IN VIVO METHODS OF MONITORING BIODISTRIBUTION

Information

  • Patent Application
  • 20140161723
  • Publication Number
    20140161723
  • Date Filed
    February 09, 2012
    12 years ago
  • Date Published
    June 12, 2014
    10 years ago
Abstract
Functional-lipid constructs of the structure F-S-L are disclosed, wherein F comprises a tyrosine or histidine residue, S is a spacer covalently linking F to L and L is a lipid. The functional residue may be iodinated and used to radiolabel a biological entity with 1251 and the iodinated constructs are used in a non-invasive method of monitoring the distribution of a biological entity in vivo.
Description
FIELD OF INVENTION

The invention relates to a non-invasive method of monitoring the distribution of cells and virions in vivo and constructs for use in the method.


BACKGROUND ART

Existing methods for monitoring the distribution of biological entities in vivo require covalent or genetic modification of the entity. Such modification may result in the behaviour of the biological entity in vivo being modified.


Therapeutic applications where viruses are administered to a subject are in development. These applications include gene therapy and tumour destruction (oncolytic virotherapy) (Lui et al (2007)). In the development of these therapies it is a requirement to be able to monitor the distribution of the virion following administration without altering its infectivity (Herschman (2003); Yamamoto and Curiel (2010))


Monitoring the distribution of virions following administration is problematic employing existing methods. Tissue biopsy is invasive and is of limited use in clinical trials (Kuruppu and Tanabe (2005); Waehler et al (2007)). Non-invasive methods such as magnetic resonance imaging (MRI), positron emission tomography (PET) and X-ray computed tomography (CT) usually require image enhancing agents or chemical modification of the virion (Piwnica-Worms et al (2004); Strable and Finn (2009)).


Viruses may be engineered to incorporate reporter genes. However, monitoring the expression of these genes only indicates where the genes of the virus are being expressed (Peng et al (2003); Waehler et al (2007)).


It is an object of this invention to provide a convenient alternative to these existing methods with application to biological entities in addition to enveloped viruses (virions).


STATEMENT OF INVENTION

In a first aspect the invention provides a method of radiolabelling a biological entity comprising the step of contacting a suspension of the biological entity with an iodinated (125I) construct of the structure F-S-L for a time and at a temperature sufficient to allow localisation of the 125I to the surface of the biological entity where F comprises an iodinated histidine (His) residue or an iodinated tyrosine (Tyr) residue, S is a spacer covalently linking F to L, and L is a lipid.


In a second aspect the invention provides a non-invasive method of monitoring the distribution of a biological entity in a subject in vivo comprising the steps of:

    • contacting a suspension of the biological entity with a an iodinated (125I) construct of the structure F-S-L for a time and at a temperature sufficient to provide a 125I-labelled biological entity;
    • administering to the subject the 125I-labelled biological entity to a subject; and
    • monitoring the distribution of the biological entity by radioactivity bioscanning,


      where F comprises an iodinated histidine (His) residue or an iodinated tyrosine (Tyr) residue, S is a spacer covalently linking F to L, and L is a lipid.


Preferably, the suspension is an aqueous suspension. S is selected to provide a construct of the structure F-S-L that is readily dispersible in water yet spontaneously incorporates into lipid bilayers, including the membranes of cells and enveloped viruses. Preferably, the biological entity is a cell or an enveloped virus. The 125I-labelled biological entity may be administered to the subject by injection. Preferably, the 125I-labelled biological entity is administered to the subject by intraperitoneal infusion or intravenous injection.


Preferably, F comprises an iodinated tyrosine (Tyr) residue. More, preferably the tyrosine (Tyr) residue is an N-carbonyl-Tyr residue. Most preferably, the tyrosine (Tyr) residue is an N-carbonyl-Tyr residue selected from the group consisting of: N—COH (N-formyl) Tyr residues and N—CO(CH2)2COOH Tyr residues.


In a third aspect the invention provides constructs of the structure F-S-L for use in the methods of the first aspect and the second aspect of the invention.


Preferably, the constructs are of the structure:




embedded image


where M is H or CH3 and * is other than H.


Preferably, F is a tyrosine residue selected from the group consisting of:




embedded image


embedded image


Preferably, L is phosphatidylethanolamine. More preferably, L is is selected from the group consisting of: 1,2-O-dioleoyl-sn-glycero-3-phosphatidylethanolamine (DOPE) and 1,2-O-distearyl-sn-glycero-3-phosphatidylethanolamine (DSPE). Most preferably, L is 1,2-O-dioleoyl-sn-glycero-3-phosphatidylethanolamine (DOPE).


In a first embodiment of the third aspect of the invention the constructs are of the structure N-formyl-(Tyr)n-S-L where n is an integer from 1 to 6 inclusive. Preferably, n is 1 and the construct is of the structure:




embedded image


designated FSL-tyrosine.


In a second embodiment of the third aspect of the invention the constructs are of the structure:




embedded image


embedded image


designated FSL-Tyr8.


In a second embodiment of the third aspect of the invention the constructs are of the structure:




embedded image


embedded image


designated FSL-Tyr4.


In the description and claims of this specification the following acronyms, terms and phrases have the meaning provided:


“Aqueous suspension” means a suspension prepared in water with or without the addition of buffers or salts and specifically includes a suspension in saline.


“Biological entity” means a cell, multicellular structure or virus.


“Localised” means associated with a surface by non-covalent interactions and “localising” and “localisation” have a corresponding meaning.


“Monovalent cation (M)” means a counter ion having a positive charge of one (+1).


“Readily dispersible in water” means forms a stable, monophasic dispersion on contact with water at 25° C. in the absence of detergents or organic solvents.


“( )x”, “( )x”, “[ ]x” and “[ ]x” mean the group contained in the parentheses is repeated a number (x) of times. By way of illustration:




embedded image


means the methylene group (—CH2—) is repeated 4 times and the structure represented is equivalent to:




embedded image


The terms “first”, “second”, “third”, etc. used with reference to elements, features or integers of the subject matter defined in the Statement of Invention and Claims, or when used with reference to alternative embodiments of the invention are not intended to imply an order of preference.


The invention will now be described with reference to embodiments or examples and the figures of the accompanying drawings pages.





BRIEF DESCRIPTION OF DRAWINGS


FIG. 1. Autoradiograph of free Na125I (left lane) and iodinated (125I) FSL-tyrosine (right lane) run on 15% acrylamide gel SDS-PAGE in non-reducing sample buffer.



FIG. 2. Iodinated (125I) FSL-tyrosine insertion into Vero cells. Vero cells 5×105 cells/well were contacted with either iodinated (125I) FSL-tyrosine or 125I (of equal cpm) and incubated for 2 hours at 37° C. Washed cells were lysed then radioactivity measured.



FIG. 3. VSV and MV incubated for 1 hour at room temperature with iodinated (125I) FSL-tyrosine or Na125I and harvested from the buffer or 20% sucrose portion of a step gradient tube following centrifugation for 75 min at 200 g.



FIG. 4. Ultracentrifuge 20% sucrose fractionations of iodinated (125I) FSL-tyrosine or 125I labeled VSV and MV.



FIG. 5. FSL-fluorescein (FSL-FLRO4) labelling of virions. (a) FACScan of FSL-fluorescein modified VSV. (b) Total fluorescence of H1N1 samples (8 haemagglutinin units of virus was taken in all cases) and labelled directly with FITC or modified with different concentrations of FSL-fluorescein (FSL-FLRO4). The fluorescence was read in 96-well plate with Victor2 multilabel counter (PerkinElmer, USA) at 495 nm. (c) FACScan of MDCK cells (transfected with 6-sialyltransferase) and infected with human A/Puerto Rico/8/1934 (H1N1) labelled either directly with FITC (green) or increasing levels of FSL-fluorescein (FSL-FLRO4). (d) FACScan of virions attached to a KAS6/1 cell suspension labelled with FSL-fluorescein (FSL-FLRO4) modified MV.



FIG. 6. Biodistribution of intraperitoneal (IP) infusions of iodinated (125I) FSL-tyrosine (FSL-125I) modified VSV, iodinated (125I) FSL-tyrosine (FSL-125I) and 125I. (a) Scans of two animals 1 hour post IP infusion and a sequential scan of one of the two animals at 4 and 24 hours post IP infusion. (b) Distribution by organ/tissue at one hour post IP infusion. (c) Distribution by organ/tissue at two hours post IP infusion.





DETAILED DESCRIPTION

The invention provides a convenient method of radio-labelling biological entities. The constructs of the invention are dispersible in water, spontaneously incorporate into membranes and conveniently iodinated (125I). The localisation of 125I to the biological entity by use of the iodinated construct permits real time monitoring of the distribution of the biological entity in vivo by non-invasive detection methods.


Known methods of radioiodination employ direct labelling of proteins or other target molecules or indirect labelling by first labelling an intermediate compound which is then used to perform the final modification (Hermanson (2008)). These known methods require termination of the direct labelling step or control of the final modification to ensure the correct degree of iodination. The constructs of the invention may be prepared with predetermined levels of radioactivity and used to quantitatively iodinate the biological entity. Use of constructs (F-S-L) comprising oligomers of tyrosine (FSL-Tyrosine) or dendrimers of tyrosine (FSL-Tyr4 and FSL-Tyr8) as the tyrosine (Tyr) residue (F) permits radiolabelling of biological entities at a range of specific activities with no variation in the degree of labelling of proteins or other target molecules.


Water dispersible constructs have been used both in vitro and in vivo to modify the surface of cells (Frame et al (2007); Heathcote et al (2010); Oliver et al (2011); Henry (2009)). The in vivo survival of red blood cells modified in this way has been demonstrated (Oliver et al (2011)). The normal in vivo development of murine embryos modified in this way has also been demonstrated (Blake et al (2003)).


The surface of enveloped virions is hydrophobic. The localisation of a fluorophore to the surface of virions has now been demonstrated in vitro using the construct designated FSL-fluorescein (Blake et al (2010)). A number of virions have been modified to incorporate this construct; vesicular stomatitis virus human IFNβ virus (VSV), measles virus encoding the human thyroidal sodium iodide symporter (MV) and H1N1 influenza virus (H1N1). The novel construct designated FSL-tyrosine can be readily iodinated (125I) and used in an analogous way to permit the real time monitoring of the distribution of virions in vivo.


The modification of virions using the dispersible constructs of the invention is dose dependent. The method also avoids exposure of the virions to incompatible reagents. The modification does not appear to significantly affect the infectivity of the virions or their ability to bind cell membranes as demonstrated by H1N1 fusion with ST cells and MV binding to KAS6/1 cells.


The distribution of VSV modified by the iodinated (125I) construct FSL-tyrosine is consistent with previously reported observations (Peng et al (2003)). Within an hour of administration the radiolabel localized to liver, spleen and bloodstream. Using the thyroid signal as an indicator it appears the modified virions are maintained in vivo for at least 4 hours. The localisation of modified virions to specific tissues can therefore be monitored quantitatively.


Materials and Methods

Trifluoroacetic acid (TFA), trifluoroethanol (TFE), 4-dimethylaminopyridine (DMAP), di-tert-Butyldicarbonate (Boc2O), 1-hydroxybenzotriazole (HOBt), DIEA-diisopropylethylamine, O-(benzotriazol-1-yl)-N,N,N′,N′-tetramethyluronium tetrafluoroborate (TBTU), Boc-Lys(Boc)-OH*DCHA and cysteamine were obtained from IRIS Gmbh (Germany). p-Nitrophenyl ester of N-ter-butyloxycarbonyl-tyrosine benzyl ether (Boc-Tyr(Bzl)-ONp) was obtained from Reanal (Hungary). Succinic anhydride and HF gas were obtained from Fluka.


Vesicular stomatitis virus human IFN□ virus (VSV), and Measles virus MV-NIS (MV) were supplied by the Viral Vector production laboratory, Mayo Clinic. Influenza virus (H1N1) A/Puerto Rico/8/1934 (H1N1) human viruses were supplied by Institute of Virology RAS, Moscow. All native and labeled viruses were purified by ultracentrifugation in 20% sucrose. Age-matched (4-6 weeks old) female C57Bl mice (Harlan Sprague Dawley, Indianapolis, Ind.) were housed in a specific pathogen-free facility. All animal studies were approved by, and performed according to guidelines of a bioethics committee.




embedded image




embedded image


Preparation of the Construct Designated FSL-Fluorescein

The construct was prepared according to Scheme I as previously described (Korchagina et al (2008)) (Route 1) or as follows (Route 2):


Preparation of Activated 1,2-O-distereoyl-sn-glycero-3-phosphatidylethanolamine (DSPE) and Activated 1,2-O-dioleoyl-sn-glycero-3-phosphatidylethanolamine (DOPE) (L-A)


To a solution of bis(N-hydroxysuccinimidyl) adipate (A) (70 mg, 205 μmol) in dry N,N-dimethylformamide (1.5 ml) were added DOPE or DSPE (L) (40 μmol) in chloroform (1.5 ml) followed by triethylamine (7 μl). The mixture was kept for 2 h at room temperature, then neutralized with acetic acid and partially concentrated in vacuo.


Column chromatography (Sephadex LH-20, 1:1 chloroform-methanol, 0.2% acetic acid) of the residue yielded the activated lipid (L-A) (37 mg, 95%) as a colorless syrup; TLC (chloroform-methanol-water, 6:3:0.5): Rf=0.5 (DOPE-A), Rf=0.55 (DSPE-A).



1H NMR (CDCl3/CD3OD, 2:1), δ:


DSPE-A—5.39 (m, 1H, —OCH2—CHO—CH2O—), 4.53 (dd, 1H, J=3.42, J=11.98, —CCOOHCH—CHO—CH2O—), 4.33 (dd, 1H, J=6.87, J=11.98, —CCOOHCH—CHO—CH2O—), 4.23 (m, 2H, PO—CH2—CH2—NH2), 4.15 (m, 2H, —CH2—OP), 3.61 (m, 2H, PO—CH2—CH2—NH2), 3.00 (s, 4H, ONSuc), 2.81 (m, 2H, —CH2—CO (Ad), 2.48 (m, 4H, 2×(—CH2—CO), 2.42 (m, 2H, —CH2—CO (Ad), 1.93 (m, 4H, COCH2CH2CH2CH2CO), 1.78 (m, 4H, 2×(COCH2CH2—) 1.43, 1.47 (2 bs, 40H, 20CH2), 1.04 (m, 6H, 2CH3).


DOPE-A—5.5 (m, 4H, 2×(—CH═CH—), 5.39 (m, 1H, —OCH2—CHO—CH2O—), 4.58 (dd, 1H, J=3.67, J=11.98, —CCOOHCH—CH0—CH2O—), 4.34 (dd, 1H, J=6.61, J=11.98, —CCOOHCH—CHO—CH2O—), 4.26 (m, 2H, PO—CH2—CH2—NH2), 4.18 (m, 2H, —CH2—OP), 3.62 (m, 2H, PO—CH2—CH2—NH2), 3.00 (s, 4H, ONSuc), 2.8 (m, 2H, —CH2—CO (Ad), 2.50 (m, 4H, 2×(—CH2—CO), 2.42 (m, 2H, —CH2—CO (Ad), 2.17 (m, 8H, 2×(—CH2—CH═CH—CH2—), 1.93 (m, 4H, COCH2CH2CH2CH2CO), 1.78 (m, 4H, 2×(COCH2CH2—), 1.43, 1.47 (2 bs, 40H, 20CH2), 1.04 (m, 6H, 2CH3).


Condensation of Activated DOPE (L-A) with Cadaverine


To a solution of cadaverine (110 μl, 940 μmol) in dichloromethane (3 mL) a solution of activated DOPE (L-A) (90 mg, 93 μmol) in dichloromethane (CH2Cl2) (0.5 mL) was added. The mixture was kept for 0.5 h at room temperature and then portions of 180 μL of acetic acid were added over the course of 5 minutes. The mixture was concentrated in vacuo and the residue chromatographed (Sephadex LH-20, 1:2 chloroform-methanol) to provide 74 mg (84%) of DOPE-Ad-cadaverine, Rf 0.35 (ethyl acetate-isopropanol-water, 2:3:1)



1H NMR (700 MHz, [D3]CHCl3/[D4]CH3OH 1:1, 30° C.): δ, ppm 5.50 (m, 4H, 2×(—CH═CH—), 5.38 (m, 1H, —OCH2—CHO—CH2O—), 4.59 (dd, 1H, J=6.6, Jgem=11.8, HHC—O—C(O)—), 4.35 (dd, 1H, J=3.2, Jgem≈11.8, HHC—O—C(O)—), 4.14 (m, 2H, —OCH—CH2—O—P—), 4.08 (m, 2H, —P—O—CH2—CH2—NH—), 3.58 and 3.39 (2m, 2×2H, N—CH2—CH2—O—P— and N—CH2—(CH2)3CH2NH2) 3.05 (m, 2H, N—CH2—(CH2)3CH2NH2), 2.48 (m, 4H, 2×(—CH2—CO), 2.39 (m, 4H, COCH2CH2CH2CH2CO), 2.19 (m, 8H, 2×(—CH2—CH═CH—CH2—), 1.8, 1.72, 1.58 (3m, 10H, 2H, 2H, COCH2CH2CH2CH2CO, 2×(COCH2CH2—), and —N—CH2(CH2)3—CH2NH2), 1.42, 1.46 (2 bs, 40H, 20 CH2), 1.05 (m ˜t, J≈47 Hz 6H, 2 CH3).


Condensation of DOPE-Ad-Cadaverine with Fluorescein Isothiocyanate (FITC)


To a solution of fluorescein isothiocyanate (FITC) (16.3 mg, 42 μmol) in DMSO (0.3 mL) a solution of DOPE-Ad-cadaverine (40.2 mg, 42 μmol) in dichloromethane (0.5 mL) and triethylamine (7 μL) were added. The mixture was kept for 2 h at room temperature and then partially concentrated in vacuo. The residue was chromatographed (Sephadex LH-20, 1:2 chloroform-methanol) to provide 8 mg (˜8%) of FSL-fluorescein (triethylamine(Et3N) salt) and about 40 mg of crude FSL-fluorescein. The latter was chromatographed (silica gel, ethyl acetate-isopropanol-water, 6:3:1) to yield 24.3 mg (˜40%) of FSL-fluorescein (sodium (Na) salt). The NMR spectra of the obtained salts of FSL-fluorescein were identical to those of the corresponding salts obtained via Route I.


Preparation of the Construct Designated FSL-Tyrosine (FSL-Tyr)

The construct was prepared according to Scheme II as follows:


Preparation of N-Oxysuccinimide Ester of N-Formyl-Tyrosine

N-formyl-tyrosine (81.2 mg) was dissolved in DMF (1.6 mL) followed by the addition of N-hydroxysuccinimide (60 mg) and dicyclohexylcarbodiimide (80 mg in 0.8 mL DMF). The mixture was stirred for 2.5 h at room temperature and the precipitate of N-dicyclohexylurea filtered off. N-formyl-tyrosine (Rf 0.53), N-formyl-tyrosine N-oxysuccinimide ester (Rf 0.64) (CHCl3/MeOH/AcOH; 40:20:3 (v/v/v)).


Preparation of N-Formyl-Tyrosine-CMG2-Ad-DOPE

The intermediate CMG2-Ad-DOPE was prepared as previously described (Bovin et al (2009)). CMG2-Ad-DOPE (250 mg) was dissolved in 5 mL of water and 3 mL of methanol. A solution of the N-oxysuccinimide ester of N-formyl-tyrosine, 1 mL of DMF and 0.647 mL of 1 M NaHCO3 were then added. The mixture was stirred for 45 min, than acidified with 0.2 mL of AcOH. The solution was evaporated in vacuo to a minimal volume. Following the addition of 200 μL of Py, the residue was separated on an LH-20 column (170 ml) (2-propanol/water; 1:2+0.05 M Py.HOAc. Fractions containing pure product were combined, evaporated and freeze-dried.


The residue (Na1, Py1 salt) was dissolved in 3 mL of water. A 60 μL volume of 8 mM NH3 was then added and the resulting solution freeze-dried. Yield 239 mg (91%). Rf=0.53 (CHCl3/MeOH/water; 3:6:1 (v/v/v)). Brutto formula C91H156N20NaO33P. molecular weight as Na1(NH4)4 salt—2112.3. MALDI TOF mass-spectrum (FLEX-PC, DHB) m/z: 2044 M+Na; 2060 M+K; 2066 M+2Na; 2082 M+Na+K; 2088 M+3Na; 2098 M+2K (FIG. 1). 1H-NMR spectrum, δ ppm (5 mg/ml in CD3OD/D2O 1:2, 303K, 800 MHz): 8.238 (s, 1H, H(CO)N), 7.324 and 6.993 (d, 2×2H, J=8.2 Hz, p-C6H4), 5.507 (m, 4H, 2 CH═CH), 5.453 (m, 1H, OCH2—CH—CH2O), 4.823 (˜t, 1H, J=7.2 Hz, αCH of tyrosine), 4.615 (dd, 1H, J1=12 Hz, J2=2 Hz, OCH2—CH—CHO), 4.442-4.063 (37H, 32H of CMG2, OCH2—CH—CHO and OCH2CH2N), 3.523-3.478 (4H, NCH2CH2N), 3.251 (dd, 1H, Jβ=13.8 Hz, Jα=6.3 Hz, βCH of tyrosine), 3.138 (dd, 1H, Jβ=13.8 Hz, Jα=8.1 Hz, βCH of tyrosine), 2.532-2.453 (m, 8H, 4 C(O)CH2), 2.189 (m, 8H, 2 CH2CH═CHCH2), 1.802 (m, 4H, 2 C(O)CH2CH2 of adipic fr.), 1.771 (m, 4H, 2 C(O)CH2CH2 of DOPE), 1.514, 1.477 and 1.459 (m, 40H, 20 CH2 of DOPE), 1.064 (t, 6H, J=7 Hz, 2 CH3) (FIG. 2).


Preparation of the Constructs Designated FSL-Tyr4 and FSL-Tyr8

The constructs were prepared according to Scheme III as follows:


Solid-Phase Synthesis (SPS) of Multivalent Tyrosine Dendrons

Solid-phase reactions were performed manually in 50, 30 or 20 mL polypropylene (PP) syringes (BD, USA) equipped with PP frit at the bottom and 19 G disposable needle used for connecting Luer outlet to the waste flask via the septum stopper during washing steps. The needle was changed for Luer stopper in the course of coupling and deprotection steps performed with occasional shaking. Volumes of solvents and reagent solutions used for every SPS operation were circa 10 mL/1 g of starting resin initially, the volume gradually increased to accommodate swelling of the peptide resin (PR) due to incorporation of peptide material. By default, during the course of all repeated coupling steps DMAP was introduced 30 to 60 min before the reactions were terminated (10 mol % with respect to resin loading). Completeness of the coupling reactions was monitored by the qualitative ninhydrin reaction (Kaiser et al (1970)). Resin loadings (mmol/g) were calculated on the basis of respective PR weight gain.


Preparation of Boc-NHCH2CH2SCH2-Resin (Resin I) and (Lys)2-Lys-NHCH2CH2SCH2-Resin (PR II) (Scheme III-Part I)


A vigorously stirred slurry of finely grounded cysteamine (1.05 g, 13.6 mmol) in DMF (10 ml) was treated with Boc2O (3.56 g, 16.4 mmol) until starting material completely dissolved (circa 0.5 hrs). (The dissolution may require brief heating at 40 to 50° C.) To the solution of N-Boc-cysteamine obtained diisopropylethylamine (DIEA; 1.5 mL, 7 mmol), NaI (102 mg, 0.7 mmol) and DMF were added to final volume of 60 mL, followed by 10 g (6.8 mmol) of chloromethylated copolymer of styrene; 1% divinylbenzene (0.68 meq of Cl/g; Peptide Institute Inc., Japan). The alkylation reaction was allowed to proceed for 2 hours at room temperature and then at 50° C. overnight. The resin was washed with IPA-DMF (2:1), DMF, IPA-DMF (2:1), DMF, IPA-DMF (2:1), dichloromethane (DCM), IPA-DCM (1:1, v/v), DCM and dried in vacuum to provide 10.96 g Boc-NHCH2CH2SCH2-resin (Resin I) with loading of 0.61 mmol/g estimated from the observed weight gain and 0.03 mmol/g of residual chloromethyl functions quantitated according to the published procedure (Tam (1985)). A 2 g (1.22 mmol) amount of the Resin I was treated with TFA-DCM (1:1, v/v) for 1 min and 25 min, DCM, DMF-IPA (1:2), 2 times [DIEA (5% v/v) in DCM, DMF-IPA (1:2)] followed by solution of Boc-Lys(Boc)-OBt. The latter was prepared by dissolving 0.63 g, (1.2 mmol) of Boc-Lys(Boc)-OH*DCHA in the solution of TBTU (0.35 g, 1.1 mmol) in DMF (5 mL) with sonication. To an essentially clean solution 0.16 g, (1.2 mmol) of HOBt and DMF were added to provide a final volume of 15 mL. Coupling was terminated after 2 hours and the resin was washed with DIEA (5% v/v) in DCM, DMF-IPA (1:2) and the residual amino groups were acetylated with Ac2O-DMF (1:4 v/v) until negative ninhydrin test obtained. The resin was treated twice with TFA-DCM (1:1, v/v) for 1 min and 40 min, DCM, DMF-IPA (1:2), 2 times [5% (v/v) DIEA in DCM, DMF-IPA (1:2)] and coupling carried out for 5 hours with Boc-Lys(Boc)-OBt solution obtained as described above from respective DCHA-salt (1.27 g, 2.4 mmol), TBTU (0.69 g, 2.16 mmol) and HOBt (0.16 g, 1.2 mmol). The resin was washed with 5% (v/v) DIEA in DCM, DMF-IPA (1:2) and coupling was repeated with the fresh solution of Boc-Lys(Boc)-OBt at 50° C. overnight. The resin washed with DMF-IPA (1:2), DCM, DCM-IPA (1:2, v/v)] was treated with TFA-DCM (1:1, v/v) for 1 min and 60 min, DCM, DMF-IPA (1:2), 2 times [5% (v/v) DIEA in DCM, DCM-IPA (1:2)] and dried in vacuum to constant weight; yield 2.81 g of PR II with loading 1.7 mmol NH2/g.


Preparation of [Suc-Tyr (Bzl)]8-Lys)4-(Lys)2-Lys-NHCH2CH2SCH2-Resin (PR III) and (Suc-Tyr)8-(Lys)4-(Lys)2-Lys-NHCH2CH2SH (Tyr8-dendron) (Scheme III-Part 2A)


1 g (1.7 mmol) of dry PR II was treated with oxybenzotriazol ester solution prepared as described above from Boc-Lys(Boc)-OH*DCHA-salt (2.1 g, 3.9 mmol), TBTU (1.12 g, 3.5 mmol) and HOBt (0.24 g, 1.7 mmol) for 6 hours at 50° C. A second coupling was performed with double quantity (7.8 mmol) of the active ester at 50° C. overnight. Ninhydrin negative resin was washed with DCM, DCM-IPA (1:2), deprotected (1 min and 70 min) and neutralized as above. The next coupling was repeated 3 times with a solution of 6.4 g (13 mmol) of Boc-Tyr(Bzl)-ONp (Reanal, Hungary) in 10 mL DMF containing 0.45 g (3.3 mmol) HOBt. The first coupling was performed at room temperature for 5 hours, the second and the third couplings were performed at 50° C. for 6 and 12 hours, respectively. The ninhydrin-negative resin obtained was washed with 2 times [DMF-IPA (1:2), 5% (v/v) DIEA in DCM], DCM, DCM-IPA (1:2), deprotected (1 min and 60 min) and neutralized as above. The final acylation with 1 g (10 mmol) of succinic anhydride (Pierce) in DMF (10 mL) was carried out for 5 hours at room temperature and repeated with fresh reagent at 50° C. for 6 and 12 hours. The PR III was thoroughly washed with DMF-IPA (1:2), DCM, DMF, DCM-IPA (1:2), DCM to remove traces of p-nitrophenol and dried in vacuo; yield 1.52 g. A part of the PR III (1.05 g) was subjected to ‘low-high’ HF cleavage procedure (Tam and Merrifield, (1987)). “Low-HF” procedure details: 12 mL DMS/5 mL HF, 0° C., 2 hrs. Volatiles were removed in vacuum and the solids were washed repeatedly with DCM and EtOAc to ensure that any traces of benzyldimethylsulfonium by-product are removed completely, and dried. “High-HF” cleavage was performed in 10 mL of HF-p-cresol (9:1, v/v) for 2 h at 0° C. After HF removal the residue was triturated with Et2O and washed 3 times [EtOAc, Et2O] (both solvents contained 1% (v/v) of mercaptoethanol) and peptide material was extracted with 3 times 6 mL of DCM-TFE (2:1). The extract was concentrated in vacuum, peptide precipitated with Et2O, centrifuged and re-precipitated two times with Et2O from a minimum volume of DCM-TFE (2:1). Yield—170 mg of Tyre-dendron which was characterized by ESI-MS and NMR and used in the next step without further purification. ESI-MS (Negative mode, 20% MeOH), m/z: 1539.3 [M-2H]2−; 1025.9 [M-3H]3−. Calculated MW 3080.4


Preparation of (Suc-Tyr)8-(Lys)4-(LYS)2-LYS-NHCH2CH2S-Mal-βAla-CMG2-Ad-DOPE (ESL-Tyr8) (Scheme III-Part 3A)

A solution of a (Suc-Tyr)8-(Lys)4-(Lys)2-Lys-NHCH2CH2SH (20.7 mg, 6.2 μmol) in 6 mL 0.1M NMM formate in 30% aqueous isopropyl alcohol (30% IPA) pH 6.6 was combined with 1.2 mL of the same buffer, in which 9.02 mg, 4.5 μmol of Mal-βAla-CMG2-Ad-DOPE (Bovin et al (2009)) were dissolved. The clear solution was kept overnight at room temperature and lyophilized. The residue thus obtained was triturated with IPA (1 mL) and the mixture was sonicated until uniform suspension was obtained (circa 10 min). The slurry was then transferred into an Eppendorf tube and centrifuged. The precipitate was further washed with IPA, re-dissolved in 200 μL 20% IPA, re-precipitated with 1 mL of IPA and washed alternately with EtOH and IPA (2 times 200 μL of each, ultrasonic bath followed by centrifugation). The wet precipitate was dissolved in 2 ml of water and lyophilized; yield 20.2 mg (88%) of amorphous white powder. ESI-MS (Negative mode, 20% IPA), m/z: 1686.6 [M-3H]3−, 1264.7 [14-4H]4−; 1271.4 [M-4H+ Na]4−; Calculated MW 5062.6.


Preparation of (Suc-Tyr)4-(Lys)2-Lys-NHCH2CH2SCH2-Resin (PR IV) and (Suc-Tyr)4-(Lys)2-Lys-NHCH2CH2SH (Tyr4-dendron) (Scheme III-Part 2B)


The title PR IV was assembled on PR II (1 g, 1.7 mmol) via two chain extension steps detailed in the preparation of PR III applying the same molar excesses of activated species with respect to resin. Yield of PR IV—1.39 g. A part of the PR IV (1.11 g) obtained was subjected to ‘low-high’ HF cleavage procedure as specified above for octavalent homologue to yield 117 mg of Tyr4-dendron. ESI-MS (Negative mode, 30% IPA), m/z: 1513.8 [M-H]; 757.5 [M-2H]2− Calculated MW 1514.7


Preparation of (Suc-Tyr)4-(Lys)2-Lys-NHCH2CH2S-Mal-βAla-CMG2-Ad-DOPE (FSL-Tyr4)(Scheme III-Part 3B)

The construct FSL-Tyr4 was obtained according to standard conjugation procedure exemplified for the construct FSL-Tyr8 as described above. Reaction of 15.1 mg (10 μmol) of (Suc-Tyr)4-(Lys)2-Lys-NHCH2CH2SH with 13.23 mg (6.6 μmol) of Mal-βAla-CMG2-Ad-DOPE in 5.5 mL of 30% v/v IPA containing 0.1M NMM formate, pH 6.6 yielded 17.5 mg (76%) of the desired construct FSL-Tyr4. ESI-MS (Negative mode, 30% IPA), m/z: 1746.7 [M-2H]2−; 1164.7 [M-3H]3−, 1172.2 [M-3H+Na]3−; 873.3 [M-4H]4−; 698.6 [M-5H]5−; Calculated MW 3496.9.




embedded image




embedded image


embedded image


embedded image




embedded image


embedded image




embedded image


embedded image




embedded image


embedded image


The following procedures and results are also described and discussed in the publication of Hadac et al (2011).


Iodination of the Construct FSL-Tyr

To oxidatively label the tyrosine residue of the construct we Pierce (Cat. 28601, Thermo Fisher Scientific Inc., Rockford, Ill.) iodination tubes were used. Briefly, a Pierce Iodination tube was wetted with 1 ml Tris-HCl—NaCl buffer (25 mM Tris-HCl pH 7.5, 0.4 M NaCl) and decantanted. In a well vented fume hood, 100 μl Tris-HCl—NaCl buffer followed by 1 mCi Na125I (Cat. NEZ-033A Perkin-Elmer, Cambridge, Mass.) was added and incubated at room temperature for 6 minutes swirling every 30 seconds. The activated Na125I was transferred to a new tube containing the construct designated FSL-tyrosine (0.3 mg/150 μL) and incubated at room temperature for 8 minutes, swirling every 30 seconds. The solution was then transferred into the sample reservoir of a Microcon-10 filter device (Millipore Corporation, Billerica, Mass.) and 250 μL Tris-HCl—NaCl buffer added to the reservoir, sealed and spun in a microcentrifuge in a fume hood for 30 minutes at 13,000 rpm. The flow through (FT1) was collected and 300 μl Tris-HCl—NaCl buffer added to the sample reservoir. The centrifugation was repeated with collection of the flow through (FT2) and retained sample (iodinated(125I) FSL-tyrosine). All fractions were quantified in a dose calibrator and aliquots of the iodinated (125I) FSL-tyrosine stored at −20° C.


Modification of VSV with the Construct Designated FSL-Fluorescein


A volume of 1.25 μL of FSL-fluorescein (20 or 200 μg/ml) to provide a final concentration of 1 and 10 μg/ml was added to 25 μL of VSV (7.8×1010 TCID50 units/mL). The suspension of VSV and FSL-fluorescein were incubated for 2 hours at 37° C. Sample of VSV modified to incorporate the construct (VSV-FSL-FLRO4) and control samples of virus were then fixed with 4% paraformaldehyde on ice for 10 minutes.


Modification of H1N1 with the Construct Designated FSL-Fluorescein


0.5 mg of FSL-fluorescein was dispersed in 50 μL 50 mM NaHCO3, pH 8.3 followed by addition of 450 μL 0.1M PBS. The obtained stock solution was used for preparation of three concentrations; 25, 100, and 200 μg/mL. To modify virus 60 μL of the stock solution was added to an equal volume of virus preparation and incubated at room temperature for 1 h. An excess of FSL-fluorescein was removed using chromatography on Sephadex G-50. Modified virus was stored in 0.1 M PBS containing 0.01% NaN3.


Influenza Virus (H1N1) Infectivity Test

Infectivity of H1N1 was tested on swine testicles cell culture (ST cells). A 24-well plate with cells was washed with 1% BSA in PBS (PBA) followed by infection with 200 μl virus preparation (200 HAU) in PBS. Cells were incubated with virus at 37° C. for 1 h followed by washing two times with PBA. The cell monolayer was treated with trypsin solution and the obtained cell suspension washed with PBA and fixed in 0.1% formaldehyde solution in PBS. Cell fluorescence was measured using a laser flow cytometer DACO Galaxy (Denmark) at 488 nm.


Modification of BV-NIS by FSL-Fluorescein and Subsequent Labelling of KAS6/1 Cells

A volume of 5 μL of FSL-fluorescein (100 μg/ml) was added to 100 μL of MV-NIS (1.5×108 TCID50 units/mL) and incubated for 2 hours at 37° C. to prepare MV-FSL-FLRO4. The suspension was then diluted to 250 μl with PBS. KAS6/1 cells were grown in RPMI 1640 supplemented with heat-inactivated 10% fetal bovine serum, 100 U/mL penicillin, 100 mg/mL streptomycin and interleukin-6 (IL-6, 1 ng/mL). A volume of 140 μL of the MV-FSL-FLRO4 preparation was added to 100 μL of a KAS6/1 cell suspension (4×106/100 μL) in OptiMEM (Invitrogen, Carlsbad Calif.) media and incubated at 37° C. for 1 hour. Following incubation the resultant MV-FSL-FLRO4 labelled KAS6/1 cells were pelleted and washed once (PBS with 1% BSA) by centrifugation and fixed on ice for 10 minutes in 4% paraformadehyde.


Modification of Vero Cells with Iodinated (125I) FSL-Tyr


In 6-well tissue culture plates 5×105 Vero cells maintained in Dulbecco-modified Eagle medium containing 10% fetal bovine serum (American Type Culture Collection, Manassas, Va.) per well were grown to confluence overnight then washed with HBSS 10 mM HEPES pH 7.3 with KOH. A volume of 1 mL of HBSS-HEPES (10 mM HEPES, pH 7.3) was added to a monolayer followed by varying amounts of the iodinated construct or 125I to give 1, 2 or 4×107 cpm per well. After a 2-hour incubation at 37° C. the plate was placed on ice, the supernatant aspirated, and the monolayer washed with 1 ml of iced HBSS buffer. Cells were lysed with 1 ml of 1M NaOH and each lysate transferred to a test tube for quantitation of radioactivity.


Monitoring Distribution In Vivo

To determine the distribution of labelled virus in mice 200 μl of VSV-hIFNβ (5.8×1010)was added to 150 pCi of iodinated (125I) FSL-tyrosine and incubated for 4 hours at room temperature. Syringes were then loaded each with a total of 50 pCi of labelled virus (VSV-FSL-125I). Control syringes were also loaded each with 50 pCi, two with Na125I and two with iodinated (125I) FSL-tyrosine (FSL-125I). Each of seven mice were injected IP with one of the 125I reagents. Prior to imaging mice were anesthetized with inhalation of isoflurane and imaged 1 hour post sample injection using micro-SPECT/CT system (X-SPECT, Gamma Medica Ideas) and image analysis using PMOD software (PMOD Biomedical Image Quantification and Kinetic Modeling Software, PMOD Technologies Zurich, Switzerland). One mouse from each sample group underwent additional imaging at 4 and 24 hour time-points. After each final imaging point the mouse was sacrificed, dissected and radioactivity in organs was quantified in a dose calibrator.


FACScan Flow Cytometry

Samples were analyzed by FACScan flow cytometry and Cell Quest Pro software (BD Biosciences, San Jose, Calif.).


Quantitation of Radioactivity

Radioactivity was quantitated with an Isodata-10 gamma spectrometer (Polymedio, Yorktown Heights, N.Y.) and radioisotope calibrator (model CRC-5R, Capintec, Inc. Ramsey, N.J.).


Results

The iodinated (125I) form of the construct designated FSL-tyrosine (FSL-125I) had the spontaneous and controlled membrane insertion character of other FSL constructs. Its ability to label Vero cells has been investigated and contrasted with direct 125I labelling. It has been shown that at equivalent radioactive counts, FSL-125I was about 10-fold more effective at labelling cells than 125I and the labelling occurred in a concentration dependent manner (FIG. 4). A comparison of 125I and FSL-125I labelling of MV and VSV, and subsequent sucrose gradient purification (FIG. 5) showed that more FSL-125I labelled virions than 125I labelled virions, could be isolated in the sucrose fraction, compared with the buffer, where the unbound label is predominantly found (FIG. 6).


VSV was determined to be labelled with FSL-FLRO4 in a manner similar to cells (Blake et al (2010)) by contacting VSV with the FSL-FLRO4 to create modified virus (VSV-FSL-FLRO4) and analysing by FACScan (FIG. 7(a)). By simply increasing the concentration of FSL construct, the intensity of modified virions increased (FIG. 7(a)). Similarly, H1N1 modified with FSL-FLRO4 showed a concentration dependent modification (FIG. 7(b)). For comparison H1N1 was labelled by the conventional direct FITC method (Yoshimura and Ohnishi (1984)) which gave about 9-times greater total fluorescence than H1N1 modified with 25 μg/ml FSL-FLRO4 (FIG. 7(b)). However, when these labelled and modified H1N1 virions were allowed to infect ST cells, essentially the same level of fluorescence was seen for 25 μg/ml FSL-FLRO4 modified as with direct FITC-labeled H1N1 (FIG. 7(c)). This result, starting with the 9-times more fluorescence of direct FITC labelled H1N1 yet obtaining only equivalent fluorescence with the 25 μg/ml FSL-FLRO4 modified H1N1 post infection of MDCK cells, can be interpreted to mean that 9-times less FITC labelled virions infected the MDCK cells. Thus, the FSL-FLRO4 labelled virions appears to conserve infective potency better than FITC-labelled virions, perhaps, due to the non-covalent nature of the modification. When a higher concentration FSL-FLRO4 construct modified H1N1 was used to infect MDCK cells (e.g. 100 and 200 μg/ml) increased fluorescent intensity was obtained (FIG. 7(b)).


MV was modified with FSL-FLRO4 (MV-FSL-FLRO4) and then allowed to react with a KAS6/1 cell line suspension (FIG. 7(d)). These results, like those for H1N1 (FIG. 7(c)) show that the modified viruses retain their ability to bind to cells, and become detectable by flow cytometry. The additional small peak seen with KAS6/1-MV-FSL-FLRO4 cells (FIG. 7(d)) is probably due to dead cells, as unbound virus was excluded by gating.


Following peritoneal infusion we compared the distribution in vivo of 125I and FSL-125I construct with that of VSV-FSL-125I (FIG. 8). Radioactive iodine has a very well described distribution in vivo (Hammond et al (2007)) to thyroid, salivary glands, stomach and bladder and the 125I results were concordant with the literature. Within 1 hour post administration to the peritoneal cavity labelled virions (VSV-FSL-125I), in contrast to 125I and FSL-125I, localized to liver, spleen and bloodstream—with some signal also retained in the peritoneal cavity (FIGS. 8(a) and 8(b)). Intravenously administered VSV-FSL-125I localized similarly, but without the strong peritoneal signal (not shown). FSL-125I alone followed a similar distribution to labelled virus, but was significantly different to free 125I, which rapidly distributed to the stomach and then to the thyroid (FIG. 8(a)). Due to the variable nature of urine collection bladder quantitation was not considered. At 4-hours post infusion the distribution (FIG. 8(a)) had not changed significantly from the 1 hour time point although more systemic spread had occurred. At 24 hours (FIGS. 8(a) and 8(c)) both 125I and FSL-125I injected animals gave essentially only thyroid distribution while the VSV-FSL-125I injected animals had a distribution equivalent to the 1 hour distribution of 125I. The accumulation of radioactive iodine in the thyroid from both VSV-FSL-1251 and FSL-125I is not surprising and suggests that degradation of the FSL-125I had occurred releasing free iodide, which then was concentrated in the thyroid gland.


Although the invention has been described with reference to embodiments or examples it should be appreciated that variations and modifications may be made to these embodiments or examples without departing from the scope of the invention. Where known equivalents exist to specific features, such equivalents are incorporated as if specifically referred to in this specification. In particular the substitution of the less favoured particle emitting radioisotope 131I for 125I in any of the claimed methods is recognised to be within the scope of the invention.


REFERENCES



  • Barr et al (2010) Function-Spacer-Lipid (FSL) constructs enable inkjet printing of blood group antigens FEBS J, Vol 277 (S1), 235.

  • Blake et al (2003) Embryo modification and implantation international application no. PCT/NZ03/00059 (publ. no. WO 03/087346).

  • Blake et al (2010) Fluorophore-kodecytes-fluorescent function-spacer-lipid (FSL) modified cells for in vitro and in vivo analyses FEES J, Vol 277 (S1), 199.

  • Bovin et al (2009) Functional lipid constructs international application no. PCT/NZ2008/000266 (publ. no. WO 2009/048343).

  • Campos et al (2004) Avidin-based targeting and purification of a protein IX-modified, metabolically biotinylated adenoviral vector Mol Ther, Vol 9, 942-954.

  • Chesla et al (2010) Solid phase syphilis test utilizing KODE technology Transfusion, Vol 50 (S1), 196A-197A.

  • Frame et al (2007) Synthetic glycolipid modification of red blood cell membranes Transfusion, Vol 47, 876-882.

  • Hadac et al (2011) Fluorescein and radiolabelled function-spacer-lipid constructs allow for simple in vitro and in vivo bioimaging of enveloped virions J. Virological Methods, 176, 78-84.

  • Hammond et al (2007) A gama camera re-evaluation of potassium iodide blocking efficiency in mice Health Phys, Vol. 92, 396-406.

  • Harrison et al (2010) A synthetic globotriaosylceramide analogue inhibits HIV-1 infection in vitro by two mechanisms Glycobiology, Vol 27, 515-524.

  • Heathcote et al (2010) Novel antibody screening cells, MUT+Mur kodecytes, created by attaching peptides onto erythrocytes Transfusion, Vol 50, 635-641.

  • Henry (2009) Modification of red blood cells for laboratory quality control use Curr Opin Hematol, Vol 16, 467-472.

  • Hermanson (2008) Bioconjugation Techniques, 2nd ed., Academic Press.

  • Herschman (2003) Molecular imaging: Looking at problems, seeing solutions Science, Vol 302, 605-608.

  • Kaiser et al (1970) Anal. Biochem., 34(2), 595-8.

  • Korchagina et al (2008) Fluorescent cell markers international PCT application no. PCT/NZ2007/000256 (publ. no. WO 2008/030115).

  • Kuruppu and Tanabe (2005) Viral oncolysis by herpes simplex virus and other viruses Cancer Biol Ther, Vol 4, 524-531.

  • Lui et al (2007) Clinical trial results with oncolytic virotherapy: a century of promise, a decade of progress Nat Rev Clin Oncol, Vol 4, 101-117.

  • Oliver et al (2011) Modeling transfusion reactions and predicting in vivo cell survival with kodecytes Transfusion; (in press).

  • Peng et al (2003) Hum Gene Ther, Vol, 14, 1565-1577.

  • Piwnica-Worms et al (2004) Molecular imaging of host-pathogen interactions in intact small animals Cell Microbiol, Vol 6, 319-331.

  • Räty et al (2006) Magnetic resonance imaging of viral particle biodistribution in vivo Gene Ther, Vol 13, 1440-1446.

  • Stokke et al (1974) Lipid composition and cholesterol esterification in lymph Scand J Clin Lab Invest, Vol 33, 199-206.

  • Strable and Finn (2009) Chemical modification of viruses and virus-like particles Curr Top Microbiol Immunol, Vol 327, 1-21.

  • Tam (1985) A gradative deprotection strategy for the solid phase synthesis of peptide amides using p-(acyloxy)benzhydrylamine resin and the SN2 deprotection method J. Org. Chem., 50, 5291-5298.

  • Tam and Merrifield (1987) Strong acid deprotection of the synthetic peptides: mechanisms and methods Udenfriend, S., Meienhofer, J., (Eds), The Peptides: Analysis, Synthesis, Biology, Vol. 9, Academic Press, New York, pp 185-248.

  • Waehler et al (2007) Engineering targeted viral vectors for gene therapy Nat Rev Genet, Vol 8, 573-587.

  • Yamamoto and Curiel (2010) Current issues and future directions of oncolytic adenoviruses Mol Ther, Vol 18, 243-250.

  • Yoshimura and Ohnishi (1984) Uncoating of influenza virus in endosomes J Virol, Vol 51, 497-504.


Claims
  • 1-14. (canceled)
  • 15. A non-invasive method of monitoring by radioactivity bioscanning the distribution of a biological entity in a subject in vivo comprising the step of administering to the subject a radioiodinated biological entity prepared by contacting an aqueous suspension of the biological entity with a radioiodinated construct of the structure F-S-L where F comprises a radioiodinated histidine residue or a radioiodinated tyrosine residue, S is selected to provide a construct that is readily dispersible in water, and L is phosphatidylethanolamine.
  • 16. The method of claim 14 where the construct is of the structure:
  • 17. The method of claim 16 where the biological entity is a cell or an enveloped virus.
  • 18. The method of claim 17 where the biological entity is administered to the subject by injection.
  • 19. The method of claim 18 where F comprises a radioiodinated tyrosine residue.
  • 20. The method of claim 19 where the tyrosine residue is:
  • 21. The method of claim 20 where L is 1,2-O-dioleoyl-sn-glycero-3-phosphatidylethanolamine (DOPE).
  • 22. The method of claim 21 where the construct is of the structure:
  • 23. The method of claim 21 where the construct is of the structure:
  • 24. The method of claim 19 where construct is of the structure N-formyl-(Tyr)n-S-L where n is an integer from 1 to 6 inclusive.
  • 25. The method of claim 24 where n is 1 and the construct is of the structure:
Priority Claims (1)
Number Date Country Kind
591047 Feb 2011 NZ national
PCT Information
Filing Document Filing Date Country Kind 371c Date
PCT/NZ12/00012 2/9/2012 WO 00 10/16/2013