Open Access

Identification of lncRNAs by microarray analysis reveals the potential role of lncRNAs in cervical cancer pathogenesis

  • Authors:
    • Jiaming Huang
    • Tianyu Liu
    • Chunliang Shang
    • Yunhe Zhao
    • Wei Wang
    • Yanchun Liang
    • Luyan Guo
    • Shuzhong Yao
  • View Affiliations

  • Published online on: February 13, 2018     https://doi.org/10.3892/ol.2018.8037
  • Pages: 5584-5592
  • Copyright: © Huang et al. This is an open access article distributed under the terms of Creative Commons Attribution License.

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Abstract

Long non-coding RNAs (lncRNAs) have been acknowledged to serve a significant role in cancer biology and abnormal expression in tumors is frequently observed. However, their mechanisms in cervical cancer remain unclear. With a genome‑wide analysis of lncRNA expression in cervical cancer tissues, the present study aimed to identify lncRNA targets for the further study of cervical cancer. To elucidate the specific role of lncRNAs in the pathogenesis of this type of cancer, 6 cervical cancer samples paired with normal cervical tissues were obtained. Expression profiles of lncRNAs and mRNAs were constructed through microarray analysis and confirmed by reverse transcription-quantitative polymerase chain reaction (RT‑qPCR) methods. Gene Ontology and pathway enrichment analyses were performed with computational methods. On the basis of correlations between the differential expression levels of lncRNAs and mRNAs, a coding‑non‑coding gene co‑expression network (CNC network) was established. The differential expression of 5,844 lncRNAs and 4,436 mRNAs were discovered in cervical cancer samples compared with normal cervical tissues. Among the differentially expressed lncRNAs, 14 were chosen at random and validated by RT‑qPCR; the majority of the results measured were consistent with the microarray results. Furthermore, the lncRNA ENST00000551152 was found to be upregulated and TCO. NS_00001368 lncRNA was downregulated in cervical cancer cell lines. The CNC network included 592 network nodes and 934 associations between 12 lncRNAs and 580 protein‑coding genes, indicating that one lncRNA could act on a maximum of 141 coding genes, and that one coding gene may corresponded with a maximum of 5 lncRNAs. Overall, the present study has provided a complete expression profile of lncRNAs and mRNAs in cervical cancer, which may now be used to establish a solid foundation for cervical cancer research. These results may provide significant information for improving the understanding of the pathogenesis of cervical cancer and indicate potential therapeutic targets.

Introduction

Cervical cancer is the most common type of malignant neoplasm in the female reproductive system and ranks as the second most common cause of gynecological cancer-associated mortality, with 47,130 new cases and 8,010 mortalities reported in the United States in 2014 (1). Despite decreases in the incidence and mortality rates of cervical cancer, which are largely due to progress in surgical treatment (2) radiotherapy (3) and chemotherapy (4), cervical cancer remains a substantial threat to women's health globally (5). It has been hypothesized that the carcinogenesis and development of cervical cancer are associated with sexual behavior, childbirth, persistent human papillomavirus (HPV) infection and smoking (6). Extensive efforts have been made to clarify the genetic and epigenetic mechanisms that underlie the growth and invasion of cervical cancer. However, the pathogenesis remains understood. Pelvic lymph node metastasis may serve as an independent prognostic factor (7); however, the lack of specific tumor markers for the prediction of cervical cancer mortality and invasion has yet to be resolved.

Long non-coding RNA (lncRNA) is defined as RNA of >200 nucleotides without protein-coding function. It has been reported that the portion of the human genome that encodes proteins may be <2% (8). A growing number of lncRNAs have been recognized as key regulators, rather than simply transcriptional noise. They are associated with various biological processes, including genomic imprinting, X chromosome inactivation, chromatin modification, transcription interference, transcription activation and nuclear transport (810). lncRNAs are one of the most highly expressed classes of non-coding RNAs in human cervical tissue, and their relevance to cervical cancer is steadily becoming more apparent (11). A previous study demonstrated that lncRNA expression levels differ, with statistical significance, between three cervical intraepithelial neoplasia grades, indicating that these transcripts may be involved in the development and progression of pre-cancerous lesions (12). Studies on this topic have revealed that aberrant expression of certain lncRNAs, including HOX transcript antisense RNA (HOTAIR), metastasis-associated lung adenocarcinoma transcript 1, cervical carcinoma-expressed PCNA regulatory lncRNA, lncRNA-EBIC (also known as thymopoietin pseudogene 2), growth arrest-specific 5, and lncRNA-LET (also known as NPTN intronic transcript 1), serves critical roles in cervical cancer development, invasion and metastasis (1318). However, none of these lncRNAs has been applied as biomarker for clinical diagnosis. Furthermore, the precise function of the majority of lncRNAs remains unknown despite extensive research efforts. Thus, there is an urgent requirement to identify the mechanisms of interaction between lncRNAs and coding genes.

In the present study, a high-throughput microarray was employed to analyze lncRNA and mRNA expression profiles in samples of cancerous and normal cervical tissue. Gene Ontology (GO) and pathway enrichment analyses investigated enriched functions of the predicted targets, allowing the establishment of an lncRNA-mRNA correlation network. The results illustrated that differences in the expression levels of lncRNAs, in addition to mRNAs, may be associated with cervical cancer pathogenesis; the comprehensive analysis of lncRNAs and mRNA may lay a foundation for further investigation in the diagnosis and treatment of cervical cancer.

Materials and methods

Patient specimens and RNA extraction

A total of 6 cervical carcinoma samples and 6 normal cervical tissues were collected for microarray. The 6 cervical carcinoma samples were labeled C1 and C3-7, C2 was diagnosed cervical carcinoma in situ and was not suitable for microarray. For validation, another 20 normal and 30 cancerous cervical tissue samples were also selected. The number of cervical cancer tissues was subsequently increased to 60 for the study of the association between ENST00000551152 expression and clinicopathological parameters. Patient characteristics are summarized in Table I. All the tissue samples were obtained between January 2014 to January 2015 from the Department of Gynecology, First Affiliated Hospital of Sun Yat-sen University (Guangzhou, China). Samples were selected based on the diagnosis of cervical cancer, determined by at least two pathologists and no patients had received chemotherapy or radiotherapy prior to surgery. All provided written, informed consent. The present study was approved by the Medical Ethics Committees at the First Affiliated Hospital of Sun Yat-sen University. All samples were stored at −80°C until RNA extraction.

Table I.

Correlation between ENST00000551152 expression and clinicopathological characteristics in early-stage squamous cervical cancer.

Table I.

Correlation between ENST00000551152 expression and clinicopathological characteristics in early-stage squamous cervical cancer.

ENST00000551152 expression, n (%)

CharacteristicAll patients, nLowHighP-value
Total6014 (23.3)46 (76.7)
Age, years 0.297
  ≤42336 (18.2)27 (81.8)
  >42278 (29.6)19 (70.4)
FIGO stage 0.017a
  IB12912 (41.4)17 (58.6)
  IB2  81 (12.5)7 (87.5)
  IIA1171 (5.9)16 (94.1)
  IIA2  60 (0.0)6 (100.0)
Tumor size, cm 0.022a
  ≤43913 (33.3)26 (66.7)
  >4211 (4.8)20 (95.2)
Differentiation grade 0.056
  Well-differentiated  74 (57.1)3 (42.9)
  Moderately differentiated256 (24.0)19 (76.0)
  Poorly differentiated284 (14.3)24 (85.7)
Extent of stromal invasion 0.001
  <1/22912 (41.4)17 (58.6)
  ≥1/2312 (6.5)29 (93.5)
LVSI 0.053a
  Yes110 (0.0)11 (100.0)
  No4914 (28.6)35 (71.4)
PLNM 0.026a
  Yes140 (0.0)14 (100.0)
  No4614 (30.4)32 (69.6)
SCC antigen, ng/ml 0.004
  <1.52711 (40.7)16 (59.3)
  ≥1.5333 (9.1)30 (90.9)

a P-value calculated using Fisher's exact test. All other P-values were calculated using χ2 test. FIGO, International Federation of Gynecology and Obstetrics; LVSI, lymphovascular space invasion; PLNM, pelvic lymph node metastasis; SCC, squamous cell carcinoma.

Extraction of total RNA from fresh tissues was performed using RNAiso Plus reagent (Takara Biotechnology Co., Ltd., Dalian, China) and the total RNA content of each sample was quantified using a NanoDrop ND-1000 (Thermo Fisher Scientific, Inc., Wilmington, DE, USA). Standard denaturing agarose gel electrophoresis was performed to evaluate the RNA integrity.

RNA labeling and array hybridization

Following the Agilent One-Color Microarray-Based Gene Expression Analysis protocol (Agilent Technologies, Inc., Santa Clara, CA, USA), sample labeling and array hybridization were implemented in the 6 cancer tissues and 6 normal cervical tissues. Ribosomal RNA was removed to leave purified mRNA using an mRNA-ONLY™ Eukaryotic mRNA Isolation Kit (Epicentre; Illumina, Inc., San Diego, CA, USA). The entire lengths of the transcripts were transcribed into fluorescent complementary RNA (cRNA) without 3′ bias by using random priming. The labeled cRNA was then purified with an RNeasy Mini Kit (Qiagen China Co., Ltd, Shanghai, China). A mixture containing 5 µl 10X blocking agent, 1 µg 25X fragmentation buffer and 1 µg of each labeled cRNA sample was fragmented and then heated for 30 min at 60°C. To dilute the labeled cRNA, 25 µl 2X GE Hybridization buffer (GE Healthcare Life Sciences, Logan, UT, USA) was added. After dispensing into the gasket slide, 50 µl of hybridization solution was applied to the lncRNA expression microarray slide. Incubation of the slides was performed in an Agilent hybridization oven at 65°C for 17 h (Agilent Technologies, Inc.). Washing, fixing and scanning of the hybridized arrays were completed with the Agilent DNA microarray scanner (part no. G25005C).

Data analysis of lncRNA and mRNA expression profiles

The general profiles of human lncRNAs and protein-coding transcripts from the 6 cervical carcinoma samples and 6 normal cervical tissues were detected using the Arraystar Human lncRNA Microarray V3.0 (Arraystar, Inc., Rockville, MD, USA); using this array, ~26,109 coding transcripts and 30,586 lncRNAs are detectable. Array images were analyzed by Agilent Feature Extraction software (version 11.0.1.1; Agilent Technologies, Inc.). Following quantile normalization and data processing in GeneSpring GX v11.5.1 software package (Agilent Technologies, Inc.), lncRNA and mRNAs flagged as Present or Marginal (‘all Target Value’) in ≥6 out of 12 samples and were selected for further analysis. Volcano plot filtering was employed to validate the significance of the differences in the lncRNA and mRNA expression levels between the cancer and normal cervical tissues. GeneSpring GX was used to perform hierarchical clustering. GO and pathway analyses were performed using standard enrichment computation.

Reverse transcription-quantitative polymerase chain reaction (RT-qPCR)

Following total RNA extraction as described, cDNA synthesis was performed for 15 min at 37°C and 5 sec at 85°C with PrimeScript RT Master Mix (Takara Biotechnology Co., Ltd.) according to the manufacturer's protocol. Primer sequences are listed in Table II. SYBR Premix Ex Taq (Takara Biotechnology Co., Ltd.) was used with 2 µl template cDNA in each reaction for qPCR with a 7500 Fast Real-Time PCR System (Applied Biosystems; Thermo Fisher Scientific, Inc.). In the 40 cycles of PCR, pre-denaturation was performed for 30 sec at 95°C, while the parameters for denaturation and annealing were set at 95°C for 5 sec and 60°C for 34 sec, respectively. The 2−ΔΔCq value [ΔCq=Cq(RNA)-Cq(GAPDH)] (19) was used to determine an average cycle threshold value from triplicate reactions and calculate the level of genomic expression (20). Single product amplification was ensured by the generated melting curves.

Table II.

Primers used for quantitative polymerase chain reaction analysis of long non-coding RNA levels.

Table II.

Primers used for quantitative polymerase chain reaction analysis of long non-coding RNA levels.

Sequence IDPrimer sequence (5′ to 3′)
TCONS_00001368F: CACACAAGGACTGGAGCAAA
R: CACCTAACCCACCACATTCA
NR_033746F: GCAGCTCAGGTTCTCCAAAT
R: CCCTCTTTAGCCTGTTGGTC
NR_027122F: CTGTCCTCCTGCTCTTTGC
R: GAGTTTTGGGTTCACGGATA
ENST00000421943F: GGGACCAGGAATGTGAACTT
R: TGCCCTCAGATGTGAAACTC
ENST00000439076F: ACAGGCGGCAGAGAAGAAG
R: GACACACGCAGTCATTCAGG
ENST00000448991F: GCAGACTTGACCTCTTGGC
R: ATAGTGGGTATCGGGGGTG
uc001iot.1F: GAGAAGAGGCGAACGAGG
R: GTGGGACAGCCAATACATAAT
ENST00000414085F: CGCAGAACTTTGCTGGAGA
R: GAAATACAGAGTCAGAGAGCGTG
ENST00000421498F: GACCATGCTGTTGAAACCAC
R: TCAAGGAGAGCACAAGGAACT
ENST00000428667F: TTTCCATACCCAGCCAACTT
R: CTTCCTGCACTGCCAACCT
ENST00000443523F: CCTGGCTGGAGATGCTTACT
R: GGTTCCTGTTGGGACTTTAGA
ENST00000551152F: GCAAGAACTGAGACCTGACG
R: TAAGCACACCACTCCACTGC
GAPDHF: GGGAAACTGTGGCGTGAT
R: GAGTGGGTGTCGCTGTTGA

[i] F, forward; R, reverse.

GO and pathway analysis

GO is a functional analysis that annotates genes and attributes associated with their expression using ontological categories, including ‘biological process’, ‘cellular component’ and ‘molecular function’. GO categories (http://www.geneontology.org) were applied to the differentially expressed lncRNAs (21). To analyze how the target genes function in the cellular pathways, the Kyoto Encyclopedia of Genes and Genomes (KEGG; http://www.kegg.jp) (22) database was used. The P-value, which represents the importance of the pathway, was used with a cut-off 0.5, with lower values indicating greater significance.

lncRNA-mRNA correlation network

The lncRNA-mRNA correlation network was established according to lncRNA target predictions along with differentially expressed lncRNA and mRNA profiles using Cytoscape (http://www.cytoscape.org) (23). The lncRNAs and mRNAs that were selected to create the network were those with Pearson correlation coefficients ≥0.99.

Cell culture

The cervical carcinoma cell lines HeLa, SiHa, MS751 and C33A were purchased from the American Type Culture Collection (Manassas, VA, USA) and cultured in Dulbecco's Modified Eagle's medium (Gibco; Thermo Fisher Scientific, Inc.) or RPMI-1640 medium (BRI, Rockville, MD, USA), supplemented with 10% fetal bovine serum (Hyclone; GE Healthcare Life Sciences), penicillin (100 U/ml), and streptomycin (100 µg/ml). The conditions during cell culture were 5% CO2, 95% humidified air, and 37°C.

Statistical analysis

Statistical analyses were performed using SPSS software (version 13.0; SPSS, Inc., Chicago, IL, USA). All data are presented as the mean ± standard deviation. The Student's t-test was used for evaluating the statistical significance of differences in the means between two groups. The association between lncRNA expression and clinicopathological features was assessed using the χ2 test and Fisher's exact test. P<0.05 was considered to indicate a statistically significant difference. Receiver operating characteristic (ROC) curve analysis was employed to define the cutoff value for high expression of lncRNA by the (0,1)-criterion, and the area under the curve was calculated as previously described (24).

Results

Aberrant lncRNA and mRNA expression in cervical cancer

The profiles of lncRNAs and mRNAs in paired cervical cancer and normal cervical tissue samples were produced using microarray technology to investigate the potential biological function of lncRNAs in cervical cancer (Fig. 1A and B). Relative to normal tissue, 5,844 (19.1%) lncRNAs presented differential expression in cancer tissue (fold-change, ≥2) among the 30,586 detected lncRNA transcripts. This included 2,574 upregulated 3,270 downregulated lncRNAs. The most prominently upregulated and downregulated lncRNAs were uc002jcf.3 (fold-change, 57.214) and NR_027122 (fold-change, 620.995), respectively.

In the mRNA expression profile data, 1,538 upregulated mRNAs and 2,898 downregulated mRNAs were detected (Fig. 1C and D). Among these mRNAs, the most prominently upregulated and downregulated mRNAs were Kelch domain-containing 7B (fold-change, 224.009) and keratin 1 (fold-change, 339.108), respectively.

Ontological and pathway analysis of target genes of differentially expressed lncRNAs

To investigate a possible correlation between functional grouping and the differentially expressed lncRNAs, GO annotation categories including ‘biological process’ (Fig. 2A and B), ‘cellular component’ (Fig. 2C and D) and ‘molecular function’ (Fig. 2E and F) were explored for the differentially expressed mRNAs of the samples. In the GO ‘biological process’ classification, the majority of the upregulated and downregulated GO annotations were associated with ‘cellular process’ and ‘regulation of cellular process’. The ‘cellular component’ classification search revealed that a large proportion of genes that were upregulated in cervical cancer were annotated as GO categories ‘intracellular’, ‘intracellular part’, ‘organelle’ and ‘intracellular organelle’; ‘cell’ and ‘cell part’ accounted for the greatest numbers of downregulated genes. The most common ‘molecular function’ GO annotations for all differentially expressed genes were associated with ‘binding’ and ‘protein binding’.

Additionally, pathway analysis was accomplished with the KEGG database (22) to investigate the biological pathways associated with the mRNAs with the most pronounced differential expression in cervical cancer. A total of 40 upregulated pathways were identified in the cervical cancer tissue, which were correlated with the KEGG pathway categories ‘cytokine-cytokine receptor interaction’, ‘chemokine signaling pathway’, ‘transcriptional misregulation in cancer’ and ‘cell cycle’. A total of 37 downregulated pathways were identified, which were associated with the categories ‘MAPK signaling pathway’, ‘pathways in cancer’ and ‘Wnt signal pathway’; all have been previously reported to be associated with cervical cancer (Fig. 3) (25,26).

Construction of lncRNA-mRNA correlation network

In total, 592 network nodes and 934 associations between 12 lncRNAs and 580 coding genes were included in the CNC network, within which there were 500 positive correlation pairs, and 434 negative correlation pairs. The co-expression network demonstrated that one lncRNA could act on 141 coding genes maximally, and that one coding gene corresponded to a maximum of 5 lncRNAs. The mutual regulation between lncRNAs and mRNAs in cervical cancer was also indicated in the CNC network.

RT-qPCR validation

To confirm the microarray results, 12 lncRNAs were selected at random and validated by RT-qPCR. The expression levels of these lncRNAs were detected in 30 cervical carcinoma tissues and 20 normal cervical tissues. The analysis revealed that the lncRNAs ENST00000414085, ENST00000428667, ENST00000551152 and ENST00000443523 were upregulated, and that ENST00000421943, NR_027122, ENST00000448991, ENST00000439076, TCONS_00001368 and NR_033746 were downregulated in the cervical carcinoma tissues relative to the normal cervical tissues (P<0.05; Fig. 4), in good consistency with the microarray results. However, the lncRNAs ENST00000421498 and uc001iot.1 showed no statistically significant differences in expression between cancerous tissue and normal tissues. In summary, the vast majority of the lncRNAs assessed by RT-qPCR were in line with the trends observed by lncRNA microarray.

For further study on the potential function of lncRNAs, the upregulated lncRNA ENST00000551152 and downregulated lncRNA TCONS_00001368 were investigated in cervical carcinoma cell lines. It was observed that ENST00000551152 was overexpressed in SiHa, HeLa, C33A and MS751 cervical cancer cell lines compared with normal cervical cancer tissues, whereas the expression of TCONS_00001368 was decreased in these cervical cancer cell lines (P<0.05; Fig. 5).

Correlation of ENST00000551152 expression and clinicopathological parameters

As ENST00000551152 had the highest level of overexpression among the 12 lncRNAs selected for validation, the association between ENST00000551152 expression level and clinicopathological characteristics in cervical cancer patients was examined to reveal the potential role of this lncRNA in cervical cancer pathogenesis. Additionally, 20 normal and 60 cancerous cervical tissue samples were selected for ENST00000551152 level quantification. The data indicated that the expression of ENST00000551152 in cancer tissues was significantly increased by 2.45 mean fold-change compared with that in normal cervical tissues (P<0.05; Fig. 6).

ROC curve analysis was employed to determine the cutoff value for high ENST00000551152 expression (Fig. 7). Based on this analysis, a total of 46 cancer tissue samples had ≥1.45-fold increased ENST00000551152 levels and were defined as having high level of expression, whereas 14 cases had <1.45-fold expression and were considered as having low level expression. Significant correlations were identified between the ENST00000551152 expression level and several prognostic risk factors, including the International Federation of Gynecology and Obstetrics (FIGO) stage (P=0.017), tumor size (P=0.022), extent of stromal invasion (P=0.001), pelvic lymph node metastasis (P=0.026) and SCC expression level (P=0.004). No significant difference was found between the expression of ENST00000551152 and other variables, including age, differentiation grade and lymphovascular space invasion (Table I). Taken together, the data indicate that the lncRNA ENST00000551152 may serve a critical role in cervical cancer pathogenesis.

Discussion

The significance of lncRNA in cancer pathogenesis and the correlations between various types of human cancers and the aberrant expression of lncRNAs have been elaborated in numerous studies in the past decade (27,28). Certain lncRNAs behave like oncogenes or tumor-suppressors, performing important functions in cancer initiation, progression, metastasis or recurrence. For example, the lncRNA HOTAIR promotes cellular proliferation, cell cycle progression, migration, and invasion via inhibiting p21 in cervical cancer, and thus functions as an oncogene (17). By contrast, lncRNA-LET serves as a tumor suppressor; the overall survival of patients with cervical cancer with downregulated lncRNA-LET is markedly poorer than in those with lncRNA-LET upregulation (14). Thus, it is hypothesized that lncRNAs may be key regulators in cervical cancer pathogenesis. However, the exact pathogenesis-associated functions of lncRNAs in cervical cancer remain unclear. Thus, it is necessary to identify the expression patterns of lncRNAs on a large scale, which is likely to aid in the identification of novel biomarkers and provide a potential therapeutic target for further research.

In the present study, the differential expression patterns of lncRNAs and mRNAs were profiled by comparing cervical cancer and normal cervical tissue samples to identify the pathogenesis-associated functions of lncRNAs. A total of 5,844 lncRNAs and 4,436 mRNAs were differentially expressed (with fold-change, ≥2) according to the microarray results. Among the 5,844 lncRNAs, 2,574 were upregulated and 3,270 were downregulated, a large portion of which have not yet been functionally characterized. To confirm the consistency of the microarray, 12 lncRNAs were randomly selected for quantification by RT-qPCR in 30 cervical cancer and 20 normal cervical tissue samples. The RT-qPCR results were largely consistent with the microarray data, demonstrating that the high-throughput microarray was able to reflect the actual expression patterns of lncRNAs in cervical cancer tissue samples. In order to gain a better understanding of the biological function of lncRNAs, the expression levels of ENST00000551152 (upregulated) and TCONS_00001368 (downregulated) were assessed in cervical cancer cell lines. Furthermore, the association between the expression of ENST00000551152 and clinicopathological variables were analyzed in tissue samples. It was identified that ENST00000551152 expression levels were closely associated with FIGO stage, tumor size, stromal invasion, pelvic lymph node metastasis and SCC antigen expression level. Thus, ENST00000551152 shows great potential as a biomarker in cervical cancer pathogenesis. Due to the limits of the present study, further study should be conducted to investigate the mechanism by which lncRNAs affect the biology of cervical cancer cells.

Analysis of differentially expressed mRNAs, which were potential targets of the differentially expressed lncRNAs, was completed utilizing the KEGG pathway annotation database in order to increase understanding of the possible functional roles of the lncRNAs. Relative to normal cervical tissues, cervical cancer tissue exhibited upregulated mRNAs that were associated with 40 KEGG pathways. The pathways included ‘cytokine-cytokine receptor interaction’, ‘chemokine signaling pathway’, and ‘cell cycle’, all of which have previously been implicated by a number of studies (2931). The downregulated mRNAs were enriched for 37 pathways, of which ‘MAPK signaling pathway’ was the most frequently reported. The CNC network suggested that the regulatory interaction between lncRNAs and mRNAs is complex in cervical cancer. Although elaboration of the exact mechanisms of those genes' involvement in cervical cancer was not achieved, lncRNAs with differential expression may be participants in cervical cancer by regulating these coding genes.

In conclusion, the present study has demonstrated the comprehensive expression profile of lncRNAs and mRNAs in cervical cancer via microarray technology. The differential expression of lncRNAs and mRNAs were observed in cervical cancer samples relative to paired normal cervical tissues. The potential correlation between lncRNAs and protein-coding genes and the roles of lncRNAs in cervical cancer were investigated via bioinformatics analyses, including a CNC network, KEGG pathway annotation and GO category classification. Detailed regulatory mechanisms remain to be further elaborated. Furthermore, each lncRNA and associated mRNA interaction could be a candidate diagnostic marker or therapeutic target for cervical cancer, and further investigation is required.

Acknowledgements

The present study was supported by National Natural Science Foundation of China (grant no. 8167100337), the Natural Science Foundation of Guangdong Province (grant no. 2015A030313073) and Science and Technology Program of Guangzhou (grant no. 201510010289).

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April-2018
Volume 15 Issue 4

Print ISSN: 1792-1074
Online ISSN:1792-1082

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Spandidos Publications style
Huang J, Liu T, Shang C, Zhao Y, Wang W, Liang Y, Guo L and Yao S: Identification of lncRNAs by microarray analysis reveals the potential role of lncRNAs in cervical cancer pathogenesis. Oncol Lett 15: 5584-5592, 2018
APA
Huang, J., Liu, T., Shang, C., Zhao, Y., Wang, W., Liang, Y. ... Yao, S. (2018). Identification of lncRNAs by microarray analysis reveals the potential role of lncRNAs in cervical cancer pathogenesis. Oncology Letters, 15, 5584-5592. https://doi.org/10.3892/ol.2018.8037
MLA
Huang, J., Liu, T., Shang, C., Zhao, Y., Wang, W., Liang, Y., Guo, L., Yao, S."Identification of lncRNAs by microarray analysis reveals the potential role of lncRNAs in cervical cancer pathogenesis". Oncology Letters 15.4 (2018): 5584-5592.
Chicago
Huang, J., Liu, T., Shang, C., Zhao, Y., Wang, W., Liang, Y., Guo, L., Yao, S."Identification of lncRNAs by microarray analysis reveals the potential role of lncRNAs in cervical cancer pathogenesis". Oncology Letters 15, no. 4 (2018): 5584-5592. https://doi.org/10.3892/ol.2018.8037