Immunohistochemical detection of mutations in the epidermal growth factor receptor gene in lung adenocarcinomas using mutation-specific antibodies

Samples for study were selected according to the following criteria: lung adenocarcinoma, surgically resected, primary, solitary and no preoperative therapy. A total of 50 cases were collected retrospectively and prospectively from the Department of Pathology, Peking University First Hospital during January 2010 to January 2012.

Informed consent for the use of these specimens for medical studies was obtained before surgery.

50 tissue blocks were cut into 4-μm-thick whole sections. EGFR mutation specific antibodies were Rabbit XP® mAbs obtained from Cell Signaling Technology (Danvers, MA), 6B6 specific for the E746-A750del mutation, and 43B2 for the L858R mutation. The antibodies were diluted 1:100 with antigen retrieval buffer before use. The antigen retrieval buffers tested were sodium citrate (pH 6.0), EDTA (pH 8.0) and EDTA (pH 9.0). Cytokeratin AE1/AE3 IHC was used as a quality control for tissue and protocol. The IHC protocol is described in greater detail in the Additional file 1.

Three sets of criteria were used for interpretation of the IHC results, referred to as Score A, B and C, respectively, in this study. A positive result using score A was moderate to strong staining of membrane and/or cytoplasm in >10% tumor cells[15]. A positive result using score B was membrane staining in >10% tumor cells with any intensity[10]. A positive result using score C was membrane and/or cytoplasmic staining in >50% of the tumor cells with any intensity[13]. In this study all 50 specimens were analyzed using Score A, B and C separately, so as to evaluate the validity of these scoring methods by comparing to the results of DNA sequencing. Both the intensity and percentage of stained cells were assessed at low magnification (objective magnification ×10). The distribution of staining, membrane or cytoplasm, was assessed at high magnification (objective magnification ×40). Four experienced pathologists (Yan Xiong, Ying Dong, Lin Nong and Jing Zhao) reviewed all of the slides independently, and then replicated the analysis 16 to 18 weeks later. The intra- and inter-observer reliability was analyzed.

Statistical analysis was done using the statistics software SPSS V16.0 (SPSS Inc., Chicago, IL). Fleiss’ Kappa was used to determine inter-observer agreement. Cohen’s Kappa was used to determine intra -observer agreement and agreement of IHC and DNA sequencing. A Kappa value between 0.81 and 1.0 was defined as nearly perfect agreement, between 0.61 and 0.8 as substantial agreement, between 0.41 and 0.60 as moderate agreement, between 0.21 and 0.40 as fair agreement, between 0.00 and 0.20 as slight agreement. For each Kappa, the 95% confidence interval (CI) was calculated. Difference was considered significant (P < 0.05), if the lower and upper boundary of the 95% CI showed no overlap.

All experiments above have been performed with the approval of Peking University First Hospital Ethics Committee.

In the total cohort of 50 samples L858R was identified in 16 cases, a deletion in exon 19 in 17 cases, and neither of them in 17 cases. Of the 17 cases with exon 19 deletion, 14 had a p.E746_A750del (c.del2235_2249 on the DNA level), one had a p.L747_T751del (c.2240_2254del), one had a p.L747_P753delinsS (c.2240_2257del), and one had a p.L747_T751delinsPT (c.2239_2253delinsCCAACG) that had not been previously reported. In our study, of all 33 cases with EGFR mutations, L858R and E746_A750del together comprised 90% (30/33) and the others, including L747_T751del, L747_P753delinsS and L747_T751delinsPT, comprised 10%, which was concordant with other studies[17]. From this point of view L858R and E746_A750del are recognized as the most common mutations and the other mutation types are described as uncommon mutations.

We evaluated three different antigen retrieval buffers on all 50 specimens to optimize the IHC results: sodium citrate (pH 6.0), EDTA (pH 8.0) and EDTA (pH 9.0). Slides in the EDTA (pH 8.0) group showed the best histological pictures with strongly specific staining and minimal background. The intensity of the positive cells in the sodium citrate (pH 6.0) group was too faint to distinguish from the background. Mesenchymal cells on slides exposed to EDTA (pH 9.0) were stained as strong as tumor cells, which made it impossible to identify the specificity of staining (Figure1). Inter-observer agreement was nearly perfect in the EDTA (pH 8.0) group, substantial in the sodium citrate (pH 6.0) group and moderate in the EDTA (pH 9.0) group. The Fleiss’ Kappa (95% confidence interval) was 0.912 (0.862, 0.962), 0.753 (0.677, 0.829), and 0.643(0.558, 0.728) in the three groups, respectively. The difference between EDTA (pH 8.0) and the others was significant (P < 0.05). Intra-observer agreement was highest in EDTA (pH 8.0), moderate in sodium citrate (pH 6.0), and lowest in EDTA (pH 9.0). The Cohen’s Kappa (95% confidence interval) was 0.955 (0.918, 0.992), 0.853 (0.790, 0.916), and 0.801 (0.730, 0.872), respectively. The difference between EDTA (pH 8.0) and the others was statistically significant (P < 0.05) (Table3).

The staining distribution included cytoplasm only or cytoplasm together with membrane. Normal tissue adjacent to adenocarcinoma was negative (Figure2). In the cases with lepidic pattern staining of lepidic tumor cells was either negative or fainter than the tumor cells of other patterns (Figure3). In our study, 80% of the cases were either negative or positive in 100% of the tumor cells, although the intensity was diverse ranging from + to +++. In only 20% of cases the tumor cells were stained in some areas and completely negative in other areas. Overall, the staining pattern showed characteristics of homogeneity more than heterogeneity.

Based on different scoring systems, the percentage of positive cases was different too. For L858R-specific IHC it was 28% (14/50) on Score A, 16% (8/50) on Score B, and 40% (20/50) on Score C; for E746_A750del-specific IHC it was 20% (10/50) on Score A, 14% (7/50) on Score B, and 24% (12/50) on Score C.

Of the 16 cases with L858R, the L858R-specific IHC was positive in 13 on Score A, 7 on Score B and 11 on Score C (Figure4). Of 34 cases without L858R the L858R-specific IHC was negative in 33 on Score A, 33 on Score B and 25 on Score C (Figure5). L858R-specific IHC showed a sensitivity of 81%, a specificity of 97%, a positive predictive value (PPV) of 93%, and a negative predictive value (NPV) of 92% on Score A; a sensitivity of 44%, a specificity of 97%, a PPV of 88%, and a NPV of 79% on Score B; and a sensitivity of 69%, a specificity of 74%, a PPV of 55%, and a NPV of 83% on Score C. Reliability analysis for L858R-specific IHC and DNA sequencing was found to be Cohen’s Kappa = 0.810 and 95% CI (0.701, 0.919) on Score A, Cohen’s Kappa = 0.470 and 95% CI (0.332, 0.608) on Score B, and Cohen’s Kappa = 0.397 and 95% CI (0.261, 0.533) on Score C. The agreement between L858R-specific IHC and DNA sequencing was the best using Score A compared to Score B and C. The difference was significant (P < 0.05) (Table4).

Of 14 cases with the E746_A750del by DNA sequencing E746_A750del-specific IHC was positive in 10 on Score A, 7 on Score B, and 9 on Score C (Figure6). All of the 3 cases with uncommon types of exon 19 deletion, includingL747_T751del, L747_P753delinsS and L747_T751delinsPT, were negative by E746_A750del-specific IHC regardless of the scoring method.

Including all 17 specimens with an exon 19 deletion detected by DNA sequencing, the E746_A750del-specific IHC found 10 (59%) were positive and 7 (41%) negative on Score A, 7 (41%) were positive and 10 (59%) negative on Score B, 9 (53%) were positive and 8 (47%) negative on Score C. Of the 33 cases without an exon 19 deletion detected by DNA sequencing all were negative by E746_A750del-specific IHC both on Score A and B (Figure5), while 3 were positive on Score C. As a method to detect deletions in exon 19 despite the exact structure of the deletion, E746_A750del-specific IHC showed a sensitivity of 59%, a specificity of 100%, a PPV of 100%, and a NPV of 82% on Score A; a sensitivity of 41%, a specificity of 100%, a PPV of 100%, and a NPV of 77% on Score B; and a sensitivity of 53%, a specificity of 91%, a PPV of 75%, and a NPV of 79% on Score C. Reliability analysis for E746_A750del-specifiac IHC and DNA sequencing was found to be Cohen’s Kappa = 0.653 and 95% CI (0.521, 0.785) on Score A, Cohen’s Kappa = 0.480 and 95% CI (0.342, 0.618) on Score B, Cohen’s Kappa = 0.472 and 95% CI (0.334, 0.610) on Score C. Similar to L858R-specific IHC the agreement between E746_A750del-specific IHC and DNA sequencing was the best using Score A compared to Score B and C, but the difference was not significant (P > 0.05) (Table5).