Serum lipidomic profiling as a useful tool for screening potential biomarkers of hepatitis B-related hepatocellular carcinoma by ultraperformance liquid chromatography–mass spectrometry

A total of 87 patients with chronic hepatitis B (CHB) were enrolled from 2012 to 2014 at the Hospital das Clínicas of the University of Sao Paulo School of Medicine, including 32 patients with HBV-HCC, 30 patients with HBV-LC and 25 patients with CHB. Additionally, 34 eligible blood donors with normal liver function and no infectious diseases were recruited at COLSAN Beneficent Association for Blood Collection to serve as healthy controls. CHB was diagnosed based on the presence of HBsAg for at least 6 months. LC was diagnosed by histopathology, clinical features and/or elastography and HCC was diagnosed using imaging or histopathology techniques, in accordance with guidelines of the Brazilian Society of Hepatology.

Blood samples were obtained by venipuncture and drained into blood collection tubes. The samples were centrifuged immediately after collection and serum was stored at −80 °C until analysis.

Demographic, clinical and laboratory data were collected from medical records. The study was approved by the ethics committee of human research of the Federal University of Sao Paulo and the University of São Paulo School of Medicine (2012/81656 and 2014/569922) and all patients gave written informed consent.

Lipids were extracted from each sample using a modified Bligh-Dyer protocol [13]. Immediately after thawing, 100 μL of serum were dissolved in 850 μL of a mixture of water/chloroform/methanol (1:2.5:5, v/v) and vortexed well for 5 min. After vortexing, 250 μL of chloroform were added and the tubes were agitated for 15 min at 700 rpm. Then, 200 μL of deionized water were added and the tubes were centrifuged at 14,000 rpm for 15 min at room temperature. Following this protocol a 2-phase system (aqueous top, organic bottom) was achieved. The bottom phase containing lipids was gently recovered using a micropipette, dried, and resuspended in 350 μL of acetonitrile/water (3:2, v/v). All chemicals were of analytical reagent grade and used as received.

Reversed-phased analysis was performed on a Waters ACQUITY IClass UPLC system equipped with a Waters Acquity CSH C18 1.7 μm x 2.1 × 100 mm column coupled to a Waters Synapt-MS hidrid quadrupole-time of flight mass spectrometer operating in the positive ion electrospray mode. A mass scan range of 200 to 1,200 mass-to-charge ratio (m/z) was set for data acquisition in continuous mode with optimized parameters for ionization and mass transmission. Acetonitrile/water (3:2, v/v) was used as mobile phase A and isopropanol/acetonitrile (9:1, v/v) was used as mobile phase B, both with 10 mM ammonium formate and 0.1 % formic acid as additives. The flow rate was set at 600 μL/min and the injection volume was 10 μL. A binary gradient was optimized as follows: the composition of mobile phase B was changed from 15 % to 30 % in 2 min, then to 48 % in 30 s and reached 82 % in 8.5 min. Subsequently, it was changed to 99 % in 30 s, held for another 30 s and then dropped to 15 % in 6 s prior to being held until a total run time of 15 min. The mass spectrometer was previously calibrated with 0.1 % phosphoric acid in water/acetonitrile (1:1, v/v) and a solution of 0.5 ng/μL leucine enkephalin in water/acetonitrile (1:1, v/v) with 0.1 % formic acid infused in the reference probe at a flow rate of 5 μL/min was used as lock mass spray at a 30 s frequency for accurate mass determination. All analyses were acquired using the lock spray and the instrument was recalibrated every 4 run-hours to ensure accuracy and reproducibility. Furthermore, a quality control of pool plasma samples was analyzed after every 10 runs, and 10 peaks well distributed from 200 to 1,200 m/z were assessed.

For multivariate analysis, the unsupervised principal component analysis (PCA) was first utilized in all samples (Additional file 1). Supervised partial least-squares-latent structure discriminate analysis (PLS-DA) was then performed to identify biomarkers that contributed to the clustering. Validation with a permutation test and 100 repetitions was performed to prevent model overfitting. Potential biomarkers that differentiated HCC from LC, CH and healthy subjects (HS) were selected based on the variable importance in the projection (VIP) values and univariate statistical significance after Mann–Whitney test and fold-change analyses. Receiver operating characteristic (ROC) curves were performed to evaluate the accuracy of the potential biomarkers and the proposed model using the ROCCET (The Metabolomics Innovation Centre, Canada).

Statistical analyses of demographic, clinical and laboratory data of subjects were performed using SPSS version 11.0 (SPSS Inc., Chicago, IL, USA). Descriptive statistics consisted of the characterization of the studied population (demographic, clinical and laboratory characteristics) through the respective percentages or mean/median and standard deviation (SD) for continuous variables. Bivariate analysis consisted of Fisher exact test to compare categorical values. For continuous variables, Student’s t-test was use to compare means of normally distributed variables, while non-normally distributed variables were subjected to Mann–Whitney U test. Statistical significance level was P < 0.050. All reported values are 2-tailed.

A tentative identification of the differentiating lipids was performed on the LIPID MAPS and HMDB databases.

Four lipids independently predicted HCC from LC with 65.6–84.4 % sensitivity, and 60.0–76.7 % specificity. Figure 3 shows the intensities and ROC curves of the 4 lipids in patients with HCC and LC.

Based on the efficiency of the ROC curves, cutoff values were determined for each ion. The number of “positive” ions in each sample was used to generate a 4-peak algorithm with cutoff value of at least 2 “positive” biomarkers, defined by ROC curve analysis and posterior univariate statistical validation (Fig. 4a). The 4-peak algorithm generated distinguished HCC from LC with an accuracy of 71.0 % (95 % CI 58.7–80.1 %), a sensitivity of 78.1 % (95 % CI 61.2–89.0 %), and a specificity of 63.6 % (95 % CI: 45.4–78.1 %). This algorithm successfully detected 25 of 32 HCC cases when applied to discriminate HCC from LC.

Conversely, AFP detected only 12 of 32 HCC cases from LC when cutoff value was set as 20 ng/mL, showing an accuracy of 64.5 % (95 % CI 52.1–75.3 %), a sensitivity of 37.5 % (95 % CI 22.9–54.8 %), and a specificity of 93.3 % (95 % CI: 78.7–98.2 %). In the range of 200 ng/mL, AFP detected 6 of 32 HCC cases, performing with an accuracy of 58.1 % (95 % CI 45.7–69.5 %), a sensitivity of 18.8 % (95 % CI: 8.9–35.3 %), and a specificity of 100 % (95 % CI 88.7–100.0 %) (Table 3).

The combination of the 4-peak UPLC-MS algorithm with AFP in the range of 20 ng/mL was able to distinguish HCC from LC with an accuracy of 79.0 % (95 % CI 67.4–87.3 %), a sensitivity of 75 % (95 % CI 57.9–86.8 %), and a specificity of 83.3 % (95 % CI: 66.4–92.7 %).

The 4 peaks independently predicted HCC from CHB with 52–90.6 % sensitivity and 68.8–86.7 % specificity. The intensities and ROC curves of the 4 lipids in patients with HCC and CHB are shown in Additional file 3. The 4-peak algorithm distinguished HCC from CHB with an accuracy of 87.1 % (95 % CI 76.6–93.3 %), a sensitivity of 93.8 % (95 % CI 79.9–98.3 %), and a specificity of 80.0 % (95 % CI 62.7–90.5 %) (Table 3).

As the ion RT 4.26_540.4255 m/z did not perform well in this comparison, we also tested the performance of the model using different combinations of the 4 ions. The best model was a combination of the ion RT 1.30_498.8315 m/z and RT 1.32_497.5731 m/z, which with a cutoff of at least 1 “positive” ion, detected 31 of the 32 HCC cases and distinguished HCC and CHB with an accuracy of 88.7 % (95 % CI 78.5–94.4 %), a sensitivity of 96.9 % (95 % CI 84.26–99.5 %), and a specificity of 80.0 % (95 % CI 62.7–90.5 %) (Fig. 4b).

We also looked at the whole lipidomic profile of HCC and CHB and, interestingly, 7 peaks independently predicted HCC from CHB with 100 % sensitivity and specificity (Additional file 4).

Table 4 shows the main classes and subclasses associated with the differentiating lipids found in this study.