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Article

Alisertib Induces Cell Cycle Arrest, Apoptosis, Autophagy and Suppresses EMT in HT29 and Caco-2 Cells

1
Department of Gastrointestinal Surgery, Shunde First People’s Hospital Affiliated to Southern Medical University, Guangdong 528300, China
2
Department of Pharmaceutical Sciences, College of Pharmacy, University of South Florida, 12901 Bruce B. Downs Blvd., MDC 30, Tampa, FL 33612, USA
*
Authors to whom correspondence should be addressed.
Int. J. Mol. Sci. 2016, 17(1), 41; https://0-doi-org.brum.beds.ac.uk/10.3390/ijms17010041
Submission received: 2 November 2015 / Revised: 7 December 2015 / Accepted: 9 December 2015 / Published: 29 December 2015
(This article belongs to the Special Issue Molecular Classification of Human Cancer: Diagnosis and Treatment)

Abstract

:
Colorectal cancer (CRC) is one of the most common malignancies worldwide with substantial mortality and morbidity. Alisertib (ALS) is a selective Aurora kinase A (AURKA) inhibitor with unclear effect and molecular interactome on CRC. This study aimed to evaluate the molecular interactome and anticancer effect of ALS and explore the underlying mechanisms in HT29 and Caco-2 cells. ALS markedly arrested cells in G2/M phase in both cell lines, accompanied by remarkable alterations in the expression level of key cell cycle regulators. ALS induced apoptosis in HT29 and Caco-2 cells through mitochondrial and death receptor pathways. ALS also induced autophagy in HT29 and Caco-2 cells, with the suppression of phosphoinositide 3-kinase (PI3K)/protein kinase B (Akt)/mammalian target of rapamycin (mTOR), but activation of 5′ AMP-activated protein kinase (AMPK) signaling pathways. There was a differential modulating effect of ALS on p38 MAPK signaling pathway in both cell lines. Moreover, induction or inhibition of autophagy modulated basal and ALS-induced apoptosis in both cell lines. ALS potently suppressed epithelial to mesenchymal transition (EMT) in HT29 and Caco-2 cells. Collectively, it suggests that induction of cell cycle arrest, promotion of apoptosis and autophagy, and suppression of EMT involving mitochondrial, death receptor, PI3K/Akt/mTOR, p38 MAPK, and AMPK signaling pathways contribute to the cancer cell killing effect of ALS on CRC cells.

Graphical Abstract

1. Introduction

Colorectal cancer (CRC) is the third most common malignancy in male and the second most common one in female worldwide in 2012 [1]. It was estimated that about 136,830 new cases and 50,310 deaths occurred in US which renders CRC as the third leading cause of cancer related death in 2014 [2]. In China, CRC was the fifth most common cancer and the fifth leading cause of cancer death in 2011 [3]. There were 253,000 new CRC cases, 139,000 CRC deaths, and 583,000 people living with CRC (within 5 years of diagnosis) in 2012 in China [1]. The overall 5-year survival rate is up to 90% in patients with localized CRC [4]; however, it was only 5%–8% in patients with distant metastases in USA [5]. In clinic, there were about 20%–30% of patients who were newly diagnosed with unresectable metastatic disease and 50%–60% patients with CRC will develop metastatic disease, mainly due to the epithelial to mesenchymal transition (EMT) [6]. Therefore, it is of great importance to develop new therapeutics for CRC treatment, in particular, the distant metastatic CRC.
In addition to the primary surgical resection, the current systemic chemotherapies for CRC, including FOLFIRI (5-fluorouracil, leucovorin and irinotecan) and FOLFOX (5-fluorouracil, leucovorin and oxaliplatin) are the cornerstone of treatment for metastatic CRC patients. The advent of targeted agents (e.g., the anti-vascular endothelial growth factor monoclonal antibody bevacizumab or the anti-epidermal growth factor receptor monoclonal antibodies cetuximab and panitumumab) were recognized as a landmark advance in the treatment of metastatic CRC. However, in many patients, all of the above schemes lead to a poor outcome due to the drug-related adverse events and drug resistance [7]. Thus, it is of clinical importance to identify more effective biological agents with specific therapeutic targets and reduced side effect.
There were three members of Aurora kinases (Aurora A, B, and C) that are affiliated to a family of serine/threonine kinases in mammals, and Aurora kinases have emerged as crucial mitotic regulators required for genome stability [8]. The Aurora kinases regulate multiple aspects of mitosis, including centrosome duplication, spindle assembly, chromosome alignment, chromosome segregation and the fidelity-monitoring spindle checkpoint [9]. Aurora kinase A (AURKA) localizes to duplicated centrosomes and spindle poles, with key functions of centrosomes maturation, timing of mitotic entry and construction and control of a bipolar spindle. Aberrant mRNA or protein expression of AURKA causes abnormalities in mitosis (e.g., aneuploidy, supernumerary centrosomes, and defective mitotic spindles) and induces resistance to apoptosis. In clinic, amplification or overexpression of AURKA was observed in many solid cancers, such as ovarian, gastric, pancreatic, and breast cancers [10]. Also, the abnormal condition of AURKA has been frequently investigated in CRC and is associated with poor prognosis and response to chemotherapy [11,12]. The expression of AURKA protein is higher in CRC liver metastasis than the corresponding primary tumor, which can be recognized as a molecular biomarker with prognostic value for patients with CRC liver metastasis, independent of established clinicopathological variables [13]. It was also suggested that AURKA was essential for CRC stem cells regeneration and resistance to cytotoxic stimuli in CRC [14].
Given the specific localization and function in cells and pathological activation of AURKA in many malignant diseases, AURKA have been an attractive target for the development of new therapeutic approaches for cancer treatment. Numerous compounds of AURKA inhibitor have undergone preclinical testing into Phase I or II trials, including AMG900, AT9283, MLN8237, AZD1152, and ENMD2076 [15]. MLN8237, also known as alisertib (ALS, Figure S1A), is one of secondary generation AURKA inhibitors. In vitro, ALS has displayed its effects on inhibition of proliferation and cell cycle progression in glioblastoma neurosphere tumor, malignant bladder cancer, pancreatic cancer, ovarian cancer, breast cancer, osteosarcoma, gastric cancer, and esophageal adenocarcinoma cell lines [16,17,18,19,20,21,22]. The anticancer effect of ALS was also examined in vivo in multiple myeloma and acute lymphoblastic leukemia xenograft models [23]. Implanted tumors shrunk considerably in multiple myeloma models and the overall survival or disease-free survival was significantly improved in animal models.
However, the role of AURKA in the tumorigenesis and development of CRC and the underlying mechanism have not been fully elucidated, which renders the anticancer effect and molecular mechanisms of ALS in the treatment of CRC remain unclear. In this study, we aimed to unveil the molecular targets, examine the cancer cell killing effect of ALS and elucidate the molecular mechanism for its anticancer effect, with a focus on the cell proliferation, cell cycle distribution, programmed cell death, and EMT in human CRC cell lines HT29 and Caco-2 cells.

2. Results

2.1. Alisertib (ALS) Inhibits the Proliferation of HT29 and Caco-2 Cells

We first examined the effect of ALS on the viability of HT29 and Caco-2 cells using 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay. Treatment of both cell lines with ALS at concentrations ranging from 0.1 to 100 μM for 24 or 48 h significantly decreased the viability (Figure S1B,C). Compared with the control cells, the viability of HT29 cells was decreased from 78.5% to 47.3% when exposed to ALS for 24 h and declined from 71.0% to 31.2% when treated with ALS for 48 h at concentrations from 0.1 to 100 μM, respectively (Figure S1B). The IC50 values were 49.31 and 17.86 μM for HT29 cells after 24 and 48 h incubation with ALS, respectively. As shown in Figure S1C, the percentage of the viability of Caco-2 cells was decreased from 89.7% to 45.7% when treated with ALS for 24 h and declined from 100.3% to 18.8% when incubated with ALS for 48 h at concentrations from 0.1 to 100 μM, respectively. The IC50 values were 88.8 and 52.1 μM for Caco-2 cells after 24 and 48 h incubation with ALS, respectively. These results suggest that ALS inhibits the cell proliferation in concentration- and time-dependent manners and displays a potent inhibitory effect on the growth of HT29 and Caco-2 cells.

2.2. Overview of Proteomic Response to ALS Treatment in HT29 and Caco-2 Cells

Following, we performed a stable isotope labeling by amino acids in cell culture (SILAC)-based proteomic study to quantitatively determine the molecular interactome in HT-29 and Caco-2 cells responding to ALS. There were 893 and 582 protein molecules identified as the potential targets of ALS in HT-29 (Table 1) and Caco-2 cells (Table 2), respectively. ALS increased the expression level of 459 protein molecules, while decreasing the expression level of 434 protein molecules in HT-29 cells. In Caco-2 cells, ALS increased the expression level of 207 protein molecules, but decreased the expression level of 375 protein molecules. Subsequently, these proteins were subject to IPA pathway and network analysis. There were 24 and 25 networks of signaling pathway and cellular function that were potentially regulated by ALS in HT-29 and Caco-2 cells, respectively. These included a number of molecules involved in cell proliferation, metabolism, migration, invasion, survival, and death (Table 1 and Table 2). As such, the following experiments were performed to validate the effect of ALS in HT-29 and Caco-2 cells, with a focus on cell cycle distribution, programmed cell death, and EMT.
Table 1. Molecules and networks were regulated by alisertib (ALS) in HT-29 cells.
Table 1. Molecules and networks were regulated by alisertib (ALS) in HT-29 cells.
IDMolecules in NetworkScoreFocus MoleculesTop Diseases and Functions
160S ribosomal ubunit, DDX1, DDX5, DDX17, DDX21, DDX3X, DHX9, EIF3E, HDGF, HNRNPU, ILF2, ILF3, KPNA6, LYAR, MTDH, NEDD8, RAD23B, RBM39, Rnr, RPL3, RPL5, RPL8, RPL9, RPL10, RPL14, RPL18, RPL24, RPL28, RPL30, RPL27A, RPLP0, RPS2, RPS15A, Vegf, XRCC55232Protein synthesis, infectious disease, gene expression
2AHSA1, ALYREF, CAND1, ERK1/2, FUBP1, GIGYF2, HNRNPK, HNRNPL, LARS, LOC102724594/U2AF1, MARS, NOLC1, NOP56, NOP58, OLA1, PABPC1, PCBP1, PCBP2, PDE6H, Pki, PTBP1, PUF60, QARS, RALY, RNA polymerase I, SF3B1, SF3B2, Srp30, SRSF1, SRSF2, SRSF3, Tap, TOP1, U2af, U2AF24429RNA post-transcriptional modification, protein synthesis, cancer
3CALU, CLIC4, creatine kinase, CUTA, EFTUD2, FUS, Histone H1, HNRNPC, HNRNPD, HNRNPF, HNRNPH1, HNRNPM, HNRNPUL1, Importin α, Importin β, IPO5, IPO7, P38 MAPK, PQBP1, PRMT1, PRMT5, PRPF19, PTMA, PYCR1, RAN, RANBP1, SF3B4, snRNP, SNRPD3, SYNC, TNPO1, Transportin, TRAP/Media, UBA2, WDR14027RNA post-transcriptional modification, amino acid metabolism, post-translational modification
4AGR2, Akt, ANXA4, Calcineurin A, CALR, Collagen α1, Collagen type VI, COP I, COPA, COPB1, COPG1, Cytoplasmic Dynein, DSTN, DYNC1LI2, FKBP4, Mre11, PA2G4, PDIA3, PDIA4, PDIA6, peptidylprolyl isomerase, peroxidase (miscellaneous), PPIA, PPIB, PPT1, PRDX1, PRDX2, PRDX4, PRDX5, PRDX6, RRBP1, SAE1, TMED9, TXNDC5, ZYX3826Cancer, endocrine system disorders, organismal injury and abnormalities
5ACTN1, ACTN4, ANP32B, ASPH, ATP synthase, C1QBP, CAMK2D, CaMKII, COX5A, CSRP1, CTNNA1, Cytochrome bc1, cytochrome C, ERP44, Filamin, ITPR, KLK3, LONP1, MAP4, Mitochondrial complex 1, MRPL12, MT-CO1, MT-CO2, MT-CYB, NDUFA5, Pde, PDS5A, PDXDC1, PHB, PHB2, Pka, PPP2R1A, PRDX3, PYGB, STMN13826Drug metabolism, lipid metabolism, small molecule biochemistry
619S proteasome, 20s proteasome, ADRM1, BUB3, COTL1, CPNE1, DAD1, FLII, Immunoproteasome Pa28/20s, MHC CLASS I (family), NFkB (complex), OTUB1, Proteasome PA700/20s, PSMA, PSMA4, PSMA7, PSMB5, PSMC2, PSMD, PSMD2, PSMD6, PSMD8, PSMD14, PSME1, PSME2, RNF13, S100, S100A2, S100P, UBA1, UBE2, UBE2L3, UBE2N, USMG5, USP143525Cellular movement, protein degradation, protein synthesis
7adenosine-tetraphosphatase, α tubulin, ATP5H, ATP5J, ATP5J2, β Tubulin, BZW1, BZW2, CCT4, CCT5, CCT8, CCT6A, DCTN1, Dynein, Ephb, ERP29, F0 ATP synthase, FAM162A, H2AFV, KDELR, LGALS3BP, MAPK1, OGFR, PGAM1, SAR1A, Sec23, TBCA, TSPO, TUBA4A, TUBB6, tubulin (family), VBP1, Vdac, VDAC1, VDAC23525Cellular assembly and organization, cell-to-cell signaling and interaction, reproductive system development and function
8CD9, chymotrypsin, CTSH, EIF1, EIF3, EIF3A, EIF3B, EIF3F, EIF3G, EIF3J, EIF3L, EIF4B, Eif4g, Erm, EZR, G6PD, GLRX3, GPIIB-IIIA, IPO9, Lamin b, LBR, Lh, PEBP1, Pkc(s), Pkg, PLCB3, PLIN3, PSIP1, RAB1A, RBM3, Rho gdi, SERPINB1, SLC12A2, TLN1, VAT13525Gene expression, protein synthesis, cellular growth and proliferation
9ABCB8, Aconitase, Adaptor protein 1, Aldose Reductase, Angiotensin II receptor type 1, AP1B1, Arf, ARF1, ARF4, ARF5, ARL1, COPB2, CRIP2, cytochrome-c oxidase, DAB2IP, DHCR24, Gef, glutathione peroxidase, glutathione transferase, GST, GSTK1, GSTO1, GSTP1, Jnk, MGST1, PARK7, RAB1B, RPN2, SFXN1, SLC25A3, SLC25A11, SOD2, SRP54, SSR3, USO13324Drug metabolism, protein synthesis, DNA replication, recombination, and repair
10ABCC1, AK2, ALDH2, ANXA3, ATPase, atypical protein kinase C, CAPG, Caveolin, CLTA, DBNL, DNPEP, Dynamin, ETFA, ETFB, GANAB, IL-2R, Integrin α 3 β 1, MTCH2, NSF, NUDC, OSBP, PAK2, PCMT1, PHGDH, PI3K (complex), Ptk, Raf, RAP1B, SEPT11, SHMT2, SLC3A2, TPP2, trypsin, VAPA, Vla-43324Developmental disorder, hereditary disorder, metabolic disease
11ALDOA, AP2B1, C11orf54, CAD, CBX3, CYP, DHCR7, DPP3, Focal adhesion kinase, GGCT, Histone h4, HMGCS1, IDI1, Ldh (complex), LDHA, LDHB, MAT2A, NPC2, NQO1, PI3K (family), POR, Rar, RBBP4, RBP2, RPN1, Rxr, SLC16A1, Sod, Sos, STAT5a/b, TGM2, thymidine kinase, TPP1, TXNRD1, UGDH3324DNA replication, recombination, and repair, energy production, nucleic acid metabolism
12ACAA1, APEX1, BTF3, BTF3L4, Cbp/p300, CPSF6, Cyclin A, Cyclin D, Cyclin E, E2f, EDF1, EEF2, EPCAM, FEN1, Hat, HAT1, Holo RNA polymerase II, HSD17B4, Ku, Mcm, MCM3, MCM7, MTHFD1, NASP, NONO, PCNA, POLβ-POLepsilon-POLγ-XRCC1-LIGI-PARP1-PCNA-FEN1, POLR2H, PRKDC, RAD50, Ras, Rb, SSRP1, TIP60, XRCC62922DNA replication, recombination, and repair, cellular response to therapeutics, cell morphology
13ANXA5, BCR (complex), CAPZA2, CAPZB, caspase, CDC37, DENR, EIF4G1, FAS, FLNA, FLNB, Hsp27, HSPB1, IFIH1, JINK1/2, Lamin, LMNB1, MAP2K1/2, MCTS1, Mlc, MTORC2, MTPN, Pak, PARP, PARP1, PDCD6, PLEC, PP2A, PYGL, RHOA, Rsk, RTN3, RTN4, Sapk, SRP722922Cellular compromise, cell morphology, cellular movement
14ACTG1, ATP5C1, Calmodulin, Caspase 3/7, CD3, CD44, CSTF2, DDX19A, ECH1, EEF1D, Eif2, HNRNPR, HSPA5, Ifn γ, LMNA, MYH9, PGK1, PPM1G, Proinsulin, RAB10, RAB8A, Ribosomal 40s subunit, RPS7, RPS24, RPS3A, RPSA, Secretase γ, SRPRB, TCF, TCR, Tgf β, TSTA3, TUBB, tubulin (complex), tyrosine kinase2922Hematological disease, immunological disease, inflammatory disease
1526s Proteasome, AMPK, CD59, CS, CTBP1, CTBP2, DDB1, GFPT1, HDL, hemoglobin, HISTONE, Hsp70, Hsp90, HUWE1, IDH3A, IL1, LMAN1, MIF, NADPH oxidase, Nos, NSUN2, PRKAA, Pro-inflammatory Cytokine, PTGES3, Ras homolog, SDHA, SGTA, SSBP1, succinate dehydrogenase, SURF4, TMED2, TRAP1, Ubiquitin, UBXN1, UCHL32520Cellular assembly and organization, cellular function and maintenance, cellular development
16ABCE1, ACLY, Ap1, ATP1A1, Calcineurin protein(s), CK1, Ck2, Gsk3, HMBS, HMGA1, HMGB1, HMGB2, HMGB3, HNRNPAB, MEF2, Mek, MVP, NAP1L1, NFAT (complex), Nfat (family), NMDA Receptor, NUDT5, p70 S6k, PDAP1, Pdgf (complex), phosphatase, PICALM, PP1 protein complex group, PP1-C, PPP1R7, Ppp2c, STARD10, TECR, WARS, XPO12419DNA replication, recombination, and repair, gene expression, nucleic acid metabolism
17ACTB, Actin, ACTR2, aldo, α actin, α Actinin, α catenin, API5, Arp2/3, ARPC2, ARPC3, Cadherin, CAP1, CLIC1, CNN2, Cofilin, DIAPH1, DPYSL2, ERK, F Actin, FCGR1A/2A/3A, G-Actin, GOT1, LASP1, LTA4H, MYH14, Profilin, Rock, Talin, TPM3, TPM4, Tropomyosin, Troponin t, TWF1, VASP2218Cellular assembly and organization, cellular function and maintenance, cell morphology
18Adaptor protein 2, AHR, AKR1A1, APP, ATIC, BIN3, BOLA2/BOLA2B, C11orf54, C14orf93, Clathrin, CORO1C, CPN2, CUL3, DDX55, DNAAF2, ERH, EWSR1, FAM98B, GCSH, HEATR5A, MYC, NLE1, NUDT21, OARD1, OLFML2A, PAICS, RAB7A, SLC25A1, SRSF10, TKT, TMEM183A, TPGS2, UBC, UBL4A, UGT1A9 (includes others)2219Cell cycle, hepatic system development and function, cell morphology
19ACY1, APMAP, APRT, BBS7, BCKDK, C21orf33/LOC102724023, CARHSP1, CLN5, CMPK1, CNN3, CNPY2, CRYZ, CS, EFHD2, FAM98B, GLS, IARS2, KIF20A, MARCH8, MDH1, MTAP, MYLIP, NME3, NME4, NME7, PADI2, PGM3, RAB6B, RABGAP1, RASA4, REXO4, SCT, SLC25A22, TTC1, UBC2020Nucleic acid metabolism, small molecule biochemistry, cell-to-cell signaling and interaction
20ACSL3, ADCY, ADRB, Alp, ANP32E, ANXA2, Creb, CTNNB1, DPY30, estrogen receptor, G protein, G protein α, G protein β γ, GTPase, Hdac, Histone h3, HSPA9, Insulin, MATR3, Mmp, NOMO1 (includes others), p85 (pik3r), Pdgfr, PLC, PMM2, RCC2, RNA polymerase II, SFPQ, Shc, SRC (family), STIP1, SUMO2, TOP2A, WDR12, WDR361816Cell cycle, hair and skin development and function, cancer
21APPBP2, ARIH2, ARL4D, CD70, CDV3, COQ6, EDNRA, ELF4, EML4, GALE, GMDS, H32, HKDC1, ISOC2, KIF6, LSM8, MAGEA11, NME4, NME1-NME2, NUP210L, OARD1, PCSK5, PODXL, RBM47, RRS1, SCFD1, SELL, SYT11, TBL3, TCIRG1, TNKS, TRMT1, UBC, YBX2, ZCCHC121515Cell-to-cell signaling and interaction, hematological system development and function, immune cell trafficking
22AAMP, ANXA1, calpain, Casein, Collagen type I, Collagen type III, Collagen type IV, Collagen(s), COMT, Cpla2, DDAH1, Fc γ receptor, Fibrin, Fibrinogen, GADD45, Growth hormone, Integrin, Laminin, LAMP1, LDL, Mac1, Mapk, MCFD2, NAMPT, PDGF BB, PLCE1, Pld, Rap1, SEC13, SERPINH1, SLIRP, SYK, thyroid hormone receptor, TSH, VAV1212Lipid metabolism, molecular transport, small molecule biochemistry
23AChR, ALDOC, FABP5, Fcer1, Gm-csf, GOT, HINT1, HLA-DR, HSP, Ifn, IFN β, Ige, IgG, IgG1, IgG2a, Igm, Ikb, Ikk (family), IL12 (complex), IL12 (family), Immunoglobulin, Interferon α, mediator, MHC Class I (complex), MHC Class II (complex), NACA, NPEPPS, OGDH, PI3K p85, PLA2, PLC γ, PRKRA, Rac, Tlr, TXLNA78Cancer, hematological disease, immunological disease
24ACPP, ACTR2, ARHGAP1, CBR1, CBR3, CDC42, CDC42EP4, Cg, chemokine, CLDN11, COL15A1, collagen, DHCR7, Endothelin, EPHA3, FCGR1A/2A/3A, FSH, GNRH, GNRH2, GNRHR, HSD3B1, Hsd3b4 (includes others), IKK (complex), LIMK2, Metalloprotease, MTORC1, MYO5B, NPC1L1, PAPPA, PEPD, PHKA2, RAB11A, Tnf (family), TNFRSF6B, UCN248Endocrine system development and function, lipid metabolism, small molecule biochemistry
Table 2. Molecules and networks were regulated by ALS in Caco-2 cell.
Table 2. Molecules and networks were regulated by ALS in Caco-2 cell.
IDMolecules in NetworkScoreFocus MoleculesTop Diseases and Functions
160S ribosomal subunit, AARS, AHSA1, AIMP1, C11orf58, DARS, EEF1A1, EEF1B2, EEF1D, EEF1G, EPRS, ERK1/2, GARS, HARS, KARS, MARS, OLA1, PDE6H, PDGF (family), Pki, QARS, RPL8, RPL10, RPL18, RPL21, RPL23, RPL27, RPL30, RPL32, RPL10A, RPL13A, RPLP0, RPLP1, RPS3A, VARS4831Protein synthesis, gene expression, RNA post-transcriptional modification
2ANXA3, APEX1, BTF3, Cbp/p300, CDH17, CTNNB1, CYB5R3, ESD, FEN1, GANAB, GOLPH3, GST, GSTO1, HDLBP, HIST2H2AC, Holo RNA polymerase II, LMNA, NACA, OAT, PCNA, PGAM1, PRKCSH, PRKDC, RUVBL1, SERBP1, SLC38A2, SSRP1, SUPT16H, TAGLN2, TCF/LEF, thymidine kinase, TMPO, XRCC5, XRCC6, YBX34530DNA replication, recombination, and repair, cellular response to therapeutics, cell morphology
3DDOST, DDX17, FUBP1, FUS, hnRNP H, HNRNPA1, HNRNPDL, HNRNPF, HNRNPH1, HNRNPK, HNRNPL, HNRNPR, HNRNPU, IGF2BP3, Karyopherin β, KHSRP, Mapk, MATR3, NONO, PCBP1, PCBP2, PDGF-AA, PSPC1, PTBP1, PUF60, RAN, RAN-GTP, RANGAP1, RBM14, SF3A3, SFPQ, SYNCRIP, TNPO1, Transportin, YBX14329RNA post-transcriptional modification, protein synthesis, DNA replication, recombination, and repair
414-3-3 (β, ε, ζ), CALU, CAPZA1, CAPZB, caspase, CLTC, DLAT, FLNA, GNB2L1, HMBS, HNRNPM, Hsp27, Hsp90, HSP90AA1, HSP90AB1, HSPA8, NCL, NPM1, NUDT21, NUMA1, p85 (pik3r), PCMT1, PKM, PLEC, RPL12, RPL22, SFMBT2, SPTBN1, TRIM28, tubulin (complex), UBXN1, VPS35, YWHAB, YWHAE, YWHAH4329Cancer, gastrointestinal disease, hepatic system disease
514-3-3(β, γ, θ, η, ζ), AChR, ACTR3, ALDOC, ALYREF, ATP5A1, Calmodulin, DDX39B, DYNC1H1, EPCAM, F1 ATPase, FABP5, GTPase, IARS2, IMMT, IQGAP1, KIF5B, LRPPRC, MARCKS, mediator, MYH9, Pde, RPL3, RPL4, RPL7, RPLP2, RTN4, SARNP, SLC25A3, TPD52L2, TPI1, TUFM, YWHAG, YWHAQ, ZFC3H14028Metabolic disease, molecular transport, RNA trafficking
614-3-3(η, θ, ζ), Cytokeratin, DSP, EIF3, EIF2S2, EIF3A, EIF3B, EIF3C, EIF3E, EIF3F, EIF3I, EIF3M, EIF4A, EIF4A1, EIF4A3, EIF4B, EIF4F, Eif4g, EIF4G1, EIF4G2, EIF4H, GPI, KRT1, KRT2, KRT8, KRT9, KRT14, KRT18, KRT19, p70 S6k, PABPC1, PI3K (complex), PKP2, PNN, YWHAZ3827Gene expression, protein synthesis, cellular assembly and organization
73-hydroxyacyl-CoA dehydrogenase, ACAA1, ACAA2, ACAT1, ACAT2, acetyl-CoA C-acetyltransferase, acetyl-CoA C-acyltransferase, CD99, CNBP, DDX21, DHX9, EDC4, FBL, GLUD1, GSR, H2AFY, HADH, HADHA, HDGF, HNRNPA3, HSD17B10, LOC102724594/U2AF1, NFkB (complex), OTUB1, PDLIM1, peptidase, PPARα-RXRα, RBM39, RCC2, SRSF1, Tap, TOP1, U2af, U2AF2, UBE23626Renal damage, renal tubule injury, endocrine system development and function
8Adaptor protein 1, α tubulin, Ap1 γ, AP1B1, AP1G1, β Tubulin, CCT4, CCT5, CCT8, CCT6A, CNN3, CS, DPYSL2, Dynein, EHD1, ERP29, ETFB, FH, Integrin α 5 β 1, LCP1, malate dehydrogenase, MAPK1, MDH1, MDH2, TKT, TUBA1B, TUBB6, TUBB8, TUBB2B, TUBB4B, tubulin (family), Vdac, VDAC1, VDAC2, WARS3626Cancer, hematological disease, immunological disease
9adenosine-tetraphosphatase, ATP synthase, ATP5B, ATP5H, collagen, Collagen α1, Collagen type III, Cytoplasmic Dynein, DCTN2, DHX15, EFTUD2, FKBP4, HNMT, HNRNPA2B1, MAPRE1, P38 MAPK, PA2G4, peroxidase (miscellaneous), PGK1, PPIA, PRDX1, PRDX2, PRDX6, PRPF8, PRPF19, RRBP1, SERPINH1, SF3B1, SF3B2, SND1, snRNP, SNRPD1, STIP1, TARS, VIL13626RNA post-transcriptional modification, free radical scavenging, small molecule biochemistry
10ACLY, ALDH1A1, ANXA5, CK1, CYB5B, DHCR7, DNAJA2, ECHS1, FASN, Focal adhesion kinase, HMGCS1, HSP, Hsp70, HSPA4, HSPA9, HSPB1, HSPE1, HSPH1, IDI1, JINK1/2, MHC Class II (complex), PGD, Pias, POR, PPA1, PSAP, SLC25A6, Srebp, ST13, TOMM22, TOMM40, UBA1, UBE2L3, Ubiquitin, UGDH3626Cell cycle, endocrine system development and function, lipid metabolism
11ADK, Akt, ARHGDIA, atypical protein kinase C, CADM1, CAPRIN1, CPNE1, EEF2, Fascin, GDI2, HN1, ILF2, ILF3, LRRC47, Mcm, MCM2, MCM3, MCM4, MCM6, N-Cadherin, Pak, PLIN3, PPP2R1B, Rab5, Rab11, RAB11A, RAB2A, RAB7A, RDX, Rho gdi, RNH1, RPA, SEC13, TWF2, VAT13425DNA replication, recombination, and repair, cell signaling, post-translational modification
12ADH5, API5, Arp2/3, ARPC2, ARPC5, CLIC1, CNN2, DDX1, Eif2, ERK, GPIIB-IIIA, HNRNPH3, IGF2BP1, Ku, LAMB1, Laminin1, LAP3, Profilin, Ribosomal 40s subunit, Rnr, RPS2, RPS7, RPS8, RPS10, RPS12, RPS14, RPS15, RPS24, RPS27A, RPS4X, RPSA, RTCB, Talin, TLN1, VCL3425Developmental disorder, hematological disease, hereditary disorder
13Arf, ARF1, ARHGAP1, B2M, B2m-Mhc1a, CALR, CANX, CCAR2, CCDC47, Cd1, CD1D-CANX-CALR-ERp57, COP I, COPA, COPB1, COPE, COPG1, DNAJ, DNAJA1, DNAJC8, HLA-B27, Hsp22/Hsp40/Hsp90, HSP90B1, HSPA5, HYOU1, Jnk, LMAN1, MHC Class I (complex), P4HB, PDIA3, PDIA4, PDIA6, PRDX4, RAB1B, RPN1, TXNDC53425Post-translational modification, protein folding, developmental disorder
14ACO2, Aconitase, AHCY, AKR1C3, AKR1C1/AKR1C2, Aldose Reductase, CACYBP, chymotrypsin, COMT, ENO1, ERP44, ETF1, Filamin, FLNB, FLNC, G6PD, GADD45, GCN1L1, glutathione peroxidase, Lamin b, LONP1, LRRC59, ME1, N-cor, PARK7, PEBP1, PFKP, Pkc(s), PTGES3, Rar, RPL7A, SEPT2, T3-TR-RXR, TALDO1, thyroid hormone receptor3023Nucleic acid metabolism, small molecule biochemistry, cellular movement
1514-3-3, APC/APC2, ATIC, CBX3, CHD4, CLIC4, CSE1L, GART, H3F3A/H3F3B, HIST1H1C, Histone H1, Histone h3, Histone h4, IDH1, IL-2R, Importin α, Importin β, IPO5, IPO7, KPNA2, KPNA3, KPNB1, Mucin, NuRD, NUTF2, PAICS, PHGDH, PTMA, RANBP1, SAE1, SNRPD3, SSB, TIP60, Vegf, WDR13023Molecular transport, protein trafficking, amino acid metabolism
16ACTA1, ACTG1, Actin, ACTN4, ACTR2, aldo, α actin, α Actinin, BASP1, Cadherin, CAP1, CFL1, CFL2, CKB, Cofilin, CORO1C, COTL1, DBN1, F Actin, G-Actin, LMO7, MYH10, MYL12A, Myosin2, NAPA, NWASP, PAFAH1B2, PDCD6IP, Pka, PLS3, TMOD3, TPM3, TPM4, Tropomyosin, TWF13023Cellular assembly and organization, cellular function and maintenance, developmental disorder
1719S proteasome, 20s proteasome, 26s Proteasome, ATP5C1, ATPase, CCT3, CCT7, Cyclin E, Immunoproteasome Pa28/20s, LRP, MHC CLASS I (family), NSFL1C, Proteasome PA700/20s, PSMA, PSMA1, PSMA2, PSMA4, PSMA7, PSMB1, PSMC4, PSMD, PSMD1, PSMD2, PSMD3, PSME1, PSME2, Rac, SLC3A2, SOD1, SQSTM1, TUBB, UBE2N, USP5, VAPA, VCP3023Developmental disorder, hereditary disorder, inflammatory disease
18ACTN1, α catenin, ANXA2, ATP6V1A, C1QBP, CAPNS1, Caveolin, CDHE/CDHN, CSRP1, CTNNA1, CTNND1, CTNNα-CTNNβ-CTNNδ, CYC1, Cyclin B, Cytochrome bc1, cytochrome C, cytochrome-c oxidase, DNM1L, Dynamin, EPPK1, ETFA, HSPD1, Il8r, JUP, MDK, Mitochondrial complex 1, PARP, PHB, PHB2, PRDX3, Ras homolog, SPTAN1, STOML2, UQCRC1, ZYX2822Cellular movement, cell morphology, cellular function and maintenance
19ALDOA, AP2B1, APOA1, ATP2A2, calpain, CAPN1, CAPN2, Casein, creatine kinase, DBI, DPP3, Fibrinogen, GC, Growth hormone, HBD, HDL, hemoglobin, HIST1H2BL, Ldh (complex), LDHA, LDHB, LDL, NAMPT, Nos, Nr1h, PF4, Pro-inflammatory Cytokine, QDPR, SAA, SERPINA1, Sod, SRC (family), TFRC, TGM2, VLDL-cholesterol2219Cellular function and maintenance, carbohydrate metabolism, free radical scavenging
20Alp, APLP2, BCAT1, CDH1, Collagen type I, Collagen type IV, Collagen(s), CTSB, CTTN, elastase, F11R, Fgf, Fgfr, Fibrin, FN1, GLG1, GOT, GOT1, GOT2, GPD2, Integrin, Laminin, LMNB1, MAT2A, Mmp, Notch, PDGF BB, Rap1, RPN2, Secretase γ, SERPINA3, SERPINB1, TAGLN, Tgf β, trypsin1917Amino acid metabolism, small molecule biochemistry, dermatological diseases and conditions
21ACTL8, AGPAT2, ANP32E, BROX, CDV3, CEP78, CHMP6, CHMP7, CHMP1B, CHMP2A, CHMP4A, CHMP4B, CMPK1, GMPS, HEBP1, HIST1H2AE, HSDL2, NAP1L2, NAP1L4, NARS, NME3, NME4, NME7, NME1-NME2, NPM3, PNPO, QPRT, RNPEP, TCEAL1, TSN, TTLL4, TUBAL3, UBC, USP54, ZBTB181716Infectious disease, cell morphology, cellular assembly and organization
22ATP1A1, ATP6V1B2, Calcineurin A, CCT2, Ck2, Dishevelled, EIF2S1, EIF5A, Gsk3, ITPR, MAP2K1/2, MIR124, Mlc, Pdgf (complex), PFN1, phosphatase, PICALM, Pkg, PP1 protein complex group, PP1-C, PP1/PP2A, PP2A, PPP1CA, Ppp2c, PPP2R4, PPP2R1A, PRKAA, Rb, RCN1, Rock, SET, SHMT2, Spectrin, STARD10, XPO11615Molecular transport, RNA trafficking, hereditary disorder
23ACKR1, ACSL3, AFP, ALDH18A1, AP4S1, APLNR, CCND1, CKAP4, DPY30, E2f, EMR2, EMR3, ENOPH1, FPR3, FSD1, γ tubulin, Gpcr, GPR15, GPR35, GPR137B, GPRC5C, Metalloprotease, MFSD1, miR-491-5p (and other miRNAs w/seed GUGGGGA), NAP1L1, NDC1, NUP155, PXN, RAB10, RXFP2, SSR4, STAT, STX2, TTLL4, UBC910Cell-to-cell signaling and interaction, cellular assembly and organization, cellular compromise
24AHNAK, BCR (complex), Complement component 1, CXADR, DDX6, ENaC, EZR, Fcer1, GTF2I, HINT1, HLA-DR, Iga, Ige, IgG1, Igg3, Igm, Ikb, IMPDH2, JAK, KHDRBS1, MEF2, MIRLET7, NFAT (complex), Nfat (family), NFkB (family), PI3K (family), PI3K p85, PLC γ, Ptk, Raf, Ras, Rsk, Sapk, SYK/ZAP, TEC79Cancer, organismal injury and abnormalities, infectious disease
25Adaptor protein 2, ADCY, ADRB, Ap1, BSG, Calcineurin protein(s), CaMKII, CDK1, Cg, Clathrin, Creb, DDX5, estrogen receptor, FSH, G protein, GFPT1, GML, GSTP1, IKK (complex), Insulin, Lh, MCTS1, MTORC1, NADPH oxidase, NMDA Receptor, Pdgfr, Pka catalytic subunit, PLC, Proinsulin, RNA polymerase II, Shc, SKP1, Sos, TCF, UCHL179Neurological disease, psychological disorders, skeletal and muscular disorders

2.3. ALS Decreases the Phosphorylation Level of Aurora Kinase A (AURKA) in HT29 and Caco-2 Cells

To determine whether ALS effectively targeted AURKA and affected cellular mitosis, we first examined the phosphorylation level of AURKA and the total expression level of AURKA after HT29 and Caco-2 cells were treated with ALS at 0.1, 1, and 5 μM for 48 h. Intriguingly, there were variable alterations in the phosphorylation and expression level of AURKA in these two cell lines when exposed to ALS (Figure 1A,B). In HT29 cells, the phosphorylation level of AURKA was decreased 54.4% and 93.7% when treated with ALS at 1 and 5 μM for 48 h, respectively (p < 0.001; Figure 1A,B). However, there was no significant difference in the expression level of AURKA (p > 0.05). Consequently, it led to a 66.4% and 93% reduction in the ratio of p-AURKA/AURKA when HT29 cells were treated with ALS 1 and 5 μM for 48 h, respectively, (p < 0.05; Figure 1A,B).
Figure 1. Alisertib (ALS) inhibits the phosphorylation of Aurora kinase A (AURKA) in HT29 and Caco-2 cells. HT29 and Caco-2 cells were exposed to ALS at 0.1, 1, and 5 μM for 48 h and protein samples were subject to Western blotting assay. (A) Representative blots of p-AURKA and total AURKA examined by Western blotting assay; (B) Bar graphs showing the level of p-AURKA and AURKA in HT29 and Caco-2 cells. β-Actin was used as the internal control. Data are shown as the mean ± SD of three independent experiments. * p < 0.05 and ** p < 0.01 by one-way analysis of variance (ANOVA).
Figure 1. Alisertib (ALS) inhibits the phosphorylation of Aurora kinase A (AURKA) in HT29 and Caco-2 cells. HT29 and Caco-2 cells were exposed to ALS at 0.1, 1, and 5 μM for 48 h and protein samples were subject to Western blotting assay. (A) Representative blots of p-AURKA and total AURKA examined by Western blotting assay; (B) Bar graphs showing the level of p-AURKA and AURKA in HT29 and Caco-2 cells. β-Actin was used as the internal control. Data are shown as the mean ± SD of three independent experiments. * p < 0.05 and ** p < 0.01 by one-way analysis of variance (ANOVA).
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Also, as shown in Figure 1, treatment of Caco-2 cells with ALS significantly inhibited the phosphorylation of AURKA at Thr288 in a concentration-dependent manner, whereas there was no significant change in the expression level of AURKA when treated with ALS at 0.1, 1, and 5 μM for 48 h. Moreover, in comparison to the control cells, incubation of Caco-2 cells with ALS at 0.1, 1, and 5 μM led to a 42.4%, 59.5%, and 82.9% reduction in the ratio of p-AURKA over AURKA, respectively (p < 0.05; Figure 1A,B). Collectively, treatment of HT29 and Caco-2 cells with ALS significantly inhibits the phosphorylation of AURKA at Thr288 in a concentration-dependent manner.

2.4. ALS Modulates the Cell Cycle Distribution of HT29 and Caco-2 Cells

As the inhibitory effect of ALS on cell proliferation and phosphorylation of AURKA has been observed, we next assessed the effect of ALS on the cell cycle distribution of HT29 and Caco-2 cells by flow cytometry. Treatment of HT29 cells with ALS at 0.1, 1, and 5 μM for 24 h resulted in a remarkable increase in the percentage of cells in G2/M phase from 10.5% at basal level to 16.8%, 85.7%, and 87.7%, respectively (p < 0.001; Figure 2A and Figure S2A). Similarly, the percentage of Caco-2 cells in G2/M phase was raised from 17.3% at basal level to 56.2%, 77.2%, and 77.5% when treated with ALS at 0.1, 1, and 5 μM for 24 h, respectively (p < 0.001; Figure 2A and Figure S2A). Meanwhile, the percentage of both cell lines in the G1 and S phases was decreased correspondingly. The data show that ALS induces significant cell cycle arrest in the G2/M phase in both cell lines in a concentration-dependent manner.
We also performed separate experiments to assess the effect of ALS at 1 μM on cell cycle distribution over 72 h in HT29 and Caco-2 cells. We found the appearance of aneuploid cells after ALS treatment over 48 h in both cell lines. Compared with control cells, the percentage of diploid HT29 cells in G2/M phase was increased from 7.0% at the basal level to 12.7%, 24.3%, 37.3%, and 71.4% after treatment with 1 μM ALS for 4, 8, 12, and 24 h and declined to 21.1% and 12% after 48 and 72 h, respectively (p < 0.001; Figure 2B and Figure S2B), while the percentage of aneuploid HT29 cells in G2/M phase was increased from 23.9% to 69.3% after treatment with ALS from 48 to 72 h (Figure 2B and Figure S2B). Similarly, the percentage of diploid Caco-2 cells in G2/M phase increased from 18.5% at the basal level to 19.9%, 20.8%, 34.1%, 80.8%, 64.7% and 57.7% when the cells were incubated with 1 μM ALS for 4, 8, 12, 24, 48 and 72 h, respectively (p < 0.001; Figure 2C and Figure S2C), while the percentage of aneuploid Caco-2 cells in G2/M phase was increased from 16.5% to 34.2% after treatment with ALS from 48 to 72 h. On the contrary, the percentage of HT29 and Caco-2 diploid cells in G1 phase was markedly reduced (p < 0.001; Figure 2 and Figure S2). Taken together, these results suggest that ALS induces a time-dependent cell cycle arrest in G2/M phase in HT29 and Caco-2 cells.
Figure 2. ALS induces cell cycle arrest in G2/M phase in HT29 and Caco-2 cells. (A) HT29 and Caco-2 cells were treated with ALS at 0.1, 1, and 5 μM for 24 h and then subjected to flow cytometric analysis. Representative DNA fluorescence histograms of propidium iodide (PI)-stained HT29 and Caco-2 cells showing the cell cycle distribution; (B) Time course of ALS-induced cell cycle change over 72 h in HT29 cells. Flow cytometric histograms showing the cell cycle distribution when HT29 cells were incubated with ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h; (C) Time course of ALS-induced cell cycle change over 72 h in Caco-2 cells. Flow cytometric histograms show the cell cycle distribution when Caco-2 cells were incubated with ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h. Cells were stained with PI and subjected to flow cytometric analysis that collected 15,000 events. Data represent the mean ± SD of three independent experiments. Dip: diploid; Ani: aneuploid.
Figure 2. ALS induces cell cycle arrest in G2/M phase in HT29 and Caco-2 cells. (A) HT29 and Caco-2 cells were treated with ALS at 0.1, 1, and 5 μM for 24 h and then subjected to flow cytometric analysis. Representative DNA fluorescence histograms of propidium iodide (PI)-stained HT29 and Caco-2 cells showing the cell cycle distribution; (B) Time course of ALS-induced cell cycle change over 72 h in HT29 cells. Flow cytometric histograms showing the cell cycle distribution when HT29 cells were incubated with ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h; (C) Time course of ALS-induced cell cycle change over 72 h in Caco-2 cells. Flow cytometric histograms show the cell cycle distribution when Caco-2 cells were incubated with ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h. Cells were stained with PI and subjected to flow cytometric analysis that collected 15,000 events. Data represent the mean ± SD of three independent experiments. Dip: diploid; Ani: aneuploid.
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2.5. ALS Differentially Alters Key Regulators of Cell Cycle in HT29 and Caco-2 Cells

To unveil the underlying mechanism for ALS-induced cell cycle arrest, we further dissected the expression of key cell cycle regulating proteins, including CDK1/CDC2, p-CDC2 (Tyr15), cyclin B1, p-cyclin B1 (Ser133), p-CDC25C (Ser216), PLK1, p53, and p21/Waf1 in HT29 and Caco-2 cells using Western blotting assay. As shown in Figure 3A and Figure S3A, incubation of HT29 cells with ALS significantly inhibited the expression of the positive regulators but enhanced the expression of negative regulators that are responsible for the G2 to M phase transition. The expression level of cyclin B1 and CDC2 was declined in a concentration-dependent manner. There was 1.3-fold reduction and a 30.0% decrease in the expression level of cyclin B1 and CDC2 when treated with 1 μM ALS, respectively (p > 0.05), whereas there was a 69.8% and 45.2% reduction in the expression level of cyclin B1 and CDC2 when treated with 5 μM ALS, compared to the control cells, respectively (p < 0.05 or 0.01; Figure 3A and Figure S3A). In contrast, the expression level of the negative regulators of cell cycle progression were significantly increased in a concentration-dependent manner. As shown in Figure 3A and Figure S3A, the expression level of p53 was increased 1.5- and 1.4-fold when HT29 cells were incubated with ALS at 1 μM (p < 0.05) and 5 μM (p > 0.05), respectively, compared to the control cells. The expression level of p21 Waf1/Cip1 was increased 3.3- and 2.5-fold when HT29 cells were treated with 1 and 5 μM ALS, respectively, compared to the control cells (p < 0.001; Figure 3A and Figure S3A). Collectively, the decreased expression of cyclin B1 and CDC2 and the increased expression of p53 and p21 contribute to ALS-induced G2/M phase arrest of HT29 cells.
For Caco-2 cells, the regulatory effect of ALS on the expression level of key cell cycle regulators was in a concentration-dependent manner (Figure 3B and Figure S3B). We found that the expression level of cyclin B1 and CDC2 were remarkably increased (Figure 3B and Figure S3B). Therefore, we further examined the level of PLK1, p-cyclin B1 (Ser133), p-CDC2 (Tyr15), and p-CDC25C (Ser216). In comparison to the control cells, the level of p-cyclin B1 (Ser133) was decreased 36.2% and 66.4% when treated with 1 and 5 μM ALS for 48 h, respectively (p < 0.01; Figure 3B and Figure S3B). Similarly, the expression level of PLK1 was decreased 87.3% and 88.3% when treated with 1 and 5 μM ALS for 48 h, respectively (p < 0.01; Figure 3B and Figure S3B). In contrast, the level of p-CDC25C (Ser216) was increased 2.3- and 2.6-fold when cells were incubated with 1 and 5 μM ALS, respectively, compared to the control cells (p < 0.01; Figure 3B and Figure S3B). The level of p-CDC2 (Tyr15) was increased 2.8- and 2.7-fold when incubated with 1 and 5 μM ALS, respectively, compared to the control cells (p < 0.01; Figure 3B and Figure S3B). Taken together, the decreased level of p-cyclin B1 (Ser133) and PLK1 and the increased level of p-CDC2 (Tyr15), critical regulators for the G2/M transition, contribute to ALS-induced G2/M phase arrest of Caco-2 cells.
Figure 3. Effect of ALS on the expression level of key regulators of cell cycle in HT29 and Caco-2 cells. (A) Representative blots showing the expression of CDK1/CDC2, cyclin B1, p21 Waf1/Cip1, and p53 when HT29 cells were treated with ALS at 0.1, 1, and 5 μM for 48 h; (B) Representative blots showing the level of PLK1, CDK1/CDC2, p-CDC2 (Tyr15), cyclin B1, p-cyclin B1 (Ser133), and p-CDC25C (Ser216) in Caco-2 cells.
Figure 3. Effect of ALS on the expression level of key regulators of cell cycle in HT29 and Caco-2 cells. (A) Representative blots showing the expression of CDK1/CDC2, cyclin B1, p21 Waf1/Cip1, and p53 when HT29 cells were treated with ALS at 0.1, 1, and 5 μM for 48 h; (B) Representative blots showing the level of PLK1, CDK1/CDC2, p-CDC2 (Tyr15), cyclin B1, p-cyclin B1 (Ser133), and p-CDC25C (Ser216) in Caco-2 cells.
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2.6. ALS Differentially Induces Cell Death in HT29 and Caco-2 Cells

To examine the cancer cell killing effect of ALS on HT29 and Caco-2 cells, the number of apoptotic cells was first quantified using flow cytometry. As shown in Figure 4A and Figure S4A, the total percentage of apoptotic cells (early + late apoptosis) was 6.2% in HT29 cells when incubated with the control vehicle only (0.05% dimethyl sulfoxide (DMSO), v/v). In comparison with the control cells, there was 2.4- and 2.6-fold increase in total apoptotic cells when HT29 cells were treated with 1 and 5 μM ALS, respectively (p < 0.05; Figure 4A and Figure S4A). In Caco-2 cells, there was a 2.0- and 1.8-fold increase in total apoptotic cells when exposed to 1 and 5 μM ALS, compared with the control cells (8.8%), respectively (p < 0.05; Figure 4A and Figure S4A).
Figure 4. ALS induces apoptotic death in HT29 and Caco-2 cells. (A) HT29 and Caco-2 cells were exposed to ALS at 0.1, 1, and 5 μM for 24 h and then subject to flow cytometric analysis. Flow cytometric dot plots of specific cell populations (live, early apoptosis and late apoptosis) in HT29 and Caco-2 cells; (B) HT29 and Caco-2 cells were treated with ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h and then subject to flow cytometric analysis. Flow cytometric dot plots showing specific cell populations (live, early apoptosis, and late apoptosis) in HT29 and Caco-2 cells. The apoptotic cells were detected by an annexin-V:PE (phycoerythrin) and 7-Aminoactinomycin D (7-AAD) double staining assay. The flow cytometer collected 15,000 events. Q1 indicated necrotic cells due to the machanical damage. Early apoptotic cells are located in the lower right corner (annexin V:PE positive only). Late apoptotic cells are located in the upper right corner (double positive with annexin V:PE and 7-AAD). The viable cells are located in the lower left corner (double negative with annexin V:PE and 7-AAD staining).
Figure 4. ALS induces apoptotic death in HT29 and Caco-2 cells. (A) HT29 and Caco-2 cells were exposed to ALS at 0.1, 1, and 5 μM for 24 h and then subject to flow cytometric analysis. Flow cytometric dot plots of specific cell populations (live, early apoptosis and late apoptosis) in HT29 and Caco-2 cells; (B) HT29 and Caco-2 cells were treated with ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h and then subject to flow cytometric analysis. Flow cytometric dot plots showing specific cell populations (live, early apoptosis, and late apoptosis) in HT29 and Caco-2 cells. The apoptotic cells were detected by an annexin-V:PE (phycoerythrin) and 7-Aminoactinomycin D (7-AAD) double staining assay. The flow cytometer collected 15,000 events. Q1 indicated necrotic cells due to the machanical damage. Early apoptotic cells are located in the lower right corner (annexin V:PE positive only). Late apoptotic cells are located in the upper right corner (double positive with annexin V:PE and 7-AAD). The viable cells are located in the lower left corner (double negative with annexin V:PE and 7-AAD staining).
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Next, we evaluated the effect of ALS on the apoptosis of HT29 and Caco-2 cells when cells were exposed to 1 μM ALS over 72 h (Figure 4B and Figure S4B). The percentage of apoptotic HT29 cells was increased from 3.8% at the basal level (time 0) to 4.6%, 4.6%, 5.3%, 6.8%, 12.1%, and 24.3% with the treatment of ALS for 4, 8, 12, 24, 48, and 72 h, respectively. Compared with the control cells, incubation with ALS for 24, 48, and 72 h caused a 1.8-, 3.2-, and 6.4-fold increase in total apoptotic cells (p < 0.001; Figure 4B and Figure S4B). For Caco-2 cells, the percentage of apoptotic cells was increased from 6.0% at the basal level (time 0) to 5.9%, 8.7%, 7.6%, 9.4%, 11.8%, and 12.9% with the treatment of ALS for 4, 8, 12, 24, 48, and 72 h, respectively. In comparison to the control cells, treatment of Caco-2 cells with ALS for 24, 48, and 72 h caused a 1.6-, 2.0-, and 2.2-fold increase in total apoptotic cells (p < 0.001; Figure 4B and Figure S4B). Taken together, the results clearly suggest that ALS induces apoptotic cell death in HT29 and Caco-2 cells in concentration- and time-dependent manners.
The mechanism for ALS-induced apoptosis was delineated in HT29 and Caco-2 cells by western blotting analysis. We evaluated the expression level of key molecules involved in apoptosis process, including Bcl-xl, Bcl-2, Bax, PUMA, cytochrome c, cleaved caspase 3, cleaved caspase 9, cleaved PARP, RIP, p-FADD, and FADD. HT29 and Caco-2 cells were treated with ALS at 0.1, 1, and 5 μM for 48 h. In comparison to the control cells, incubation of HT29 cells with 1 and 5 μM ALS increased Bax level 1.8- and 2.1-fold, respectively (p < 0.05; Figure 5A and Figure S5A); whereas incubation of HT29 cells with 5 μM ALS decreased Bcl-2 and Bcl-xl level 72.1% and 47.7%, respectively, compared to the control cells (p < 0.01 or 0.05; Figure 5A and Figure S5A). Given the marked increase in the expression level of Bax but a dramatic decrease in the expression level of Bcl-xl and Bcl-2, the disturbed balance of mitochondria-mediated apoptotic status may shift to pro-apoptotic state. We assessed the expression of other pro-apoptotic and anti-apoptotic proteins involved in mitochondria-mediated apoptotic pathway. Compared to the control cells, treatment of HT29 cells with 1 and 5 μM ALS for 48 h markedly increased 2.7- and 3.3-fold in the expression level of PUMA, respectively (p < 0.01; Figure 5A and Figure S5A). The cytosolic level of cytochrome c was increased 2.6-fold when treated with 5 μM ALS (p < 0.05; Figure 5A and Figure S5A). Furthermore, a significant increase in the level of cleaved caspases 9, cleaved caspase 3, and cleaved PARP was observed. Compared to the control cells, incubation of HT29 cells with ALS at 1 and 5 μM resulted in a 2.2- and 2.3-fold increase in the level of cleaved caspase 3, a 2.0- and 1.7-fold rise in the level of cleaved caspase 9, and a 4.4- and 5.3-fold elevation in the level of cleaved PARP, respectively (p < 0.01; Figure 5A and Figure S5A). Taken together, these data demonstrate that ALS induces apoptotic death of HT29 cells via mitochondria-mediated apoptotic pathway.
Figure 5. Effect of ALS on the expression level of key proapoptotic and antiapoptotic molecules in HT29 and Caco-2 cells. (A) Effect of ALS on the expression level of Bcl-xl, Bax, Bcl-2, PUMA, cytochrome c, cleaved caspase 3, cleaved caspase 9, and cleaved PARP in HT29 cells; (B) Effect of ALS on the expression level of Bcl-xl, Bax, Bcl-2, p-FADD (Ser194), FADD, RIP, cytochrome c, cleaved caspase 3, and cleaved PARP in Caco-2 cells.
Figure 5. Effect of ALS on the expression level of key proapoptotic and antiapoptotic molecules in HT29 and Caco-2 cells. (A) Effect of ALS on the expression level of Bcl-xl, Bax, Bcl-2, PUMA, cytochrome c, cleaved caspase 3, cleaved caspase 9, and cleaved PARP in HT29 cells; (B) Effect of ALS on the expression level of Bcl-xl, Bax, Bcl-2, p-FADD (Ser194), FADD, RIP, cytochrome c, cleaved caspase 3, and cleaved PARP in Caco-2 cells.
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For Caco-2 cells, we also first evaluated the expression levels of the pro-apoptotic protein Bax and the anti-apoptotic proteins Bcl-2 and Bcl-xl. Caco-2 cells were exposed to ALS at 0.1, 1, and 5 μM for 48 h. Surprisingly, the expression level of Bax was decreased 61% and 62.7% when treated with 1 and 5 μM ALS for 48 h, compared with the control cells, respectively (p < 0.05; Figure 5B and Figure S5B). In contrast, the level of Bcl-2 was increased 1.5- and 1.5-fold when treated with 1 and 5 μM ALS for 48 h, respectively, compared to the control cells (Figure 5B and Figure S5B). There was no significant alteration in expression level of Bcl-xl between the control cells and ALS-treated cells (Figure 5B and Figure S5B). These results suggest that mitochondrial pathway is not involved in the ALS-induced apoptosis in Caco-2 cells. Therefore, we next assessed the expression level of key proteins regulating death receptor signaling pathway. There was a 1.5- and 2.5-fold increase in the expression level of RIP when cells were treated with ALS at 1 and 5 μM for 48 h, respectively, compared to the control cells (p < 0.01; Figure 5B and Figure S5B). There was a 1.5-, 1.3-, and 1.8-fold increase in the level of p-FADD, although there was no statistical significance, while there was a 15.4%, 34.2%, and 36.9% decrease in the expression level of FADD, when cells were incubated in ALS at 0.1, 1, and 5 μM for 48 h, respectively, compared to the control cells (Figure 5B and Figure S5B). Consequently, the p-FADD/FADD ratio was remarkably increased 2.0- and 3.0-fold when cells were treated with 1 and 5 μM ALS for 48 h, respectively, compared to control cells (p < 0.01; Figure 5B and Figure S5B). Furthermore, the expression of downstream regulators was also tested. There was a 2.3- and 3.2-fold increase in the cytosolic level of cytochrome c when cells were treated with ALS at 1 and 5 μM for 48 h, respectively, compared to the control cells (p < 0.05; Figure 5B and Figure S5B). There was a 1.9- and 2.2-fold increase in the level of cleaved caspase 3 when treated with ALS at 1 and 5 μM for 48 h, respectively, compared to the control cells (p < 0.01; Figure 5B and Figure S5B). There was a 1.9- and 2.1-fold increase in the level of cleaved PARP when treated with ALS at 1 and 5 μM for 48 h, respectively, compared to the control cells (p < 0.01; Figure 5B and Figure S5B). Taken together, these results reveal that ALS induces apoptotic death of Caco-2 cells via death receptor signaling pathway. The differential responses to ALS treatment may be ascribed to the different cell type, in particular, the difference in p53 in these cell lines.

2.7. ALS Induces Autophagy of HT29 and Caco-2 Cells

As there was a clear ALS-induced apoptosis in HT29 and Caco-2 cells, we next investigated the effect of ALS on the autophagy of HT29 and Caco-2 cells by flow cytometric analysis and confocal microscopic examination. As shown in Figure 6A and Figure S6A, treatment of HT29 and Caco-2 cells with ALS for 24 h induced autophagy in a concentration-dependent manner. The percentage of intracellular autophagic signal at the basal level was 6.9% and 9.6% for HT29 and Caco-2 cells, respectively. Incubation of HT29 cells with 1 and 5 μM ALS for 24 h resulted in a 5.3- and 6.1-fold increase in the percentage of autophagic signal, respectively, compared to the control cells (p < 0.01; Figure 6A and Figure S6A). For Caco-2 cells, incubation with 1 and 5 μM ALS for 24 h resulted in a 1.7- and 2.0-fold increase in the percentage of autophagic signal, respectively, compared to the control cells (p < 0.01; Figure 6A and Figure S6A).
Furthermore, the effect of ALS on intracellular autophagy of HT29 and Caco-2 cells over time-course was evaluated. Both cells were exposed to ALS at 1 μM for 4, 8, 12, 24, 48, and 72 h. The percentage of autophagic signal was increased 3.2-, 5.6-, and 7.0-fold when HT29 cells were treated for 24, 48, and 72 h, respectively, compared to control cells (p < 0.001; Figure 6B and Figure S6B). For Caco-2 cells, the percentage of autophagic signal was increased 2.0-, 3.0-, and 2.5-fold when cells were treated for 24, 48, and 72 h, respectively, compared to control cells (p < 0.001; Figure 6B and Figure S6B). These results indicate that ALS induces a remarkable autophagy of HT29 and Caco-2 cells in concentration- and time-dependent manners.
Next, we performed the confocal microscopy to determine the autophagy-inducing effect of ALS in HT29 and Caco-2 cells. As shown in Figure 6C and Figure S6C, in comparison to the control cells, there was a 2.2- and 3.1-fold increase in the autophagy level of HT29 cells when treated with ALS at 1 and 5 μM for 24 h, respectively (p < 0.001). For Caco-2 cells, treatment with ALS at 1 and 5 μM for 24 h caused a 1.9- and 2.2-fold increase in the autophagy level when compared with the control cells, respectively (p < 0.001; Figure 6C and Figure S6C). There was no significant change in the autophagy level when both cell lines were treated with ALS at low concentration (0.1 µM). These results show that ALS treatment induces a significant concentration-dependent increase in autophagy of HT29 and Caco-2 cells.
Figure 6. ALS induces autophagic cell death in HT29 and Caco-2 cells. (A) Cells were treated with ALS at concentrations of 0.1, 1, and 5 µM for 24 h and cell samples were subject to flow cytometry analysis. Flow cytometric dot plots showing autophagic HT29 and Caco-2 cells stained by Cyto-ID®; (B) HT29 and Caco-2 cells were treated with ALS at 1 µM for 4, 8, 12, 24, 48, and 72 h and then subject to flow cytometry analysis. Flow cytometric dot plots showing autophagic HT29 and Caco-2 cells stained by Cyto-ID®; (C) HT29 and Caco-2 Cells were treated with ALS at 0.1, 1, and 5 µM for 24 h. Cells were stained with green fluorescent Cyto-ID® and subjected to confocal microscopy to detect autophagy. Confocal microscopic images showing autophagy in HT29 and Caco-2 cells. The box indicates the events that were counted. FL: fluoresence. Maganification: 40×.
Figure 6. ALS induces autophagic cell death in HT29 and Caco-2 cells. (A) Cells were treated with ALS at concentrations of 0.1, 1, and 5 µM for 24 h and cell samples were subject to flow cytometry analysis. Flow cytometric dot plots showing autophagic HT29 and Caco-2 cells stained by Cyto-ID®; (B) HT29 and Caco-2 cells were treated with ALS at 1 µM for 4, 8, 12, 24, 48, and 72 h and then subject to flow cytometry analysis. Flow cytometric dot plots showing autophagic HT29 and Caco-2 cells stained by Cyto-ID®; (C) HT29 and Caco-2 Cells were treated with ALS at 0.1, 1, and 5 µM for 24 h. Cells were stained with green fluorescent Cyto-ID® and subjected to confocal microscopy to detect autophagy. Confocal microscopic images showing autophagy in HT29 and Caco-2 cells. The box indicates the events that were counted. FL: fluoresence. Maganification: 40×.
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2.8. ALS Regulates PI3K/Akt/mTOR Axis, AMPK, and p38 MAPK Signaling Pathways in HT29 and Caco-2 Cells

After determining the autophagy-inducing effect of ALS in HT29 and Caco-2 cells, we further elucidated the latent mechanism for the ALS-induced autophagy. ALS treatment results in remarkable changes in the expression and phosphorylation levels of key functional molecules involved in autophagy signaling pathway. First, we assessed the phosphorylation level of PI3K at Tyr199, AMPK at Thr172, and p38 MAPK at Thr180/Tyr182. These proteins execute critical roles in the regulation of cell proliferation, cell survival, cell migration and cell death as the upstream signaling molecules of the protein kinase B (Akt)/mammalian target of rapamycin (mTOR) pathway [24,25,26]. Exposure of HT29 cells to ALS for 48 h declined the phosphorylation level of PI3K (Tyr199) and increased the expression level of total PI3K (Figure 7A,B). Consequently, the p-PI3K/PI3K ratio was decreased 4.4%, 29.1%, and 33.7% (p < 0.001; Figure 7A,B) when treated with ALS at 0.1, 1, and 5 μM, respectively, compared to control cells. The p-AMPK/AMPK ratio was increased 1.3-, 1.3-, and 1.2-fold when HT29 cells were treated with ALS at 0.1, 1, and 5 μM, respectively, compared to control cells (Figure 7A,B); while the p-p38/p38 ratio was increased 1.6-, 3.1-, and 3.0-fold when HT29 cells were treated with ALS at 0.1, 1, and 5 μM, respectively, compared to control cells (p < 0.05 or 0.01; Figure 7A,B).
Figure 7. Effect of ALS on the expression or phospharylation levels of key autophagy-regulating molecules in HT29 and Caco-2 cells. Cells were treated with ALS at 0.1, 1, and 5 µM for 48 h. The phosphorylation level of PI3K, AMPK, Akt, p38 MAPK, and mTOR, and the total level of mTOR, beclin 1, PTEN, LC3-I, and LC3-II in HT29 and Caco-2 cells determined by Western blotting assay. (A) Representative blots of p-PI3K, PI3K, p-AMPK, AMPK, p-Akt, Akt, p-p38 MAPK, p38 MAPK, p-mTOR, mTOR, beclin 1, LC3-I, and LC3-II in HT29 and Caco-2 cells treated with ALS for 48 h; and (B) Bar graphs showing the ratio of p-PI3K/PI3K, p-AMPK/AMPK, p-Akt/Akt, p-p38 MAPK/p38 MAPK, p-mTOR/mTOR, LC3-II/LC3-I, and the expression levels of beclin 1 and PTEN in HT29 and Caco-2 cells treated with ALS for 48 h. β-Actin was used as the internal control. Data are expressed as the mean ± SD of three independent experiments. * p < 0.05, ** p < 0.01, and *** p < 0.001 by one-way ANOVA.
Figure 7. Effect of ALS on the expression or phospharylation levels of key autophagy-regulating molecules in HT29 and Caco-2 cells. Cells were treated with ALS at 0.1, 1, and 5 µM for 48 h. The phosphorylation level of PI3K, AMPK, Akt, p38 MAPK, and mTOR, and the total level of mTOR, beclin 1, PTEN, LC3-I, and LC3-II in HT29 and Caco-2 cells determined by Western blotting assay. (A) Representative blots of p-PI3K, PI3K, p-AMPK, AMPK, p-Akt, Akt, p-p38 MAPK, p38 MAPK, p-mTOR, mTOR, beclin 1, LC3-I, and LC3-II in HT29 and Caco-2 cells treated with ALS for 48 h; and (B) Bar graphs showing the ratio of p-PI3K/PI3K, p-AMPK/AMPK, p-Akt/Akt, p-p38 MAPK/p38 MAPK, p-mTOR/mTOR, LC3-II/LC3-I, and the expression levels of beclin 1 and PTEN in HT29 and Caco-2 cells treated with ALS for 48 h. β-Actin was used as the internal control. Data are expressed as the mean ± SD of three independent experiments. * p < 0.05, ** p < 0.01, and *** p < 0.001 by one-way ANOVA.
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As a downstream effector of PI3K, Akt plays a key role in regulating diverse cellular functions including metabolism, cell proliferation, survival, growth, migration, invasion, and angiogenesis [27]. The mTOR kinase is a downstream target of Akt, which is phosphorylated and activated at Ser473 by mTORC2 and at Thr308 by 3-phosphoinositide-dependent protein kinase-1 [28]. mTOR is regulated by signaling pathway originating from starvation, growth factors, and cellular stressors, and plays a critical role in cell growth, autophagic cell death, and homeostasis [29]. We next evaluated the phosphorylation of Akt at Ser473 and mTOR at Ser2448 after ALS treatment of HT29 cells. There was a concentration-dependent decline in the phosphorylation level of Akt and mTOR with ALS treatment at 0.1, 1, and 5 µM (Figure 7A,B). However, the expression of total Akt and mTOR was not significantly altered after ALS incubation (Figure 7A,B). Thus, in comparison to the control cells, the ratio of p-Akt over Akt was markedly reduced 18.6%, 14.8%, and 72.8% and the ratio of p-mTOR over mTOR was declined 18.4%, 23.3%, and 33.1% when HT29 cells were treated with ALS at 0.1, 1, and 5 μM, respectively (p < 0.01; Figure 7A,B). PTEN is a dual-specificity phosphatase and tumor suppressor gene, acting as a negative regulator of Akt/mTOR and MAPK signaling, with a key function of cell death [30]. Therefore, we examined the expression level of PTEN when HT29 cells were treated with ALS for 48 h. Exposure of HT29 cells to ALS at 0.1, 1, and 5 µM resulted in a 1.6-, 2.0-, and 2.8-fold increase in the expression level of PTEN, respectively, compared to the control cells (p < 0.01; Figure 7A,B).
Beclin 1 and LC3 are two important markers of vesicle expansion and formation during the autophagy process. Thus, we examined the effect of ALS on expression of beclin 1, LC3-I, and LC3-II in HT29 cells. There was a significant increase in the expression of beclin 1 and ratio of LC3-II over LC3-I when cells were treated with ALS (Figure 7A,B). In comparison with the control cells, the expression level of beclin 1 was increased 1.6- and 1.9-fold with the treatment of ALS at 1 and 5 µM, respectively, and the level of LC3-II was increased after ALS treatment in HT29 cells. The ratio of LC3-II/LC3-I was increased 1.8- and 1.8-fold when cells were treated with ALS at 1 and 5 μM, respectively (p < 0.01; Figure 7A,B). These results indicate that inhibition of the PI3K/Akt/mTOR pathway and activation of AMPK and p38MAPK contribute to the autophagy-inducing effect of ALS on HT29 cells.
For Caco-2 cells, incubation with ALS for 24 h led to marked alteration in the phosphorylation level of PI3K, p38 MAPK, and AMPK, but did not affect the total expression level (Figure 7A,B). There was a 37.4% and 54.8% decline in the ratio of p-PI3K over PI3K, a 51.0% and 69.6% decrease in the ratio of p-p38 over p38, and a 1.9- and 1.9-fold increase in the ratio of p-AMPK over AMPK when treated with ALS at 1 and 5 µM, respectively (Figure 7A,B). We further assessed the change in the phosphorylation of Akt at Ser473 and mTOR at Ser2448. In comparison with the control cells, there was a concentration-dependent decrease in the phosphorylation level of Akt and mTOR, while there was no significant alteration in the total expression level of Akt and mTOR when treated with ALS at 0.1, 1, and 5 µM (Figure 7A,B). Consequently, compared to the control cells, there was a 49.6%, 69.9%, and 61.8% decrease in the ratio of p-Akt over Akt (p < 0.01; Figure 7A,B), and a 58.7%, 67.5%, and 79.9% reduction in the ratio of p-mTOR over mTOR in Caco-2 cells incubated with ALS at 0.1, 1, and 5 µM, respectively (p < 0.001; Figure 7A,B). We also observed the expression level of PTEN after ALS incubation. In comparison with the control cells, there was a 1.2- and 1.4-fold increase in the expression level of PTEN in Caco-2 cells exposed to ALS at 1 and 5 µM, respectively (Figure 7A,B). Finally, we evaluated the expression levels of beclin 1, LC3-I, and LC3-II in Caco-2 cells treated with ALS. ALS caused a prominent increase in the expression levels of beclin 1 and LC3-II, but did not caused alteration in the expression level of LC3-I (Figure 7A,B). In comparison to the control cells, there was a 1.6- and 1.9-fold increase in the expression level of beclin 1 when treated with ALS at 1 and 5 µM, respectively; and there was a 1.7-, 1.4-, and 1.5-fold increase in LC3-II/LC3-I ratio when treated with ALS at 0.1, 1, and 5 µM, respectively (p < 0.01; Figure 7A,B). These findings show that inhibition of PI3K/Akt/mTOR pathway, suppression of p38MAPK, and activation of AMPK contribute to the autophagy-inducing effect of ALS on Caco-2 cells.

2.9. There Is a Crosstalk between ALS-Induced Apoptosis and Autophagy in HT29 and Caco-2 Cells

To further dissect the crosstalk between autophagy and apoptosis in HT29 and Caco-2 cells responding to ALS treatment, the flow cytometry was used to simultaneously examine cellular autophagy and apoptosis. First, we assessed the effect of induction or inhibition of autophagy on basal and ALS-induced autophagy in both cell lines. In HT29 cells, incubation with 0.5 µM rapamycin (a mTOR inhibitor and autophagy inducer ), 10 µM WM (a PI3K inhibitor and autophagy blocker), 1 µM MK2206 (a selective inhibitor of Akt and autophagy inducer), or 10 µM SB202190 (a selective p38 MAPK inhibitor and autophagy inducer) alone for 24 h led to a 5.4-, 4.3-, 2.0-, or 3.7-fold increase in basal autophagy compared to the control cells, respectively (p < 0.001; Figure 8A and Figure S7). Co-incubation with 0.5 µM rapamycin or 10 µM SB202190 increased ALS-induced autophagy 1.9- or 1.9-fold in HT29 cells, respectively (p < 0.001; Figure 8A and Figure S7), while co-incubation with 10 µM WM or 1 µM MK2206 only slightly enhanced ALS-induced autophagy. In Caco-2 cells, treatment with 0.5 µM rapamycin, 1 µM MK2206, or 10 µM SB202190 alone for 24 h induced a 2.7-, 6.5-, or 3.4-fold increase in basal autophagy compared to the control cells, respectively (p < 0.001; Figure 8A and Figure S7), while 10 µM WM diminished the basal autophagy. Pre-incubation with 0.5 µM rapamycin, 1 µM MK2206, or 10 µM SB202190 increased ALS-induced autophagy 1.5-, 3.1-, or 1.9-fold in Caco-2 cells (p < 0.001; Figure 8A and Figure S7). Of note, pre-treatment with 10 µM WM significantly decreased ALS-induced autophagy (Figure 8A and Figure S7).
Figure 8. Effect of various inducers and inhibitors on the apoptosis and autophagy induced by ALS in HT29 and Caco-2 cells. The cells were pretreated with each of the compounds for 1 h before ALS was added and incubated for a further 24 h. Cells were double stained with Annexin V:PE (phycoerythrin) and 7-Aminoactinomycin D (7-AAD) to detect cellular apoptosis, after the cells were treated with ALS for 24 h. The autophagy was detected using the Cyto-ID® green fluorescent dye to stain autophagy-associated vacuoles. (A) Flow cytometric dot plots showing the effects of a series of compounds on basal and ALS-induced apoptosis in HT29 and Caco-2 cells; (B) Flow cytometric dot plots showing the effects of the compounds on basal and ALS-induced autophagy in HT29 and Caco-2 cells. The box indicates the events that were counted. DMSO: dimethyl sulfoxide.
Figure 8. Effect of various inducers and inhibitors on the apoptosis and autophagy induced by ALS in HT29 and Caco-2 cells. The cells were pretreated with each of the compounds for 1 h before ALS was added and incubated for a further 24 h. Cells were double stained with Annexin V:PE (phycoerythrin) and 7-Aminoactinomycin D (7-AAD) to detect cellular apoptosis, after the cells were treated with ALS for 24 h. The autophagy was detected using the Cyto-ID® green fluorescent dye to stain autophagy-associated vacuoles. (A) Flow cytometric dot plots showing the effects of a series of compounds on basal and ALS-induced apoptosis in HT29 and Caco-2 cells; (B) Flow cytometric dot plots showing the effects of the compounds on basal and ALS-induced autophagy in HT29 and Caco-2 cells. The box indicates the events that were counted. DMSO: dimethyl sulfoxide.
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Next, we evaluated the effect of induction or inhibition of autophagy on basal and ALS-induced apoptosis in HT29 and Caco-2 cells. Incubation of HT29 cells with 10 µM SB202190 alone for 24 h remarkably induced apoptosis (9.6% vs. 19.4%, p < 0.05 Figure 8B and Figure S7), while incubation of the cells with 0.5 µM rapamycin, 10 µM WM, or 1 µM MK2206 for 24 h had no significant effect on the basal apoptosis of HT29 cells (Figure 8B and Figure S7). In addition, co-incubation of HT29 cells with 10 µM SB202190 increased ALS-induced apoptosis (14.4% vs. 23.7%, p < 0.001; Figure 8B and Figure S7), whereas co-incubation with 0.5 µM rapamycin, 10 µM WM, or 1 µM MK2206 only slightly altered ALS-induced apoptosis. In Caco-2 cells, exposure to 0.5 µM rapamycin, 10 µM WM, 10 µM SB202190 or 1 µM MK2206 alone only slightly increased the basal apoptosis (Figure 8B and Figure S7). Pre-incubation with 10 µM WM enhanced ALS-induced apoptosis (9.7% vs. 14.0%, p < 0.001; Figure 8B and Figure S7), whereas co-incubation with 0.5 µM rapamycin, 1 µM MK2206, or 10 µM SB202190 only slightly altered ALS-induced apoptosis (Figure 8B and Figure S7). Taken together, these data shows that regulation of p38 MAPK by SB202190 may alter ALS-induced autophagy and apoptosis in HT29 cells and modulation of PI3K by WM may alter ALS-induced autophagy and apoptosis in Caco-2 cells with differential effects depending on the cell type. The autophagy inducer SB202190 enhances the ALS-induced apoptosis in both HT29 and Caco-2 cells, whereas the autophagy blocker WM increases ALS-induced autophagy in HT29 cells but decreases it in Caco-2 cells.

2.10. ALS Suppresses EMT in HT29 and Caco-2 Cells

Epithelial-to-mesenchymal transition (EMT) is a critical event in which epithelial cells trans-differentiate into fibroblastic migratory cells through losing intracellular adhesion and cellular polarity and obtaining mesenchymal properties and increased motility. It has been suggested that EMT contributes to the cancer cells spreading and migrating to distant organs to form metastases [31,32]. E-cadherin is a hallmarker of the epithelial phenotype while N-cadherin is considered a key mesenchymal phenotype. Loss of E-cadherin and increasing N-cadherin expression facilitates the occurring of EMT and metastasis [33]. We speculated that ALS can inhibit EMT phenotype in HT29 and Caco-2 cells. So we examined the expression of EMT-associated regulators, including E-cadherin, N-cadherin, slug, TCF-8, and ZO-1. First, ALS incubation resulted in remarkable effect on the expression level of E-cadherin and N-cadherin (Figure 9A,B). Treatment of HT29 cells with ALS at 1 and 5 µM led to a 2.3- and 2.6-fold increase in the expression level of E-cadherin, respectively, compared to the control cells (p < 0.01; Figure 9A,B), but treatment of HT29 cells with ALS at 0.1, 1, and 5 µM resulted in a 3.4%, 5.3%, and 27.4% decrease in the expression level of N-cadherin, respectively (Figure 9A,B). Although there was no significant difference in the expression of N-cadherin, an increased ratio of E-cadherin over N-cadherin was observed. The ratio of E-cadherin/N-cadherin was increased 1.4-, 2.5-, and 3.7-fold when HT29 cells were exposed to ALS at 0.1, 1, and 5 µM for 48 h, respectively (p < 0.01; Figure 9A,B). In Caco-2 cells, in comparison to the control cells, the expression level of E-cadherin was increased by 2.7- and 2.7-fold when cells were treated with ALS at 1 and 5 μM, respectively, (p < 0.01; Figure 9A,B). Meanwhile, the expression level of N-cadherin was decreased by 46.4%, 72.8%, and 69.1% when cells were incubated with ALS at 0.1, 1, and 5 μM, respectively, (p < 0.01; Figure 9A,B). The ratio of E-cadherin/N-cadherin was increased 3.2-, 13.0-, and 9.8-fold when Caco-2 cells were incubated with ALS at 0.1, 1, and 5 μM for 48 h, respectively, (p < 0.01; Figure 9A,B).
Slug is a zinc finger transcriptional factor, together with TCF8/ZEB1 acting as suppressors of E-cadherin in EMT [34]. We further examined the effect of ALS incubation of HT29 and Caco-2 cells on the expression of slug and TCF-8/ZEB1. As shown in Figure 9A,B, there was a significant reduction in the expression levels of slug and TCF-8/ZEB1. In comparison with control cells, exposure of HT29 cells to ALS at 1 and 5 µM led to a 55.3% and 44.1% decline in the expression level of slug, respectively (p < 0.05; Figure 9A,B). Exposure of HT29 cells to ALS at 1 and 5 µM resulted in a 44.5% and 53.4% reduction in the expression level of TCF-8/ZEB1, respectively (p < 0.001; Figure 9A,B). Similarly, in Caco-2 cells, treatment of cells to ALS led to a concentration-dependent reduction in the expression level of slug and TCF-8/ZEB1 (p < 0.05 or 0.01; Figure 9A,B).
In the end, we assessed the effect of ALS on expression of ZO-1 in HT29 and Caco-2 cells. ZO-1 is a member of Zonula occludens proteins which are involved in the regulation of cytoskeletal organization, signal transduction, transcriptional modulation and cell polarity maintenance. ZO-1 are required for tight junction formation and function. It has been suggested that the cytoplasmic/nuclear relocalization of β-catenin and ZO-1 from the adhesions and tight junctions are common processes of the epithelial-mesenchymal transition associated with tumor invasion [35]. As shown in Figure 9, ALS significantly increased the expression level of ZO-1 in both cell lines. Compared to the control cells, there was a 2.1- and 3.1-fold increase in the expression level of ZO-1 when HT29 cells were treated with ALS at 1 and 5 µM, respectively (p < 0.01; Figure 9A,B). For Caco-2 cells, there was a 1.2-, 1.4-, and 4.5-fold increase in the expression level of ZO-1 when treated with ALS at 0.1, 1, and 5 µM respectively, compared to the control cells (p < 0.01; Figure 9A,B). In aggregate, all these results demonstrate that ALS has a strongly inhibitory effect on EMT by upregulating the expression level of E-cadherin and ZO-1, and down-regulating the expression level of N-cadherin, slug, and TCF-8 in HT29 and Caco-2 cells.
Figure 9. Effect of ALS on expression levels of epithelial to mesenchymal transition (EMT) associated markers in HT29 and Caco-2 cells. Cells were treated with ALS at concentrations of 0.1, 1, and 5 µM for 48 h and then protein samples were subject to Western blotting assay. (A) Representative blots showing the expression level of E-cadherin, N-cadherin, slug, TCF-8/ZEB1, and ZO-1 in HT29 and Caco-2 cells determined by Western blotting assay; (B) Bar graphs showing the expression level of E-cadherin, N-cadherin, slug, TCF-8/ZEB1, and ZO-1, and the ratio of E-cadherin over N-cadherin in HT29 and Caco-2 cells. β-Actin was used as the internal control. Data represent as the mean ± SD of three independent experiments. * p < 0.05, ** p < 0.01, and *** p < 0.001 by one-way ANOVA.
Figure 9. Effect of ALS on expression levels of epithelial to mesenchymal transition (EMT) associated markers in HT29 and Caco-2 cells. Cells were treated with ALS at concentrations of 0.1, 1, and 5 µM for 48 h and then protein samples were subject to Western blotting assay. (A) Representative blots showing the expression level of E-cadherin, N-cadherin, slug, TCF-8/ZEB1, and ZO-1 in HT29 and Caco-2 cells determined by Western blotting assay; (B) Bar graphs showing the expression level of E-cadherin, N-cadherin, slug, TCF-8/ZEB1, and ZO-1, and the ratio of E-cadherin over N-cadherin in HT29 and Caco-2 cells. β-Actin was used as the internal control. Data represent as the mean ± SD of three independent experiments. * p < 0.05, ** p < 0.01, and *** p < 0.001 by one-way ANOVA.
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3. Discussion

Due to the high mortality and morbidity resulted from CRC worldwide, CRC places a substantial heavy burden on individual and society [36]. It requires novel therapeutic agent with more therapeutic efficacy and less severe side effects. In particular, patients with advanced stages of CRC often suffer from the recurrence, metastasis, and complications, and frequently display poor therapeutic outcome, despite the application of various therapeutic strategies, including potentially curable surgery, chemotherapy, selective radiotherapy and other forms of treatment. Recently, compelling evidence indicates that AURKA can act as a novel and promising antineoplastic target; its selective inhibitor, ALS, is a small molecule which has demonstrated the potent anticancer effect in the treatment of various types of cancer in preclinical and clinical studies [15,16,17,19,20,21,22,37]. In the present study, a potent anti-proliferative effect of ALS was observed in HT29 and Caco-2 cells. We have found that ALS exerts a remarkable inducing effect on cell cycle arrest in G2/M phase and markedly promotes apoptosis and autophagy in concentration- and time-dependent manners in both cell lines with the involvement of multiple signaling pathways, including mitochondrial pathway, death receptor signaling pathway, PI3K/Akt/mTOR, p38 MAPK, and AMPK signaling pathways. Moreover, the inhibitory effect of ALS on the EMT may also contribute to its antitumor potential.
The cell cycle regulatory proteins, which have been found involved in proliferation of tumor cells, including the cyclins, the cyclin dependent kinases (CDKs), their downstream substrates, the CDK inhibitors (CKIs), and the tumor suppressor proteins (e.g., p53 and Rb). Activated CDK1 (CDC2) bound to cyclin B1 promotes entry into M-phase in cell cycle. So it is pivotal to maintain the activity of the cyclin B1-CDC2 (CDK1) complex in promoting G2/M transition process. There are many upstream regulators modifying the activity of the cyclin B1-CDC2 (CDK1) complex. p53 is a critical tumor suppressor protein and a positive regulator of cell cycle arrest. Normally, the G2/M DNA damage or chromosomal instability promote the phosphorylation of p53 and accelerates its dissociation from MDM2 and MDM4. Consequently, the transcriptional ability of p53 is activated. The p53 downstream-regulated genes including 14-3-3, p21, GADD45, and WIP1 ultimately serve to inactivate the Cyclin B1-CDC2 complex and suppress the entry into G2/M transition. AURKA is localized at the mitotic spindle and centrosome, where it interacts with many functional proteins/substrates, including PP1, p53, Cdh-1, TPX-2, RasGAP, and Ajuba. It was reported that in the absence of hyperactivation of AURAK, the crosstalk of AURKA with p53 caused tumorigenesis transformation of cells by counteracting the p53 mediated tumor suppression [38]. In our work, we detected a potent effect of ALS on G2/M phase cell cycle arrest in HT29 and Caco-2 cells, and we found that the active form of p-AURKA at Thr288 was significantly suppressed by ALS. There was an increase in expression level of p53 and p21 and a decrease in expression level of cyclinB1 and CDC2 which were observed as well. Collectively, these results indicate that ALS-induced G2/M cell cycle arrest may be attributed to its inhibitory effect on the interaction of AURKA and p53, however, this explanation needs to be further verified for CRC treatment.
On the other hand, due to the lack of p53 expression in Caco-2 cells, we, therefore, examined the upstream molecules regulating the cyclin B1-CDC2 (CDK1) complex. PLK1 could be activated by the concerted function of AURKA and the cofactor Bora [39]. CDC25 that can be activated by PLK1 and inactivated by Chk kinases through phosphorylation, is a positive regulator of CDC2 by removal of phosphates at Thr14 and Tyr15 [40,41,42]. In addition, PLK1 can phosphorylate cyclin B1 at Ser133 resulting in a rapid nuclear import of cyclin B1, which promotes the mitosis entry [43]. In the present study, we found a significant increase in the level of p-CDC25C (Ser216), total cyclinB1, and p-CDC2 (Tyr 15), but a decline in the level of PLK1, p-cyclinB1 (Ser133), suggesting that the PLK1-CDC25C-cyclinB1 and CDC2 complex axis is involved in ALS-induced G2/M cell cycle arrest in Caco-2 cells. Also, we also found that ALS induced cell cycle arrest in G2/M phase in gastric cancer cells [19], pancreatic cancer cells [21], osteosarcoma cells [22], breast cancer cells [44], and ovarian cancer cells [20].
Apoptosis is a distinct genetic and biochemical pathway of cell death necessary for cell growth, development and maintenance of homeostasis in metazoans. There are two specific pathways activating cell apoptosis, including intrinsic and extrinsic death pathway [45,46]. In this study, cytochrome c was released from mitochondria after ALS treatment, which might be caused by the increased expression level of Bax and decreased expression level of Bcl-2 and Bcl-xl. Subsequently, caspase 9 was activated with the elevated level of cleaved caspase 9, which in turn cleaved caspase 3 and PARP and ultimately induced apoptosis. The expression level of PUMA, which acted as one of pro-apoptotic members of Bcl-2 family, was increased in a concentration-dependent manner. These data indicate that ALS induces mitochondria-dependent apoptosis of HT29 cells. For Caco-2 cells, a decrease in the expression level of Bax and increased expression level of Bcl-2 were observed after ALS treatment, which suggests that mitochondrial pathway might be not involved in the ALS-induced apoptosis. Then, we found a significant increase in the expression level of RIP and the p-FADD/FADD ratio, which might initiate the death receptor signaling pathway. Consequently, caspase cascades was activated, including activated caspase-8 and cleaved caspase-3. Therefore, ALS induces apoptosis of Caco-2 cells via death receptor signaling pathway. Additionally, in comparison to previous studies on the apoptosis inducing effect of ALS, it showed that ALS induced mitochondria-dependent apoptosis cell death in gastric cancer cells [19], pancreatic cancer cells [21], osteosarcoma cells [22], breast cancer cells [44], and ovarian cancer cells [20], showing the most potent cancer cell killing effect in pancreatic cancer cell lines PANC-1 and BxPC-3 [21].
Autophagy is a cellular process of catabolic degradation in which damaged, dysfunctional, or superfluous organelles and proteins are sequestered, engulfed, and recycled to maintain cellular metabolism, viability and homeostasis [25]. Autophagy is generally induced by the deprivation of nutrient or stress. The mTOR kinase, which is activated by signaling pathway originating from growth factors and nutrient availability but inhibited in response to starvation, plays a critical role in regulating autophagy progression. Suppression of mTOR is required for induction of autophagy by limiting the inhibitory effect on the ULK1 kinase complex [47]. There are diverse signaling pathways implicated in the regulation of mTOR signaling, including positive regulation of mTOR (PI3K/Akt and p38 MAPK signaling) suppressing autophagy and negative regulation of mTOR (AMPK and p53 signaling) promoting autophagy [48,49,50]. The role of autophagy in tumorigenesis is controversial. Under certain circumstances, autophagy suppresses tumorigenesis by increasing programmed cell death [51]. However, in other cases, autophagy provides cancer cells with a rescue mechanism to sustain cell viability [52]. The present study showed a remarkable autophagy-inducing effect of ALS on HT29 and Caco-2 cells. The underlying mechanism of this autophagy-inducing effect may be ascribed to the inhibition of PI3K/Akt/mTOR pathway and activation of AMPK in both cell lines. Interestingly, there is a differential alteration in the modification of p38 MAPK signaling pathway. This phenomenon may be associated with the existence of four isoforms of p38 MAPK (p38α, p38β, p38γ, and p38δ), which differ in their tissue distribution profile, upstream regulators and downstream targets in a cell type- and stimulus-dependent manner in the mammals [49]. In addition, HT29 cells do not have mutations in the p53 gene, while Caco-2 cells have a mutated p53 gene without p53 expression. These different characteristics may also contribute to the differential alteration in the regulation of p38 MAPK signaling pathway. On the other hand, the previous studies showed that ALS inhibited PI3K/Akt/mTOR, p38 MAPK, or Erk1/2 signaling pathways while activating AMPK signaling pathway, contributing to the pro-autophagic effects of ALS in gastric cancer cells [19], pancreatic cancer cells [21], osteosarcoma cells [22], breast cancer cells [44], and ovarian cancer cells [19,20,21].
Furthermore, autophagy and apoptosis are highly conserved and tightly regulated processes that play essential roles in development, tissue homeostasis and disease [53]. Generally, the two biological processes involved in similar regulatory pathways and even share initiator and effector molecules, which indicates a perplexing crosstalk. Accumulating evidence suggests that autophagy and apoptosis can cooperate in a balanced interplay to allow cells to decide which route to take, thus influencing differentially the fate of the cell. Our study showed a crosstalk between apoptosis and autophagy by using rapamycin (a mTOR inhibitor and autophagy inducer), WM (a PI3K inhibitor and autophagy blocker), MK2206 (a selective inhibitor of Akt and autophagy inducer), and SB202190 (a selective p38 MAPK inhibitor and autophagy inducer). Similar regulatory effect of the autophagy inducer SB202190 on the ALS-induced apoptosis were observed, whereas differential influence of other chemical modulators on apoptosis and autophagy were present in both HT29 and Caco-2 cells. It can be speculated that several important molecules or pathways coordinated and mediated the complex interplay between autophagy and apoptosis, including TOR kinase pathway, p53, beclin 1, and Akt. Herein, ALS can induce apoptosis and autophagy in a coordinated manner in HT29 and Caco-2 cells.
Additionally, EMT is a cellular process in epithelial cells changing their adhesive repertoire, polarized arrange and cytoskeletal organization, and acquiring mesenchymal characteristics and migratory and invasive properties [54]. When it comes to cancer cells, EMT represents the conversion of fully differentiated epithelial cells into poorly differentiated and invasive mesenchymal cells [55]. EMT involves numerous distinct genetic and epigenetic alterations, including the decline in expression of epithelial markers, such as E-cadherin, ZO-1, claudins, occludins, β-catenin, and cytokeratins, and the elevation in expression of mesenchymal markers, such as N-cadherin, vimentin, TCF-8/ZEB-1, and slug [56]. The present study showed an increase in the expression level of E-cadherin and a decrease in the expression level of N-cadherin in HT29 and Caco-2 cells, with an elevated ratio of E-cadherin over N-cadherin, which demonstrate that the “cadherin switch” was closed and EMT was suppressed. We also found a significant alteration in the expression of ZO-1, TCF-8/ZEB-1, and slug. The down-regulation of epithelial cell-cell adhesion molecule E-cadherin and the up-regulation of mesenchymal cell-cell adhesion molecule N-cadherin expression, which is called the “cadherin switch”, is a major hallmark of EMT in cancer cells [57,58,59]. Taken together, the findings suggest that inhibitory effect on EMT contributing to the beneficial effects of ALS in HT29 and Caco-2 cells.
In conclusion, in the present study, we have explored the anticancer effect of ALS and the potential molecular mechanisms for its cancer cell killing effect in vitro. The mechanism of actions of ALS includes the inhibition of cell proliferation, cell cycle arrest, activation of the mitochondria-dependent and death receptor-dependent apoptosis, and induction of autophagy in human HT29 and Caco-2 cells. Suppression of PI3K/Akt/mTOR and activation of AMPK signaling pathways are involved in the autophagy-inducing effect of ALS in HT29 and Caco-2 cells. In addition, the inhibitory effect on EMT contributes to the anticancer activity of ALS (Figure 10). In aggregate, ALS may represent a new targeted therapeutic agent that can kill CRC cells. However, more studies are warranted to fully delineate the underlying anticancer mechanism and the interaction of other potential targets of ALS in the treatment of colorectal cancer.
Figure 10. Schematic mechanism underlies the cancer cell killing effect of ALS in HT29 and Caco-2 cells.
Figure 10. Schematic mechanism underlies the cancer cell killing effect of ALS in HT29 and Caco-2 cells.
Ijms 17 00041 g010

4. Materials and Methods

4.1. Chemicals and Reagents

ALS was bought from Selleckchem Inc. (Houston, TX, USA). DMSO, 13C6-l-lysine, l-lysine, 13C6,15N4-l-arginine, l-arginine, fetal bovine serum (FBS), dialyzed FBS, ammonium persulfate, propidium iodide (PI), ribonuclease (RNase A), protease and phosphatase inhibitor cocktails, MTT, bovine serum albumin, ethylenediaminetetraacetic acid (EDTA), and Dulbecco’s phosphate buffered saline (PBS) were sourced from Sigma-Aldrich (St Louis, MO, USA). FASP™ protein digestion kit was obtained from Protein Discovery Inc. (Knoxville, TN, USA). 8-well chamber slide was purchased from Lab-Tek® Inc. (Hatfield, PA, USA). Dulbecco’s Modified Eagle’s Medium (DMEM) were sourced from Corning Cellgro Inc. (Herndon, VA, USA). 4’,6-Diamidino-2-phenylindole (DAPI), 5-(and 6)-chloromethyl-2’,7’-dichlorodihydrofluorescein diacetate (CM-H2DCFDA), wortmannin (WM; a selective inhibitor of PI3K and a blocker of autophagosome formation), MK2206 (a selective inhibitor of Akt), and SB202190 (4-(4-fluorophenyl)-2-(4-hydroxyphenyl)-5-(4-pyridyl)-1H-imidazole; a selective inhibitor of p38 MAPK used as an autophagy inducer) were obtained from InvivoGen Inc. (San Diego, CA, USA). Pierce™ bicinchoninic acid (BCA) protein assay kit, skim milk, radioimmunoprecipitation assay (RIPA) buffer, and Western blotting substrate were bought from Thermo Fisher Scientific Inc. (Waltham, MA, USA). The annexin V:PE (phycoerythrin) apoptosis detection kit was obtained from BD Biosciences Inc. (San Jose, CA, USA). Cyto-ID® Autophagy detection kit was bought from Enzo Life Sciences Inc. (Farmingdale, NY, USA). Primary antibodies against human CDC2, phospho(p)-CDC2 (Tyr15), cyclin B1, p-cyclin B1 (Ser133), p-CDC25C (Ser216), p53, p21 Waf1/Cip1, Bax, Bcl-2, Bcl-xl, PUMA, cytochrome c, cleaved caspase 9, cleaved caspase 3, cleaved PARP, p-FADD (Ser194), FADD, RIP, p-PI3K (Tyr458), PI3K, p-p38 MAPK (Thr180/Tyr182), p38 MAPK, p-Akt (Ser473), Akt, p-mTOR (Ser2448), mTOR, beclin 1, and LC3-I/II were all purchased from Cell Signaling Technology Inc. (Beverly, MA, USA). The antibody against human β-actin was purchased from Santa Cruz Biotechnology Inc. (Dallas, TX, USA). The polyvinylidene difluoride (PVDF) membrane was bought from EMD Millipore Inc. (Billerica, MA, USA).

4.2. Cell Lines and Cell Culture

The HT29 and Caco-2 cells are two well-recognized CRC cell lines and were obtained from American Type Culture Collection (Manassas, VA, USA). These cells were maintained in DMEM supplemented with 10% heat-inactivated FBS and 1% penicillin/streptomycin in a 5% CO2/95% air humidified incubator at 37 °C. HT29 cells do not have mutations in the p53 gene, while Caco-2 cells have a mutated p53 gene without p53 expression. ALS was dissolved in DMSO at a stock concentration of 100 mM and stored at −20 °C. The drug was freshly diluted with the final concentration of DMSO at 0.05% (volume per volume (v/v)). The control cells received 0.05% DMSO only.
For proteomic analysis, HT29 and Caco-2 cells were cultured in DMEM for SILAC (Sigma-Aldrich) with (heavy) or without (light) stable isotope labeled amino acids (13C6-l-lysine and 13C6,15N4-l-arginine) and 10% dialyzed FBS. Cells were cultured in SILAC medium for six cell doubling times to achieve a high level (>98%) of labeled amino acid incorporation. Then, the cells were grown in “light” media were treated with 0.5% DMSO for 48 h to function as the negative control; cells grown in “heavy” media were treated with predetermined ALS for 48 h. All the experiments were performed three times independently. After ALS treatment, cell samples were harvested, lysated with hot lysis buffer (100 mM Tris base, 4% sodium dodecyl sulfate (SDS) and 100 mM dithiothreitol), and denatured for 5 min at 95 °C. Then, the samples were stored at −80 °C till further analysis.

4.3. Proteomic Response to ALS Treatment Analyzed by Stable Isotope Labeling by Amino Acids in Cell Culture (SILAC)-Based Approach

4.3.1. Digestion and Desalting SILAC Protein Samples

Prior to the quantitative proteomic analysis, the protein samples were subject to digestion and desalting which were performed using SILAC-based approach. Briefly, the thermal denatured cell lysate was sonicated, the supernatant was collected, and the protein concentration was determined. Subsequently, equal amount of heavy and light protein samples were combined to reach a total volume of 30–60 μL containing 300–600 μg protein. The combined samples were digested using FASP™ protein digestion kit according to the manufacturer’s instruction. After the digestion, the resultant sample was acidified to pH of 3 and desalted using a C18 solid-phase extraction column to desalt. The desalted samples were concentrated and resuspended in 0.1% formic acid prior to liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis.

4.3.2. LC-MS/MS and Statistical Analysis

The concentrated samples (5 μL) were subject to the hybrid linear ion trap-Orbitrap (LTQ Orbitrap XL, Thermo Scientific Inc., Hudson, NH, USA). Peptide SILAC ratio was calculated using MaxQuant version 1.2.0.13 (Max Planck Institute of Biochemistry, Munich, Germany). The SILAC ratio was determined by averaging all peptide SILAC ratios from peptides identified of the same protein.

4.3.3. Pathway and Network Analysis

The protein IDs were identified using Scaffold 4.3.2 from Proteome Software Inc. (Portland, OR, USA) and the pathway and network were analyzed using Ingenuity Pathway Analysis (IPA, www.ingenuity.com) from QIAGEN (Redwood City, CA, USA) as previously described [60].

4.4. Cell Viability Assay

The MTT assay was used to determine the effect of ALS on the viability of HT29 and Caco-2 cells. HT29 and Caco-2 cells were seeded into 96-well plates at a density of 6000 (Caco-2) or 8000 (HT29) cells/well. After cells were incubated for 24 h at a volume of 100 µL complete culture medium, the HT29 and Caco-2 cells were treated with ALS at concentrations ranging from 0.1 to 100 µM for 24 or 48 h. Following the ALS treatment, 10 µL of MTT stock solution (5 mg/mL) was added to each well and cultured for another 4 h. Then the solution was carefully aspirated and 100 µL of DMSO was added into each well. The plate was shaken for 10 min for crystal dissolution. Then the cell viability was examined by reduction of MTT. The absorbance was measured and the IC50 values were determined as previously described [61].

4.5. Cell Cycle Distribution Analysis

The effect of ALS on cell cycle distribution was tested using PI as a DNA stain to determine DNA content by flow cytometry as previously described [21]. In brief, HT29 and Caco-2 cells were seeded into 60 mm Petri dishes for attaching overnight. When the cells reached ~75% confluence and were then treated with ALS at concentrations of 0.1, 1, and 5 μM for 24 h. In separate experiments, HT29 and Caco-2 cells were treated with 1.0 μM ALS for 4, 8, 12, 24, 48, or 72 h. The collected cells were fixed and stained, then subject to flow cytometry. A total of 10,000 events were analyzed.

4.6. Quantification of Cellular Apoptosis

Following the examination of the effect of ALS on cell growth, the effect of ALS on cell apoptosis was determined and the percentage of apoptotic cells was quantified using the annexin V:PE apoptosis detection kit after the cells were treated with ALS at different concentrations (0.1, 1, and 5 μM) for 24 h. In separate experiments, cells were treated with 1 μM ALS for 4, 8, 12, 24, 48, or 72 h as previously described [61].

4.7. Quantification of Cellular Autophagy

To determine the effect of ALS on autophagy in HT29 and Caco-2 cells, cellular autophagy was examined using flow cytometry. Briefly, HT29 and Caco-2 cells were seeded into 60 mm Petri dishes for incubation overnight. The cells were treated with ALS at 0.1, 1, and 5 μM for 24 h when they reached ~75% confluence. Also, in separate experiments, HT29 and Caco-2 cells were treated with 1.0 μM ALS for 4, 8, 12, 24, 48, or 72 h as previously described [61].

4.8. Simultaneous Determination of Apoptosis and Autophagy Using Flow Cytometry

We further examined the two modes of programmed cell death simultaneously in order to investigate the potential crosstalk between ALS-induced apoptosis and autophagy. HT29 and Caco-2 cells were seeded into 60 mm Petri dishes. After incubation overnight, cells were pretreated with 10 μM WM (a PI3K inhibitor and autophagy blocker), 1 μM rapamycin (an mTOR inhibitor and autophagy inducer), 10 μM SB202190 (a selective inhibitor of p38 MAPK) or 1 μM MK2206 (a selective inhibitor of Akt) for 1 h, then co-treated with 5 μM ALS for further 24 h. At the end of treatment, the cells were trypsinized and centrifuged at 250× g for 5 min. The cells were divided into two samples of equal volume for detection of apoptosis and autophagy respectively. The subsequent steps follow the procedure mentioned above.

4.9. Confocal Fluorescence Microscopy

To further examine the cellular autophagy level, confocal microscopic examination was performed using a Cyto-ID® autophagy detection kit as previously described [61]. Briefly, HT29 and Caco-2 cells were seeded into an 8-well chamber slide at 30% confluence. The cells were treated with ALS at 0.1, 1, and 5 µM for 24 h. Next, cells were incubated with 100 µL of dual detection reagents and examined using a TCS SP2 laser scanning confocal microscope (Leica, Wetzlar, Germany) at wavelengths of 405/488 nm.

4.10. Western Blotting Analysis

Western blotting assays were used to examine the expression level of key regulators involved in cell cycle, apoptosis, autophagy, and EMT processes as previously described [61]. Briefly, HT29 and Caco-2 cells were collected and lysed after 48-h treatment with ALS at 0.1, 1, and 5 μM. The supernatant was collected and the protein concentrations were measured using a Pierce™ BCA protein assay kit. Thirty microgram proteins were subjected to Western blotting assay. Visualization was performed using an enhanced chemiluminescence kit (Thermal Scientific, Waltham, MA, USA) and the blots were analyzed using Image Lab 3.0 (BioRad, Hercules, CA, USA). Protein expression level was normalized to the matching densitometric value of the internal control β-actin.

4.11. Statistical Analysis

Data are expressed as the mean ± standard deviation (SD). Multiple comparisons were assessed by one-way analysis of variance (ANOVA) followed by Tukey’s multiple comparison procedure. p < 0.05 was considered statistically significant. All the assays were performed in triplicate.

Supplementary Materials

Supplementary materials can be found at https://0-www-mdpi-com.brum.beds.ac.uk/1422-0067/17/1/41/s1.

Acknowledgments

The authors appreciate the financial support from the Startup Fund of the College of Pharmacy, University of South Florida, Tampa, Florida 33612, USA. Zhi-Wei Zhou is a holder of a postdoctoral scholarship from the College of Pharmacy, University of South Florida, Tampa, Florida 33612, USA.

Author Contributions

Bao-Jun Ren, Zhi-Wei Zhou, and Shu-Feng Zhou conceived and designed the experiments; Bao-Jun Ren performed the experiments; Da-Jian Zhu, Yong-Le Ju, Jin-Hao Wu, and Man-Zhao Ouyang analyzed the data; Xiao-Wu Chen and Shu-Feng Zhou contributed reagents/materials/analysis tools; Zhi-Wei Zhou and Shu-Feng Zhou wrote the paper.

Conflicts of Interest

The authors declare no conflict of interest.

References

  1. Torre, L.A.; Bray, F.; Siegel, R.L.; Ferlay, J.; Lortet-Tieulent, J.; Jemal, A. Global cancer statistics, 2012. Cancer J. Clin. 2015, 65, 87–108. [Google Scholar] [CrossRef] [PubMed]
  2. Siegel, R.; Desantis, C.; Jemal, A. Colorectal cancer statistics, 2014. Cancer J. Clin. 2014, 64, 104–117. [Google Scholar] [CrossRef] [PubMed]
  3. Chen, W.; Zheng, R.; Zeng, H.; Zhang, S.; He, J. Annual report on status of cancer in China, 2011. Chin. J. Cancer Res. 2015, 27, 2–12. [Google Scholar] [CrossRef] [PubMed]
  4. Society, A.C. Cancer facts and figures. Available online: http://www.cancer.org/acs/groups/content/@epidemiologysurveilance/documents/document/acspc-036845.pdf (accessed on 16 May 2013).
  5. Chu, E. An update on the current and emerging targeted agents in metastatic colorectal cancer. Clin. Colorectal Cancer 2012, 11, 1–13. [Google Scholar] [CrossRef] [PubMed]
  6. Lombardi, L.; Morelli, F.; Cinieri, S.; Santini, D.; Silvestris, N.; Fazio, N.; Orlando, L.; Tonini, G.; Colucci, G.; Maiello, E. Adjuvant colon cancer chemotherapy: Where we are and where we’ll go. Cancer Treat. Rev. 2010, 36 (Suppl. 3), S34–S41. [Google Scholar] [CrossRef]
  7. Troiani, T.; Martinelli, E.; Orditura, M.; de Vita, F.; Ciardiello, F.; Morgillo, F. Beyond bevacizumab: New anti-VEGF strategies in colorectal cancer. Expert Opin. Investig. Drugs 2012, 21, 949–959. [Google Scholar] [CrossRef] [PubMed]
  8. Nigg, E.A. Mitotic kinases as regulators of cell division and its checkpoints. Nat. Rev. Mol. Cell Biol. 2001, 2, 21–32. [Google Scholar] [CrossRef] [PubMed]
  9. Bolanos-Garcia, V.M. Aurora kinases. Int. J. Biochem. Cell Biol. 2005, 37, 1572–1577. [Google Scholar] [CrossRef] [PubMed]
  10. Gautschi, O.; Heighway, J.; Mack, P.C.; Purnell, P.R.; Lara, P.N., Jr.; Gandara, D.R. Aurora kinases as anticancer drug targets. Clin. Cancer Res. 2008, 14, 1639–1648. [Google Scholar] [CrossRef] [PubMed]
  11. Dotan, E.; Meropol, N.J.; Zhu, F.; Zambito, F.; Bove, B.; Cai, K.Q.; Godwin, A.K.; Golemis, E.A.; Astsaturov, I.; Cohen, S.J. Relationship of increased aurora kinase A gene copy number, prognosis and response to chemotherapy in patients with metastatic colorectal cancer. Br. J. Cancer 2012, 106, 748–755. [Google Scholar] [CrossRef] [PubMed]
  12. Baba, Y.; Nosho, K.; Shima, K.; Irahara, N.; Kure, S.; Toyoda, S.; Kirkner, G.J.; Goel, A.; Fuchs, C.S.; Ogino, S. Aurora-A expression is independently associated with chromosomal instability in colorectal cancer. Neoplasia 2009, 11, 418–425. [Google Scholar] [CrossRef] [PubMed]
  13. Goos, J.A.; Coupe, V.M.; Diosdado, B.; Delis-Van Diemen, P.M.; Karga, C.; Belien, J.A.; Carvalho, B.; van den Tol, M.P.; Verheul, H.M.; Geldof, A.A.; et al. Aurora kinase A (AURKA) expression in colorectal cancer liver metastasis is associated with poor prognosis. Br. J. Cancer 2013, 109, 2445–2452. [Google Scholar] [CrossRef] [PubMed]
  14. Cammareri, P.; Scopelliti, A.; Todaro, M.; Eterno, V.; Francescangeli, F.; Moyer, M.P.; Agrusa, A.; Dieli, F.; Zeuner, A.; Stassi, G. Aurora-a is essential for the tumorigenic capacity and chemoresistance of colorectal cancer stem cells. Cancer Res. 2010, 70, 4655–4665. [Google Scholar] [CrossRef] [PubMed]
  15. Boss, D.S.; Beijnen, J.H.; Schellens, J.H. Clinical experience with aurora kinase inhibitors: A review. Oncologist 2009, 14, 780–793. [Google Scholar] [CrossRef] [PubMed]
  16. Hong, X.; O’Donnell, J.P.; Salazar, C.R.; van Brocklyn, J.R.; Barnett, K.D.; Pearl, D.K.; deCarvalho, A.C.; Ecsedy, J.A.; Brown, S.L.; Mikkelsen, T.; et al. The selective Aurora-A kinase inhibitor MLN8237 (alisertib) potently inhibits proliferation of glioblastoma neurosphere tumor stem-like cells and potentiates the effects of temozolomide and ionizing radiation. Cancer Chemother. Pharmacol. 2014, 73, 983–990. [Google Scholar] [CrossRef] [PubMed]
  17. Zhou, N.; Singh, K.; Mir, M.C.; Parker, Y.; Lindner, D.; Dreicer, R.; Ecsedy, J.A.; Zhang, Z.; Teh, B.T.; Almasan, A.; et al. The investigational Aurora kinase A inhibitor MLN8237 induces defects in cell viability and cell-cycle progression in malignant bladder cancer cells in vitro and in vivo. Clin. Cancer Res. 2013, 19, 1717–1728. [Google Scholar] [CrossRef] [PubMed]
  18. Sehdev, V.; Peng, D.; Soutto, M.; Washington, M.K.; Revetta, F.; Ecsedy, J.; Zaika, A.; Rau, T.T.; Schneider-Stock, R.; Belkhiri, A.; et al. The Aurora kinase A inhibitor MLN8237 enhances cisplatin-induced cell death in esophageal adenocarcinoma cells. Mol. Cancer Ther. 2012, 11, 763–774. [Google Scholar] [CrossRef] [PubMed]
  19. Yuan, C.X.; Zhou, Z.W.; Yang, Y.X.; He, Z.X.; Zhang, X.; Wang, D.; Yang, T.; Wang, N.J.; Zhao, R.J.; Zhou, S.F. Inhibition of mitotic Aurora kinase A by alisertib induces apoptosis and autophagy of human gastric cancer AGS and NCI-N78 cells. Drug Des. Dev. Ther. 2015, 9, 487–508. [Google Scholar]
  20. Ding, Y.H.; Zhou, Z.W.; Ha, C.F.; Zhang, X.Y.; Pan, S.T.; He, Z.X.; Edelman, J.L.; Wang, D.; Yang, Y.X.; Zhang, X.; et al. Alisertib, an Aurora kinase A inhibitor, induces apoptosis and autophagy but inhibits epithelial to mesenchymal transition in human epithelial ovarian cancer cells. Drug Des. Dev. Ther. 2015, 9, 425–464. [Google Scholar]
  21. Wang, F.; Li, H.; Yan, X.G.; Zhou, Z.W.; Yi, Z.G.; He, Z.X.; Pan, S.T.; Yang, Y.X.; Wang, Z.Z.; Zhang, X.; et al. Alisertib induces cell cycle arrest and autophagy and suppresses epithelial-to-mesenchymal transition involving PI3K/Akt/mTOR and sirtuin 1-mediated signaling pathways in human pancreatic cancer cells. Drug Des. Dev. Ther. 2015, 9, 575–601. [Google Scholar]
  22. Niu, N.K.; Wang, Z.L.; Pan, S.T.; Ding, H.Q.; Au, G.H.; He, Z.X.; Zhou, Z.W.; Xiao, G.; Yang, Y.X.; Zhang, X.; et al. Pro-apoptotic and pro-autophagic effects of the Aurora kinase A inhibitor alisertib (MLN8237) on human osteosarcoma U-2 OS and MG-63 cells through the activation of mitochondria-mediated pathway and inhibition of p38 MAPK/PI3K/Akt/mTOR signaling pathway. Drug Des. Dev. Ther. 2015, 9, 1555–1584. [Google Scholar]
  23. Gorgun, G.; Calabrese, E.; Hideshima, T.; Ecsedy, J.; Perrone, G.; Mani, M.; Ikeda, H.; Bianchi, G.; Hu, Y.; Cirstea, D.; et al. A novel Aurora-A kinase inhibitor MLN8237 induces cytotoxicity and cell-cycle arrest in multiple myeloma. Blood 2010, 115, 5202–5213. [Google Scholar] [CrossRef] [PubMed]
  24. Cantley, L.C. The phosphoinositide 3-kinase pathway. Science 2002, 296, 1655–1657. [Google Scholar] [CrossRef] [PubMed]
  25. Klionsky, D.J.; Emr, S.D. Autophagy as a regulated pathway of cellular degradation. Science 2000, 290, 1717–1721. [Google Scholar] [CrossRef] [PubMed]
  26. Kim, J.; Klionsky, D.J. Autophagy, cytoplasm-to-vacuole targeting pathway, and pexophagy in yeast and mammalian cells. Annu. Rev. Biochem. 2000, 69, 303–342. [Google Scholar] [CrossRef] [PubMed]
  27. Manning, B.D.; Cantley, L.C. AKT/PKB signaling: Navigating downstream. Cell 2007, 129, 1261–1274. [Google Scholar] [CrossRef] [PubMed]
  28. Heras-Sandoval, D.; Perez-Rojas, J.M.; Hernandez-Damian, J.; Pedraza-Chaverri, J. The role of PI3K/AKT/mTOR pathway in the modulation of autophagy and the clearance of protein aggregates in neurodegeneration. Cell Signal. 2014, 26, 2694–2701. [Google Scholar] [CrossRef] [PubMed]
  29. Lozy, F.; Karantza, V. Autophagy and cancer cell metabolism. Semin. Cell Dev. Biol. 2012, 23, 395–401. [Google Scholar] [CrossRef] [PubMed]
  30. Mester, J.; Eng, C. When overgrowth bumps into cancer: The PTEN-opathies. Am. J. Med. Genet. Part C Semin. Med. Genet. 2013, 163C, 114–121. [Google Scholar] [CrossRef] [PubMed]
  31. Shin, K.; Fogg, V.C.; Margolis, B. Tight junctions and cell polarity. Annu. Rev. Cell Dev. Biol. 2006, 22, 207–235. [Google Scholar] [CrossRef] [PubMed]
  32. Heerboth, S.; Housman, G.; Leary, M.; Longacre, M.; Byler, S.; Lapinska, K.; Willbanks, A.; Sarkar, S. EMT and tumor metastasis. Clin. Transl. Med. 2015, 4, 6. [Google Scholar] [CrossRef] [PubMed]
  33. Derksen, P.W.; Liu, X.; Saridin, F.; van der Gulden, H.; Zevenhoven, J.; Evers, B.; van Beijnum, J.R.; Griffioen, A.W.; Vink, J.; Krimpenfort, P.; et al. Somatic inactivation of E-cadherin and p53 in mice leads to metastatic lobular mammary carcinoma through induction of anoikis resistance and angiogenesis. Cancer Cell 2006, 10, 437–449. [Google Scholar] [CrossRef] [PubMed]
  34. Nauseef, J.T.; Henry, M.D. Epithelial-to-mesenchymal transition in prostate cancer: Paradigm or puzzle? Nat. Rev. Urol. 2011, 8, 428–439. [Google Scholar] [CrossRef] [PubMed]
  35. Polette, M.; Mestdagt, M.; Bindels, S.; Nawrocki-Raby, B.; Hunziker, W.; Foidart, J.M.; Birembaut, P.; Gilles, C. β-catenin and ZO-1: Shuttle molecules involved in tumor invasion-associated epithelial-mesenchymal transition processes. Cells Tissues Organs 2007, 185, 61–65. [Google Scholar] [CrossRef] [PubMed]
  36. Ferlay, J.; Steliarova-Foucher, E.; Lortet-Tieulent, J.; Rosso, S.; Coebergh, J.W.; Comber, H.; Forman, D.; Bray, F. Cancer incidence and mortality patterns in Europe: Estimates for 40 countries in 2012. Eur. J. Cancer 2013, 49, 1374–1403. [Google Scholar] [CrossRef] [PubMed]
  37. D'Assoro, A.B.; Liu, T.; Quatraro, C.; Amato, A.; Opyrchal, M.; Leontovich, A.; Ikeda, Y.; Ohmine, S.; Lingle, W.; Suman, V.; et al. The mitotic kinase Aurora—A promotes distant metastases by inducing epithelial-to-mesenchymal transition in ERα+ breast cancer cells. Oncogene 2014, 33, 599–610. [Google Scholar] [CrossRef] [PubMed]
  38. Chen, S.S.; Chang, P.C.; Cheng, Y.W.; Tang, F.M.; Lin, Y.S. Suppression of the STK15 oncogenic activity requires a transactivation-independent p53 function. EMBO J. 2002, 21, 4491–4499. [Google Scholar] [CrossRef] [PubMed]
  39. Macurek, L.; Lindqvist, A.; Medema, R.H. Aurora-A and hBora join the game of Polo. Cancer Res. 2009, 69, 4555–4558. [Google Scholar] [CrossRef] [PubMed]
  40. Hunter, T. Protein kinases and phosphatases: The yin and yang of protein phosphorylation and signaling. Cell 1995, 80, 225–236. [Google Scholar] [CrossRef]
  41. Chow, J.P.; Siu, W.Y.; Ho, H.T.; Ma, K.H.; Ho, C.C.; Poon, R.Y. Differential contribution of inhibitory phosphorylation of CDC2 and CDK2 for unperturbed cell cycle control and DNA integrity checkpoints. J. Biol. Chem. 2003, 278, 40815–40828. [Google Scholar] [CrossRef] [PubMed]
  42. Tyagi, A.; Singh, R.P.; Agarwal, C.; Siriwardana, S.; Sclafani, R.A.; Agarwal, R. Resveratrol causes CDC2-tyr15 phosphorylation via ATM/ATR-Chk1/2-CDC25C pathway as a central mechanism for S phase arrest in human ovarian carcinoma Ovcar-3 cells. Carcinogenesis 2005, 26, 1978–1987. [Google Scholar] [CrossRef] [PubMed]
  43. Yuan, J.; Eckerdt, F.; Bereiter-Hahn, J.; Kurunci-Csacsko, E.; Kaufmann, M.; Strebhardt, K. Cooperative phosphorylation including the activity of polo-like kinase 1 regulates the subcellular localization of cyclin B1. Oncogene 2002, 21, 8282–8292. [Google Scholar] [CrossRef] [PubMed]
  44. Li, J.P.; Yang, Y.X.; Liu, Q.L.; Pan, S.T.; He, Z.X.; Zhang, X.; Yang, T.; Chen, X.W.; Wang, D.; Qiu, J.X.; et al. The investigational Aurora kinase A inhibitor alisertib (MLN8237) induces cell cycle G2/M arrest, apoptosis, and autophagy via p38 MAPK and Akt/mTOR signaling pathways in human breast cancer cells. Drug Des. Dev. Ther. 2015, 9, 1627–1652. [Google Scholar]
  45. Danial, N.N.; Korsmeyer, S.J. Cell death: Critical control points. Cell 2004, 116, 205–219. [Google Scholar] [CrossRef]
  46. Chinnaiyan, A.M.; O’Rourke, K.; Tewari, M.; Dixit, V.M. FADD, a novel death domain-containing protein, interacts with the death domain of fas and initiates apoptosis. Cell 1995, 81, 505–512. [Google Scholar] [CrossRef]
  47. Jung, C.H.; Ro, S.H.; Cao, J.; Otto, N.M.; Kim, D.H. mTOR regulation of autophagy. FEBS Lett. 2010, 584, 1287–1295. [Google Scholar] [CrossRef] [PubMed]
  48. Alers, S.; Loffler, A.S.; Wesselborg, S.; Stork, B. Role of AMPK-mTOR-Ulk1/2 in the regulation of autophagy: cross talk, shortcuts, and feedbacks. Mol. Cell. Biol. 2012, 32, 2–11. [Google Scholar] [CrossRef] [PubMed]
  49. Tang, G.; Yue, Z.; Talloczy, Z.; Hagemann, T.; Cho, W.; Messing, A.; Sulzer, D.L.; Goldman, J.E. Autophagy induced by Alexander disease-mutant GFAP accumulation is regulated by p38/MAPK and mTOR signaling pathways. Hum. Mol. Genet. 2008, 17, 1540–1555. [Google Scholar] [CrossRef] [PubMed]
  50. Mizushima, N.; Komatsu, M. Autophagy: Renovation of cells and tissues. Cell 2011, 147, 728–741. [Google Scholar] [CrossRef] [PubMed]
  51. Mathew, R.; Kongara, S.; Beaudoin, B.; Karp, C.M.; Bray, K.; Degenhardt, K.; Chen, G.; Jin, S.; White, E. Autophagy suppresses tumor progression by limiting chromosomal instability. Genes Dev. 2007, 21, 1367–1381. [Google Scholar] [CrossRef] [PubMed]
  52. Lum, J.J.; Bauer, D.E.; Kong, M.; Harris, M.H.; Li, C.; Lindsten, T.; Thompson, C.B. Growth factor regulation of autophagy and cell survival in the absence of apoptosis. Cell 2005, 120, 237–248. [Google Scholar] [CrossRef] [PubMed]
  53. El-Khattouti, A.; Selimovic, D.; Haikel, Y.; Hassan, M. Crosstalk between apoptosis and autophagy: Molecular mechanisms and therapeutic strategies in cancer. J. Cell Death 2013, 6, 37–55. [Google Scholar] [PubMed]
  54. Kalluri, R.; Weinberg, R.A. The basics of epithelial-mesenchymal transition. J. Clin. Investig. 2009, 119, 1420–1428. [Google Scholar] [CrossRef] [PubMed]
  55. Nieto, M.A. The ins and outs of the epithelial to mesenchymal transition in health and disease. Annu. Rev. Cell Dev. Biol. 2011, 27, 347–376. [Google Scholar] [CrossRef] [PubMed]
  56. Thiery, J.P.; Sleeman, J.P. Complex networks orchestrate epithelial-mesenchymal transitions. Nat. Rev. Mol. Cell Biol. 2006, 7, 131–142. [Google Scholar] [CrossRef] [PubMed]
  57. Hulit, J.; Suyama, K.; Chung, S.; Keren, R.; Agiostratidou, G.; Shan, W.; Dong, X.; Williams, T.M.; Lisanti, M.P.; Knudsen, K.; et al. N-cadherin signaling potentiates mammary tumor metastasis via enhanced extracellular signal-regulated kinase activation. Cancer Res. 2007, 67, 3106–3116. [Google Scholar] [CrossRef] [PubMed]
  58. Lehembre, F.; Yilmaz, M.; Wicki, A.; Schomber, T.; Strittmatter, K.; Ziegler, D.; Kren, A.; Went, P.; Derksen, P.W.; Berns, A.; et al. NCAM-induced focal adhesion assembly: A functional switch upon loss of E-cadherin. EMBO J. 2008, 27, 2603–2615. [Google Scholar] [CrossRef] [PubMed]
  59. Aigner, K.; Dampier, B.; Descovich, L.; Mikula, M.; Sultan, A.; Schreiber, M.; Mikulits, W.; Brabletz, T.; Strand, D.; Obrist, P.; et al. The transcription factor ZEB1 (dEF1) promotes tumour cell dedifferentiation by repressing master regulators of epithelial polarity. Oncogene 2007, 26, 6979–6988. [Google Scholar] [CrossRef] [PubMed]
  60. Harel, M.; Oren-Giladi, P.; Kaidar-Person, O.; Shaked, Y.; Geiger, T. Proteomics of microparticles with SILAC Quantification (PROMIS-Quan): A novel proteomic method for plasma biomarker quantification. Mol. Cell. Proteom. 2015, 14, 1127–1136. [Google Scholar] [CrossRef] [PubMed]
  61. Zhou, Z.W.; Li, X.X.; He, Z.X.; Pan, S.T.; Yang, Y.; Zhang, X.; Chow, K.; Yang, T.; Qiu, J.X.; Zhou, Q.; et al. Induction of apoptosis and autophagy via sirtuin1- and PI3K/Akt/mTOR-mediated pathways by plumbagin in human prostate cancer cells. Drug Des. Dev. Ther. 2015, 9, 1511–1554. [Google Scholar] [CrossRef] [PubMed]

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MDPI and ACS Style

Ren, B.-J.; Zhou, Z.-W.; Zhu, D.-J.; Ju, Y.-L.; Wu, J.-H.; Ouyang, M.-Z.; Chen, X.-W.; Zhou, S.-F. Alisertib Induces Cell Cycle Arrest, Apoptosis, Autophagy and Suppresses EMT in HT29 and Caco-2 Cells. Int. J. Mol. Sci. 2016, 17, 41. https://0-doi-org.brum.beds.ac.uk/10.3390/ijms17010041

AMA Style

Ren B-J, Zhou Z-W, Zhu D-J, Ju Y-L, Wu J-H, Ouyang M-Z, Chen X-W, Zhou S-F. Alisertib Induces Cell Cycle Arrest, Apoptosis, Autophagy and Suppresses EMT in HT29 and Caco-2 Cells. International Journal of Molecular Sciences. 2016; 17(1):41. https://0-doi-org.brum.beds.ac.uk/10.3390/ijms17010041

Chicago/Turabian Style

Ren, Bao-Jun, Zhi-Wei Zhou, Da-Jian Zhu, Yong-Le Ju, Jin-Hao Wu, Man-Zhao Ouyang, Xiao-Wu Chen, and Shu-Feng Zhou. 2016. "Alisertib Induces Cell Cycle Arrest, Apoptosis, Autophagy and Suppresses EMT in HT29 and Caco-2 Cells" International Journal of Molecular Sciences 17, no. 1: 41. https://0-doi-org.brum.beds.ac.uk/10.3390/ijms17010041

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