Mitotic and apoptotic activity in colorectal neoplasia

A total of 18 patients with non-advanced colorectal adenoma (13 men, 5 women, aged 41–84, mean 66 ± 12; 8/18 right sided neoplasia), 13 patients with advanced colorectal adenoma (10 men, 3 women, aged 58–79, mean 67 ± 7; 4/13 right sided neoplasia) and 13 patients with colorectal carcinoma (5 men, 8 women, aged 50–87, mean 66 ± 10; CRC: 4/13 right sided neoplasia) were included into the prospective study. Inclusion criteria for those with colorectal neoplasia were: sporadic neoplasia, absence of previous colorectal surgery, negative history of inflammatory bowel disease, absence of any type of colitis (including inflammatory bowel disease, pseudomembranous colitis, ischaemic colitis), absence of serrated lesion, absence of hyperplastic polyps proximal to the rectosigmoid colon, absence of diverticulitis and postradiation proctopathy. Two patients with well differentiated carcinoma and 11 patients with moderately differentiated carcinoma were included. A total of 7 patients with dedifferentiated carcinoma were excluded from the original group of 20 patients with CRC as mitotic and apoptotic activity could not be evaluated due to presence of excessive necrotic tissue. A total of 17 controls, individuals with normal findings on colonoscopy, with no previous history of colorectal neoplasia or inflammatory bowel disease (6 men, 11 women, aged 25–75, mean 55 ± 14), were enrolled into the study.

Biopsy samples were taken during diagnostic and/or therapeutic colonoscopy. Paired biopsies were obtained in patients with colorectal neoplasia: one sample was taken from the pathology and the second sample was taken from a healthy mucosa, 10 cm distally from the side of neoplasia. In healthy individuals, one biopsy sample was obtained, usually in the rectum, after the exclusion of a colorectal neoplasia in the colon and the rectum.

All biopsy samples were formalin-fixed (10% formalin), embedded into paraffin (Paramix, Holice, the Czech Republic), and tissue sections 5 μm thick were cut (Microtome model SM2000 R, Leica, Heidelberg, Germany). Sections were stained with haematoxylin-eosin (Merck, Kenilworth, NJ, USA) and evaluated using a BX-51 microscope (Olympus Czech Group, Prague, Czech Republic). The grade of mitosis, conveyed as a mitotic index [mitotic index (%) = number of mitotic figures × 100 / number of all evaluated cells] and grade of apoptosis, conveyed as an apoptotic index [apoptotic index (%) = number of apoptotic cells × 100 / number of all evaluated cells] were assessed in three different compartments: in the superficial compartment (which is in the direct contact with the lumen of the large intestine), in the upper part of intestinal crypts and in the lower part of intestinal crypts. Single apoptotic fragments of similar size, when compared to the adjacent non-apoptotic cells, or a cluster of at least three small apoptotic bodies were considered to be apoptotic cells. A minimal amount of 750 cells were evaluated in each compartment in each biopsy sample.

Apoptotic activity was also assessed immunohistochemically by detection of activated (cleft) caspase-3, which is a key element regulating the apoptotic process. For that, a rabbit monoclonal antibody (1:200; Cell Signaling Technology, Danvers, MA, USA) and standard peroxidase technique in 5 μm thick tissue sections were used [12]. After the detection of activated caspase-3, samples were counterstained with haematoxylin (Fig. 1). Clusters of ≥3 apoptotic bodies would have been positive in haematoxylin-eosin staining, but might not have shown activated caspase-3 positivity, as apoptotic bodies were seen if the cytoplasmatic tissue was maintained. If the apoptotic body contained nuclear material only, positivity was not observed.

The original effort was to evaluate apoptosis similarly to the samples stained with haematoxylin-eosin. Nevertheless, high false positivity in marginal areas was observed (Fig. 2), probably due to trauma when biopsy sample was taken. Mild intensity of trauma does not seem to induce necrotic cell death, however, it seems to be sufficient enough to result in a rapid activation of apoptotic signaling pathways. Subsequently, some samples (especially of small size) could not be assessed at all. In the remaining samples, apoptotic activity could not have been evaluated in the superficial compartment and at the outfall of the crypts. At least 1500 cells per compartment in each biopsy sample were analysed. Therefore, after an exclusion of false positive areas, apoptotic activity was evaluated in the upper and lower part of crypts. Firm conclusion were drawn from the upper cryptal compartment as sufficient numbers for statistics were obtained from this compartment only.

Preliminary data without controls in each group of patients with colorectal neoplasia and without any data on mitosis have been published previously [13].

Obtained data were tested statistically by means of descriptive statistics and Mann-Whitney rank sum test using Statistica software, version 13, 2013, Tulsa, OK, USA.

All patients included in the study were given the necessary information and provided informed consent via a signed form. The project was approved by the Joint Ethical Committee (Charles University, Faculty of Medicine in Hradec Kralove, University Hospital Hradec Kralove); approval number: 201107 S54. For all obtained data, all personal identification information was removed in compliance with the Czech laws for protection of confidentiality.