Abstract
KDR (kinase insert domain receptor) phosphorylation induces several effects which lead eventually to cell proliferation and survival. The precise mechanisms by which KDR, once it is activated, communicates with the nucleus are starting to be understood but have not yet been completely unravelled. Two in vitro studies on animal cell lines reported in the literature have demonstrated that, following stimulation with VEGF, KDR is actually translocated within the nucleus. Our aim was to investigate whether this translocation occurs in human cells both in vitro and in vivo. Using laser scanning confocal microscopy, a variable nuclear localization of phosphorylated and total KDR in cell lines and tumour samples was found. In human neoplastic cell lines, hypoxic stimulation greatly increased the nuclear amount of total KDR but less so that of the phosphorylated form. Only after hypoxia and VEGF stimulation there was a comparably increased expression of phosphorylated and total KDR observed in the nuclei of these cells. We conclude that neoplastic cells show a variable expression of total and phosphorylated KDR in the nucleus. The precise functional meaning of nuclear location remains to be established.
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Introduction
Angiogenesis, the process of blood vessel formation from pre-existing vessels and vascular endothelial cells, is essential for normal growth and tissue repair, but is also critical in a wide variety of pathological conditions, such as diabetic retinopathy, arthritis, tumour growth and metastasis 1, 2, 3.
Vascular endothelial growth factor (VEGF) is essential for the development of the vascular system and acts as an endothelial cell-specific mitogen as well as a mediator of vascular growth 4, 5. Two high affinity receptors for VEGF, namely Flt-1 (VEFGR-1) and KDR (Flk-1/VEGFR-2), have been identified 6, 7, 8, 9. These receptors belong to the tyrosine kinase receptor family. This family of receptors is characterised by the presence of seven immunoglobulin-like domains (Ig domains) in their extracellular ligand-binding part. Their intracellular domain in contrast comprises a single transmembrane domain and an intracellular tyrosine kinase domain split by a kinase insert that is important for substrate recognition 9. All VEGFRs are expressed at an early stage during development and they display overlapping expression profiles, mostly confined to endothelial cells 6, 9.
KDR (VEGFR2) is a 230 kDa protein which exerts its effect through activation of its intracellular tyrosine kinase domain. KDR can be phosphorylated on several tyrosine residues (Y801, Y951, Y996, Y1054, Y1059, Y1175 and Y1214) 10, 11. Phosphorylation of the activation-loop tyrosine residues is required for activation of the catalytic activity of the KDR kinase 10. KDR is expressed on endothelial cells. On the basis of ligand specificity, most functional VEGF cell signalling on endothelial cells described to date is mediated via KDR. This means that the major biological functions of VEGF, such as endothelial cell survival, proliferation and migration, increase of endothelial Nitrous Oxide (NO) and prostacycline production, increase of vascular permeability and promotion of mitogenic effects, are related to KDR mediated signalling 12, 13.
KDR is also expressed in haematopoietic stem cells, megakaryocytes, platelets and retinal cell progenitors 14, 15, 16. KDR knock-out mice display embryonic lethality through their failure to produce endothelial and haematopoietic cells. Furthermore, KDR has been shown to be present in a number of neoplastic cell lines including melanoma, ovarian carcinoma, prostatic carcinoma 16 and in tumours, healing wounds and inflammatory sites 17.
Hypoxia is a major regulator of VEGF production under both physiological and pathological conditions. Regulation of VEGFR expression appears to be less straightforward. Experiments in mice have shown that both VEGFR-1 and KDR are induced under hypoxic conditions 18, 19. In endothelial cells lining the blood vessels of tumours VEGFR expression is also induced by hypoxia which causes the local concentration of VEGF to be increased 20.
It has been reported that there is a redistribution and internalisation inside the cytoplasm of KDR after phosphorylation 21. Two other studies in vitro on bovine 20 and rat endothelium 22 have demonstrated that following stimulation with VEGF, KDR is actually translocated within the nucleus. However it is not known whether this translocation occurs in vivo and no studies have been carried out on human cells
An immunohistochemical study from our laboratory with anti-phosphorylated KDR antibodies showed that KDR can be expressed on normal cells other than endothelium and on neoplastic cells. It also showed the presence of what looked like nuclear KDR after staining with both anti phosphorylated and wild type antibodies 23. These novel and somewhat surprising findings are potentially very important for understanding the function of KDR.
The aim of this study was to indicate whether total and/or phosphorylated forms of KDR could be demonstrated inside the nuclei of human cells using laser scanning confocal microscopy.
Material and methods
Cell culture
The following cell lines were obtained from ATCC (American Type Culture Collection): MCF-7 (breast carcinoma), HeLa (carcinoma of the cervix) and HL60 (Acute Myeloid Leukaemia, Promyelocytic). MCF-7 cells were cultured at 37°C and 5% CO2 in E4 medium (GIBCO) containing 10% fetal calf serum (FCS) in 75 cm2 flasks growing until 80-90% of confluence. HeLa and HL60 cells were cultured at 37°C with 5% CO2 in RPMI 1640 medium (GIBCO) containing 10% fetal calf serum (FCS) in 75 cm2 flasks growing to 80-90% confluence.
Cell stimulation
The HeLa cells were investigated not only in basal conditions but also after stimulation with hypoxia alone or hypoxia and VEGF 165.
Hypoxic stimulation: HeLa cells at approximately 70-80% confluence were transferred to a serum-free medium for 24 h and incubated for 16 h at 37°C with 0.1% O2, fixed in PBS containing 10% of formalin, paraffin embedded and 5 mm sections were obtained.
Hypoxic and VEGF stimulation: HeLa cells at approximately 70-80% confluence were transferred to a serum-free medium for 24 h and incubated for 16 h at 37°C with 0.1% O2 before being stimulated with 50 ng/ml VEGF 165 (Astro Zeneca, R&D Systems) for 8 min. Cells were subsequently fixed in PBS with 10% formalin, paraffin embedded and 5 mm sections were obtained.
Tumour samples
Tumour tissues were obtained from the Department of Cellular Pathology, John Radcliffe Hospital, Oxford. The samples were formalin fixed, paraffin embedded and 5 mm sections were produced. Ethical approval for the use of the tissue was obtained.
Tumours studied included 5 of renal clear cell carcinomas, 4 of leukaemias (2 of acute myeloid and 2 of acute lymphoid), 6 of lymphomas (2 of mantle cell, 2 of peripheral T cell and 2 of small lymphocytic) and 4 of non- small cell lung cancers.
Double immunofluorescence staining and laser scanning confocal microscopy
To detect phosphorylated KDR we employed the monoclonal antibodies 34a and 126a produced in our laboratory and described elsewhere 23. 34a recognises peptide 31 of KDR that contains the tyrosine residue Y1214, a potential Grb2 SH2 binding site that is related to an autophosphorylation site. 126a recognises peptide 25 of KDR containing the tyrosine residues Y1054/1059 located in the KDR activation loop.
We also used a polyclonal commercial antibody against phosphorylated KDR, Tyr996 (Cell Signaling Technology USA) that recognizes the peptide containing tyrosine 996 located in the tyrosine kinase insert loop.
Finally, we studied the localisation and expression of total KDR in cells using the commercial monoclonal antibody Flk-1 (A3) (Santa Cruz, USA) that recognizes the amino acid sequence corresponding to 1158-1345 of the protein independently from its phosphorylation status.
Cell membrane was stained using the anti Epithelial Membrane Antigen (EMA) mouse monoclonal antibody E29 (DACOCYTOMATION).
Sections were deparaffinised and rehydrated. Antigen retrieval was carried out by immersing the slides in 10 mM citrate at pH 6.0 and boiling them for 3 min. Slides were incubated for 1.5 h with the primary antibodies at the following dilutions: 34a (1:20), 126a (1:50) Tyr996 (1:50) and Flk-1 (A3) (1:50). After washing with TBS, the slides were incubated for 1 h with a mixture of the secondary Alexa Fluor 488 goat anti-mouse IgM (m chain) and Alexa Fluor 546 goat anti-mouse IgG1 (g1) (1:400 for tumour samples, 1:100 for cell samples) (Molecular Probes Europe BV) in the case of monoclonal antibodies. A mixture of the secondary Alexa Fluor 488 goat anti-mouse IgG1 (g1) and Alexa 546 goat anti-rabbit IgG (H+L) (1:400 for tumour samples, 1:100 for cell samples) (Molecular Probes Europe BV) was used to detect the primary polyclonal commercial antibody.
All of the incubations were carried out at room temperature and in darkness. After washing with TBS, the sections were fixed with paraformaldehyde 1% for 10 min, and mounted with DAKO's fluorescence mounting medium containing TOTO-3 iodide (1:500) (Molecular Probes Europe BV) to stain nuclei. Confocal fluorescent images were acquired using a ZEISS LSM510 microscope. Colour channels in the images were assigned as follows: Red-546nm excitation; Green-488nm excitation; Blue-633nm excitation.
Results
pKDR expression in neoplastic cell lines
Using confocal microscopy double immunofluorescence staining of MCF-7, HeLa and HL60 cells with 34a and 126a showed an internal distribution of the phosphorylated form of KDR with a predominant perinuclear localisation and a variable nuclear expression. With the commercial polyclonal anti-phosphorylated VEGF Receptor-2 (Tyr996), the fluorescence staining was stronger and more staining was located inside the nucleus.
Total KDR detected with the Flk-1 (A3) antibody showed a wide distribution inside the cell, as cytoplasmic, perinuclear and nuclear fluorescence staining was observed. Figure 1 illustrates the staining achieved on MCF-7 cells stained with Flk-1(A3), the anti total KDR antibody and the anti-phosphorylated KDR antibody 34a.
pKDR expression in HeLa cells after VEGF and/or hypoxia treatment
Hypoxic stimulation, with or without VEGF greatly increased the nuclear localization of total KDR but less so that of the phosphorylated form (Figure 2). The staining pattern of phosphorylated KDR was again mostly perinuclear with antibody 126a (Figure 2B) and 34a.
pKDR expression in human tumours
In the tumours a heterogeneous pattern of expression of KDR was observed using the monoclonal antibodies 34a and 126a. Overall the pattern of staining observed on the neoplastic cells from tissue sections was comparable to that seen on neoplastic cell lines (Figure 3).
Kidney tumours: Immunostaining with monoclonal antibodies 34a and 126a showed that pKDR was present on the membrane and within the cytoplasm and perinuclear regions. Some spots were also found inside the nucleus of malignant cells in some of the cases studied. Total KDR [antibody Flk-1 (A3)] showed a similar pattern but with more staining localized to the nucleus of tumour cells.
Leukaemias: In the 2 AML cases, 34a staining showed both cytoplasmic and strong nuclear expression of pKDR in the neoplastic cells. Similarly, though more granular and less intense staining was found with antibody 126a. In contrast, in the 2 cases of ALL pKDR expression was mostly cytoplasmic with only weak labelling in the nucleus. In all cases, total KDR [antibody Flk-1 (A3)] was mostly observed in the cytoplasm with only a slight expression in the nucleus.
Lymphomas: 2 cases of peripheral T cell lymphoma showed cytoplasmic and strong perinuclear and nuclear staining for pKDR with both 34a and 126a. In contrast, in mantle cell lymphomas (MCL) and chronic lymphocytic leukaemia (B-CLL) the expression was only cytoplasmic and perinuclear. Total KDR [antibody Flk-1 (A3)] was present in the cytoplasm and the nucleus of all the lymphoma cases.
Lung, non-small cell carcinomas: 34a and 126a showed a strong granular fluorescence staining for pKDR in the membrane and cytoplasm of all 4 cases of lung cancer studied. Clear nuclear expression, although much weaker, was also recorded not only in the tumour cells but also in adjoining stromal cells. The Flk-1 (A3) antibody showed a widely distributed fluorescence staining throughout the tumour cells with total KDR being present in the membrane, cytoplasm and nucleus.
Discussion
KDR undergoes phosphorylation and induces several effects eventually leading to cell proliferation and survival. How KDR, once activated by VEGF, communicates with the nucleus is not yet completely understood. An earlier group of studies has shown that KDR phosphorylation leads to re-localisation in the cytoplasm but offers no proof of any nuclear localisation 21, 25, 26. One in vitro study has shown that, following VEGF stimulation, KDR can be internalised within the cytoplasm 21. Then, as shown in HUVEC cells after stimulation, KDR (but not Flt1) activation via multiple pathways such as MAPK/MSK-1 or C/p90RSK, can trigger CRE binding protein phosphorylation inside the nucleus 25.
Another pathway has been described in which non phosphorylated KDR (but not Flt-1) induces the translocation into the nucleus of STAT1 and STAT6. Indeed STAT1 is also known to co-precipitate with KDR. These data suggest, but do not prove, that KDR may be translocated inside the nucleus as well 26.
A number of other studies provide indirect evidence for a nuclear localization of pKDR. Li et al showed that in bovine endothelial cells VEGF can be transiently translocated into the nuclei 19 and KDR, but not Flt1, was necessary for this to happen though there was no direct evidence of KDR itself within the nucleus.
Finally, two studies have demonstrated that KDR is translocated inside the nucleus 20, 21, 22 in association with endothelial Nitric Oxide Synthase (eNOS) by a process that may be mediated by a caveolar transport system 20. None of this in vitro data can be automatically considered to be representative of what happens in vivo 28.
Our results conclusively demonstrate that in human cells, both in vitro and in vivo, phosphorylated KDR can be present inside the nuclei of normal and neoplastic cells. These results were obtained with each of the antibodies 34a and 126a - generated in our laboratory – and were confirmed on cell lines with an even clearer and stronger nuclear expression of phosphorylated KDR when the completely independent commercial antibody Tyr996 was used. This difference of intensity may be due to the fact that the antibodies recognise different tyrosine residues of the protein and also that the signal may be magnified by the polyclonal nature of the commercial antibody. Nevertheless the consistency of the nuclear staining is strong evidence in favour of its existence.
A number of representative tumours were selected in order to analyse the staining patterns of KDR expression. As might be expected, we obtained a variety of staining patterns finding membranous, cytoplasmic and nuclear expression of phosphorylated KDR that varied with the origin of the tumour cells. It is interesting to note that HL60 is a myeloid leukaemia cell line and, as in the case of myeloid leukaemia tissue, it showed strong and clear nuclear expression of activated KDR. This nuclear distribution might be related to the transcriptional activation of genes involved in the angiogenic cascade, but, at the moment, the precise function of this process is completely unknown. We also do not know the functional meaning of having phosphorylated KDR in the nucleus rather than in the cytoplasm.
However it is clear that nuclear translocation of the intracellular portion of membrane bound tyrosine kinase receptors upon activation has been described recently for other receptor molecules such as Erb B4, epidermal growth factor (EGF) receptor and FGFR-1 29. This suggests that this is an important mechanism involving their direct transcriptional regulatory activity in addition to roles in signal transduction. The mechanism whereby the membrane bound receptor tyrosine kinase, Erb B4, a member of the EGF receptor family, moves to the nucleus has been explored. This receptor undergoes proteolysis within the plasma membrane domain by regulated intramembranous proteolysis (RIP) and its intracellular portion moves to the nucleus where it may affect transcription of target genes 29, 30. However, prior to this, the ectodomain of the receptor is usually cleaved by a membrane associated metalloprotease. The intramembrane proteolysis described above is mediated by enzymes of the gamma secretase family which belongs to the group of presenilins or in some instances caspases 31.
Another possible mechanism of nuclear translocation is that the receptor undergoes secondary modifications, such as reduction in size possibly via intramembranous or cytoplasmic cleavage. These smaller receptor fragments may then relocate either alone or in concert with other molecules such as STAT-1. The role of such relocation can only be speculated upon. It may well be that these fragments have a direct transcriptional effect in tumour cells. This is an exciting possibility because if proven it should be possible to combine an anti-KDR small molecule inhibitor with conventional tumour treatment.
In conclusion, neoplastic cells showed a variable expression pattern of phosphorylated KDR between nucleus and cytoplasm. The functional meaning of these different intracellular locations remains to be established.
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Acknowledgements
This work was funded by Cancer Research UK. Cristina Blazquez was supported by a grant from the Federation of European Biochemical Societies (FEBS).
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Blazquez, C., Cook, N., Micklem, K. et al. Phosphorylated KDR can be located in the nucleus of neoplastic cells. Cell Res 16, 93–98 (2006). https://doi.org/10.1038/sj.cr.7310012
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DOI: https://doi.org/10.1038/sj.cr.7310012
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