In situ localization of S‐phase‐specific histone (H3) mRNA in Bowen's disease

PCNA and Ki‐67 immunohistochemistry has been used to assess cell proliferation in place of tritiated thymidine or BrdU labeling of S‐phase cells. Recently, it has been possible to reliably demonstrate histone H3 mRNA by in situ hybridization in formalin‐fixed and paraffin‐embedded tissue sections. We have compared this new proliferation marker with Ki‐67 and PCNA with regard to distribution of positive cells and labeling indices (LI%) for 22 cases of Bowen's disease. In normal skin, Ki‐67‐IHC positive cells and histone mRNA positive cells were observed in the basal and suprabasal layers of the epidermis. In Bowen's disease, positive cells with each marker were more frequent in upper neoplastic epidermis than in suprabasal layers, and the average LI%s were markedly elevated with all markers, the scores decreasing in the following order: PCNA‐IHC, Ki‐67‐IHC and H3mRNA‐ISH. However, the results of double staining demonstrated that S‐phase cells do not necessarily show exactly the same distributions as with PCNA and Ki‐67‐IHC labeling. H3mRNA‐ISH showed three different degrees of reaction with significantly different LI%s, whereas PCNA and Ki‐67 LI% did not vary essentially in the same areas. These results strongly suggest that Bowen's disease, which is well known as a low‐grade neoplastic state with malignant potential, also demonstrates clear intratumoral heterogeneity of S‐phase cells using the H3mRNA‐ISH method.