetonide protected catechol groups may be deprotected as described in Example 5.
[0069] The multivalent dendrons of various embodiments of the present invention may be attached to metal oxide surfaces such as, Ti02, Zr02, Ce02, and Fe304, Si02, as well as other inorganic surfaces such as hydroxyapatite, silver, fluorapatite, calcium carbonate and gold by any suitable method. In some embodiments, the multivalent dendrons may be dissolved in a suitable aqueous or organic solvent and then contacted to the substrate surface in any convenient manner. In some embodiments, the surface may subsequently be rinsed with a buffered solution to remove any unattached dendrons.
[0070] Accordingly, through a straightforward synthesis, a series of multivalent catechol-bearing modular peptides may be generated to providing a simple and efficient method of functionalizing metal-oxide based orthopaedic implants with bioactive peptides. As will be described in detail below, with a multivalent binding strategy, tetravalent dendrons according to embodiments of the present invention were shown to persist on the metal oxide surfaces in vitro beyond two weeks under near physiological conditions. The bioactivity of immobilized peptides was demonstrated in an in vitro cell culture study and it was found that the tethered OGP(10-14) promoted the proliferation, osteogenic differentiation and mineralization of MC3T3-E1 cells. Considering their strong adhesion to versatile metal oxide surfaces, it is believed that the multivalent dendrons of various embodiments of the present invention represent a substantial improvement over prior art systems and a large step toward the development of translational implants with improved bioactivity.
Experimental
[0071] In order to evaluate the functionality of multivalent dendrons according to various embodiments of the present invention, lysine-based dendrons were used as the platform to construct the catechol-bearing multivalent binding ligands with a bioactive peptide at the core as shown in Formulas I, II, and III, above. In the periphery of these dendrons, tunable numbers of catechol (Cat) functional groups were attached with a valence of 1, 2 or 4. In the focal point of the dendron, an osteoconductive peptide, OGP(10-14), with the amino acid sequence YGFGG was linked. (See PEP in Formulas I, II, and III). The two domains were connected with (m= l) or without (m=0) a hexaethylene glycol flexible linkage (a =6) (See Formulas IV, V, and VI). The embodiments without the hexaethylene glycol flexible linkage are generally referred to herein as OGP-(Cat)n and the embodiments with the hexaethylene glycol flexible linkage are generally referred to herein as OGP-PEG- (Cat)n, wherein n is 1, 2, or 4.
[0072] The synthesis of OGP-(Cat)n and OGP-PEG-(Cat)n (n= l, 2, 4.) were carried out using Fmoc based solid phase synthesis as described above, and in particular, OGP-PEG-(Cat)2 was synthesized as shown in Scheme 1 as an example. (See, Examples 1-5) As set forth above, the last coupling step of acetonide-protected 3,4-dihydroxyhydrocinnamic acids XII with amines in the peptide chain terminus cannot tolerate microwave-assisted conditions, and the protection of catechol groups is essential for successful synthesis. No intervening purification was required, and synthetic process only took 6 hours in all. After Reversed Phase High Performance Liquid Chromatography (RP-HPLC) purification, the OGP(10-14) peptide- functionalized catechol-bearing dendrons were achieved with high purity with the yield of 9%-25% as shown in electrospray ionization (ESI) or matrix-assisted laser desorption/ionization time-of-flight (MALDI-ToF) mass spectrometry (FIG. 1).
Adsorption to Ti02 measured by QCM-d.
[0073] The adsorption processes of all molecules to Ti02 surfaces at 25°C and pH 7.4 were monitored by quartz crystal microbalance with dissipation (QCM-d). (See Example 7). Multivalent binding effects that enhanced the binding affinity were clear. In FIG. 2, to obtain a similar level of adsorption, ~ 6Hz frequency shift, the concentration of monovalent ligand, OGP-Cat, was 13 μΜ, while that of tetravalent ligand, OGP-(Cat)4 and OGP-PEG-(Cat)4, was 0.32 and 0.16 μΜ, respectively due to the mass differences. A much smaller amount of sample (~ 80-fold less) was needed for the tetravalent ligand OGP-PEG-(Cat)4 compared with the monovalent ligand OGP-Cat to achieve the same level (mass) of surface adsorption. Moreover, it was found that the tetravalent ligands remained on the Ti02 surface under buffer washing, as no frequency shift was observed after switching the solution to HEPES buffer. This indicates that the tetravalent ligands are sequestered on the Ti02 surface and are unlikely to diffuse away after being implanted into the body. Under similar conditions, the monovalent ligand was partially washed away. The adsorption kinetics were recorded by QCM-d, with regard to OGP-PEG-(Cat)4, and 2 hours were needed to reach the equilibrium state at a concentration of 0.16 μΜ.
Binding affinity and maximum adsorption.
[0074] To quantitatively compare the binding affinities of the multivalent binding ligands, their adsorption properties at several different concentrations were measured. The solutions at higher concentrations were switched to flow above the sensor, until the adsorption of previous solution at lower concentration reached the equilibrium state (the change in frequency shift is smaller than the signal fluctuation, 0.05 Hz/min), taking OGP-Cat as an example shown in FIG. 3A. In these experiments, the adsorption of OGP-Cat onto Ti02 surface at different concentrations was measured by QCM-d, while the concentration was increased sequentially ( = 0.068 μιηοΙ/L, c2 = 0.34 μιηοΙ/L, c3 = 1.8 μmol/L, c4 = 7.3 μιηοΙ/L, cs = 13 μιηοΙ/L, and c6 = 34 μιηοΙ/L) . At last the adsorbed layer was washed with 25 mM HEPES buffer. The flow rate was 0.150 mL/min. Three independent measurements (Sensors 1-3) are shown on FIG.3A. The corresponding frequency shift was calculated using Sauerbrey Equation to get the adsorbed area mass. The adsorption isotherm of each molecule was drawn and fit with a single-site specific binding model to get the apparent disassociation constant (Kd~) and maximum adsorption (Bmax) of OGP-Cat as in FIG. 3B and others in FIGS. 4A-F from the adsorbed area mass at the respective concentrations. The results are summarized in Table 1, below.
Table 1
The apparent disassociation constant (Kd), maximum adsorption (Bmax) and enhancement parameter (β) of catechoi-functionaiized
dendrons to T1O2 surface.
Ligands to Ti02 Κά{μΜ) α R ί η3 Λ 6b
max m2)
OGP-Cat 5.7 ± 0.2 54 ± 4 -
OGP-PEG- Cat 1.0 ± 0.1 59 ± 2 -
OGP-(Cat)2 1.1 ± 0.3 55 ± 3 5
OGP-PEG-(Cat)2 0.08 ± 0.01 73 ± 4 12
OGP-(Cat)4 0.031 ± 0.003 160 ± 6 184
OGP-PEG-(Cat)4 0.028 ± 0.008 196 ± 23 36
" Adsorption isotherm was fit with sinj ;le-site specific binding model,
Am = -ί— where Am is the amount of adsorbed analyte, c is the
Kd+ C
concentration of the analyte solution, Bmax is the maximum adsorption, and Kd is the apparent dissociation constant.
6 Enhancement parameter is defined as the ratio of association constant of multivalent ligand to that of monovalent ligand, β = Ka multi/Ka mono. And it was calculated based on two sets of molecules with or without PEG linkage.
[0075] The Kd decreased as the valency changed from 1, to 2, and to 4. This clearly proved that multivalent dendrons provide a stronger binding affinity. The enhancement parameters were calculated for the two series of molecules, with or without the PEG linkage. There is a 184-fold enhancement in binding affinity for OGP-(Cat)4 with the Kd of 31 ± 3 nM, when compared to OGP-Cat. Surprisingly, the PEG linkage also influenced the binding affinity. When the valency equaled 1 or 2, the molecules with PEG showed a 6-fold and 14-fold stronger binding compared with molecules without PEG. While not wanting to be bound by theory, it is believed that this is most likely because the PEG linkage serves as a spacer and weakens the effect of any intramolecular H-bond that may form between catechol groups and the OGP(10-14) peptide chain. From the quantification results of apparent Kd and Bmax, for the tetravalent ligand, it is believed that the binding is strong enough to saturate and sequester the whole molecule on Ti02 surface at very low bioconjugate concentrations. A solution of OGP-(Cat)4 at 2.8 μΜ (100iQ) covers 99% of the binding sites on Ti02 surfaces, at a OGP(10-14) concentration of 103 pmol/cm2. The immobilization procedure simply involves immersing the Ti02 surface in the solution for more than two hours.
Binding ability of OGP-(Cat)4 to versatile surfaces.
[0076] The adsorption of tetravalent binding ligand OGP-(Cat)4 to a wide range of materials was tested to identify common features of materials to which the catechol- bearing ligands of various embodiments of the present invention strongly bind. As shown in FIG. 5, OGP-(Cat)4 showed the strongest binding to Ce02, Ti02 and Zr02, strong binding to iron oxide (Fe304 and Fe203), some adsorption to gold, and weak adsorption to Si02. While not wanting to be bound by theory, it is believed that this is because the coordination bond between catechol and metals with empty d-orbitals or /-orbitals provides a stronger interaction than Hydrogen bonding. Limited adsorption of OGP-(Cat)4 with materials of compounds from main group elements, including Si02, Al203 and hydroxyapatite (HA), was confirmed even when applying a solution at 10-times higher concentration (FIG. 6) . Stronger adsorption was observed for transition metal and transition metal oxide, which was attributed to coordination bonding. Despite the strong binding with Ti02, OGP-(Cat)4 showed similar strong binding affinity and persistence under buffer washing to other biomaterial-related surfaces, including zirconia, Zr02, a widely used material in prosthetic devices, cerium oxide, Ce02, and iron oxide, Fe304. Therefore, it is believed that OGP-(Cat)4 will be highly useful for the functionalization of transition metal oxides.
OGP-(Cat)n on Ti02 surface.
[0077] To directly prove the existence of OGP-(Cat)n on T1O2 surface, X-ray photoelectron spectroscopy (XPS) and fluorescein labeling experiments were carried out. The T1O2 layer was prepared by RF sputter coating on glass slides or silica wafers. The thickness of T1O2 layer was measured to be around 36 nm with O/Ti ratio equaling to 2.0 (FIG. 7). The surfaces roughness of deposited T1O2 was measured by atomic force microscopy (AFM) with an RMS roughness around 1 nm (FIG. 8). As used herein, RMS roughness refers to a root mean square average of the profile height deviations from the mean line, recorded within the evaluation length RMS.
[0078] Immobilization of peptides onto Ti02 surface was accomplished by immersing the Ti02 substrates into the corresponding modular peptide solution and incubating it overnight at ambient temperature. The successful immobilization of OGP-Cat and OGP-(Cat)4 onto Ti02-coated substrates were confirmed by XPS. Nitrogen is the element contained only in the modular peptides while not in bare Ti02, as shown in the XPS survey scan of bare Ti02 and OGP-(Cat)4 in FIG. 9A. Thus Nls signal at 400.3 eV corresponding to the amide in peptides can be used to prove the immobilization of OGP-(Cat)4 onto Ti02 surfaces (FIG. 9A). The adsorbed OGP- (Cat)4 layer was readily removed with Ar+ plasma treatment for 1 min, indicating that the Nls indeed came from the very top adsorbed peptides layer (FIG. 9B). It is noted that the Nls peaks in FIG. 9B are normalized to the highest intensity (Ols) for comparison of the signal to noise ratio.
[0079] To quantify the increase in nitrogen due to adsorption of OGP-Cat and OGP-(Cat)4, the nitrogen content (Nls) was normalized with Ti content (Ti2p), and compared with Ti02 substrate after incubation in HEPES buffer overnight (Ti02 as control), as show in Table 2, below.
Table 2.
The immobilization of OGP-Cat and OGP-(Cat)4 and their retention on T1O2 substrates. Atomic Ratios of N/Tifor the T1O2 surface, the surfaces after OGP-Cat and OGP-(Cat)4 immobilization, and the OGP-Cat and OGP-(Cat)4 bearing surfaces after incubation in HEPES buffer. a b
Figure imgf000028_0001
" Standard deviations are typically below 10% relative.
6 Oh incubation in 25 mM HEPES buffer (pH = 7.41 at 25 °C) means surfaces just after Ti02 coating or
OGP-(Cat)n (n = 1,4) immobilization without incubation in buffer. [0080] The N/Ti ratio increased from 0.03 (Ti02 control) to around 0.4 (OGP-Cat: Oh incubation in buffer, OGP-(Cat)4: 0 day incubation). The presence of modular peptide OGP-(Cat)4 was further proven by the significant change of Cls and Ols signatures in high resolution XPS spectra before and after the immobilization. In FIGS. 9C-D, the Cls signals were fit with Gaussian model into three components based on their respective binding energy, including carbon of C-C bond (CI, 284.8 eV), of C-0 bond (C2, 286.1 eV), and of amide bond (C3, 287.8 eV). Similarly, the Ols signals were deconvoluted into three peaks: oxygen of Ti-0 bond (01, 530.2 eV), of C = 0 bond (02, 531.5 eV), and of C-0 bond (03, 533.0 eV). The significant increase in the atomic ratios of C2/C1, C3/C1, 02/01, and 03/01 (Table 3) indicates the amide bonds and phenol rings contained in the OGP-(Cat)4. The C3/N ratio, from amide bond of OGP-(Cat)4, is 0.93, which is close to the theoretical value of 1.
Table 3
Figure imgf000029_0001
[0081] Fluorescein-labeled modular peptide (FITC-labeled OGP-Cat) was also synthesized to visualize the presence of the immobilized peptides on Ti02 surface using fluorescence microscopy. (See, Example 13). After immobilization of FITC- labeled OGP-Cat onto Ti02 surfaces, the fluorescence intensity was much stronger compared to the control sample, which incubating Ti02-coated substrates in a solution of FITC at identical concentration. When a Ti02 pattern was present on the glass slides, it was observed that the Ti02 region showed a significantly stronger fluorescence signal due to the stronger binding affinity of FITC-labeled OGP-Cat to Ti02 compared with Si02. See, FIGS. 10A-B.
Retention of OGP-(Cat)n on Ti02 surface.
[0082] To study the stability of sequestered modular peptides on targeting surfaces, the modular peptide immobilized Ti02 substrates were immersed in 25 mM HEPES buffer (pH= 7.4 at 25°C) and incubated for different durations. The mean intensity of FITC-labeled OGP-Cat immobilized Ti02 substrates after incubation was quantified to detect the diffusion of FITC-labeled OGP-Cat into surrounding solution. (See FIG. 11). After 3 days incubation, the intensity deceased by about a half of the original intensity coming from FITC-labeled OGP-Cat on surfaces, indicating the dissociation of monovalent ligand. Because the Nls signals were assigned to the modular peptides, the decrease of Nls corresponds to the dissociation of adsorbed peptides from Ti02 surface. As can be seen in FIGS. 12 and 13, the tetravalent ligand OGP-(Cat)4 showed a longer retention time on the targeted surface (the decrease of Nls signal was not detected until after 14 days), while the monovalent ligand OGP- Cat showed a reduction in the Nls signal after only 12 hours. The atomic ratio of N/Ti for each was calculated and, as shown in Table 2, the half-life of the immobilized OGP-Cat and OGP-(Cat)4 present on Ti02 surface was around 36 hours and 14 days, respectively. It is believed that the mismatch of retention time for the monovalent ligands may be attributed to the sensitivity difference of XPS and fluorescence microscopy. Nevertheless, the tetravalent ligands OGP-(Cat)4 were clearly present on the Ti02 surface beyond 2 weeks, which is enough to trigger the cascade signaling reactions in adjacent cells.
Preferential immobilization of OGP-(Cat)n
[0083] It has been found that that the catechol-bearing dendrons have strong binding to transition metal compounds due to coordination bonding, while weaker binding to materials when only Hydrogen bond or other weak non-covalent interactions exist. Thus, if materials with both Si02 and Ti02 present immersed on the surface into a solution of OGP-(Cat)4, it has been found that the OGP-(Cat)4 will preferentially adsorb onto the Ti02 region. This provides a method to preferentially functionalize selected regions on the surface, which is useful in the fabrication of surfaces with locally restricted functionality of peptides. It was demonstrated with a partially coated glass slides containing Si02 region in the middle and Ti02 in the surrounding region. After incubating the slides in the solution of OGP-(Cat)4 (ΰ= 1μΜ) overnight, the elements present on the surface in the respective regions was detected by XPS. The signals from Si02 and Ti02 regions are quite different. The local existence of Si and Ti was confirmed in XPS. And notably, the Ti02 region showed a much stronger signal in Nls, which corresponds to the adsorbed OGP-(Cat)4. The atomic percentage of nitrogen from Nls in Ti02 and Si02 region were 8 ± 1% and 1.7 ± 0.8%, respectively.
Cytotoxicity
[0084] The toxicity of the dendron of the embodiments of the present invention was tested using mouse calvarial pre-osteoblast cells (MCZTZ El ) cells. The MC3T3- El cells were seeded on the Ti02 substrates with immobilized FITC-labeled OGP-Cat and cultured for 24 hours. The dominant green fluorescence (viability > 98%) from live cells in the live/dead cell staining demonstrated that the modular peptide bioconjugates are not toxic when tethered to the surface. The cells were well spread on the peptide-bearing surfaces, which is a consistent with an adherent proliferating cell population. See also, Example 17.
XPS of OGP(10-14) immobilized Ti02-coated substrates.
[0085] The loading amount was calculated based on the adsorption isotherm fitted with signal site specific model as shown in Table 1, above. The XPS characterization was applied to detect the immobilized peptides from the Nls signal, which is an element only contained in the amide bond in OGP-PEG-(Cat)4 for Ti02. substrates having 99% OGP-PEG-(Cat)4 coverage (OGP-99% substrates) and 50% OGP-PEG-(Cat)4 coverage (OGP-50%). The nitrogen content normalized with total amount of elements on surface was 5.8 ± 0.3 for OGP-99% substrates, while that of OGP-50% were not distinguished from noise due to low content. See also, Example 15 below.
Effects of immobilized OGP(10-14) on cell adhesion and morphology.
[0086] Because the capacity for cells to interact with growth factors is an important cell behavior, the MC3T3-E1 cells were fluorescently stained to visualize actin and vinculin proteins, to assess the organization of cytoskeleton and the spatial distribution of focal adhesion contacts respectively. After 24 hours, the MC3T3-E1 cells were attached on both OGP-99% and bare Ti02 substrates and the focal adhesion contacts between cells and substrates formed. As expected, there was there was no statistical difference in cell area and aspect ratio for the cell adhesion to OGP- 99% and bare Ti02 substrates as it is known that OGP peptides, immobilized or dissolved, show no effects in the adhesion of MC3T3-E1 cells.
Effects of immobilized OGP(10-14) on cell proliferation.
[0087] The OGP-99%, OGP-50% and Ti02 substrates were seeded with preosteoblast MC3T3-E1 cells with a cell density of 18 cell/mm2. In the first 24 hours, the cells were mostly attaching to the surface and adjusting to the new environment, therefore, the cell number after 1 day for all three substrates was comparable. After 3 days, the MC3T3-E1 cells on OGP-99% substrates showed the highest cell number compared with the others, indicating that the OGP(10-14) peptide promoted a faster cell proliferation rate in a concentration dependent manner, as shown in FIG. 14. (See also, Examples 16 and 17, below).
Effects of immobilized OGP(10-14) on osteogenic differentiation.
[0088] Bone sialoprotein (BSP) constitutes approximately 8% of all non- collagenous proteins found in bone, and is important in the nucleation process of hydroxyapatite formation. Osteocalcin (OCN) is expressed solely by the osteoblast, thus it is the most specific protein for osteoblast differentiation and mineralization. The fluorescent staining of BSP and OCN, the maker proteins of osteogenic differentiation, revealed that the MC3T3-E1 cells on the OGP-99%, OGP-50% and Ti02 substrates secreted abundant amounts of BSP and OCN after 2 weeks, as indicated by the strong fluorescence of red (OCN) and green (BSP) on the substrates. Similar results were observed for OGP-50% and Ti02 substrates. From the enlarged images, a difference in the distribution of OCN and BSP was observed. The amount of BSP in the cytoplasm and extracellular matrix (ECM) is similar, while the OCN showed a higher concentration in the cytoplasm. This is consistent with the fact that BSP is a component in bone matrix, while OCN is secreted by osteoblasts to regulate the metabolic activities and bone-building process. Using RT-PCR, a quantitative comparison of the expressed mRNA level of BSP and OCN demonstrated a significant increase in expression of these osteogenic genes in cells on OGP-99% substrates. With enough OGP(10-14) present on the surface, the osteogenic differentiation of MC3T3- El cells was enhanced. Effects of immobilized OGP(10-14) on ALP activity.
[0089] Alkaline phosphatase (ALP) plays a critical role in the process of mineral formation in tissues such as bone, cartilage, and dentin. ALP activity is a widely recognized biochemical marker for bone forming ability. A standard colorimetric assay was performed to quantify the ALP activity after culture for 18 days, and the values were normalized with total amount of protein to account for the difference of cell number content in samples. The immobilized OGP(10-14) at high concentrations exhibited an enhancement effect on the ALP activity (FIG. 15A). MC3T3-E1 cells on OGP-99% showed a 3-fold higher ALP level compared with those on OGP-50% and Ti02. This up-regulation of ALP activity indicates the immobilized OGP(10-14) preserves its ability to stimulate the dephosphorylation, which is an essential activity involved in the mineralization process. The mRNA expression level of ALP in cells on OGP-99% is also higher in comparison with those on OGP-50% and Ti02 as indicated in RT-PCR (FIG. 15B).
Effects of immobilized OGP(10-14) on mineralization.
[0090] The appearance of calcium deposition is the phenotypic marker for the last stage of mature osteoblast. The extent of mineralized extracellular matrix (ECM) formed on OGP-99%, OGP-50% and Ti02 substrates after 2 weeks was examined by staining with Alizarin Red S., a red dye that forms a complex with calcium depositions in ECM. The cell films on all three substrates were positively stained red, indicating the MC3T3-E1 cells differentiated to osteoblast and secreted mineralized ECM. Under the microscope, the mineralized osteoids, spherulites with dark red color, ranging from 0.5 to 2 μπι, were observed on all three substrates (FIGS. 16A-C). But only cell films on OGP-99% substrates showed the dark mineralized chunks, ranging from 2 to 10 μπι, which is attributed to the higher content of calcium in the cell films on OGP-99% substrates. The calcium content was quantified with ICP-OES after 18 days culture in non-osteogenic medium. The result is consistent with that of Alizarin Red S. staining, as show in FIG. 15C. The cell films on OGP-99% substrates exhibited more than two times higher concentration of Ca2+ normalized by total amount of protein to account for the difference in cell numbers. Therefore it is apparent that the immobilized OGP(10-14) on surfaces promotes the mineralization of osteoblasts. EXAMPLES
[0091] The following examples are offered to more fully illustrate the invention, but are not to be construed as limiting the scope thereof. Further, while some of examples may include conclusions about the way the invention may function, the inventor do not intend to be bound by those conclusions, but put them forth only as possible explanations. Moreover, unless noted by use of past tense, presentation of an example does not imply that an experiment or procedure was, or was not, conducted, or that results were, or were not actually obtained. Efforts have been made to ensure accuracy with respect to numbers used (e.g., amounts, temperature), but some experimental errors and deviations may be present. Unless indicated otherwise, parts are parts by weight, molecular weight is weight average molecular weight, temperature is in degrees Centigrade, and pressure is at or near atmospheric.
Materials and Equipment
[0092] Fmoc-protected amino acids were purchased from Novabiochem (San Diego, CA). Fmoc-NH-PEG6-Propionic acid was purchased from AAPPTec (Louisville, KY). Solvents were purchased from Sigma-Aldrich (St. Louis, MO). Unless otherwise stated, all solvents used were reagent grade and all chemicals were used as supplied. The peptide synthesis was performed on a Liberty 1 peptide microwave synthesizer (CEM Cooperation, Matthews, NC). Reserved-phase high performance liquid chromatography (RP-HPLC) was performed on an Akta Purifier HPLC system by using a ZORBA 300SB-C18 column (5 μιη, 9.4x250 mm). The HPLC-grade solvent was degassed before usage, with recipes as A: 0.1 % trifluoroacetic acid in H20 and B: 0.085% trifluoroacetic acid in 95% acetonitrile and 5% H20. The flow rate was 4 mL/min with the pressure around 13 MPa. Fluorescence images were viewed on an 1X81 Microscope (Olympus, Center Valley, PA). Quantification of the adsorption of catechol-bearing peptides onto surfaces was performed by a Q-sense E4 system (Biolin Scientific AB, Sweden). Electrospray ionization mass spectrometry (ESI-MS) spectra were recorded on a Waters Synapt HDMS quadrupole/time-of-flight (Q/ToF) instrument in positive mode. Matrix-assisted laser desorption/ionization time-of-flight (MALDI-ToF) mass spectra were recorded on a Bruker Ultraflex III ToF/ToF mass spectrometer (Bruker Daltonics, Billerica, MA) equipped with Nd:YAG laser which emits at 355 nm. XPS measurements were performed on a Kratos AXIS Ultra DLD spectrometer (Manchester, U.K.) using silicon wafers or glass as substrates. A customized deposition system equipped with DC and RF magnetron sputtering sources was used to do the RF sputter coating. Thickness measurement was measured with NewView™ 7100 3D Optical Surface Profiler (Zygo, Middlefield, CT, USA) . AFM images were achieved with a Veeco Nanoscope IIIA Atomic Force Microscope (Plainview, NY, USA) . Absorbance or fluorescence was measured using a monochromator-based multi-mode microplate reader (Biotek, Winooski, VT). Cell culture media, immunohistochemical staining reagents, protein assays, Live/Dead assay, PrestoBlue Assay, RNA extraction kit and cDNA reverse transcription kit was all purchased from Life technologies (Grand Island, NY). The concentration of calcium ions in the supernatant was measured with inductively coupled plasma optical emission spectrometry (ICP-OES) (Agilent Technologies 700 series, Santa Clara, CA, USA) . Real time polymerase chain reaction (RT-PCR) was performed in the Applied Biosystems Real-Time PCR Instruments - 7500 Fast System (Life technologies, Grand Island, NY).
Statistics.
[0093] Unless otherwise indicated, all experiments were conducted at three replicates (n=3) . All quantitative data is presented as the average ± standard deviation.
Example 1
Synthesis of Fmoc-YGFGG-Resin
[0094] The synthesis of Fmoc-YGFGG-Resin was carried out with solid phase synthesis via microwave assistance in a Liberty 1 peptide synthesizer, as shown in Scheme 2 below.
Scheme 2
Figure imgf000035_0001
0.25 mmol Fmoc-Gly-Wang Resin was added to the reaction vessle. The resin was first swelled in DMF for 15 minutes. And then the deprotection step, which was removing the Fmoc group to generate amine, was followed by adding 20 v% piperidine in DMF with 0.1 M HOBt with microwave assisstance programed by the Liberty 1 software. After thouroughly washing the resins, in the coupling step, 5 mL Fmoc-AA-OH (AA represents amino acid) solution (4 equiv., 0.2 M in DMF), the activator HBTU (4 equiv., 2 mL of 0.5 M in DMF) and the activator base of DIPEA (8 equiv., 1 mL of 2 M in NMP) were added to couple the amino acid to the the N- termini of peptides on resin with microwave assistance. The whole process was programed and carried out automatically by the Liberty 1 peptide synthesizer. The obtained Fmoc-protected peptides on resin directly went to Example 2.
Example 2
Synthesis of dendron-YGFGG-Resin.
[0095] The Lys-based dendron was conjugated to the OGP(10-14) peptide of Example 1, above by using Fmoc-Lys(Fmoc)-OH XV in the coupling step as shown in Schme 3, below.
Scheme 3 i. deprotection, mw. H2N ^/ F-G-G-
Fmoc— Y-G-F
ii. Fmoc-Lys(Fmoc)-OH,
coupling, mw.
(XV) iii. deprotection, mw.
(XVI) i. Fmoc-Lys(Fmoc)-OH,
coupling, mw.
mw.
Figure imgf000036_0001
Peptide XVI was used for the synthesis of OGP-(Cat)2, and peptide XVII was used for the synthesis of OGP-(Cat)4. (See, Example 5). The deprotectioin and coupling was carried out in peptide synthesizer under standard conditions. The obtained peptides on resin directly went to Example 3.
Example 3
Synthesis of dendron-PEG-YGFGG-Resin
[0096] The hexaethylene glycol flexible linkage IX was conjugated to the peptides on resin XV of Example 2 by using Fmoc-NH-PEG6-propionic acid IX in the coupling step, as shown in Scheme 4 below.
Scheme 4
Figure imgf000037_0001
Then the Lys-based dendron was linked to the peptides, as shown in Scheme 4 above. Peptide XI was used for the synthesis of OGP-PEG-(Cat)2, and peptide XVIII was used for the synthesis of OGP-(Cat)4. (See Example 5). The deprotection and coupling were carried out in a peptide synthesizer under standard conditions. The obtained peptides on resin directly went to Example 5.
Example 4
Synthesis of 2,2-Dimethyl-l,3-benzodioxole-5-propanoic acid XII
[0097] 2,2-Dimethyl-l,3-benzodioxole-5-propanoic acid XII was synthesized as set forth in Scheme 5, below.
Scheme 5
Figure imgf000037_0002
[0098] Synthesis of methyl 3-(3,4-dihvdroxyphenyl)propanoate XX. 3,4- dihydroxyhydrocinnamic acid XIX (12.5 g, 68.6 mmol) was dissolved in 100 niL anhydrous MeOH and cooled with ice bath. Thionyl chloride (13.0 mL, 171.5 mmol) was added dropwise with stirring. Ice bath was removed after 30min and the reaction was stirred at r.t. for 24 h. Solvent was removed by rotary evaporation. Dried under high vacuum gave product as a dark blue viscous oil quantitatively. The oily product became solid after being placed in the freezer. ¾ NMR (500 MHz, CDC13) : 2.61 (t, J = 7.70 Hz, 2H), 2.83 (t, J = 7.70Hz, 2H), 3.69 (s, 3H), 5.69 (br. s., 2H), 6.60 (dd, J = 8.07, 1.96 Hz, 1H), 6.71 (d, J = 1.96 Hz, 1H), 6.77 (d, J = 8.07 Hz, 1H). 13C NMR (125 MHz, CDC13) : 30.25, 35.94, 51.89, 115.43, 120.51, 133.19, 142.12, 143.66, 174.38.
[0099] Synthesis of 2,2-Dimethyl-l ,3-benzodioxole-5-y>rov>anoic acid methyl ester XXI. Methyl 3-(3,4-dihydroxyphenyl)propanoate XX (5.18 g, 26.4 mmol) and 2,2- dimethoxypropane (13 mL, 106 mmol) were added to 200 mL anhydrous benzene in a 250 mL two-neck round bottom flask. One neck of the flask was equipped with Soxhelet extractor and the other neck was sealed with a septum for sampling. The thimble in the extractor was filled with granular anhydrous CaCl2 to trap MeOH and H20. The mixture was flushed with argon for 10 min and then heated to reflux under N2 for 5 min. p-Toluenesulfonic acid monohydrate (PTSA, 0.25 g, 1.3 mmol) was added quickly and the reaction was monitored by the ferric chloride test. The reaction was stopped and cooled to room temperature once a negative test was achieved (about 3 hrs). The yellow reaction mixture was filtered through a short silica-gel column and washed with DCM. The combined filtrate and washings were concentrated via rotovap and purified by silica-gel column. The eluent was DCM/hexane (1/50, v/v) followed by EtOAc/hexane (1/25, v/v) . Yellow oil (5.5 g, 88%) was obtained as the product. ¾ NMR (300 MHz, CDC13) : 1.65 (s, 6H), 2.58 (t, J = 7.90 Hz, 2H), 2.85 (t, J = 7.76 Hz, 2H), 3.67 (s, 3H), 6.56 - 6.67 (m, 3H) . 13C NMR (75 MHz, CDC13) : 25.81, 30.71, 36.05, 51.57, 108.01, 108.52, 117.63, 120.39, 133.60, 145.79, 147.45, 173.31.
[00100] Synthesis of 2,2-Dimethyl-l ,3-benzodioxole-5-propanoic acid XII. LiOH aqueous solution (0.33 g, 13.9 mmol dissolved in 8 mL H20) was added to a methanol solution of 2,2-Dimethyl-l,3-benzodioxole-5-propanoic acid methyl ester XXI (1.64 g, 6.93 mmol dissolved in 8 mL of methanol) in portions. After overnight reaction, methanol was removed by rotovap. The pH of the remaining solution was adjusted to 5 - 6 by 2 M HCl. The mixture was then extracted with EtOAc for three times. The combined organic layers were dried with Na2S04 and evaporated in vacuo to obtain a white solid as product (1.30 g, 84%). ¾ NMR (500 MHz, CDC13): 1.65 (s, 6H), 2.55 - 2.63 (m, 2H), 2.79 - 2.88 (m, 2H), 6.55 - 6.66 (m, 3 H), 9.34 (br. s., 1H). 13C NMR (125 MHz, CDC13) : 25.79, 30.72, 36.70, 108.01, 108.53, 117.60, 120.37, 133.61, 145.80, 147.48, 179.38.
Example 5
Synthesis of OGP-(Cat)n and OGP-PEG-(Cat)n.
[00101] OGP-(Cat)n and OGP-PEG-(Cat)n. were synthesized as shown in Scheme 6, below.
Scheme 6
η( Η2
Figure imgf000039_0001
The resins with peptides 1-4 (See Examples 2, 3, above) were each transferred into a peptide reaction vessle. For each peptide, the resins were firstly swelled in DMF for 15 minutes. After aspiration, 20 mL DMF was added into each reaction vessle. With nitrogen boubling the solution, acetonide-protected 3,4-dihydroxyhydrocinnamic acid (4 equiv. to each amine), HOBt (10 equiv. to each amine), and DIC (10 equiv. to each amine) were added sequetially to each reaction vessel. Each reaction was carried out at ambient temperature with nitrogen boubling for 4 hours.
[00102] After aspiration, the resin in each reaction vessel was washed by DMF, DCM and MeOH, three times each for 2 minutes. Then, each of the resins were immersed in 30 mL cleavage cocktail (trifluoroacetic acid 95%, triisopropylsilane 2.5%, H20 2.5%, v/v) for 0.5 hour with nitrogen boubling. The solutions were collected and concentrated to ~ 3 mL with Roto Vapor. The peptides were precipitated in cold ether three times. Due to the poor solubility of products in IxPBS buffer, all of the peptides were dissolved in a mixed solvent of IxPBS buffer and ethanol (v/v 1 :1), followed by transfer into dialysis tube (MWCO 500 Da), and dialysis against dilute HCl solution (pH= 3—4) . After dialysis, the product may precipitate, so the insoluble portion was dissolved with ethanol, combined with the solution inside the dialysis tube, and freeze dried. The gradient elution of RP-HPLC changed linearly from 10% to 80% B within 15 column volumes.
[00103] The catechol-bearing peptides were characterized with either Electrospray Ionization Mass Spectrometry (ESI-MS) or MALDI-ToF mass spectrometry, depending on their molecular weight. OGP-Cat: [M+ H] + m/z was calculated to be 792.4 and measured at 792.6. OGP-(Cat)2: [M + H] + m/z was calculated to be 956.4 and measured at 956.5. OGP-(Cat)4: [M+Na] + m/z was calculated to be 1562.7 and measured at 1562.7. OGP-PEG-Cat: [M+ H] + m/z was calculated to be 1127.5 and measured at 1127.6. OGP-PEG-(Cat)2: [M+Na] + m/z was calculated to be 1313.6 and measured at 1313.7. OGP-PEG-(Cat)4: [M+Na] + m/z was calculated to be 1897.9 and measured at 1898.3. See FIGS. 1A-F. The total yield calculated from the staring Fmoc-Gly-Wang Resin (0.25mmol) was: OGP-Cat: 25%, OGP-(Cat)2: 23%, OGP-(Cat)4: 12%, OGP-PEG-Cat: 20%, OGP-PEG-(Cat)2: 15%, and OGP-PEG-(Cat)4: 9%.
Example 6
Synthesis of FITC-labeled OGP-Cat.
[00104] FITC-labeled OGP-Cat was synthesized as set forth in Scheme 7, below.
Scheme 7
Figure imgf000040_0001
(xxiv) (xxvi)
To the solution of OGP-Cat (6 mg) XXIV and N,N-Diisopropylethylamine (DIPEA) (3 mg, 3 equiv.) in 0.2 mL anhydrous DMF, the solution of fluorescein isothiocyanate (FITC) XXV (6 mg, ~2 equiv.) in 0.2 mL anhydrous DMF was added dropwise. The mixture was covered with aluminum foil and stirred at ambient temperature overnight. After the reaction, DMF was evaporated under vacuum, and the obtained orange solid was dissolved in 15 mL 25 mM HEPES buffer and filtered through a 0.22 μπι filter to separate the overdosed insoluble FITC. The product was characterized with MALDI-ToF mass spectrometry. FITC-labeled OGP-Cat [M + H] + m/z was calculated to be 1181.4 and found in 1181.6. The solution of FITC-labeled OGP-Cat (0.5 mM) was used directly to immobilize onto Ti02 surface without further purification.
Example 7
Quartz crystal microbalance with dissipation (QCM-d) measurement.
[00105] Quartz crystal microbalance with dissipation (QCM-d) was used to determine the binding isotherm for OGP-(Cat)4 on Ti02, Fe203, Fe304, Zr02, Ce02, Si02, and Au substrates. The AT cut sensors were purchased from Biolin Scientific AB (Sweden) and cleaned before use according to the protocol provided by the company. The sensor was excited at 5 MHz as its fundamental frequency. The frequency shift (Af) and dissipation (AD) were measured at 3rd, 5th, 7th, 9th, 11th and 13th overtones. 25 mM HEPES buffer (pH= 7.40 at 25°C) was used as the flow medium. Sensors were mounted in the modules immediately after cleaning. HEPES buffer flowed above the sensors until a flat baseline was achieved at flow rate of 0.150 mL/min. Then solutions of catechol-bearing peptide (OGP-(Cat)4) in HEPES buffer were introduced and the flow continued until the adsorption reached its equilibrium state. If necessary, solutions at higher concentrations were introduced sequentially. Lastly, HEPES buffer was introduced again to wash the adsorbed layer. Three independent measurements were done simultaneously. The results are reported on FIG. 5.
Example 8
Calculation of adsorbed area mass.
[00106] The QCM-d measurements in Example 7 above may be used to calculate the adsorbed area mass. The adsorbed area mass was proportional to the frequency shift (Af) and calculated by the Sauerbrey Equation. Sauerbrey Equation is Am = — ^Δ η, where C is the mass sensitivity constant with the value of 17.7 ng Hz"1 cm"2 for 5 MHz fundamental frequency crystal, n is the frequency overtone number, and n= 7 was chosen to calculate the adsorption area mass. As long as the adsorbed mass is small compared to the crystal, sufficiently thin, and has limited viscoelastic coupling with the surrounding medium (AD < l x lO"6 per 10 Hz), this relationship is valid. Adsorbed area mass measured from QCM-d includes water contained in the adhering layer. For adsorptions of OGP-(Cat)n and OGP-PEG-(Cat)n (n= 1, 2, 4) onto substrates, AD were below l x lO"6 per 10 Hz, and measurements from multiple overtones were close to each other, indicating adsorbed films were rigid, and the effect from content of water was slight.
Example 9
Models used to fit the adsorption isotherm.
[00107] The adsorption isotherms of OGP-(Cat)n and OGP-PEG-(Cat)n (n = 1, 2, 4) binding to Ti02 surface respectively were fit using a single-site specific binding model,
Am = -J≡— , where Am is the amount of adsorbed analyte, c is the concentration of
Kd+ c
the analyte solution, Bmax is the maximum adsorption of analyte on the surface, and Kd is the apparent dissociation constant.
Example 10
Sputtering coating of Ti02.
[00108] For the Ti02 substrates used herein, glass slides and silicon wafers were cleaned by sonication in 2% SDS solution for 30 minutes followed by thoroughly rinsing with water, dried with nitrogen and UV-ozone treatment for 20 minutes. The Ti02 target (99.99% pure, 2.00" diameter x 0.125" thickness) were purchased from Kurt J. Lesker (USA). The Ti02 films were deposited by RF-magnetron sputtering using the following conditions at ambient temperature for lh, power 75 W, 5 Vbias, deposition distance 5 cm, Ar 86 seem, 02 9 seem, and total pressure 42 mtorr (pAr=34 mtorr, po2= 8 mtorr) . For the fabrication of Ti02 patterns on glass slides, 300 mesh Cu grids were placed on the top of glass.
[00109] The obtained Ti02 shows the O/Ti ratio of 2, matching with the theoretical stoichiometry. Some carbon and fluorine contamination existed. See FIG. 7. Example 11
Immobilization of OGP-(Cat)n and OGP-PEG-(Cat)n onto Ti02-coated substrates.
[00110] OGP-(Cat)n and OGP-PEG-(Cat)n (n= 1, 2, 4) were dissolved in HEPES buffer at concentrations of 50 μηιοΙ/L. Substrates were immersed into the solution (800 μϋ, for 20 mm x 20 mm glass slides, 500 μϋ, for 5 mm x 5 mm silica wafer) and incubated at ambient temperature overnight. After that, the substrates were rinsed thoroughly with water to wash away the unbounded molecules, dried with nitrogen and subjected to further study.
Example 12
X-ray photoelectron spectroscopy (XPS).
[00111] X-ray photoelectron spectroscopy (XPS) was used to confirm the presence of the OGP peptide on the surface of the substrate by the presence of nitrogen. The XPS measurements were performed on a Kratos AXIS Ultra DLD spectrometer. The X- ray source was monochromated Al Ka, scanning over a binding-energy range of (0 to 700) eV with a dwell time of 100 ms. The analyzer pass energy was 110 eV for the survey spectra and 11 eV for the high-resolution Cls, Nls, and Ols scans. Each spectrum was collected over a 300 x 700 μπι sample area. The results are reported in FIGS. 7, 9A-D, 12, 13, and 17. .
Example 13
Fluorescence intensity measurement.
[00112] The florescence intensity of FITC-OGP-(Cat)n (n= l, 2, and 4) on Ti02, Fe203, Fe304, Zr02, Ce02, Si02, and Au substrates was viewed with an inverted 1X81 Microscope (Olympus, Center Valley, PA) with mercury bulb excitation and the appropriate filters. Displayed images were taken using identical settings, including exposure time (4.99 s), gain (10.04) and magnification ( x 20) . The mean intensity was calculated based on at least 10 randomly chosen sites observed under the same conditions. The results for Ti02 and Si02 substrates are reported in FIGS. 10A-B and 11. Example 14
Sterilization of substrates and OGP-PEG-(Cat)4 solution.
[00113] The Ti02-coated glass slides were sterilized by washing with ethanol and UV irradiation for 30 minutes. The OGP-PEG-(Cat)4 in HEPES buffer solution was sterilized by filtration through a 0.2 μπι sterile syringe filter (EMD Millipore Millex).
Example 15
Fabrication of substrates for cell study.
[00114] The immobilization of OGP-PEG-(Cat)4 onto Ti02 substrates is convenient by immersion the substrates into the solution of OGP-PEG-(Cat)4 and followed incubation for overnight. Due to the strong binding affinity, the concentration of the OGP-PEG-(Cat)4 solution is very low. By using = 100 x Kd = 2.8 μτηοΙ/L and C2 = Kd = 28 nmol/L, OGP-PEG-(Cat)4 modified Ti02 substrates, OGP-99% and OGP- 50%, were successfully prepare with 99% and 50% coverage of maximum adsorption, respectively, as shown in Table 4. Table 4 shows the immobilization of OGP(10-14) on Ti02 surface by immersion the substrates in the solution of OGP-PEG-(Cat)4 at different concentration for overnight and their respective load amount calculated in theory and measured with XPS.
Table 4.
Substrates for bioactivity evaluation.
Figure imgf000044_0001
Note: The load amount was calculated with the single site specific binding model, Am =
^222— , where Am is the amount of adsorbed analyte, c is the concentration of the analyte solution, Bmax is the maximum adsorption of analyte onto the surface, and Kd is the apparent dissociation constant. For OGP-PEG-(Cat)4, Kd is 0.028 + 0.008 μιηοΙ/L, and Bmax is 196 + 23 ng/cm2, as characterized in the previous work.
Example 16
Cell culture
[00115] MC3T3-E1 mouse preosteoblast (passage 17) were expanded and cultured in a-MEM media (Gibco, Life Technoligies, Grand Island, NY) supplemented with 10% fetal bovine serum (FBS) (Invitrogen), 100 units/mL penicillin (Invitrogen), and 100 μg/mL streptomycin (Invitrogen) at 37°C in a 5% C02 humidified atmosphere. The cells were subcultured every 3 days in the presence of 0.25% (w/v) trypsin and 0.5 % (w/v) ethylenediaminetetraacetic acid tetrasodium salt (EDTA) solution. Cells were seeded on substrates at 18 cells/mm2 and fed every two days.
Example 17
Viability assay
[00116] Viability of the cell culture of Example 16 above was evaluated using a Live/Dead viability/cyto toxicity kit (Invitrogen, UK) . Briefly, 5 μϋ, of the 4 mM Calcein-AM stock solution and 10 μϋ, of the 2 mM ethidium homodimer-1 (EtmD-1) stock solution were added to 10 mL of cell culture medium to prepare the Live/Dead staining solution. 1 mL of staining solution was added into each well in a 6-well plate, after aspiration of the old medium. The samples were incubated for 10 min in Live/Dead staining solution. The staining solution was removed and the samples were viewed under the IX81fluorescence microscope (Olympus) with 494 nm (green, Calcein) and 528 nm (red, EthD-1) emission filters. For quantitative analysis a total of 250 cells were counted from each sample over 25 randomly chosen areas and the viable and non-viable cells counts were recorded. The results are reported in FIGS. 7 and 17.
Example 18
Immunohistochemical staining of cytoskeletal actin and vinculin.
[00117] All samples of cell coated substrates (See Examplel6 and 17) were prefixed in pre-warmed 0.8 mL cell culture media and 1.2 mL 3.7% paraformaldehyde (PFA) in CS buffer for 5 minutes on a dry block at 37°C. After aspiration, samples were fixed in 3.7 % PFA solution at 37°C for 5 minutes. After washing with lxPBS 3 times, 1.5 mL of Triton X-100 in CS buffer (0.5% v/v) was added to each well to permeabilize the cells for 10 minutes on a dry block at 37°C. The substrates were washed 3 times with l xPBS. Freshly made 0.1 wt% NaBH4 in lxPBS was then added for 10 minutes at r.t. to quench the aldehyde fluorescence, followed by aspiration and incubation in 5% donkey serum for 20 minutes at r.t. to block the non-specific binding. After aspiration, the substrates were incubated in vinculin primary antibody Mouse in l xPBS (v/v 1 :200) at 4°C overnight. After washing with 1% donkey serum 3 times, the substrates were stained in a solution of rhodamine phalloidin (v/v 1 :40) and Alexa Flour 488 secondary antibody Mouse (v/v 1 :200) for 1 hour at r.t., avoiding light. After washing with lxPBS 3 times, the nuclei were stained with DAPI in l xPBS (6 μΐ/ 10 mL) for 20 minutes at r.t. in the dark. After washing with lxPBS 3 times to remove excess staining, the samples were mounted and viewed under an 1X81 Microscope (Olympus, Center Valley, PA) with mercury bulb excitation and the filters of FITC, TRITC and DAPI. The images showed the differences in cell morphology imparted by each concentration.
Example 19
Cell proliferation assay
[00118] Cell proliferation of MC3T3-E1 cells of Example 16 on OGP-99%, OGP- 50% and Ti02 substrates was evaluated by the PrestoBlue Assay (Life technologies, Grand Island, NY) following the provided protocol. The standard curve was prepared in duplicate by seeding cell suspensions at known concentrations into a 24-well plate at least 6 hours before the experiment for full attachment. Nine descending cell concentration and one blank were included in the standard curve. The PrestoBlue solution was prepared by dilution with cell culture medium (v/v 1 :9) . After aspirating the old medium, 1.5 mL of PrestoBlue solution was added to each well, followed by incubation at 37°C in the incubator for 2-4 hours. A color change from blue to purple and to pink ultimately was observed during incubation. When the standard curve fluorescence could be fit to a linear line, the samples' fluorescence was read. 100 μί solution was taken from each well in triplicate and placed in a 96-well plate. The change in cell viability was detected by fluorescence intensity (FI) in Plate Reader by excitement at 570 nm and emission at 615 nm. The standard curve was fit with a linear relationship by plotting FI vs Cell Number. The coefficient of determination (R2) was above 0.99.
Example 20
Immunohistochemical staining of bone sialoprotein (BSP) and osteocalcin (OCN).
[00119] All samples of cell coated substrates (Examples 16 and 17) were pre-fixed in pre-warmed 0.8 mL cell culture media and 1.2 mL 3.7% paraformaldehyde (PFA) in CS buffer for 5 minutes on a dry block at 37°C. After aspiration, samples were fixed in 3.7 % PFA solution at 37°C for 5 minutes. After washing with lxPBS 3 times, blocking buffer (10% normal donkey serum, 0.3% Triton X-100 in IxPBS) was added into each well and incubated for 45 minutes at r.t. to block the non-specific binding. After aspiration, the substrates were incubated in bone sialoprotein (BSP) primary antibody Mouse (v/v 1:400) and osteocalcin (OCN) primary antibody Goat in IxPBS (v/v 1:100) overnight at 4°C. After washing with 1% donkey serum 3 times, the substrates were stained by incubation in a solution of Alexa Flour 488 secondary antibody Mouse (v/v 1:200) and Alexa Flour 546 secondary antibody Goat (v/v 1:200) in IxPBS for 1 hour at r.t. in the dark. After washing with 1% donkey serum 3 times, the nuclei were stained with DAPI in IxPBS (6 μϋ, / 10 mL) for 20 minutes at r.t. avoiding light. After washing with IxPBS once, the samples were mounted and viewed under an 1X81 Microscope (Olympus, Center Valley, PA) with mercury bulb excitation and the filters of FITC, TRITC and DAPI. These images showed that the cells having 99% OGP coverage expressed a much higher gene level of BSP and OCN on all of the substrates tested..
Example 21
Alizarin Red S. Staining
[00120] Samples of cell coated substrates (Examples 16 and 17)were pre-fixed in pre-warmed 0.8 mL cell culture media and 1.2 mL 3.7% paraformaldehyde (PFA) in CS buffer for 5 minutes on a dry block at 37°C. After aspiration, samples were fixed in 3.7 % PFA solution at 37°C for 5 minutes. Freshly made Alizarin Red S. solution (0.8 g in 40 mL dd H20, pH adjusted to 4.2), was added into substrates that are washed 3 times with dd H20 to remove soluble calcium. After incubation at r.t. for 40 minutes, the Alizarin Red S. solution was carefully removed. The substrates were washed with double distilled H20 4 times, mounted and observed under bright field microscope. These images showed significantly higher Ca+2 levels for the OGP-99% than the OGP- 50% or Ti02 substrates. See FIG. 15C.
Example 22
Alkaline phosphatase (ALP) activity assay
[00121] ALP activity was measured by SensoLyte pNPP ALP Assay Kit (AnaSpec Inc, San Jose, CA, USA) following the provided protocol. The MC3T3-E1 cells on OGP-99%, OGP-50% and Ti02 substrates were washed with lx Assay Buffer twice. (See FIG. 15A). The cell film was peeled from the substrates and transferred into a 1.5 mL centrifuge tube, followed by addition of 0.5 mL lysis buffer (20 μϋ, Triton X- 100 in 10 mL l x Assay Buffer) . The cells was resuspended and incubated in the lysis buffer for 10 min at 2500 xg at 4°C. After centrifuge, the supernatant was collected for analysis. A standard curve was measured with an ALP solution at concentrations of 0, 3.1, 6.2, 12.5, 25, 50, 100, 200 ng/mL. 50 μί of sample/standard solution and 50 μϋ, pNPP solution was added into each well in a 96-well plate. The solution was mixed by gently shaking for 30 sec. After incubation for 30 min, the 96-well plate was shaken for 1 min before measuring the absorbance at 405 nm. Three replicates were measured for each sample. The standard curve was fitted with a linear relationship by plotting Ab. vs ALP concentration, with a coefficient of determination (R2) above 0.98. See FIGs. 15A-B.
[00122] To normalize the ALP activity with total protein amount, the amount of total protein was quantified with a DC protein assay (Bio-Rad, Hercules, CA, USA) . A standard curve was measure with BSA solution at amount of 0, 0.2, 0.5, 0.8, 1.1, 1.43 mg/mL with lx ALP Assay Buffer as the dilution buffer. 5 μΐ, of standards and samples were added into a 96-well plate. Then 25 μΐ, of reagent A and 200 μΐ, reagent B were added. The plate was shaken for 30 sec to well mix the solution, which was left to incubate for 15 min. The absorbance at 750 nm was read. The standard curve was fitted with a linear relationship by plotting Ad. vs BSA amount, with a coefficient of determination (R2) above 0.96.
Example 23
Calcium quantification.
[00123] The MC3T3-E1 cells on OGP-99%, OGP-50% and Ti02 substrates were washed with DPBS buffer (Mg2+, Ca2+ free) once. The cell film was peeled from the substrates and transferred into a 1.5 mL centrifuge tube, followed by addition of 300 μΐ, double distilled H20. Three freeze-thaw cycles were carried out to destroy the cell membrane, followed by the addition of 300 μί 1 M HCl. The samples were agitated at r.t. overnight. The concentration of calcium ions in the supernatant was measured with inductively coupled plasma optical emission spectrometry (ICP-OES) (Agilent Technologies 700 series, Santa Clara, CA, USA). The emission wavelength was set at 393.366 nm to quantify Ca2+. A standard curve was measured with solutions of c(Ca2+) equal to 0.125, 0.25, 0.5, 1, and 2 ppm. Triplicate measurements were carried out for each sample. The calcium amount of each sample was normalized with total protein amount, which was done in the same way as set forth above for the ALP activity assay. See FIG. 15C.
Example 24
Real time-polymerase chain reaction (RT-PCT).
[00124] Total RNA was isolated from the cell coated substrates (See, Examples 16 and 17) on day 18 with an RNA extraction and isolation kit (Applied Biosystems, Life Technologies), following the provided protocol, and was quantified by ultraviolet spectroscopy. The synthesis of complementary DNA (cDNA) was performed with a high-capacity cDNA reverse transcription kit with RNase inhibitor (Applied Biosystems, Life Technologies) using 800 ng total RNA as the template in a 100 μί reaction following the provided protocol. RT-PCR was performed with non-specific detection fluorescence, SYBR Green, or double-dye probe detection, and TaqMan probes system (Applied Biosystems, Life Technologies) . For SYBR Green system, 10 ng of cDNA product and lx SYBR Green master mixture (Applied Biosystems, Life Technologies) were included in 50μΙ, reaction mixture (209.4 nM each primer). For TaqMan system, 24 ng of cDNA product and lxTaqMan master mixture (Applied Biosystems, Life Technologies) were included in 25μΙ, reaction mixture. The housekeeping gene was glyceraldehyde-3-phosphate dehydrogenase (GAPDH). All oligonucleotide primers (See Table 5, below) were purchased from Applied Biosystems (Life Technologies). The ALP primer (alpl gene from Mouse) was also purchased from Applied Biosystems (Life Technologies) . RT-PCR was performed in the Applied Biosystems Real-Time PCR Instruments - 7500 Fast System (Life technologies, Grand Island, NY) with recommended programs by the supplier.
Table 5
Primers used to examine OGP (10-14) on cell markers of osteogenic differentiation.
Figure imgf000050_0001
The results are shown in FIGS. 15B and 18. The data reported in FIG. 18 represents relative expression to the level of the control (cells on Ti02), set at 1, and mean value and standard deviation calculated from triplicates. The cells having 99% OGP coverage (OGP-99% substrate) expressed a much higher gene level of BSP and OCN, compare to cells on bare Ti02.
[00125] In light of the foregoing, it should be appreciated that the present invention significantly advances the art by providing a multivalent dendron that is structurally and functionally improved in a number of ways. While particular embodiments of the invention have been disclosed in detail herein, it should be appreciated that the invention is not limited thereto or thereby inasmuch as variations on the invention herein will be readily appreciated by those of ordinary skill in the art. The scope of the invention shall be appreciated from the claims that follow.

Claims

CLAIMS What is claimed is:
1. A multivalent dendron comprising a bioactive peptide domain and one or more surface-binding catechol domains.
2. The multivalent dendron of claim 1, further comprising a flexible linkage between said bioactive peptide domain and said one or more surface- binding catechol domains.
3. The multivalent dendron of claim 1, wherein said bioactive peptide domain comprises a bioactive peptide selected from the group consisting of:— NH- KIPKASSVPTELSAISTLYL-COOH, BMP-2, OGP, OGP C-terminal sequence (YGFGG), and combinations thereof.
4. The multivalent dendron of claim 3, wherein said bioactive peptide is less than 30 amino acids in length.
5. The multivalent dendron of claim 3, wherein said bioactive peptide is less than 20 amino acids in length.
6. The multivalent dendron of claim 3, wherein said bioactive peptide is OGP C-terminal sequence (YGFGG).
7. The multivalent dendron of claim 1 having a valence of from 1 to 8.
8. The multivalent dendron of claim 1 wherein said flexible linkage comprises an oligomer of polyethylene glycol, polyethylene glycol, polypropylene glycol, or polyethylene.
9. The multivalent dendron of claim 1 wherein said flexible linkage comprises a polyethylene glycol oligomer having from 1 to 20 ethylene glycol units.
10. The multivalent dendron of claim 1 having the formula:
Figure imgf000052_0001
wherein PEP is a bioactive peptide; R is selected from the group consisting of -CH3, -(CH2)3NHC(NH2)C=NH, -CH2CONH2,-CH2COOH, -CH2SH, - (CH2)2COOH, -(CH2)2CONH2, -NH2, -CH2C = CH-N=CH-NH,
CH(CH3)CH2CH3, -CH2CH(CH3)2, -(CH2)4NH2, -(CH2)2SCH3, -CH2Ph, - C! 1,01 1, -CH(OH)CH3, -CH2-C= CH-NH-Ph, -CH2-Ph-OH, -CH(CH3)2, and combinations thereof; a is an integer from 1 to 20; and m is 0 or 1.
11. The multivalent dendron of claim 1 having the formula:
Figure imgf000052_0002
wherein PEP is a bioactive peptide; a is an integer from 1 to 20 and m is 0 or 1.
12. The multivalent dendron of claim 1 having the formula:
Figure imgf000052_0003
wherein PEP is a bioactive peptide; a is an integer from 1 to 20; and m is 0 or 1.
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