Cannabinoid CB1 Receptor Is Downregulated in Clear Cell Renal Cell Carcinoma
Abstract
Several studies in cell cultures and in animal models have demonstrated that cannabinoids have important antitumoral properties. Because many of these effects are mediated through cannabinoid (CB) receptors CB1 and CB2, the study of their expression in human neoplasms has become of great interest in recent years. Fresh and formalin-fixed tissue samples of 20 consecutive clear cell renal cell carcinomas (CCRCCs) were collected prospectively and analyzed for the expression of both CB receptors by using RT-PCR, Western blot (WB), and immunohistochemical techniques. RT-PCR assays demonstrated the expression of mRNA encoding the CB1 in tumor tissue and in adjacent non-neoplastic kidney. Conversely, WB and IHC revealed a marked downregulation of CB1 protein in tumor tissue; CB2 was not expressed. The obtained data suggest a possible implication of the endocannabinoid system in renal carcinogenesis. A posttranscriptional downregulation of CB1 and the absence of expression of CB2 characterize CCRCC. (J Histochem Cytochem 58:1129–1134, 2010)
The endocannabinoid system (ECS) consists of cannabinoid (CB) receptors, endocannabinoids, and the enzymes responsible for synthesis and degradation of their endogenous ligands (Mackie 2008). This system is widely distributed in mammalian tissues and regulates nervous, cardiovascular, digestive, reproductive, immune, and metabolic functions by activating CB1 and CB2 receptors (Graham et al. 2009).
There is increasing evidence that endocannabinoids modulate the activity of enzymes and nuclear factors involved in the control of fundamental processes of cell homeostasis and in neoplastic transformation (Flygare and Sander 2008; Pisanti and Bifulco 2009). Actually, numerous pharmacological studies carried out in vitro and in animal models have proposed antitumoral properties to natural and synthetic CBs (Pisanti and Bifulco 2009).
Recent works have reported changes in the expression of the CBs in neoplasms of diverse topographies, such as large bowel (Wang et al. 2008), breast (Caffarel et al. 2006), prostate (Sarfaraz et al. 2005), pancreas (Carracedo et al. 2006; Michalski et al. 2008), and liver (Xu et al. 2006). However, studies in vivo are still scarce in human tissues. In addition, ECS dysregulation needs to be evaluated in other human cancer types (Alpini and DeMorrow 2009).
Very few studies have focused on the ECS in the kidney and its neoplasms. We have found very recently the presence of CB1 and the absence of CB2 receptors in human fetal and adult kidneys (Larrinaga et al. 2010). Other authors (Hart et al. 2004) have studied the effect of CBs on renal cancer cell cultures several years ago.
CB receptors have not been tested to date in renal tumors. They are included in the top ten list of the commonest tumors in males and females and account for ~4% of adult malignancies (Jemal et al. 2009). Roughly 70% of them are clear cell renal cell carcinomas (CCRCCs) (Lopez Beltran et al. 2009). The 2004 WHO classification of renal tumors in adults links for the first time histology and genetics and attributes the origin of most histological subtypes of renal cancer to distinct parts of the nephron (Lopez Beltran et al. 2006). So, the proximal convoluted tubule cell is considered to be the origin of CCRCC (Lopez Beltran et al. 2006).
Despite the latest advances in genetics, the biology of renal tumors is still far from being completely understood. This study, which includes the analysis of mRNA and protein [Western blot (WB) and IHC] expression of CB in CCRCCs, is an attempt to shed some light on the underlying mechanisms involved in renal neoplasia.
Materials and Methods
All the experiments carried out in this study comply with current Spanish and European Union laws and conform to the principles outlined in the Declaration of Helsinki.
mRNA Expression
An end point PCR assay was used to detect the mRNAs of the CB1 (CNR1) and CB2(CNR2) receptors and to establish the identity of the amplified products. Fresh renal tissue was obtained from surgical specimens of 20 CCRCCs (16 males, 4 females; mean age: 62 years). Patient consent and Hospital Ethics Committee approval were obtained a priori. Tissue samples were immersed in RNAlater (Ambion; Huntingdon, UK) immediately after dissection and stored at −80C until use.
RT-PCR reactions were performed as previously described (Candenas et al. 2001; Varona et al. 2007; Blanco et al. 2008; Larrinaga et al. 2010). Total RNA of ~30 mg of human renal tissue was isolated in every case according to the method described by Chomczynski and Sacchi (1987). First-strand cDNA was synthesized from 25 μg of total RNA of each human sample using Moloney murine leukemia virus RT and random hexamers according to the manufacturer’s instructions (First-strand cDNA Synthesis Kit; Amersham Biosciences, Essex, UK). The resulting cDNA samples were amplified using PCR with specific oligonucleotide primer pairs designed with the analysis software Primer3 (Rozen and Skaletsky 2000). The sequences of the primer pairs used for human CNR1 and CNR2are expressed in Table 1. On the basis of previous experiments on human renal cell carcinoma (Jung et al. 2007; Varona et al. 2007; Blanco et al. 2008), the human gene succinate dehydrogenase complex, subunit A (SDHA) was chosen as endogenous reference gene and used to assure that similar amounts of cDNA were used in all RT-PCR reactions. Sequences for SDHA are also displayed in Table 1. All primers were synthesized and purified by Sigma-Genosys (Cambridge, UK). A pool of cDNAs from 20 different human tissues (Human Total RNA Master Panel; Clontech, Mountain View, CA) was used as a positive control of amplification.
PCR mixes contained 0.2 μmol primers, 1.5 U of heat-activated thermostable DNA polymerase (Immolase; Bioline, London, UK), the buffer supplied, 2.5 mmol MgCl2, 200 μmol dNTPs, and 25 μl cDNA. PCR was performed for 35 cycles with cycling parameters of 15 sec at 94C, 20 sec at 60C, and 20 sec at 72C. The PCR products were separated by agarose gel electrophoresis, and the amplicon sizes were verified by comparison with a DNA mass ladder. mRNA levels for the CB receptors and SDHA were analyzed on each tissue, with each RT-PCR assay being performed in triplicate. The identity of each product was established by DNA sequence analysis.
WB Assays
We performed a WB analysis of eight CCRCCs. Membrane proteins (10 μg) were solubilized in sample buffer and were resolved by electrophoresis in 12% SDS-PAGE gel. Then, proteins were transferred to polyvinylidene difluoride membranes. Blots were blocked in milk and incubated overnight with the CB1 (1:250 dilution; catalog ref. PA1-743, ABR Affinity BioReagents, Golden, CO) and CB2 (1:200 dilution; catalog ref. 101550, Cayman Chemical, Ann Arbor, MI) polyclonal antibodies. Later, the blots were washed and incubated for 2 hr at room temperature with a horseradish peroxidase–conjugated goat anti-rabbit IgG secondary antibody (1:2500 dilution; ABR Affinity BioReagents). Membranes incubated without the primary antiserum were used as negative controls. Immunoreactive bands were visualized using the enhanced chemiluminescence system.
Immunohistochemistry
Archival material obtained from the files of the Department of Anatomic Pathology, University Hospital of Cruces, University of the Basque Country, Barakaldo, Spain, was used for this study. Representative formalin-fixed and paraffin-embedded material obtained from 20 consecutive CCRCCs including cases with conventional histology and Furhman’s grades 1–3 (Fuhrman et al. 1982) was analyzed.
Consecutive slides of the selected blocks in every case were immunostained with CB receptors CB1 and CB2 following routine methods in an automatized immunostainer (Dako Autostainer Plus; Dako, Glostrup, Denmark). CB1 (working dilution 1:1000; ABR Affinity BioReagents) and CB2 (working dilution 1:200; Cayman Chemical) polyclonal antibodies were used. The specificity of these antibodies in human cells was previously assessed by our group (Agirregoitia et al. 2010; Larrinaga et al. 2010). Negative control slides were not exposed to the primary antibody and were incubated in PBS and then processed in the same conditions as the test slides. Immunohistochemical slides were studied using a Nikon Eclipse 80i microscope (Tokyo, Japan).
Results
mRNA Expression of CB Receptors
RT-PCR revealed the presence of a single transcript, corresponding to the expected product size encoding the cannabinoid CB1 receptor (131 bp). The identity of the amplified fragment was confirmed by DNA sequence analysis. The CNR1 transcript could be observed in both tumor and surrounding normal tissues assayed after amplification of cDNA for 35 cycles. Conversely, the mRNA encoding the 110-bp product expected for the cannabinoid CB2 receptor was undetectable in cDNA from tumor or normal renal tissues. The mRNAs of CNR1, CNR2, and SDHA genes were all detected in the cDNA pool used as positive control (Figure 1).
No PCR product was detectable when the samples were amplified without the RT step, suggesting that genomic DNA contamination was eliminated by DNase treatment. Similarly, no products were detected when the RT-PCR steps were carried out with no added RNA, indicating that all reagents were free of target sequence contamination. Figure 1 shows the negative control with no RNA in the RT reaction.
Protein Expression of CB Receptors
WB assays showed that CB1 receptor expression was practically nonexistent in CCRCC (Figure 2). Two immunoreactive bands were observed in each lane corresponding to normal tissue, one at around 60 kDa, corresponding in size to the putative CB1 monomer, and a lower molecular mass form at around 37 kDa (Figure 2A). The lower band could correspond to a deglycosylation and/or proteolysis product of the 60-kDa-band receptor (De Jesús et al. 2006). The lane on the right shows the presence of similar bands in samples of cerebral cortex, which is used as a positive control for the CB1 receptor (Figure 2A). The CB2 protein was undetectable both in normal and tumor tissues. Positive staining was, however, observed in Jurkat cells, used as a positive control for the CB2receptor, with the appearance of the expected band at 44 kDa (Figure 2B).
IHC studies corroborated these data. CB1 immunostaining was negative in CCRCC and positive in adjacent normal proximal convoluted tubules (Figure 3), whereas CB2 was absent both in CCRCC and in normal tissue.
Discussion
In the last decade, several studies in cell cultures and in animal models have demonstrated that CBs have proapoptotic, antiproliferative, antimetastatic, and antiangiogenic effects in various cancer types (Alexander et al. 2009). Although no clinical basis exists to recommend the use of natural/synthetic CBs in patients with renal cancer, this knowledge has spurred a clinical trial examining the efficacy and safety of giving Δ9-tetrahydrocannabinol locally to patients with other neoplasias, such as recurrent glioblastoma multiforme (Guzmán et al. 2006).
Because many of these antitumoral effects of cannabinoids are mediated through CB receptors, the analysis of the expression of CB1 and CB2 receptors in a wide variety of human neoplasms has become of great interest, with some promising results appearing in the recent literature (Flygare and Sander 2008; Alpini and DeMorrow 2009). Although CCRCC is a paradigm of multi–antitumoral-drug-resistant neoplasia, a study on the role of ECS on this tumor is lacking.
As we previously observed in human normal kidneys (Larrinaga et al. 2010), tumor tissues expressed mRNA of the CB1, whereas the mRNA of CB2 was absent. Conversely, there was no correlation between CB1 mRNA and its protein expression because both WB and IHC failed to demonstrate any trait of CB1 protein in tumor tissue. This finding was constant in all the CCRCCs studied, irrespective of the tumor stage and grade. This result suggests that the protein modification of CB1 could occur in these tumors at a posttranscriptional level, thus illustrating the importance of not relying only on mRNA level for the evaluation of any protein change. This assertion has also been indicated by several authors in other kidney diseases (Kasinath et al. 2006).
The CB1 is highly expressed in proximal convoluted tubules of the nephron in both normal adult kidney and mature tubules of fetal kidney (Larrinaga et al. 2010). However, this receptor is not immunohistochemically expressed in the nephrogenic zone of the fetal kidney, where tubular cells are still poorly differentiated (Larrinaga et al. 2010). Interestingly, a parallelism between poorly differentiated tubule cells of fetal kidney and CCRCCs can be raised because CB1 appears downregulated in a renal tumor that supposedly originates in the proximal nephron (Lam et al. 2005; Lopez Beltran et al. 2006). For this reason, we consider that this CB1-related tumor dedifferentiation observed in CCRCCs approaches the tumor to its cell of origin and confirms the current belief on the distinct tumor origin of renal neoplasms expressed in the current WHO classification. Additionally, this immunoprofile may eventually be used as an additional tool with practical interest in the routine diagnosis of CCRCCs.
The precise role of the CB1 in renal cancer still remains to be clarified. It should be noted that a similar CB receptor expression profile has been reported recently in human colorectal cancer by Wang et al. (2008). The authors have suggested that CB1 loss would make cancer cells resistant to the antitumoral effect of endocannabinoids, thus accelerating intestinal tumor growth and biological aggressiveness (Wang et al. 2008). This evidence favors the hypothesis that CB1 downregulation is a general mechanism in some different cancer types. In this sense, Caffarel et al. (2006) also observed downregulation of CB1 in human breast cancer cells. However, CB1 upregulation has also been reported in other human neoplasms, such as prostatic adenocarcinoma (Sarfaraz et al. 2005), hepatocellular carcinoma (Xu et al. 2006), and pancreatic ductal adenocarcinoma (Carracedo et al. 2006; Michalski et al. 2008). Therefore, further studies are needed to clarify the precise mechanisms underlying these apparently divergent results.
Acknowledgments
This work was supported by grants from the Jesús Gangoiti-Barrera Foundation, Gobierno Vasco (GIC07/84), Ministerio de Educación y Ciencia (CTQ2007-61024/BQU), and SAIOTEK (SA-2008/00046).
The authors thank Ana Abascal, Alicia Esteve, and Mar Gonzalez, lab technicians at the Department of Anatomic Pathology, University Hospital of Cruces, University of the Basque Country, Barakaldo, Spain, for their excellent immunohistochemical work.
Notes
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