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High expression of long non-coding RNA NEAT1 indicates poor prognosis of human cancer

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Oncotarget. 2017; 8:45918-45927. https://doi.org/10.18632/oncotarget.17439

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Jian Fang, Fuhao Qiao, Jingjing Tu, Jinfeng Xu, Fangfang Ding, Yun Liu, Bufugdi Andreas Akuo, Jianpeng Hu and Shihe Shao _

Abstract

Jian Fang1, Fuhao Qiao1, Jingjing Tu1, Jinfeng Xu1, Fangfang Ding1, Yun Liu1, Bufugdi Andreas Akuo1, Jianpeng Hu2 and Shihe Shao1

1Department of Pathogenic Biology, School of Medicine, Jiangsu University, Zhenjiang, Jiangsu 212013, China

2Department of Urinary Surgery, Zhenjiang First People’s Hospital, Zhenjiang, Jiangsu 212013, China

Correspondence to:

Shihe Shao, email: [email protected]

Keywords: NEAT1, cancer, OS, meta-analysis, poor prognosis

Received: September 07, 2016     Accepted: April 11, 2017     Published: April 26, 2017

ABSTRACT

The nuclear paraspeckle assembly transcript 1 (NEAT1) is a long non-coding RNA. Many studies have reported that NEAT1 plays critical oncogenic roles and facilitates tumorigenesis of various human cancers. High NEAT1 expression is associated with a poor prognosis in cancer patients. This meta-analysis was conducted to assess the association between NEAT1 levels and survival times of cancer patients. Overall survival (OS) was the primary endpoint. Thirteen publications with 1,496 cancer patients from 5 databases (PubMed, EMBASE, Cochrane Library, Wiley Online Library, and Medline) met the criteria for this meta-analysis. Results of the analysis showed that NEAT1 expression in human cancer was significantly associated with OS (hazard ratio [HR]=1.53, 95% confidence interval [CI]: 1.39–1.68), including digestive system tumor (HR=1.54, 95% CI: 1.37–1.73) and respiratory carcinomas (HR=1.44, 95% CI: 1.11–1.85). The results also indicated that NEAT1 expression was highly associated with tumor size (>3 cm vs. ≤3 cm; odds ratio [OR]=2.51, 95% CI: 1.27–4.99; p=0.009), TNM stage (III+IV vs. I+II; OR=4.17, 95% CI: 2.42–7.18; p=0.00001), and distant metastasis (OR=2.73, 95% CI: 1.28–5.79; p=0.01). However, there was no significant association with differentiation (poor vs. well + moderate, OR=1.45, 95% CI: 0.72–2.91) and lymph node metastasis (OR=1.39, 95% CI: 0.54–3.60). This meta-analysis showed that NEAT1 expression may be a useful biomarker for predicting a poor prognosis in patients with cancer.


INTRODUCTION

Long non-coding RNA (LncRNA) is a class of non-coding RNA, and has more than 200 nucleotides [1]. Initially, LncRNA was considered as spurious transcriptional noise without biological functions because of its lack of protein-coding function [2]. However, later studies indicated that LncRNA plays an important role in pathophysiological processes such as cancers [3, 4]. In recent years, few LncRNAs, such as AFAPI-ASI, MALAT-1, and UCA1 have been confirmed to play a significant role in cancer progression [58]. Therefore, LncRNAs might have complex and extensive functions in carcinogenesis and progression of human cancers [9].

The nuclear paraspeckle assembly transcript 1 (NEAT1) is a newly identified nuclear-restricted LncRNA and is located on chromosome 11 (11q13.1). It is an essential component of nuclear paraspeckles [10, 11], and has been confirmed to overexpress in many human cancers, including prostate, lung, and breast cancers [1214]. High NEAT1 expression in cancerous tissues was reported to be associated with prognosis and overall survival (OS) in several cancers. However, the effect of NEAT1 on the outcome of cancer patients has been controversial. No meta-analysis has been conducted to date on the correlation of NEAT1 with the survival of cancer patients. NEAT1 might act as a potential diagnostic biomarker and prognostic factor. This meta-analysis is the first to explore the correlation between NEAT1 expression and prognosis of cancer patients.

RESULTS

Literature search and description of studies

As shown on Figure 1, 163 studies were found in the 5 databases (PubMed, EMBASE, Cochrane Library, Wiley Online Library and Medline). We reviewed the titles and abstracts, and 49 irrelevant studies and duplicates were excluded. Of the remaining 99 studies, 86 were eliminated because they used different statistics methods, were animal experiments, or were not in English. After data extraction, 13 studies [1426], all from China, were selected for the final meta-analysis with a total of 1,496 cancer patients. The main characteristics are summarized in Table 1. The 13 studies covered 9 different types of cancer, including ovarian cancer (n=2), colorectal cancer (n=3), non-small cell lung cancer (NSCLC; n=2), gastric cancer (n=1), hepatocellular carcinoma (n=1), glioma (n=1), nasopharyngeal carcinoma (NPC; n=1), pancreatic cancer (PC; n=1) and esophageal squamous cell carcinoma (n=1). Among the 13 studies, 12 involved tissue collection, and 1 involved a whole blood analysis. All of the detection methods used quantitative polymerase chain reaction.

Flow chart of studies selection procedure.

Figure 1: Flow chart of studies selection procedure.

Table 1: Characteristics of studies included in this meta-analysis

Author

Year

Country

Sample size

Sample type

Cancer type

Tumor size (cm)

TNM stage

Follow-up

Method

Outcome

HR statistics

Variance

NOS

≤3VS>3

I/II Vs III/IV

(Month)

Analysis

He

2015

China

94

Tissue

Glioma

30/64

23/71

>50

qRT-PCR

OS

Reported

Univariate

8

Guo

2015

China

95

Tissue

HCC

NA

22/73

>60

qRT-PCR

OS

Survival curve

Univariate

7

Fu

2016

China

140

Tissue

GC

NA

63/77

96

qRT-PCR

OS

Reported

Multivariate

8

Sun

2016

China

96

Tissue

NSCLC

41/55

28/68

41

qRT-PCR

OS

Survival curve

Univariate

8

Li

2015

China

239

Tissue

CC

82/157

92/147

>60

qRT-PCR

OS, DFS

Reported

Univariate

8

Wu

2015

China

191

Whole blood

CC

NA

26/165

80

qRT-PCR

OS

Reported

Multivariate

8

Chen

2015

China

96

Tissue

ESCC

NA

35/61

>60

qRT-PCR

OS

Reported

Multivariate

8

Lu

2015

China

71

Tissue

NPC

NA

36/35

>40

qRT-PCR

OS

Reported

Multivariate

8

Aderiaens

2016

Belgium

58

Tissue

OC

NA

NA

>60

qRT-PCR

OS

Reported

Univariate

8

Huang

2016

China

86

Tissue

PC

NA

56/32

>50

qRT-PCR

OS

Survival curve

Univariate

7

Peng

2016

China

56

Tissue

CC

NA

NA

60

qRT-PCR

OS

Survival curve

Multivariate

7

Chen

2016

China

149

Tissue

OC

NA

53/96

>60

qRT-PCR

OS

Reported

Multivariate

8

Pan

2015

China

125

Tissue

NSCLC

60/65

54/71

>40

qRT-PCR

OS

Survival curve

Univariate

8

HCC: hepatocellular carcinoma; GC: gastric cancer; NSCLC: non-small cell lung cancer; CC: colorectal cancer; NPC: nasopharyngeal carcinoma; OC: ovarian cancer; PC: pancreatic cancer; ESCC: esophageal squamous cell carcinoma; NA: not available.

Correlation of high NEAT1 expression with OS in human cancer

All 13 studies showed OS according to NEAT1 expression levels among the 1,496 patients. The pooled hazard ratio (HR) was 1.53 (95% confidence interval [CI]: 1.39–1.68) for the high NEAT1 expression group versus low expression group (p<0.00001; Figure 2). There was no significant heterogeneity (I2=0%, PQ=0.51), and the fixed-effects model was chosen to estimate the pooled HR. This suggested that high expression of NEAT1 was a predicator of poor prognosis among human cancers.

Forest plot of HR for NEAT1 high expression and overall survival.

Figure 2: Forest plot of HR for NEAT1 high expression and overall survival.

Correlation of NEAT1 expression with clinicopathological parameters and cancer type

In this meta-analysis, correlation of NEAT1 expression with digestive system tumor and respiratory carcinomas and clinicopathological parameters are illustrated in Figure 3 and Table 2. High NEAT1 expression correlated with poor prognosis of digestive system tumor (HR=1.54, 95% CI: 1.37–1.73; Figure 3A) and Respiratory carcinomas (HR=1.44, 95% CI: 1.11–1.85; Figure 3B) patients. Furthermore, we found correlation of NEAT1 expression with more advanced tumor size (>3 cm vs. ≤3 cm; odds ratio [OR]=2.51, 95% CI: 1.27–4.99; p=0.009; Figure 4A), distant metastasis (M1 vs. M0; OR=2.72, 95% CI: 1.28–5.79; p=0.010; Figure 4B), and TNM stage (III+IV vs. I+II; OR=4.17, 95% CI: 2.42–7.18; p=0.00001; Figure 4C). However, NEAT1 expression was not significantly associated with differentiation (poor vs. well + moderate, OR=1.45, 95% CI: 0.72–2.91; p=0.30) and lymph node metastasis (yes vs. no, OR=1.39, 95% CI: 0.54–3.60, p=0.5) (Table 2).

Forest plot of NEAT1 expression with OS in digestive system tumor and respiratory carcinomas patients.

Figure 3: Forest plot of NEAT1 expression with OS in digestive system tumor and respiratory carcinomas patients. (A) Digestive system tumor and (B) respiratory carcinomas.

Forest plot of NEAT1 expression and OR for clinicopathological features.

Figure 4: Forest plot of NEAT1 expression and OR for clinicopathological features. The investigated clinicopathological parameters are (A) tumor size, (B) DM and (C) TNM stage.

Table 2: Results of the association between NEAT1 and clinicopathological parameters

Outcome

Studies (n)

OR (HR)

95%CI

P Value

Model

Heterogeneity

Chi2, I2, P Value

Tumor size (>3 cm vs. ≤3 cm)

3

2.51

1.27-4.99

0.009

Random

4.60, 57%, 0.10

TNM stage (III+IV vs. I+II)

5

4.17

2.42-7.18

0.00001

Random

8.46, 53%, 0.08

Differentiation (poor vs. well + moderate)

4

1.45

0.72-2.91

0.3

Random

11.97, 75%, 0.007

Lymph node metastasis (Yes vs. No)

5

1.39

0.54-3.60

0.5

Random

29.01, 86%, 0.0001

Distant metastasis (M1 vs. M0)

6

2.72

1.28-5.79

0.01

Random

17.75, 72%, 0.003

Digestive system tumor

7

1.54

1.37-1.73

0.00001

Fixed

6.98, 14%, 0.32

Respiratory carcinomas

3

1.44

1.11-1.85

0.005

Fixed

0.71, 0%, 0.70

NEAT1 expression in other cancer types

In order to understand the expression level of NEAT1 in other cancer types, we used two public cancer database The Cancer Genome Atlas (TCGA) and Oncomine (https://www.oncomine.org) to analyze the expression of NEAT1 in 15 cancer types. The results indicated that the expression of NEAT1 was higher in the tumor tissues than the corresponding normal issues (Figure 5A and 5B).

The expression level of NEAT1 analyzed by cancer public database.

Figure 5: The expression level of NEAT1 analyzed by cancer public database. (A) The expression of NEAT1 analyzed by Oncomine. 1, prostate cancer; 2, myeloma; 3, breast cancer; 4, lung cancer; 5, gastric cancer; 6, adrenal cancer; 7, colon cancer; 8, liver cancer; 9, renal cancer; 10, lymphoma; 11, pancreas cancer; 12, leukemia. (B) The expression of NEAT1 analyzed by TCGA database.1, head and neck squamous cancer; 2, kidney cancer; 3, hepatocellular carcinoma; 4, prostate cancer; 5, stomach adenocarcinoma; 6, uterine corpus endometrioid carcinoma; 7, bladder urothelial carcinoma; 8, cervical squamous cell carcinoma and endocervical adenocarcinoma.

Sensitivity analysis

A sensitivity analysis was conducted to analyze the association between NEAT1 and OS by deleting one study at a time from the pooled analysis to examine the influence of the removed data set to the overall HR. The result was not influenced by the exclusion of each study, suggesting that the result of the synthetic analysis was robust (Figure 6).

Sensitivity analysis of the effect of the individual study on the pooled HRs for the correlation between NEAT1 expression and overall survival (OS).

Figure 6: Sensitivity analysis of the effect of the individual study on the pooled HRs for the correlation between NEAT1 expression and overall survival (OS).

Publication bias

To evaluate the potential for publication bias in this meta-analysis, funnel plots were made (Figure 7). No significant publication bias was observed across studies.

Funnel plot was used to evaluate publication bias on OS.

Figure 7: Funnel plot was used to evaluate publication bias on OS.

DISCUSSION

This meta-analysis is the first to evaluate the association between NEAT1 levels and cancer prognosis. The results indicated that high NEAT1 expression was significantly associated with shorter OS times in cancer patients. Subgroup analyses showed that NEAT1 levels were significantly associated with tumor size, TNM stage, and distant metastasis. Yang et al.[27] reported that high expression level of NEAT1 was significantly associated with shorter overall survival in cancer patients, which is similar to our results. However, we also found that the expression of NEAT1 was higher in respiratory carcinomas and correlated with poor prognosis of respiratory carcinomas patients. Xiong et al.[28] used 57 microarrays and other RNA-seq datasets to analyzed correlation of NEAT1 expression with digestive system tumor, and arrived at the same conclusion with us. These results also shown the reliability of our conclusion.

Recently, many LncRNAs have been reported to function as oncogenes or tumor suppressor genes, including PVT1 [29], MALAT1 [30], and HOTAIR [31]. Choudhry et al. reported that NEAT1 is a direct transcription target of HIF-2 in many breast cancer lines and solid tumors. NEAT1 is an essential structural component of paraspeckles, and the hypoxic induction of NEAT1 induces paraspeckle formation in a manner that is dependent upon both NEAT1 and HIF-2. This then leads to accelerated cellular proliferation, improved clonogenic survival, and reduced apoptosis [14]. You et al. reported that NEAT1 is a target of miR-449a and is involved in cell growth and apoptosis of lung cancer cell lines [12]. Yoon et al. reported that NEAT1 can be modulated by RNA-binding protein AUF1, thus affecting the organization of nuclear paraspeckles [32]. Blume et al. reported that NEAT1 is also an important element of the p53-dependent DNA damage response machinery in chronic lymphocytic leukemia [33]. Lastly, Chakravarty et al. reported that NEAT1, as an estrogen receptor alpha specific LncRNA, drives oncogenic growth by altering the epigenetic landscape of target gene promoters [13]. Previous studies revealed that NEAT1 overexpression could influence cell apoptosis and migration [34, 35]. On the contrary, silencing of NEAT1 expression by small interfering RNA could suppress cell apoptosis and metastasis. Therefore, NEAT1 expression level may be an indicator of the intrinsic characteristics of cancer progression. Furthermore, the relationship between NEAT1 expression and a variety of cancer patients’ clinicopathological parameters were reported in previous studies [1421]. These data might explain why high levels of NEAT1 were significantly associated with shorter OS in cancer patients in this meta-analysis. However, the detailed mechanisms of why NEAT1 was associated with oncologic outcome in cancer were unclear. Wu et al. reported that a 5-LncRNA signature was detected in clear cell renal cell carcinoma patients and normal controls, and further study indicated that this 5-LncRNA signature appears to provide a promising biomarker for the detection of clear cell renal cell carcinoma [36]. Therefore, NEAT1 might also be a tumor marker for predicting tumorigenesis and cancer progression. Although the results revealed the relationship between NEAT1 and OS and patients’ clinicopathological parameters, there are some limitations of this meta-analysis: the number of studies and cancer patients were limited. Most of the studies were conducted in China; therefore, differences may occur between ethnic groups. Additionally, there were 5 studies in which HR could not directly be calculated, thus they may not have provided the most accurate HR estimate. Our results should be confirmed in further studies.

In all, our results indicated that high NEAT1 expression may be a risk factor for shorter OS and a useful biomarker to predict poorer prognosis in human cancers. However, to reinforce the findings, better standardized methods with large sample sizes are needed to further confirm the association between NEAT1 and clinical outcomes of cancers in various ethnic populations.

MATERIALS AND METHODS

Literature search strategies

PubMed, EMBASE, Cochrane Library, Wiley Online Library, and Medline were searched, and articles published from January 1, 1996 to February 10, 2017 were considered. The search strategies were the following: “long non-coding RNA NEAT1” or “lncRNA NEAT1” or “NEAT1” or “nuclear paraspeckle assembly transcript 1” and “Cancer” or “Tumor” or “Neoplasia” and “prognos*” or “surviv*” or “outcome” or “mortality” or “predict.” Reference lists of relevant articles and review papers were also searched manually to identify potential studies.

Inclusion and exclusion criteria

Inclusion criteria were: (1) Studies were written in English, (2) the level of NEAT1 expression was examined in cancer tissues, (3) investigation of the correlation between NEAT1 expression level and survival outcome (OS or progression-free survival), and (4) HR and its 95% CI for survival time were reported or could be calculated from the reported data. Exclusion criteria were: (1) animal studies, case reports, meta-analyses, and review articles and (2) papers lacking all raw data or inability to calculate its HR, 95% CI, and p values.

Data extraction and study quality assessment

All data information of eligible studies included the first author’s name, publication year, study regions, sample size, cancer type, tumor size, TNM stage, and method of NEAT1 testing. The HR, corresponding 95% CI, and HR statistics for outcome (OS and progression-free survival [PFS]) were calculated independently.

Study quality was assessed using the Newcastle–Ottawa quality assessment scale (NOS). The NOS score items included selection, outcome, and comparability, and ranged between 0 and 9.

Statistical analysis

The extracted data of this meta-analysis were analyzed using Review Manager 5.3 software (Cochrane network). The HR and its 95% CI were used to evaluate the strength of the association between NEAT1 and OS. If they were reported in a study, HR with 95% CI was extracted directly. If not, the data were extracted from Kaplan–Meier curve using Engauge Digitizer version 4.1 (http://digitizer.sourceforge.net/) [37]. The chi-square-based Q test and I2 statistics were used to determine the heterogeneity [38], and I2 >50% and a P-value for Q test <0.05 were considered significant heterogeneity. Conversely, the I2<50% and a P-value for Q test >0.05 were considered as having no heterogeneity. If there was heterogeneity in the included studies, we chose the random-effects model. The fixed-effects model was chosen when no significant heterogeneity was observed [39]. Sensitivityanalyses were carried out using Stata 12.0 (Stata Corporation, College Station, TX, USA).

CONFLICTS OF INTEREST

All authors declare that they have no conflicts.

FUNDING

This work were funded by the National Natural Science Foundation of China (Grant no. 81271795), Natural Science Foundation of Jiangsu Province, China (Grant no. BK20161345) and Key R and D programs - social development of Zhenjiang, Jiangsu, China (Grant no. SH2015080).

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