Seventy-eight consecutive eligible CHB patients who underwent a liver biopsy in March 2006-August 2008 at Zhongshan Hospital, Fudan University, Shanghai, China, were included in this study. Blood serum was collected and stored at -80°C for further test. Chronic HBV infection was diagnosed based on positive surface antigen of HBV (HBsAg) and fluctuated alanine aminotransferase. Exclusion criteria included chronic liver disease due to other causes or co-infection with hepatitis D, clinically overt cirrhosis, previous or concomitant anti-HBV therapy, alcohol consumption exceeding 20 g/d in men and exceeding 10 g/d in women. Data were retrospectively analyzed. The study protocol was approved by the Institutional Review Board in our hospital. Written informed consent was obtained from each patient.

Liver tissue was obtained by sono-guided percutaneous biopsy (Bard^®, Magnum^®, 18G, USA) and stained with hematoxylin-eosin-safran and Masson’s trichrome. Fibrosis staging (F) and inflammatory activity (A) were decided according to the METAVIR system. Fibrosis staging was divided into F0-F4 (F0 = no fibrosis, F1 = portal fibrosis without septa, F2 = periportal fibrosis with few septa, F3 = septal fibrosis with many septa, and F4 = cirrhosis). Inflammatory activity was divided into A0-A3 (A0 = no histologic necroinflammatory activity, A1 = minimal activity, A2 = moderate activity, A3 = severe activity). The activity was assessed by integrating the severity and intensity of piecemeal (periportal) and lobular necrosis[13]. According to the American Association for the Study of Liver Disease Practice Guidelines, we defined significant fibrosis as METAVIR fibrosis with a score ≥ 2 (F2, 3, 4) and severe liver fibrosis as METAVIR fibrosis with a score ≥ 3 (F3, 4)[14].

Following parameters, including AST, alanine aminotransferase (ALT), γ-glutamyl transpeptidase (GGT), bilirubin, total cholesterol, urea, prothrombin time (PT), prothrombin index (PI), hemoglobin and platelet count (PLT) were assayed. AST, ALT, GGT, bilirubin, total cholesterol, urea were tested with Hitachi 7600, Japan. PT and PI were tested with Sysmex CA7000, Japan. Hemoglobin and PLT was tested with Sysmex routine blood test pipeline, Japan. The reference value was 0-75 IU/L for ALT and AST. Serum α₂-macroglobulin (A₂M) (GenWay Biotech, San Diego, USA) and hyaluronic acid (HA) (Shanghai High Medical Biotech, Shanghai, China) concentrations were measured by enzyme linked immunosorbent assay.

APRI, FIB-4, Forn’s index, SLFG, Hepascore, and Fibrometer were detected according to the following formulas: APRI = [AST (/ULN)/PLT (10⁹/L)] × 100, FIB-4 = [age (yr) × AST (U/L)]/{[PLT (10⁹/L)] × (ALT (U/L)]^1/2}, Forn’s index = 7.811 - 3.131 × ln [PLT (10⁹/L)] + 0.781 × ln [GGT (U/L)] + 3.467 × ln [age (yr)] - 0.014 × [cholesterol (g/L)], SLFG = 10 × e^Y/(1+e^Y), Y = - 13.995 + 3.220 × lg [A₂M (g/L)]+ 3.096 × lg [age (yr)] + 2.254 × lg [GGT (U/L)] + 2.437 × lg [HA (ng/mL)], Hepascore = e^Y/(1+e^Y), Y = - 4.185818 - [0.0249 × age (yr)] + [0.7464 × sex (male = 1, female = 0)] + [1.0039 × A₂M (g/L)] + [0.0302 × HA (ng/mL)] + [0.0691 × TB (μmol/L)] - [0.0012 × GGT (U/L)]; Fibrometer = - 0.007 × PLT (10⁹/L) - 0.049 × PI (%) + 0.012 × AST (U/L) + 0.005 × A₂M (g/L) + 0.021 × HA (ng/mL) - 0.270 × urea (mmol/L) + 0.027 × Age (yr) + 3.718.

Statistical analysis was performed using Spearman’s two-tail test and univariate analysis. P < 0.05 was considered statistically significant. Sensitivity, specificity, positive and negative predictive values (NPV and PPV) were calculated by using cutoffs according to the original studies. The overall diagnostic performance of scores was evaluated by area under ROC curves (AUROCs). We used DANA method, which was developed by Poynard et al[15,16], to adjust the observed AUROCs in our study. All the AUROCs were adjusted to a standard DANA of 2.5 using the formula: Adjusted AUROC (AdAUC) = Observed AUROC + 0.1056 × (2.5 - Observed DANA). The AUROCs were compared with the method of Hanley-McNeil[17].

The mean age of the 78 patients (66 males, 12 females) was 32.6 ± 12.3 years. The mean length of liver biopsies was 18.2 ± 3.4 mm, and the liver specimen length was longer than 15 mm. Significant fibrosis was found in 32 patients (41.0%), severe fibrosis in 19 patients (24.4%), and early cirrhosis in 9 patients (11.5%), respectively. Main features of the patients are summarized in Table 1.

METAVIR fibrosis stages were significantly correlated with APRI, FIB-4, Forn’s index, Fibrometer, Hepascore and SLFG. A better correlation was observed between Fibrometer (r = 0.69), SLFG (r = 0.68) and Hepascore (r = 0.62) (P < 0.001). The box-plots of fibrosis scores are shown in Figure 1. A correlation was also found between scores and histological activity, especially between SLFG (r = 0.55), Fibrometer (r = 0.54) and APRI (r = 0.51) (P < 0.001).

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Figure 1 Model values according to METAVIR fibrosis stages. The top and bottom of each box are the 25th and 75th centile interval, the line through the box is the median and the error bars are the 5th and 95th centile interval. 1 and 2 indicate the extreme values.

The mean levels of AST, GGT, PT, PI, A₂M and HA were higher in patients with F2-F4 fibrosis than in those with F0-F1 fibrosis (P < 0.01). The mean levels of hemoglobin, PLT and albumin were lower in patients with F2-F4 fibrosis than in those with F0-F1 fibrosis (P < 0.01). Multiple regression analysis showed that A₂M and HA were the independent factors for significant fibrosis (A₂M, OR = 5.36, 95% CI: 1.58-18.13, P = 0.007; HA, OR = 1.01, 95% CI: 1.00-1.02, P = 0.007). AUROC was used to evaluate the overall diagnostic performance of scores (Table 2).

The APRI, FIB-4, Forn’s index, Hepascore, SLFG and Fibrometer were 0.71, 0.75, 0.79, 0.80, 0.83, and 0.85 respectively under the AUROC for F0-F4 (Figure 2A), and 0.75, 0.79, 0.83, 0.84, 0.86, and 0.88 respectively under the adjusted AUROC for F0-F4 with DANA method. The AUROC for Fibrometer, SLFG and Hepascore was better than that for APRI and FIB-4 (P < 0.01).

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Figure 2 ROC curves for the 6 fibrosis models to discriminate METAVIR fibrosis stages F0-1 from F2-4 (A) and F0-2 from F3-4 (B).

The APRI, FIB-4, Forn’s index, Hepascore, SLFG and Fibrometer were 0.80, 0.87, 0.86, 0.95, 0.93, and 0.94 under the AUROC for F0-F4 (Figure 2B). The Hepascore, Fibrometer and SLFG levels were significantly higher than the APRI level under the AUROC for F0-F4 (P < 0.01).

NPV and PPV for the diagnosis of significant fibrosis are presented in Table 3. Cutoffs were chosen for each model as previously described. This analysis could not be performed for Fibrometer since no cutoff was provided in the study by Calès et al[10]. When different cutoffs were used for each model, the percentage of classifiable subjects was 45%-78%, with a diagnostic accuracy of 67%-86% (Table 4). Significant fibrosis (F2-4) was predicted in 13%-32% of patients with their PPV ranged 62%-88%. Since lower cutoffs were originally described to rule out significant fibrosis, attention must be paid to NPV ranging 76%-85%. The best positive predictive value (PPV = 0.88) for significant fibrosis was observed when SLFG > 8.7.

Clinically, developing noninvasive methods for diagnosing liver fibrosis is important. Noninvasive models have been established most in hepatitis C patients.

Noninvasive models have been proposed for the assessment of liver fibrosis. These models have been evaluated at many medical centers in chronic hepatitis C (CHC), but few in chronic hepatitis B (CHB). In this study, the efficacy of 6 noninvasive models was evaluated and the more valuable models were identified for predicting liver fibrosis in CHB.

The efficacy of 6 noninvasive models was evaluated in a cohort of Chinese patients with CHB. The results indicate that their efficacy is not influenced by ethnic and virus factors. This study also showed that the serologic models containing direct serum markers, such as hyaluronic acid (HA) and α₂-macroglobulin (A₂M) have better diagnostic values in CHB patients than in those not containing direct serum markers.

Noninvasive models can be used in diagnosis of liver fibrosis in patients with CHB in China or in Asia.

DANA method: A method used to adjust the differences caused by the prevalence of fibrosis stages. Standard prevalence is defined as a prevalence of 0.20 for each of the five stages.

The study adds information that helps establishment of strategies against liver fibrosis diagnosis using noninvasive methods. The study was scientifically designed. The manuscript is logical and readable.