Regulation of LCoR and RIP140 expression in cervical intraepithelial neoplasia and correlation with CIN progression and dedifferentiation

Immunohistochemical quantification of LCoR and RIP140 expression was obtained in the embedded samples of cervical dysplasia (CIN I–III). Immunohistochemical staining was obtained as described in earlier publications (Hester et al. 2019; Vattai et al. 2017). Tissue samples were surgically generated and instantly fixed in neutral buffered formalin (3.7%) followed by standardized paraffin bedding. Immunohistochemistry was initiated by deparaffinization of the formalin-fixed paraffin embedded tissue slices (3 µm) in xylol. Inactivation of endogenous peroxidase was obtained with 3% H₂O₂ in methanol for 20 min followed by a descending ethanol gradient for rehydration of the slides. Next, a pressure cooker filled with sodium citrate buffer (pH 6.0) was used to prepare the tissue for epitope retrieval. To prevent non-specific binding of the primary antibodies, blocking solution was applied. The tissue slides were incubated over night for 16 h consecutively with the following antibodies: anti-LCoR (polyclonal rabbit IgG, Novus Biologicals, Littleton, USA) and anti-RIP140 (polyclonal rabbit IgG, Sigma Aldrich, St. Louis, USA). Analyzation of the antibody reactivity was obtained with the ZytoChemPlus HRP Polymer System (mouse/rabbit) (Zytomed Systems, Berlin, Germany) according to the manufacturer’s protocol. Substrate and chromogen (3,3′-diaminobenzidine DAB; Dako, Glostrup, Denmark) was applied on the samples. Counterstaining was obtained with Mayer’s acidic hematoxylin. After dehydrating the slides in an ascending row of ethanol, the slides were cover slipped. Both nuclear and cytoplasmic staining of LCoR and RIP140 were further correlated with EP3 staining which has been carried out and published previously (Hester et al. 2019).

Analyzation of cervical dysplasia tissues was conducted by two different and independent observers using Leitz Diaplan microscope (Leitz, Wetzlar, Germany). To quantify each slide’s staining, the semiquantitative immunoreactive score (IRS) was used. Intensity and distribution pattern of the antigen are optically evaluated with the immunoreactive score (IRS) (Remmele and Stegner 1987). It was calculated by multiplying staining intensity (0: none; 1: weak; 2: moderate; 3: strong) with the number of positively stained cells (in %) (0: no staining, 1: < 10% of the cells; 2: 11–50%; 3: 51–80%; 4: > 80%). A scale from 0 (no expression) to 12 (very high expression) was used. Photos were taken with a CCD color camera (JVC, Victor Company of Japan, Japan).

For data analysis IBM SPSS Statistics for Windows, Version 25, was used. P values p < 0.05 were considered statistically significant. Comparative analysis between different grades of CIN was obtained using nonparametric Kruskal–Wallis rank-sum test and Mann–Whitney U test. Spearman’s rank correlation coefficient was used for correlation analysis. Figures were designed using IBM SPSS Statistics for Windows, Version 25 as well as Microsoft® PowerPoint for Mac Version 16.30 (19101301).

Differences in nuclear LCoR expression were examined by comparing LCoR immunoreactive scores (IRS) between the groups of cervical tissue as shown in Fig. 1. While CIN I and CIN II showed a median IRS of four, median IRS in CIN III was two (p = 0.008). LCoR expression compared between CIN I and CIN II is not significantly changed (p = 0.088). Exemplary staining for all CIN grades is shown in Fig. 1.

For positive nuclear LCoR expression in cervical dysplasia tissue, a significant correlation with cytoplasmic LCoR (p = 0.014, Spearman Rho 0.270) was detected. Cytoplasmic RIP140 expression was negatively correlated with nuclear LCoR expression (p = 0.043; Spearman Rho − 0.224).

RIP140 expression was observed in the nucleus as well as the cytoplasm. In both compartments RIP140 expression significantly increased with higher grading of dysplasia as shown in Figs. 2 and 3. While CIN I showed a nuclear RIP140 expression with a median of two, the median in CIN II was five and in CIN III the median IRS was six (Kruskal–Wallis test p = 0.000). Cytoplasmic RIP140 expression in CIN I and CIN II with a median of zero increased significantly to the median of one in CIN III (Kruskal–Wallis test p = 0.001). Exemplary staining for all grades of CIN is shown in Figs. 2 and 3.

Correlation analysis showed that nuclear RIP140 expression correlated positively with cytoplasmic RIP140 (p = 0.000; Spearman Rho 0.552). Nuclear RIP140 correlated negatively with EP3 expression (p = 0.010; Spearman Rho − 0.290) in cervical dysplasia tissue. Cytoplasmic RIP140 expression correlated negatively with EP3 expression (p = 0.001, Spearman Rho − 0.365).

We compared nuclear LCoR expression between CIN II cases with histologically confirmed progress or regress to evaluate if LCoR expression is a prognostic marker for a progressive or regressive course in CIN. The median IRS of CIN II that showed a regressive course was three whereas the median IRS of CIN II with a progressive course was six (Fig. 4, Kruskal–Wallis test p = 0.004).