Introduction
Overexpression of human epidermal growth factor receptor-2 (HER2) enhances signal transduction through the PI3K/Akt and the Ras/Raf/MEK/MAPK pathways, enabling cancer cell proliferation and survival [
1]. HER2 is overexpressed in 20 – 25 % of patients with breast cancer and gastrooesophageal cancer, and in these cancers HER2 is an established therapeutic target [
2,
3]. There are a range of HER2-targeted therapies, including the monoclonal antibody trastuzumab, licensed for the treatment of breast and gastric cancers, and the trastuzumab–drug conjugate, T-DM1, licensed for the treatment of breast cancer [
3,
4]. Novel therapies targeting the HER2 receptor, downstream effectors and compensatory signalling pathways are in clinical development [
1].
Currently, patients are selected for anti-HER2 therapy based on histological analysis, using immunohistochemistry or fluorescence in situ hybridization (FISH) of biopsied or surgically resected tissues [
5]. These analyses are limited by the use of single-site and single time-point sampling, and furthermore they fail to provide information about heterogeneity of expression or changes in expression that occur over time [
6]. Dependence on histological analyses risks misclassifying patients’ HER2 status and selecting a suboptimal therapy. Discordance in HER2 status between the primary breast tumour and synchronous as well as metachronous metastases has consistently been reported [
7]. HER2 status has also been reported to change, from negative to positive and vice versa, and also between metastatic disease relapses [
8,
9]. Although the impact of HER2 misclassification on clinical outcomes is unclear, 20 – 30 % of patients with HER2-positive advanced breast cancer do not respond to first-line treatment combinations, despite advances in anti-HER2 therapies [
10]. In the adjuvant setting, some patients with breast cancer histologically classified as HER2-negative benefit from adjuvant anti-HER2 therapy, casting doubt on their classification [
11].
HER2 molecular imaging could potentially overcome the limitations of histological analysis by providing new information on HER2 expression at all metastatic sites. Radiolabelled trastuzumab has been used for this purpose, but although the pharmacokinetics of trastuzumab are well suited to therapy, its long half-life compromises tumour-to-blood ratios needed for imaging. Consequently, HER2 scans must be performed at least 2 days after radiolabelled trastuzumab administration, and even then tumours in highly vascular regions may be difficult to visualize [
12]. In clinical studies, SPECT imaging with
111In-trastuzumab and PET imaging with both
64Cu-trastuzumab and
89Zr-trastuzumab have shown lower rates of tumour detection in patients with advanced HER2-positive breast cancer than conventional imaging, including CT [
12‐
14]. Therefore, a novel approach is needed to overcome these limitations, potentially utilizing low molecular weight high-affinity proteins [
15].
Designed ankyrin repeat proteins (DARPins) are recombinant binding proteins composed of ankyrin repeats, which stack together to make a contiguous binding surface [
16,
17]. Each ankyrin repeat consists of 33 amino acids, which form a β-turn followed by two anti-parallel α-helices and a loop binding to the β-turn of the next ankyrin repeat [
18,
19]. Synthetic DARPin libraries have been designed [
18], from which specific binders can be selected and further evolved by methods such as ribosome display [
20].
The DARPin G3 is a low molecular weight protein (14 – 15 kDa) with picomolar affinity (91 pmol/L) for HER2 [
21‐
23]. It has a short half-life in mice (<3 min), lacks biological activity and binds to HER2 in the presence of trastuzumab and pertuzumab in vitro [
21,
23]. The DARPin G3 tagged with hexahistidine (His
6) and labelled with
99mTc-tricarbonyl ([
99mTc(CO)
3]
+) can be used to visualize HER2-positive tumours [
21]. Our goal was to use the DARPin G3 for routine clinical HER2 SPECT and PET imaging, and we set out to generate and evaluate different radiolabelled G3 formats to select a lead for clinical development.
The His
6 tag can be employed for purification of recombinant proteins by immobilized metal affinity chromatography (IMAC). We evaluated the effect of the His
6 tag on DARPin G3 biodistribution and compared it with the DARPin G3 tagged with histidine glutamate (HE)
3, which has a negative excess charge at physiological pH. The (HE)
3 tag has been reported to reduce background liver uptake in some cases, while still allowing tag-mediated IMAC [
24,
25]. We developed a GMP-compatible
Pichia pastoris production platform that allows cleavage of histidine-based tags after IMAC purification, enabling comparisons among variants of G3.
We hypothesized that the DARPin G3 would be capable of selectively imaging HER2-positive tumours and aimed to identify a suitable format for clinical application. Thus, we systematically investigated the effect of tag and label on the quality of imaging. First, we assessed the sensitivity and specificity of DARPin G3 radiolabelled with [99mTc(CO)3]+ via a His6 tag in HER2-positive and HER2-negative tumour-bearing mice. Subsequently, we assessed the biodistribution of His6-G3, (HE)3-G3 and untagged G3 DARPins radiolabelled with 111In and 125I in non-tumour-bearing mice. Thus, both residualizing and non-residualizing radioisotopes were tested, as they have different cellular fates which can affect tumour-to-normal tissue ratios. Finally, the construct with the lowest normal tissue uptake was taken forward for evaluation as an imaging agent.
Materials and methods
Details of DARPin G3 constructs (Supplementary Fig.
1), production, purification, conjugation with 1,4,7,10-tetraazacyclododecane-1,4,7-Tris-acetic acid-10-maleimidoethylacetamide (mal-DOTA) and radiolabelling are provided in the
Supplementary Materials and methods.
DARPin G3 radiolabelling
DOTA-conjugated DARPins (5 – 60 μg) in 0.2 M ammonium acetate, pH 6.5, were mixed with a solution of 111InCl3 (Covidien, The Netherlands; 10 – 30 MBq) and incubated for 2 h at 37 °C (reaction volumes 40 – 60 μl). The reactions were stopped by adding 0.1 M disodium edetate (EDTA) and the radiolabelled DARPins were purified by elution into PBS using a NAP-5 column (GE Healthcare, Little Chalfont, UK) pre-equilibrated with PBS. Radiochemical purity was determined using instant thin-layer chromatography (iTLC), using iTLC silica gel (SG) strips (Varian, Palo Alto, CA). To test for 111In-EDTA, iTLC strips were eluted with 0.1 M ammonium acetate containing 25 mM EDTA (final pH 5.5) in which system 111In-EDTA eluted to the solvent front, while 111In-G3 DARPin and insoluble material remained at the origin. Formation of radioactive insoluble material was evaluated using iTLC-SG eluted with 35 % ammonia (v/v)/ethanol/water (1:2:5), in which system 111In-DOTA-G3 DARPin and 111In-EDTA both had Rf values >0.5, while any insoluble material present in the reaction mixture remained at the origin. If insoluble material was detected, reaction mixtures were filtered through a 0.2-μm sterile syringe filter with a Supor membrane (Pall Life Science, Portsmouth, UK). The radiochemical purity of 111In-G3 DARPins was 70 – 80 % before purification and >95 % after purification (see below for specific activities, SA).
Iodine radiolabelling was performed in precoated Pierce iodination tubes (Thermo Scientific, Runcorn, UK) with unconjugated G3 DARPins (5 – 60 μg) in PBS for 10 min at room temperature, using either 10 MBq 125I (PerkinElmer, Llantrisant, UK) or 15 – 20 MBq 123I (GE Healthcare). The iodination reactions were stopped by adding sodium metabisulphite to a final concentration of 1 μM. Radioiodinated DARPins were purified by buffer exchange into PBS with a NAP-5 column. Radiochemical purity was assessed with iTLC-SG strips (Varian) using 0.1 M ammonium acetate containing 25 mM disodium EDTA (final pH 5.5) as 123/125I-G3 DARPin remained at the origin and free 123/125I eluted at the solvent front. Radiochemical purity increased from 60 – 70 % before purification to >95 % after purification (see below for SA). An equivalent molar amount of ‘cold’ potassium iodide (3.4 × 10−10 mol) was coadministered with 123I-G3 DARPin to minimize normal tissue uptake of ‘free’ 123I (formed by deiodination in vivo).
iTLC analysis was supplemented with size-exclusion high-performance liquid chromatography (HPLC). A Beckman System Gold 128 solvent module and a 168 UV detector module (monitoring at 280 and 220 nm; Beckman Coulter, High Wycombe, UK), combined with a Raytest GABi radiochemical detector (Raytest, Straubenhardt, Germany) were used. The radiolabelled DARPin G3 was eluted from a YMC-Pack Diol-60 (YMC Europe, Dinslaken, Germany) column, dimensions 300 mm length × 8.0 mm inner diameter, spherical shape, 5 μm particle size and 6 nm pore size, using a mobile phase of 0.2 M phosphate buffer (pH 6.8) at a flow rate of 0.5 ml/min.
In vitro assessment
The unconjugated and DOTA-conjugated G3 counterparts had comparable subnanomolar binding affinities for the HER2 extracellular domain (ECD) assessed by surface plasmon resonance, indicating that DOTA conjugation to the C-terminus does not compromise binding to HER2 (data not shown). Saturation binding assays of radiolabelled DARPin G3 were performed with BT474 HER2-expressing human breast cancer cells (ATCC, Manassas, VA) as previously described [
26]. On BT474 cell-binding assays,
111In-(HE)
3-G3 and
125I-(HE)
3-G3 had saturable binding and similar binding affinities to each other.
To assess stability of the label, aliquots of radiolabelled DARPin G3 were incubated in PBS or in human serum/PBS (1:1). Serum stability was assessed at 37 °C for 24 h, while PBS stability was assessed at 4, 20 and 37 °C for 24 h after radiolabelling by iTLC, as previously outlined. After incubation, the stability of radiolabelled G3 was assessed by SDS-PAGE using non-reducing conditions, followed by autoradiography using a Cyclone storage phosphor system (PerkinElmer).
Biodistribution studies
All animal studies were ethically reviewed and performed in accordance with the UK Animals (Scientific Procedures) Act 1986, UK Home Office regulations and local regulations.
For non-tumour studies, female BALB/c mice (Charles River, Erkrath, Germany) aged 6 – 11 weeks (mean weight 19 g) received an intravenous dose of 0.3 MBq of 111In-G3 DARPin (2.2 μg, SA 2.0 MBq/nmol, to 4.3 μg, SA 1 MBq/nmol) or 125I-G3 DARPin (2.8 μg, SA 1.6 MBq/nmol, to 4.3 μg, SA 1 MBq/nmol) in 200 μl of PBS/0.1 % BSA. Mice were killed at 4 h (four mice) or 24 h (four mice) after administration. Tissues were removed and radioactivity measured in a gamma counter (1282 CompuGamma CS, LKB Wallac). Uptakes are expressed as means ± SD of the percentage of injected radioactive dose per gram of tissue (% ID/g).
For tumour studies, a single 60-day release 0.72-mg 17β-oestradiol pellet (Innovative Research of America, Sarasota, FL) was inserted into the scruff of female SCID-beige mice (Charles River) aged 6 – 8 weeks (mean weight 17 g). The following day, the mice were inoculated with BT474 cells by subcutaneous injection (7.5 × 10
6 cells; ATCC) in PBS mixed with equal volumes of Matrigel (BD Biosciences, Oxford, UK). When tumours reached 25 – 100 mm
2 (5 – 7 weeks after inoculation) the mice received 0.3 MBq of
111In-G3 DARPin (2 μg, SA 2.2 MBq/nmol) or 0.3 MBq of
125I-G3 DARPin (3 μg, SA 1.5 MBq/nmol) and biodistribution was calculated as outlined. Excised BT474 tumours from untreated SCID-beige mice were HER2-positive (immunohistochemistry 3+, defined as consistent with circumferential membrane staining that is complete, intense and within >10 % of tumour cells) as assessed using the HercepTest (Dako, Ely, UK) according to the manufacturer’s instructions [
5].
In the trastuzumab blocking study, three female SCID-beige mice with BT474 tumours received intravenous trastuzumab (14.2 mg/kg) 24 h prior to intravenous injection of 111In-G3 DARPin. Three control mice received 111In-G3 DARPin alone. The mice were killed at 4 h after administration of 0.3 MBq 111In-G3 DARPin (1.9 μg per mouse, SA 2.3 MBq/nmol).
MicroSPECT/CT imaging
Female SCID-beige mice bearing BT474 tumours were injected intravenously with either 10.5 MBq of
123I-G3 (2.1 MBq/μg, SA 30.1 MBq/nmol) or 8.4 MBq of
111In-G3 (4 MBq/μg, SA 58 MBq/nmol). Preliminary work had demonstrated that HER2-positive tumour signals on SPECT scans were compromised at lower SAs of radiolabelled G3 DARPin (data not shown). Thus, the SA for imaging was increased compared to the biodistribution studies to enhance the quality of images, but mice assessed for biodistribution and imaging studies received a similar molar dose of G3 DARPin. The radiolabelling reactions for imaging studies were performed with both a lower amount of G3 DARPin and higher radiation activity within the parameters outlined in the
radiolabelling section.
Imaging was performed under 2 % isoflurane anaesthesia 4 h after administration using a microSPECT/CT animal scanner (Bioscan, Poway, CA). Helical SPECT images were acquired in 20 projections over 30 – 40 min using a four-headed camera with 4 × 9 (1.4 mm) pinhole collimators. The CT images were acquired in 180 projections with an exposure time of 1,000 ms using a peak kilovoltage of 45 kVp over 6 min. Radionuclide images were reconstructed using HiSPECT (Scivis, Göttingen, Germany) iterative reconstruction software and fused with CT images using proprietary InVivoScope (Bioscan) software.
DARPin G3 specificity for HER2 in vivo
Mice were inoculated with tumours as previously described. G3 DARPins were radiolabelled with [
99mTc(CO)
3]
+ via a C-terminal His
6 tag ([
99mTc(CO)
3]
+-G3 DARPin-His
6) according to the published protocol [
27]. Briefly, [
99mTc(CO)
3]
+ was prepared using an IsoLink kit (Mallinckrodt, Petten, The Netherlands) according to the manufacturer’s instructions. Following neutralization and the addition of 150 μg of G3 DARPin, the mixture was reacted at room temperature for 30 min. Radiolabelling efficiency was determined by size exclusion HPLC using the same methods as previously outlined. The product was purified from 50 % to 100 % radiochemical purity using a NAP-10 column (GE Healthcare). MicroSPECT/CT imaging was performed 1 h after administration of about 30 MBq [
99mTc(CO)
3]
+-G3 DARPin-His
6 (10 μg, SA 44 MBq/nmol) to three mice with HER2-positive (BT474) tumours and three mice with HER2-negative (MDA-MB-468) tumours, as previously described. Mice were killed at 24 h.
DARPin G3 specificity for HER2 in vitro
The DOTA-conjugated G3 DARPins were labelled using naturally abundant indium chloride (natInCl3; Sigma-Aldrich, St. Louis, MO) in 0.05 M HCl solution, and unconjugated G3 DARPins were labelled using NanatI (Sigma-Aldrich) in 0.1 M sodium hydroxide, using the same conditions required for 111In and 125I radiolabelling reactions, respectively.
Competition assay
BT474 cells (ATCC) were seeded at a density of 1 × 106 per well into Cellstar six-well plates (Greiner bio-one, Frickenhausen, Germany) and grown to confluence over 24 h. The confluent cells were incubated in triplicate with 0.1 nM [99mTc(CO)3]+-G3 DARPin-His6 with or without 1,000 nM natIn-DARPin or natI-DARPin in Dulbecco’s modified Eagle’s medium (DMEM) with high glucose concentration (4.5 g/L) containing 1 % fetal calf serum (Biosera, Boussens, France ) and 0.1 % sodium azide (Sigma-Aldrich) for 1 h 30 min at 20 °C. An unlabelled epidermal growth factor receptor (EGFR) binding DARPin (K. Chester, unpublished) was used as a control.
The assays were stopped by removing the medium and washing the cells with 2 ml ice-cold PBS. The cells were lysed with 1 ml of 1 M sodium hydroxide and the lysate was collected. The wells were washed twice with 1 ml of PBS. The washes were pooled with the cell lysate for analysis. The radioactivity was measured in a gamma counter. The mean percentage of radioactivity was calculated for each condition in relation to the controls treated with [99mTc(CO)3]+-G3 DARPin-His6 alone.
Flow cytometry analysis
BT474 (ATCC), MDA-MB-468 (ATCC) and OE-19 (Sigma-Aldrich) cells were individually prepared for flow cytometry by removal of medium and incubation with 5 ml of 0.2 % EDTA for 10 min. The cells were then transferred to tubes and centrifuged (4 °C, 4 min, 1,000 rpm). The EDTA solution was removed and 5 ml of fresh medium was added. Cells were counted and diluted to 1 million/ml, and 1 ml was used for each test condition. After washing with cold PBS, 200 μl of DARPin at 10 μg/ml was added followed by incubation for 1 h at 4 °C. Cells were washed with cold PBS and incubated with 200 μl of mouse anti-DARPin (K. Chester, unpublished) for 1 h at 4 °C. Subsequently the cells were washed with cold PBS and incubated with 200 μl of Alexa Fluor® 488 goat anti-mouse IgG (Life Technologies, Paisley, UK) for 30 min at 4 °C. After further washing with cold PBS, the cells were suspended in 500 μl of cold PBS. Samples were analysed on a CyAn ADP high-performance flow cytometer (Becton Dickinson, Oxford, UK); cells were gated according to size scattering, forward scattering and pulse width so only single cells were analysed. A total of 10,000 cell events were recorded per sample and data were analysed using FlowJo software (Tree Star, Ashland, OR).
Statistical analysis
An independent samples t test was performed with SPSS Statistics 21 software (IBM, Armonk, NY) to compare normal liver uptake between the different radiolabelled G3 DARPins (p values <0.05 were considered statistically significant).
Discussion
111In-(HE)
3-G3 DARPin was found to be better for HER2 imaging than all other formats tested in this study. There are limitations in comparing HER2 radioligands assessed in different HER2-positive human tumour xenografts, including different levels of HER2 expression. However, within 24 h of administration to mice bearing HER2-positive tumours,
111In-(HE)
3-G3 DARPin achieved higher tumour-to-blood ratios than other reported HER2 radioligands, including whole antibodies, Fab fragments of antibodies and small high-affinity proteins [
28‐
31].
111In-(HE)
3-G3 also had greater potential for HER2 imaging than
125I-(HE)
3-G3, reflected by superior microSPECT/CT scans.
The BT474 tumour-bearing mice were confirmed to have immunohistochemistry scores of 3+ with the HercepTest. The HER2-positive tumour uptake of
111In-(HE)
3-G3 and
125I-(HE)
3-G3 achieved at 4 h was 8.82 ± 1.25 % ID/g and 11.29 ± 3.24 % ID/g, respectively. By contrast,
111In-DOTA-Z
HER2:342-pep2 achieved 39.9 percentage of injected activity per gram tissue (% IA/g) [
32]. Although higher HER2-positive tumour uptake could have been anticipated, the tumour uptake was sufficient for microSPECT/CT imaging and impressive tumour-to-blood ratios were achieved.
The G3 DARPins were radioiodinated directly at their tyrosine residues. It is likely that only one of the two tyrosine residues within each G3 DARPin was radioiodinated, owing to the molar ratios of radioiodide and G3 DARPin used for radiolabelling. Although direct radioiodination is convenient and the most widely used methodology, it is recognized that the radioligand is likely to undergo in vivo dehalogenation. In future studies, we plan to compare methods using bifunctional coupling agents, to determine whether this approach can improve in vivo stability of radioiodinated G3 DARPins [
33]. Nanobodies (12 – 15 kDa) are isolated from the heavy chain of Camelidae antibodies. The anti-HER2 5F7GGC Nanobody radioiodinated via the residualizing agent
N-succinimidyl 4-guanidinomethyl 3-
125/131I-iodobenzoate (*I-SGMIB-Nanobody) has superior targeting of HER2-positive human breast carcinoma in vitro and in vivo than its directly radioiodinated counterpart, as *I-SGMIB-Nanobody has enhanced tumour retention of radioactivity [
34].
Importantly, we observed that
111In-(HE)
3-G3 was able to bind to HER2 in the presence of trastuzumab. This confirms the results of structural modelling which demonstrate that DARPin G3 and trastuzumab bind to non-overlapping epitopes of HER2 domain IV [
35]. Thus,
111In-(HE)
3-G3 DARPin has the potential to image both treatment-naive patients and patients receiving concomitant trastuzumab without requiring a delay to treatment.
111In-(HE)
3-G3 imaging would provide completely new information with the potential to improve understanding of HER2 breast cancer evolution and heterogeneity. Current literature based on biopsy sampling is inconsistent with a wide-range of reported rates of HER2 expression discordance between primary and metastatic sites, from 0 to 34 % [
7]. Whole-body assessment of HER2 expression at tumour sites over time and during therapy with HER2 imaging is both more feasible and acceptable to patients than serial and multiple biopsies. Furthermore, considerably less is known about gastric cancer HER2 biology, and
111In-(HE)
3-G3 imaging could help address this knowledge gap [
36].
HER2 is an important therapeutic target in cancer. DARPin HER2 imaging could be used to improve the selection of patients for anti-HER2 therapy, by identifying increased HER2 expression and the need to introduce anti-HER2 therapy, as well as HER2 loss, necessitating discontinuation of anti-HER2 therapy [
1]. This could not only save patients from unnecessary treatments, but also improve healthcare economics by ensuring appropriate use of expensive anti-HER2 therapies.
The pharmacokinetics of
111In-(HE)
3-G3, including short half-life in serum, high tumour-to-blood ratios and low non-renal tissue uptake, are well suited to HER2 imaging. The kidneys received the highest radiation dose. However, based on medical internal radiation dose (MIRD) estimates, the maximum absorbed kidney dose in patients with the proposed clinical dose of
111In-(HE)
3-G3 (300 MBq) is 1,000-fold lower than the dose associated with a 5 % rate of radiation nephritis within 5 years of administration (TD
5/5; 9.75 mGy vs. 10 Gy) [
37].
Imaging trials of most HER2 radioligands have had disappointing results due to limitations related to their pharmacokinetics for imaging which were already apparent in preclinical assessment [
28‐
31]. It should be noted that the majority of clinical HER2 imaging studies have not assessed HER2 tumour status histologically for correlation with HER2 scans, thus limiting the evaluation of these imaging agents. Trastuzumab radiolabelled with
64Cu,
89Zr or
111In has demonstrated the potential for HER2 imaging by identifying known and/or previously unknown tumour lesions in patients, but lacks sensitivity compared with conventional imaging owing to a long half-life and high blood pool activity [
12‐
14]. Fab fragments of trastuzumab were developed for HER2 imaging because their lower molecular weight is associated with a shorter half-life in serum and faster clearance of background radiation from the blood compared with trastuzumab. However,
68Ga-F(ab’)
2-trastuzumab PET imaging failed to identify any tumours among four of the eight patients with metastatic HER2-positive breast cancer assessed, due to relatively high liver uptake and blood pool activity as well as potential competition with therapeutically administered trastuzumab [
38].
A radiolabelled HER2 binding Affibody molecule, Z
HER2:342 (about 7 kDa), was used to assess three patients with HER2-positive metastatic breast cancer by PET and/or SPECT imaging. Although not all known tumour lesions were identified in two patients, there was limited tumour biopsy sampling to systematically evaluate the accuracy of HER2 Affibody molecule imaging. Unfortunately, there was high background liver uptake in this initial study [
39]. Recently, a phase I trial demonstrated that the second generation Affibody
111In-ABY-025 has improved distribution, dosimetry and accuracy in assessing patients with HER2-positive and HER2-negative metastatic breast cancer. There was a good correlation between HER2 status assessed by SPECT/CT
111In-ABY-025 imaging and immunohistochemistry with the HercepTest, including confirmation that a patient who had had HER2-positive primary disease developed HER2-negative metastases [
15].
In our evaluation of the DARPin G3, the (HE)
3 tag is a beneficial component as it appeared to lower normal liver uptake of the DARPin G3 without compromising uptake in other assessed normal tissues. This is advantageous for clinical application as HER2 molecular imaging requires high tumour-to-liver tissue ratios and the liver is a common site for breast cancer metastases, yet is also involved in drug metabolism and excretion. Histidine-based tags enable IMAC purification and can also be used for chelation of [
99mTc(CO)
3]
+ [
21,
27]. The His
6 tag is well established and has been used safely in patients [
40], but (HE)
3-G3 DARPin was superior to His
6-G3. Affibody molecules with an (HE)
3 tag also have lower normal liver uptake than counterparts with alternative histidine-based tags [
24,
25]. The G3 DARPins assessed in this study only differed by the presence or composition of their tags and thus the study was able to confirm that (HE)
3-G3 DARPin had the lowest normal liver uptake.
The mechanism of (HE)
3 tag-mediated reduction in liver uptake of DARPin G3 has not been established. For Affibody molecules it has been proposed that positive charge and hydrophobicity in the tag play a crucial role in liver uptake [
25]. However, the untagged and His
6-tagged Affibody molecules have basic isoelectric points (pI), which are brought to a more acidic region by switching to an (HE)
3 tag, such that the overall pI of the different Affibody constructs tested differed greatly. By contrast the (HE)
3-tagged, His
6-tagged and untagged G3 DARPins have similar pI values of 4.79, 5.41 and 4.71, respectively [
25]. Furthermore, the (HE)
3-tagged, His
6-tagged and untagged G3 DARPins have similar grand average of hydropathy (GRAVY) scores of −0.12, −0.12 and +0.02, respectively, indicating that other factors are involved, while the corresponding Affibody molecules have slightly more divergent scores of −1.03, −0.97 and −0.85.
Although in preclinical studies histidine-tagged proteins have been shown to exert greater immunogenicity than their untagged counterparts, several histidine-tagged proteins have been well tolerated in human trials [
40]. For example, Endostar a novel recombinant human endostatin which inhibits angiogenesis has a histidine tag, and was safe and well tolerated in large clinical trials [
41]. Interestingly, a Blast search (NCBI) for a short input sequence with HEHEHE as the query, yielded a variety of hits in the database of almost identical sequences, e.g. HEHEH in the human zinc transporter (gene ID SLC39A9) and HEHEQE in kinase 3 (gene ID TAOK3). The HHHHHH sequence cannot be found using a Blast search in the
Homo sapiens database. Instead clusters of histidine are found that are coordinated with metal ions, e.g. Ca
2+, Mg
2+ and Zn
2+. The occurrence of the HEHEH sequence in human proteins could mean that the HE
3 tag is a potentially safer alternative to the His
6 tag.
Conclusion
A clinically valuable radioligand for HER2 molecular imaging in breast cancer and gastric cancer would require minimal normal liver and stomach uptake, as well as the ability to bind to HER2 in the presence of concomitant anti-HER2 therapy. We have demonstrated that 111In-(HE)3-G3 DARPin has specificity for HER2, binds in the presence of trastuzumab, and achieves high tumour-to-blood ratios and reasonable tumour to non-renal tissue ratios, including tumour-to-liver and tumour-to-stomach ratios. Based on the presented preclinical data, 111In-(HE)3-G3 could realize the clinical potential of HER2 imaging and may be suitable for assessment in a first-in-human study.