Standardization of the [68Ga]Ga-PSMA-11 Radiolabeling Protocol in an Automatic Synthesis Module: Assessments for PET Imaging of Prostate Cancer

Prostate-specific membrane antigen (PSMA) is a glycoprotein present in the prostate, that is overexpressed in prostate cancer (PCa). Recently, PSMA-directed radiopharmaceuticals have been developed, allowing the pinpointing of tumors with the Positron Emission Tomography (PET) or Single Photon Emission Computed Tomography (SPECT) imaging techniques. The aim of the present work was to standardize and validate an automatic synthesis module-based radiolabeling protocol for [68Ga]Ga-PSMA-11, as well as to produce a radiopharmaceutical for PET imaging of PCa malignancies. [68Ga]Ga-PSMA-11 was evaluated to determine the radiochemical purity (RCP), stability in saline solution and serum, lipophilicity, affinity to serum proteins, binding and internalization to lymph node carcinoma of the prostate (LNCaP) cells, and ex vivo biodistribution in mice. The radiopharmaceutical was produced with an RCP of 99.06 ± 0.10%, which was assessed with reversed-phase high-performance liquid chromatography (RP-HPLC). The product was stable in saline solution for up to 4 h (RCP > 98%) and in serum for up to 1 h (RCP > 95%). The lipophilicity was determined as −3.80 ± 0.15, while the serum protein binding (SPB) was <17%. The percentages of binding to LNCaP cells were 4.07 ± 0.51% (30 min) and 4.56 ± 0.46% (60 min), while 19.22 ± 2.73% (30 min) and 16.85 ± 1.34% (60 min) of bound material was internalized. High accumulation of [68Ga]Ga-PSMA-11 was observed in the kidneys, spleen, and tumor, with a tumor-to-contralateral-muscle ratio of >8.5 and a tumor-to-blood ratio of >3.5. In conclusion, an automatic synthesis module-based radiolabeling protocol for [68Ga]Ga-PSMA-11 was standardized and the product was evaluated, thus verifying its characteristics for PET imaging of PCa tumors in a clinical environment.


Introduction
Prostate cancer (PCa) is the second most prevalent type of cancer among men, with an incidence rate of 109.8 new cases/100,000 individuals each year from 2013 to 2017 in the US, and with 191,930 new cases estimated for 2020 [1]. In Brazil, according to data from the National Cancer Institute for 2020, 65,840 new cases of PCa are estimated, which corresponds to a gross rate of 66.12 cases/100,000 individuals [2].
The prostate-specific membrane antigen (PSMA) is a type-II transmembrane glycoprotein that has several enzymatic functions. This antigen is expressed in the prostatic tissue, as well as in other organs, such as the small intestine, kidneys, liver, brain, salivary glands, and lacrimal glands [3]. However, PSMA is overexpressed in the PCa tissue in direct association with the cancer's aggressiveness, in lymph nodes and bone metastases, and also in other castration-resistant PCa lesions [4][5][6][7], with levels reaching from 100 to 1000 times the values found in non-cancerous prostatic cells [8]. It was previously detected in the lymph node carcinoma of the prostate (LNCaP) human cell line [9]. Given all of these factors, PSMA is considered an appropriate biomarker for PCa and an attractive target for theranostic applications [10].
Since 2001, small-sized PSMA-inhibiting molecules that interact with the binuclear active site of zinc have been developed, successfully radiolabeled, and tested to obtain Single Photon Emission Computed Tomography (SPECT) and Positron Emission Tomography (PET) images of PCa tumors [11]. These small molecules have been labeled with different radioisotopes ( 99m Tc, 111 In, 18 64 Cu, 225 Ac, 211 As, and 90 Y, has opened the possibility of using them as therapeutic agents [12][13][14][15][16][17][18]. The first attempt at using PSMA as a tumor marker in order to obtain images was done in the form of an 111 In-labeled monoclonal antibody (mAb)-[ 111 In]In-capromab pendetide or ProstaScint ® -to be used in SPECT tomography. This radiopharmaceutical presented low sensitivity and specificity, mainly because it was aimed at the intracellular domain of PSMA, targeting apoptotic, necrotic, or damaged cells [19,20]. Another mAb was developed to target the extracellular domain of PSMA; however, its applicability is mainly limited because of its long half-life in the circulation system, which has implications for images with high backgrounds or long time periods from injection to imaging [21]. A real advance in image-based PCa diagnosis was reached with the development of the 68 Ga-labeled PSMA-HBED-CC compound (also named PSMA-11), which presents advantageous characteristics for imaging PCa metastases as a PET radiopharmaceutical [22]. PSMA-11 corresponds to a glutamine-urea-lysine inhibitor, which is conjugated with the highly efficient and galliumspecific N,N -bis-[2-hydroxy-5-(carboxyethyl)benzyl]ethylenediamine-N,N -diacetic acid (HBED-CC) chelator by means of a spacer based on aminohexanoic acid. This ureabased inhibitor presents a high affinity and specificity for PSMA, as well as high and fast internalization to LNCaP cells [8], which is better than that of its corresponding 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic acid (DOTA)-chelator analogue [23]. Additionally, HBED-CC can be labeled with 68 Ga in low concentrations and at room temperature. Currently, [ 68 Ga]Ga-PSMA-11 is probably the most used radiopharmaceutical for PCa imaging around the world.
In comparison with other radiopharmaceuticals for PCa imaging (e.g., [ 11  Ga]Ga-PSMA-11), as well as images with higher SUV max and increased contrast (tumor-to-background ratio) in most of the lesions [22]. Based on a literature review and meta-analysis, imaging studies using five different PET radiopharmaceuticals were compared, and, in spite of the limited data, it was verified that tracers targeting PSMA are superior to other radiopharmaceuticals, such as [ 18 F]F-FDG, [ 11 C]C-Acetate, [ 11 C]C-or [ 18 F]F-Choline, and anti-1-amino-3-[ 18 F]F-fluorocyclobutane-1carboxylic acid, in detecting extraprostatic lesions [24].
Additional aspects to be considered include accessibility to the radioisotope, production time and procedure, exposure during production, the number of patients that can be attended in the long term, and the effect of the radioisotope on image quality. In this sense, most of these parameters are favored when working with the automatic synthesis module-based production of [ 68 Ga]Ga-PSMA-11-like that presented in this work-which provides further advantages for this product [25]. Although there are other possibilities for synthesis, such as direct cyclotron production or manual-based production, automatic synthesis module-based production of [ 68 Ga]Ga-PSMA-11 allows very low radiation exposure for technicians, high reproducibility, and compliance with local health regulatory and good manufacturing practice (GMP) standards [26,27]. Furthermore, considering that a 68 Ge/ 68 Ga generator can be eluted from two to three times per day, in-house automatic synthesis module-based production of [ 68 Ga]Ga-PSMA-11 provides enough doses for six to eight patients, making it a convenient alternative to direct cyclotron production.
In this sense, the present work aimed to standardize an automatic synthesis modulebased radiolabeling protocol for [ 68 Ga]Ga-PSMA-11 as a radiopharmaceutical for PET imaging of PCa malignancies that is produced in-house. In vitro and ex vivo assays were performed to determine the characteristics of the radiopharmaceutical in order to validate in-house production while attending to national health regulatory standards.

Radiolabeling and Radiochemical Purity (RCP) Evaluation
Initially, the radiolabeling protocol was manually evaluated (n = 4) previous to the installation of a Modular-Lab PharmTracer synthesis module at the hospital's radiopharmacy. In this phase, 10 µg/10.56 nmol or 15 µg/15.84 nmol of PSMA-11 were diluted in 1.0 mL of 0.1 M NaOAc buffer with a pH of 4.5. Depending on the activity eluted from the 68 Ge/ 68 Ga generator, 1090 ± 35 MBq of labeled product was obtained, with a labeling yield of 73.1 ± 2.2%, a pH of 4.5, and a radiochemical purity (RCP) of 93.1 ± 2.7%, determined with ascending chromatography, using instant thin layer chromatographic (iTLC) glass microfiber impregnated with silica gel (SG)-iTLC-SG-and 0.1 M NH 4 OAc solution/MeOH (1:1) as eluent.
After appropriate training on using the automatic synthesis module and validation of the quality control methods, routine production was initiated under GMP standards using 20 µg/21.12 nmol of PSMA-11. Radiolabeling yields of >85% were obtained. Data corresponding to the routine production during 2019 (n = 30) are illustrated in Table 1. Values are expressed as "mean ± SD" (n = 30).
In the ascending chromatographic system, free gallium chloride ([ 68 Ga]GaCl 3 ) remains in the strip origin (retention factor (R f ) = 0.1-0.2) and [ 68 Ga]Ga-PSMA-11 migrates with the solvent front (R f = 0.9-1.0), providing an adequate chromatographic resolution, as illustrated in Figure 1. By using the Sep-Pak C 18 method, it was possible to quantify the amount of insoluble gallium species or gallium colloids ([ 68 Ga]Ga(OH) x ) retained in the cartridge. Once the Sep-Pak C 18 method separated both radiochemical impurities, [ 68 Ga]GaCl 3 (collected in the waste vial) and [ 68 Ga]Ga(OH) x (retained in the cartridge), the RCP was slightly smaller (~95%) than the value obtained with the iTLC method (~97%), which separated only [ 68 Ga]GaCl 3 . The difference between both methods corresponds to the [ 68 Ga]Ga(OH) x retained in the Sep-Pak C 18 cartridge. Both the iTLC-SG and Sep-Pak C 18 methods were introduced into the routine to assess RCP, considering that their results were compatible with data provided by a reversed-phase high-performance liquid chromatography (RP-HPLC) analysis ( Figure 2), which was used to validate the iTLC-SG and Sep-Pak C 18 assays. Additionally, it is worth mentioning that the iTLC-SG and Sep-Pak C 18 methods are faster, have lower costs, and are easier to perform in a hospital's radiopharmacy. Furthermore, all of the batches produced with this standardized automatic synthesis module-based method showed acceptable pH values and were sterile and pyrogen-free. Operating with two technicians and under the supervision of an experienced radiopharmacist, the synthesis was completed within 15 min. An additional 10 min were required for quality control tests (iTLC-SG, Sep-Pak C 18 , pH, and pyrogen). Overall, the final labeled product was ready to be used in roughly 25 min. Given the properties of the 68 Ge/ 68 Ga generator and according to the number of patients, it is possible to have from two to three productions per day, allowing for six to eight patients to be injected with a dose of 130-222 MBq (3.5-6.0 mCi).

Evaluation of the Stability of the Radiolabeled Compound
The stability of [ 68 Ga]Ga-PSMA-11 in saline solution at room temperature was evaluated for up to 4 h by measuring the RCP of the samples using RP-HPLC analysis. The results are presented in Table 2, demonstrating appropriate stability (RCP > 98%) all along this time period. The stability of [ 68 Ga]Ga-PSMA-11 in serum at 37 • C was also evaluated for up to 1 h through RP-HPLC analysis. In this case, the RCP values obtained at 0.5 and 1 h were >97% and >95%, respectively (n = 3).

Ex Vivo Biodistribution
The ex vivo biodistribution of [ 68 Ga]Ga-PSMA-11 was assessed after injection into healthy and LNCaP-tumor-bearing mice ( Figure 4). The data showed that the radiopharmaceutical presented rapid blood clearance, followed by high uptake by the kidneys. Beyond that, high [ 68 Ga]Ga-PSMA-11 uptake by the spleen was observed. Ex vivo biodistribution data that were obtained in xenografted prostate-tumor-bearing mice showed that [ 68 Ga]Ga-PSMA-11 uptake by the tumor was >8% at 30 and 60 min after the radiopharmaceutical administration. No significant difference was observed between the time intervals (t = 0.40; df = 8; p = 0.6989) for tumor uptake (n = 5). Target-to-non-target ratios were calculated, and the values were >8.5 and >3.5 for the tumor-to-contralateral-muscle ratio and tumor-toblood ratio, respectively. In addition, in this case, no significant difference was observed between the evaluated time intervals (tumor-to-contralateral-muscle ratio: t = 0.13; df = 4; p = 0.9026; tumor-to-blood ratio: t = 1.10; df = 5; p = 0.3226) of biodistribution (n = 5).  Values are expressed as "mean ± SD": (n = 3). RCP: radiochemical purity.  3. Discussion 68 Ga-labeled molecules must present high RCP values (>90%) to be applicable in a clinical setup [28,29]. The radiolabeling procedure with 68 Ga can yield free [ 68 Ga]GaCl 3 and [ 68 Ga]Ga(OH) x , the main radiochemical impurities, which may interfere with imaging interpretation. In this sense, ascending chromatography (using iTLC-SG and 0.1 M NH 4 OAc solution/MeOH (1:1) as an eluent), solid-phase extraction (using a Sep-Pack C 18 cartridge), and an RP-HPLC analysis were performed in order to evaluate the RCP of [ 68 Ga]Ga-PSMA-11. The results obtained by the three analytical methods were >95%. A similar RCP for [ 68 Ga]Ga-PSMA-11 was previously described [30,31]. Therefore, the data obtained in the present work showed that [ 68 Ga]Ga-PSMA-11 was obtained with high RCP with this standardized automatic synthesis module-based method. It is worth mentioning that the automatic synthesis module-based method has many advantages compared to manual-based methods once the automated module is placed inside a hot cell and under laminar flow, allowing high reproducibility, low radiation exposure, and compliance to GMP standards. [ 68 Ga]Ga-PSMA-11 was stable in saline solution for up to 4 h (RCP > 98%). These data are in agreement with those that were previously described, which showed in vitro stability of [ 68 Ga]Ga-PSMA-11 for up to 3 h [31]. Moreover, [ 68 Ga]Ga-PSMA-11 was stable in serum for up to 1 h (RCP > 95%). Thus, the standardized automatic synthesis module-based method is able to produce [ 68 Ga]Ga-PSMA-11 with high RCP and suitable in vitro stability. The automated Modular-Lab PharmTracer synthesis module was effectively applied in the routine for [ 68 Ga]Ga-PSMA-11 production and is a useful tool for the clinical development of other 68 Ga-labeled compounds. High-quality [ 68 Ga]Ga-PSMA-11 was obtained over four years in more than 1300 syntheses for clinical applications in more than 3000 patients, as exemplified in Figure 5. No adverse reactions were found in this population. Furthermore, clinical applications of [ 68 Ga]Ga-PSMA-11 produced by this standardized automatic synthesis module-based method were reported, such as a rare finding of testicular metastasis from PCa [32], the description of an irreversible two-tissue compartment model for the kinetics of this radiopharmaceutical in humans [33], and its high performance for the detection of recurrent PCa after prostatectomy [34].
The P of [ 68 Ga]Ga-PSMA-11 was determined by the ratio between n-octanol and water. Then, Log P was calculated, and its negative value confirmed the hydrophilic characteristics of [ 68 Ga]Ga-PSMA-11 [35]. Furthermore, low SPB values were observed, which were in agreement with the obtained Log p value [36]. These results are in accordance with previously published data for the same or similar molecules [37][38][39].
The binding of [ 68 Ga]Ga-PSMA-11 to LNCaP cells was evaluated; it represents the radiopharmaceutical molecules that bound to LNCaP cells, including the fraction of molecules that were internalized. This issue can be explained by PSMA expression on the surface of LNCaP cell membranes [9]. Internalization represents the fraction of [ 68 Ga]Ga-PSMA-11 that was internalized into LNCaP cells relative to the radiopharmaceutical bound to PSMA expressed on the cell surfaces [40]. The data obtained in the present work are in accordance with those obtained by Ferro-Florez and co-workers for [ 99m Tc]Tc-EDDA/HYNIC-iPSMA binding and internalization in LNCaP cells [41].
The ex vivo biodistribution profile of [ 68 Ga]Ga-PSMA-11, which was evaluated in healthy and LNCaP-tumor-bearing mice, showed rapid blood clearance and elimination by the urinary tract, which is consistent with the hydrophilic nature of the molecule (Log p < 0) and its low SPB, as previously described. It is important to comment that the substantial [ 68 Ga]Ga-PSMA-11 uptake by the spleen observed in our data has also been previously reported in animals [42] as well as in humans [43], although it is not a specific target. The high [ 68 Ga]Ga-PSMA-11 uptake by the tumor and, consequently, high tumor-tocontralateral-muscle ratio are explained by the presence of PSMA on the surfaces of LNCaP cells [9]. Therefore, the radiolabeled ligand bound to this antigen and was internalized into the tumor cells according to in vitro assays. On the other hand, the high tumor-toblood ratio is due to the low SPB of [ 68 Ga]Ga-PSMA-11 and its rapid blood clearance and elimination by the urinary tract, as previously discussed. Thus, these results corroborate the in vivo specificity of [ 68 Ga]Ga-PSMA-11 for prostate tumor tissue and indicate that this radiopharmaceutical is appropriate for PET images in adequate quality for PCa diagnosis. Considering all of these in vitro and ex vivo data, the standardized automatic synthesis module-based in-house production of [ 68 Ga]Ga-PSMA-11 was validated according to national health regulatory standards.

[ 68 Ga]Ga-PSMA-11 Radiolabeling Procedure
The synthesis of [ 68 Ga]Ga-PSMA-11 was initially carried out manually to determine the optimal synthesis and quality control parameters. Later on, the synthesis protocol was implemented in an automated Modular-Lab PharmTracer synthesis module (Eckert and Ziegler-Berlin, Germany) for routine production. The precursor Glu-NH-CO-NH-Lys(Ahx)-HBED-CC (PSMA-11) and the synthesis cassettes were acquired from ABX Advanced Biochemical Compounds (Radeberg, Germany). The IGG 100 68 Ge/ 68 Ga generator was obtained from Eckert and Ziegler (Berlin, Germany), which has a guarantee that the 68 Ge breakthrough is <0.001% over time. Solvents and other reagents were acquired from Merck (Darmstadt, Germany) or Sigma-Aldrich Sweden (Stockholm, Sweden) in high chemical degrees and metal-free media.
[ 68 Ga]GaCl 3 was eluted with 6 mL of 0.1 M HCl solution and purified in a cationic filter. The purified 68 Ga retained in the filter was then eluted with 0.5 mL of 5 M NaCl solution/5.5 N HCl solution (97:3) into a reaction vial containing 10 to 20 µg of PSMA-11 diluted in 1.0 mL of 0.1 M NaOAc buffer with a pH of 4.5 and heated at 85 • C for 3-5 min. After this reaction time, the [ 68 Ga]Ga-PSMA-11 was purified using a Sep-Pak C 18 cartridge (Waters-Milford, MA, USA) and preconditioned with 5 mL of EtOH/H 2 0 (1:1) solution and 5 mL of 0.9% NaCl solution. The final product was eluted from the Sep-Pak C 18 cartridge with 0.4 mL of EtOH/H 2 0 (1:1) solution and diluted with 6 mL of 0.9% NaCl solution through a 0.22 µm Cathivex-GV filter (Millipore-Burlington, MA, USA). The labeling yield was determined at the end of the automated synthesis as the ratio between the activity of the final product (purified [ 68 Ga]Ga-PSMA-11) vial and the total activity in the module; the latter was obtained as the sum of the activities in the different parts or components of the module (final product vial + empty reaction vial + waste vial + cationic filter + Sep-Pak C 18 cartridge + 0.22 µm filter). This calculation was made without correcting the activity decay. The activities were measured in a CRC 25 PET dose calibrator (Capintec-New Jersey, NJ, USA). For the integrity filter test, a bubble-point method was performed at the end of the synthesis. The pyrogen was evaluated in all batches with an Endosafe ® -PTS (Charles River Laboratories-Wilmington, MA, USA) at a dilution factor of 1:50. In order to attest sterility, the microbiological assays were carried out by the hospital's clinical analysis laboratory.
All equipment used in this work for measurements and quality control assessments was previously calibrated, and preventive maintenance was carried out periodically.

Ascending Chromatography and Solid-Phase Extraction (SPE)
Ascending chromatography was performed with iTLC-SG obtained from Agilent Technologies (

Evaluation of the Stability of the Radiolabeled Compound
The stability of [ 68 Ga]Ga-PSMA-11 was evaluated in saline solution and in serum. In saline solution (room temperature), this evaluation was performed 1, 2, 3, and 4 h after the radiolabeling procedure. The stability of [ 68 Ga]Ga-PSMA-11 in serum-incubated at 37 • C under slight agitation-was evaluated at 0.5 and 1 h post-incubation. Briefly, an aliquot of [ 68 G h with 450 µL of serum under slight agitation. For each time analyzed, an aliquot was precipitated with cold ACN (1:1), and the sample was centrifuged (825 g, 5 min) with Minispin ® plus (EppendorfAG-Hamburg, Germany). The supernatant was filtered with a 0.22 µm Millex-GV syringe filter (Merck-Burlington, MA, USA). In both cases-saline solution and serum-aliquots of [ 68 Ga]Ga-PSMA-11 were analyzed with RP-HPLC as previously described.

LNCaP Cell Culture
The LNCaP human cell line was obtained from the Banco de Células do Rio de Janeiro (code 0149) (Rio de Janeiro, RJ, Brazil). LNCaP cells (passage 3-6) were grown in RPMI-1640 medium (Sigma-Aldrich-Darmstadt, Germany) and supplemented with 10% (v/v) fetal bovine serum (Sigma-Aldrich-Darmstadt, Germany) and 1% (v/v) penicillin and streptomycin antibiotic solution (Sigma-Aldrich-Darmstadt, Germany). The cells were kept in humidified air containing 5% CO 2 at 37 • C. The cells were grown to confluence and then harvested via trypsinization. After centrifugation (1200 rpm, 5 min), the cells were resuspended in RPMI-1640 medium for in vitro binding and internalization assays or in a 1:1 mixture of Matrigel and RPMI-1640 medium for development of the prostate tumor animal model.

LNCaP Prostate Tumor Animal Model
Male BALB/c nude mice (~20 g/~60 days) were supplied by the vivarium of the Centro de Experimentação e Treinamento em Cirurgia of the Hospital Israelita Albert Einstein (Sao Paulo, SP, Brazil). The animals were maintained under specific pathogen-free conditions with free access to food and water. The housing suite was temperature (22 ± 2 • C) and humidity (50 ± 10%) controlled with filtered air and a regulated light-dark cycle of 12:12 h, with lights turning on at 07:00 am. All procedures involving mice were conducted in agreement with the Brazilian Guidelines on Care and Use of Animals for Scientific Research or Teaching Activities (DBCA) and were approved by the Ethics Committee on Animal Use of the Hospital Israelita Albert Einstein, protocol codes 2843/16 and 3241/17.
In order to produce the tumor model, an aliquot (200 µL) containing 1 × 10 7 LNCaP cells in a 1:1 mixture of Matrigel and RPMI-1640 medium was injected subcutaneously into the right upper flank of the BALB/c nude mice, as previously described [47], with some modifications. Tumors were allowed to grow in vivo for a maximum period of 40 days after inoculation or until reaching a diameter of 10 mm. LNCaP-tumor-bearing animals were then used for ex vivo biodistribution studies of [ 68 Ga]Ga-PSMA-11. Healthy (non-xenografted) male BALB/c nude mice were used as control animals.

[ 68 Ga]Ga-PSMA-11 Ex Vivo Biodistribution Studies
LNCaP-tumor-bearing (n = 10) and healthy (n = 10) male BALB/c nude mice were randomly distributed into two groups for the ex vivo biodistribution study of [ 68 Ga]Ga-PSMA-11. Mice were anesthetized with a ketamine-xilazine combination (100:10 mg/Kg) and intravenously injected with an aliquot of~11.1 MBq of the radiopharmaceutical. At 30 or 60 min after injection (n = 5 per time and per group), mice were euthanized. Organs and tissues of interest, such as the blood, carcass, contralateral muscle, heart, intestines, kidneys, liver, lungs, spleen, stomach, and tumor, were dissected and dried on a filter paper. Then, each organ or tissue was weighed, and its associated radioactivity was measured in a Wizard 2 ™ 3" 2480 automatic gamma counter (PerkinElmer-Norwalk, CT, USA). A standard dose containing the same amount of radioactivity injected into the mice and defined as 100% was counted simultaneously in a separated tube to correct for the physical decay of 68 Ga. The data were expressed as the percentage of injected dose per gram of tissue (% ID/g).

Statistical Analysis
Quantitative data were expressed as "mean ± standard deviation (SD)". Pairs of means were compared using a Student t-test. The statistical significance threshold for mean differences was set at 0.05. The data were analyzed using the GraphPad Prism v8.0.2 software (GraphPad Software Inc.-La Joya, CA, USA).

Conclusions
The production of [ 68 Ga]Ga-PSMA-11 in an automatic synthesis module was standardized, resulting in a sterile and endotoxin-free final product with high RCP and stability. All of the synthesis and quality control methods take around 25 min, making them highly reproducible under GMP standards for in-house production in a hospital radiopharmacy for routine PET imaging of PCa according to national health regulatory standards. This automated method allows multiple patient applications using one generator elution. After four years of daily work, more than 3000 patients have benefited from its high accuracy and great clinical value. Quality control methods were also standardized, and RCP evaluation using iTLC-SG and Sep-Pak C 18 assays was shown to be efficient and fast for routine purposes. Finally, in vitro and ex vivo assays were used to validate the quality of the synthesized product for PET imaging in PCa patients.

Data Availability Statement:
The data presented in this study are available on request from the corresponding author. The data are not publicly available due to privacy.