NF-κB Hyper-Activation by HTLV-1 Tax Induces Cellular Senescence, but Can Be Alleviated by the Viral Anti-Sense Protein HBZ
Activation of I-κB kinases (IKKs) and NF-κB by the human T lymphotropic virus type 1 (HTLV-1) trans-activator/oncoprotein, Tax, is thought to promote cell proliferation and transformation. Paradoxically, expression of Tax in most cells leads to drastic up-regulation of cyclin-dependent kinase inhibitors, p21CIP1/WAF1 and p27KIP1, which cause p53-/pRb-independent cellular senescence. Here we demonstrate that p21CIP1/WAF1-/p27KIP1-mediated senescence constitutes a checkpoint against IKK/NF-κB hyper-activation. Senescence induced by Tax in HeLa cells is attenuated by mutations in Tax that reduce IKK/NF-κB activation and prevented by blocking NF-κB using a degradation-resistant mutant of I-κBα despite constitutive IKK activation. Small hairpin RNA-mediated knockdown indicates that RelA induces this senescence program by acting upstream of the anaphase promoting complex and RelB to stabilize p27KIP1 protein and p21CIP1/WAF1 mRNA respectively. Finally, we show that down-regulation of NF-κB by the HTLV-1 anti-sense protein, HBZ, delay or prevent the onset of Tax-induced senescence. We propose that the balance between Tax and HBZ expression determines the outcome of HTLV-1 infection. Robust HTLV-1 replication and elevated Tax expression drive IKK/NF-κB hyper-activation and trigger senescence. HBZ, however, modulates Tax-mediated viral replication and NF-κB activation, thus allowing HTLV-1-infected cells to proliferate, persist, and evolve. Finally, inactivation of the senescence checkpoint can facilitate persistent NF-κB activation and leukemogenesis.
Published in the journal:
. PLoS Pathog 7(4): e32767. doi:10.1371/journal.ppat.1002025
Category:
Research Article
doi:
https://doi.org/10.1371/journal.ppat.1002025
Summary
Activation of I-κB kinases (IKKs) and NF-κB by the human T lymphotropic virus type 1 (HTLV-1) trans-activator/oncoprotein, Tax, is thought to promote cell proliferation and transformation. Paradoxically, expression of Tax in most cells leads to drastic up-regulation of cyclin-dependent kinase inhibitors, p21CIP1/WAF1 and p27KIP1, which cause p53-/pRb-independent cellular senescence. Here we demonstrate that p21CIP1/WAF1-/p27KIP1-mediated senescence constitutes a checkpoint against IKK/NF-κB hyper-activation. Senescence induced by Tax in HeLa cells is attenuated by mutations in Tax that reduce IKK/NF-κB activation and prevented by blocking NF-κB using a degradation-resistant mutant of I-κBα despite constitutive IKK activation. Small hairpin RNA-mediated knockdown indicates that RelA induces this senescence program by acting upstream of the anaphase promoting complex and RelB to stabilize p27KIP1 protein and p21CIP1/WAF1 mRNA respectively. Finally, we show that down-regulation of NF-κB by the HTLV-1 anti-sense protein, HBZ, delay or prevent the onset of Tax-induced senescence. We propose that the balance between Tax and HBZ expression determines the outcome of HTLV-1 infection. Robust HTLV-1 replication and elevated Tax expression drive IKK/NF-κB hyper-activation and trigger senescence. HBZ, however, modulates Tax-mediated viral replication and NF-κB activation, thus allowing HTLV-1-infected cells to proliferate, persist, and evolve. Finally, inactivation of the senescence checkpoint can facilitate persistent NF-κB activation and leukemogenesis.
Introduction
Human T-lymphotropic virus type 1 (HTLV-1) is the causative agent of adult T-cell leukemia/lymphoma (ATL), a malignancy of CD4+ T cells that develops in 2–5% of infected individuals over a course of several decades [1], [2]. HTLV-1 transactivator/oncoprotein, Tax, is thought to play a key role in ATL development. Tax is a potent activator of HTLV-1 transcription and NF-κB [2]. To promote viral mRNA synthesis, it acts as an adaptor that links three 21-bp Tax-responsive enhancer elements in the HTLV-1 long terminal repeats (LTRs) to transcription factors CREB/ATF-1 and transcriptional co-activators CBP/p300, p300-CBP-associated factor (PCAF) and transducers of regulated CREB (TORCs) [3]–[5]. Activation of NF-κB by Tax is mediated by direct binding of Tax to the regulatory subunit of I-κB kinase (IKK), NF-κB essential modulator (NEMO), also known as IKKγ. This interaction results in constitutive activation of IKKα and IKKβ, degradation of all I-κBs, and activation of both classical and alternative NF-κB pathways [6]–[8]. The oncogenic activity of Tax in cell culture and in transgenic mice is driven by NF-κB [9]–[13].
We have shown recently that Tax can activate the anaphase promoting complex/cyclosome (APC/C), an E3 ubiquitin ligase that controls metaphase to anaphase transition and mitotic exit [14]. APC/C activation by Tax leads to premature poly-ubiquitination and degradation of mitotic regulators including cyclin B and Skp2 [14]. Skp2 is the substrate-recognition subunit of another E3 ubiquitin ligase known as SCFSkp2, which mediates the destruction of cyclin E/A-CDK2 inhibitor (CKI), p27Kip1 (referred to as p27 henceforth) during S/G2 [15], [16]. The premature degradation of Skp2 as induced by Tax leads to SCFSkp2 inactivation and p27 protein stabilization. The mRNA level of another CKI: p21CIP1/WAF1 (referred to as p21 henceforth) also increases dramatically as a result of promoter activation and mRNA stabilization brought on by Tax [17]. The massive surge in p21 and p27 in turn leads to p53- and pRb-independent cellular senescence termed Tax-induced rapid senescence (Tax-IRS) [14].
Here we show that the p21-/27-mediated cellular senescence induced by Tax constitutes a cellular checkpoint response towards chronic NF-κB hyper-activation. We further demonstrate that RelA is the primary effector of this pathway and RelA acts upstream of the APC/C and RelB to stabilize p27 protein and p21 mRNA respectively. Our results suggest that Impairment to the p21-/27-mediated senescence checkpoint facilitates constitutive NF-κB activation and leukemia development. This is best evidenced by the loss of p27 expression and cytoplasmic localization of p21 in HTLV-1-transformed T cells [14], [18]. Importantly, we found that the HTLV-1 anti-sense RNA-encoded bZip protein, HBZ, could mitigate Tax-induced senescence by virtue of its ability to inhibit NF-κB [19]. HBZ has been shown previously to block trans-activation of viral mRNA expression by Tax [20], [21]. Thus, active HTLV-1 replication characterized by potent Tax-mediated LTR and NF-κB activation leads to senescence, while moderation of Tax activities and attenuation of viral replication by HBZ allow HTLV-1-infected T cells to proliferate, expand, and persist.
Results
NF-κB activation by Tax correlates with senescence induction
To investigate the mechanism by which Tax induces senescence, we analyzed five well-characterized Tax mutants. TaxV89A and TaxL319R, L320S (M47) are deficient in HTLV-1 LTR trans-activation, but competent in NF-κB activation [22], [23]. By contrast, TaxH43Q and TaxT130A, L131S (M22) are defective in NF-κB activation, but are able to trans-activate the HTLV-1 LTR [23], [24]. Finally, TaxK85A mutant is inactive for both [22]. We use the degradation of I-κBα as an indicator of NF-κB activation and the decrease in cyclin B1 and Skp2 levels with concomitant increase in the levels of p21 and p27 as surrogate markers for senescence induction. HeLa cells were transduced with lentivirus vectors carrying each of the Tax alleles or the control GFP gene, and analyzed by immunoblots. As shown in Fig. 1, wild-type Tax (WT) and those Tax mutants (V89A and M47) that are potent activators of NF-κB greatly reduced the levels of cyclin B and Skp2, and dramatically elevated p21 and p27 expression. Tax mutants that are impaired in NF-κB activation (H43Q, K85A, and M22), in comparison, had only moderate or no effect on cyclin B, Skp2, p21, or p27. These data suggest a link between Tax-IRS and persistent NF-κB activation.
NF-κB inhibition by a degradation-resistant I-κBα mutant prevents Tax-induced rapid senescence
We next asked if direct inhibition of NF-κB could prevent Tax-IRS. To this end, we used a lentivirus vector to derive HeLa cell lines that expressed ΔN-I-κBα, a truncated form of I-κBα lacking 36 NH2-terminal amino acid residues that constitute the IKK phosphorylation and degradation domain of I-κBα [25]. This deletion renders ΔN-I-κBα resistant to IKK-mediated degradation. As a result, ΔN-I-κBα constitutively retains NF-κB in the cytoplasm and blocks NF-κB activation [26]. A pool of ΔN-I-κBα-expressing HeLa-G cells (HeLa-G/ΔN-I-κBα) and two cloned cell lines: HeLa-G/ΔN-I-κBα L6 and H5 were generated. HeLa-G/ΔN-I-κBα L6 and H5 respectively express ΔN-I-κBα at lower (L6) and higher (H5) levels than that of the endogenous I-κBα. As expected, E-selectin-Luc reporter assays indicated that NF-κB activation by Ad-Tax (an adenovirus vector for Tax) versus Ad-tTa (an adenovirus vector for the tet trans-activator) control in the HeLa-G/ΔN-I-κBα cell lines were repressed, and the degrees of repression correlated with the extent of ΔN-I-κBα expression (Fig. 2A). We noticed that HeLa-G/ΔN-I-κBα cells in general grew more slowly and took longer to attach to a culture dish after plating. These phenotypes reflect the role of basal NF-κB activity in growth, survival, and expression of adhesion molecules. Efforts to establish ΔN-I-κBα-expressing human T cell lines were unsuccessful however, most likely because of the importance of NF-κB for T cell proliferation and survival.
HeLa-G (CTRL), HeLa-G/ΔN-I-κBα, HeLa-G/ΔN-I-κBα L6, and HeLa-G/ΔN-I-κBα H5 cells were then transduced with Ad-Tax and Ad-tTa vectors respectively, and analyzed for their levels of Tax, I-κBα cyclin B, p21, p27, and actin. As shown in Fig. 2B & C, 48 hours after transduction by Ad-Tax, the endogenous wild-type I-κBα level became greatly reduced in both parental HeLa-G (CTRL) and HeLa/ΔN-I-κBα cells due to Tax-mediated IKK activation (Fig. 2B lanes 2 & 4, Fig. 2C lanes 2, 4 & 6). As expected, Tax was unable to induce ΔN-I-κBα degradation (Fig. 2B lane 4, Fig. 2C lanes 4 & 6). Rather, the level of ΔN-I-κBα was increased by Tax. This is because the cis regulatory element used for ΔN-I-κBα expression is a composite of the HIV LTR and the CMV immediate early promoter known to be activated by Tax. ΔN-I-κBα also blocked the induction and processing of the NF-κB2 precursor, p100, by Tax (compare Fig. 2B lanes 2 & 4), thereby dampening activation of the alternative NF-κB pathway. Importantly, while Tax greatly elevated the levels of p21 and p27 in the parental HeLa-G cells (compare Fig. 2B lanes 1 & 2, and Fig. 2C lanes 1 & 2), little change in p21 or p27 was observed in HeLa-G/ΔN-I-κBα cells (compare Fig. 2B lanes 3 & 4, and Fig. 2C lanes 3 & 4 and 5 & 6). At 48 hours after Ad-Tax transduction, most if not all cell cycle activities ceased for HeLa-G cells as indicated by the complete absence of cyclin B1 (Fig. 2B lane 2). By contrast, HeLa/ΔN-I-κBα cells continued to produce normal levels of cyclin B1 irrespective of Tax (Fig. 2B lane 4, Fig. 2C lanes 4 & 6), suggesting that their cell cycle progression is not significantly influenced by Tax.
HeLa-G/ΔN-I-κBα cells and their parental cell line, HeLa-G (abbreviated from HeLa/18×21-EGFP), all contain a reporter cassette, 18×21-EGFP, composed of the enhanced green fluorescent protein (EGFP) gene transcriptionally regulated by 18 copies of the 21-bp-repeat Tax-responsive enhancer element [27]. Cells harboring the reporter cassette synthesize little EGFP when untreated, but produce it abundantly when infected by an adenovirus (Ad-Tax) or a lentiviral vector (LV-Tax) for Tax, thereby rendering Tax-expressing cells to be easily scored microscopically [18], [27]. To demonstrate further that Tax-IRS can be prevented by blocking NF-κB activation, HeLa-G, HeLa-G/ΔN-I-κBα L6 and HeLa-G/ΔN-I-κBα H5 cells were plated sparsely on a culture dish. Cells were then transduced with Ad-Tax at a multiplicity of infection (MOI) of approximately 1 (viral titer determined on HEK 293 cells) such that 30–50% of the population became transduced, and then monitored for 5 days. As shown in Fig. 3A, Tax-expressing EGFP-positive HeLa-G cells became enlarged, flattened, highly vacuolated, and expressed the senescence-associated β-galactosidase over 5 days. The nuclei of the senescent cells also became significantly larger as previously reported [14], [18]. Soon after Ad-Tax transduction, EGFP-positive (Tax-expressing) HeLa-G cells ceased proliferation (Fig. 3B left column). By contrast, neighboring EGFP-negative cells divided 5–6 times over 5 days to form sizable colonies of approximately 40–50 cells. Importantly, Tax-expressing HeLa-G/ΔN-I-κBα L6 and H5 cells continued to grow and divide (Fig. 3B middle and right columns), albeit their rate of cell division was slightly reduced compared to the un-transduced cells, with most colonies smaller in size and containing 14–30 cells (see Fig. 3 Day 5 middle and right panels). After 5 days in culture, the EGFP expression in the dividing Ad-Tax-transduced colonies decreased moderately and sometimes became variegated. This is likely a result of the transient nature of Ad-vector-driven Tax expression and the dilution of Tax upon successive cell divisions. Interestingly, as long as ΔN-I-κBα was expressed at a level comparable to that of the endogenous I-κBα (Fig. 3B, ΔN-I-κBα L6), Tax-IRS could be effectively prevented (Fig. 3B and supplemental Fig. S3A). No advantage was seen with a higher level of ΔN-I-κBα expression (Fig. 3B, ΔN-I-κBα H5). This suggests that once a threshold level of ΔN-I-κBα sufficient to block NF-κB is reached, additional ΔN-I-κBα has little biological impact. Finally, HeLa-G/ΔN-I-κBα L6 and H5 cells were transduced with a lentivirus vector for Tax. Indeed, stable Tax expression was readily established in these cells (Fig. 3C). In HeLa-G/ΔN-I-κBα/Tax cell lines (L6 Tax-1 L6 Tax-7, H5 Tax-1, and H5 Tax-5), endogenous I-κBα was undetectable, consistent with its degradation after IKK activation by Tax. Their levels of cyclin B1, p27, and p21, however, were similar to the Tax-null parental cell lines (Fig. 3C, HeLa-G, ΔN-I-κBα L6, and ΔN-I-κBα H5). Finally, the flow cytometry DNA histogram of the L6 Tax-7 cell line was similar to that of the parental ΔN-I-κBα L6 cell line except for a small increase and a corresponding decrease of cells in the G1 and the S phases respectively (Fig. 3D), reflecting slower growth of Tax-expressing cells, but in stark contrast to the dramatic change seen in Tax-expressing HeLa-G cells (Fig. 3E and previous publications [14], [18]). It should be pointed out that time-lapse microscopy of reporter cells expressing fluorescent-ubiquitin-cell-cycle indicators [28] has revealed that many Ad-Tax-transduced cells completed S/G2, but bypassed mitosis and became arrested in G1/senescence, but with G2/M DNA content (Yang et al. manuscript in revision). These results demonstrate that Tax-induced senescence is NF-κB-driven and suggest that many of the cell cycle abnormalities induced by Tax may also be caused by NF-κB. Once NF-κB is blocked by ΔN-I-κBα, constitutively activated IKK has minimal impact on cell cycle progression or senescence.
Hyper-activated NF-κB stabilizes p27 protein and p21 mRNA
We have shown recently that Tax stablizes p27 protein in part by causing APC/C-mediated poly-ubiquitination and degradation of Skp2, the substrate-recognition subunit of SCFSkp2, the E3 ubiquitin ligase that targets p27 for destruction [14]. Tax also up-regulates p21 expression by promoter trans-activation and mRNA stabilization [17]. Since NF-κB inhibition prevented the up-regulation of p21 and p27 by Tax, we asked if p27 protein stabilization and p21 mRNA stabilization were also NF-κB-driven. The stabilities of p21 and p27 proteins in HeLa-G and its ΔN-I-κBα progenies L6 and H5 were similar after infection with the control Ad-tTa vector, (Fig. 4A) suggesting that NF-κB in HeLa-G cells was already regulated by endogenous I-κBα, additional blocking of NF-κB with ΔN-I-κBα did not alter the levels of p21 and p27. By contrast, the stabilization of p27 protein and the increase of p21 mRNA (through stabilization) caused by Tax were abrogated by ΔN-I-κBα (Fig. 4B & C, compare HeLa-G control, CTRL, with its ΔN-I-κBα-expressing progenies L6 and H5). Trans-activation of the p21 promoter by Tax was unaffected by NF-κB inhibition except for a reduction in overall luciferase reporter activities in ΔN-I-κBα H5 cells (Fig. 4D). This is as might be expected if NF-κB mediates the stabilization of p21 mRNA. These data support the notion that NF-κB is the upstream effector of the increase in p21 mRNA stability and APC/C-mediated p27 protein stabilization.
RelA mediates senescence induction by Tax
As Tax activates all NF-κB/Rel family members including RelA, c-Rel, RelB, p50 and p52, we ask which NF-κB/Rel member(s) is/are responsible for Tax-IRS. To this end, we over-expressed RelA, RelB, and c-Rel, the three NF-κB/Rel members that contain trans-activation domains by transducing HeLa-G cells with adenovirus expression vectors: Ad-RelA, Ad-RelB, and Ad-c-Rel respectively. RelA dramatically activated the E-selectin-Luc NF-κB reporter construct in a dose-dependent manner as expected (supplemental Fig. S1A). Since I-κBα mRNA transcription is under NF-κB control, the levels of I-κBα in Ad-RelA-transduced cells also increased sharply in accordance with RelA levels (Fig. 5A). Likewise, the levels of RelB, p100, and p52 were also elevated in a dose-dependent manner in response to RelA (Fig. 5A), indicating that RelA is a critical activator of the alternative NF-κB pathway. Surprisingly, except for a small increase in p27, no dramatic change in p21 or cyclin B level was detected in cells over-expressing RelA (Fig. 5A), and no overt cellular senescence was observed (supplemental Fig. S1B). RelB and to a lesser extent, c-Rel, increased p21 expression. C-Rel, but not RelB, further raised p27 level (Fig. 5B & C). These increases in p21 and p27 levels are relatively modest when compared to those caused by Tax however. Similar to RelA, c-Rel dramatically induced I-κBα expression. By contrast, RelB had only a moderate effect on I-κBα, but significantly induced the expression, but not the processing of p100, which is expected to bind and retain RelB in the cytoplasm in its inactive form (Fig. 5B). Finally, c-Rel also increased p100 expression (Fig. 5A & C) and elevated RelB levels, but had little effect on RelA and vice versa (Fig. 5A). No overt senescence was observed for cells over-expressing RelB and c-Rel (supplemental Fig. S1B).
While these data suggest that the classical NF-κB pathway, when activated, can positively affect p100 expression and processing as reported recently [29] and that RelA and c-Rel can up-regulate p27 while RelB, p21, the effects of RelA, RelB and c-Rel on p21 and p27 induction were modest most likely because their activities were quickly dampened by the surge in I-κBα and p100 (Fig. 5A–C). As such, these results were inconclusive in implicating a specific NF-κB/Rel family member as the key mediator of Tax-induced senescence. For this reason, stable expression of small hairpin RNA (shRNA) in HeLa-G cells was carried out to knockdown RelA, RelB, c-Rel, and p100 respectively (Fig. 5D). Most interestingly, knockdown of RelA and to a rather limited extent, that of RelB, but not that of c-Rel or p100 prevented Tax-induced senescence (Fig. 5E and supplemental Fig. S3B). This is evidenced by the proliferation of EGFP+ HeLa-G/RelAKD cells (Fig. 5E sh-RelA Day 5) and the absence of p21 and p27 up-regulation therein after Ad-Tax transduction (Fig. 5F, sh-RelA). We observed limited cell division of EGFP+ HeLa-G/RelBKD cells after Tax expression (sh-RelB panels of Fig. 5E). This partial effect correlated with the muted p21 but highly robust p27 induction by Tax in HeLa-G/RelBKD cells (sh-RelB panels 5F). These results demonstrate RelA to be the major effector of Tax-IRS. Furthermore, the facts that RelB knockdown prevents Tax/RelA-/NF-κB-induced p21 increase and RelA can up-regulate RelB expression (Fig. 5A) indicate that RelB acts downstream of RelA to stabilize p21 mRNA (Fig. 5F).
HBZ mitigates senescence induction by Tax
The 3′ region of HTLV-1 encodes an mRNA transcript of opposite polarity to the major HTLV-1 mRNA. This anti-sense mRNA is singly spliced and encodes a basic domain-leucine zipper protein known as the HTLV-1 b-Zip (HBZ) protein [20]. Earlier studies have indicated that HBZ could down-regulate Tax-mediated trans-activation of the HTLV-1 LTR by binding CREB, c-Jun, and CBP/p300 [20], [21]. Most recently, HBZ has been shown to selectively inhibit the classical NF-κB pathway by blocking RelA binding to DNA and by targeting RelA for ubiquitin-mediated degradation [19]. That HBZ antagonizes the activities of Tax by dampening LTR trans-activation and NF-κB activation, and the results herein showing that NF-κB hyper-activation by Tax triggers senescence raise the possibility that HBZ may prevent Tax-IRS. Indeed, in agreement with published results, NF-κB and LTR activation by Tax are both attenuated by HBZ (supplemental Fig. S2A & B). The HBZ TTG mutant wherein the HBZ translational initiation site ATG had been mutated to TTG failed to block NF-κB or LTR activation by Tax (supplemental Fig. S2A & B).
To determine if HBZ can mitigate or prevent Tax-IRS, a Flag-epitope-tagged HBZ cDNA construct was generated by PCR using the cDNA of the spliced HBZ mRNA as template, and inserted into the pBabe-Puro murine retroviral vector [30] to yield pBabe-Flag-HBZ. Like native HBZ, Flag-HBZ efficiently inhibits NF-κB activation by Tax (supplemental Fig. S2C). HeLa-G cells expressing Flag-HBZ (HeLa-G/Flag-HBZ) were then derived after retroviral gene transfer and puromycin selection, and confirmed for HBZ expression by immunoblotting (compare Fig. 6A lanes 2 & 3). Consistent with the notion that HBZ inhibits NF-κB, the level of p100, an endogenous NF-κB-inducible gene (see Fig. 5A), was lowered in HBZ-expressing cells (compare Fig. 6A lanes 4 & 5). This is in contrast to the previous report that HBZ down-regulates only the classical but not the alternative NF-κB pathway [19]. No significant change in the level of RelA was detected in HBZ-expressing cells (Fig. 6A). Thus, the inhibition of NF-κB by HBZ is likely due more to a direct inhibition of NF-κB binding to DNA and less to HBZ-induced RelA degradation. Importantly, a significant number of HeLa-G/Flag-HBZ cell clones transduced by Ad-Tax continued to divide up to 3–4 cell division cycles but eventually ceased proliferation, indicating that Ad-Tax-induced senescence was delayed by HBZ (Fig. 6B). The degree of senescence resistance of HeLa-G/Flag-HBZ is approximately 25% (supplemental Fig. S3C), hence no dramatic change in p21 and p27 up-regulation was observed (not shown). Finally, stable cell lines (H3-6 HBZ+Tax+ is shown as an example) that express low levels of Tax could be established in HeLa-G/Flag-HBZ cells (H3 HBZ+) after transduction by the Tax lentivirus vector, LV-Tax (Fig. 6C & D). While NF-κB activation in these cells was undetectable due to HBZ and a low level of Tax expression (Fig. 6E, E-selectin-Luc reporter assay), the 18×21-EGFP reporter remained significantly induced (see Fig. 6C fluorescence image) and LTR-Luc reporter trans-activation readily detected (Fig. 6E, compare H3 HBZ+ and H3-6 HBZ+Tax+). These results support the notion that HBZ can moderate NF-κB activation by Tax and thereby delay or prevent the onset of senescence. This in turn allows cells expressing low to moderate levels of Tax to grow, divide, and produce viral particles. Importantly, these results strongly suggest that in order for NF-κB hyper-activation by Tax to drive pre-leukemic or leukemic cell growth, inactivation of the senescence checkpoint is still necessary.
Discussion
The data reported herein have revealed constitutive IKK activation and NF-κB hyper-activation to be the cause for Tax-induced cellular senescence. These results have further established RelA to be the major driver of cellular senescence. Because NF-κB activation is often associated with cell survival and proliferation, we previously thought that a mechanism distinct from IKK/NF-κB activation is responsible for the cellular senescence induced by Tax [31]. Present data show unequivocally that the potentially deleterious IKK/NF-κB hyper-activation by Tax (or other means) immediately triggers a checkpoint mediated by p21 and p27, which act independently of pRb and p53 to induce cellular senescence [14].
We have previously reported that the stabilization of p27 by Tax is a result of premature activation of the APC/C, which brings about degradation of Skp2 and inactivation of SCFSkp2, the E3 ligase that targets p27 for degradation [14]. Present data indicate that hyper-activated NF-κB acts upstream of APC/C to stabilize p27. How NF-κB (RelA specifically) affects unscheduled activation of the APC/C remains to be elucidated. In agreement with our results, the loss of Skp2 has been shown recently to facilitate p21-/p27-mediated and Arf/p53-independent senescence in Skp2-/p19Arf-null mice [32].
The dramatic induction of p21 mRNA by Tax is a result of both promoter trans-activation and mRNA stabilization [17]. The increase in p21 mRNA stability is now shown to be RelB-dependent. Since RelB expression is up-regulated by RelA [29] (also see Fig. 5A), repression or knockdown of RelA effectively prevents p21 mRNA increase. How RelB increases p21 mRNA stability is not clear at present. It may promote the expression of a cellular factor crucial for blocking p21 mRNA degradation.
We think p21-/p27-mediated senescence constitutes a checkpoint for blocking potentially oncogenic IKK-NF-κB hyper-activation. Since NF-κB is constitutively active in many human cancers, especially leukemia, present data would suggest that cellular changes that disable this senescence pathway must accompany NF-κB de-regulation in human cancers. Indeed, impairments of p21 and p27 function and expression have been observed in most if not all HTLV-1-transformed T cells previously [14], [33]. Studies of human breast cancers also show a correlation between the over-expression of IKK (i.e. chronic NF-κB activation) and the cytoplasmic localization of p21, in support this conclusion [34]. We think Tax-induced cell cycle aberrations such as DNA damage, and chromosome instability is likely to be NF-κB-mediated. That HeLa-G/ΔN-I-κBα/Tax cell lines are largely normal in their growth and division is consistent with this conclusion.
Cellular signaling pathways activated by oxidative stress, inflammation, and DNA damage are known to cause aging and shortened lifespan, and these pathways impact NF-κB activation [35]. Earlier studies have also implicated NF-κB/Rel in aging, cell cycle arrest, or senescence [36]–[39]. Senescent cells are known to secret chemo-attractants for macrophages and NK cells [40], which are responsible for their eventual elimination. Whether senescent HTLV-1-infected cells may use this mechanism for virus transmission and spread, especially to macrophages, can only be speculated upon at this point.
Our results also show that NF-κB activation caused by the over-expression of RelA, RelB, or c-Rel, however potent it may be, occurs transiently and leads rapidly to a steep surge in I-κBα and p100 (and possibly other I-κB proteins), which promptly dampen NF-κB activity and prevent drastic p21/p27 up-regulation and senescence. This contrasts with the NF-κB hyper-activation by Tax that is mediated by the destruction of I-κBα and I-κB-like molecules via activated IKKs.
How does HTLV-1 infection lead to adult T-cell leukemia when the expression of Tax causes senescence? Based on our results, moderation of Tax activities by HBZ, especially at the level of NF-κB activation, is obligatory for the proliferation and expansion of infected cells. Thus, the balance between Tax and HBZ expression, determined by the sites of proviral integration and the availability of cellular transcription factors, can modulate the extent of viral replication and NF-κB activation during infection. This, in turn, may determine the fate of infected cells, which likely ranges from robust viral replication and senescence, oligoclonal expansion, to viral latency and persistence (Fig. 7). Recently, Tax has been shown to up-regulate the expression of HBZ and this up-regulation is influenced by the HTLV-1 integration sites [41]. Furthermore, HBZ has been found to enhance viral infectivity and persistence, and facilitate proliferation of HTLV-1-infected lymphocytes [42], [43]. Finally, HBZ mRNA expression has been shown to correlate with HTLV-1 proviral load while Tax expression was found to decline over time after HTLV-1-infection in a rabbit model [44]. These results are consistent with the notion that HBZ plays a critical role in viral persistence in part by down-regulating the senescence-inducing activity of Tax (Fig. 7). Finally, Tax-induced senescence should be considered as a precancerous condition. While HBZ may either delay or prevent the onset of senescence by attenuating the expression of Tax and NF-κB activation by Tax, cellular changes that inactivate the senescence checkpoint may ultimately facilitate potent and persistent NF-κB activation by Tax to promote leukemia development.
ATL cells often cease to express Tax, but continue to produce HBZ mRNA and, presumably, HBZ protein [45]. Whereas Tax, in association with HBZ, may facilitate cell proliferation and survival in the early stage of HTLV-1 infection, at a later time, cytotoxic T lymphocyte killing of Tax-expressing cells likely select for loss of Tax expression. It is conceivable that defects in the senescence checkpoint that develop during the evolution of the infected cells then facilitate the emergence of Tax-independent NF-κB activation (Fig. 7). Finally, the mitogenic activity of HBZ mRNA [46] may also play a role in leukemia maintenance.
Materials and Methods
Immunoblotting
Standard methods were used for immunoblotting and flow cytometry. Each sample typically contains 20-30 µg of whole cell proteins. HTLV-1 Tax hybridoma antibody 4C5 was as described [14]. The rabbit polyclonal antibody against HBZ was a kind gift of Dr. Jean-Michel Mesnard. Other antibodies used are as listed (supplemental Table S1).
Adenovirus vectors
Recombinant adenovirus vectors Ad-Tax, Ad-tTA, Ad-RelA, Ad-RelB, and Ad-c-Rel were grown and titered as previously published [14].
Derivation of HeLa cell lines
The cDNA for the degradation-resistant I-κBα, ΔN-I-κBα, was generated by PCR (see supplemental Table S2 for primer sequences). BamHI and EcoRI restriction endonuclease sites were used to subclone the cDNA into LV-SV-puro vector [18], [27]. HeLa/18×21-EGFP (HeLa-G) cells [18] were transduced with LV-ΔN-I-κBα-SV-puro, grown in DMEM containing fetal bovine serum (10%) and puromycin (1 µg/ml, Sigma-Aldrich) for one week with change of medium every 48 hours. HeLa-G/ΔN-I-κBα clones were then isolated in 96-well plates after limiting dilution and confirmed for ΔN-I-κBα expression by immunoblotting. The cDNA of the COOH-terminus Flag-tagged HBZ (Flag-HBZ) was generated by PCR (primer sequences listed in supplemental Table S2) using the cDNA of the spliced HBZ transcript as the template [45] and cloned into an MuLV-based retroviral vector, pBabe-Puro [30]. The pBabe-Flag-HBZ retroviral vector was produced as described [47]. HeLa-G transduced by the Flag-HBZ retroviral vector was selected in medium containing puromycin (1 µg/ml) and cloned by limiting dilution.
Luciferase reporter assay
Each of the NF-κB, HTLV-1 LTR and p21 promoter constructs (E-selectin-Luc, LTR-Luc and p21-Luc) together with pRL-TK, a control plasmid that contains the HSV thymidine kinase (TK) promoter-driven Renilla luciferase reporter cassette (Promega), were used in the luciferase reporter assays according to standard procedures [17]. The p21 (−2.4 kb to +16)-Luc (also known as WWP-luc) was kindly provided by Dr. Wafik S EL-Deiry.
Flow cytometry
Cells were harvested after trypsin treatment, and washed twice with 2 ml of cold phosphate-buffered saline solution (PBS), resuspended in 0.5 ml of PBS and fixed in 5 ml of 70% ethanol overnight at 4°C. Ethanol-fixed cells were then washed twice with 5 ml of cold PBS containing 1% bovine serum and incubated for 30 min at 37°C in 1.0 ml of a solution containing propidium iodide (PI) (20 µg/ml) and RNase (1 mg/ml), filtered through a 70-micron cell strainer (BD Falcon, Cat. 35-2350) to remove cell clumps. The cellular DNA content was determined by fluorescence-activated cell sorting (FACS) (EPICS XL-MCL flow cytometer; Beckman-Coulter). The percentages of cells in G0/G1, S, and G2/M phases of the cell cycle were computed using the ModFit LT software. Ordinate: cell numbers; abscissa: DNA content.
Protein half-life determination and quantitation of p21 mRNA
The half-lives of p21 and p27 were measured as previously published [17]. The mRNA levels of p21 were measured by real-time PCR as described [17] using the primers listed (supplemental Table S2).
Knockdown of NF-κB genes
HeLa-G cell lines with stable knockdown of each of the NF-κB members, RelA, RelB, c-Rel and p100, were isolated after screening cell clones (by immunoblotting) transduced by pooled shRNA lentiviral vectors containing the puromycin-resistance gene. The sequences targeted for each gene are as listed (supplemental Table S3).
Accession numbers
The GENBANK accession numbers or ID numbers for genes encoding the proteins described in this article are: HTLV-1 Tax: AB038239; HTLV-1 HBZ: DQ273132; p21: NM_000389; p27: NM_004064; Cyclin B1: NM_031966; Skp2: NM_005983; I-κBα: NM_020529; p100/p52: NM_002502; p105/p50: NM_003998; RelA: NM_021975; RelB: NM_006509; and c-Rel: NM_002908.
Supporting Information
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