Defining the value of CD56, CK19, Galectin 3 and HBME-1 in diagnosis of follicular cell derived lesions of thyroid with systematic review of literature

This tissue microarray based study is a unique in a methodological way because it gives information of expression of investigated markers on tumour front. It provides answers to questions asked in introductory part of this paper. We provided the readers with extensive review of literature on the subject, with fast insights in methodological approach, cut off values and results of reviewed studies.

All analysed immunomarkers may make a difference between benign lesions/tumours from differentiated thyroid carcinomas. CK19 and HBME-1 can differentiate between papillary carcinoma and follicular carcinoma. Expression of all markers is significantly higher in papillary carcinoma than in follicular adenoma. Galectin-3 could not distinct papillary from follicular carcinoma. CD56 and Galectin-3 could not differentiate between follicular variant of papillary carcinoma and follicular carcinoma. Interestingly, Galectin-3 and CD56 made statistically significant difference between follicular carcinoma and follicular adenoma. The only marker which makes statistically significant difference between adenoma and carcinoma of Hurthle cells was Galectin 3. Best balanced marker in our study, in terms of sensitivity and specificity for malignancy, was HBME-1. The most sensitive marker was Galectin 3, and the most specific marker in our study was CD56. Former mentioned marker, at the same time, had the lowest specificity, and latter had the lowest sensitivity of all. When we combined two, three or four co-expressed markers, we did not reach specificity of 100 % for malignancy, nonetheless values increased compared to single marker expression. On the other hand, the unfavourable result was lowering of sensitivity for malignancy, compared with use of single marker. The best combination of co-expressing markers for identifying malignancy was HBME-1 and Gal-3. Best discriminatory combinations of markers for papillary carcinoma from follicular adenoma, and non-neoplastic lesions were CD56 with Galectin 3, and CK19 with Galectin 3, respectively. For discriminating follicular variant of papillary carcinoma from follicular adenoma or carcinoma, best combinations were CK19 with Galectin 3, and CD56 with HBME1, respectively.

Cytokeratin 19 is the smallest member of cytokeratins family, a heterogeneous group of intermediate filaments. Physiologically, it is expressed in simple and glandular epithelia, basal layer of stratified epithelium, and in hair follicles [12]. Healthy thyroid follicular cells do not produce this protein, and upregulation of CK19 is connected with neoplastic transformation. Strong and diffuse immunoreactivity of CK19 is most often related to papillary thyroid carcinoma [13].

Our result show that CK19 is overexpressed in papillary thyroid carcinoma, diffusely and intensively in most cases. Overexpression of this marker is related not just to PTC, but to malignancy. Discouraging thing, is that serious number of benign cases also expressed CK19, although focally and weakly. Only hyperplastic adenomas were completely negative in our investigation.

We reviewed 23 papers [10, 11, 14‐34], and than recalculated average sensitivity and specificity for carcinomas (80 %, 78 % respectively). The results of our study are in concordance with the results from majority of papers we have reviewed. Sensitivity values varied from 13 to 100 % (median_sens = 84 %), while specificity values varied from 0 to 100 % (median_spec = 75 %) (see Table 9). Control group non tumor tissues, follicular adenoma, follicular carcinoma, and papillary carcinoma had positive expression of this marker which varied from study to study: 4–89 % (median = 20 %); 0–100 % (median = 24 %); 0–50 % (median = 40 %); 46–100 % (median = 95 %), respectively.

Generally, studies showed that CK19 is more expressed in malignant lesions than in benign follicular cells derived thyroid lesions [14, 15]. The expression of CK19 in papillary carcinoma (general) and follicular variant PTC was significantly higher than in follicular thyroid carcinoma (FTC) [15]. Further, it can serve to differentiate papillary thyroid carcinoma from follicular adenoma [31], but can not help in differentiation between follicular adenoma and follicular carcinoma [30, 10]. Also, it does not make difference between follicular carcinoma and normal tissue [26].

In the end, we may make few conclusions: CK19 can help in diagnosis of papillary thyroid carcinoma, but one must take into account the intensity and distribution of marker within the tumour; CK19 intensive immunoreactivity, plus missing criteria for PTC, should alert on possibility of malignancy; due to its relatively low specificity, we recommend the use of marker in combination with others.

HBME1 (Hector Battifora Mesothelial 1), is monoclonal antibody which reacts with uncharacterized antibody in microvilli of mesothelial cells. HBME-1 has been assessed in thyroid with the aim to help in differentiation of benign from malignant lesions.

HBME-1 is more expressed in malignant lesions compared to benign lesions [10, 14, 15, 18, 23, 25, 32, 35]. Benign lesions expressed HBME-1 focally, rather than diffusely. It is more extensively expressed in papillary carcinomas compared to follicular carcinomas and follicular adenomas [18, 25]. Follicular variant of papillary carcinoma has significantly higher expression of this marker than follicular adenoma or follicular carcinoma [25, 31]. The aforementioned studies and their results are in concordance with our study. The results of a few other studies were showing higher expression of HBME-1 in follicular carcinoma than in follicular adenoma. [10, 27, 32, 35], which is not the case with results of our study and some other studies [15, 25, 31]. When we pulled out all the results of expression of HBME-1 in follicular adenomas and follicular carcinomas from reviewed studies, and made comparison of those two groups, we have obtained significant difference in expression between two above mentioned groups (Fisher’s exact test, the two-tailed P value is less than 0.0001).

Among 25 reviewed studies [10, 11, 14‐19, 22‐25, 27, 28, 31, 32, 34‐42], the sensitivity and specificity of this marker varied markedly (34–100 % for sensitivity, 54–100 % for specificity), with average sensitivity of 76 % and specificity of 87 % for carcinomas compared to benign lesions (median_sens = 77 %; median_spec = 89 %). Control non tumor tissues showed positive expression of this marker in the range 0–35 % (median = 10 %) of cases. Follicular adenomas, follicular carcinomas and papillary carcinomas through the studies show positive expression in given ranges: 0–56 % (median = 25 %); 17–100 % (median = 65 %); 55–100 % (median = 92 %), respectively. The increasing trend of expression is noticeable, starting from non-tumour tissues to papillary carcinomas.

Simultaneous immunopositivity for HBME-1 and Galectin 3, and HBME-1 and CK19 in the diagnosis of differentiated thyroid carcinoma have sensitivities of 85,9 %, and 86.4 % respectively, and specificities of 100 % for both combinations. Specificities values increased, but sensitivities values decreased comparing to single markers values [10].

Co-expression of HBME1 and CK19 has a sensitivity of 83 % and specificity of 100 % of diagnosing papillary carcinoma compared to follicular adenoma. Opposite, the HBME1-CK19 negative staining for both markers was highly indicative of follicular adenoma (99 % specificity and 82 % sensitivity) [16].

The combined use of HBME-1 and Gal-3 was able to improve sensitivity up to 99 % and specificity up to 80 % in diagnosis of malignant Hurthle cell tumours compared to Hurthle cell adenomas [41].

Galectin 3 is a structurally unique member (31-kDa) of galectins family. Galectin-3 is capable to make cross links with cell membrane glycoproteins, thus forming new network involved in cellular signaling and receptors endocytosis. Galectin 3 is detected in nucleus, cytoplasm and in extra cellular space. Galectin 3 plays roles in apoptosis regulation, cell motility, and it is involved in thyroid carcinoma progression [43, 44].

Long ago, Xu et al. [44], had been investigating expression of Galectin 1 and Galectin 3 in small series of thyroid tumours, and they had found expression in papillary and follicular carcinomas, but not in adenomas, nodular goiter, nor in normal thyroid tissue. On the grounds of those investigations they deduced that galectins could bu useful in making distinction between benign and malignant thyroid tumours [44].

Expression of Galectin 3 is higher in malignant compared to benign thyroid lesions [10, 14, 15, 18, 23, 25, 35]. Some authors found difference in expression of Galectin 3 between papillary carcinoma, and its follicular variant, compared to follicular carcinoma [10, 25, 31]. Nevertheless, others have not found those differences, including here the results of our study too [15, 35]. Galectin 3 have been found to have higher immunoreactivity in papillary (also follicular variant) carcinoma compared to follicular adenoma [15, 25, 27, 31, 35], which is comparable to our results. Few studies, including the current, found difference in expression of Galectin 3 between follicular carcinoma and follicular adenoma [10, 35]. Galectin 3 was the only marker able to make a difference between Hurthle cell carcinoma and adenoma, which is also confirmed by the study of Volante M et al. [41].

Having made insight in data from reviewed studies [15‐19, 23‐32, 35, 36, 41, 45‐60], once again, we have noticed high variability in sensitivity and specificity for carcinoma of this marker. The values of sensitivity have varied from 8–100 % (median = 88 %), and 40–100 % (median = 82 %) for specificity. The average values were not much different from median values (84 %; 83 %).

The percent of immunopositive cases for control groups (non-tumour), follicular adenomas, follicular carcinomas and papillary carcinomas have varied greatly: 0–52 %(median = 8 %);0–63 %(median = 17 %); 8–100 %(median = 66 %); 46–100 %(median = 93 %), respectively.

Three markers co-expression (HBME1,Gal-3,CK19) had sensitivities of 83 %, 87 %, and 54 % as well as specificities of 100 %, 89 % and 100 %, respectively [14, 16, 27]. Concurrent absence had sensitivity of 38% and specificity of 100 % for benign [14].

In the study of Zhu X et al. [15], more than three immunohistochemical markers were simultaneously positive in 100 % of PTC cases and in 0–30 % of patients with other types of disease.

CD56 is a neural cell adhesion molecule (NCAM), which is expressed normally in thyroid follicular cells. Reduced CD56 expression is correlated with tumour progression of patients with cancer. Its expression is reduced, or totally lost, in cases of papillary carcinoma, follicular carcinoma and anaplastic carcinoma [61‐63].

The results of our study showed that malignant tumours had lost or expressed CD56 less than benign thyroid lesions, which is in agreement with previously published data [64‐66]. CD56 expression is more reduced in papillary carcinomas in respect to follicular carcinomas and follicular adenomas [62, 63].

On the other side, we had not found significant difference in CD56 expression between follicular variant of papillary carcinoma and follicular carcinoma what is partially supported with results of other study [67]. Intriguingly, we found the difference in expression between follicular carcinoma and follicular adenoma, which is in disagreement with results of other authors [62‐64]. If we connect previous information with findings that follicular carcinomas has significantly reduced expression of CD56 relative to benign follicular lesions we could conclude that reduces expression of CD56 is not exclusive property of papillary carcinoma.

Variation among studies in respect to sensitivity and specificity was substantial [11, 61‐66, 68, 69]. Sensitivity for carcinoma varied from 58 to 100 % with a median value of 84 % (recalculated average value for all studies is 80 %). Specificity values ranged from 46 to 100 %, with a median value of 92 % (recalculated average value for all studies is 93 %).

The highest sensitivity this marker shows for papillary carcinoma, and the lowest for follicular carcinoma.

Having in mind that we have obtained tissue cores from tumour periphery, our results could be substantiated by the results of other studies [61, 62], which found that within the PTC groups, occasional CD56-positive cells were identified, and in all cases, these cells were located at the tumour/non-tumour interface. Therefore, the low value of sensitivity (58 %) of CD56 in our investigation might be the result of tissue sampling.

Nechifor-Boilă A et al. [11] found that panels consisting of CD56 and/or CK19/Gal-3 (they used Gal-3/CK19 formula because similar results were obtained in the panels containing either CK19 or Gal-3), and CD56 and/or HBME-1 had highest sensitivities (90.9 %) and negative predictive values (87.5 and 83.3, respectively), while the most specific combination of markers was represented by association of HBME-1 with CK19/Gal-3 (72.7 %) in identifying PTC cases. The panel consisting of CD56 and/or HMBE-1 was highly sensitive and specific (100 %, 90 %) in differentiating cases of FVPTC from benign thyroid lesions/tumours. When three-marker panels were evaluated, the best combination for FVPTC cases was HBME-1, CD56 and/or CK19, with a sensitivity reaching 91.1 % [69]. In the studies of Mi KS et al. [66] and W Y Park et al. [63], sensitivities were 93,8 % and 88.1 % and specificities were 90.9 % and 93.8 % respectively, to distinguish PTC from other benign thyroid lesions with the combination of three markers CD56, GAL3, and CK19.

This marked heterogeneity of diagnostic value of investigated markers could stem from few reasons. Primarily, cut off values varied from more than 0 to 25 % of positive cells. Secondarily, some study designs included other tumours beside well differentiated thyroid carcinomas. Further, there is still no consensus about technical points, e.g., HMBE-1 membranous and/or cytoplasmatic staining delivers significant amount of freedom in deciding what is positive. Lastly, some studies employed TMA, others not. At the end, there are results which showed that more than one marker could be co-expressed even in benign lesions, which oblige us to continue the quest of searching more reliable markers. Until then, H&E slides stays golden standard in diagnostics of follicular cells thyroid lesions.

It will not be fair not to mention weaknesses of this study. We shed some light to tumour/normal tissue interface, but we did not have proper representatives of tissue from tumours core. The number of cases, especially Hurthle cell adenomas, and follicular adenomas, was borderline. Some authors also claim that is mistake to include Hurthle cell tumours, but from practical standpoint, because we experienced real dilemmas if tumour is papillary carcinoma (oncocytic variant) or Hurthle cell adenoma for example, we included those tumours also.