Abstract
Single-photon emission computed tomography (SPECT) and position emission tomography (PET) are the two main imaging modalities in nuclear medicine. SPECT imaging is more widely available than PET imaging and the radionuclides used for SPECT are easier to prepare and usually have a longer half-life than those used for PET. In addition, SPECT is a less expensive technique than PET. Commonly used gamma emitters are: 99mTc (Emax 141 keV, T 1/2 6.02 h), 123I (Emax 529 keV, T 1/2 13.0 h) and 111In (Emax 245 keV, T 1/2 67.2 h). Compared to clinical SPECT, PET has a higher spatial resolution and the possibility to more accurately estimate the in vivo concentration of a tracer. In preclinical imaging, the situation is quite different. The resolution of microSPECT cameras (<0.5 mm) is higher than that of microPET cameras (>1.5 mm). In this report, studies on new radiolabelled tracers for SPECT imaging of angiogenesis in tumours are reviewed.
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Introduction
Angiogenesis, the formation of new blood vessels from pre-existing vasculature, is one of the key requirements if solid tumours are to grow beyond 2–3 mm3, since diffusion is no longer sufficient to supply the tissue with oxygen and nutrients [1]. Tumour-induced angiogenesis is a complex multistep process that follows a characteristic cascade of events mediated and controlled by growth factors, cellular receptors and adhesion molecules [2–4]. In this process, five phases can be distinguished: (1) endothelial cell activation, (2) basement membrane degradation, (3) endothelial cell migration, (4) vessel formation and (5) angiogenic remodelling [5].
The activation of pre-existing quiescent vessels can be triggered by hypoxia. Hypoxia induces the expression of hypoxia-inducible factor (HIF), which binds to the hypoxic response element. As a result, the expression of hypoxia-inducible genes, such as vascular endothelial growth factor (VEGF), carbonic anhydrase IX (CAIX), platelet-derived growth factor (PDGF) and transforming growth factor-α (TGF-α), is induced [6].
Activated endothelial cells express the dimeric transmembrane integrin αvβ3, which interacts with extracellular matrix proteins (vitronectin, tenascin, fibronectin, a.o.) and regulates migration of the endothelial cell through the extracellular matrix during vessel formation [7, 8]. The activated endothelial cells synthesize proteolytic enzymes, such as matrix metalloproteinases (MMPs), used to degrade the basement membrane and the extracellular matrix [9]. Initially, endothelial cells assemble as solid cords. Subsequently, the inner layer of endothelial cells undergoes apoptosis leading to the formation of the vessel lumen. Finally this primary, immature vasculature undergoes extensive remodelling during which the vessels are stabilized by pericytes and smooth muscle cells. This step is often incomplete in tumours resulting in the characteristic, increased permeability of tumour vessels.
Based on a balance between proangiogenic and antiangiogenic factors, a tumour can stay dormant for a very long time period until the so-called angiogenic switch occurs. In most tissues tumours can only grow to a life-threatening size if the tumour is able to trigger angiogenesis. In tissues with high vessel densities (e.g. liver, brain, a.o.), tumours may also progress via angiogenesis-independent co-option of the pre-existent vasculature [10].
In summary, tumour-induced angiogenesis is a multistep process and a key feature of a tumour lesion that has major impact on the biological behaviour of the lesion. Inhibition of angiogenesis is a new cancer treatment strategy that is now being widely investigated clinically. Researchers have begun to search for objective measures that indicate pharmacological responses to antiangiogenic drugs. Therefore, there is great interest in techniques to visualize angiogenesis in growing tumours non-invasively. During the past decade several markers of angiogenesis have been identified and specific tracers targeting these markers have been developed.
VEGF receptors
VEGF is a key regulator of angiogenesis during embryogenesis, skeletal growth and reproductive functions. The expression of VEGF is upregulated by environmental stress caused by hypoxia, anaemia, myocardial ischaemia and tumour progression to initiate neovascularization [11]. Via alternative mRNA splicing, the human VEGF-A gene gives rise to four isoforms having 121, 165, 189 and 206 amino acids (VEGF121, VEGF165, VEGF189 and VEGF206, respectively) [12, 13]. Less frequent splice variants have been identified more recently, including VEGF145 [14], VEGF183 [15], VEGF162 [16] and VEGF165b [17]. The VEGF isoforms differ not only in their molecular mass, but also in their solubility and receptor-binding characteristics.
Initially, VEGF receptors were identified on the cell surface of vascular endothelial cells in vitro [18, 19] and in vivo [20, 21]. Subsequently, it was demonstrated that receptors for VEGF also are expressed on bone marrow-derived cells such as monocytes [22]. VEGF-A binds two related receptor tyrosine kinases (RTKs), VEGFR-1 and VEGFR-2. Both receptors consist of seven Ig-like domains in the extracellular domain, a single transmembrane region and a consensus tyrosine kinase sequence that is interrupted by a kinase insert domain [23–25]. VEGFR-1 binds VEGF with a higher affinity compared to VEGFR-2 (Kd: 25 vs 75–250 pM) [26–28]. VEGFR-1 is considered to be a decoy receptor and VEGF-A only signals through VEGFR-2 [29].
SPECT imaging of VEGF receptors
Two VEGF isoforms, VEGF121 and VEGF165, have been investigated for their potential to visualize VEGFR expression by SPECT. VEGF121 and VEGF165 were radioiodinated with 123I and the binding properties of 123I-VEGF121 and 123I-VEGF165 to human umbilical vein endothelial cells, various human tumour cell lines and a variety of primary human tumours were determined [30].These studies showed that 123I-VEGF121 and 123I-VEGF165 specifically bound to various tumour cell types. In comparison with 123I-VEGF121, 123I-VEGF165 bound to a higher number of different tumour cell types with a higher capacity. In a subsequent preliminary clinical study, 123I-VEGF165 appeared to be safe and 123I-VEGF165 visualized gastrointestinal tumours and metastasis expressing VEGF receptors [31]. Although CT/MRI was superior compared to 123I-VEGF165 scintigraphy in a lesion-by-lesion comparison, the authors concluded that 123I-VEGF165 might be useful for visualization of tumour angiogenesis.
In another clinical study, the biodistribution, safety and absorbed dose of 123I-VEGF165 in patients with pancreatic carcinoma were investigated [32]. A majority of primary pancreatic tumours and their metastases were visualized at 3 h after 123I-VEGF165 administration.
In order to develop non-invasive, specific techniques to estimate tumour vascularity, Yoshimoto and co-workers evaluated 125I-VEGF121 and 125I-VEGF165 as angiogenesis imaging agents in mice with LS180 tumours [33]. 125I-VEGF121 displayed significantly higher tumour uptake and higher tumour to non-tumour (T/N) ratios as compared to 125I-VEGF165. The tumour accumulation of 125I-VEGF121 decreased with increasing tumour volume. However, in this study it was not investigated whether the uptake of 125I-VEGF121 and 125I-VEGF165 in the tumour and other organs and tissues was VEGF receptor-mediated.
Besides radioiodinated VEGF-based isoforms, also VEGF-based isoforms labelled with radiometals such as 99mTc and 111In have been investigated. Blankenberg and co-workers described a novel imaging complex comprised of a standardized 99mTc-radiolabelled adapter protein non-covalently bound to a “docking tag” fused to a “targeting protein”. The assembly of this complex was based on interactions between human 109-amino acid (HuS) and 15-amino acid (Hu-tag) fragments of ribonuclease I, which served as an “adapter protein” and a docking tag, respectively. The resulting 99mTc-HuS/Hu-VEGF complex could be effectively used to image the murine tumour neovasculature in lesions as small as a few millimetres in soft tissue in mice with 4T1-luc tumours [34]. In the same animal model, the HYNIC-conjugated 99mTc-HYNIC-VEGF had a similar biodistribution as the 99mTc-HuS/Hu-VEGF complex. SPECT imaging using 99mTc-HYNIC-VEGF showed highly heterogeneous focal accumulation in the tumour area. SPECT imaging with 99mTc-HYNIC-VEGF could also readily detect the effects of chemotherapeutic treatment of 4T1 tumours [35]. Binding specificity was confirmed by the 75% decrease in tumour uptake of 99mTc-biotin-inactivated VEGF, as compared to 99mTc-HYNIC-VEGF.
Chan et al. synthesized a recombinant protein VEGF composed of VEGF165 fused through a flexible polypeptide linker (GGGGS)3 to the n-lobe of human transferrin (hnTf) for imaging angiogenesis [36]. The VEGF construct was conjugated to the n-lobe of hnTf to allow labelling with 111In at a site remote from the VEGF receptor-binding domain. 111In-hnTf-VEGF accumulated in U87MG glioblastoma xenografts [6.7%ID/g, 72 h post-injection (p.i.)] in athymic mice and its tumour uptake decreased 15-fold by coadministration of a 100-fold excess VEGF, indicating that the tracer specifically accumulated in U87MG tumours.
The studies described above were all done with VEGF isoforms. Alternatively, studies with radiolabelled anti-VEGF antibodies and derivatives thereof have also been reported. Bevacizumab is a humanized variant of the anti-VEGF-A monoclonal antibody (mAb) A.4.6.1. It is directed against a common epitope encoded by exon 4, present on all VEGF isoforms, and prevents interaction of VEGF with VEGFR-1 and VEGFR-2 [37]. Nagengast et al. were the first to demonstrate non-invasive VEGF imaging using radiolabelled bevacizumab. In their study, they demonstrated the potential of 89Zr-bevacizumab and 111In-bevacizumab as a specific VEGF tracer in nude mice with human SKOV-3 ovarian tumour xenografts [38]. At the same time, our group showed specific imaging of VEGF-A expression using 111In-bevacizumab in mice with s.c. human colon carcinoma xenografts LS174T [39]. We were the first to investigate the potential of 111In-labelled bevacizumab to image the expression of VEGF-A in tumours in cancer patients. In a study in colorectal cancer patients with liver metastases, the liver metastases in 9 of 12 patients were visualized with 111In-bevacizumab (Fig. 1). In this study, the liver metastases were resected after scintigraphic imaging allowing further immunohistochemical analysis. The VEGF-A expression in these resected liver metastases was determined by in situ hybridization and by measuring VEGF in tumour extracts by enzyme-linked immunosorbent assay (ELISA). Surprisingly, no correlation was found between the level of antibody accumulation and the level of VEGF-A expression.
In a preclinical study, the biodistribution of 111In-labelled bevacizumab and 111In-labelled ranibizumab, an anti-VEGF Fab fragment, were compared in nude mice with SKOV-3 ovarian tumours. Although bevacizumab showed the highest tumour uptake, ranibizumab allowed imaging earlier after injection of the tracer, making the Fab fragment tracer more suited to monitor rapid changes of VEGF expression following therapy. SPECT imaging using 111In-labelled bevacizumab revealed tumour lesions in both melanoma and metastatic colon cancer patients [40].
αvβ3 integrin receptor
The αvβ3 integrin, also referred to as the vitronectin receptor, belongs to the integrin receptors. Integrins are a family of heterodimeric transmembrane glycoproteins that function in cellular adhesion, migration and signal transduction. Each member of this family consists of two non-covalently bound transmembrane polypeptide subunits, alpha and beta.
Activated endothelial cells express the integrin αvβ3 receptor, whereas this integrin receptor is absent on quiescent endothelial cells. In addition, αvβ3 is expressed on the cell membrane of various tumour cell types such as: ovarian cancer, neuroblastoma, breast cancer, melanoma, a.o. αvβ3 Integrin expressed on endothelial cells modulates cell migration and survival during angiogenesis, whereas αvβ3 integrin expressed on carcinoma cells potentiates metastasis by facilitating invasion and movement across blood vessels. Due to this restricted expression of αvβ3 in tumours, αvβ3 is considered a suitable target for imaging angiogenesis [41]. Radiolabelled ligands for this integrin can be used as tracers to non-invasively visualize αvβ3 expression in tumours. Non-invasive visualization of αvβ3 expression might provide information about the angiogenic process and the responsiveness of a tumour to antiangiogenic drugs.
SPECT imaging of αvβ3 expression
Integrin αvβ3 binds extracellular matrix proteins (e.g. vitronectin, fibrinogen, laminin, collagen) through exposed tripeptide arginine-glycine-aspartic acid (RGD) amino acid moieties [42]. Several research groups have investigated the potential of RGD-containing peptides to target αvβ3 expressed in tumours with radionuclides. It was found that the cyclic pentapeptide cyclo(Arg-Gly-Asp-D-Phe-Val), having an IC50 value in the lower nanomolar range, was a 100-fold better inhibitor of cell adhesion to vitronectin compared to the linear variant [43, 44]. It was found that besides the essential RGD sequence, a hydrophobic amino acid in position 4 increases the affinity for αvβ3 [45]. Based on this finding Haubner and co-workers designed five peptides that could be radioiodinated by introducing a tyrosine residue. Two of these peptides, cyclo(Arg-Gly-Asp-D-Tyr-Val) and cyclo(Arg-Gly-Asp-D-Phe-Tyr) (designated as P1 and P4, respectively) were studied in vivo [46]. The biodistribution of the radioiodinated peptides was studied in nude mice with various s.c. human tumours (M21 melanoma, MaCaF mammary carcinoma and osteosarcoma). The peptides rapidly cleared from the blood (<1%ID/g at 10 min p.i.). In the M21 melanoma model, the tumour uptake peaked at 10 min p.i. (1.12 ± 0.98%ID/g) and decreased to 0.12 ± 0.04%ID/g at 2 h p.i. However, both peptides cleared via the hepatobiliary route and revealed relatively high hepatic uptake, especially at early time points (∼5%ID/g, 1 h p.i.). Therefore, the pharmacokinetics of these RGD peptides were improved by conjugating them with sugar amino acids. A glucose-based sugar amino acid (SAA1) was conjugated to the epsilon-amino function of lysine in the pentapeptide. Compared to the non-carbohydrate radioiodinated P4, the resulting iodine-labelled glycopeptide 3-[*I]iodo-D-Tyr4-cyclo(Arg-Gly-Asp-D-Tyr-Lys (SAA1)) (*I-gluco-RGD) showed reduced activity accumulation in the liver, enhanced blood levels and increased uptake and retention in the tumour [47]. Based on these data a galactose-based sugar amino acid (SAA2) was conjugated with cyclo(Arg-Gly-Asp-D-Phe-Lys) allowing prosthetic group labelling [47, 48].
van Hagen and co-workers conjugated a DTPA moiety via the epsilon group of the lysine residue in the cyclic pentapeptide cyclo(Arg-Gly-Asp-D-Tyr-Lys). The resulting ligand could be radiolabelled with both 111In and radioiodine. The radiolabelled peptide bound specifically to αvβ3-positive cells. DTPA conjugation made the peptide more hydrophilic and facilitated renal clearance, in contrast to the non-DTPA-conjugated radioiodinated peptide which cleared predominantly via the hepatobiliary route [49].
An alternative lead structure compared to the head-to-tail cyclized RGD-containing pentapeptide is the disulphide-bridged RGD-4C (Cys2-Cys10, Cys4-Cys8) H-Ala-Cys-Asp-Cys-Arg-Gly-Asp-Cys-Phe-Cys-Gly-OH which binds with high affinity to both αvβ3 and αvβ5 (KD ∼ 100 nM) [50]. Its derivative (Cys1-Cys9, Cys3-Cys7) H-Cys-Asp-Cys-Arg-Gly-Asp-Cys-Phe-Cys-OH was conjugated with HYNIC and subsequently radiolabelled with 99mTc. In in vivo studies, this 99mTc-HYNIC-RGD had marginal tumour uptake in mice with αvβ3-positive tumours [51, 52]. The deletion of the terminal amino acids, the conjugation with HYNIC and/or the labelling with 99mTc could have impaired the affinity of the peptide for the receptor.
Clinical studies
Sivolapenko and colleagues were the first who investigated the synthetic linear RGD analogue αP2 (Arg-Gly-Asp-Ser-Cys-Arg-Gly-Asp-Ser-Tyr) to image tumour angiogenesis in patients [53, 54]. Fourteen melanoma patients received 185–1222 MBq of the 99mTc-labelled peptide intravenously (i.v.) and were imaged up to 3 h p.i. The peptide cleared rapidly from the blood (T 1/2α = 5.5 ± 2.2 min and T 1/2β = 34.3 ± 11.0 min) by filtration through the kidneys and excretion in the urine (>90%ID in kidneys and bladder at 1 h p.i.). Of the 22 metastatic lesions in these patients, 17 were visualized.
The 99mTc-labelled RGD-containing peptide (NC100692, Fig. 2) was evaluated in ischaemic models and showed high uptake in areas of neovascularization with αvβ3 integrin overexpression [55]. In these models it was shown that NC100692 bound to αvβ3-expressing endothelial cells in regions of angiogenesis [56].
Subsequently, 99mTc-NC100692 was tested in women with histologically proven breast cancer. 99mTc-NC100692 detected malignant breast tumours efficiently [57]. Of 20 malignant tumours, 19 were detected and there were no safety concerns related to the administration of 99mTc-NC100692 [58].
To determine the feasibility of detecting metastatic lesions in liver, lung, bone and brain with scintigraphy, 99mTc-NC100692 was used in an open-label, multicentre, phase 2a study in late-stage cancer patients [59]. Therefore, 25 patients, 15 with lung cancer and 10 with breast cancer, were recruited at 10 centres. In patients with breast cancer, 99mTc-NC100692 scintigraphy detected 1 of 7 liver, 4 of 5 lung, 8 of 17 bone and 1 of 1 brain metastases. The corresponding numbers in lung cancer patients were 0 of 2, 17 of 18, 2 of 2 and 7 of 9. Despite the low number of patients with liver metastases included in this study, the authors concluded that the sensitivity to detect liver metastases was poor and the detection of bone metastases is equivocal with 99mTc-NC100692. However, it was feasible to detect lung and brain metastases from breast and lung cancer.
Multivalent cyclo(RGD) peptides
To improve tumour targeting and to obtain better in vivo imaging properties, several research groups aimed to enhance the affinity toward the αvβ3 integrin by using multimeric RGD peptides. Janssen et al. conjugated two cyclo(RGDfK) peptides via a glutamic acid linker, conjugated it with HYNIC and radiolabelled it with 99mTc. The dimeric 99mTc-HYNIC-E-[c(RGDfK)]2 showed a tenfold higher affinity for αvβ3 and a better retention than the monomeric 99mTc-HYNIC-E-c(RGDfK) [60]. However, the dimer also had higher uptake in the kidneys. Possibly, the presence of more guanidine groups in the dimer caused the enhanced renal uptake [61].
In another study, the tumour targeting potential of both a 111In- and 99mTc-labelled dimeric RGD peptide derivatized with the chelators DOTA or HYNIC, respectively, was investigated in mice with s.c. NIH:OVCAR-3 tumours [62]. Tumour uptake peaked at 7.5%ID/g for 111In-DOTA-E-[c(RGDfK)]2 (2 h p.i.) and 6.0%ID/g for 99mTc-HYNIC-E-[c(RGDfK)]2 (1 h p.i.).
The multivalency effect was further explored by the synthesis of the DOTA-conjugated tetrameric analogue E{E[c(RGDfK)]2}2 [63]. The in vitro affinity and the in vivo tumour targeting characteristics of the 111In-labelled mono-, di- and tetramer to αvβ3-expressing tumours were determined (IC50 values; monomer: 120 nM, dimer: 69.9 nM and tetramer: 19.6 nM). The tetramer showed improved tumour targeting (7.40 ± 1.12%ID/g) compared to the dimer (5.17 ± 1.22%ID/g at 8 h p.i.). Analogously, the dimer demonstrated improved tumour targeting compared to the monomer (2.30 ± 0.34%ID/g at 8 h p.i., Fig. 3).
The application of dimers and tetramers as SPECT radiotracers by tethering together c(RGDfK) units via a glutamic acid tree has been studied extensively. Recently, a variety of c(RGDfK) multimers assembled via the RAFT template [64] or click chemistry [65] was studied as well. In all of the multimeric RGD studies described above, it was found that multimerization of cyclic RGD peptides enhanced their integrin αvβ3-binding affinity and improved the tumour uptake of the radiotracer. However, the uptake of the radiotracers in kidney and liver also increased significantly as the peptide multiplicity increased. In addition, the synthesis of the c(RGDxK)-based tetra- and octamers (x = f or y) is much more complicated and could limit their introduction into clinical practice.
In general, there are two main factors that contribute to a higher αvβ3-binding affinity of multimeric RGD peptides compared to their monomeric counterparts: (1) simultaneous αvβ3 integrin binding by two RGD motifs or (2) the locally enriched RGD concentration. To achieve simultaneous integrin αvβ3 binding (=multivalency), the distance between the RGD motifs in multimeric RGD peptides must be long enough and flexible enough. There are some disadvantages of using tetra- or octameric RGD peptides over their dimeric counterparts, such as the more complicated synthesis and higher uptake in non-target organs. To solve these problems, pharmacokinetic modifier (PKM) linkers between the two RGD motifs in dimeric RGD peptides have been tested in several studies.
In an attempt to increase the affinity of E[c(RGDfK)]2, Shi and co-workers developed a series of cyclic RGD dimers containing triglycine (G3) and PEG4 linkers, which were used to increase the distance between two cyclic RGD units from 6 bonds in E[c(RGDfK)]2 to 24 bonds in 3G3-dimer and 38 bonds in 3PEG4-dimer [66, 67]. In in vitro binding studies on U87MG human glioma cells, the linker-containing dimers HYNIC-3PEG4-dimer (IC50 = 60 ± 4 nM) and HYNIC-3G3-dimer (IC50 = 61 ± 2 nM) had a higher affinity than HYNIC-PEG4-dimer (IC50 = 84 ± 7 nM), which had a short linker between the RGD units. The HYNIC-tetramer had a higher binding affinity (IC50 = 7 ± 2 nM) probably due to its two extra RGD units. In mice with s.c. U87MG glioma and MDA-MB-435 breast tumour xenografts, the tumour uptake of 99mTc-HYNIC-3PEG4-dimer and 99mTc-HYNIC-3G3-dimer was similar to that of the 99mTc-HYNIC-tetramer, indicating divalent binding of the three tracers. The tumour uptake of the 99mTc-HYNIC-PEG4-dimer was much lower, suggesting monovalent binding. Furthermore, 99mTc-HYNIC-3PEG4-dimer and 99mTc-HYNIC-3G3-dimer had kidney and liver uptake that was half of that of the 99mTc-HYNIC-tetramer. In a subsequent study, 111In-DOTA-3PEG4-dimer, 111In-DTPA-3PEG4-dimer and 111In-DTPA-Bn-3PEG4-dimer were synthesized and compared in in vitro and in vivo studies [68]. The affinities were 1.3 ± 0.2, 1.4 ± 0.3 and 1.3 ± 0.3 nM, respectively. In mice with s.c. U87MG glioma xenografts, all three radiotracers had a high tumour uptake and excellent tumour to background (T/B) ratios up to 4 h p.i. After that time point, both DTPA-conjugated derivatives showed a much faster tumour washout and poorer T/B ratios than the DOTA-conjugated derivative.
So far, 3PEG4-dimer and 3G3-dimer seem suitable candidates for SPECT imaging of angiogenesis in clinical studies.
Extracellular matrix proteins
A few antigens in the extracellular matrix (ECM) have been identified that are preferentially expressed in the surroundings of newly formed blood vessels, such as fibronectin, laminin, tenascin and collagen type IV. A series of SPECT tracers targeting the extra domain B of fibronectin for imaging tumour angiogenesis have been developed
Extra domain B of fibronectin
Fibronectin is a large glycoprotein in the ECM. The extra domain B (ED-B) of fibronectin is a sequence of 91 amino acids, identical in mice, rats and humans, that is inserted into the fibronectin molecule at sites of tissue remodelling due to alternative splicing. ED-B is specifically expressed around neovascular structures in tumours and other tissues undergoing angiogenesis, but is undetectable in normal adult tissues. Using phage display technology, single-chain antibodies (scFv) directed against ED-B have been isolated. The human single domain antibody (scFv) L19 was shown to have subnanomolar affinity for ED-B [69].
Demartis et al. showed that radioiodinated scFv L19 selectively accumulated around tumoural blood vessels in a murine tumour model. Since the ED-B domain of fibronectin has an identical sequence in mouse and man, they suggested clinical utility for the scintigraphic detection of angiogenesis in vivo [70]. Two years later, it was shown by scintigraphic imaging that 123I-L19 selectively localized in tumour lesions of aggressive lung cancer as well as in liver metastases of colorectal cancer patients [71]. More recently, the amino acid sequence (Gly)3-Cys-Ala was inserted at the C terminus of L19, resulting in the anti-ED-B scFv named AP39, which could be labelled with 99mTc. The data revealed the feasibility of targeting ED-B fibronectin with 99mTc-labelled L19 in nude mice with s.c. teratocarcinoma tumours [72].
Subsequently a series of different L19 antibody formats were constructed, including dimeric scFv, a human bivalent “small immunoprotein” (SIP) and a complete human IgG. In comparing these different formats labelled with 125I/131I, L19-SIP proved to be the most suitable tracer for imaging ED-B expression in tumours.
Prostate-specific membrane antigen
Prostate-specific membrane antigen (PSMA) is a transmembrane protein which is overexpressed in prostate cancer. The anti-PSMA antibody, capromab pendetide, labelled with 111In is marketed as ProstaScint®, an antibody preparation approved by the US Food and Drug Administration (FDA) for the detection of nodal metastases in prostate cancer patients [73]. However, this antibody is directed against an intracellular epitope of PSMA, which is considered a suboptimal target for antibody imaging. PSMA was also found to be expressed on the neovascular endothelium of most solid tumour types, while there is no expression on the endothelial cells of normal tissue [74].
J591 is a monoclonal antibody directed against an epitope on the extracellular domain of PSMA [75]. Previous studies have shown that J591 accumulated in metastatic prostate cancer lesions [76]. In a recent phase I trial the feasibility of targeting the neovasculature of a wide range of adenocarcinomas using 111In-labelled humanized J591 was investigated. Patients with melanoma and cancers of the breast, colon, liver and kidney received 111In-J591. In these patients (n = 24) the antibody accreted in all known tumour sites. Of 18 patients with soft tissue disease on standard scans, 17 (94%) showed uptake in the soft tissues on antibody scans as did 6 of 6 patients with bone disease. These data show selective targeting of PSMA expressed on tumour endothelium [77]. 111In-huJ591 has the potential to become a suitable tracer for imaging angiogenesis.
Conclusions
In the last few years, significant progress has been made in the development of SPECT tracers (peptides, proteins and antibodies) for the non-invasive imaging of tumour angiogenesis. These tracers might have the potential to select patients who might benefit from treatment with antiangiogenic drugs and these tracers might also be used to therapeutic effect with these antiangiogenic drugs. Small animal SPECT cameras have a higher resolution than microPET cameras and in the clinical situation the difference in resolution is marginal. PET isotopes are more expensive than SPECT isotopes and single photon agents can provide more specific targeting abilities than PET agents, by enabling dual-tracer imaging, which is still unique to SPECT.
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Dijkgraaf, I., Boerman, O.C. Molecular imaging of angiogenesis with SPECT. Eur J Nucl Med Mol Imaging 37 (Suppl 1), 104–113 (2010). https://doi.org/10.1007/s00259-010-1499-9
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DOI: https://doi.org/10.1007/s00259-010-1499-9