Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma

Youli Zu; Seth M. Steinberg; Elias Campo; Christine P. Hans; Dennis D. Weisenburger; Rita M. Braziel; Jan Delabie; Randy D. Gascoyne; Konrad Muller-Hermlink; Stefania Pittaluga; Mark Raffeld; Wing C. Chan; Elaine S. Jaffe

doi:10.1080/10428190500051844

Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma

Youli Zu, Seth M. Steinberg, Elias Campo, Christine P. Hans, Dennis D. Weisenburger, Rita M. Braziel, Jan Delabie, Randy D. Gascoyne, Konrad Muller-Hermlink, Stefania Pittaluga, Mark Raffeld, Wing C. Chan, Elaine S. Jaffe

Pathology

Research output: Contribution to journal › Review article › peer-review

46 Scopus citations

Abstract

Tissue microarrays (TMAs) show concordance with whole tissue sections in the immunohistochemical evaluation of tumor cells. However, potential inter-institutional variability among observers and immunohistochemical staining methods has not been fully addressed. We selected 21 cases of diffuse large B-cell lymphoma (DLBCL) to process for TMAs. Immunohistochemical stains were performed in 3 laboratories, and reviewed independently by 3 hematopathologists at the 3 institutions. Stains were scored on a 4-point scale. Statistical analyses of variation in the scoring among observers and among different institutions' stains were performed. Stains for CD3, CD10, CD20, BCL-2, BCL-6, MIB-1, and FOX-P1 revealed little variation among observers, with an average 51-82% complete agreement and 82-100% agreement ± 1 numerical score. The rate of concordance when evaluating most stains performed in different laboratories was also relatively good, with an average of 55-72% complete agreement and 70-97% agreement ± 1 score. However, scoring of MUM-1 and p53 stains showed wider variation, with an average of only 37 and 30% complete agreement among observers, and 11 and 45% agreement when stains from different institutions were examined. Further statistical analyses were performed to compare the observers' scoring of their own institution's stains (self-review) vs. observers' scoring of other institutions' stains (non-self). The agreement rate for the p53 stain was significantly higher when based on self-review (average 58% complete agreement) compared with an agreement rate of only 10.5% when based on a review of stains performed in another laboratory, non-self review, P < 0.01. This difference in the self- vs. non-self review was not seen when data for MUM-1 were analysed. In conclusion, most phenotypic markers used in the analysis of DLBCL can be evaluated in TMAs with adequate agreement among observers and laboratories. These include CD3, CD20, CD10, BCL-2, BCL-6, MIB-1, and FOX-P1. However, some markers, such as p53 and MUM-1, are more prone to inter-institutional variation. Variations in interpretation can be partially overcome by self-adjusted/adapt tendency, as seen with p53. Especially with newly developed markers, such as MUM-1, the development of standardized techniques for staining and interpretation is critical to reduce inter-observer variability.

Original language	English (US)
Pages (from-to)	693-701
Number of pages	9
Journal	Leukemia and Lymphoma
Volume	46
Issue number	5
DOIs	https://doi.org/10.1080/10428190500051844
State	Published - May 2005

Keywords

Diffuse large B-cell lymphoma
Immunohistochemistry
Monoclonal antibodies
Prognostic markers
Tissue microarray
Validation

ASJC Scopus subject areas

Hematology
Oncology
Cancer Research

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10.1080/10428190500051844

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Zu, Y., Steinberg, S. M., Campo, E., Hans, C. P., Weisenburger, D. D., Braziel, R. M., Delabie, J., Gascoyne, R. D., Muller-Hermlink, K., Pittaluga, S., Raffeld, M., Chan, W. C., & Jaffe, E. S. (2005). Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma. Leukemia and Lymphoma, 46(5), 693-701. https://doi.org/10.1080/10428190500051844

Zu, Y, Steinberg, SM, Campo, E, Hans, CP, Weisenburger, DD, Braziel, RM, Delabie, J, Gascoyne, RD, Muller-Hermlink, K, Pittaluga, S, Raffeld, M, Chan, WC & Jaffe, ES 2005, 'Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma', Leukemia and Lymphoma, vol. 46, no. 5, pp. 693-701. https://doi.org/10.1080/10428190500051844

@article{011c3e165513479ebd798a905decac60,

title = "Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma",

abstract = "Tissue microarrays (TMAs) show concordance with whole tissue sections in the immunohistochemical evaluation of tumor cells. However, potential inter-institutional variability among observers and immunohistochemical staining methods has not been fully addressed. We selected 21 cases of diffuse large B-cell lymphoma (DLBCL) to process for TMAs. Immunohistochemical stains were performed in 3 laboratories, and reviewed independently by 3 hematopathologists at the 3 institutions. Stains were scored on a 4-point scale. Statistical analyses of variation in the scoring among observers and among different institutions' stains were performed. Stains for CD3, CD10, CD20, BCL-2, BCL-6, MIB-1, and FOX-P1 revealed little variation among observers, with an average 51-82% complete agreement and 82-100% agreement ± 1 numerical score. The rate of concordance when evaluating most stains performed in different laboratories was also relatively good, with an average of 55-72% complete agreement and 70-97% agreement ± 1 score. However, scoring of MUM-1 and p53 stains showed wider variation, with an average of only 37 and 30% complete agreement among observers, and 11 and 45% agreement when stains from different institutions were examined. Further statistical analyses were performed to compare the observers' scoring of their own institution's stains (self-review) vs. observers' scoring of other institutions' stains (non-self). The agreement rate for the p53 stain was significantly higher when based on self-review (average 58% complete agreement) compared with an agreement rate of only 10.5% when based on a review of stains performed in another laboratory, non-self review, P < 0.01. This difference in the self- vs. non-self review was not seen when data for MUM-1 were analysed. In conclusion, most phenotypic markers used in the analysis of DLBCL can be evaluated in TMAs with adequate agreement among observers and laboratories. These include CD3, CD20, CD10, BCL-2, BCL-6, MIB-1, and FOX-P1. However, some markers, such as p53 and MUM-1, are more prone to inter-institutional variation. Variations in interpretation can be partially overcome by self-adjusted/adapt tendency, as seen with p53. Especially with newly developed markers, such as MUM-1, the development of standardized techniques for staining and interpretation is critical to reduce inter-observer variability.",

keywords = "Diffuse large B-cell lymphoma, Immunohistochemistry, Monoclonal antibodies, Prognostic markers, Tissue microarray, Validation",

author = "Youli Zu and Steinberg, {Seth M.} and Elias Campo and Hans, {Christine P.} and Weisenburger, {Dennis D.} and Braziel, {Rita M.} and Jan Delabie and Gascoyne, {Randy D.} and Konrad Muller-Hermlink and Stefania Pittaluga and Mark Raffeld and Chan, {Wing C.} and Jaffe, {Elaine S.}",

note = "Funding Information: We gratefully acknowledge the technical assistance of Patrick Wong and the Genetic Pathology Evaluation Center of the British Columbia Cancer Agency in the preparation of the tissue microarray blocks; and Angelica Vivero of the National Cancer Institute for performing the immunohistochemical studies. We acknowledge the leadership and support of Louis M. Staudt, National Cancer Institute, for the Lymphoma/Leukemia Molecular Profiling Project. This study was presented in part at the 93rd Annual Meeting of the United States and Canadian Academy of Pathology, March 2004.",

year = "2005",

month = may,

doi = "10.1080/10428190500051844",

language = "English (US)",

volume = "46",

pages = "693--701",

journal = "Leukemia and Lymphoma",

issn = "1042-8194",

publisher = "Informa Healthcare",

number = "5",

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TY - JOUR

T1 - Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma

AU - Zu, Youli

AU - Steinberg, Seth M.

AU - Campo, Elias

AU - Hans, Christine P.

AU - Weisenburger, Dennis D.

AU - Braziel, Rita M.

AU - Delabie, Jan

AU - Gascoyne, Randy D.

AU - Muller-Hermlink, Konrad

AU - Pittaluga, Stefania

AU - Raffeld, Mark

AU - Chan, Wing C.

AU - Jaffe, Elaine S.

N1 - Funding Information: We gratefully acknowledge the technical assistance of Patrick Wong and the Genetic Pathology Evaluation Center of the British Columbia Cancer Agency in the preparation of the tissue microarray blocks; and Angelica Vivero of the National Cancer Institute for performing the immunohistochemical studies. We acknowledge the leadership and support of Louis M. Staudt, National Cancer Institute, for the Lymphoma/Leukemia Molecular Profiling Project. This study was presented in part at the 93rd Annual Meeting of the United States and Canadian Academy of Pathology, March 2004.

PY - 2005/5

Y1 - 2005/5

N2 - Tissue microarrays (TMAs) show concordance with whole tissue sections in the immunohistochemical evaluation of tumor cells. However, potential inter-institutional variability among observers and immunohistochemical staining methods has not been fully addressed. We selected 21 cases of diffuse large B-cell lymphoma (DLBCL) to process for TMAs. Immunohistochemical stains were performed in 3 laboratories, and reviewed independently by 3 hematopathologists at the 3 institutions. Stains were scored on a 4-point scale. Statistical analyses of variation in the scoring among observers and among different institutions' stains were performed. Stains for CD3, CD10, CD20, BCL-2, BCL-6, MIB-1, and FOX-P1 revealed little variation among observers, with an average 51-82% complete agreement and 82-100% agreement ± 1 numerical score. The rate of concordance when evaluating most stains performed in different laboratories was also relatively good, with an average of 55-72% complete agreement and 70-97% agreement ± 1 score. However, scoring of MUM-1 and p53 stains showed wider variation, with an average of only 37 and 30% complete agreement among observers, and 11 and 45% agreement when stains from different institutions were examined. Further statistical analyses were performed to compare the observers' scoring of their own institution's stains (self-review) vs. observers' scoring of other institutions' stains (non-self). The agreement rate for the p53 stain was significantly higher when based on self-review (average 58% complete agreement) compared with an agreement rate of only 10.5% when based on a review of stains performed in another laboratory, non-self review, P < 0.01. This difference in the self- vs. non-self review was not seen when data for MUM-1 were analysed. In conclusion, most phenotypic markers used in the analysis of DLBCL can be evaluated in TMAs with adequate agreement among observers and laboratories. These include CD3, CD20, CD10, BCL-2, BCL-6, MIB-1, and FOX-P1. However, some markers, such as p53 and MUM-1, are more prone to inter-institutional variation. Variations in interpretation can be partially overcome by self-adjusted/adapt tendency, as seen with p53. Especially with newly developed markers, such as MUM-1, the development of standardized techniques for staining and interpretation is critical to reduce inter-observer variability.

AB - Tissue microarrays (TMAs) show concordance with whole tissue sections in the immunohistochemical evaluation of tumor cells. However, potential inter-institutional variability among observers and immunohistochemical staining methods has not been fully addressed. We selected 21 cases of diffuse large B-cell lymphoma (DLBCL) to process for TMAs. Immunohistochemical stains were performed in 3 laboratories, and reviewed independently by 3 hematopathologists at the 3 institutions. Stains were scored on a 4-point scale. Statistical analyses of variation in the scoring among observers and among different institutions' stains were performed. Stains for CD3, CD10, CD20, BCL-2, BCL-6, MIB-1, and FOX-P1 revealed little variation among observers, with an average 51-82% complete agreement and 82-100% agreement ± 1 numerical score. The rate of concordance when evaluating most stains performed in different laboratories was also relatively good, with an average of 55-72% complete agreement and 70-97% agreement ± 1 score. However, scoring of MUM-1 and p53 stains showed wider variation, with an average of only 37 and 30% complete agreement among observers, and 11 and 45% agreement when stains from different institutions were examined. Further statistical analyses were performed to compare the observers' scoring of their own institution's stains (self-review) vs. observers' scoring of other institutions' stains (non-self). The agreement rate for the p53 stain was significantly higher when based on self-review (average 58% complete agreement) compared with an agreement rate of only 10.5% when based on a review of stains performed in another laboratory, non-self review, P < 0.01. This difference in the self- vs. non-self review was not seen when data for MUM-1 were analysed. In conclusion, most phenotypic markers used in the analysis of DLBCL can be evaluated in TMAs with adequate agreement among observers and laboratories. These include CD3, CD20, CD10, BCL-2, BCL-6, MIB-1, and FOX-P1. However, some markers, such as p53 and MUM-1, are more prone to inter-institutional variation. Variations in interpretation can be partially overcome by self-adjusted/adapt tendency, as seen with p53. Especially with newly developed markers, such as MUM-1, the development of standardized techniques for staining and interpretation is critical to reduce inter-observer variability.

KW - Diffuse large B-cell lymphoma

KW - Immunohistochemistry

KW - Monoclonal antibodies

KW - Prognostic markers

KW - Tissue microarray

KW - Validation

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U2 - 10.1080/10428190500051844

DO - 10.1080/10428190500051844

M3 - Review article

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SN - 1042-8194

VL - 46

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JO - Leukemia and Lymphoma

JF - Leukemia and Lymphoma

IS - 5

ER -

Validation of tissue microarray immunohistochemistry staining and interpretation in diffuse large B-cell lymphoma

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