Abstract
Purpose: Vascular endothelial growth factor (VEGF) expression is a critical component in tumor growth and metastasis. Capabilities to monitor VEGF expression in vivo can potentially serve as a useful tool for diagnosis, prognosis, treatment planning, monitoring, and research. Here, we present the first report of in vivo hyperspectral molecular imaging strategy capable of monitoring treatment-induced changes in VEGF expression.
Experimental Design: VEGF was targeted with an anti-VEGF antibody conjugated with a fluorescent dye and was imaged in vivo using a hyperspectral imaging system. The strategy was validated by quantitatively monitoring VEGF levels in three different tumors as well as following photodynamic treatment. Specificity of the molecular imaging strategy was tested using in vivo competition experiments and mathematically using a quantitative pharmacokinetic model.
Results: The molecular imaging strategy successfully imaged VEGF levels quantitatively in three different tumors and showed concordance with results from standard ELISA. Changes in tumoral VEGF concentration following photodynamic treatment and Avastin treatment were shown. Immunohistochemistry shows that (a) the VEGF-specific contrast agent labels both proteoglycan-bound and unbound VEGF in the extracellular space and (b) the bound VEGF is released from the extracellular matrix in response to photodynamic therapy. In vivo competition experiments and quantitative pharmacokinetic model-based analysis confirmed the high specificity of the imaging strategy.
Conclusion: This first report of in vivo quantitative optical molecular imaging-based monitoring of a secreted cytokine in tumors may have implications in providing tools for mechanistic investigations as well as for improved treatment design and merits further investigation.
The critical role vascular endothelial growth factor (VEGF) plays in angiogenesis as well as the development of primary, recurrent, and metastatic disease has made it the focus of several investigations as a clinical biomarker for diagnosis, prognosis, and treatment monitoring (1). The role of VEGF in the overall tumor development and treatment response is complex and may depend on the site, individual subjects, and the type of the malignancy (2–6). In particular, several studies (7–9) showed that cancer treatments including photodynamic therapy (PDT), radiotherapy, and chemotherapy can lead to increased tumoral VEGF expression and subsequently to more aggressive disease (10, 11). It would therefore be very useful to establish VEGF levels in vivo and in situ to clearly understand the significance of its expression and alterations both from a mechanistic viewpoint and for the design of improved combination protocols. However, current biochemical assays that determine VEGF concentration ex vivo or from circulation are either invasive and/or limited in sensitivity. Circulating VEGF has been evaluated as a surrogate marker for tumor angiogenesis as well as prognosis only with mixed success, as it is not only specific to tumoral VEGF but also reflects those secreted by other cells such as platelets, granulocytes, monocytes, mast cells, and lymphocytes (12). VEGF levels have also been evaluated directly from the tumor using ex vivo techniques such as immunohistochemistry, but they are invasive, semiquantitative, capture only a temporal snapshot and suffer from procedural variability (4, 13, 14).
Molecular imaging has enabled direct visualization of various molecular targets such as statically anchored cell-surface proteins (15) and enzymatic proteins (16). Similar strategy can lead to in vivo, in situ, quantitative monitoring of not only the overall VEGF expression but also its temporal dynamics and spatial distribution. Capabilities to monitor the spatiotemporal dynamics of VEGF may provide important insights for diagnosis, prognosis, and therapeutic design (17–19). However, in vivo molecular imaging of dynamically secreted cytokines such as VEGF is not developed. A previous study (20) investigated the biodistribution of a radiolabeled anti-VEGF antibody in tumors but did not address the capabilities or limitations of in vivo VEGF monitoring. In the present study, we report the development of an optical molecular imaging strategy to monitor tumoral VEGF expression in vivo. To our knowledge, this is the first systematic study to evaluate the capabilities and limitations of imaging VEGF expression using an exogenous contrast agent. We show that the molecular imaging strategy allows quantitative monitoring of tumoral VEGF levels in different tumor types as well as dynamic changes in VEGF expression following PDT and antiangiogenic therapy with high specificity. This method offers a quantitative and specific paradigm for monitoring the spatial and temporal dynamics of VEGF expression that can help mechanistic investigation of response to cancer therapy.
Materials and Methods
Materials. Avastin anti-VEGF antibody, MLN591 anti-prostate-specific membrane antigen antibody, C225 anti–epidermal growth factor receptor (EGFR) antibody, and benzoporphyrin derivative were a kind gift from Genentech, Millennium Pharmaceuticals, ImClone Systems, and QLT, respectively. Anti-PECAM-1 FITC-conjugated monoclonal antibody (CBL1337F), anti-perlecan antibody (ab23418), and Alexa Fluor 680 fluorescent dye were purchased from Chemicon, Abcam, and Invitrogen, respectively.
Conjugation of antibody with fluorescent dye. VEGF-specific contrast agent (CAVEGF) was formulated by conjugating Avastin with Alexa Fluor 680 fluorescent dye with succinimidyl esters according to manufacturer's specifications. Briefly, 10 mg/mL Avastin (250 μL) was mixed with 1 mol/L sodium bicarbonate buffer (25 μL) and 10 mg/mL fluorescent dye (25 μL). The mixture was incubated for 1 h at room temperature. To separate the CAVEGF from the unconjugated dye, the mixture was eluted in a PD-10 desalting column (Amersham Biosciences). MLN591 was conjugated with Alexa Fluor 680 fluorescent dye with succinimidyl ester in a similar manner. The antibody/fluorescent dye molar ratio resulting from the reaction was determined according to the manufacturer's specifications using the absorbance at 280 and 679 nm for the antibody and the fluorescent dye, respectively. All absorbance readings were measured in a quartz cuvette using the 8453 UV-visible spectrophotometer (Agilent Technologies). The average ± SE molar ratio from nine conjugations throughout the experiment was 5.96 ± 0.22, showing a high level of uniformity of the conjugation reaction.
Animals. PC-3 prostate cancer cells, AsPC-1 pancreatic cancer cells, or Capan-1 pancreatic cancer cells (3 × 106) in 50 μL Matrigel (BD Biosciences) were injected s.c. in both left and right hind flanks of severe combined immunodeficient mice. The tumor was allowed to grow to a size of 5 to 6 mm in 2 weeks. All animal studies were approved by the Subcommittee on Research Animal Care at the Massachusetts General Hospital.
In vivo fluorescence imaging and calibration. Either CAVEGF or the MLN591-Alexa Fluor 680 conjugate (100 μg) was delivered via i.v. injection in the tail vein of the tumored mouse. A single injection of 100 μg Avastin in mice is a subtherapeutic dose that has not been shown to induce therapeutic effect on these tumors (data not shown). One hour following the delivery of the conjugated antibody, photosensitizer or PBS (100 μL) was injected i.v. in the tail vein in the PDT-treated mice and nontreated mice, respectively. PDT was then done according to the procedure outlined below. To allow sufficient tumoral delivery and target binding of the conjugated antibody, wavelength-resolved fluorescence hyperspectral images of the tumor were acquired with the Maestro imaging system (CRI) 24 h following the delivery of the conjugated antibody unless specified otherwise. The tumor was exposed during the imaging procedure to eliminate any potential optical distortion through skin and thus enhance accuracy of the model-based quantitative image analysis. A 615- to 665-nm excitation filter and a 700-nm long-pass emission filter (M-MSI-FLTR-640) were used to acquire fluorescence images of Alexa Fluor 680. Hyperspectral images were acquired between 700 and 800 nm at 10-nm intervals. Any potential variation in imaging system sensitivity was accounted for by calibrating spectrally unmixed CAVEGF images with Oxazine 725 (Exciton), a highly photostable laser dye with fluorescence characteristics similar to Alexa Fluor 680 (21). A quartz cuvette containing 200 nmol/L Oxazine laser dye was imaged with the Maestro imaging system before each imaging session and subsequently acquired images were normalized by the fluorescence intensity of the laser dye. CAVEGF fluorescence was quantified by spectrally unmixing Alexa Fluor 680 fluorescence spectrum with the tissue autofluorescence spectrum using linear least-squares optimization.
Photodynamic therapy. Photosensitizer was delivered to the tumored mouse by i.v. injection of 0.25 mg/kg benzoporphyrin derivative in the tail vein. One hour following photosensitizer delivery, an incision was made on the skin to expose the s.c. tumor and a 690-nm diode laser module (High Power Devices) was irradiated on the tumor at an irradiance of 100 mW/cm2 and a fluence of 50 J/cm2. Following PDT, the incision was closed using 9-mm wound clips (BD Diagnostics).
ELISA. Tumors were harvested 24 h following PDT and frozen in liquid nitrogen. The frozen tumors were pulverized with a tissue homogenizer and lysed in lysis buffer. The total protein concentration was determined using a standard Lowry method. A human VEGF DuoSet ELISA Development System (R&D Systems) was used to quantify human VEGF levels. Resulting VEGF concentrations were normalized by total protein concentration.
Immunofluorescence. To count the microvessel density (MVD), tumors were harvested immediately following in vivo fluorescence imaging. The tumors were embedded in OCT compound and sectioned into 5-μm-thick cryosections. The sections were air dried, fixed in acetone, and incubated with anti-mouse PECAM-1 FITC-conjugated antibody overnight at 4°C. Average MVD was calculated by averaging the number of CD31+ vessel structures counted from five randomized fields per tumor section at a magnification of ×200 under the Olympus BX-51 fluorescence microscope.
To study tumoral localization of CAVEGF, tumors were harvested 24 h following i.v. injection of CAVEGF and PDT, embedded in OCT compound, and sectioned into 5-μm-thick cryosections. To stain for EGFR, the sections were blocked with 1% bovine serum albumin and incubated with C225 antibody-Alexa Fluor 488 conjugate overnight at 4°C. To stain for perlecan, the sections were fixed in acetone, blocked with 1% bovine serum albumin, and incubated with anti-perlecan antibody (ab23418)-Alexa Fluor 488 conjugate overnight at 4°C. Slides were imaged using a Leica LCS laser scanning confocal microscope with a ×100 oil immersion objective.
Model-based quantitative analysis. A standard curve to convert fluorescence intensity from the acquired images into CAVEGF concentration was generated from fluorescence images of pulverized s.c. tumor mixed with known concentration (0, 5, 10, 20, and 30 nmol/L) of CAVEGF loaded into 384-well plates. A mathematical pharmacokinetic model describing antibody uptake in solid tumors (22) was applied to estimate VEGF-bound and unbound tumoral CAVEGF concentrations ([CAVEGF]Bound and [CAVEGF]Free, respectively) from the contrast agent labeling. The model describes the temporal kinetics of [CAVEGF]Total (sum of [CAVEGF]Bound and [CAVEGF]Free) in the tumor compartment and [CAVEGF]Plasma in the plasma compartment in terms of CAVEGF binding affinity (Ka) and plasma pharmacokinetics (λ1, λ2), tumoral VEGF concentration (B0), the vascular permeability-surface area product (PS), as well as the rate of antibody loss from the tumor (L).
Plasma compartment:
.
Tumor compartment:
.
Among the input variables to the model, the Ka of CAVEGF was set to that of Avastin (9.1 × 108 mol/L-1; ref. 23), as the molar ratio of antibody/fluorescent dye below 10 does not significantly affect the Ka (24–26). Initial and terminal circulation half-lives of CAVEGF, λ1 and λ2, were set to those of Avastin (1.2 h and 6.81 days, respectively) measured in mice (27). Although not reported, the SD of the Avastin circulation half-life in mice is expected to be ±15% based on measurements in rats (27). B0 was set to the results of the ELISA. The two unknown input variables (PS and L) were iteratively adjusted using the Gauss-Newton algorithm to fit the mathematical model to the observed contrast agent labeling. [CAVEGF]Bound and [CAVEGF]Free were then calculated using the estimated PS and L as well as the tumoral VEGF concentration, binding affinity, and murine circulation half-life of Avastin.
Statistics. Data are presented as mean ± SE. The significance of the difference between groups was evaluated with unpaired Student's t test. Pearson correlation coefficient (r) and the corresponding P value were used to investigate the strength and the significance of the correlation between CAVEGF fluorescence and MVD, respectively. P < 0.05 was considered statistically significant.
Results
Monitoring VEGF levels in different tumors. We initially tested the molecular imaging strategy in s.c. tumors from three different human cancer cell lines that express different levels of VEGF: one from prostate cancer (PC-3) and two from pancreatic cancer (AsPC-1 and Capan-1). Temporal kinetics of CAVEGF labeling in each tumor was monitored by acquiring images at 1, 3, 6, and 24 hours following i.v. injection of the CAVEGF. The fluorescence intensity increased during the first 6 hours and leveled by 24 hours, suggesting that CAVEGF uptake has saturated (Fig. 1A). To confirm that the fluorescent dye remains conjugated to the antibody throughout the 24-hour imaging period, we monitored the fluorescence of the unconjugated dye within the tumor following i.v. injection of an equivalent dose (4 nmol unconjugated Alexa Fluor 680). Ninety percent of the dye fluorescence cleared within 5 hours of injection (data not shown). The rapid clearance of the unconjugated dye suggests that the CAVEGF fluorescence observed at 24 hours following injection originates from the fluorescent dye conjugated to Avastin. To validate that CAVEGF labeling corresponds to tumoral VEGF levels, tumoral VEGF concentration was quantified ex vivo using ELISA. Good correlation with the results of the biochemical assay (Fig. 1B) shows that average fluorescence intensity of CAVEGF labeling at 24 hours is indicative of VEGF levels in different tumor types.
In all three tumors, Pearson's statistic showed a linear association (r = 0.64, P < 0.05) between CAVEGF fluorescence and MVD among the tumor samples from three different cell lines (Fig. 1C). It is important to note that VEGF is one of many angiogenic molecules (28). As a result, not all tumor types may show strong correlation between tumoral VEGF levels and MVD. However, a positive linear association shows that tumoral VEGF measured with CAVEGF plays an important role in angiogenesis (29). Vasculature was not observed in some of the s.c. PC-3 tumors partly because the vasculature in these tumors may not have fully developed at 2 weeks following implantation (data not shown) as well as due to random sampling of the image field within a section of the tumor.
Monitoring VEGF up-regulation following PDT. To test the feasibility of monitoring treatment response with the molecular imaging strategy, CAVEGF labeling was imaged in nontreated and PDT-treated s.c. PC-3 tumors. Figure 2A shows the typical images of CAVEGF labeling in a PDT-treated tumor and a nontreated tumor at different time points following laser irradiation. Statistically significant increase in CAVEGF labeling was observed in PDT-treated tumors as early as 1 hour post-PDT and continued up to 24 hours post-PDT (Fig. 2B).
To validate that the increase in CAVEGF labeling corresponds to post-PDT changes in VEGF expression, tumoral VEGF concentration was quantified ex vivo with ELISA from PDT-treated tumors harvested at 24 and 72 hours following treatment. At both time points, PDT-treated tumors showed a 2-fold increase in both tumoral VEGF concentration and CAVEGF labeling, suggesting that the molecular imaging strategy can be used to monitor relative changes in VEGF expression following PDT (Fig. 2C).
To further understand the capabilities of the molecular imaging strategy, spatial localization of the CAVEGF was studied using frozen sections from PDT-treated and nontreated s.c. PC-3 tumors. The sections were stained for human EGFR to visualize the tumor cells (Fig. 2D). Similar to in vivo imaging, increased CAVEGF labeling was observed in sections from PDT-treated tumors compared with nontreated tumors. More importantly, CAVEGF labeling did not colocalize with EGFR staining, suggesting that the CAVEGF localizes in the extracellular space and binds to the secreted form of VEGF. VEGF are known to bind to heparan sulfate proteoglycans on cell surface as well as in the basement membrane (30). To investigate the role of proteoglycans, we stained the frozen tumor sections for perlecan, one of the most abundant forms of proteoglycan in tissue (Fig. 2D). In nontreated tumor sections, partial colocalization of the perlecan staining with the CAVEGF is observed, suggesting that the contrast agent labels proteoglycan-bound VEGF as well as those that are unbound. It is interesting to note that colocalization of the perlecan staining with the CAVEGF is not observed in PDT-treated tumor sections, suggesting that most of the VEGF proteins have been released from the extracellular matrix in response to PDT.
Specificity of CAVEGF against VEGF. To investigate CAVEGF specificity against VEGF in vivo, we did an in vivo antigen blocking experiment. Tumored mice were pretreated with i.v. injection of either 300 μg or 1 mg Avastin 24 hours before PDT. As shown in Fig. 3A, the pretreatment resulted in a decrease in CAVEGF labeling proportional to the dose of Avastin. To further validate that Avastin pretreatment specifically blocks the VEGF protein, tumored mice were pretreated 24 hours before PDT with i.v. injection of either 1 mg bovine serum albumin or 1 mg MLN591 anti-prostate-specific membrane antigen antibody that do not bind to VEGF and should not affect CAVEGF labeling. Pretreatment with bovine serum albumin and with MLN591 did not result in a statistically significant change in CAVEGF labeling (Fig. 3B).
PDT is known to induce physiologic changes in vascular permeability (31), which could increase tumoral CAVEGF uptake regardless of the changes in tumoral VEGF concentration. The effect of PDT-induced vascular permeability on labeling of antibody-based contrast agents was investigated using MLN591, as prostate-specific membrane antigen expression does not change with PDT in s.c. PC-3 tumors (data not shown). In vivo labeling of MLN591 conjugated with Alexa Fluor 680 did not show significant difference between PDT-treated and nontreated tumors (Fig. 3C), suggesting that the PDT treatment did not result in nonspecific uptake of the fluorescently labeled antibody.
Targeting efficiency of CAVEGF. Although Fig. 3 shows specificity of CAVEGF against VEGF, it is not clear how much tumoral VEGF is labeled by CAVEGF. To study the targeting efficiency, average CAVEGF fluorescence intensity in Fig. 1A was converted to total tumoral CAVEGF concentration using a standard curve generated with pulverized tumors (Supplementary Fig. S1). Then, [CAVEGF]Bound and [CAVEGF]Free were determined by fitting the mathematical model to the total tumoral CAVEGF concentration determined from the fluorescence images (Supplementary Fig. S2). Table 1 shows the values of PS and L estimated by the model-based quantitative analysis and the resulting [CAVEGF]Bound and [CAVEGF]Free. The estimates of PS and L were comparable with values determined in tumors (22, 32). The ratio of [CAVEGF]Bound and [CAVEGF]Free shows approximately 80% of CAVEGF delivered to the tumor are bound to VEGF in all three tumors, confirming CAVEGF specificity. However, CAVEGF delivered to the tumor labels only about 40% to 60% of the total tumoral VEGF determined by ELISA (Fig. 4).
. | [VEGF] (nmol/L)* . | [CAVEGF]Bound (nmol/L)† . | [CAVEGF]Free (nmol/L)† . | PS (mL/min/g)†,‡ . | L (mL/min/g)†,‡ . |
---|---|---|---|---|---|
PC-3 | 10.1 ± 0.2 | 5.1 ± 0.07 | 1.1 ± 0.03 | 0.08 ± 0.005 | 6.4 ± 0.3 |
AsPC-1 | 11.7 ± 0.2 | 5.8 ± 0.1 | 1.1 ± 0.05 | 0.12 ± 0.006 | 10.0 ± 0.0 |
Capan-1 | 15.6 ± 0.3 | 8.6 ± 0.1 | 1.3 ± 0.04 | 0.14 ± 0.01 | 9.6 ± 0.3 |
. | [VEGF] (nmol/L)* . | [CAVEGF]Bound (nmol/L)† . | [CAVEGF]Free (nmol/L)† . | PS (mL/min/g)†,‡ . | L (mL/min/g)†,‡ . |
---|---|---|---|---|---|
PC-3 | 10.1 ± 0.2 | 5.1 ± 0.07 | 1.1 ± 0.03 | 0.08 ± 0.005 | 6.4 ± 0.3 |
AsPC-1 | 11.7 ± 0.2 | 5.8 ± 0.1 | 1.1 ± 0.05 | 0.12 ± 0.006 | 10.0 ± 0.0 |
Capan-1 | 15.6 ± 0.3 | 8.6 ± 0.1 | 1.3 ± 0.04 | 0.14 ± 0.01 | 9.6 ± 0.3 |
Variable that was determined ex vivo by ELISA and input to the pharmacokinetic model.
Margin of error was derived from a potential 15 % variation in CAVEGF circulation half life.
Variables estimated by the pharmacokinetic model.
Discussion
VEGF plays a pivotal role in tumor angiogenesis, tumor growth, and metastasis and has been widely reported as a significant prognostic indicator of patient survival (33–36). At the same time, there are reports that VEGF does not provide significant prognostic information (4, 6, 37). In fact, the xenograft models of human pancreatic cancer show higher level of VEGF with the AsPC-1 cell line compared with Capan-1 (Fig. 1), but it is the Capan-1 that develops into a more aggressive phenotype (38, 39). The understanding of the complexity of the role VEGF plays in tumor development has been somewhat limited by the absence of methods of in situ measurement of this cytokine spatially and temporally. Although the snapshot of VEGF levels measured in circulation or ex vivo may reflect overall VEGF levels, subtle differences in its spatial distribution and temporal change can have a major effect on prognosis and treatment response. For example, localized microenvironmental VEGF concentration and the spatial redistribution of VEGF in different tissue compartments have been shown to play an important role in aberrant angiogenesis and cancer progression (18, 19, 40). As a result, capabilities to monitor the spatial and temporal dynamics of VEGF expression in vivo can provide more robust and accurate information regarding disease progression and appropriate targeted intervention strategies.
Here, we developed an optical molecular imaging strategy to monitor VEGF expression and its dynamics in various tumors and following cancer therapy. Average CAVEGF labeling in three different tumors (Fig. 1) as well as following PDT (Fig. 2) correlated well with the tumoral VEGF concentration determined ex vivo. Furthermore, a more quantitative analysis using a pharmacokinetic model shows that in vivo CAVEGF labeling is proportional to and labels approximately half of the tumoral VEGF concentration (Fig. 4), demonstrating that the VEGF imaging strategy can be used to monitor the tumoral VEGF levels. The fact that in vivo CAVEGF labeling is associated with the MVD further shows that VEGF detected by the imaging strategy is functionally active in promoting angiogenesis (Fig. 1C).
Because of its complexity, the in vivo environment can lead to nonspecific binding of molecular specific contrast agents. In particular, in vivo specificity of contrast agents targeted at nonanchored cytokines has not been studied previously. We rigorously tested the specificity of CAVEGF using various approaches. In vivo antigen blocking experiment shows that Avastin pretreatment before imaging blocks the tumoral VEGF and that CAVEGF labeling decreased in proportion to the pretreated Avastin dose, showing that CAVEGF specifically binds to the VEGF protein in vivo (Fig. 3). In fact, quantitative analysis using the pharmacokinetic model shows approximately 80% of the CAVEGF delivered to the tumor is bound to VEGF (Fig. 4). In addition to the specificity of the contrast agent to its antigen, any physiologic changes could also affect the specificity of the contrast agent labeling. Investigation with a fluorescently labeled antibody against prostate-specific membrane antigen, whose levels do not change with PDT, showed that PDT conditions used in this study do not affect the delivery of antibody-based contrast agents to the tumor (Fig. 3). However, it is still possible that vascular targeting PDT resulting in a significant change in vascular permeability (31) could potentially increase nonspecific uptake of antibody-based contrast agents as observed in ref. 41.
In addition to analyzing the overall CAVEGF labeling in tumors, microscopic localization of CAVEGF was investigated using immunohistochemistry of tumors labeled with CAVEGF in vivo (Fig. 2D). CAVEGF did not colocalize with EGFR staining, suggesting that the contrast agent labels the VEGF proteins localized in the extracellular space. More importantly, potential release of VEGF from extracellular matrix following PDT was observed from sections stained for proteoglycans. Although the precise mechanism needs further investigation, PDT-generated reactive oxygen could potentially degrade proteoglycans and release heparin-binding growth factors (42). Along with cell-secreted VEGF (9), heparin-binding VEGF released from the extracellular matrix by PDT may also play an important role in tumor growth and metastasis (43). These microscopic temporal and spatial details can potentially be probed in vivo and in a minimally invasive manner by combining the VEGF imaging strategy with high-resolution fluorescence endoscopic imaging system (44).
Capabilities to monitor VEGF expression following cancer treatment is particularly important as cancer treatments including radiotherapy (7), chemotherapy (8), and PDT (9) can lead to increased expression of VEGF and potentially stimulate tumor regrowth and metastasis to distant organs (10, 11). Combination with antiangiogenic therapies enhanced the antitumor effect and reduced the metastatic burden of these treatments (45, 46), strongly suggesting that post-treatment VEGF expression plays an important role in recurrent disease and metastasis. Capabilities of the in vivo optical molecular imaging strategy to monitor changes in tumoral VEGF expression following PDT can potentially be used to monitor the response in these different treatment modalities.
In addition to contrast agent specificity, decrease in CAVEGF labeling following Avastin pretreatment (Fig. 3A) also show the capabilities to monitor the pharmacodynamics of Avastin, an antiangiogenic agent. In situ, in vivo monitoring of antiangiogenic agent pharmacodynamics can potentially help optimize treatment planning for these novel therapies (47). As a result, the in vivo VEGF imaging strategy reported here can potentially help predict the treatment response, monitor the pharmacodynamics of antiangiogenic agents, and plan appropriate intervention strategies.
As shown in Fig. 4, the concentration of [CAVEGF]Total is approximately 50% of the tumoral VEGF concentration, suggesting that CAVEGF labels approximately half the VEGF protein in the tumor. The relatively low targeting efficiency could be partly explained by the fact that the ex vivo ELISA assay measures both the intracellular and the extracellular VEGF, whereas the contrast agent targets only the extracellular protein. Another possible explanation is the limited penetration of antibodies in solid tumors (48), compromising the delivery of antibody-based CAVEGF in tumor regions distant from blood vessels. The targeting efficiency of the CAVEGF can potentially be improved by using targeting agents other than antibodies with enhanced tumor penetration.
Optical imaging, particularly planar macroscopic imaging used in this report, is inherently limited by the depth of light penetration in tissue (∼2 mm; ref. 49). However, recent advances in optical imaging technologies such as endoscopy (44) can help access to organs deep inside the body. Tumors that are large in size can still pose a challenge due to limited field of view and depth of imaging associated with optical technologies. Advances in optical imaging technologies such as diffuse optical tomography will potentially enable interrogation of whole organs (50). At the same time, the molecular imaging strategy investigated in this report can be applied to other imaging modalities with whole-body imaging capabilities such as nuclear imaging if interrogation of a large volume is necessary. The molecular imaging strategy described in this report in combination with these technologies can help monitor VEGF expression in vivo in various organ sites.
In summary, we report an optical molecular imaging strategy to monitor VEGF expression in vivo. Experimental results show that the antibody-based CAVEGF labeled VEGF proteins with high specificity. The molecular imaging strategy was capable of monitoring VEGF levels in different tumors as well as changes in VEGF expression following a therapeutic intervention such as PDT and Avastin treatment. These capabilities could potentially serve as a useful tool for monitoring treatment response, studying mechanisms, and designing appropriate mechanism-based interventions in the future.
Disclosure of Potential Conflicts of Interest
No potential conflicts of interest were disclosed.
Grant support: NIH grant P01 CA84203.
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Note: Supplementary data for this article are available at Clinical Cancer Research Online (http://clincancerres.aacrjournals.org/).
Current address for I. Rizvi: Thayer School of Engineering, Dartmouth College, Hanover, NH. Current address for N. Solban: Acceleron Pharma, 24 Emily Street, Cambridge, MA 02139.
Acknowledgments
We thank Genentech for Avastin, Millennium Pharmaceuticals for MLN591, ImClone Systems for C225, and QLT for benzoporphyrin derivative.