| Literature DB >> 16205698 |
L Lessard1, L R Bégin, M E Gleave, A-M Mes-Masson, F Saad.
Abstract
Several reports suggest that the canonical nuclear factor-kappaB (NF-kappaB) pathway is constitutively activated in a subset of prostate cancer cells. However, except for RelA (p65), little is known about the status of NF-kappaB transcription factors in prostate cancer tissues. To clarify the status of NF-kappaB subunits, we analysed the expression and subcellular localisation of RelA, RelB, c-Rel, p50, and p52 on tissue array sections containing respectively 344, 346, 369, 343, and 344 cores from 75 patients. The subcellular localisation of NF-kappaB factors was tested against relevant clinical parameters (preoperative prostate-specific antigen, pathological stage, and postoperative Gleason grade). With the exception of c-Rel, each subunit was detected in the nucleus of cancer cells: significant nuclear expression of RelB, RelA, p52, and p50 was seen in 26.6, 15.6, 10.7, and 10.5% of cores, respectively. Surprisingly, cores expressing both nuclear RelA and p50 canonical pathway proteins were less frequently observed than cores expressing other subunit combinations such as RelB-p52 and RelA-RelB. In addition, the nuclear localisation of RelB correlated with patient's Gleason scores (Spearman correlation: 0.167; P=0.018). The nuclear localisation of both canonical and noncanonical NF-kappaB subunits in prostate cancer cells suggests for the first time that different NF-kappaB pathways and dimers may be activated in the progression of the disease.Entities:
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Year: 2005 PMID: 16205698 PMCID: PMC2361687 DOI: 10.1038/sj.bjc.6602796
Source DB: PubMed Journal: Br J Cancer ISSN: 0007-0920 Impact factor: 7.640
Figure 1Immunohistochemical detection of c-Rel (A–C), RelA (D–F), p50 (G–I), RelB (J–L), and p52 (M–O) in normal, PIN, and cancerous prostate tissues (× 400). Note nuclear RelB staining in a subset of normal glands (J). Also note a mixture of weak and strong p52 cytoplasmic staining in normal glands (M). Enlargements are provided to more clearly distinguish the subcellular localisation in cancer specimens.
Nuclear localisation of NF-κB transcription factors in prostatic tissue cores
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| Normal | 39 | 0 (0) | 37 | 0 (0) | 40 | 2 (5.0) | 39 | 1 (2.6) | ||||
| PIN | 23 | 1 (4.3) | 21 | 0 (0) | 24 | 0 (0) | 24 | 0 (0) | ||||
| Cancer | 282 | 44 (15.6) | 0.001 | 285 | 30 (10.5) | 0.004 | 282 | 75 (26.6) | <0.001 | 281 | 30 (10.7) | 0.025 |
χ2 was used to test the association of nuclear NF-κB expression with tissue type (cancer vs noncancer).
P-value less than 0.05 was considered as significant.
NF-κB=nuclear factor-κB; PIN=prostatic intraepithelial neoplasia.
Nuclear localisation of NF-κB transcription factors in low to intermediate (2, 2/3, 3) and high (3/4, 4, 4/5, 5) Gleason grade scores
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| Low | 170 | 24 (14.1) | 174 | 16 (9.2) | 169 | 40 (23.7) | 167 | 16 (9.6) | ||||
| High | 112 | 20 (17.9) | 0.405 | 111 | 14 (12.6) | 0.431 | 113 | 35 (31.0) | 0.104 | 114 | 14 (12.3) | 0.555 |
χ2 was used to test the association between nuclear NF-κB and tissue grade. P-value less than 0.05 was considered as significant. NF-κB=nuclear factor-κB.
Figure 2Frequencies of NF-κB subunit combinations in the prostate cancer cores. The vertical pattern is for the canonical RelA–p50 pair. Noncanonical combinations are represented as follows: the diagonal pattern is for other class 1/class 2 dimers, and the dashed pattern is for class 1/class 1 or class 2/class 2 dimers. **P<0.01 χ2 between RelA–p50 and RelA–RelB.
Correlation between NF-κB nuclear localisation and patient's Gleason scores
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| RelA | 0.078 | 0.272 |
| p50 | −0.018 | 0.803 |
| RelB | 0.167 | 0.018 |
| p52 | −0.019 | 0.793 |
Spearman's σ coefficient was used to test the relationship between nuclear NF-κB expression and Gleason scores.
P-value less than 0.05 was considered as significant. NF-κB=nuclear factor-κB.