Andrea J North1, John A Karas1, Michelle T Ma2, Philip J Blower2, Uwe Ackermann3, Jonathan M White1, Paul S Donnelly1. 1. The School of Chemistry and Bio21 Molecular Science and Biotechnology Institute, University of Melbourne , 3010, Victorria, Australia. 2. Division of Imaging Sciences and Biomedical Engineering, King's College London , Fourth Floor Lambeth Wing, St Thomas' Hospital, London SE1 7EH, U.K. 3. Department of Molecular Imaging and Therapy, Department of Medicine, University of Melbourne , Austin Health, Studley Road, Heidelberg, Victoria 3010, Australia.
Abstract
This research aimed to develop new tumor targeted theranostic agents taking advantage of the similarities in coordination chemistry between technetium and rhenium. A γ-emitting radioactive isotope of technetium is commonly used in diagnostic imaging, and there are two β- emitting radioactive isotopes of rhenium that have the potential to be of use in radiotherapy. Variants of the 6-hydrazinonicotinamide (HYNIC) bifunctional ligands have been prepared by appending thioamide functional groups to 6-hydrazinonicotinamide to form pyridylthiosemicarbazide ligands (SHYNIC). The new bidentate ligands were conjugated to the tumor targeting peptides Tyr3-octreotate and cyclic-RGD. The new ligands and conjugates were used to prepare well-defined {M═O}3+ complexes (where M = 99mTc or natRe or 188Re) that feature two targeting peptides attached to the single metal ion. These new SHYNIC ligands are capable of forming well-defined rhenium and technetium complexes and offer the possibility of using the 99mTc imaging and 188/186Re therapeutic matched pairs.
This research aimed to develop new tumor targeted theranostic agents taking advantage of the similarities in coordination chemistry between technetium and rhenium. A γ-emitting radioactive isotope of technetium is commonly used in diagnostic imaging, and there are two β- emitting radioactive isotopes of rhenium that have the potential to be of use in radiotherapy. Variants of the 6-hydrazinonicotinamide (HYNIC) bifunctional ligands have been prepared by appending thioamide functional groups to 6-hydrazinonicotinamide to form pyridylthiosemicarbazide ligands (SHYNIC). The new bidentate ligands were conjugated to the tumor targeting peptides Tyr3-octreotate and cyclic-RGD. The new ligands and conjugates were used to prepare well-defined {M═O}3+ complexes (where M = 99mTc or natRe or 188Re) that feature two targeting peptides attached to the single metal ion. These new SHYNIC ligands are capable of forming well-defined rhenium and technetium complexes and offer the possibility of using the 99mTc imaging and 188/186Re therapeutic matched pairs.
The technetium-99m
isotope has excellent properties for detection with single photon
emission computed tomography (SPECT) due to its low energy and nonparticulate
gamma-ray emission (t1/2 = 6.01 h, Emax = 141 keV γ-ray emission, λ
< 10 pm). Despite recent concerns over production related shortages
of technetium-99m and the advent of positron emission tomography technetium-99m
retains its importance to nuclear medicine to the extent that the
isotope is used in over 80% of nuclear imaging procedures worldwide.[1] The heavier third row Group VII congener, rhenium,
has an ionic radius similar to technetium due to the lanthanide contraction.
Technetium and rhenium display similar coordination chemistry often
resulting in essentially isostructural technetium and rhenium complexes.
It is common for technetium and rhenium complexes to be essentially
isostructural. There are two isotopes of rhenium that are of potential
use in targeted radiotherapeutics, rhenium-186 (t1/2 = 89.3 h, Emax = 1.07
MeV β– particle emission, 137 keV γ-ray
emission) and rhenium-188 ((t1/2 = 16.9
h, Emax = 2.12 MeV β– particle emission, 155 keV γ-ray emission). The similar coordination
chemistry of technetium and rhenium offers the possibility of using
their radioisotopes as an imaging (99mTc) and therapeutic
(186/188Re) matched pair using a single targeted ligand
to form essentially isostructural complexes.[2−6]One approach to targeted imaging and therapy
is to incorporate appropriate metalradionuclides into coordination
complexes that are attached to biological targeting vectors such as
tumor targeting peptides, antibodies or antibody fragments. Peptides
that feature the −RGD- (arginine-glycine-aspartic acid) fibronectin
fragment such as the cyclic-RGDfK pentapeptide (cRGDfK) bind to αvβ3 integrin receptors that are overexpressed
in certain invasive tumors including osteosarcomas, glioblastoma,
melanomas, and breast cancer, and can be used to selectively target
tumor cells.[7−16] Metabolically stabilized somatostatin analogues such as octreotide
and octreotatebind to somatostatin subtype 2 receptors (sstr2) that
are overexpressed in many types of neuroendocrine tumors compared
to relatively low levels of expression in other tissues and organs.[17−21]Tumor targeting technetium based imaging agents can be prepared
using 6-hydrazinonicotinamide (HYNIC) derivatives conjugated to targeting
molecules as ligands to form technetium(III) diazenido complexes.[22−31] The HYNIC ligand forms remarkably stable technetium complexes, and
manipulation of the carboxylate functional group to attach a variety
of targeting molecules is generally straightforward. HYNIC binds to
technetiumthrough the terminal hydrazinenitrogen but probably forms
bidentate complexes through coordination to the pyridyl nitrogen.[29,32] In all the crystallographically characterized technetium and rhenium
complexes with one or more HYNIC-like ligands, such as 2-hydrazinopyridine,
the pyridyl nitrogen is also coordinated to the metal center.[33] A variety of coligands such as tricine, nicotinic
acid, EDDA, and phosphines (TPPTS, TPPDS, TPPMS = tri/bi/sodium triphenylphosphinetri/di/monosulfonate) are required to complete the coordination sphere
and stabilize the metal oxidation state, and this leads to a high
degree of uncertainty in the exact nature of the primary coordination
sphere as well as challenges in ensuring structural homogeneity in
the formulated product. Variation of the coligand can modify the in
vivo metabolism and excretion.[34] A well-established
“ternary ligand system” involves combining the HYNIC
ligand with tetradentate tricine and monodentate trisodium 3,3′,3″-phosphanetriyltris(benzenesulfonate)
(TPPTS) coligands, but the possibility of forming multiple isomers
adds complications.[33,35−39]Despite the superficial similarities in coordination
chemistry between technetium and rhenium extrapolation of the HYNIC
strategy to radioactive rhenium isotopes is challenging presumably
due to their differences in kinetic lability and redox chemistry.[33] Some of the difficulty in isolating pure Re-HYNIC-peptide
conjugates can be understood by considering the reaction of [ReO4]− with 2-hydrazinopyridine (used as model
for HYNIC).[33,40] This reaction results in relatively
complex coordination chemistry due to the ability of the pyridylhydrazine
derived ligands to coordinate as either monodentate or bidentate ligands
and the existence of protic equilibria as well as the formation of
complexes where two pyridylhydrazine derived units are coordinated
to the rhenium (Figure ).[26,33,40−43]
Figure 1
(a)
6-Hydrazinonicotinic acid. (b) Metal complex (M = Tc or Re) with 6-hydrazinonicotinimide
(HYNIC) acting as a monodentate ligand. It is necessary to complete
the coordination sphere with coligands (L). (c) Metal complex (M =
Tc or Re) with 6-hydrazinonicotinimide (HYNIC) acting as a bidentate
ligand. (d) Pyridylphenylthiocarbazide (SHYNIC) ligand. (e) ReV-oxo complex featuring two SHYNIC ligands.[44]
(a)
6-Hydrazinonicotinic acid. (b) Metal complex (M = Tc or Re) with 6-hydrazinonicotinimide
(HYNIC) acting as a monodentate ligand. It is necessary to complete
the coordination sphere with coligands (L). (c) Metal complex (M =
Tc or Re) with 6-hydrazinonicotinimide (HYNIC) acting as a bidentate
ligand. (d) Pyridylphenylthiocarbazide (SHYNIC) ligand. (e) ReV-oxo complex featuring two SHYNIC ligands.[44]Modification of the terminal hydrazinic
nitrogen of hydrazinopyridine to incorporate an additional thiourea
functional group results in a ligand system that is capable of forming
well-defined, very stable complexes with {ReVO}3+ cores while retaining the bioconjugation possibilities well established
for HYNIC.[44,45] A preliminary communication reported the structural
characterization of a ReV-oxo complex featuring two pyridylphenylthiocarbazide
(SHYNIC) ligands (Figure ).[44] In this manuscript
we extend this concept by synthesizing a family of different substituted
pyridylthiosemicarbazide ligands with carboxylate or ester functional
groups that were used to tether octreotate and cyclic-RGD peptides
to the ligands. The new ligands were used to prepare {MO}3+ complexes (where M = Tc or Re) that feature two targeting peptides
attached to the single metal ion. These modified HYNIC ligands are
capable of forming well-defined rhenium and technetium complexes and
offer the possibility of using the two radionuclides as imaging and
therapeutic matched pairs.
Results and Discussion
Synthesis
of H2L, and Their Ester Derivatives, H2L(OMe) and {ReO}3+ Complexes
Synthesis of 6-hydrazinonictonic acid (HYNIC), 2, required treatment of 6-chloronicotinic acid (1) with aqueous hydrazine.[47] Ligands H2L to H2L were prepared by reaction of either
the ethyl, tert-butyl, phenyl, or nitrophenyl isothiocyanate
with 6-hydrazinonictonic acid (1) in anhydrous N,N-dimethylacetamide (DMA) (Scheme ).
Scheme 1
Synthesis of Ligands
H2L–H2L and Their Methyl Ester
Derivatives H2L(OMe)–H2L(OMe)
The rhenium complexes of the methyl ester derivatives
of H2L complexes, [ReO(HL(OMe))2]+, can be prepared by
reaction of the either trans-[ReOCl3(PPh3)2] or [tBu4N][ReOCl4] with the two equivalents of ligand (Scheme ). The IR spectra for the three complexes,
[ReO(H2L(OMe))2]+, display medium intensity bands
at ν̅ 960–963 cm–1 characteristic
of Re=O stretches.[48] Bands, which
occur between ν̅ 1553 and 1557 cm–1 due
to carbonyl stretching of the ester functional group, shift approximately
150 cm–1 lower in energy when compared to the metal-free
ligands.
Scheme 2
Synthesis of Rhenium Complexes [ReO(HL)(OMe))2]+
Analysis of the complexes by 1H NMR data reveals that the two coordinated ligands are magnetically
equivalent, with three resonances at δ 8.63, 8.25, and 7.86
ppm corresponding to the six pyridinyl CH protons
for [ReO(HL(OMe))2]+, and similar resonances for the phenyl and tert-butyl derivatives. The pyridine proton which is closest
to the rhenium ion shifts from δ 6.55 ppm in free ligand to
δ 7.86 ppm in the complex. The methyl ester functional group
gives rise to singlets at δ 3.89 (DMSO-d6), 3.86 (CHCl3-d), and 3.92 (DMSO-d6) for complexes [ReO((HL)(OMe))2]+ respectively.
The [ReO(HL(OMe))2]+ complex was stable to cysteine and histidine challenge
experiments with very little decomposition evident (<5%), as detected
by analysis by HPLC and UV/vis spectroscopy, when incubated at 37
°C for 24 h in the presence of a 100-fold excess of cysteine
and histidine.Red crystals of [ReO(HL(OMe))2]CF3CO2 suitable for X-ray crystallographic analysis were obtained by evaporation
of a solution of the compound that had been purified by semipreparative
HPLC using an aqueous/CH3CN mobile phase with 0.1% trifluoracetic
acid (Figure a). The
compound crystallizes in the triclinic space group, P1̅, and the rhenium ion is in a distorted square pyramidal
environment with the oxo group in the apical position relative to
the pseudo basal plane of two five-membered chelate rings. Each thiocarbahydrazide
functional group is doubly deprotonated and serves as a dianionic
ligand fragment and a N,N/S,S trans configuration about the Re-oxo. The selective formation
of the N,N/S,Strans geometric isomer presumably reflects
a strong “trans effect”, although steric
requirements may also play some role.[49−51] Protonation of the pyridyl
nitrogen atom in each ligand results in each ligand having a single
negative charge and resulting an overall monocationic complex. The
two pyridinium protons and the hydrogen atoms of the ethylamino functional
group are involved in hydrogen bonds interactions leading to a hydrogen
bonded centrosymmetric dimer (Figure b) with the two remaining H-bond donors capped by water
molecules.
Figure 2
(a) ORTEP representation of [ReO(HL(OMe))2]+ (50% probability ellipsoids).
The trifluoroacetate counterion and hydrogen atoms (except those bound
to nitrogen) are omitted. (b) Representation of hydrogen bonded centrosymmetric
dimer with the two remaining H-bond donors capped by water molecules.
(a) ORTEP representation of [ReO(HL(OMe))2]+ (50% probability ellipsoids).
The trifluoroacetate counterion and hydrogen atoms (except those bound
to nitrogen) are omitted. (b) Representation of hydrogen bonded centrosymmetric
dimer with the two remaining H-bond donors capped by water molecules.The Re–O1 bond distance
(1.679(3) Å) is typical for five-coordinate, rhenium(V)-monooxo
complexes and consistent with IR spectroscopy (Re=O, ν̅
963 cm–1).[52−55] The N2–C6 and N6–C14 bond lengths (1.287(6)
Å) are significantly shorter than the other bonds within the
chelate ring suggesting significant sp2 hybridized C=N
bond character. The Re–N bond distances average 2.05 Å
and are marginally shorter than typical Re–N bonds (ca. 2.15–2.18
Å) suggesting some degree of multiple bond character.[51,56] The Re–N1–N2 and Re–N5–N6 bond angles
average 124°, suggesting an approximately sp2 hybridized
nitrogen. The Re–S bond distances average 2.29 Å and are
similar to the Re–S bond distances in rhenium(V) complexes
with amino thiolate ligands and Re–S bond distances in rhenium
complexes with thiosemicarbazonato ligands.[51,57,58]Trifluoroacetate
counterion bond lengths and angles are not provided.Crystals were grown from a concentrated
solution of the complex in methanol.The potential of the substituted pyridylthiosemicarbazide
(SHYNIC) ligands H2L to be modified with amino acids using standard solid
phase peptide synthesis techniques was first accomplished by attaching l-lysine to H2L to give H2L(Lys).
The doubly N-protected lysine derivative, Nα-tBoc-Nε-Fmoc-l-Lys, was immobilized on chlorotrityl resin, and the Nε-Fmoc group was removed by treatment with piperidine.
The ligand, H2L,
was added to the resin in a mixture of DMF followed by the coupling
agent HATU (HATU = 1-[bis(dimethylamino)methylene]-1H-1,2,3-triazolo[4,5-b]pyridinium-3-oxid hexafluorophosphate) in the
presence of N,N-diisopropylethylamine
(DIPEA). The product was cleaved from the resin using trifluoroacetic
acid that also resulted in the deprotection of the Nα-t-butoxycarbonyl group (Scheme ). This lysine amino acid conjugate provides
an amino acid with an appended chelator, which with appropriate protecting
groups, could be incorporated into biological targeting molecules
with total site specificity via solid-phase peptide synthesis.[59−63]
Scheme 3
“On-Resin” Formation of H2L(Lys) and the Corresponding Rhenium-oxo
Complex, [ReO(HL(Lys))2]+
The rhenium complex,
[ReO(HL(Lys))2]+, was prepared by adding either trans-[ReOCl3(PPh3)2] or [tBuN][ReOCl4] suspended in DMF to the reaction mixture, while the ligand
remained immobilized on the resin. Performing the complexation while
the ligand remained immobilized on the resin and with the amino group
still protected ensured that the functional groups of the lysine did
not complicate the coordination chemistry. When green trans-[ReOCl3(PPh3)2] is used as the
starting material the green colored suspension gradually changes to
colorless, and the resin beads turn dark red indicative of the formation
of [ReO(HL(Lys))2]+. After being stirred at room temperature, the resin
was washed with dimethylformamide and dichloromethane and cleaved
off the resin with a 10% trifluoroacetic acid/dichloromethane mixture
(Scheme ). Analysis
of [ReO(HL(Lys))2]+ complex by electrospray ionization mass spectrometry
(ESI-MS) reveals the expected peaks. Analysis by 1H NMR
shows the singlet attributed to the aromatic proton on the pyridine
ring (pyH2) shifts upon coordination to
the metal center from δ 8.48 in H2L(Lys) to 8.58 ppm in [ReO(HL(Lys))2]+. The four downfield 13C{1H} NMR signals in [ReO(HL(Lys))2]+, 173.0 (CO2H),
169.0 (N=CS), 165.4 (CONH), and 163.6 (pyC6), were assigned using HSQC and HMBC techniques.
Synthesis
of Peptide-Conjugated Ligands, H2L(cRGDfK) and H2L(Tyr3-Octreotate), and Corresponding Rhenium Complexes [ReO((HL)(cRGDfK))2] and [ReO((HL)(Tyr3-Octreotate))2]
The cyclic
pentapeptide, cRGDfK, was prepared using standard solid phase peptide
synthesis techniques with Fmoc (Fmoc = 9-fluorenylmethyloxycarbonyl)
protected amino acids, using HATU/DIPEA coupling methodology on chlorotrityl
resin. The Fmoc protecting groups were removed with 20% piperidine
in DMF on the solid phase, followed by cleavage from the resin and
cyclization using a small modification of published procedures.[64] The ligands, H2L, were conjugated to cRGDfK
using standard peptide coupling conditions (HATU, DIPEA) to give H2L(cRGDfK) (Scheme ). The new conjugates were purified by semipreparative RP-HPLC and
characterized by electrospray mass spectrometry and analytical HPLC.
The reaction for the ethyl-SHYNIC derivative, H2L(cRGDfK), resulted in a higher isolated
yield (80%) than H2L(cRGDfK) (24%) and H2L(cRGDfK) (55%). Analysis of aqueous solutions of H2L(cRGDfK)
by RP-HPLC revealed no degradation over a 24 h.
Scheme 4
Synthesis of H2L(cRGDfK) and
[ReO(HL(cRGDfK))2]+
The {ReO}3+ complexes of H2L(cRGDfK) were
prepared by adding [ReOCl4]− in DMF at
ambient temperature followed by isolation and purification using semipreparative
RP-HPLC (Scheme ).
Analysis of the complexes by ESI-MS revealed the 2+ molecular ion
peaks at m/z 926.343, 954.372, and
974.371 for [ReO(HL(cRGDfK))2]+, [ReO(HL(cRGDfK))2]+, and [ReO(HL(cRGDfK))2]+ respectively.An intramolecular disulfide bridge between the
second and seventh cysteine residues in Tyr3-octreotate
improves the metabolic stability of the peptide, and this disulfide
is often introduced by oxidation of the linear octapeptide with 2,2′-dithiodipyridine.
Unfortunately the bioconjugation of ligands H2L to Tyr3-octreotate was complicated by degradation of the pyridylthiocarbazide
(SHYNIC) ligands (H2L) in the presence of the two cysteine thiol containing
residues in the linear peptide, leading to loss of H2S
identified in the ESI-MS by a loss of 34 atomic mass units. This loss
of H2S from the ligand was most prominent during reactions
attempting intramolecular oxidation of thiol groups in the two cysteine
residues. The loss of H2S results in the formation of a
carbodiimide form of the SHYNIC ligands. The formation of carbodiimides
from thioureas is well-known.[65] This degradation
and loss of sulfur were not observed for RGD-based conjugates, suggesting
that in the case of the octreotate conjugates, thiocarbazide-thiol-disulfide interchange/scrambling promotes the loss
of H2S from the ligands (Scheme ).
Scheme 5
Suggested Mechanism for the Formation
of a Carbodiimide from H2L(Tyr3-Oct) Resulting in Loss of H2S
As conventional off-resin oxidative
cyclization methodologies were inadequate for this synthesis, H2L(Tyr3-Oct) was prepared entirely on solid support, where
intramolecular oxidation/cyclization preceded bioconjugation of H2L. The eight-residue peptide was synthesized by sequential addition
of the amino acid residues via solid-phase peptide synthesis, using
acetamidomethyl (Acm) protected cysteine residues followed by in situ
Acm removal and simultaneous disulfide bond formation using thallium(III)
trifluoroacetate.[66] Following cyclization,
the preactivated SHYNIC derivative (H2L) is reacted at the deprotected d-phenylalanine N-terminus. Cleavage and deprotection of remaining
protecting groups are achieved by treatment with trifluoracetic acid
(Scheme ).
Scheme 6
Reaction
Scheme for the Formation of Octreotate-Derived Ligands H2L(Tyr3-Oct)
and Corresponding Complexes, [ReO(HL(Tyr3-Oct))2]+
The rhenium complexes of H2L(Tyr3-Oct) could be prepared on-resin or in-solution by treatment with
[tBu4N][ReOCl4] in methanol
(Scheme ). The on-resin
approach is potentially of interest in producing radioactive complexes
in high specific activity as unreacted [ReO4]− and other impurities such as colloidal rhenium could be readily
removed by filtration of the resin. The pure complex can be cleaved
from the resin with 50% trifluoracetic acid and is stable to this
relatively high concentration of acid. Analysis by HPLC and ESI-MS
confirmed the identity of the complexes, with the [ReO(HL(Tyr3-Oct))2]+ complexes showing signals in the ESI-MS that
could be attributed to the 3+ molecular ion with expected rhenium
isotope peak patterns (Figure ).
Figure 3
RP-HPLC chromatogram (UV absorbance, a.u., λ 254 nm) of Tyr3-octreotate rhenium complexes, [ReO(HL(Tyr3-Oct))2]+. Inset: Positive ion ESI-MS data of major isotope peaks
corresponding to each complex as the tripositive cation, [ReO(HL(Tyr3-Oct))2]3+.
RP-HPLC chromatogram (UV absorbance, a.u., λ 254 nm) of Tyr3-octreotaterhenium complexes, [ReO(HL(Tyr3-Oct))2]+. Inset: Positive ion ESI-MS data of major isotope peaks
corresponding to each complex as the tripositive cation, [ReO(HL(Tyr3-Oct))2]3+.
Preparation of [188Re(HL (Tyr3-Oct))2]+
Preliminary
radiolabeling of H2L(Tyr3-Oct) with radioactive 188Re was performed
using generator-produced [188ReO4]−. A solution of [188ReO4]−, in an aqueous mixture of sodium chloride (0.9% w/v concentration)
and sodium tartrate, was reduced with stannous chloride. This mixture
was then reacted with H2L(Tyr3-Oct) at 100 °C, leading to the formation
of [188ReO(HL(Tyr3-Oct))2]+ in ca. 67% radiochemical yield.
The compound was characterized by analytical reversed phased HPLC
(Figure ), where [188ReO(HL(Tyr3-Oct))2]+ (retention time = 11.6 min, detected
using a NaI(Tl)) elutes with a similar retention time to the nonradioactive
analogue [natReO(HL(Tyr3-Oct))2]+ (retention time =
11.3 min, detected at λ220), where natRe refers to naturally abundant Re isotopes. The small difference
in retention times is due to the different configurations of the radioactivity
and UV detectors. This elution profile of [ReO(HL(Tyr3-Oct))2]+ is distinct from that of the free ligand, H2L(Tyr3-Oct) that elutes at 9.7
min under the same conditions. Unreacted 188Re species,
presumably [188ReO4]−, elute
with the solvent front at 2.1 min (Figure ).
Figure 4
RP-HPLC chromatogram (UV absorbance, λ
224 nm and radiation detection) of [188/natReO(HL(Tyr3-Oct))2]+ and free ligand H2L(Tyr3-Oct). The signal at 2.1 min in the chromatogram
of [188ReO(HL(Tyr3-Oct))2]+ corresponds to unreacted 188Re species.
RP-HPLC chromatogram (UV absorbance, λ
224 nm and radiation detection) of [188/natReO(HL(Tyr3-Oct))2]+ and free ligand H2L(Tyr3-Oct). The signal at 2.1 min in the chromatogram
of [188ReO(HL(Tyr3-Oct))2]+ corresponds to unreacted 188Re species.
Preparation of 99mTc-Labeled Complexes, [99mTcO(HL(cRGDfK))2]+ and [99mTcO(HL(Tyr3-Oct))2]+
The technetium-99m complexes
[99mTcO(HL(cRGDfK))2]+ and [99mTcO(HL(Tyr3-Oct))2]+ were prepared in
ca. 60–80% radiochemical yield using mild conditions and relatively
simple procedures (Supporting Information, Figures S1 and S2). Preparation of [99mTcO(HL(cRGDfK))2]+ and [99mTcO(HL(Tyr3-Oct))2]+ involved adding an excess of the appropriate
ligand dissolved in aqueous sodium chloride (0.5 mg mL–1, 0.9% NaCl, pH 7.4) to a mixture of [99mTcO4]− that has been reduced by tin(II) chloride in
0.1 M HCl in the presence of tartrate (pH 1–4) at room temperature.
The radiolabeled 99mTc complexes were characterized by
analysis by HPLC equipped with a radioactivity detector, and the elution
profiles were compared to the analogous nonradioactive rhenium compounds
(detected by UV absorbance). The close correlation between the retention
times of the rhenium and technetium complexes strongly suggests that
the complexes are isostructural (Table ). The small difference in the retention times between
the traces for 99mTc and Re complexes is, in part, due
to the detector configurations but could also reflect the difference
in polarity between the oxorhenium(V) and oxotechnetium(V) cores.
Table 3
RP-HPLC Retention Times (min) for Ligands and [MO(HL)2]+ Complexes (M = Re, 99 mTc)·L (ethyl), L (t-butyl), and L (phenyl) Compoundsa
compound
H2Lx
rhenium complex
technetium complex
L1-cRGDfK
10.0
11.4
11.5
L2-cRGDfK
9.3
10.3
10.9
L3-cRGDfK
10.9
12.0
12.7
L1-(Tyr3-Oct)
10.1
11.4
11.9
L2-(Tyr3-Oct)
10.9
11.7
12.1
L3-(Tyr3-Oct)
11.0
12.9
13.0
Linear gradient from 0 to 90% Buffer
B to A. Buffer A: 0.1% TFA in Milli-Q water. Buffer B: 0.1% TFA in
CH3CN.
Linear gradient from 0 to 90% Buffer
B to A. Buffer A: 0.1% TFA in Milli-Q water. Buffer B: 0.1% TFA in
CH3CN.The stability
of [99mTcO(HL(Tyr3-Oct))2]+ was assessed by incubation
in human plasma at 37 °C. The complex was stable for at least
2 h with only small amounts of degradation products (<5%) evident
that, based on their retention times in analytical HPLC, are most
likely due to degradation of the peptide.
Concluding Remarks
The new pyridylthiocarbazide ligands (SHYNIC, H2L) described
here offer a useful alternative to the standard HYNIC system. While
HYNIC has proved a very successful and versatile bifunctional ligand
for 99mTc coligands are required to complete the coordination
sphere of the metal ion and extrapolation to radioactive rhenium isotopes
has been challenging.[3,63] This family of bidentate ligands
form stable complexes with the {ReO}3+ core with two ligands
coordinated to a single metal ion. A rhenium complex with a methyl
ester functional group has been characterized by X-ray crystallography
and features the rhenium ion in a distorted square pyramidal environment
with the oxo group in the apical position relative to the pseudo basal
plane of two five-membered chelate rings with a N,N/S,S trans configuration
about the Re-oxo core. The basic ligands have been decorated with
the tumor targeting peptides cyclic-RGD and Tyr3-octreotate,
and these conjugates form complexes with rhenium to give well-defined
single species, [ReO((HL)(cRGDfK))2] and [ReO((HL)(Tyr3-octreotate))2], without having to add coligands resulting
in the formation of a single structural and geometrical isomer. It
is possible to form the rhenium complexes using either standard solution
chemistry or “on-resin”, and the latter approach may
prove useful in isolating radioactive 188/186Re analogues
in high specific activity. These complexes feature two targeting peptides
separated by 14 chemical bonds, and there is evidence that molecules
containing more than one targeting peptide, sometimes referred to
as bivalent, can display enhanced receptor binding due to simultaneous
binding to more than one receptor on the surface on any given cell.[14,67−72] It is possible to prepare [188ReO(HL(Tyr3-Oct))2]+ in ∼67% yield from generator produced [188ReO4]−, and improved yields should be possible
by optimizing the reaction conditions. The analogous technetium complexes,
[TcO((HL)(cRGDfK))2] and [TcO((HL)(Tyr3-Octreotate))2], were prepared directly from [99mTcO4]− with tin chloride acting as a reducing agent.
Comparison of HPLC profiles suggests the rhenium and technetium complexes
are isostructural. The complexes described in this manuscript have
two ligands coordinated to a single metal ion, whereas conventional
HYNIC systems involve one HYNIC ligand binding to one metal ion. It
is likely the two different systems will exhibit quite different biodistribution
in vivo. These new systems warrant further investigation as potential
theranostic agents employing an imaging (99mTc) and therapeutic
(186/188Re) matched pair for a single targeted agent.
General
Experimental
All reagents were purchased from standard commercial
sources. Nuclear magnetic resonance (NMR) spectra were acquired on
either an Agilent 400-MR (1H NMR at 400 MHz and 13C{1H} NMR at 101 MHz) or a Varian FT-NMR 500 spectrometer
(1H NMR at 500 MHz and 13C{1H} NMR
at 126 MHz) at 298 K. Chemical shifts were referenced to residual
solvent peaks and are quoted in ppm relative to TMS.Fmoc-l-amino acids, Fmoc-d-amino acids, Nvoc-Cl, HATU, DIC,
Wang resin, 2-chlorotrityl, Fmoc-Lys(ivDde)–OH, and Fmoc-Cys(Acm)–OH
were purchased from standard commercial sources.Linear protected
RGDfK peptide (Arg(Pbf)-Gly(tBoc)-Asp(OtBu)-dPhe-Lys(tBoc)) was synthesized
manually using standard Fmoc solid phase peptide synthesis (SPPS)
procedures on the 2-chlorotrityl chloride resin. The linear pentapeptide
was cleaved from the resin (with retention of protecting groups) using
1% TFA in dichloromethane and shaking for 40 min. The mixture was
filtered and the filtrate was reduced in volume to afford crude linear
product. Cyclization involved reacting the crude material in a mixture
of dichloromethane (1 mg mL–1), HATU (0.9 equiv),
and DIPEA (6 equiv) at RT for 2 h, then evaporation to dryness in vacuo. A solution of TFA (97.5%) and Milli-Q water (2.5%)
was added to the crude material to deprotect the peptide, followed
by removal of the trifluoroacetic acid by sparging with a stream of
N2. The peptide was precipitated with diethyl ether, isolated
by centrifugation (3 min, 3600 rpm) and dissolved in Milli-Q water
(5 mL), and finally purified by semiprep RP-HPLC (Column 1); Gradient
elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1%
TFA in CH3CN) from 0 to 40% B to A, over 40 min (1.0% min–1), UV detection at λ 220 nm with a flow rate
of 5 mL min–1.Linear protected Tyr3-octreotate peptide, dPhe-Cys(Trt)-Tyr(tBu)-dTrp(tBoc)-Lys(tBoc)-Thr(tBu)-Cys(Trt)-Thr(tBu)–OH,was
synthesized using standard automated Fmoc SPPS procedures on a 2-chorotrityl
chloride or Wang resin unless otherwise specified.[73]Analytical reversed phase high performance liquid
chromatography (RP-HPLC) was undertaken using an Agilent 1100 Series
HPLC system at a flow rate of 1 mL min–1 with either
Column 1: A Zorbax Eclipse XDB-C18 column (150 mm × 4.6 mm, 5.0
μm) or Column 2: A Phenomenex Aeris Peptide XB-C18 column (250
mm × 4.6 mm, 3.6 μm). Solvent gradients for analytical
analysis were either using System A: Gradient elution of Buffer A
(0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 0 to 100% B over 25 min and UV detection at λ 214,
254, and 280 nm, System B: Gradient elution of Buffer A (0.1% TFA
in H2O) and Buffer B (0.1% TFA in CH3CN) from
0 to 60% B over 30 min and UV detection at λ 214, 220, 254,
280, and 350 nm or System E: Gradient elution of Buffer A (0.1% TFA
in H2O) and Buffer B (0.1% TFA in CH3CN) from
20 to 80% B, over 30 min and UV detection at λ 220, 254, and
350 nm with a flow rate of 1 mL min–1.Semipreparative
reversed phase high performance liquid chromatography (semiprep RP-HPLC)
was performed using an Agilent 1200 series preparative HPLC unit with
variable wavelength detector. An automated Agilent 1200 fraction collector
collected 0.5–4 mL fractions. Peak separation was achieved
using either Column 3: Kinetex C18 100 Å, AXIA column (150 mm
× 21.2 mm, 5 μm), Column 4: Phenomenex Synergi Hydro-RP
80 Å (50 mm × 21.2 mm, 4 μm), Column 5: Varian Pursuit
XRs C18 100 Å (150 × 21.2 mm, 5 μm) or Column 6: SGE
ProteCol C18 120 Å (250 mm × 10 mm, 5 μm). Gradient
elution, flow rate, and wavelength detection are compound specific
and are detailed under the Experimental Section of a particular compound. Each fraction collected above 400 mAU
was analyzed using ESI-MS and analytical HPLC.Analytical HPLC
traces of radiolabeled 188Re compounds were acquired using
an Agilent 1200 LC system with in-line UV and gamma detection (Flow-Count,
LabLogic). Peak separation was achieved using an Agilent Eclipse XDB-C18
column (4.6 × 150 mm, 5 μm), with column 1 and system F:
Gradient elution of Buffer A (0.1% TFA in H2O) and Buffer
B (0.1% TFA in CH3CN) from 0 to 100% B over 20 min and
UV detection at λ 220 nm.Analytical HPLC traces of radiolabeled 99mTc compounds were acquired using a Shimadzu 10 AVP UV–visible
spectrophotometer (Shimadzu, Kyoto, Japan) and a sodium iodide scintillation
detector with two LC-10ATVP solvent delivery systems for solvents
A and B. Peak separation was achieved using Column 7: Nacalai Tesque
Cosomosil 5C18-AR Waters column (4.6 × 150 mm, 5 μm) (Kyoto,
Japan) at a flow rate of 1 mL min–1. Gradient elution
followed System C: Gradient elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 0 to 100%
B over 20 min and UV detection at λ 254 nm.X-ray structure
determination and refinement was obtained for [ReO(HL(OMe))2]TFA on an Oxford Diffraction
SuperNova CCD diffractometer using Cu–Kα radiation, and
the temperature during data collection was maintained at 130.0(1)
using an Oxford Cryosystems cooling device. The structure was solved
by direct methods using SHELXT and refined using least-squares methods
using SHELXL.[74,75] Thermal ellipsoid plots were
generated using ORTEP-3 integrated within the WINGX suite of programs.[76] The trifluoroacetate counterion, although recognizable
from the difference electron density maps, was badly disordered and
could not be modeled satisfactorily. Application of the Squeeze procedure
gave a void volume of 272 Å3 containing 127 electrons,
consistent with the presence of two trifluoroacetate anions per unit
cell.[77] The charge on the complex is unambiguously
(+1) given the presence of the two pyridinium protons which are involved
in intramolecular hydrogen bonds and the ethylamino protons which
are also involved in hydrogen bonds. The crystallographic data has
been deposited in the Cambridge Structural Database (CCDC 1543360).
Ligand Synthesis
Note: The
designation of H2refers to the structure with a carboxylic acid-substituted, pyridylhydrazine
with the different thiocarbahydrazide functional groups (Et, tBu,
and Ph respectively). Further derivatization of the carboxylate functional
group is represented by placing the substituted group at the carboxylic
carbon in replacement of the OH group (e.g., H2(OMe), denotes the substitution of
a methoxy at the carbonyl carbon to give a methyl ester.
To a suspension of 6-hydrazino-3-pyridinecarboxylic acid (0.45 g,
2.9 mmol) in anhydrous DMA (5 mL) was added tert-butyl
isothiocyanate (0.56 mL, 4.4 mmol) under an atmosphere of nitrogen.
The suspension was heated to 85 °C and after 30 min became a
yellow mixture, which was heated at 85 °C for a further 3 h.
The mixture was concentrated by evaporation under reduced pressure
to a volume of approximately 1 mL and cold diethyl ether (15 mL) was
added. The suspension was stirred vigorously overnight at RT. The
precipitate was collected via filtration and washed with copious amounts
of cold diethyl ether to afford an off-white solid (0.68 g, 86%). 1H NMR [MeOH-d4, 500 MHz]: δ
(ppm) 8.73 (1H, d, J = 2.2 Hz, pyH2), 8.18 (1H, dd, J = 8.7, 2.2 Hz, pyH4), 6.76 (1H, dd, J = 8.7,
0.7 Hz, pyH5), 1.51 (9H, s); 13C{1H} NMR [MeOH-d4, 125.7
MHz]: δ (ppm) 181.0 (C, NCS), 166.1 (C, CO2H), 162.0 (C, pyC6), 150.4 (C, pyC2), 138.8 (C, pyC4), 117.8 (C, pyC3), 105.6 (C, pyC5), 54.7 (C, -C(CH3)3), 29.0 (3C, -C(CH3)3); IR: ν̅max (cm–1) 1604 (s/sh, C=O), 1533 (s/sh), 1280 (s/sh),
1252 (s/sh), 1133 (m/sh), 1002 (m/sh), 779 (s/sh); HRMS (ESI+): m/z calc’d for C11H17N4O2S 269.1072, found
269.1110 {[M + H]+, 100%}; RP-HPLC (Column 1, System A): RT (min) 10.6.
To a suspension of 6-hydrazino-3-pyridinecarboxylic acid (0.45 g,
2.9 mmol) in anhydrous dimethylacetamide (DMA) (5 mL) was added phenyl
isothiocyanate (0.59 mL, 4.4 mmol) under an atmosphere of nitrogen.
The suspension was heated to 65 °C and after 5 min became a yellow
solution, which was heated at 65 °C for a further 2 h. The mixture
was concentrated by evaporation under reduced pressure to a volume
of approximately 1 mL, and cold diethyl ether (15 mL) was added A
precipitate was collected by filtration and washed with copious amounts
of cold diethyl ether to afford an off-white powder (0.81 g, 97%). 1H NMR [DMSO-d6, 400 MHz]: δ
(ppm) 9.88 (1H, br s, NH), 9.84 (1H, br s, NH), 9.22 (1H, br s, NH), 8.67 (1H, d, J = 1.9 Hz, pyH2), 8.07 (1H,
d, J = 8.4 Hz, pyH4),
7.47 (2H, d, J = 7.2 Hz, ArH), 7.30
(2H, t, J = 7.2 Hz, ArH), 7.13 (1H,
t, J = 7.2 Hz, ArH), 6.66 (1H, d, J = 8.8 Hz, pyH5); 13C{1H} NMR [MeOH-d4, 125.7
MHz]: δ (ppm) 181.3 (C, NCS), 166.4 (C, CO2H), 161.7 (C, pyC6), 150.3 (C, pyC2), 139.2 (C, pyC4), 138.7 (C, ArC1), 127.9 (2C, ArC3,5), 125.6 (C, ArC4), 124.9 (2C, ArC2,6), 117.8 (C, pyC3), 106.1 (C, pyC5); IR: ν̅max (cm–1) 1607 (s/sh, C=O), 1596 (s/sh), 1537 (s/sh),
1280 (s/sh), 1254 (s/sh), 1140 (m/sh), 1019 (m/sh), 782 (m/sh); HRMS
(ESI+): m/z calc’d
for C13H13N4O2S 289.0759,
found 289.0749 {[M + H]+, 100%}; RP-HPLC (Column 1, System
A): RT (min) 9.9.
Methyl 6-Chloropyridine-3-carboxylate, 3
A suspension of 6-chloronicotinic acid (5.0 g,
32 mmol) in methanol (100 mL) was cooled to 0 °C, and H2SO4 (0.5 mL) was added dropwise. The mixture was heated
at 60 °C for 8 h. The crude reaction mixture was evaporated to
dryness under reduced pressure. The residue was dissolved in ethyl
acetate and washed with sat. NaHCO3. The organic layer
was dried over MgSO4, filtered, and evaporated to dryness
in vacuo. The pale yellow solid was recrystallized from methanol to
form clear, plate-like crystals (5.0 g, 91%). 1H NMR [CHCl3-d, 400 MHz]: δ (ppm) 9.00 (1H, dd, J = 2.4, 0.7 Hz, pyH2), 8.25
(1H, dd, J = 8.3, 2.4 Hz, pyH4), 7.42 (1H, dd, J = 8.3, 0.8 Hz, pyH5), 3.96 (3H, s, CH3); 13C{1H} NMR [CHCl3-d, 125.7 MHz]: δ (ppm) 165.0 (C, CO2Me), 155.8 (C, pyC6), 151.3 (C, pyC2), 139.8 (C, pyC4), 125.2 (C, pyC3), 124.4 (C, pyC5), 52.8 (C, OCH3); ESI-MS (+): m/z calc’d
for C7H7ClNO2 172.0165, found 171.9965
{[M + H]+, 100%}; RP-HPLC (Column 2, System A): RT (min) 8.7.
Methyl 6-Hydrazinyl-3-pyridinecarboxylate, 4
Methyl 6-chloropyridine-3-carboxylate, 3, (0.10 g, 0.58 mmol), and hydrazine hydrate (50–60% N2H4, d = 1.029 g cm–3, 0.10 mL, approximately 3 equiv) were added to a 5 mL microwave
vial, which was evacuated and purged with N2. Degassed
methanol (5 mL) was added to the vial, and the suspension was subjected
to microwave irradiation for 15 min at 105 °C. The mixture was
filtered and concentrated in vacuo. The residue obtained was dissolved
in ethyl acetate and washed with sat. NaHCO3 and sat. NaCl.
The organic layer was collected and dried over Na2SO4, filtered, and concentrated to afford a chalky, yellow powder
(0.08 g, 81%). 1H NMR [CHCl3-d, 600 MHz]: δ (ppm) 8.95 (1H, d, J = 2.4 Hz,
pyH2), 8.21 (1H, dd, J = 8.3, 2.4 Hz, pyH4), 7.40 (1H, d, J = 8.3 Hz, pyH5), 3.92 (3H,
s, OCH3); 13C{1H}
NMR [CHCl3-d, 151 MHz]: δ (ppm)
165.0 (C, CO2Me), 155.7 (C, pyC6), 151.1 (C, pyC2), 139.7 (C, pyC4), 125.1 (C, pyC3), 124.3 (C, pyC5), 52.7 (C, OCH3); HRMS (ESI+): m/z calc’d for C7H10N3O2 168.0773, found 168.0777
{[M + H]+, 100%}; RP-HPLC (Column 2, System A): RT (min) 7.6.
Dichloromethane (10 mL) was added to 2-chlorotrityl resin (1.00 mmol
g–1 loading) (3.1 g, 3.1 mmol) swelling the resin.
A mixture of Nα-tBoc-Nε-Fmoc-l-Lys (1.7
g, 3.6 mmol) and DIPEA (2.1 mL, 12 mmol) in dichloromethane (15 mL)
was added to the resin, which was then shaken at ambient temperature
for 2 h. The resin was filtered and the filtrate was discarded. The
resulting resin was washed with dichloromethane (3 mL), DMF (3 mL),
dichloromethane (3 mL), and finally diethyl ether (3 mL). After several
hours of suction drying the resin was weighed and loading determined
(0.77 mmol g–1). To the dried resin-bound tBoc-Lys(Fmoc)–OH (0.51 g, 0.39 mmol) was added a
DMF/piperidine (80:20 v/v) solution
(20 mL), which was manually stirred. After 20 min, the supernatant
was removed by filtration through a sintered frit, and the remaining
resin was washed with DMF (3 mL). A positive TNBSA assay (2,4,6-trinitrobenzenesulfonic
acid in methanol (5% w/v)) was used
to indicate deprotection of the Fmoc protected epsilon (ε) amine.
A mixture of HATU (285 mg, 0.75 mmol), H2L (176 mg, 0.75 mmol), and DIPEA (261 μL,
1.5 mmol) in DMF (4 mL) was added to the resin and reacted for 4 h
at ambient temperature. The liquid was drained and the resin was washed
successively with dichloromethane (3 mL), then DMF (3 mL), and again
with dichloromethane (3 mL). A TFA/H2O/dichloromethane
(18:2:80 v/v) solution was added
to half the resin (approximately 0.19 mmol), and the mixture shaken
for 1 h and then filtered. The filtrate was concentrated in vacuo
and diethyl ether (40 mL) was added to form a suspension, which was
centrifuged (3 min, 3600 rpm) and the supernatant was discarded. The
crude material was dissolved in H2O/CH3CN (90:10 v/v), filtered (Millipore 0.45 μm
porosity syringe filter), and then purified by semipreparative RP-HPLC
(Column 5). The HPLC system involved a gradient elution of Buffer
A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 20 to 40% B to A, over 20 min (1.0% min–1) then 40–60% over 40 min (0.5% min–1) and
UV detection at 220 nm with a flow rate of 5 mL min–1. Fractions containing the desired compound were identified by HPLC-MS,
consolidated and lyophilized to afford an off-white, fluffy compound
(10 mg, 14%). ESI-MS (+): m/z calc’d for C15H25N6O3S 369.1709, found 369.1798 {[M + H]+, 100%}; RP-HPLC
(Column 2, System A): RT (min) 6.00, (Column
2, System B) 24.0.
H2L(NαOAc-Lys-OMe)
A solution of HATU
(0.23 g, 0.56 mmol) and DIPEA (0.29 mL, 1.1 mmol) in DMSO (1 mL) was
added to H2L (0.15
g, 0.56 mmol) and shaken for 2 min. Nα-Acetyl-l-lysinemethyl ester hydrochloride (0.10 g, 0.42
mmol) in DMSO (1 mL) was added and shaken for 2 h. Diethyl ether (40
mL) was added and the mixture was centrifuged. The supernatant was
discarded and the remaining yellow oil was purified by semipreparative
RP-HPLC (Column 5). The HPLC system involved a gradient elution of
Buffer A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 10 to 60% B to A, over 50 min (1.0% min–1) and UV detection at λ 220 and 254 nm with a flow rate of
5 mL min–1. Fractions containing the desired compound
were identified by HPLC-MS, consolidated, and lyophilized to afford
a colorless fluffy solid (0.19 g, 27%). 1H NMR [MeOH-d4, 600 MHz]: δ (ppm) 8.48 (1H, d, J = 2.1 Hz, pyH2), 8.29 (1H,
dd, J = 9.1, 2.2 Hz, pyH4), 7.05 (1H, d, J = 9.1 Hz, pyH5), 4.38 (1H, dd, J = 8.9, 5.2 Hz, αCH), 3.70 (3H, s, CO2CH3), 3.38 (2H, t, J = 7.2 Hz, εCH2), 1.97 (3H, s, COCH3), 1.87–1.84
(1H, m, βCH2), 1.75–1.69
(1H, m, βCH2), 1.65–1.61
(2H, m, δCH2), 1.53 (9H, s, (CH3)3), 1.49–1.41 (2H, m, γCH2); 13C{1H} NMR [MeOH-d4, 150.9 MHz]: δ (ppm) 184.0 (C, NCS), 174.2 (C, -COCH3), 173.4
(C, -CO2CH3), 165.9 (C, CONH), 159.1 (C, pyC6), 149.4
(C, pyC2), 141.4 (C, pyC4), 123.7 (C, pyC3), 110.6
(C, pyC5), 54.9 (C, -C(CH3)3), 53.7 (C, αCH2), 52.7 (C, −CO2CH3), 40.7 (C, εCH2),
32.1 (C, βCH2), 29.8 (C, δCH2), 28.9 (3C, -C(CH3)3), 24.2 (C, −COCH3), 22.3 (C, γCH2); HRMS (ESI+): m/z calc’d for C20H33N6O4S 453.2284, found 453.2288 {[M
+ H]+, 100%}; RP-HPLC (Column 2, System A): RT (min) 12.5.
H2L(cRGDfK)
To a solution of 6-[(2-ethylcarbamothioyl)hydrazinyl]-3-pyridinecarboxylic
acid, (H2L) (16 mg,
66 μmol) in DMF (0.5 mL) was added HATU (25 mg, 66 μmol)
and DIPEA (23 μL, 0.13 mmol). A solution of cRGDfK (10 mg, 17
μmol) in DMF (0.3 mL) was added to the initial mixture and then
shaken for 2 h at ambient temperature. Diethyl ether (40 mL) was added
and the subsequent suspension centrifuged (3 min, 3600 rpm). The supernatant
was discarded and the process repeated. The remaining solid was dissolved
in a H2O/CH3CN (90:10 v/v) solution, filtered (Millipore 0.45 μm porosity
syringe filter), and then purified by semipreparative RP-HPLC (Column
4). The HPLC system involved a gradient elution of Buffer A (0.1%
TFA in H2O) and Buffer B (0.1% TFA in CH3CN)
from 0 to 50% B to A, over 65 min (1.3% min–1) and
UV detection at λ 220, 254, 275, and 350 nm with a flow rate
of 8 mL min–1. Fractions containing the desired
compound were identified by HPLC-MS, consolidated and lyophilized
to afford a colorless solid (10 mg, 80%). ESI-MS (+) m/z calc’d for [C36H52N13O8S]+ 826.378, found
826.376, calc’d for [C36H53N13O8S]2+ 413.693, found 413.692; RP-HPLC (Column
2, System A): RT (min) 11.3.The same
procedure was used as for H2L(cRGDfK), except H2L was replaced with 6-[(2-tert-butylcarbamothioyl)hydrazinyl]-3-pyridinecarboxylic
acid, (H2L) (5.3
mg, 19 μmol), and other reagent quantities were adapted accordingly;
HATU (6.5 mg, 17 μmol), DIPEA (45 μL, 0.13 mmol), and
cRGDfK (10 mg, 17 μmol). Semipreparative RP-HPLC purification
(Column 4) involved a gradient elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 0 to 40%
B to A, over 80 min (0.5% min–1) and UV detection
at λ 220, 254, 275, and 350 nm with a flow rate of 8 mL min–1. Fractions containing the desired compound were identified
by HPLC-MS, consolidated and lyophilized to afford a light yellow
solid (3.4 mg, 24%). ESI-MS (+) m/z calc’d for [C38H56N13O8S]+ 854.4096, found 854.4097, calc’d
for [C38H57N13O8S]2+ 427.7087, found 427.7083; RP-HPLC (Column 2, System A): RT (min) 12.9.The same procedure was
used as for H2L(cRGDfK),
except H2L was replaced
with 6-[(2-phenylcarbamothioyl)hydrazinyl]-3-pyridinecarboxylic acid,
(H2L) (5.2 mg, 19
μmol) and other reagent quantities were adapted accordingly;
HATU (6.8 mg, 18 μmol), DIPEA (45 μL, 0.13 mmol), and
cRGDfK (10 mg, 17 μmol). Semipreparative RP-HPLC purification
(Column 4) involved a gradient elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 0 to 40%
B to A, over 80 min (0.5% min–1) and UV detection
at λ 214, 220, and 254 nm with a flow rate of 8 mL min–1. Fractions containing the desired compound were identified by HPLC-MS,
consolidated, and lyophilized to afford a colorless solid (8.6 mg,
55%). ESI-MS (+) m/z calc’d
for [C40H52N13O8S]+ 874.3783, found 874.3380, calc’d for [C40H53N13O8S]2+ 437.6930,
found 437.6992; RP-HPLC (Column 2, System A): RT (min) 14.2.
H2L(Tyr3-Oct)
Linear protected Tyr3-octreotate peptide (dPhe-Cys(Acm)-Tyr(tBu)-dTrp(tBoc)-Lys(tBoc)-Thr(tBu)-Cys(Acm)-Thr(tBu)-OH) was prepared manually by standard Fmoc SPPS on
Wang resin preloaded with H-Thr(tBu)–OH (100
mg, 0.5 mmol g–1). Amino acid coupling: Coupling
of each amino acid was achieved by addition to the resin of a premade
solution of Fmoc-amino acid (2 mmol, 4 equiv), HATU (1.9 mmol, 3.8
equiv), and DIPEA (4 mmol, 8 equiv) in DMF (5 mL). The resin mixture
was shaken in a reaction vessel equipped with a sintered bottom for
1 h then filtered and washed with DMF (3 mL), dichloromethane (3 mL),
and again with DMF (3 mL). Successful coupling was confirmed by a
negative TNBSA test. Fmoc deprotection: Cleavage of the Fmoc groups
was achieved after each successive coupling reaction. A DMF/piperidine
(80:20 v/v) solution was added to
the protected resin, which was contained in a reaction vessel with
a sintered frit. The mixture was stirred for 5 min, and then the resin
was filtered and washed with cleavage solution, then DMF (2 mL), dichloromethane
(2 mL) and again DMF (3 mL). Complete deprotection was confirmed with
a positive TNBSA test. Acm-group deprotection and on-resin cyclization:
After the final Fmoc deprotection of resin-bound Fmoc-dPhe-OH, thallium(III)
trifluoroacetate (Tl(CF3CO2)3) (0.54
g, 1.0 mmol, 2 equiv) in DMF (4 mL) was added to the resin, and the
mixture was stirred for 2 h. The liquid was decanted from the resin
and the resin was washed with DMF (15 mL), dichloromethane (3 mL),
and diethyl ether (2 mL). SHYNIC coupling: Half the resin-bound peptide
(approximately 0.25 mmol) was used for the following reaction. H2L (0.18 g, 0.75 mmol,
3 equiv) was dissolved in DMF (3 mL) and HATU (0.29 g, 0.75 mmol,
3 equiv) added to preactivate the ligand. DIPEA (0.26 mL, 1.5 mmol,
6 equiv) was added and the mixture shaken for 2 min until full dissolution
had occurred. The yellow solution was added to the dry resin in a
reaction vessel equipped with a sintered frit and shaken for 2 h.
The reaction solution was drained and the resin was washed with DMF
(15 mL), dichloromethane (3 mL) and again DMF (3 mL). Resin and acid-sensitive
protecting group cleavage: The petide-loaded resin was treated with
a TFA/TIPS/H2O (96:1.5:2.5 v/v/v) solution (20 mL) and shaken for 2 h. The mixture
was filtered and sparged with a steady stream of N2 to
reduce the volume by 90%. Cold diethyl ether (40 mL) was added to
precipitate the peptide that was isolated by centrifugation (3 min,
3600 rpm). The crude material was dissolved in CH3CN/H2O (50:50 v/v) and lyophilized.
The solid was dissolved in CH3CN/H2O (40:60 v/v) and filtered (Millipore 0.45 μm
porosity syringe filter). The compound was purified by semipreparative
RP-HPLC (Column 5) with a linear gradient elution of Buffer A (0.1%
TFA in H2O) and Buffer B (0.1% TFA in CH3CN)
from 20 to 80% B to A, over 120 min (0.5% min–1)
and UV detection at λ 214, 220, 254, 280, and 350 nm with a
flow rate of 8 mL min–1. Fractions containing the
desired compound were identified by HPLC-MS, consolidated and lyophilized
to afford a pale yellow solid (56 mg, 18%). HRMS (+) m/z calc’d for [C58H75N14O13S3]+ 1271.4800,
found 1271.4760, calc’d for [C58H75N14O13S3]2+ 636.2439, found
636.2416; RP-HPLC (Column 2, System A): RT (min) 13.0.The same procedure was used
as for H2L(Tyr3-Oct), except H2L was replaced with H2L (0.20 g, 0.75 mmol, 3 equiv), and all other reagents were
used according to their reported equivalencies. The precipitate after
lyophilization was dissolved in CH3CN/H2O (8
mL, 50:50 v/v) and filtered (Millipore
0.45 μm porosity syringe filter). The compound was purified
by semipreparative RP-HPLC (Column 5) with an isocratic step gradient
system of Buffer A (0.1% TFA in H2O) and Buffer B (0.1%
TFA in CH3CN). The elution method involved 28% B for 10
min then 32% B for 40 min (desired peak at 34 min) and UV detection
at λ 214, 220, 254, 280, and 350 nm with a flow rate of 8 mL
min–1. Fractions containing the desired compound
were identified by HPLC-MS, consolidated, and lyophilized to afford
a fluffy, colorless compound (18 mg, 5.5%). HRMS (+) m/z calc’d for [C60H79N14O13S3]+ 1299.5113,
found 1299.5110, calc’d for [C60H80N14O13S3]2+ 650.2596, found
650.2599; RP-HPLC (Column 2, System A): RT (min) 14.4.The same procedure was used
as for H2L(Tyr3-Oct), except H2L was replaced with H2L (0.22 g, 0.75 mmol, 3 equiv). The precipitate after lyophilization
was dissolved in CH3CN/H2O (10 mL, 50:50 v/v) and filtered (Millipore 0.45 μm
porosity syringe filter). The compound was purified by semipreparative
RP-HPLC (Column 5) with a linear gradient system of Buffer A (0.1%
TFA in H2O) and Buffer B (0.1% TFA in CH3CN)
from 20% to 50% B to A over 60 min (0.5% min–1)
(or isocratic elution at 29% Buffer B) and UV detection at λ
254 nm with a flow rate of 7 mL min–1. Fractions
containing the desired compound were identified by HPLC-MS, consolidated
and lyophilized to afford a fluffy white solid (14 mg, 4.2%). HRMS
(+) m/z calc’d
for [C62H75N14O13S3]+ 1319.4800, found 1319.4849, calc’d for
[C62H75N14O13S3]2+ 650.2596, found 636.2425; RP-HPLC (Column 2, System
A): RT (min) 14.1.
Synthesis of
Rhenium Complexes
Note: Unless specified Re represents
‘rhenium with natural isotope abundance’.
[ReO(HL(OMe))2]Cl
To
H2L1(OMe) (90 mg, 0.35 mmol) and
(tBu4N)[ReOCl4] (103 mg, 0.18
mmol) was added anhydrous MeOH (13 mL). The mixture immediately turned
deep red and was stirred at room temperature for 4 h. The reaction
mixture was filtered, diethyl ether (ca. 15 mL) was added, and the
resulting precipitate was collected by filtration to give [ReO(HL(OMe))2]Cl as a dark-red,
microcrystalline solid (0.11 g, 84%). 1H NMR [DMSO-d6, 400 MHz]: δ (ppm) 8.63 (2H, s, pyH2), 8.26 (2H, dd, J = 9.3,
1.8 Hz, pyH5), 7.87 (2H, d, J = 9.4 Hz, pyH4), 7.43 (2H, br m, NH), 3.89 (6H, s, OCH3), 3.47
(4H, qd, J = 13.6, 7.0 Hz, CH2CH3), 1.16 (6H, t, J = 7.5 Hz,
CH2CH3); 13C{1H} NMR [CH3CN-d3, 150.9
MHz]: δ (ppm) 173.7 (2C, CO2CH3), 165.1 (2C, N=CS), 162.5 (2C, pyC6), 140.5 (2C, pyC5), 139.9 (2C, pyC2), 123.9 (2C, pyC4), 122.0 (2C, pyC3), 52.3 (2C, CO2CH3), 42.6
(2C, CH2CH3), 14.5 (2C, CH2CH3); IR: ν̅max (cm–1) 1553 (s/sh, C=O), 1287 (s/sh), 963
(m/sh, Re=O), 764 (m/sh); HRMS (ESI+): m/z calc’d for ReC20H26N8O5S2 709.0916, found 709.0898
{[M]+, 100%}; RP-HPLC (Column 2, System A): RT (min) 14.8.
Histidine and Cysteine Challenge Experiments
A 50-fold excess of histidine or cysteine was added to a solution
of [ReO(HL(OMe))2]+ (1 mg/L) in PBS Buffer (10 mM, pH 7.4, 4 mL) and the
mixture was heated to 37 °C. At 2, 4, and 24 h after initiation
of the experiment, 10 μL aliquots of the reaction mixture were
diluted with 90 μL of Milli-Q water and analyzed using analytical
HPLC methods. The HPLC traces showed little or no decomposition (<5%)
of the rhenium complex at all the time-points.
[ReO(HL(OMe))2]BPh4
To a stirred suspension of trans-[ReOCl3(PPh3)2] (0.15 g, 0.17 mmol) in MeOH
(10 mL) was added H2L(OMe) (0.10 g, 0.35 mmol) and 2 drops of Et3N. The mixture
was heated at reflux for 16 h, then filtered, and diethyl ether was
added to the filtrate. The resulting precipitate was collected by
filtration, washed with cold diethyl ether, and then dissolved in
MeOH. Addition of excess NaBPh4 resulted in the precipitation
of a red-brown precipitate that was collected, and washed with hot
hexane (10 mL) to afford [ReO(HL(OMe))2]BPh4 (72 mg, 39%). 1H NMR
[CHCl3-d, 600 MHz]: δ (ppm) 8.10
(2H, d, J = 9.5 Hz, pyH2), 7.75 (2H, d, J = 9.4 Hz, pyH5), 7.62 (8H, m, BArH), 7.33 (2H, m,
pyH4), 6.93 (8H, t, J = 7.1 Hz, BArH), 6.72 (4H, t, J = 7.1 Hz, BArH), 3.86 (6H, s, CO2CH3), 1.39 (18H, s, (CH3)3); 13C{1H} NMR [CHCl3-d, 150.9 MHz]: δ (ppm) 164.5, 142.5, 135.8–135.8
(8C, BArC), 133.9–133.8, 128.9, 128.6, 128.5,
127.5, 126.2–126.1 (8C, BArC), 122.0 (4C,
BArC), 54.9 (2C, -OCH3), 52.6 (2C, -C(CH3)3), 29.0
(6C, -C(CH3)3); IR: ν̅max (cm–1) 1555 (s/sh, C=O), 1284
(s/sh), 960 (m/sh, Re=O), 756 (m/sh); HRMS (ESI+): m/z calc’d for ReC24H34N8O5S2 765.1651,
found 765.1559 {[M]+, 100%}; RP-HPLC (Column 2, System
A): RT (min) 15.0.The
same procedure was used as for [ReO(HL(OMe))2]+, except H2L(OMe) was replaced with H2L(OMe) (0.10 g, 0.33 mmol).
All other reagents quantities were used accordingly; (tBu4N)[ReOCl4] (95 mg, 0.16 mmol) and MeOH (20
mL). The reaction afforded a red microcrystalline solid (69 mg, 51%). 1H NMR [DMSO-d6, 400 MHz]: δ
(ppm) 9.84 (2H, s, NH), 8.79 (2H, s, pyH2), 8.42 (2H, dd, J = 9.1, 1.7 Hz, pyH5), 8.03 (2H, d, J = 9.2 Hz,
pyH4), 7.73 (4H, d, J = 7.8 Hz, ArH2,6), 7.32 (4H, t, J = 7.9 Hz, ArH3,5), 6.95 (2H,
t, J = 7.3 Hz, ArH4),
3.92 (6H, s, CO2CH3); 13C{1H} NMR [DMSO-d6, 150.9 MHz]: δ (ppm) CO2Me signal not detected,
164.2 (2C), 145.5 (2C), 142.2 (2C, pyC5), 139.5 (2C, pyC2), 130.0 (2C, ArC3,5), 129.3 (4C, ArC4), 128.9 (2C, ArC1), 122.3 (2C, pyC4), 121.4 (2C, pyC3), 117.6 (4C, ArC2,6), 52.6 (2C, CO2CH3)3); IR: ν̅max (cm–1) 1557 (s/sh, C=O), 1282
(s/sh), 960 (m/sh, Re=O), 752 (m/sh); HRMS (ESI+): m/z calc’d for ReC28H26N8O5S2, 805.1014,
found 805.1004 {[M]+, 100%}; RP-HPLC (Column 2, System
A): RT (min) 15.4.
[ReO(HL(Nα-Ac-Lys-OMe))2]+
To H2L(Nα-Ac-Lys-OMe)
(15 mg, 33 μmol) in MeOH (1 mL) was added a solution of (tBu4N)[ReOCl4] (0.9 mg, 15 μmol)
in MeOH (0.3 mL). The mixture was stirred at ambient temperature for
2 h, then diluted with Milli-Q water and purified by semipreparative
RP-HPLC (Column 4). The HPLC system involved a gradient elution of
Buffer A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 10 to 20% B to A, over 10 min (1.0% min–1), then 20 to 40% B to A over 40 min (0.5% min–1) and UV detection at λ 214, 220, 254, and 280 nm with a flow
rate of 8 mL min–1. Fractions containing the desired
compound were identified by HPLC-MS, consolidated and lyophilized
to afford a red solid (5 mg, 27%, assuming [ReO(HL(Nα-Ac-Lys-OMe))2]CF3CO2). 1HNMR [MeOH-d4, 600 MHz]: δ (ppm) 8.68 (2H, s, pyH2), 8.36 (2H, d, J = 9.6 Hz, pyH5), 8.03 (2H, d, J = 9.5 Hz,
pyH4), 4.43–4.40 (2H, m, αCH), 3.72 (6H, s, CO2CH3), 3.43 (4H, q, J = 6.6 Hz, εCH2), 1.99 (6H, s, COCH3), 1.92–1.86
(4H, m, βCH2), 1.78–1.72
(4H, m, δCH2), 1.71–1.66
(4H, m, γCH2), 1.50 (18H, s, (CH3)3); 13C{1H} NMR [MeOH-d4, 150.9 MHz]: δ
(ppm) 174.2 (2C, COCH3), 173.4 (2C, CO2CH3), 167.2 (2C, N = CS), 165.1 (2C, CONH), 163.3 (2C, pyC6), 140.7 (2C, d, pyC5), 139.1
(2C, d, pyC2), 124.5 (2C, pyC4), 122.6 (2C, pyC3), 55.3
(2C, -C(CH3)3), 53.7 (C, αCH2), 52.7 (C, −CO2CH3), 40.8 (2C, εCH2), 32.1 (2C, βCH2), 29.9
(2C, δCH2), 28.9 (6C, -C(CH3)3), 24.3 (2C, COCH3), 22.3 (2C, γCH2);
HRMS (ESI+) m/z calc’d
for [ReC40H62N12O9S2]+ 1105.3762, found 1105.4079, calc’d for
[ReC40H62N12O9S]2+ 553.1920, found 553.2094; RP-HPLC (Column 2, System A): RT (min) 16.9.
[ReO(HL(Lys))2]+
To resin-bound
H2L(Lys) (approximately
0.19 mmol) was added trans-[ReOCl3(PPh3)2] (78 mg, 0.09 mmol) suspended in DMF (5 mL).
The slurry was stirred for 2 h. The green suspension turned colorless
and the resin turned dark red. The red resin was isolated by filtration
and washed with DMF (3 mL), dichloromethane (3 mL), and again with
DMF (3 mL). The rhenium complex was cleaved from the resin by treatment
with TFA/dichloromethane (50:50 v/v) solution (30 mL) for 3 h. The mixture was sparged with N2 to reduce the volume to 10% of the original volume. Cold diethyl
ether (40 mL) was added, the mixture was centrifuged (3 min, 3600
rpm), and the supernatant was discarded. This process was repeated
twice. The precipitate was dissolved in CH3CN (1.0 mL)
and then Milli-Q water (2.0 mL) was added. The complex was purified
by semipreparative RP-HPLC purification (Column 5) involved a gradient
elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1%
TFA in CH3CN) from 10 to 70% B to A, over 120 min (0.5%
min–1) and UV detection at λ 214, 220, and
254 nm, with a flow rate of 8 mL min–1. Fractions
containing the desired compound were identified by HPLC-MS, consolidated,
and lyophilized to afford a red, fluffy solid (22 mg, 23%, assuming
[ReO(HL(Lys))2]CF3CO2). 1H NMR [MeOH-d4, 600 MHz]: δ (ppm) 8.58 (2H, s, pyH2), 8.34 (2H, dd, J = 9.5, 1.8 Hz, pyH5), 7.97 (2H, d, J = 9.5 Hz,
pyH4), 3.80 (2H, t, J = 6.1 Hz, αCH), 3.60 (4H, dtd, J = 20.2, 13.2, 7.0 Hz, −CH2CH3), 3.46 (4H, dd, J = 8.9, 5.1 Hz, εCH2), 1.99–1.92 (4H, m, βCH2), 1.72 (4H, dt, J = 14.5,
7.3 Hz, δCH2), 1.60–1.50
(4H, m, γCH2), 1.27 (6H, t, −CH2CH3); 13C{1H} NMR [MeOH-d4, 150.9 MHz]: δ
(ppm) 172.8 (2C, CO2H), 169.0 (2C, N=CS), 165.4 (2C, CONH), 163.6 (2C, pyC6), 140.5 (2C, pyC5), 138.9 (2C, pyC2), 123.9 (2C, pyC4), 122.5 (2C, pyC3), 54.9 (2C, αCH), 42.5 (2C, CH2CH3), 40.6 (2C, εCH2), 31.5 (2C, βCH2),
29.9 (2C, δCH2), 23.4 (2C, γCH2), 14.9 (2C, CH2CH3); ESI-MS (+) m/z calc’d for [ReC30H46N12O7S2]+ 937.2611, found 937.2574,
calc’d for [ReC30H47N12O7S2]2+ 469.1345, found 469.1355, calc’d
for [ReC30H48N12O7S2]3+ 313.0256, found 313.0939; RP-HPLC (Column 2,
System A): RT (min) 10.1.
[ReO(HL(cRGDfK))2]+
A solution of H2L(cRGDfK) (5 mg, 6.1 μmol) in MeOH (250 μL) was
added to a mixture of [tBu4N][ReOCl4] (1.8 mg, 3.0 μmol) in MeOH (250 μL). The mixture
was shaken for 2.5 h, then diluted with Milli-Q water (5 mL), filtered
(Millipore 0.45 μm porosity syringe filter), and purified by
semiprep RP-HPLC (Column 6). The HPLC system involved isocratic elution
of 77% Buffer A (0.1% TFA in H2O) and 23% Buffer B (0.1%
TFA in CH3CN) (0.5% min–1) and UV detection
at λ 214, 220, 254, 280, and 350 nm with a flow rate of 5 mL
min–1. Fractions containing the desired compound
were identified by HPLC-MS, consolidated, and lyophilized to afford
a white solid (3.1 mg, 53%, assuming [ReO(HL(cRGDfK))2]CF3CO2). HRMS (ESI+) m/z calc’d
for [ReC72H101N26O17S2]2+ 926.3413, 926.3433, calc’d for [ReC72H102N26O17S2]3+ 617.8968, found 617.9939; RP-HPLC (Column 2, System A): RT (min) 11.0.The
same procedure was used as for [ReO(HL(cRGDfK))2]+, except H2L(cRGDfK) was replaced with
H2L(cRGDfK) (8.0
mg, 9.4 μmol) in MeOH (250 μL); (tBu4N)[ReOCl4] (2.7 mg, 4.7 μmol) in MeOH (500
μL). The compound was purified by semipreparative RP-HPLC purification
(Column 4) involved gradient elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1% TFA in CH3CN) from 0 to 20%
over 20 min (1% min–1), then 20 to 60% B to A over
40 min (0.5% min–1) and UV detection at 214, 220,
254, 280, and 350 nm with a flow rate of 8 mL min–1. Fractions containing the desired compound were identified by HPLC-MS,
consolidated and lyophilized to afford a white solid (5.1 mg, ∼54%,
assuming [ReO(HL(cRGDfK))2]CF3CO2). HRMS (ESI+) m/z calc’d for [ReC76H109N26O17S2]2+ 954.3732, found 954.3715, calc’d for [ReC76H110N26O17S2]3+ 636.5847, found 636.5837; RP-HPLC (Column 2, System A): RT (min) 12.5.The
same procedure was used as for [ReO(HL(cRGDfK))2]+, except H2L(cRGDfK) was replaced with H2L(cRGDfK) (4.0 mg, 4.6
μmol) in MeOH (200 μL), and other reagent quantities were
adapted accordingly, [tBu4N][ReOCl4] (1.3 mg, 2.3 μmol) in MeOH (200 μL). The HPLC
system (Column 6) involved a linear gradient elution of Buffer A (0.1%
TFA in H2O) and Buffer B (0.1% TFA in CH3CN)
from 0 to 20% over 20 min (1% min–1), then 20 to
60% B to A over 40 min (0.5% min–1) and UV detection
at 214, 220, 254, 280, and 350 nm with a flow rate of 8 mL min–1. Fractions containing the desired compound were identified
by HPLC-MS, consolidated, and lyophilized to afford a white solid
(2.0 mg, ∼42%, assuming [ReO(HL(cRGDfK))2]CF3CO2).
HRMS (ESI+) m/z calc’d
for [ReC80H101N26O17S2]2+ 974.3419, found 974.3711, calc’d for
[ReC80H102N26O17S2]3+ 649.8972, found 650.0023; RP-HPLC (Column 2,
System A): RT (min) 12.9.
[ReO(HL(Tyr3-Oct))2]+
A solution of H2L(Tyr3-Oct) (9.0 mg, 7.1 μmol)
in MeOH (50 μL) was added to a mixture of (tBu4N)[ReOCl4] (2.1 mg, 3.5 μmol) and
MeOH (100 μL). The reaction mixture was shaken vigorously for
2 h. Milli-Q water was added (4 mL) and the reaction was filtered
(Millipore 0.45 μm porosity syringe filter). The compound was
purified by semipreparative RP-HPLC purification (Column 6) with a
gradient elution of Buffer A (0.1% TFA in H2O) and Buffer
B (0.1% TFA in CH3CN) from 10 to 80% B to A, over 70 min
(1.0% min–1) and UV detection at λ 214, 220,
and 254 nm, with a flow rate of 5 mL min–1. Fractions
containing the desired compound were identified by HPLC-MS, consolidated,
and lyophilized to afford a red, fluffy material (6.8 mg, ∼
68%, assuming [ReO(HL(Tyr3-Oct))2]CF3CO2). ESI-MS
(+) m/z calc’d
for [ReC116H148N28O27S6]2+ 1371.9470, found 1372.0024, calc’d for
[ReC116H149N28O27S6]3+ 914.9673, found 915.0145; RP-HPLC (Column 2,
System A): RT (min) 15.4.The same procedure was used as for [ReO(HL(Tyr3-Oct))2]+, except H2L(Tyr3-Oct) was replaced with H2L(Tyr3-Oct) (8.0 mg, 6.2
μmol) in MeOH (200 μL) and other reagent quantities were
adapted accordingly: (tBu4N)[ReOCl4] (1.8 mg, 3.1 μmol) in MeOH (100 μL). The compound
was purified by semipreparative RP-HPLC (Column 6) with isocratic
elution of Buffer A (0.1% TFA in H2O) and Buffer B (0.1%
TFA in CH3CN) at 38% Buffer B, over 60 min (1.0% min–1) and UV detection at λ 214, 220, and 254 nm,
with a flow rate of 4 mL min–1. Fractions containing
the desired compound were consolidated and lyophilized to afford a
red, fluffy material (5.5 mg, ∼61%, assuming [ReO(H(Tyr3-Oct))2]CF3CO2). ESI-MS
(+) m/z calc’d
for [ReC120H154N28O27S6]2+ 1399.9784, found 1399.4720, calc’d for
[ReC120H156N28O27S6]3+ 933.6548, found 933.6460; RP-HPLC (Column 2,
System A): RT (min) 16.2.Preloaded, resin-bound (Wang) ligand, H2L(Tyr3-Oct)
(approximately 6.0 μmol), was swollen in CH2Cl2 and drained twice. Anhydrous DMF (2 × 10 mL) was added
to the resin the mixture was stirred and drained. DMF (1 mL) was added
to the washed resin and (tBu4N)[ReOCl4] (2.1 mg, 2.9 μmol) in DMF (50 μL) was added
to the resin. The resin mixture was reacted for 2 h at RT. The solution
was drained and the resin was washed with copious amounts of DMF (5
× 10 mL), CH2Cl2 (3 × 10 mL), and
diethyl ether (10 mL). The crude material was cleaved off the resin
by addition of TFA/CH2Cl2/TIPS/H2O (50:46:1:3 v/v) (20 mL). The
mixture was shaken for 1.5 h and filtered and the filtrate sparged
with a stream of N2 until the red mixture had reduced to
approximately 0.5 mL. Diethyl ether (2 × 10 mL) was added to
the crude material, and the resulting precipitate was collected via
centrifugation (3 min, 3600 rpm). The compound was purified by semipreparative
RP-HPLC purification (Column 6) by gradient elution of Buffer A (0.1%
TFA in H2O) and Buffer B (0.1% TFA in CH3CN)
from 10 to 80% B to A, over 70 min (1.0% min–1)
and UV detection at λ 214, 220, and 254 nm, with a flow rate
of 4 mL min–1. Fractions containing the desired
compound were consolidated and lyophilized to afford a red, fluffy
material (5.0 mg, ∼58%, assuming [ReO(HL(Tyr3-Oct))2]CF3CO2). ESI-MS (+) m/z calc’d for [ReC124H148N28O27S6]2+ 1419.9470, found
1419.9281, calc’d for [ReC124H149N28O27S6]3+ 946.9673, found
946.1960; RP-HPLC (Column 2, System A): RT (min) 16.2.
Synthesis of [188ReO(HL(Tyr3-Oct))2]+
Rhenium-188 was produced from an ITG 188W/188Re generator (ITG Isotope Technologies, Garching,
Germany). Generator-produced 188ReO4– (86 MBq) in aqueous sodium chloride solution (200 μL, 0.9%
w/v) was added to a sealed, N2-purged vial containing sodium
tartrate (0.2 mg) and stannous chloride (0.1 mg) in water (400 μL),
followed by heating at 80 °C for 30 min. An aliquot of this solution
(50 μL) was added to a separate sealed, N2-purged
vial containing H2L(Tyr3-Oct) (100 μg) dissolved in water (100 μL).
The reaction was left for 30 min at ambient temperature, after which
an aliquot was removed for HPLC analysis, revealing that there was
no reaction between 188Re and peptide. The reaction vial
was then heated at 100 °C for 1 h, after which an aliquot was
analyzed by HPLC (column 1, system F). Radiochemical yield: 67%, retention
time of [188ReO(HL(Tyr3-Oct))2]+ = 11.6 min, compared
to retention time of [natReO(HL(Tyr3-Oct))2]+ = 11.3
min and H2L(Tyr3-Oct) = 9.7 min.
Synthesis of Technetium-99m
Complexes
Sodium pertechnetate, Na[99mTcO4] (1000 MBq), was eluted from a Gentech 99 Mo/99mTc sterile generator (Austin Health: Nuclear Medicine and
Centre for PET, Australia, via ANSTO Health) as a 1.0 mL saline solution
(0.9% v/v). A solution of SnCl2 in 0.1 M HCl (0.5 mg mL–1) was prepared
and purged with nitrogen. Disodium tartrate dihydrate was dissolved
in water (1 mg mL–1) in a separate evacuated vial,
and a 0.5 mL aliquot was taken from both solutions and mixed together.
To the solution was added [99mTcO4]− (0.1 mL in 0.9% saline, 108 MBq). The conjugated peptide, H2L(cRGDfK) or H2L(Tyr3-Oct), was dissolved in degassed Milli-Q
water (1 mg mL–1), and 100 μL of this mixture
was added to the technetium solution. The sample was neutralized with
NaHCO3 (pH 6.5, approximately 55 μL) then filtered
or allowed to react without neutralizing at ambient temperature for
30 to 120 min. The samples were filtered (Supelco, Iso-disc Filter,
4 mm x 0.45 μm). Radiochemical yields were evaluated by reverse-phase
high-performance liquid chromatography (Column 7, System C).
Stability
Studies in Human Serum
Human blood samples were centrifuged
with a Heraeus Labofuge 6000 centrifuge at 3000g for
10 min (Heraeus, Hanau, Germany). Radioactivity readings for serum
stability studies were taken with a Capintec CRC-35R dose calibrator
(Capintec, New Jersey, USA) and were measured in MBq. Centrifugation
of radioactive compounds was undertaken using an Eppendorf 5415 D
centrifuge (Eppendorf, Hamburg, Germany). Partition coefficient data
were collected with a PerkinElmer, Wizard 1470 (PerkinElmer, Massachusetts,
USA) automatic γ counter, which measured the radioactive decay
of each sample in counts per minute (cpm).For serum stability
studies, blood from a healthy male (20 mL) was centrifuged (10 min,
3000 rpm) to separate blood plasma and red blood cells. The plasma
was transferred to a separate vial and the red blood cells were discarded.
An aliquot of plasma (0.6 mL) was added to labeled compound, [99mTc(HL(Tyr3-Oct))2]+ (0.15 mL), the radioactivity was
monitored and the mixture was then incubated at 37 °C. Aliquots
(0.1 mL) of the mixture were removed from heating at 10 min and after
2 h. Acetonitrile (0.1 mL) was added to the serum/tracer mix to precipitate
serum proteins. The suspension was shaken for 5 min and then centrifuged
(5 min, 13 200 rpm). The radioactivity of the supernatant and pellet
was recorded. The supernatant (20 μL) was analyzed by analytical
RP-HPLC (Column 7, System C) for UV and radioactivity analysis and
the pellet were washed with acetonitrile (3 × 0.1 mL), and radioactivity
levels were again recorded (radioactivity levels of the pellet were
negligible).
Table 1
Selected Bond Lengths (Å) and Angles (deg) for
the Rhenium Complex for [ReO(HL(OMe))2]CF3CO2a
Bond Lengths
Re–O(1)
1.679(3)
Re–S(1)
2.2820(11)
Re–S(2)
2.2917(11)
N(1)–C(1)
1.350(6)
Re–N(1)
2.049(4)
Re–N(5)
2.050(4)
C(6)–N(3)
1.343(6)
N(1)–N(2)
1.422(5)
N(5)–N(6)
1.418(5)
C(14)–N(7)
1.350(6)
N(2)–C(6)
1.287(6)
N(6)–C(14)
1.287(6)
N(5)–C(9)
1.356(6)
C(6)–S(1)
1.784(5)
C(14)–S(2)
1.769(4)
Bond Angles
O(1)–Re–S(1)
115.44(11)
N(1)–Re–S(1)
80.74(11)
O(1)–Re–S(2)
116.75(11)
N(5)–Re–S(2)
80.23(11)
O(1)–Re–N(1)
101.73(15)
N(5)–Re–S(1)
89.71(11)
O(1)–Re–N(5)
102.61(15)
N(1)–Re–S(2)
87.98(11)
N(1)–Re–N(5)
155.64(15)
C(1)–N(1)–Re
125.0(3)
S(1)–Re–S(2)
127.80(4)
C(9)–N(5)–Re
126.2(3)
Torsion Angles
N(4)–C(1)–N(1)–Re
169.5(3)
N(6)–C(14)–N(7)–C(15)
13.8(7)
N(8)–C(9)–N(5)–Re
173.3(3)
N(2)–C(6)–N(3)–C(7)
5.1(7)
N(4)–C(1)–N(1)–N(2)
–10.5(6)
N(2)–C(6)–S(1)–Re
3.7(4)
N(8)–C(9)–N(5)–N(6)
–7.8(6)
N(6)–C(14)–S(2)–Re
4.1(4)
C(2)–C(1)–N(1)–N(2)
167.1(4)
N(3)–C(6)–S(1)–Re
–174.7(3)
C(10)–C(9)–N(5)–N(6)
168.4(4)
N(7)–C(14)–S(2)–Re
–175.1(3)
Trifluoroacetate
counterion bond lengths and angles are not provided.
Table 2
Summary of Crystal
Data and Structure Refinement for [ReO(HL(OMe))2]CF3CO2a
data collection
compound details
data collection
compound details
empirical formula
C20H26N8O5ReS2.H2O.CF3CO2
V (Å3)
1551.05(13)
formula weight
839.84
Z
2
crystal
size (mm3)
0.26 × 0.10 × 0.022
Dcalc. (Mg m–3)
1.797
crystal system
triclinic
μ (mm–1)
9.599
space group
P1̅
F(000)
828
T (K)
130.00(10)
reflections measured
10363
λ (Å)
1.54184
independent reflections
5568 [Rint = 0.0449]
a (Å)
10.9154(4)
final R indices [I > 2σ(I)]
R1 = 0.0329
b (Å)
11.1201(6)
wR(F2) = 0.0794
c (Å)
13.2651(7)
final R indices (all data)
R1 = 0.0398
α (deg)
86.355(4)
wR(F2) = 0.0831
β (deg)
74.965(4)
goodness-of fit on F2
1.027
γ (deg)
87.273(4)
Crystals were grown from a concentrated
solution of the complex in methanol.
Authors: Heather M Bigott-Hennkens; Shorouk F Dannoon; Samantha M Noll; Varyanna C Ruthengael; Silvia S Jurisson; Michael R Lewis Journal: Nucl Med Biol Date: 2010-12-03 Impact factor: 2.408
Authors: Michelle T Ma; Oliver C Neels; Delphine Denoyer; Peter Roselt; John A Karas; Denis B Scanlon; Jonathan M White; Rodney J Hicks; Paul S Donnelly Journal: Bioconjug Chem Date: 2011-09-27 Impact factor: 4.774
Authors: Clemens Decristoforo; Bluma Faintuch-Linkowski; Ana Rey; Elisabeth von Guggenberg; Marco Rupprich; Ignacio Hernandez-Gonzales; Teodoro Rodrigo; Roland Haubner Journal: Nucl Med Biol Date: 2006-11 Impact factor: 2.408
Authors: Cinzia Imberti; Samantha Y A Terry; Carleen Cullinane; Fiona Clarke; Georgina H Cornish; Nisha K Ramakrishnan; Peter Roselt; Andrew P Cope; Rodney J Hicks; Philip J Blower; Michelle T Ma Journal: Bioconjug Chem Date: 2016-12-14 Impact factor: 4.774
Authors: Scott P Fletcher; Asif Noor; James L Hickey; Catriona A McLean; Jonathan M White; Paul S Donnelly Journal: J Biol Inorg Chem Date: 2018-07-07 Impact factor: 3.358
Authors: Ingebjørg N Hungnes; Fahad Al-Salemee; Peter J Gawne; Thomas Eykyn; R Andrew Atkinson; Samantha Y A Terry; Fiona Clarke; Philip J Blower; Paul G Pringle; Michelle T Ma Journal: Dalton Trans Date: 2021-11-16 Impact factor: 4.390
Figure 1
Scheme 1
Scheme 2
Figure 2
Scheme 3
Scheme 4
Scheme 5
Scheme 6
Figure 3
Figure 4