Simplified sensitive method for the detection of B-cell clonality in lymphoid malignancies

I. Jilani; M. Keating; A. Day; W. William; H. Kantarjian; S. O'Brien; F. J. Giles; M. Albitar

doi:10.1111/j.1365-2257.2006.00813.x

Simplified sensitive method for the detection of B-cell clonality in lymphoid malignancies

I. Jilani, M. Keating, A. Day, W. William, H. Kantarjian, S. O'Brien, F. J. Giles, M. Albitar

Research output: Contribution to a Journal (Peer & Non Peer) › Article › peer-review

8 Citations (Scopus)

Abstract

Molecular response and monitoring of minimal residual disease (MRD) is becoming an essential part of most protocols for treating leukemia and lymphoma patients. Detection of abnormal clones by PCR analysis of complementarity determining regions (CDRs) in immunoglobulin genes is currently standard practice for diagnosis, but is not widely used to monitor MRD because of the low sensitivity of assays that use consensus primers. Use of specific primers can improve the sensitivity of the assay, but is a cumbersome, expensive, and time-consuming process. We developed a simple and cost-effective approach to detect MRD in B-cell malignancies that is usable in clinical laboratories. The new assay uses ligase chain reaction (LCR) to detect clonality. The sensitivity of the LCR assay is 1 per 500 000 cells, and it can detect all subclones that were present in the pretherapy diagnostic sample.

Original language	English
Pages (from-to)	325-331
Number of pages	7
Journal	Clinical and Laboratory Haematology
Volume	28
Issue number	5
DOIs	https://doi.org/10.1111/j.1365-2257.2006.00813.x
Publication status	Published - Oct 2006
Externally published	Yes

Keywords

Clonality
Immunoglobulin
Ligase chain reaction
Lymphoid neoplasm
Minimal residual disease
PCR

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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10.1111/j.1365-2257.2006.00813.x

Cite this

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abstract = "Molecular response and monitoring of minimal residual disease (MRD) is becoming an essential part of most protocols for treating leukemia and lymphoma patients. Detection of abnormal clones by PCR analysis of complementarity determining regions (CDRs) in immunoglobulin genes is currently standard practice for diagnosis, but is not widely used to monitor MRD because of the low sensitivity of assays that use consensus primers. Use of specific primers can improve the sensitivity of the assay, but is a cumbersome, expensive, and time-consuming process. We developed a simple and cost-effective approach to detect MRD in B-cell malignancies that is usable in clinical laboratories. The new assay uses ligase chain reaction (LCR) to detect clonality. The sensitivity of the LCR assay is 1 per 500 000 cells, and it can detect all subclones that were present in the pretherapy diagnostic sample.",

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AU - Jilani, I.

AU - Keating, M.

AU - Day, A.

AU - William, W.

AU - Kantarjian, H.

AU - O'Brien, S.

AU - Giles, F. J.

AU - Albitar, M.

PY - 2006/10

Y1 - 2006/10

N2 - Molecular response and monitoring of minimal residual disease (MRD) is becoming an essential part of most protocols for treating leukemia and lymphoma patients. Detection of abnormal clones by PCR analysis of complementarity determining regions (CDRs) in immunoglobulin genes is currently standard practice for diagnosis, but is not widely used to monitor MRD because of the low sensitivity of assays that use consensus primers. Use of specific primers can improve the sensitivity of the assay, but is a cumbersome, expensive, and time-consuming process. We developed a simple and cost-effective approach to detect MRD in B-cell malignancies that is usable in clinical laboratories. The new assay uses ligase chain reaction (LCR) to detect clonality. The sensitivity of the LCR assay is 1 per 500 000 cells, and it can detect all subclones that were present in the pretherapy diagnostic sample.

AB - Molecular response and monitoring of minimal residual disease (MRD) is becoming an essential part of most protocols for treating leukemia and lymphoma patients. Detection of abnormal clones by PCR analysis of complementarity determining regions (CDRs) in immunoglobulin genes is currently standard practice for diagnosis, but is not widely used to monitor MRD because of the low sensitivity of assays that use consensus primers. Use of specific primers can improve the sensitivity of the assay, but is a cumbersome, expensive, and time-consuming process. We developed a simple and cost-effective approach to detect MRD in B-cell malignancies that is usable in clinical laboratories. The new assay uses ligase chain reaction (LCR) to detect clonality. The sensitivity of the LCR assay is 1 per 500 000 cells, and it can detect all subclones that were present in the pretherapy diagnostic sample.

KW - Clonality

KW - Immunoglobulin

KW - Ligase chain reaction

KW - Lymphoid neoplasm

KW - Minimal residual disease

KW - PCR

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DO - 10.1111/j.1365-2257.2006.00813.x

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SP - 325

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JO - Clinical and Laboratory Haematology

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ER -

Simplified sensitive method for the detection of B-cell clonality in lymphoid malignancies

Abstract

Keywords

UN SDGs

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