Identification of SPOP related metabolic pathways in prostate cancer

INTRODUCTION

Prostate cancer (PCa) is the second most common cancer and the fifth leading cause of death from malignant carcinoma in men [1, 2]. It is estimated that approximately 603,000 men were diagnosed with PCa and 266,000 men died of PCa in China in 2015 [3]. The incidence rates of PCa have shown an increasing trend in almost all countries [4]. However, the pathogenesis and etiology of PCa remain largely unknown. SPOP has been identified as one of the most frequently mutated genes in PCa with 6–15% mutation rate [5]. SPOP is a cullin-based E3 ubiquitin ligase, involving meprin and TRAF homology (MATH) protein interaction domain and Bric-a-brac/Tramtrack/Broad complex (BTB) domain [6]. Most of SPOP mutations have been reported to occur in conserved residues at MATH domain which play key roles in substrate interaction [5, 6]. Previous studies demonstrated that the ubiquitination complex of SPOP-CUL3 can regulate the degradation of various substrates, such as DEK proto-oncogene (DEK) [7], nuclear receptor coactivator 3 (NCOA3) [8], androgen receptor (AR) [9], V-Ets avian erythroblastosis virus E26 oncogene homolog (ERG) [10, 11] and cell division cycle 20 (CDC20) [12]. Thereby, the function of degrading oncogenic substrates of SPOP can be abrogated by SPOP mutations, which can partly explain the reason for PCa initiation and progression.

Accumulating evidence supports the notion that metabolic pathway reprogramming plays a critical role during cancer progression in various types of neoplasias including PCa [13–16]. One of the most well-known metabolic characteristics observed in tumor cells is the Warburg effect, in which ATP and lactate are produced by high rates of glycolysis instead of oxidative phosphorylation [17]. Several recent studies have revealed the occurrence of metabolic reprogramming in PCa. Jonathan et al. demonstrated that almost thirty metabolites exhibited statistically significant changes in aggressive prostate tumors relative to cancer-free prostate tissues, including amino acid catabolites, lipid compounds and energetics-related metabolites [18]. Metabolomics profiles in PCa clinical samples showed that the accumulation of sarcosine, a methylated metabolite of the amino acid glycine, positively correlates with PCa progression [19]. Also, previous findings from our laboratory identified sphingosine and cholesteryl oleate as potential molecular biomarkers to distinguish PCa and benign prostatic hyperplasia [20, 21]. Importantly, a recent review by Liu et al. reported that fatty acids oxidation is a main pathway for producing energy in PCa [22]. Furthermore, various proteins have been determined to be involved in metabolic pathway reprogramming in neoplastic prostate cells, such as AR [23], steroid receptor coactivator 2 (SRC-2) [24], MYC and AKT [25]. However, whether SPOP mutations are associated with metabolic reprogramming in PCa has not been explored before.

In this study, transcriptomics profiling was applied for 66 matched prostate cancer tumor (PCT) and adjacent non-tumor (ANT) samples. Mutation information of corresponding patients was obtained. Additionally, to obtain the comprehensive landscapes of metabolic alterations in PCa patients, metabolomics and lipidomics were performed by gas chromatography-mass spectrometry (GC-MS) and liquid chromatography-mass spectrometry (LC-MS) in matched PCT and ANT tissues. Moreover, we characterized the metabolites and metabolic enzymes related to SPOP mutations by integration of transcriptomics and metabolomics as well as lipidomics.

RESULTS

Patient information and genetic alterations in PCa patients

In this study, 66 patients with PCa were enrolled for transcriptomic analysis and characterized by the clinical pathological features (Table 1). The expression data of 66 matched PCT and ANT tissues were profiled at transcriptional level by RNA-Seq analysis. As shown in Figure 1A, 16 highly mutated genes were found in PCT tissues compared with matched ANT tissues, including SPOP, myeloid/lymphoid or mixed-lineage leukemia 2 (MLL2), titin (TTN), collagen type XXII alpha 1 (COL22A1), myosin heavy chain 2 (MYH2), ryanodine receptor 1 (RYR1), semaphorin 5A (SEMA5A), ATM serine/threonine kinase (ATM), cyclin dependent kinase 12 (CDK12), phosphatase and tensin homolog (PTEN), tumor protein P53 (TP53), RUNX1 translocation partner 1 (RUNX1T1), GLI family zinc finger 3 (GLI3), collagen type IV alpha 1 chain (COL4A1), colony stimulating factor 1 receptor (CSF1R), and catenin beta 1 (CTNNB1). Among these mutated genes, SPOP was identified as the most frequently mutated one in PCT tissues with a 16.7% frequency, which was consistent with the previous report [5] (Figure 1A–1B). It was interesting that all SPOP mutations occurred at the conserved residues in the substrate-binding cleft of MATH (Figure 1C, Table 2).

Differential metabolites between the matched PCT and ANT tissues in SPOP-mutated PCa patients

Although SPOP is the most frequently mutated gene in PCa, the metabolic pathways regulated by SPOP are still unclear. To uncover the potential SPOP-related metabolic pathways, we profiled metabolite alterations using GC-MS and LC-MS in SPOP-mutated PCT tissues and their matched ANT tissues. A total of 51 differential metabolites were identified in SPOP-mutated PCT tissues relative to the matched ANT tissues (Supplementary Table 1). Of these, only 3 metabolites including glycochenodeoxycholic acid (GCDCA), histamine and carnitine C8:0, significantly decreased in SPOP-mutated PCT tissues, whereas other 48 metabolites (lipids, organic acids, carbohydrates etc.) increased obviously (Supplementary Table 1, Figure 2A). The top six remarkably upregulated metabolites were nicotinamide adenine dinucleotide (NAD), cholesteryl ester (CE) 24:5, CE 20:1, ceramide (Cer) 38:2, 2, triacylglycerol (TAG) 55:1 and phosphatidylcholine (PC) 28:0 (Figure 2B–2G). These results suggest that several metabolic pathways may be associated with SPOP mutations.

Integration of transcriptomics, metabolomics and lipidomics in SPOP-mutated PCa patients

One omics was insufficient to illustrate the alterations occurring in PCa, hence integrated studies of transcriptomics, metabolomics and lipidomics data were performed to further identify the metabolic pathways related to SPOP mutations. Gene set analysis was applied for finding altered metabolic pathways in 11 SPOP-mutated patients using Kyoto Encyclopedia of Genes and Genomes (KEGG) database [26] by online software Consensuspathdb [27]. Total 3766 differential transcripts were used for gene set analysis to calculate the related metabolic pathways, of which 1840 transcripts were upregulated whereas 1926 transcripts were down-regulated. Most of the related metabolic pathways were significantly upregulated in PCT tissues of SPOP-mutated cohort (Table 3). Only two metabolic pathways involving thyroid hormone synthesis and arachidonic acid metabolism were down-regulated in SPOP-mutated PCT tissues.

Next, to understand SPOP-regulated metabolic pathways, we combined the transcriptomics data with our metabolomics and lipidomics data from SPOP-mutated cohort and constructed an overall network of metabolic pathways. As presented in Supplementary Figure 1, four sections of metabolic pathways including glycolysis, TCA cycle, fatty acid metabolism and glycerophospholipid metabolism, exhibited obvious alterations in SPOP-mutated PCT tissues. Moreover, most of differential metabolites involved in these metabolic pathways were significantly upregulated in SPOP-mutated PCT tissues, which were consistent with the altered trends of the relevant transcripts.

Increasing evidence indicates that altered fatty acid metabolism, including biosynthesis, transportation and degradation, frequently occurs during PCa progression [22, 28]. Our transcriptomics data showed that 5 genes involved in fatty acid biosynthesis such as fatty acid synthase (FASN), acetyl-CoA carboxylase alpha (ACACA), malonyl-CoA-acyl carrier protein transacylase (MCAT), ELOVL fatty acid elongase 2 (ELOVL2) and 3-oxoacyl-ACP synthase, mitochondrial (OXSM), 6 genes involved in fatty acid oxidation including acyl-CoA dehydrogenase, long chain (ACADL), hydroxyacyl-CoA dehydrogenase/3-ketoacyl-CoA thiolase/enoyl-CoA hydratase (trifunctional protein), beta subunit (HADHB), acyl-CoA dehydrogenase, short/branched chain (ACADSB), enoyl-CoA hydratase 1 (ECHS1), enoyl-CoA, hydratase/3-hydroxyacyl CoA dehydrogenase (EHHADH) and hydroxyacyl-CoA dehydrogenase (HADH), and 3 genes involved in fatty acid transportation such as solute carrier family 27 member 2 (SLC27A2), solute carrier family 27 member 4 (SLC27A4) and solute carrier family 27 member 5 (SLC27A5), were obviously upregulated in SPOP-mutated PCT tissues (Supplementary Figure 1A and Supplementary Figure 2). Additionally, 9 free fatty acids (FFAs) were found to increase significantly in SPOP-mutated PCT tissues in metabolomics profiling, including saturated and unsaturated fatty acids (Figure 3A–3I). These findings indicated that fatty acid metabolism might be a dominant energy source for tumor growth in SPOP-mutated PCa patients. Furthermore, integrated analysis was conducted by calculating Pearson correlation coefficients (PCC) between 58 transcripts and 52 metabolites involved in fatty acid metabolic pathways and showed strong correlations between transcripts and metabolites in SPOP-mutated cohort (Figure 3J). Of these transcripts, ACADL and ELOVL2 exhibited the strongest correlations with most of fatty acid metabolites, suggesting that the alterations of ACADL and ELOVL2 may be regulated by SPOP mutations.

In addition, glycerophospholipid metabolism was another remarkably altered pathway in SPOP-mutated cohort (Supplementary Figure 1B and Supplementary Table 1). Metabolomics and lipidomics analyses showed that most of the key intermediate metabolites involved in glycerophospholipid metabolism, such as PC and phosphatidylethanolamine (PE), were obviously increased in SPOP-mutated PCT tissues. Consistently, our results of transcriptomics also showed significant elevation of 8 involving genes, such as 1-acylglycerol-3-phosphate O-acyltransferase 6 (AGPAT6), membrane bound O-acyltransferase domain containing 2 (MBOAT2), lysocardiolipin acyltransferase 1 (LCLAT1), 1-acylglycerol-3-phosphate O-acyltransferase 3 (AGPAT3), ethanolaminephosphotransferase 1 (EPT1), lysophospholipase I (LYPLA1), phospholipase A2 group XIIA (PLA2G12A) and lysophosphatidylcholine acyltransferase 3 (LPCAT3) (Supplementary Figure 1B). These findings indicated that an overall upregulated glycerophospholipid metabolic pathway in SPOP-mutated PCT tissues.

It is well-accepted that TCA cycle plays a critical role in cancer progression [29]. Here, based on the metabolomics analysis, fumarate and malate, two key intermediates involved in TCA cycle, were found to upregulate markedly in SPOP-mutated cohort (Figure 4A and 4B). Surprisingly, the catabolic enzymes of fumarate hydratase (FH) and malic dehydrogenase 2 (MDH2) transcripts were significantly upregulated in transcriptomics profiles in SPOP-mutated cohort (Figure 4C and 4D). Moreover, a correlation network based on PCC between transcripts and metabolites in TCA cycle showed obvious correlations between FH, isocitrate dehydrogenase 1 (IDH1) transcripts and fumarate as well as malate (Figure 4E). However, there was neither correlation between MDH2 transcript and metabolites nor significant alteration for IDH1 transcript in transcriptomics profiles. Hence, these alterations revealed that the obvious upregulation of FH gene in PCa might be associated with SPOP mutations.

Transcriptomics and metabolomics differences between SPOP-WT (wild type) and SPOP-mutated PCT tissues

To find out the transcriptomic differences between SPOP-WT and SPOP-mutated PCT tissues, the transcriptomic data from 11 SPOP-mutated PCT tissues were analyzed by comparing with those of 52 SPOP-WT PCT tissues. Totally, 1357 differential transcripts were found out and used to analyze the related pathways by Consensuspathdb [27]. Several pathways such as cell cycle, steroid hormone biosynthesis and others displayed obvious differences between SPOP-WT and SPOP-mutated PCT tissues (Figure 5A). Five transcripts related to fatty acid degradation, including acyl-CoA dehydrogenase, C-2 To C-3 short chain (ACADS), acyl-CoA synthetase long-chain family member 1 (ACSL1), ECHS1, ACADSB and HADH, were shown remarkable upregulation in SPOP-mutated PCT tissues (Figure 5B–5F), of which ECHS1, ACADSB and HADH were also upregulated significantly when compared to their matched ANT tissues. Moreover, based on the metabolomics and lipidomics data, the top six differential metabolites between SPOP-WT and SPOP-mutated PCT tissues were found, of which diacylglycerol (DAG) 36:4, as an important diacylglycerol metabolite, exhibited obvious increase in SPOP-mutated PCT tissue (Figure 5G–5L). These results were consistent with the alterations summarized in Supplementary Figure 1.

Validation of the correlation between SPOP and metabolic genes including FH, ELOVL2 and ACADL

To further validate the correctness of aforementioned findings, the big database of cBioportal [30, 31] was used to search for the alteration frequency of SPOP, FH, ELOVL2 and ACADL genes in PCa and analyze the potential correlations of SPOP with FH, ELOVL2 and ACADL. ACTB was used as negative control and ERG was used as positive control. Of note, SPOP (18%), FH (9%), ELOVL2 (5%) and ACADL (5%) were significantly altered in PCa cohorts (Supplementary Figure 3A, 333 samples; Primary Prostate Carcinomas; TCGA, Cell 2015) [32]. Frequently, the mRNA expression of FH, ELOVL2 and ACADL was upregulated in SPOP mutated patients (Supplementary Figure 3A). The SPOP mutations exhibited remarkable co-occurrence correlations with genetic alterations of FH, ELOVL2 and ACADL and significant exclusivity correlation with ERG, but not with ACTB (Supplementary Figure 3B). These results were consistent with our findings of transcriptomics that the expression of FH, ELOVL2 and ACADL were obviously upregulated in SPOP mutated patients.

Furthermore, the expression of FH, ELOVL2 and ACADL were validated in SPOP_WT and SPOP_Y87N transduced HEK293T, LNCaP and PC3 cells (Figure 6, Supplementary Figure 4). The protein levels of FH and ELOVL2 were significantly decreased in SPOP_WT transduced LNCaP cells compared with the control and SPOP_Y87N transduced LNCaP cells (Figure 6A). In 293T cells, transducing SPOP_WT caused a significant decrease in the protein levels of FH and ACADL compared with the control and SPOP_Y87N transduced cells (Supplementary Figure 4). Additionally, compared with the control as well as SPOP_Y87N transduced LNCaP and PC3 cells, the mRNA level of FH was also decreased in SPOP_WT transduced cells (Figure 6C–6D). Taken together, our findings suggest that FH, ELOVL2 and ACADL genes might be the downstream transcripts of SPOP and play critical roles in the upregulation of metabolic pathways mediated by SPOP mutations.

DISSCUSSION

SPOP is recognized as one of the most frequently mutated genes in PCa [5], which was also confirmed in our current study (Figure 1A). Increasing evidence supports the notion that SPOP mutations define a distinct molecular subclass of PCa [5, 9, 33]. Although a large body of studies focus on the functions of SPOP mutations in PCa, less is known about SPOP-mutation-related metabolic pathways. Here, our study reported for the first time that several altered metabolic pathways in PCT tissues might be intimately associated with SPOP mutations.

Traditionally, metabolomics and transcriptomics have been investigated alone. Transcriptomics, defined as a global expression profiling of RNA transcripts, has been widely applied as a valuable tool to comprehensively understand genetic alterations [34–36]. Metabolomics, as a global analysis of numerous metabolites, can provide data-rich information of metabolic alterations and is usually applied for discovering biomarkers [19, 37]. However, transcriptomics is limited to post-transcriptional modifications and metabolomics is limited to the functional analysis of metabolites. To avoid the limitations of single omics, integration of transcriptomics and metabolomics was performed in this study, which could precisely identify the altered metabolic pathways during disease progression and deeply understand the alterations of metabolites. Here, we investigated the alterations of metabolic pathways in SPOP-mutated PCa patients by integration of transcriptomics and metabolomics as well as lipidomics, followed by validation of the correlation between SPOP and metabolic genes through cBioportal. Importantly, our transcriptomics data and metabolomics data could support each other, which could also be confirmed by the results from correlation analysis, suggesting a high credibility.

It is well-known that SPOP usually acts as a tumor suppressor in PCa and somatic missense mutations of SPOP occur frequently in PCa [5]. AR has been identified as a central player in PCa progression including cell proliferation, migration and metabolism, and also a validated therapeutic target [38]. Several previous studies demonstrated that SPOP could directly bind to AR and contribute to its ubiquitination and degradation [9, 39]. Additionally, AR has been reported to be intimately associated with the alterations in metabolism and biosynthesis in PCa [40]. Hence, we speculated that there might be a relationship between SPOP mutations and metabolic alterations in PCa. As expected, numerous metabolites were found to express aberrantly in SPOP-mutated PCT tissues, most of which were significantly upregulated. Specifically, five of the top six remarkably upregulated metabolites were lipids (Figure 2B–2G). Moreover, almost all differential metabolites and transcripts involved in fatty acid metabolic pathway and glycerophospholipid metabolic pathway were notably upregulated in SPOP-mutated PCT tissues (Figure 3, Supplementary Figures 1–2 and Supplementary Table 1). Therefore, these findings suggest that lipid accumulation in PCT tissues may be closely associated with SPOP mutations.

TCA cycle plays a critical role in the transformation of energy metabolites and frequently dysregulated during cancer progression [29, 41]. In PCT tissues, TCA cycle is highly activated by loss of zinc accumulation, which can produce energy to fuel prostate tumorigenesis [42, 43]. In our data, fumarate and malate increased obviously in PCT tissues of SPOP-mutated cohort and exhibited highly correlations with the upregulation of FH by integration of transcriptomics and metabolomics (Figure 4). Surprisingly, it was also found that SPOP mutations positively correlated with upregulation of FH based on cBioportal analysis (Supplementary Figure 3). Our findings revealed that the increase of fumarate and malate in PCT tissues might be mediated by SPOP mutations at the transcriptional level (Supplementary Figure 3).

As another key metabolic pathway, fatty acid metabolism is usually upregulated in PCa [44], which is consistent with our results that various metabolites and transcripts were markedly upregulated in SPOP-mutated PCT tissues. Among these transcripts, ACADL has been identified as a key modulator in fatty acid β-oxidation and its expression can contribute to the malignant phenotypes of PCa cells [45]. Fatty acid oxidation is an important energy supplement in PCa [46]. Moreover, the over-expression of FASN, a key enzyme involved in fatty acid biosynthesis, can promote the PCa progression [47]. In the present study, ACADL showed notable upregulation and strong correlation with most of fatty acid metabolites in PCT tissues with SPOP mutations. In addition, ELOVL2, an elongase of long-chain fatty acid, also exhibited the similar alterations with ACADL in SPOP-mutated tissues (Figure 3J, Supplementary Figure 1A, and Supplementary Figure 2). Of note, cBioportal database showed a highly positive correlation between SPOP mutations and the genetic alteration of both two genes in primary PCa (Supplementary Figure 3). Therefore, our data indicated that the elevated fatty acid metabolism in PCa might be affected by SPOP mutations.

Although FH, ELOVL2 and ACADL were recognized as key genes in SPOP mutated PCa patients in this study, their oncogenic roles still need to be proved in PCa. Previously, several studies have been reported that FH is frequently mutated in renal cancer [48], ELOVL2 is upregulated in hepatocellular cancer [49], and ACADL is associated with prostate cancer progression[45]. Moreover, AR and ERG are important substrates of SPOP. AR, a type of nuclear receptor that is activated by binding to the androgenic hormones, can regulate eukaryotic gene expression and affect cellular proliferation and differentiation. Importantly, AR is highly activated in prostate cancer and fuels prostate cancer by upregulating glycolysis and fatty acid metabolism [23]. Also, AR transcriptional activity is increased in SPOP mutated prostate cancer [50]. In addition, ERG is an oncogenic regulator, which can modulate citrate, polyamines and choline-associated metabolites in PCa [51]. In this study, we found that fatty acid metabolism and choline-associated metabolism were upregulated in SPOP mutated PCa patients.

Moreover, the data of transcriptomics and metabolomics between SPOP-WT and SPOP-mutated PCT tissues were also analyzed and several critical metabolic pathways during PCa development showed obvious differences (Figure 5A). Among these pathways, steroid hormone pathway has been reported to be associated with the risk of PCa progression [52]. In addition, several important transcripts related to fatty acid metabolic pathway, especially ECHS1, ACADSB and HADH, were remarkably upregulated in SPOP-mutated PCT tissues when compared to their matched ANT tissues as well as SPOP-WT PCT tissues (Figure 5B–5F). Furthermore, DAG 36:4, as an important diacylglycerol metabolite, also obviously increased in SPOP-mutated PCT tissue (Figure 5G). Although lipid accumulation and upregulated fatty acid metabolism were found in PCT tissues in an overall analysis [21, 22], our findings demonstrated that such changes were more significant in SPOP-mutated PCT tissue. Nevertheless, no many differential metabolites between SPOP-WT and SPOP-mutated PCT tissues were found, which was probably due to the small size of samples. Hence, large-scale population-based studies are needed to be performed to further explore the SPOP mutation-related metabolic pathways as well as the molecular mechanisms.

In summary, various metabolic pathways were demonstrated upregulation at both transcriptional and metabolic levels in PCT tissues by integration of transcriptomics and metabolomics as well as lipidomics. Furthermore, we found that three upregulated metabolic pathways in PCT tissues including TCA cycle, fatty acid metabolism and glycerophospholipid metabolism, showed intimate association with SPOP mutations. Our study provided new insights in understanding the relationship between SPOP mutations and metabolic pathways in PCa. However, only the comparison of SPOP mutated PCT and ANT tissues is not enough to obtain the SPOP regulated metabolic pathways. Here, only a few differential metabolites were found between SPOP mutated and non-mutated PCT tissues. Additionally, SPOP mutated patients also obtained some other genetic alterations, which could be the main reason why only got few differences between SPOP-mutated and SPOP-WT cancer tissues. Further research would be needed to better understand such relationship in a large number of SPOP-mutated PCa patients as well as by functional detection in vitro and in vivo.

MATERIALS AND METHODS

Chemicals, reagents, plasmids and transfection

Ultrapure water was prepared using Milli-Q water purify system (Millipore, Billerica, MA, USA). Some chemical standards including methyl tert-butyl ether (MTBE), pyridine, dichloromethane, methoxyamine hydrochloride, (N-methyl-N-(trimethylsilyl)-trifluoroacetamide (MSTFA), ammonium acetate, formic acid and ammonium bicarbonate were obtained from Sigma-Aldrich (St. Louis, MO, USA), and other standards such as LC or MS grade methanol, acetonitrile, chloroform and isopropanol were purchased from Merck (Darmstodt, Germany).

SPOP WT plasmid was kindly provided by Prof. Jiang Liu from Beijing Institute of Genome Research, Chinese Academy of Sciences. SPOP-mutated plasmids Y87N were kindly provided by Dr. Chenji Wang from Fudan University. SPOP WT, Y87N were cloned into Ploc.RFP vector with 3 × Flag label. TurboFect Transfection Reagent (Thermo Scientific; Waltham, MA, USA) was used for transfection.

Clinical sample collection and preparation

Totally, 66 patients were enrolled from Shanghai Changhai Hospital and wrote informed consent. The patient information of 66 PCa patients was listed on Table 1 with information of GS score, pathological stage and pathological progression, including SPOP-WT and SPOP-mutated PCa patients. All experimental protocols were approved by Institutional Review Board of the Shanghai Changhai Hospital, Second Military Medical University, Shanghai, China. All matched ANT and PCT tissues were obtained from surgery, flash-frozen in liquid nitrogen and kept at –80°C until analysis. Hematoxylin and eosin staining was used for histological diagnosis. In SPOP-WT and SPOP-mutated patient comparison, the SPOP-WT and SPOP-mutated patients were analyzed at the same batch by metabolomics and lipidomics studies and the patient information had been listed with SPOP-WT and SPOP-mutated PCa patients [21].

LC-MS based metabolomics and lipidomics analyses

LC-MS based metabolomics and lipidomics analyses of PCT and ANT tissues were performed as previously described [20, 21]. Briefly, the extraction of metabolites was performed using a system containing menthol, MTBE and water. ACQUITY™ Ultra Performance Liquid Chromatography (UPLC) system (Waters, Milford, MA, USA) was used for chromatographic separation, followed by global metabolomics and lipidomics profiling performed by a coupled AB Sciex tripleTOF 5600 plus mass spectrometer (Applied Biosystems Sciex, Foster City, CA, USA).

GC-MS based metabolomics analysis

GC-MS based metabolic profiling of PCT and ANT tissues was analyzed using GCMS-QP 2010 analytical system (Shimadzu, Kyoto, Japan) equipped with EI (electron impact) ionization source as previously described with slight modifications [53]. In brief, the extraction of metabolites was conducted using a system containing 80% menthol, water and 10 μg/mL tridecanoic acid on ice. Chromatographic separation of metabolites was performed on a DB-5 MS capillary column (J & W scientific, Folsom, CA, USA).

Transcriptomics analysis

The data of gene expression and somatic mutations were obtained using RNA-seq analysis as previously described [54]. Briefly, the total RNA was extracted by using TRIzol reagent and cDNA sequencing was performed by using Illumina Kit (San Diego, CA, USA) according to the manufacturers’ instructions. TopHat software was used to calculate the clean reason of RNA nucleotide sequences.

cBioportal data analysis

Genetic alteration frequency of SPOP, ACADL, ELOVL2, FH, ACTB and ERG in PCa was analyzed using cBioportal (http://www.cbioportal.org/index.do) [30, 31]. All searches were conducted according to the online protocols of cBioportal. Additionally, the correlation analyses between SPOP and FH, ELOVL2 as well as ACADL were performed based on their mutation and expression in primary prostate carcinomas (TCGA, Cell 2015).

Immunoblotting

Immunoblotting was performed as previously described [21]. Cells were prepared by RIPA (radio-immunoprecipitation assay) buffer with phosphatase inhibitors (Sigma). After vortex 30 s, cells were lysed at ice for 15 min and centrifuged at 12000 rpm for 15 min at 4°C. Supernatant was denatured and used for sodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE) separation. The proteins were then transferred to a polyvinylidene fluoride (PVDF) membrane (Bio-Rad; Hercules, CA, USA). Subsequently, the membranes were immunoblotted with the corresponding primary antibodies followed by peroxidase-conjugated secondary antibodies. The bonds were visualized by Chemiluminescence (Thermo Scientific; Waltham, MA, USA). SPOP (1:1000 Proteintech; 16750-1-AP), Flag (1:1000 Proteintech; 66008-2-Ig), GAPDH (1:2000 Cell Signaling Technology; #5174), FH (1:1000 Proteintech; 10966-1-AP), ELOVL2 (1:500 Abcam; EPR11880), ACADL (1:1000 Proteintech; 17526-1-AP) and Vinculin (1:2000 Sigma; V4505) antibodies were used in the study.

Real-time PCR

For real-time PCR analysis, mRNA was extracted by RNAiso Plus (Takara, Dalian, China). Then, the mRNA was reverse transcription to cDNA by PrimeScript™ RT reagent Kit with gDNA Eraser (Perfect Real Time) (Takara, Dalian, China). SYBR^® Premix Ex Taq™ (Tli RNaseH Plus) (Takara, Dalian, China) was used for quantitative analysis. The CFX96™ Real-Time PCR Detection Systems was used. The FH primers were: FH-F, GGAGGTGTGACAGAACGCAT; FH-R, CATCTGCTGCCTTCATTATTGC; ACTB-F; TGACGTGGACATCCGCAAAG; ACTB-R, CTGGA AGGTGGACAGCGAGG.

Data processing and statistics

For comparing the differential metabolites between the matched PCT and ANT tissues in SPOP-mutated patients in metabolomics and lipidomics profiling, two-sided Mann–Whitney U test was used and P < 0.05 was considered to indicate statistical significance. The heatmap was visualized using Multi Experiment Viewer (MeV, version 4.8.1) according to the ratios of normalized peak intensity between paired PCT and ANT tissues [55]. Two-sided Mann Whitney U test (Matlab, 2014b) was also used to find out the differential transcripts between 11 matched PCT and ANT tissues in SPOP-mutated patients. P-value was set less than 0.05 and fold change was set more than 2 or less than 0.5. A total of 1840 upregulated and 1926 down-regulated transcripts were used for gene set analysis by ConsensusPathDB (http://consensuspathdb.org/) [27], and KEGG [26] was used as database. Minimum overlap with input list was defined as 2 and P < 0.01 was set as statistically significant. The comparison of SPOP mutated and not mutated PCT tissues were calculated by two-sided Mann Whitney U test and P < 0.05 was considered statistical significance.

The ratios of metabolites and transcripts in PCT tissues to that in matched ANT tissues were calculated using normalized peak intensity of metabolites and gene expression data, respectively. The correlations between PCT to ANT ratio of transcripts and metabolites were analyzed based on PCC (Matlab, 2014b) and the correlation network was visualized using cytoscape (3.3.0) [56]. Human metabolome database (HMDB) was used to search for the functions of metabolites (http://www.hmdb.ca/) [57]. The networks between metabolites and genes were searched at KEGG (http://www.kegg.jp/kegg/) [26]. The Scatter plot is drawn by GraphPad Prism 5.

ACKNOWLEDGMENTS AND FUNDING

We thank members of the Dr. Piao and Dr. Xu laboratories for discussion, and H. Qi for editing the manuscript. This study has been supported by the National Key Research and Development Program of China (2017YFC0906900), Innovation program of science and research from the DICP, CAS (DICP TMSR201601) and the 100 Talents Program of Chinese Academy of Sciences.

CONFLICTS OF INTEREST

The authors declare no competing financial interests.

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