Selective targeting of bioengineered platelets to prostate cancer vasculature: new paradigm for therapeutic modalities (2025)

Keywords: platelets, androgen deprivation, human prostate xenografts, SPIO nanoparticles

Human prostate primary xenografts

Human prostate tissue was collected in accordance with National Institutes of Health guidelines on the use of human cases, with approval by the IRB at Roswell Park Cancer Institute (RPCI). Human prostate tissue samples were obtained from fresh radical prostatectomy remnants (within 2hrs of resection) from at eight different patients. The majority of these male patients were over 55years old with a median age of 68years old and Gleason grades of the prostate cancers that varied between 3+3 and 4+3. None of the patients had undergone treatment for BPH or hormonal therapy prior to surgery. Prostate tissue was macro-dissected by a pathologist and designated as benign tissue (non-involved), or tumour (>70% cancer cells) tissue, using a recently reported protocol 13. After evaluation by the pathologist, tissue specimens were submerged immediately in ice-cold ViaSpan solution (Barr Laboratories Inc., Pomona, NY, USA), and transported on ice to the laboratory for transplantation. A specimen of the initial tissue (IT) remnant of at least 8mm³ was removed from each surgical tissue sample before transplantation, fixed in 10% formalin, and paraffin-embedded for histological confirmation of the tissue as benign or malignant.

Primary xenografts of freshly harvested human prostate tissues were established in Severe Combined Immunodeficiency (SCID) mice as described previously 9,10,14. All experimental protocols that involved laboratory animals were performed in accordance with the National Institutes of Health guidelines and were approved by theInstitutional Animal Care and Use Committee at RPCI. In brief, the tissue specimen was cut into wedge-shaped pieces 2–3mm in length, and 2mm in width at the broadest end, and the wedges were transplanted into male SCID mice, 3months of age, that previously had been castrated and implanted subcutaneously with a 12.5mg sustained-release testosterone pellet (Innovative Research of America, Sarasota, FL, USA) to maintain serum testosterone levels at ∽4.0ng/ml throughout the study. For transplantation of prostate tissue, small (∽3mm) incisions were made in the skin on the right and left flanks of immunocompromised mouse hosts anaesthetized with Domitor (1mg/kg i.p.; Pfizer, Inc., New York, NY, USA), tissue wedges to be implanted dipped in Matrigel™ (BD Biosciences, Bedford, MA, USA), and the coated tissue wedges inserted into the subcutaneous space through a 10-gauge trocar device (Popper & Sons, Inc., Lincoln, RI, USA). Between 3 and 5 wedges were implanted along each flank through individual incisions; up to 10 fragments from a single patient were transplanted per animal. Incision sites were closed with Nexband tissue glue (Veterinary Products Laboratories, Phoenix, AZ, USA).

hRLP adherence to vascular damage induced by androgen deprivation

Primary xenografts of human prostate tissue from control hosts (non-castrate) were harvested from animals pre-implanted with sustained-release testosterone pellets, maintained for 30days, and administered platelets (hRL-P) by injection into the tail vein on day 30 after xenograft transplantation. Xenografts with microvasculature perturbed by ADT were harvested from animals pre-implanted with testosterone pellets, maintained for 30days, ADT-initiated on day 30 (testosterone pellet removed) after transplantation with tissue, and administered hRL-P on day 1, 2 or 3 after initiation of ADT (castration). hRL-P were administered to living host animals 30minutes before the animal was killed by exsanguination during perfusion to remove unbound platelets that had not adhered to the vasculature, and the xenografts harvested. Harvested xenografts were fixed in 10% formalin for a minimum of 24hrs, after which the fixed tissues were paraffin-embedded. Paraffin blocks were sectioned (5.0μm) onto ProbeOn Plus slides (Fisher Scientific International, Suwanee, GA, USA). Digital images of fields of the histological sections were collected, and the adhesion of hRL-P was quantitated as the area of the digital images occupied by platelets, as determined by CD42b immunostaining (DataS1), versus the total area of the xenograft tissue.

Preparation of SPIO-RL platelets

Lyophilized human platelets were prepared as described 12. In brief, fresh platelets were incubated for 1hr with paraformaldehyde (1.8%) and washed with citrated saline (0.006M trisodium citrate/0.154M NaCl, pH 6.8) with 5% bovine serum albumin. Platelets were lyophilized at −20°C to −40°C for 20–24hrs. Dried platelets were stored at −80°C until used. Dried platelets were re-hydrated in 1.0ml of imidazole buffer (IB; 0.084M imidazole, pH 7.35) and centrifuged at 1000×g for 8min. to pellet the platelets. The re-hydrated platelets were freed of albumin and imidazole by three washes in citrated saline. For use, platelet pellets were resuspended in platelet-poor plasma (p2918, Sigma-Aldrich, St.Louis, MO, USA), or in a modified Hanks’ buffered salt solution (0.17M NaCl/6.7mM KCl/1.0mM MgSO₄/0.5mM K₂HPO₄/2.8mM Na₂HPO₄/13.8mM dextrose, pH 7.2), for in vitro studies and in normal saline for in vivo studies.

Super-paramagnetic iron oxide nanoparticles (SPIOs: Feridex, Advanced Magnetics, Lexington, MA, USA), which were comprised of ∽5-nm SPIO cores with a dextran coating provided at an iron content of 11.2mg Fe/ml 15, were diluted 1/10 with infusion-grade saline, combined with freshly harvested apheresis platelets at 1×10⁹/ml, and incubated overnight, which resulted in phagocytosis of the SPIOs by the platelets 16. After SPIO internalization, the iron nanoparticle-loaded platelets were separated from extracellular SPIO using size-exclusion chromatography, and the platelets were fixed with paraformaldehyde by the same procedures used for the production of hRL-Ps 12, to obtain SPIO-RL platelets.

In vitro and in vivo binding of hRL platelets

hRL-P (2×10⁵ platelets/well) labelled with Green BODIPY or CMF2HC fluorescent dyes (Molecular Probes, Eugene, OR, USA) were used for visualization and quantification of specific binding in vitro of platelets to cultures of HUVEC that were activated with either thrombin (0.01–10Units/ml) or ADP (adenosine 5′-diphosphate, 0.01–10μM). For visualization and quantitation of platelet binding to human prostate endothelial cells perturbed by ADT, human prostate tissue xenografts transplanted to immunocompromised mouse hosts pre-implanted with slow-release pellets of testosterone were employed. Xenografts were maintained for 30days on the host in the presence of human serum levels of testosterone. Control animals were treated with platelets on day 30 post-transplantation (androgen-stimulated or non-castrated). ADT treated animals had the testosterone pellet removed on day 30 post-transplantation, and animals were treated with platelets on day 1, 2 or 3 after ADT 10. At the time of analysis, animals were injected i.v. with hRL-P (10⁶ platelets/μl; 50μl total volume), platelets allowed to circulate for 30min., the vascular volume perfused with saline (3ml) to remove unbound platelets, and the xenografts and select host tissues harvested for analysis of platelet localization. Prostate vasculature-bound platelets were visualized using immunohistochemistry analyses (CD42b immunostaining).

Time of flight secondary ion mass spectroscopy (ToF-SIMS) analysis of xenografts of human prostate tissue incubated in vivo with SPIO-loaded platelets

ToF-SIMS experiments were performed on an ION ToF V 5–100 time of flight secondary ion mass spectrometer (ION ToF, gmbh), equipped with Bi, Cs and C₆₀ primary ion beam sources operated in the high current bunched mode at 25kV. The operation mode utilized for this analysis had an ultimate spatial resolution of 5–7μm which is determined by the beam diameter of the Bi₃⁺⁺ primary ion gun on the ToF-SIMS instrument. A characteristic series of iron ions were identified to be present in isolated SPIO nanoparticles, in hRL-P loaded with SPIOs, and in xenografts tissues harvested from animals treated by IV injection with SPIO-hRL-P. The iron ions detected by ToF-SIMS were Fe, FeH, FeOH, FeO₂H, FeH₃O₄ and Fe₂O₈H. The identification of the individual iron ion species was based on the theoretical mass of each iron containing ion as determined using the IonSpec® software program. The normalized level of iron in the xenograft tissue specimens was determined as the average intensity of five experimental spectra of either xenograft tissue from androgen-stimulated host animals or xenograft tissue harvested from animals on day 3 post-ADT.

Binding of hRL platelets to primary cultures of human endothelial cells

Initial experiments were focused on validation of the ability of fluorescently labelled hRL-P to adhere selectively in vitro to human endothelial cells that were pre-activated by exposure to increasing concentrations of thrombin or ADP. Thrombin, the key regulatory protein of haemostasis, is a potent stimulus for endothelial cell activation 17,18, thrombin-activated hRL-P demonstrated an intracellular stimulus response that was coupled through intracellular kinases 19 and hRL-P degranulated in response to ADP during fibrin clot formation 20. hRL-Ps covalently labelled with Green BODIPY (Fig.1A) or CMF2HC (Fig.1B) dyes were used for visualization and quantification of specific binding to activated HUVEC in culture (Fig.1C). In four independent experiments, activation of HUVEC using either, thrombin or ADP, induced marked increases in adherence of hRL-P (Fig.1D and E). Thrombin-induced adherence increased in a dose-dependent manner, peaking at a thrombin exposure of 0.1U/ml, and decreasing at higher concentrations to levels comparable to un-stimulated HUVEC controls (Fig.1D). This dose–response curve for platelet adherence was similar to published observations for thrombin-induced endothelial cell inter-cellular gap-formation and erythrocyte adhesion, including the curve shape and maximum concentration 17. In contrast, ADP-induced adherence of hRL-Ps to activated HUVEC peaked at an ADP concentration of 1.0μM, and the maximal response plateaued at ADP concentrations between 1.0 and 100μM. These in vitro studies validated previous reports that hRL-P retained the native primary haemostatic function of native platelets 12. Moreover, fluorescent labelling of hRL-Ps did not degrade their central biological activity of binding to activated endothelial cells.

Optical Imaging of in vivo binding of hRL-P to damage human vasculature in primary xenografts of prostate tissue

Fluorescence labelling of RL platelets before injection into animal hosts offered many potential advantages for analysis of platelet localization in histological sections prepared from human prostate. However, prostate tissue is notable for extremely high levels of auto-fluorescence. Consequently, in contrast to the immunofluorescence-based visualization used for the in vitro studies, immuno-histochemical analysis based upon a monoclonal antibody specific for a human platelet marker, CD42b, was utilized for visualization and localization of RL platelets in the human prostate xenografts and host mouse tissues. CD42b is a platelet-specific glycoprotein (GPIb) that serves as a receptor for von Willebrand factor, and it is a high-affinity receptor for thrombin. As proof-of-concept, immuno-histochemical staining with anti-CD42b identified both free RL platelets and RL platelets adherent to activated HUVEC (Fig.2A and B).

Primary xenografts of intact human prostate tissue provide a unique system for characterization of the targeted binding of human platelets to human vasculature acutely damaged by androgen deprivation. Primary xenografts of fresh surgical tissue recapitulate both the tissue architecture of the intact human prostate tissue and the prostate-specific vascular response to ADT. Microvessel density in xenografts of both benign prostate tissue and prostate cancer tissue decreased acutely after ADT, and rebounded to pre-castration levels between days 7–14 post-ADT, in the continued absence of testosterone 10 (Fig.2C).

Analysis of the ADT-induced binding of hRL-Ps to human prostate endothelial cells selectively damaged by ADT revealed a marked increased in adherence of hRL-P within prostate xenografts treated with platelets on day 3 post-initiation of ADT relative to xenografts from androgen-stimulated host mice treated with platelets in a normal androgenic environment (Fig.3A and B). From a clinical/therapeutic perspective, a critical question was whether hRL-P targeted predominantly the transiently damaged human prostate vasculature, with minimal binding to endothelial cells in an intact androgenic environment or in tissues. Selective binding to only the prostate vasculature would minimize collateral morbidity after systemic administration of multi-functional therapeutic vehicles. Tissue harvested from the heart (Fig.3C and D), liver, lungs, spleen and intestine (data not shown) of host control mice, or mice exposed to platelets after ADT, revealed no evidence of hRL-P localization to the microvasculature of host organs. Quantitation of the area occupied by platelets in the post-ADT human prostate xenograft specimens relative to the area occupied by platelets in control human prostate xenograft specimens showed increased adherence of hRL-P in the xenografts on the day 3 after ADT (Fig.3E). To verify the targeting of hRL-P was to the endothelial cells of the transiently damaged human prostate vasculature in the ADT-perturbed xenografts, visualization of localization of hRL-P in the xenografts was performed with dual immuno-histochemical staining for endothelial cells (anti-CD31) and platelets (anti-CD42b). hRL-P (red stain) were demonstrated to co-localize with human prostate endothelial cells (brown stain) only on day 3 post-ADT; hRL-P were not observed to localize in the microvasculature of the prostate xenografts from control animals (non-ADT) injected with platelets, or animals injected with platelets on day 1 post-ADT (Fig.4A–C). These results confirmed that platelets modulated ex vivo by loading with SPIOs retained the haemostatic properties necessary for in vivo haemostasis.

ToF-SIMS chemical images of in vivo binding of bioengineered hRL-P to damage human vasculature in primary xenografts of prostate tissue

Human re-hydrated lyophilized platelets loaded with SPIO nanoparticles before fixation and lyophilization were employed as a proof-of-concept to demonstrate that exogenously bioengineered platelets could serve as a prototype for multi-functional therapeutic vehicles, and could provide a tool for evaluation of the PK/PD characteristics of vehicles that can be targeted specifically to transiently destabilized human prostate vasculature, or possibly the unstable vasculature of tumours. The iron component of the SPIO nanoparticles pre-loaded into the platelets provided a unique tool for validation of organ-specific localization of platelets by identification by ToF-SIMS analysis of the presence of characteristic Fe ions. ToF-SIMS relies on the capacity of the iron to be readily ionizable, and the ions identified in Fig.5 as present in the xenograft tissue on day 3 after castration were identical to those that were identified in the static spectra of SPIO-hRL-P alone. The small mass deviation (±20ppm) between the experimentally observed and theoretical masses of the Fe ions demonstrated that iron ions from SPIO nanoparticles localized in hRL-Ps were the result of the adherence to the ADT-perturbed xenograft vasculature of hRL-P pre-loaded with SPIO (TableS1). Chemical imaging analysis (ToF-SIMS) allowed determination of the relative quantity and crude spatial distribution of SPIO nanoparticles in xenograft tissue samples (Figure5 and Table1). The images in Figure5 show the distribution of the SPIO iron ions in xenograft tissue from animals from control (non-castrate; Fig.5A–C) versus in xenograft tissue on day 3 after initiation of ADT, correlated with adherence of SPIO-hRL-P (Fig.5D–F). The SPIO iron ion signal in the chemical image of the xenografts harvested on day 3 after castration was significantly higher than in the chemical image of the matched control, and the spatial localization of the signals suggests aggregates of platelets, consistent with the IHC observations in histological specimens. Analysis of the relative intensity of the SPIO iron ions in the xenografts from control hosts versus xenografts from hosts after ADT demonstrated approximately a 200-fold increase in SPIO in the xenografts harvested from hosts on day 3 post-ADT (Table1). This data, coupled with the imaging data, demonstrated that mild aldehyde stabilization of fresh platelets, or ex vivo loading of platelets with SPIO nanoparticles, allowed production of a lyophilized platelet product that when re-hydrated (hRL-P) exhibited targeting comparable to fresh platelets.

Data S1. Supplemental experimental procedures.

Table S1. Summary of mass accuracy analysis by TOF-SIMS.

1. Folkman J. Tumor angiogenesis: therapeutic implications. N Engl J Med. 1971;285:1182–6. doi: 10.1056/NEJM197111182852108. [DOI] [PubMed] [Google Scholar]
2. Ebos JM, Kerbel RS. Antiangiogenic therapy: impact on invasion, disease progression, and metastasis. Nat Rev Clin Oncol. 2011;8:316. doi: 10.1038/nrclinonc.2011.21. [DOI] [PMC free article] [PubMed] [Google Scholar]
3. Jain RK. Normalization of tumor vasculature: an emerging concept in antiangiogenic therapy. Science. 2005;307:58–62. doi: 10.1126/science.1104819. [DOI] [PubMed] [Google Scholar]
4. 1Vartanian RK, Weidner N. Endothelial cell proliferation in prostatic carcinoma and prostatic hyperplasia: correlation with Gleason’s score, microvessel density, and epithelial cell proliferation. Lab Invest. 1995;73:844–50. [PubMed] [Google Scholar]
5. Weidner N, Carroll PR, Flax J, et al. Tumor angiogenesis correlates with metastasis in invasive prostate carcinoma. Am J Pathol. 1993;143:401–9. [PMC free article] [PubMed] [Google Scholar]
6. Lissbrant IF, Stattin P, Damber JE, et al. Vascular density is a predictor of cancer-specific survival in prostatic carcinoma. Prostate. 1997;33:38–45. doi: 10.1002/(sici)1097-0045(19970915)33:1<38::aid-pros7>3.0.co;2-5. [DOI] [PubMed] [Google Scholar]
7. Alonzi R, Padhani AR, Taylor NJ, et al. Antivascular effects of neoadjuvant androgen deprivation for prostate cancer: an in vivo human study using susceptibility and relaxivity dynamic MRI. Int J Radiat Oncol Biol Phys. 2011;80:721–7. doi: 10.1016/j.ijrobp.2010.02.060. [DOI] [PubMed] [Google Scholar]
8. Kravchick S, Cytron S, Mamonov A, et al. Effect of short-term dutasteride therapy on prostate vascularity in patients with benign prostatic hyperplasia: a pilot study. Urology. 2009;73:1274–8. doi: 10.1016/j.urology.2008.08.461. [DOI] [PubMed] [Google Scholar]
9. Montecinos VP, Godoy A, Hinklin J, et al. Primary xenografts of human prostate tissue as a model to study angiogenesis induced by reactive stroma. PLoS ONE. 2012;7:e29623. doi: 10.1371/journal.pone.0029623. [DOI] [PMC free article] [PubMed] [Google Scholar]
10. Godoy A, Montecinos VP, Gray DR, et al. Androgen deprivation induces rapid involution and recovery of human prostate vasculature. Am J Physiol Endocrinol Metab. 2011;300:E263–75. doi: 10.1152/ajpendo.00210.2010. [DOI] [PMC free article] [PubMed] [Google Scholar]
11. Fischer TH, Bode AP, Parker BR, et al. Primary and secondary hemostatic functionalities of rehydrated, lyophilized platelets. Transfusion. 2006;46:1943–50. doi: 10.1111/j.1537-2995.2006.01002.x. [DOI] [PubMed] [Google Scholar]
12. Read MS, Reddick RL, Bode AP, et al. Preservation of hemostatic and structural properties of rehydrated lyophilized platelets: potential for long-term storage of dried platelets for transfusion. Proc Natl Acad Sci USA. 1995;92:397–401. doi: 10.1073/pnas.92.2.397. [DOI] [PMC free article] [PubMed] [Google Scholar]
13. Morrison C, Cheney R, Johnson CS, et al. Central quadrant procurement of radical prostatectomy specimens. Prostate. 2009;69:770–3. doi: 10.1002/pros.20925. [DOI] [PMC free article] [PubMed] [Google Scholar]
14. Gray DR, Huss WJ, Yau JM, et al. Short-term human prostate primary xenografts: an in vivo model of human prostate cancer vasculature and angiogenesis. Cancer Res. 2004;64:1712–21. doi: 10.1158/0008-5472.can-03-2700. [DOI] [PubMed] [Google Scholar]
15. Clement O, Siauve N, Cuenod CA, et al. Liver imaging with ferumoxides (Feridex): fundamentals, controversies, and practical aspects. Top Magn Reson Imaging. 1998;9:167–82. [PubMed] [Google Scholar]
16. Oldenburg AL, Gallippi CM, Tsui F, et al. Magnetic and contrast properties of labeled platelets for magnetomotive optical coherence tomography. Biophys J. 2010;99:2374–83. doi: 10.1016/j.bpj.2010.08.007. [DOI] [PMC free article] [PubMed] [Google Scholar]
17. Manodori AB, Matsui NM, Chen JY, et al. Enhanced adherence of sickle erythrocytes to thrombin-treated endothelial cells involves interendothelial cell gap formation. Blood. 1998;92:3445–54. [PubMed] [Google Scholar]
18. Garcia JG. Molecular mechanisms of thrombin-induced human and bovine endothelial cell activation. J Lab Clin Med. 1992;120:513–9. [PubMed] [Google Scholar]
19. Fischer TH, Merricks EP, Russell KE, et al. Intracellular function in rehydrated lyophilized platelets. Br J Haematol. 2000;111:167–74. doi: 10.1046/j.1365-2141.2000.02343.x. [DOI] [PubMed] [Google Scholar]
20. Fischer TH, Merricks EP, Bode AP, et al. Thrombus formation with rehydrated, lyophilized platelets. Hematology. 2002;7:359–69. doi: 10.1080/1024533021000047954. [DOI] [PubMed] [Google Scholar]
21. Dvorak HF. Rous-Whipple Award Lecture. How tumors make bad blood vessels and stroma. Am J Pathol. 2003;162:1747–57. doi: 10.1016/s0002-9440(10)64309-x. [DOI] [PMC free article] [PubMed] [Google Scholar]
22. Bode AP, Fischer TH. Lyophilized platelets: fifty years in the making. Artif Cells Blood Substit Immobil Biotechnol. 2007;35:125–33. doi: 10.1080/10731190600974962. [DOI] [PubMed] [Google Scholar]
23. Fischer TH, Merricks E, Nichols TC, et al. The co-infusion of rehydrated, lyophilized platelets with HBOC-201 for hemostasis in dilutional thrombocytopenia. Blood. 2001;98:2250. [Google Scholar]

Supplementary Materials