Ki-67

Various indices of cellular proliferative activity have been investigated. Mitotic counts only detect cells in the M phase, are dependent on the period of time between surgical removal and fixation of the specimen, and suffer from heterogeneous distribution and confusion between mitoses and nuclear pyknosis and karyorrhexis. Counting nucleolar organiser regions (AgNORs) and 5-bromodeoxyuridine or tritiated thymidine labelling are also not practical in a routine situation. Ki-67 recognises a proliferation specific nuclear antigen

Immunohistochemical expression

Ki-67 is expressed by proliferating cells in late G₁, S, G₂ and M phases, but not in resting cells in G_0. Staining is commonly nucleolar or perinucleolar. In conjunction with Ki-S2, it may be used to derive a cell cycling ratio.

The prototypic monoclonal antibody works only in frozen sections. Subsequently, antibodies against formalin-resistant epitopes, MIB-1 and NCL-Ki-67-MM1 (MM1), have been raised. Polyclonal antibodies such as NCL-Ki-67p and rabbit anti-human (Rah) Ki-67, are also immunoreactive in paraffin sections. Staining is nuclear and may be diffuse or granular, or a combination¹. There are good correlations between immunoreactivity using monoclonal Ki-67 in frozen section, polyclonal antibodies in paraffin sections and other indices of cell proliferation. In one study¹, MIB-1 gives a higher labelling index than other antibodies, with good inter-reading reproducibility, although this was not reproduced in a second study², which showed considerable variation between readings. It is therefore important to identify the antibody used in every study.

prototypic Ki-67

MIB-1

MM1

NCL-Ki-67p

Rah Ki-67

tonsillar squamous epithelium (Counts were performed twice by the same observer in constant areas)¹

granular & diffuse

diffuse only

granular & diffuse

diffuse only

granular & diffuse

diffuse only

granular & diffuse

diffuse only

30.8 to 30.9%¹

18.2 to 18.3%¹

13.9 to 14.50%¹

5.8, 5.8%¹

20.2 to 21.2%¹

7.2 to 7.2%¹

16.6 to 17.9%¹

7.7 to 7.8%¹

glioblastoma (For MIB-1 and Rah Ki-67, counts were performed twice. This tumour is known to show heterogeneity)

5.7%¹

6.1 to 9.4% (granular staining)¹

7.9% (granular staining)¹

5.9% (granular staining)¹

5.2 to 10.9% (granular staining)¹

Immunoreactivity has therefore been shown not to be fixation dependent, an advantage over PCNA.

Lymphoproliferative disorders may show characteristic patterns of proliferation as assessed by the Ki-67 staining⁷:

diagnosis

pattern of staining with Ki-67

Resting lymphoid tissue

The proliferation rate is low. Distinction from follicular lymphoma may be made by the negativity of the follicles for CD10 and bcl-6. (bcl-2 may be positive.)

Follicular hyperplasia

Follicles show a high level of staining, with a polarity; there is almost 100% staining of nuclei in the dark zone, which tends to form a meniscus. The borders of the follicles are sharply demarcated from the mantle which has a low proliferation rate. Some follicles may lack the typical pattern, so multiple follicles should be assessed: this is the case if the section is purely through the light zone.

Mixed pattern hyperplasia

Follicles show a high level of staining and interfollicular areas a low to moderate level

Progressive transformation of germinal centres

There are large follicles within which there are small aggregates of proliferating cells: the non-proliferating cells are T-cells or mantel zone B-cells. The pattern overlaps with that of the floral variant of follicular lymphoma. The few large follicles showing PTGC are present alongside obviously benign reactive follicles.

Castleman's disease

A nodular pattern of staining of low intensity, similar to follicular lymphoma, but the nodules are smaller and more widely spaced.

Follicular lymphoma

Follicles show a lower level of staining than in follicular hyperplasia and polarity is lacking. Margins are ill-defined. Grade 3 lymphomas may have a proliferation rate approaching that of benign follicles but are distinguished by the uniformity of the pattern among many follicles.

Floral variant of follicular lymphoma

There are large follicles within which there are small aggregates of proliferating cells: the non-proliferating cells are centrocytes. The pattern overlaps with that of progressive transformation of germinal centres. In addition to the floral type follicles, there are typical neoplastic follicles.

Marginal zone lymphoma

Diffuse low level of (interfollicular) staining, with or without residual follicles. Colonisation of follicles gives a pattern similar to that of follicular lymphoma.

Small lymphocytic lymphoma

Ki-67 accentuates the proliferation centres, which may resemble the pattern of neoplastic follicles.

Burkitt and Burkitt-like lymphoma

proliferation index approaching 100%

Transformation of indolent lymphomas

May be suggested by an anomalously high proliferation rate

T-cell rich B-cell lymphoma

The neoplastic cells are highlighted

Hodgkin lymphoma

Angioimmunoblastic T-cell lymphoma

Hyalinising trabecular tumour of the thyroid shows cytoplasmic staining with MIB-1

Diagnostic utility

The rate of cell proliferation as assessed by Ki-67 immunoreactivity has been studied as a prognostic indicator in numerous malignant neoplasms and shown to correlate with tumour grade and clinical course. This includes:

Non-Hodgkin lymphoma: low grade lymphomas have a labelling index of less than 20%, high grade lymphomas greater than 20%. Low grade lymphomas with a labelling index in excess of 5% have a worse prognosis than those with an index of less than 5%. In particular, grade 1 and 2 follicular lymphomas with a higher than usual proliferation index have similar clinical behaviour to high grade follicular lymphoma⁸. However, high grade lymphoma with a very high index (>80%) tend to have a better prognosis than high grade lymphomas with a lower index, being less likely to relapse if remission is achieved.³ In Burkitt and Burkitt-like lymphoma, the nuclear labelling by Ki67 is nearly 100% and this can be used as a diagnostic criterion⁶. The pattern of proliferation as assessed by Ki-67 may be diagnostically useful in lymphoproliferative disorders (vide supra)⁷.
Glioma: the indices ranged from 0% to 4.5% for 16 low grade astrocytomas; from 0.7% to 7.4% for 8 anaplastic astrocytomas; and from 1.7% to 32.2% for 27 glioblastomas. The differences among the means of each group are statistically significant. Five patients with malignant gliomas with an index of less than 2.5 had survival times of more than 40 weeks.⁴
Soft tissue sarcoma: Ki-67 index (the number of Ki-67-positive tumor cells/10 HPF) positively correlated with mitotic count , cellularity and the histological grade. The Ki-67 low index group (less than 50/10 HPF) showed a more favorable prognosis than the high index group (more than 50/10 HPF). Three cases with low mitotic count and unfavorable prognosis were proved to be in the Ki-67 high index group (142-382/10 HPF).⁵
Breast carcinoma: tumors with high Ki-67 proliferation indices (> 20%) were associated with a higher 4-year probability of relapse of disease and death when compared with tumors with low Ki-67 values. In addition, this proliferative parameter maintained its prognostic significance when the patients were stratified according to lymph node involvement, menopausal status, and nuclear estrogen receptor content.⁶

It has also been used to distinguish benign from malignant neoplasms.

References

¹ Lindboe, C.F. and Torp, S.H. Comparison of Ki-67 equivalent antibodies. J Clin Pathol 2002;55:467-71.

² Torp, S.H. Proliferative activity in human glioblastomas: evaluation of different Ki67 equivalent antibodies. Mol Pathol 1997;50:198-200.

³ Hall, P.A., Richards, M.A., Gregory, W.M., d'Ardenne, A.J., Lister, T.A. and Stansfeld, A.G. The prognostic value of Ki67 immunostaining in non-Hodgkin's lymphoma. J Pathol 1988;154:223-35.

⁴ Zuber, P., Hamou, M.F. and de Tribolet, N. Identification of proliferating cells in human gliomas using the monoclonal antibody Ki-67. Neurosurgery 1988;22:364-8.

⁵ Ueda, T., Aozasa, K., Tsujimoto, M., Ohsawa, M., Uchida, A., Aoki, Y., Ono, K. and Matsumoto, K. Prognostic significance of Ki-67 reactivity in soft tissue sarcomas. Cancer 1989;63:1607-11.

⁶ Veronese, S.M., Gambacorta, M., Gottardi, O., Scanzi, F., Ferrari, M. and Lampertico, P. Proliferation index as a prognostic marker in breast cancer. Cancer 1993;71:3926-31.

⁷Bryant RJ, Banks PM,O'Malley D P. Ki67 staining pattern as a diagnostic tool in the evaluation of lymphoproliferative disorders. Histopathology 2006; 48:505-15

⁸Wang SA, Wang L, Hochberg EP, et al. Low histologic grade follicular lymphoma with high proliferation index: morphologic and clinical features. Am J Surg Pathol 2005; 29:1490-6

This page last revised 29.4.2006.

	prototypic Ki-67	MIB-1		MM1		NCL-Ki-67p		Rah Ki-67
tonsillar squamous epithelium (Counts were performed twice by the same observer in constant areas)¹		granular & diffuse	diffuse only	granular & diffuse	diffuse only	granular & diffuse	diffuse only	granular & diffuse	diffuse only
		30.8 to 30.9%¹	18.2 to 18.3%¹	13.9 to 14.50%¹	5.8, 5.8%¹	20.2 to 21.2%¹	7.2 to 7.2%¹	16.6 to 17.9%¹	7.7 to 7.8%¹
glioblastoma (For MIB-1 and Rah Ki-67, counts were performed twice. This tumour is known to show heterogeneity)	5.7%¹	6.1 to 9.4% (granular staining)¹		7.9% (granular staining)¹		5.9% (granular staining)¹		5.2 to 10.9% (granular staining)¹