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Published in final edited form as: J Pain. 2012 Apr 5;13(6):524–531. doi: 10.1016/j.jpain.2012.01.006

Analgesia targeting IB4-positive neurons in cancer-induced mechanical hypersensitivity

Yi Ye 1, Dongmin Dang 1, Chi T Viet 2, John C Dolan 1,3, Brian L Schmidt 1,2,*
PMCID: PMC3786360  NIHMSID: NIHMS504163  PMID: 22483679

Abstract

Cancer patients often suffer from pain and most will be prescribed μ-opioids. μ-opioids are not satisfactory in treating cancer pain and are associated with multiple debilitating side effects. Recent studies show that μ and δ opioid receptors are separately expressed on IB4 (−) and IB4 (+) neurons which control thermal and mechanical pain, respectively. In this study we investigated IB4 (+) and IB4 (−) neurons in mechanical and thermal hypersensitivity in an orthotopic mouse oral cancer model. We used a δ opioid receptor agonist and a P2X3 antagonist to target IB4 (+) neurons and to demonstrate that this subset plays a key role in cancer-induced mechanical allodynia, but not in thermal hyperalgesia. Moreover, selective removal of IB4 (+) neurons using IB4-SAP impacts cancer-induced mechanical but not thermal hypersensitivity. Our results demonstrate that peripherally administered pharmacological agents targeting IB4 (+) neurons, such as a selective δ-opioid receptor agonist or P2X3 antagonist, might be useful in treating oral cancer pain.

Perspective

To clarify the mechanisms of oral cancer pain, we examined the differential role of IB4 (+) and IB4 (−) neurons. Characterization of these two subsets of putative nociceptors is important for further development of effective clinical cancer pain relief.

Keywords: δ-opioid receptor (DOR), μ-opioid receptor (MOR), NGF, isolectin B4, cancer pain

Introduction

Pain represents one of the worst symptoms for cancer patients and remains the most difficult to treat. Opioid analgesics (e.g., morphine) that target μ opioid receptors (MORs) are the most common therapy for cancer pain. Although μ opioids are initially effective for cancer pain management, they are associated with undesired side effects, including opioid tolerance, physical dependence, nausea, respiratory depression, constipation, and immunosuppression11, 14. There is no effective analgesic regimen for treating intractable cancer pain. As a result, patients often experience agonizing pain and resultant debilitation if tolerance to MORs agonists develops.

The contribution by δ opioid receptor (DORs) to cancer pain is not as well characterized as that of MORs. Some studies report that DOR agonists produce potent analgesia in several pain conditions including bone cancer pain in animal models9, 15, 30, 56. Moreover, DOR agonists produce minimal side effects and do not lead to tolerance13, 15, 30. These characteristics make them a promising alternative for the treatment of cancer pain.

Recently it has been shown that MORs and DORs are expressed in different subsets of putative nociceptors that serve distinct functions 46. DORs are located on IB4 (+) neurons and DOR agonists produce analgesia to mechanical pain with no effect on thermal pain. In contrast, MORs are expressed on IB4 (−) neurons and MOR agonists reduce heat pain without affecting mechanical pain. However, the complete segregation between MORs and DORs in mice has been challenged recently 59. Nevertheless, IB4 (+) and IB4 (−) neurons differ in their neurochemical expression, sensitivity to neurotrophins, electrophysiological properties, and anatomical locations, which might ultimately lead to distinct functions 18, 21, 35, 41, 52, 53. IB4 (−) neurons express TrkA receptors that bind nerve growth factor (NGF), depend on NGF for survival, express substance P (SP) and calcitonin gene-related peptide (CGRP) 4, 36. In contrast, IB4 (+) neurons express receptors for glial cell line-derived neurotrophic factor (GDNF), depend on GDNF for survival, express P2X3 receptors, and have poor expression of SP and CGRP 3, 5, 8, 22, 37, 58. Centrally, IB4 (+) neurons terminate predominantly in inner lamina II whereas IB4 (−) neurons terminate in lamina I and outer lamina (II) 36, 51. Despite distinct characteristics of the two subsets, the specific function of IB4 (+) and IB4 (−) neurons is not known in oral cancer pain.

NGF, which primarily acts on IB4(−)/TrkA(+) neurons, plays a role in pancreatic cancer pain 62 as well as bone cancer pain 23, 34, 47. Neutralizing NGF attenuates both spontaneous and movement-evoked pain in mice with both cancer 23, 34, 47. Oral squamous cell carcinoma (OSCC), which is characterized by mechanical allodynia and is clinically distinct from bone cancer, also expresses high levels of NGF16, 28, 61. The limited antinociceptive effect of anti-NGF in our OSCC mouse paw model 61 implies that IB4 (−)/TrkA (+) neurons are not solely responsible for carcinoma-induced mechanical pain. The involvement of IB4 (+) neurons in oral cancer pain has never been studied. It is also unknown whether OSCC cells secrete neurotrophins from the GDNF family that can activate and sensitize IB4 (+) neurons. GDNF and neurturin are particularly of interest as they both maintain a subset of IB4 (+)/ P2X3 (+) neurons that do not express CGRP 2, 32. In addition, GDNF has been shown to reduce mechanical thresholds of IB4 (+) neurons 7, 38.

In the present study, we examined the role of IB4 (+) and IB4 (−) neurons in processing mechanical and thermal nociception following OSCC supernatant injection in mice. In addition, we evaluated whether pharmacological agents such as P2X3 antagonist and DOR agonist are effective against OSCC-induced nociception.

Materials and Methods

Experimental animals

42 male C57BL/6 mice (6–8 weeks old, Charles River Laboratories, Hollister, CA) were used in this study. They were exposed to a light-dark cycle (L:D 12:12-h) and kept in a temperature-controlled room with food and water ad libitum. All procedures were approved by the New York University Institutional Animal Care and Use Committee.

Cell culture

The human tongue SCC cell line, HSC-3 (ATCC, Manassas, VA), and human normal oral keratinocytes (NOK) were cultured at 37 °C with 5% CO2. Both cell cultures were grown to confluence and then washed to remove all unattached cells. The media for both SCC and NOK cell cultures were replaced with Defined Keratinocyte–Serum Free Media (SFM) and then further incubated for 72 h prior to supernatant collection for behavioral testing and ELISA, as we previously described 29.

Intrathecal administration of IB4-saporin

2μl of IB4-SAP (1.2mg/ml, 53% saporin/mole IB4) or 3μl unconjugated saporin (SAP) (1mg/ml) (Advanced Targeting Systems, San Diego, CA) was diluted with PBS to a total volume of 8μl were anesthetized with 2.5% isoflurane. With the use of a Hamilton syringe, IB4-SAP (n=6 mice) or SAP (control, n=6 mice) was injected into the subarachnoid space on the midline between the L4 and L5 vertebrae. All behavioral testing of IB4-SAP and SAP treated mice was performed 14 days after injection.

Supernatant injection and behavioral testing

50μl supernatant from HSC-3 or NOK cells was injected in the mid-plantar right hind paw of each mouse (n=6 in each group) 29. Our previous study demonstrated that HSC-3 supernatant induced mechanical allodynia for a duration of 3 or more hours 29. In this current study, mechanical sensitivity was measured 1 hr post-injection using an electronic von Frey anesthesiometer (IITC Life Science, Woodland Hills, CA). The withdrawal-threshold was defined as the force (g) that was sufficient to elicit a withdrawal response. Six measurements were taken for each animal. Thermal sensitivity was measured using a paw thermal stimulator (Hargreaves’ Apparatus, Department of Anesthesiology, UC San Diego, La Jolla, CA). Mice were placed in plastic chambers on a heated glass surface (25°C). A radiant heat source was focused on the hindpaw and latency to withdraw was measured as the average of 6 trials per animal taken ≥ 5 minutes apart. The cutoff latency was set at 20 seconds to avoid tissue damage. In all behavioral experiments, the observer was blind to the treatment groups.

Drugs

TNP-ATP is a selective P2X antagonist which potently blocks P2X1, P2X3, and heteromeric P2X2/3 receptors. SNC80 is a highly selective agonist for DORs. Naltrindole (NTI) is a selective DOR antagonist. SNC80 (Tocris Bioscience, Ellisville, MI) was dissolved in sterile acidic (0.2% HCl) saline solution. NTI (Sigma, St. Louis, MO), TNP-ATP (Sigma, St. Louis, MO), and NGF neutralizing antibody (Mab 256, R&D Systems, San Jose, CA) were mixed directly into 50μl of cancer supernatant and injected into the right hind paw of the mice 1h prior to behavioral testing. 10nmol of SNC80, 0.2nmol NTI, 2μmol TNP-ATP, and 12.5μg anti-NGF were administered to each animal. Drug dosage was based on previous findings 1, 24, 46.

IB4 labeling

Animals were euthanized with 4% isoflurane and perfused with cold 0.1M PBS solution followed by 4% paraformaldehyde (PFA). The spinal cord was removed, post-fixed in 4% PFA, and cryo-protected in sucrose gradient (20%–50%) at 4°C. Serial frozen spinal cord sections (12μm) were cut on a cryostat and thaw-mounted on gelatin-coated slides for processing. Following tissue sectioning, spinal cord sections were briefly rinsed in PBS and then incubated in 5% goat serum in PBS with 0.1% Triton X-100 for 1h followed by incubation overnight in IB4-FITC (1:400 Sigma, St. Louis, MO). The specificity of IB4-FITC was reported in previous studies 25, 55, and was confirmed by distinct patterns of IB4 and SP labeling in the spinal cord (data not shown). Image analysis was performed using NIH Image J software. The area of staining was outlined and pixel density within the selected area was then measured and divided by the total area. Data were collected from 6 randomly selected sections from 3 animals per treatment group.

ELISA measurement of GDNF and Neurturin

Supernatant content of GDNF and neurturin from both HSC-3 cells and NOKs was measured using human GDNF (RayBiotech, Inc., Norcross, GA) and neurturin ELISA kit (Antigenix America, Inc, Huntingston Sta, NY), respectively. The optical density of the standards and samples was read at 450 nm wavelength using a Model 680 Microplate Reader (Bio-Rad Laboratories, Inc., Hercules, CA). All samples (n=3) were run in quadruplicate.

Statistical analysis

The statistics software SigmaPlot for Windows (version 11.0) was used to perform Students’ t test, or one-way ANOVA for Multiple Comparisons. Significance level was set at P < 0.05. Results are presented as mean ± SEM.

Results

OSCC supernatant induces both mechanical and thermal hypersensitivity

Consistent with our previous findings 29, intraplantar injection of OSCC supernatant induced significant mechanical allodynia as shown by decreased paw withdrawal thresholds to mechanical stimulation (Fig. 1A). In addition, we showed that OSCC supernatant produced thermal hyperalgesia. The paw withdrawal latency to noxious heat stimulus in OSCC supernatant-treated mice was shorter than vehicle treated ones (Fig. 1B).

Figure 1.

Figure 1

OSCC supernatant injected into the mice hind paws resulted in both mechanical and thermal hypersensitivity. A. OSCC supernatant decreased paw withdrawal latency to mechanical stimulus compared with normal oral keratinocytes (NOK) supernatant injection in mice. B. OSCC supernatant decreased paw withdrawal latency to thermal stimulus compared with NOK supernatant injection in mice. ***P<0.001

Both IB4 (+) and IB4 (−) neurons mediate OSCC supernatant-induced mechanical allodynia

We first treated mice with DOR selective agonist SNC80 mixed in OSCC supernatant. SNC80 significantly inhibited OSCC supernatant-induced mechanical allodynia (Fig. 2A, n=6). The anti-nociceptive action of SNC80 on mechanical allodynia was blocked by co-administration of a low dose of the DOR selective antagonist naltrindole (Fig. 2A). Since a proportion of IB4 (+) neurons express the purinergic receptor P2X3, we used the P2X3 antagonist TNP-ATP to determine whether antagonism of P2X3 blocks OSCC induced mechanical hypersensitivity. TNP-ATP also reduced OSCC supernatant induced mechanical allodynia (Fig. 2A). Involvement of IB4 (+) nociceptors in OSCC-induced mechanical hypersensitivity is further confirmed by selective ablation of IB4 (+). Two weeks after the intrathecal administration of IB4-SAP, IB4 (+) neurons in the dorsal horn of the spinal cord degenerated. As shown in figure 3, IB4 (+) labeling was significantly decreased in the spinal cord of IB4-SAP treated mice compared to SAP-treated controls. Pretreatment with IB4-SAP (n=6) eliminated mechanical hypersensitivity induced by cancer supernatant (Fig. 2A) while mechanical hypersensitivity remained in SAP injected controls. The mechanical thresholds of SAP control mice were not significantly different from naïve control mice after OSCC supernatant injection.

Figure 2.

Figure 2

IB4 (+) and IB4 (−) neurons in OSCC-induced nociceptive behaviors. A. OSCC-induced mechanical allodynia was attenuated by DOR selective agonist SNC80 and P2X3 antagonist TNP-ATP. The effect of SNC80 was blocked by coadministration of DOR selective antagonist naltrindole (NTI). Note that anti-NGF was also effective in blocking OSCC-induced mechanical allodynia. Removal of IB4 (+) neurons by IB4-SAP significantly abolished OSCC-induced mechanical allodynia. B. SNC80 or TNP-ATP was not effective against thermal hyperalgesia. In contrast, anti-NGF significantly blocked OSCC-induced thermal hypersensitivity. Removal of IB4 (+) neurons by IB4-SAP showed no effect on OSCC-induced thermal hyperalgesia. IB4-SAP and SAP treated mice exhibited similar reduction after OSCC-supernatant injection. *P<0.05; **P<0.01; ***P<0.001, groups were compared with OSCC-supernatant injection alone. # P<0.05; IB4-SAP vs. SAP treatment group.

Figure 3.

Figure 3

Two weeks after intrathecal IB4-SAP injection, IB4 staining in the superficial dorsal horn of L4 and L5 spinal segments was reduced. A. Spinal cord section of SAP treated control mice. B. Spinal cord section of IB4-SAP treated mice. C. Immuno-intensity was reduced after IB4-SAP compared with SAP treated mice. *P<0.05; Scale bar=100μm.

Neutralization of NGF in the OSCC supernatant also effectively decreased cancer supernatant-induced mechanical hypersensitivity (Fig. 2A), indicating that IB4 (−)/TrkA (+) nociceptors are involved as well.

IB4 (+) neurons do not participate in cancer supernatant induced thermal hyperalgesia

Neither SNC-80 (DOR selective agonist) nor TNP-ATP (P2X3 selective antagonist) exhibited efficacy against thermal hypersensitivity induced by cancer supernatant (Fig. 2B). In addition, IB4-SAP treated mice still showed thermal hypersensitivity after OSCC supernatant injection and their paw withdrawal latency did not differ from mice injected with nonconjugated saporin controls (Fig. 2B). In contrast, anti-NGF significantly reduced OSCC supernatant-induced thermal hyperalgesia (Fig. 2B).

Increased neurturin but not GDNF in oral SCC supernatant

It is known that GDNF reduces mechanical sensitivity thresholds of IB4 (+) nociceptors 7, 38, we further investigated whether OSCC cells secrete higher than normal levels of GDNF. OSCC supernatant had similar GDNF concentration compared to normal oral keratinocyte supernatant (Fig. 4A). In contrast, neurturin levels were higher in OSCC cells compared with supernatant from normal oral keratinocytes (Fig. 4B, P < 0.05).

Figure 4.

Figure 4

Neurotrophin concentration in OSCC cells. A. OSCC supernatant had similar GDNF concentration compared with that of NOKs. OD=optical density. B. OSCC supernatant had higher neurturin concentration compared with that of NOKs. Values are expressed in OD values measured at 450 nm wavelength.

Discussion

In this study we provide evidence that IB4 (+) and IB4 (−) nociceptors are differentially involved in OSCC-induced pain. While both neuronal subpopulations are responsible for mechanical allodynia induced by OSCC supernatant in our mouse model, IB4 (−)/TrkA (+) neurons exclusively mediated thermal hyperalgesia.

We have shown from our previous studies that OSCC causes mechanical allodynia in both a mouse paw and a tongue model 29, 61. However the cellular source of nociceptive mediators is difficult to isolate due to the heterogeneous nature of the cancer microenvironment. Other than cancer cells, the cancer microenvironment includes many cellular types such as immune cells, fibroblasts, and endothelial cells. All these cells can secrete factors that directly excite or sensitize nociceptors. Here by injecting OSCC supernatant directly into the mouse paw, we clearly demonstrate that mediators secreted by cancer cells alone are sufficient to cause mechanical and thermal nociception in mice.

We then employed several pharmacological approaches to identify the subpopulation of putative nociceptors that are involved in OSCC-induced mechanical and thermal hypersensitivity. While it is still a question as to whether DORs are expressed exclusively on IB4 (+) neurons in mice 46, a selective DOR agonist effectively decreased OSCC-induced mechanical allodynia. In mice DRG neurons, the majority of IB4 (+) nociceptors express P2X3 receptors 8, 58. We therefore used the P2X3 receptor antagonist to target IB4 (+) nociceptors as our second pharmacologic approach. P2X3 receptor antagonist also attenuated OSCC-induced mechanical allodynia. Lastly, to confirm the involvement of IB4 (+) neurons in OSCC-induced mechanical allodynia, IB4 (+) neurons were eliminated using IB4-Saporin conjugates. We conclude that mechanical allodynia is decreased by IB4-SAP treatment. In contrast to the results found with mechanical allodynia, the DOR agonist, P2X3 antagonist, and IB4-SAP treatment showed no significant effect on OSCC-induced thermal hypersensitivity. Consistent with previous findings on IB4 (+) neurons 12, 46, our study suggests that IB4 (+) neurons do not play a significant role in OSCC-induced thermal nociception. Our finding that anti-NGF successfully abolishes OSCC-induced thermal hyperalgesia suggests that in the setting of oral cancer, thermal hyperalgesia is mediated by IB4 (−)/TrkA (+) neurons.

The involvement of IB4 (−)/TrkA (+) neurons in mechanical pain is not surprising. Cancers of different histological types, including OSCC, produce high levels of NGF, and NGF neutralizing antibodies decrease cancer-induced mechanical pain 23, 34, 47, 61. Peripherally administered NGF produces robust mechanical hypersensitivity in mice, rats, and humans 6, 19, 27, 33, 54, suggesting the role of IB4 (−)/TrkA (+) neurons in mechanical nociception.

While Scherrer and colleagues found complete segregation of IB4 (+)/DOR (+) and IB4 (−) /MOR (+) neurons in mechanical and thermal processing 46, a more recent study found overlap between MOR and DOR expression in mice DRGs 59. However, this finding of overlap could not fully explain our results, and functional differences between IB4 (−) and IB4 (+) subsets have been reported extensively 18, 21, 35, 41, 52, 53. In agreement with that of Scherrer et al., we found that DOR agonism inhibited mechanical allodynia but not thermal hyperalgesia. Furthermore, functional convergence of IB4 (+) and IB4 (−) neurons was only found in mechanical allodynia but not thermal hyperalgesia. Lastly, unlike in the rats where IB4 (+) and TrkA (+) neurons overlap substantially21, 53, it has been reported that there is little overlap between these two subpopulations in mice 22, 37, 43. It appears that IB4 (+) neurons might be lacking receptors necessary for thermal processing in mice. Indeed, IB4 (+) neurons express few TRPV1 channels10, 32, 60, 63, but the role of IB4 (+) neurons in thermal sensitivity remains unclear 10, 18, 53, 60.

Discrepancy in Scherrer and colleagues’ and current experimental results might reflect differences in the routes of drug delivery. While Scherrer and colleagues used spinal administration of opioid agonists 46, we administered all drugs into the paw. Therefore, the difference between our study and Scherrer et al.’s might result from functional differences between the central and peripheral terminals of nociceptors. Although peripheral administered drugs could have a central effect, in our case, opioid agonists would have a direct effect on peripheral terminals first.

Differences in the pain behavioral models could also contribute to the disparate findings. We injected cancer supernatant containing a complex mixture of algogenic chemicals; therefore, cross activation or sensitization by chemical mediators on the two subsets of neurons is likely to occur. In addition to endothelin, NGF, proteases, IL-6, and TNF-α, as we have previously reported 29, 44, 45, 61, OSCC releases neurturin which might activate IB4 (+) neurons. Since GDNF acts on IB4 (+) neurons to produce mechanical allodynia 25, we investigated whether cancer supernatant contains a high level of GDNF. Both normal oral keratinocytes and HSC-3 cell supernatant produced and secreted a low concentration of GDNF demonstrating that the activity of IB4 (+) neurons is not likely driven by GDNF in our model. Future studies should scan the full spectrum of mediators secreted by cancer cells and their actions on IB4 (+) and IB4 (−) neurons which might differentially modulate thermal and mechanical nociception. It has been reported that IB4 (+) neurons express receptors for a number of mediators including neurturin 32, ATP 8, 58, bradykinin 57 and VEGF 31. Therefore, IB4 (+) neurons are likely to be activated by a multiple mediators in the cancer microenvironment.

It should be noted that there are differences in the nociceptive circuitry and neurochemical expression patterns in trigeminal ganglia and DRG. In rats, there are substantial differences in SP, CGRP, and IB4 expression patterns between the DRG and trigeminal ganglia 43. In mice, only 10% of the peptidergic (i.e. contains SP or CGRP) and IB4 (+) neurons overlap in trigeminal ganglia43. While this percentage is comparable to what has been reported in mouse DRGs 22, 37 the lack of information regarding other nociceptive markers in trigeminal ganglia and DRGs prevented us from drawing further conclusions. We have used a paw model in this oral cancer pain study because there are well established mechanical and thermal nociceptive assays for this model. A more complete understanding of the putative nociceptors mediating oral cancer pain will require an anatomically correct oral cancer model and validated thermal and nociceptive assays.

Our finding that peripherally administered DOR agonists and P2X3 antagonists are effective in reducing OSCC-induced mechanical hypersensitivity has significant clinical implications. Function or movement provoked (mechanical) pain represents a major clinical problem in oral cancer patients who often experience difficulty with eating, drinking, swallowing, and speaking, and experience a much lower quality of life 16, 20. Oral cancer patients report pain as the worst symptom, and in their final months of life, 85% of these patients suffered from pain 48. While μ-opioids are initially effective in alleviating pain, tolerance develops quickly, doses escalate, and side effects abound.

DOR-selective agonists have been shown to produce potent analgesia when administered intrathecally 42, 46, 50, 56 and subcutaneously 26, 39, 40, with a reduction or absence in the development of physical dependence 17, reduced constipation 49, and reduced respiratory depression 13. Additionally, systemic application of a δ-opioid receptor agonist exhibited much higher potency than morphine in treating bone cancer induced mechanical pain and had fewer side effects 9. In this study, we demonstrated for the first time that DORs and P2X3 receptors play a role in oral cancer pain. Peripheral action of the DOR agonist and P2X3 antagonist might also increase efficacy and minimize unwanted effects. Accordingly, analgesics targeting IB4 (+) neurons present a promising avenue for future drug development to treat oral cancer pain.

Conclusion

IB4 (+) and IB4 (−) neurons are differentially involved in OSCC-induced pain. Mechanical hypersensitivity is mediated by both IB4 (+) and IB4 (−) neurons, while thermal hypersensitivity is mediated predominantly by IB4 (−) neurons. Pharmacological agents targeting IB4 (+) neurons exhibit great therapeutic potential in oral cancer pain treatment.

Acknowledgments

This work was funded by NIH/NIDCR R21DE01856

Footnotes

Disclosures

The authors declare no conflict of interest for these studies.

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