Abstract
The posttranslational modifications (PTMs) of microtubules have been reported to play an important role in cancer aggressiveness, including apoptosis resistance. In this study, we aimed to investigate the biological role of microtubule PTMs in the regulation of paclitaxel responsiveness. The acetylated tubulin (Ace-tub) level was strongly associated with paclitaxel sensitivity, as observed in patient-derived primary lung cancer cells and xenografted immunodeficient mice. We showed that paclitaxel-resistant H460 lung cancer cells, generated by a stepwise increase in paclitaxel, exhibited markedly increased tubulin acetylation and consequently acquired paclitaxel resistance. Upregulation of tubulin acetylation by overexpression of α-tubulin acetyltransferase 1 wild-type (αTAT1wt), an enzyme required for acetylation, or by treatment with trichostatin A (TSA), a histone deacetylase 6 (HDAC6) inhibitor, significantly attenuated paclitaxel-induced apoptosis. Investigation of the underlying mechanism revealed that the levels of antiapoptotic Mcl-1 appeared to increase in αTAT1wt-overexpressing and TSA-treated cells compared to control cells, whereas the levels of other antiapoptotic regulatory proteins were unchanged. On the other hand, decreased tubulin acetylation by αTAT1 RNA interference downregulated Mcl-1 expression in patient-derived primary lung cancer and paclitaxel-resistant lung cancer cells. A microtubule sedimentation assay demonstrated that Mcl-1 binds to microtubules preferentially at Ace-type, which prolongs the Mcl-1 half-life (T1/2). Furthermore, immunoprecipitation analysis revealed that polyubiquitination of Mcl-1 was extensively decreased in response to TSA treatment. These data indicate that tubulin acetylation enhances the resistance to paclitaxel-induced cell death by stabilizing Mcl-1 and protecting it from ubiquitin–proteasome-mediated degradation.
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Introduction
Lung cancer is an aggressive malignancy being the highest causes of cancer-related mortality1. The 5-year survival rate of lung cancer patients has considerably declined to only to 19%, even though the therapeutic interventions have greatly improved. Most of lung cancer patients acquire chemotherapeutic resistance, an important hallmark of cancer, and some exhibited intrinsic deregulation of cell death mechanisms2. Paclitaxel is a potent anticancer drug that binds to microtubules and inhibits microtubule depolarization during mitosis3. Paclitaxel is a first-line treatment for late-stage lung cancer that exhibits high efficacy4,5; however, the clinical response rate remains unsatisfactory6,7, as chemotherapeutic resistance limits its effective clinical use. A better understanding of the molecular basis of apoptotic deregulation is essential.
Several mechanisms of resistance to paclitaxel-induced apoptosis have been reported, and the significant role of microtubule physiology has been emphasized. Microtubules, which are important cytoskeletal proteins, govern numerous cellular activities, including cell division and cell migration. The altered patterns of microtubule posttranslational modifications (PTMs) and tubulin isotypes in cancer cells play critical roles in mediating aggressive behaviors in cancer through the intracellular trafficking of not only cytoplasmic components but also diverse signaling molecules8,9. Tubulin acetylation, a stable form of microtubule PTM in which α-tubulin is acetylated, is increased in breast cancer, which promotes the formation of microtentacles, tubulin-based membrane protrusions that facilitate breast cancer cell migration10,11. Tubulin acetylation preserves the active status of protein kinase B/Akt, a core component of a key oncogenic signaling pathway, and consequently enhances epithelial-to-mesenchymal transition in lung cancer12. Mutation at lysine 40 on α-tubulin, which interferes with tubulin acetylation, conferred resistance to paclitaxel-mediated suppression of cancer cell growth13. A recent study also demonstrated that an increase in acetylated microtubules suppresses the activity of caspase-3, an executioner enzyme in apoptosis and that this process is mediated by apolipoprotein C-I pseudogene 114. In addition, a clinical investigation reported that mutation of the β-tubulin gene is tightly associated with a low paclitaxel response rate8, and overexpression of βIII-tubulin enhances paclitaxel resistance and disease progression by altering microtubule instability15. Furthermore, an increase in the level of βII- and βIII-tubulin, coexisting with acetylated tubulin (Ace-tub), contributes to paclitaxel resistance in ovarian cancer cells16. The modulation of tubulin isotype composition on paclitaxel sensitivity is well characterized; however, the potential effect of microtubule PTMs on paclitaxel resistance as well as the molecular signaling involved are not yet fully understood.
In this study, we aimed to investigate the biological roles of microtubule PTMs in paclitaxel sensitivity in lung cancer cells. Our results showed that Ace-tub exhibited a strong correlation with paclitaxel responsiveness. Multiple administrations of paclitaxel-mediated drug resistance by enhancing tubulin acetylation. Genetic manipulation and chemical inhibitors were applied to increase tubulin acetylation, which upregulated the antiapoptotic Mcl-1 level by preventing its degradation through the ubiquitin–proteasome pathway. This study, therefore, provides intriguing evidence that microtubule PTMs confer paclitaxel resistance by altering acetylation and targeting to the antiapoptotic Mcl-1 protein in lung cancer cells.
Results
Tubulin acetylation levels are related to paclitaxel sensitivity in patient-derived primary lung cancer cells
We first investigated the correlation of paclitaxel responsiveness and microtubule PTMs in patient-derived primary lung cancer cells. Analysis of the 50% inhibitory concentration (IC50) of paclitaxel demonstrated that ELC17 cells had the highest value (IC50 = 55.71 ± 2.13 nM), followed by ELC12 (IC50 = 50.60 ± 3.81 nM), ELC20 (IC50 = 49.09 ± 3.86 nM), and ELC16 (IC50 = 47.59 ± 4.34 nM) cells, respectively. Western blot analysis revealed that the Ace-tub expression level appeared to follow the trend for the IC50 value, suggesting that greater Ace-tub expression levels are associated with lower responsiveness to paclitaxel (Fig. 1a). However, tyrosinated tubulin (Tyro-tub) and detyrosinated tubulins (Detyro-tub) levels did not clearly correspond to the IC50. To confirm this finding, Pearson’s correlation analysis was performed between the microtubule PTM level and the IC50. The results showed that tubulin acetylation exhibited the most relevance to drug sensitivity, with a correlation coefficient of 0.7506, while other PTMs have lower correlation coefficients (Fig. 1b). These data indicated that the level of tubulin acetylation might be related to paclitaxel sensitivity.
Multiple paclitaxel administrations upregulate tubulin acetylation in an in vivo xenograft
We investigated in vivo paclitaxel responsiveness in xenografted immunodeficient mice. The mice were subcutaneously injected with H460 non-small-cell lung cancer (NSCLC) cells and then treated with drug or normal saline every 2 days for five cycles (Fig. 2a). Tumor nodules were further monitored for 30 days and collected at the end of the experiment. The results showed that during the first period of time (days 10–30), paclitaxel slightly suppressed in vivo tumor growth (Fig. 2b), but after 30 days posttreatment, the tumor nodules in the treatment group gradually expanded, and the size was comparable to that in the control group. However, the mouse weight was not significantly altered from that of the control (Fig. 2c). Interestingly, tubulin acetylation was extensively upregulated in the paclitaxel-treated group (Fig. 2d), suggesting that repetitive paclitaxel administration increased tubulin acetylation levels and might be involved in paclitaxel resistance.
Tubulin acetylation is upregulated in paclitaxel-resistant lung cancer cells
To investigate whether lung cancer cells acquired paclitaxel resistance by upregulation of tubulin acetylation, paclitaxel-resistant H460 NSCLC cells were established by a stepwise increase in paclitaxel concentration from 12.5 nM (cycle 1) to 800 nM (cycle 7) (Fig. 3a), and cell viability in response to paclitaxel was examined. The data revealed that multiple increasing doses of paclitaxel significantly enhanced drug resistance in H460 NSCLC cells (Fig. 3b). The IC50 was markedly increased from cycle 1 to 7, cells at cycle 7 (H460/PTXR-C7) treated with paclitaxel up to 800 nM had an IC50 ~100-fold greater than that of control cells. Consistently, the number of apoptotic cells with DNA condensation and apoptotic bodies was strikingly decreased in H460/PTXR-C7 cells treated with paclitaxel (Fig. 3c). A dose of 100 nM paclitaxel induced the apoptosis of ~75% of H460/Ctrl cells, whereas ~40% of H460/PTXR-C7 cells underwent apoptosis. Western blot analysis demonstrated that tubulin acetylation was gradually upregulated in paclitaxel-resistant cells compared to their passage-matched controls (Fig. 3d). These results indicate that repeated paclitaxel treatment mediates drug resistance and increases tubulin acetylation levels in NSCLC and that upregulation of tubulin acetylation might be involved in resistance to this drug.
The overexpression of Ace-tub, triggered by α-tubulin N-acetyltransferase 1 (αTAT1) transfection and histone deacetylase 6 (HDAC6) inhibitor treatment, mediates paclitaxel resistance
αTAT1 is a primary enzyme responsible for the addition of an acetyl group on α-tubulin at lysine 4012; thus, to verify the role of tubulin acetylation on paclitaxel sensitivity, tubulin acetylation was induced by transfection with GFP-tagged αTAT1 wild-type (GFP-αTAT1wt) or its dominant-negative mutant (GFP-αTAT1D157N) plasmid, whose enzymatic activity was suppressed. Western blot analysis demonstrated the corresponding GFP expression in these transfectants. Tubulin acetylation was upregulated in GFP-αTAT1wt-transfected H460 cells (H460/αTAT1wt), whereas it was not altered in H460/αTAT1D157N cells compared to mock-transfected control cells (H460/Ctrl) (Fig. 4a). Immunofluorescence assays also revealed that the ratio of acetylated microtubules in the GFP-positive group was greater than that in the GFP-negative group of H460/αTAT1wt cells, whereas no significant change was observed between the GFP-positive and -negative cells of the H460/αTAT1D157N group (Fig. 4b). Because the transfection efficiency was very low, apoptotic cell death was closely observed at an individual cell level. The data showed that apoptotic cell death mediated by paclitaxel was clearly attenuated in GFP-positive H460/αTAT1wt cells, whose tubulin acetylation was enhanced, compared to GFP-negative H460/αTAT1wt cells (Fig. 4c). However, the apoptosis rate of GFP-positive H460/αTAT1D157N cells was comparable to that of GFP-negative cells.
To confirm the above finding, H460 and A549 NSCLC cells were treated with various noncytotoxic concentrations of trichostatin A (TSA), an inhibitor of HDAC6, which is a dominant enzyme required for the removal of the acetyl group from α-tubulin, to minimize the interference of this factor in cell death (Supplementary Fig. 1). Western blot analysis showed that tubulin acetylation was gradually upregulated in a dose-dependent manner (Fig. 4d). Furthermore, paclitaxel-mediated apoptosis was attenuated by TSA treatment. The apoptosis rate was ~80% among H460 cells treated with paclitaxel (200 nM), whereas it was reduced to 45% in the presence of TSA (Fig. 4e, left). Consistently, the apoptosis rate of A549 cells was significantly lower in the TSA-pretreated group than in the group treated with paclitaxel alone (Fig. 4e, right). These data indicate the important role of tubulin acetylation in the regulation of paclitaxel responsiveness.
Tubulin acetylation upregulates the levels of antiapoptotic Mcl-1
To gain insight into the molecular mechanism, the antiapoptotic regulatory proteins in the Bcl-2 family were investigated. H460 and A549 NSCLC cells were treated with TSA, and protein expression was examined by western blot analysis. The data showed that antiapoptotic Mcl-1 was extensively elevated in a dose-dependent manner, whereas the other antiapoptotic proteins, Bcl-xL and Bcl-2, were unchanged in both H460 and A549 NSCLC cells (Fig. 5a); the changes in Mcl-1 levels corresponded to the changes in tubulin acetylation levels (Fig. 4d). Consistently, immunofluorescence assays demonstrated that GFP-αTAT1wt-overexpressing H460 cells (H460/GFP-αTAT1wt) exhibited an increase in Mcl-1 levels compared to those in GFP-negative cells, whereas the Mcl-1 levels were not altered in H460/GFP-αTAT1D157N cells (Fig. 5b). Interestingly, an in vivo xenograft experiment revealed that upregulation of Mcl-1 was clearly observed in the paclitaxel-treated group (Fig. 5c). Furthermore, paclitaxel-resistant cells exhibited elevated Mcl-1 expression compared to that in their passage-matched controls (Fig. 5d), indicating an association of Mcl-1 expression and tubulin acetylation levels.
To test the hypothesis that tubulin acetylation regulates Mcl-1 levels, ELC17, and H460/PTXR-C7 cells, which have the highest tubulin acetylation levels among the cells assessed, were transfected with siRNA targeting αTAT1. Western blot analysis revealed that tubulin acetylation was decreased in response to αTAT1 knockdown in both ELC17 cells (Fig. 5e) and H460/PTXR-C7 cells (Fig. 5f). Furthermore, Mcl-1 expression was significantly decreased in siαTAT1-transfected cells, suggesting that tubulin acetylation positively regulates Mcl-1 expression.
Tubulin acetylation stabilizes the antiapoptotic protein Mcl-1 and prevents its ubiquitin–proteasome-mediated degradation
Since microtubules have been reported to be involved in cellular trafficking and to regulate several molecules interacted17, we hypothesize that microtubule PTMs, especially acetylation, might modulate Mcl-1 binding on them. The interaction of Mcl-1 with microtubules was first investigated by a microtubule sedimentation assay. The results revealed that Mcl-1 was observed in both the pellet fraction (P) of microtubules and the supernatant fraction (S) of other intracellular compartments (Fig. 6a). However, after treatment with nocodazole, a microtubule-disrupting agent, Mcl-1 in the microtubule fraction (P) was clearly diminished, and the ratio of Mcl-1 in the pellet to the total fraction in both cell lines was significantly decreased, indicating that Mcl-1 adhered to the microtubules. Furthermore, the accumulation of Mcl-1 in the microtubule compartment (P) was notably increased in the presence of TSA, a deacetylation inhibitor (Fig. 6b), indicating that Mcl-1 localized preferentially to microtubule acetylation.
The ubiquitin–proteasome-mediated degradation process is reported to regulate intracellular Mcl-1 levels18,19. The degradation rate of Mcl-1 was examined by pretreatment of the cells with cycloheximide (CHX), a protein synthesis inhibitor, and the endogenous Mcl-1 levels were investigated. Western blot analysis revealed that Mcl-1 levels were declined over time, with T1/2 values of 0.89 ± 0.11 h and 0.35 ± 0.16 h in H460 and A549 cells, respectively (Fig. 6c). However, in the presence of TSA, the Mcl-1 level was stable, and the T1/2 appeared to increase to 2.35 ± 0.25 h in H460 cells and to 2.99 ± 0.54 h in A549 cells (Fig. 6c). Furthermore, to test the hypothesis that Ace-tub prevents Mcl-1 degradation via a ubiquitin–proteasome-mediated mechanism, the polyubiquitination of Mcl-1 was investigated. Immunoprecipitation assay demonstrated that the polyubiquitination of Mcl-1 was notably suppressed in response to TSA treatment in a dose-dependent manner (Fig. 6d). This result indicates that tubulin acetylation is required for Mcl-1 stability, contributing to paclitaxel resistance.
Discussion
Apoptosis resistance remains a serious clinical problem, especially in lung cancer20. Although its clinical management has advanced, resistance to chemotherapeutic drugs often occurs, leading to undesirable outcomes. Paclitaxel, a standard therapy in lung cancer, exhibits an effective curative rate; however, the acquisition of drug resistance and cancer relapse appears to be major obstacles21. A better understanding of the underlying molecular mechanism could provide a therapeutic strategy or drug target for achieving satisfactory outcomes in the clinical. In the current work, we showed for the first time on the mechanism of resistance to paclitaxel-mediated apoptosis, which is regulated by microtubule PTMs in NSCLCs. Multiple administrations of paclitaxel enhanced tubulin acetylation and consequently upregulated Mcl-1 levels. We further found that Mcl-1 interacts with microtubules, preferentially on Ace-tub, which is important for Mcl-1 stabilization, protecting it from degradation and mediating drug resistance.
Microtubules, important intracellular cytoskeletal components, are well known as key players in maintaining of cellular morphology and supporting several cellular activities. The hollow-like structure of microtubules consisted of α- and β-tubulin dimers, and the elongation and shrinkage of tubulin dimers enable their dynamic nature and thus their cellular functions22. Their regulatory roles, in association with oncogenic functions, are often emphasized in cancer cell biology and are targets for various anticancer drugs8,23. Paclitaxel, a microtubule-stabilizing drug, directly binds to β-tubulin and inhibits microtubule disassembly during cell division, consequently mediating cell death24. Accumulating studies have demonstrated that prolonged treatment with paclitaxel leads to drug resistance in an association with tubulin-related changes, including alterations in tubulin isotypes and microtubule PTMs. Clinical investigations have reported that patients with mutations in β-tubulin have a low response rate to such drugs15 and that upregulation of class III β-tubulin leads to resistance to paclitaxel in ovarian cancer25,26,27. Likewise, microtubule PTMs, paclitaxel-resistant breast cancer cells exhibit an elevation in Tyro-tub28 and an increase in polyglutamylated microtubules in cooperation with septin filaments29. We also found a strong correlation of α-tubulin acetylation with paclitaxel sensitivity in patient-derived primary lung cancer cells (Fig. 1). Upregulation of tubulin acetylation was observed in xenograft tissues after the complete course of drug administration (Fig. 2d), but tumor size was not affected. Consistently, paclitaxel-resistant cells, established by treatment with increasing concentrations of this drug, exhibited markedly elevated microtubule acetylation and resistance to cell death (Fig. 3), indicating the possible role of α-tubulin acetylation in apoptosis evasion. Since paclitaxel has been reported to stabilize polymerized microtubules, in which tubulins are marked by acetylation30, hyperacetylation of tubulin mediated by long-term treatment with paclitaxel might conversely cause aberrant cell death signaling rather than apoptosis induction31,32.
Accumulating studies have provided evidence that paclitaxel resistance is mediated by the dysregulation of apoptotic signaling pathways, including apoptotic regulatory proteins in the Bcl-2 family33. Upregulation of antiapoptotic Bcl-2, Mcl-1, and Bcl-xL was found in paclitaxel-resistant esophageal cell lines and xenograft tissues34. The restoration of Bcl-2 family proteins, either by suppression of antiapoptotic proteins or by induction of proapoptotic proteins, was shown to confer paclitaxel resistance35,36. Here, we demonstrated that Mcl-1 levels appeared to increase in paclitaxel-resistant lung cancer cells and in the tumor nodules of mice who completed the paclitaxel treatment cycles (Fig. 5c, d). Since tubulin alterations are closely associated with paclitaxel sensitivity, there is less conclusive evidence demonstrating the interplay of microtubules in the regulation of Bcl-2 family proteins. Notably, microtubule filaments play an important role in the intracellular translocation of organelles and molecules, preserving their cargo activities37. Recently, we reported that tubulin acetylation of microtubules maintains Akt activity, and promotes epithelial-to-mesenchymal transition in lung cancer cells12. The trafficking of vesicles containing focal adhesion components to the leading edge of migrating cells requires microtubule acetylation38. In addition, microtubules act as scaffolds for Hsp90, which is necessary for the stimulation of apoptosis and cell proliferation-related targets39. In this study, we underscore the important role of microtubules in regulating the antiapoptotic protein Mcl-1. Overexpression of αTAT1, but not the negative mutant, induced upregulation of tubulin acetylation that led to an increase in Mcl-1 and resistance to paclitaxel-mediated apoptosis (Figs. 4c and 5b), indicating that microtubule acetylation is essential for Mcl-1 expression, facilitating the apoptosis avoidance mechanism of this drug.
It is well known that the ubiquitin–proteasome pathway is a dominant pathway for protein degradation that involves with apoptotic regulatory proteins40. Substrates degraded via this pathway are chemically ubiquitinated prior to binding with and be degraded by the proteasome. A previous study reported that the intracellular level of Mcl-1 was mainly determined by its degradation mechanism through the proteasomal pathway41,42,43. Inhibition of the Mcl-1 degradation process was shown to be related to apoptotic susceptibility to microtubule-targeting drugs44. In the present study, we identified a novel connection between microtubules and Mcl-1 degradation, in which tubulin acetylation functions to stabilize Mcl-1 by protecting it from ubiquitin-mediating proteasomal degradation (Fig. 6d). Increasing of the Ace-tub level with the deacetylase inhibitor TSA strikingly increased Mcl-1 levels by suppressing its degradation (Fig. 6c). Taken together, the present findings provide mechanistic insight regarding the role of microtubule PTMs in apoptosis regulation and highlight the linkage of microtubule acetylation to the stability of antiapoptotic Mcl-1, which has a significant impact on paclitaxel responsiveness (Fig. 7). This study indicated the potential role of tubulin acetylation as a predictive marker for paclitaxel susceptibility and a promising target against drug resistance in cancer.
Materials and methods
Cell culture and chemicals
Non-small-cell lung cancer (NSCLC) H460 and A549 cells were obtained from American Type Culture Collection (ATCC; Manassas, VA, USA). The patient-derived malignant cancer cells (ELC12, ELC16, ELC17, and ELC20) were isolated from pleural effusions of recurrent or advanced stage non-small-cell lung cancer patients who had been diagnosed at the King Chulalongkorn Memorial Hospital. The protocol of conduction was approved by the Ethics Committee of the Faculty of Medicine, Chulalongkorn University, Bangkok, Thailand (IRB 365/62), and was obtained informed consent from all participants. This study was carried out in an accordance with the principles of the World Medical Association Declaration of Helsinki. All cells were maintained in RPMI supplemented with 10% fetal bovine serum, 1% l-glutamine, and 1% penicillin/streptomycin under 37 °C and 5% CO2.
Paclitaxel, 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT), dimethyl sulfoxide (DMSO), Hoechst 33342, and DAPI were purchased from Sigma (St Louis, MO, USA). Paclitaxel Injection USP (Intaxel®) was obtained from Fresenius Kabi Oncology Co., Ltd. (Solan, India). A 0.9% sodium chloride injection was from Thai Nakorn Patana Co., Ltd. (Bangkok, Thailand). The primary antibodies used were anti-Mcl-1 (Cell Signaling Technology #94296), anti-Bcl-2 (Cell Signaling Technology #4223), anti-Bcl-xL (Cell Signaling Technology #2764), anti-GAPDH (Cell Signaling Technology #97166), anti-tubulin (Sigma #T6199), anti-tyrosinated tubulin (Sigma #MAB1864-I), anti-detyrosinated tubulin (Sigma #AB3201), anti-acetylated tubulin (Sigma #T7451), and anti-ubiquitin (Dako #Z0458). The secondary antibodies used were HRP-conjugated anti-rabbit IgG (Cell Signaling Technology #7074) and anti-mouse IgG (Cell Signaling Technology #7076).
Establishment of paclitaxel-resistance cells
Paclitaxel-resistance H460 (H460/PTX) cells were established by a stepwise increment with paclitaxel12. At each step, cells were maintained in a cell culture medium containing paclitaxel for at least two weeks and subcultured every 2 days. The drug concentration was gradually increased two-fold from 12.5 to 800 nM. Cell viability assay was performed to evaluate drug sensitivity, and at least a 100-fold increase of IC50 comparing with control cells was considered as drug-resistant cells.
In vivo xenograft tumorigenesis
A 10 of 6-week-old male BALB/cMlac-nu nude mice were purchased from Nomura Siam International (Bangkok, Thailand). Mice were housed with an environmental enrichment maintaining under stringently hygiene conditions with 24 ± 2 °C temperature-controlled, 40–60% humidity, and a 12:12 h light–dark cycle at the Laboratory Animal Center at Faculty of Pharmaceutical Sciences, Chulalongkorn University. The study was approved by the Institutional Animal Care and Use Committee of the Faculty of Pharmaceutical Sciences, Chulalongkorn University, Bangkok, Thailand (CU-AUP 19-33-003). Both flanks of mice were subcutaneously inoculated with 5 × 106 cells of H460 cells. Mice were weighed, and the tumor volume was observed every 2 days using Vernier caliper as following: (length × width × width)/2. After 7 days, mice were randomly divided into two groups (n = 5), and 10 mg/kg paclitaxel or 0.9% normal saline was intraperitoneal injection every 2 days for five times. After 45 days, mice were euthanized, and the tumors were dissected and stored at −20 °C for further biochemical assays.
Cell viability assay
A number of 104 cells/well were cultured onto a 96-well plate overnight. Cells were treated with paclitaxel for 48 h, and then media was replaced by MTT (5 mg/mL) solution and incubated for 3 h. The formazan product was solubilized by DMSO, and its absorbance was measured at 570 nm by a microplate reader (Perkin Elmer VICTOR3/Wallac 1420). Viable cells were calculated and represented as a percentage of cell viability, by which the control group was considered as 100%. The inhibitory concentration at 50% of cell viability was identified using Prism 8 software (GraphPad).
Apoptosis assay
After treatment with paclitaxel for 48 h, cells were incubated with H33342 (2 μg/mL) at 37 °C for 15 min in the dark. Cells were imaged at least five random field/groups under a fluorescent microscope (Nikon Inverted Microscope Eclipse Ti-U/B, NY, USA). A number of apoptotic cells to total cell number was calculated and presented as percentage of apoptotic cells.
Plasmids and transfections
GFP-tagged-α tubulin acetyltransferase 1 wild-type (αTAT1-wt) and its dominant-negative, D157N plasmids (αTAT1-DN) were gifted from Professor Takeichi Masatoshi (RIKEN Center for Biosystems Dynamic Research, Japan). Plasmid transfection was performed using Lipofectamine® 2000 (Invitrogen, Waltham, MA, USA) according to the manufacturer’s protocol. Briefly, a 2 μg of plasmid in optiMEM media was mixed with 4 μl of Lipofectamine® 2000 and incubated for 15 min at room temperature. The mixture was drooped onto the cells and incubated further at 37 °C for 6 h. Protein overexpression was examined by either western blot analysis or immunofluorescence assay. Cells were subcultured and seeded for other biochemical assays.
siRNA and transfections
αTAT1 knockdown was performed using Lipofectamine® RNAiMAX following the manufacturer’s instruction. Stealth RNAi to αTAT1 and control were purchased from Invitrogen (Invitrogen, Waltham, MA, USA). The sequence of siαTAT1 was 5′-ACCGCACCAACTGGCAATTGA-3. Briefly, 100 nM of stealth RNAi targeting to αTAT1 in OptiMEM (Invitrogen) was incubated with Lipofectamine® RNAiMAX in OptiMEM for 15 min at room temperature. The mixture was dropped wisely added onto the cells and incubated further at 37 °C for 6 h. After transfection for 72 h, cells were subjected to western blot analysis.
Western blot analysis
Cells were lysed with TMEN buffer (20 mM Tris-HCl, pH 7.5; 1 mM MgCl2; 150 mM NaCl; 20 mM NaF; 0.5% sodium deoxycholate; 1% nonidet-40; 0.1 mM phenylmethylsulfonyl fluoride; and cOmpleteTM protease inhibitor cocktail, Roche) on ice for 40 min. The supernatant was collected by centrifugal at 12,000 × g at 4 °C for 20 min. Protein content was measured by BCA Protein Assay Kit (PierceTM, Thermo Fisher Scientific, CA, USA). An equal amount of protein was dissolved in SDS-polyacrylamide gel electrophoresis and transferred to the PVDF membrane. Blots were incubated with 5% skim milk in TBS-T buffer (Tris buffer saline with 0.075% Tween-20) for 30 min at room temperature, specific primary antibody at 4 °C overnight, and correspondent secondary antibody for 2 h at room temperature. An equal of loading was confirmed by GAPDH expression, using anti-GAPDH antibody (Cell Signaling Technology #97166). Protein signals were detected by the chemiluminescence system (Merck Millipore, MA, USA). The relative protein intensity was analyzed and normalized to GAPDH by ImageJ software (NIH).
Immunofluorescence assay
Cells were seeded onto coverslip in a 24-well plate. After indicated treatment, cells were fixed with cold methanol at −20 °C for 5 min and blocked in 3% bovine serum albumin (BSA) at room temperature for 30 min. Cells were incubated with rabbit anti-GFP antibody (1:500, MBL #598), mouse anti-acetylated tubulin (1:2000, Sigma #T7451) or rat anti-α-tubulin (1:2000, Millipore #MAB1864) at 4 °C overnight, washed with PBS followed by incubation with goat AlexaFluor 488-conjugated anti-rabbit (1:500, Invitrogen #A32731), 568-conjugated anti-mouse (1:1000, Invitrogen #A11031) or 647-conjugated anti-rat IgG (1:000, Invitrogen #A21236) for 2 h at room temperature. After washing with PBS containing DAPI, coverslips were washed with deionized water and mounted with FluorSave (EMD Millipore). Images were acquired by fluorescence microscope (Nikon Inverted Microscope Eclipse Ti-U/B, NY, USA). Fluorescence intensity was quantified by ImageJ software (NIH) as described12.
Microtubule sedimentation assay
The interaction of proteins on microtubule was analyzed as described12. Briefly, after indicated treatment, cells were incubated with 1 μM Taxol for 30 min at 37 °C and dissolved in a microtubule-stabilizing buffer containing 80 mM PIPES, 80 mM K-1,4-piperazinediethanesulfonic acid (pH 6.8), 1 mM EGTA, 1 mM MgCl2, 0.5% (vol/vol) nonidet P-40, 20 mM NaF, 0.5% sodium deoxycholate, 10 mM Taxol, 0.1 mM phenylmethylsulfonyl fluoride, and cOmpleteTM protease inhibitor cocktail (Roche) for 5 min at 37 °C in the dark. The microtubule fraction was separated by centrifugal at 18,000 × g for 15 min at 30 °C. The pellet was washed with microtubule-stabilizing buffer without detergent and resuspended with the same buffer in an equal volume of supernatant. Both pellet and supernatant fractions were boiled in a sampling buffer at 95 °C and analyzed by western blot analysis.
Immunoprecipitation assay
Cells were pretreated with proteasomal inhibitor MG132 (10 μM) for 1 h and incubated with 5 μM trichostatin A (TSA) for indicated time points. Cells were then lysed in TMEM lysis buffer for 45 min on ice. The supernatant was collected by centrifuged at 12,000 × g at 4 °C for 20 min, precleared with Protein G-conjugated Sepharose beads (GE Healthcare) at 4 °C for an hour, and incubated with antibody to Mcl-1 or control IgG at 4 °C for overnight. The complex was precipitated by Protein G-conjugated Sepharose beads at 4 °C for an hour and washed with lysis buffer. Precipitates were separated by boiling in sample buffer at 95 °C for 5 min. Polyubiquitination was detected by western blot analysis with antibody to ubiquitin.
Statistical analysis
The data are presented as the mean ± SEM obtained from at least three independent experiments. Statistical analysis was performed using unpaired Student’s t test or Mann–Whitney U test using Prism 8 (GraphPad). P values <0.05 was considered as statistically significant.
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Acknowledgements
We would like to thank Professor Takeichi Masatoshi (RIKEN Center for Biosystems Dynamic Research, Japan) for providing the plasmids.
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V.P. designed the experiments and wrote the paper. O.W., R.T., R.R., and V.P. performed the experiments and analyzed the data. P.C. and C.V. isolated and characterized patient-derived malignant cancer cells. V.P. and O.W. wrote the paper and reviewed all the data. All authors have read and approved the paper.
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This work was supported by the Thailand Research Fund [MRG6280235] to V.P., and the Royal Golden Jubilee Ph.D. Program [PHD/0037/2561] to O.W.
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Wattanathamsan, O., Thararattanobon, R., Rodsiri, R. et al. Tubulin acetylation enhances lung cancer resistance to paclitaxel-induced cell death through Mcl-1 stabilization. Cell Death Discov. 7, 67 (2021). https://doi.org/10.1038/s41420-021-00453-9
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DOI: https://doi.org/10.1038/s41420-021-00453-9
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